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PRACTICAL
PHYSIOLOGICAL CHEMISTRY

HAWK

Absorption Spectra,

Oxyhaemoglobin.

Haemoglobin.

Carboxy-
haemoglobln.

Neutral Met-
haemogtobln.

Alkaline Met-
haemoglobln.

Alkali
Haematin.

Absorption Spectra.

■^ %

Reduced Alkali
Haematin or
Haemochromogen.

Acid Haematin in
ethereal solution.

Acid Haemato-
porphyrln.

Alkaline

Haematopor-

phyrln.

Urobilin or Hydro-
bilirubin In acid
solution.

Urobilin or Hydro-
bilirubin 4n alkaline
solution after the
addition of zinc
chloride solution.

Bllicyanin or
Cholecyanin in
alkaline solution.

PRACTICAL

PHYSIOLOGICAL CHEMISTRY

A BOOK DESIGNED FOR USE IN COURSES IN PRACTICAL

PHYSIOLOGICAL CHEMISTRY IN SCHOOLS

OF MEDICINE AND OF SCIENCE

BY
PHILIP B. HAWK, M. S., Ph. D.

PROFESSOR OF PHYSIOLOGICAL CHEMISTRY AND TOXICOLOGY IN THE
JEFFERSON MEDICAL COLLEGE OF PHILADELPHIA

FIFTH EDITION, REVISED AND ENLARGED

WITH TWO FULL-PAGE PLATES OF ABSORPTION SPECTRA IN COLORS

FOUR ADDITIONAL FULL-PAGE COLOR PLATES AND ONE

HUNDRED AND SEVENTY-TWO FIGURES OF WHICH

TWELVE ARE IN COLORS

PHILADELPHIA

P. BLAKISTON'S SON & CO.

1012 WALNUT STREET
1916

First Edition, Copyright, 1907, by P. Blakiston's Son & Co.
Second Edition, Copyright, 1909, by P. Blakiston's Son & Co.
Third Edition, Copyright, 1910, by P. Blakiston's Son & Co.
FoxniTH Edition, Copyright, 191 2, by P. Blakiston's Son & Co.

Reprinted, October, 1913 and May, 1915
Fifth Edition, Copyright, 1916, by P. Blakiston's Son & Co.

THE. MAPLE. PRESS. YORK. PA

THESE PAGES ARE

AFFECTIONATELY DEDICATED

TO

MY PARENTS

1866-1916

PREFACE TO FIFTH EDITION

The book has been thoroughly revised and in part rewritten. Five
additional chapters have been inserted, in order to increase the useful-
ness of the volume and to keep thoroughly abreast with recent develop-
ments in Physiological Chemistry. The new Chapters are, Chapter VI
on Nucleic Acids.'and Nucleoproteins, Chapter VIII on Gastric Analysis,
Chapter XI on Intestinal Digestion, Chapter XVI on Blood Analysis
and Chapter XXVII on Metabolism.

The Chapter on Metabolism consists in large part of directions
for typical metabolism tests which may be conducted by the student in
order to demonstrate important principles of metabolism.

The Chapter on Blood Analysis includes the most recent methods
which have played such an important part in adding to our knowledge
regarding the composition of the blood under normal and pathological
conditions.

The Chapter on Gastric Analysis includes a general discussion of
titratable acidity and hydrogen-ion concentration as well as an expo-
sition of the Fractional Method of Gastric Analysis which was elabo-
rated in the author's laboratory by Dr. Martin E. Rehfuss, and which
has been very widely adopted.

The Chapter on Nucleic Acids and Nucleoproteins is a brief dis-
cussion of basic facts accompanied by experiments suitable for student
use.

In order to facihtate the selection of tests and methods for courses
in which but httle time is devoted to the subject, the actual laboratory
procedure involved in such tests and methods as the author considers
most important has been printed in black face type to differentiate
such tests and methods from those which he considers of less impor-
tance, which are set in smaU type. In certain instances, however, tests
and methods which the author beHeves to be of first importance, but
which are not so readily adapted to student use, have been printed in
small type.

The latest and best methods of quantitative analysis have been
introduced throughout the volume. The nephelometer has been dis-
cussed and certain nephelometric methods described.

Certain tests and methods which had obviously outlived tlieir
usefulness have been omitted from this edition. Others which the

Vlll PREFACE TO FIFTH EDITION

author believes might well have been omitted have been retained in
small type. The author believes that it is preferable that each indi-
vidual instructor shall use his own judgment as to which tests and
methods he will omit from his course. For this reason, in connection
with certain quantitative procedures more than a single approved
method has been given.

Thirty-five new illustrations have been incorporated.

The author takes pleasure in acknowledging the important part
played by Dr. Olaf Bergeim in the preparation of this new edition.
Dr. Bergeim's suggestions and assistance have been invaluable in
connection with all phases of the re\dsion, as well as in the preparation
of new material for introduction. To Dr. Martin E. Rehfuss the
author is indebted for the drawings of the microscopical constituents
of the feces and gastric contents and the curves which are introduced
in the Chapter on Gastric Analysis, as well as for timely suggestions
as. to certain clinical aspects of fecal and gastric analysis. Other
members of the author's staff who have aided in certain phases of the
revision are Drs. H. Rodell Fishback,-Mehdn A. Saylor and Clarence A.
Smith.

To Professors Lafayette B. Mendel, Paul E. Howe, Marshall P.
Cram, A. P. Sy and J. C. Blake, the author is also indebted for helpful
suggestions, and to Professors WiUiam J. Gies and Walter Jones for
permission to insert selected experiments from their laboratory direc-
tions. The author is under further obligation to Professor Jones for
crystals of hypoxanthine chloride and guanine chloride from which
were prepared the microphotographs appearing in the Chapter on
Nucleic Acids and Nucleoproteins. He also wishes to thank Professor
Chester C. Fowler for permission to insert unpublished material.

The author is very appreciative of the unfailing courtesy and con-
sideration of the publishing house of P. Blakiston's Son & Co.; the
timely suggestions of Mr. C. V. Brownlow, Mr. I. A. Hagy and Mr.
Horace G. White have been very helpful.

CONTENTS

CHAPTER I

t Page

Enzymes and Their Action i

CHAPTER II
Carbohydrates 19

CHAPTER III
Salivary Digestion 54

CHAPTER IV
Proteins: Their Decomposition and Synthesis 63

CHAPTER V
Proteins: Their Classification and Properties 92

CHAPTER VI
Nucleic Acids and Nucleoproteins 123

CHAPTER VII

Gastric Digestion 138

CHAPTER VIII
Gastric Analysis 148

CHAPTER IX
Fats 176

CHAPTER X
Pancreatic Digestion 185

CHAPTER XI
Intestinal Digestion 195

CHAPTER XII

Bile 202

CHAPTER XIII
Putrefaction Products 212

CHAPTER XIV

Feces 221

ix

X CONTENTS

CHAPTER XV

Paqb

Blood and Lymph 245

CHAPTER XVI
Blood Analysis 270

CHAPTER XVII

Milk 313

CHAPTER XVIII
Epithelial and Connectwe Tissues 330

CHAPTER XIX
Muscular Tissue . 339

CHAPTER XX
Nervous Tissue 353

CHAPTER XXI

Urine: General Characteristics of Normal and Pathological
Urine 359

CHAPTER XXII
Urine: Physiological Constituents 369

CHAPTER XXIII
Urine: Pathological Constituents 412

CHAPTER XXIV
Urine: Organized and Unorganized Sediments 457

CHAPTER XXV
Urine: Calculi 475

CHAPTER XXVI
Urine: Quantitative Analysis 479

CHAPTER XXVII

Metabolism 564

Reagents and Solutions 594

Index 612

LIST OF ILLUSTRATIONS

Plate

I. Absorption Spectra 1 .

II. Absorption Spectra J ^^

III. Osazones Opposite page 22

IV. Normal Erythrocytes and Leucocytes Opposite page 249

V. Uric Acid Crystals Opposite page 380

VI. Ammonium Urate Opposite page 462

Figure Page

1. Apparatus for Quantitative Determination of Catalase 17

2. Dialyzing Apparatus for Students' Use 24

3. Einhorn Saccharometer 31

4. Illustrating Different Stages in Fermentation 31

5. One Form of Laurent Polariscope 32

6. Diagrammatic Representation of the Course of the Light through

the Laurent Polariscope 33

7. Polariscope (Schmidt and Hansch Model) 34

8. Iodoform 42

9. Potato Starch 44

10. Bean Starch 44

11. Arrowroot Starch 44

12. Rye Starch 44

13. Barley Starch 44

14. Oat Starch 44

15. Buckwheat Starch 44

16. Maize Starch 44

17. Rice Starch 44

18. Pea Starch 44

19. Wheat Starch 44

20. Microscopical Constituents of Sahva 58

21. Glycocoll Ester Hydrochloride 72

22. Serine 73

23. Phenylalanine 74

24. Fischer Apparatus 75

25. Tyrosine 76

26. Cystine 76

27. Histidine Dichloride 78

28. Leucine 80

29. Lysine Picrate 81

30. Aspartic Acid Si

31. Glutamic Acid S^

32. Levo-a-ProUne 84

33. Copper Salt of Proline 84

xi

XU LIST OF ILLUSTRATIONS

FiGUBE < PaQB

34. Van Slyke Amino Nitrogen Apparatus 88

35. Section of Van Slyke Apparatus 88

36. Coagulation Temperature Apparatus 106

37. Edestin 109

38. Excelsin, the Protein of the Brazil Nut 110

39. Guanine Chloride 135

40. Hypoxanthine Chloride 136

41. Normal and Pathological Curves after an Ewald Meal 148

42. Rehfuss Stomach Tube 149

43. Influence of Acid Introduced into the Normal Human Stomach . 150

44. Hydrogen Ion Concentration Chart 157

45. Acidity Curves of Normal Human Stomach 163

46. Acidity Curves from a Case of Hyperacidity 164

47. Acidity and Protein Curves in Gastric Carcinoma 164

48. Total Acidity and Protein Curves in Benign Achylia 165

49. Microscopical Constituents of the Gastric Contents 172

50. Beef Fat 176

51. Mutton Fat 179

52. Pork Fat 181

53. Palmitic Acid 182

54. Melting-point Apparatus 183

55. Bile Salts 205

56. Bilirubin (Hematoidin) 205

57. Cholesterol 210

58. Taurine 211

59. Glycocoll 211

60. Ammonium Chloride 216

61. Hematoidin Crystals from Acholic Stools 222

62. Charcot-Leyden Crystals 225

63. Boas' Sieve 229

64-69. Microscopical Constituents of Feces 230-31

70. Oxyhemoglobin Crystals from Blood of the Guinea-pig 251

71. Oxyhemoglobin Crystals from Blood of the Rat 251

72. Oxyhemoglobin Crystals from Blood of the Horse 252

73. Oxyhemoglobin Crystals from Blood of the Squirrel 252

74. Oxyhemoglobin Crystals from Blood of the Dog 253

75. Oxyhemoglobin Crystals from Blood of the Cat 253

76. Oxyhemoglobin Crystals from Blood of the Necturus 254

77. Effect of Water on Erythrocytes 261

78. Hemin Crystals from Human Blood 265

79. Hemin Crystals from Sheep Blood 265

80. Sodium Chloride 267

81. Bang Reduction Flask 281

82. Apparatus for Epstein's Sugar Method 283

83. Bloor's Nephelometer 291

LIST OF ILLUSTRATIONS XIU

FiGCRE Page

84. Nephelometer in Position, Showing Relation to Source of Light . 292

85. Lenzmann-Kober Nephelometer 293

86. Direct-vision Spectroscope 296

87. Angular-vision Spectroscope Arranged for Absorption Analysis . 297

88. Diagram of Angular- vision Spectroscope 297

89. Fleischl's Hemometer 300

90. Pipette of Fleischl's Hemometer 301

91. Colored Glass Wedge of Fleischl's Hemometer 301

92. Dare's Hemoglobinometer 302

93. Horizontal Section of Dare's Hemoglobinometer 303

94. Method of FilUng the Capillary Observation Cell of Dare's Hemo-

globinometer 303

95. Thoma-Zeiss Counting Chamber 304

96. Thoma-Zeiss Capillary Pipettes 305

97. Ordinary Ruling of Thoma-Zeiss Counting Chamber 306

98. Zappert's Modified Ruling of Thoma-Zeiss Counting Chamber . . 307

99. Biirker's Pipettes, Mixing Flasks, and Counting Chamber. . . . 309

100. Ruling of Burker Counting Chamber 310

loi. Schema 311

102. Burker Counting Chamber 312

103. Normal Milk and Colostrum 315

104. Lactose 318

105. Calcium Phosphate 322

106. Centrifuge Tube used in Babcock Fat Method 324

107. Croll's Fat Apparatus 325

108. Soxhlet Apparatus 326

109. Feser's Lactoscope 326

no. Creatine 342

111. Xanthine 344

112. Hypoxanthine Silver Nitrate 351

113. Xanthine Silver Nitrate 351

114. Deposit in Ammoniacal Fermentation 362

115. Deposit in Acid Fermentation 363

116. Urinometer and Cylinder 364

117. Beckmann-Heidenhain Freezing-point Apparatus 365

118. Urea 372

119. Urea Nitrate 374

120. Melting-point Tubes Fastened to Bulb of Thermometer 375

121. Urea Oxalate 376

122. Pure Uric Acid 380

123. Creatinine 382

124. Creatinine-Zinc Chloride 385

125. Hippuric Acid 389

126. AUantoin from Cat's Urine 392

127. Benzoic Acid 396

Xiv LIST OF ILLUSTRATIONS

FiGUBE Page

128. Calcium Sulphate 405

129. "Triple Phosphate" 408

130. Albumoscope 424

131. Marsh Apparatus 449

132. The Purdy Electric Centrifuge 457

133. Sediment Tube for the Purdy Electric Centrifuge 457

134. Calcium Oxalate 459

135. Calcium Carbonate 459

136. Various Forms of Uric Acid 461

137. Acid Sodium Urate 462

138. Cystine 462

139. Crystals of Impure Leucine 463

140. EpitheHum from Different Areas of the Urinary Tract 466

141. Pus Corpuscles 467

142. Hyaline Casts 468

143. Granular Casts 469

144. Granular Casts 47°

145. Epithelial Casts 47°

146. Blood, Pus, HyaUne and EpitheUal Casts 470

147. Fatty Casts 471

148. Fatty and Waxy Casts 471

149. Cylindroids 472

150. Crenated Erythrocytes 473

151. Human Spermatozoa 474

152. Folin Fume Absorber 483

153. Duboscq Colorimeter 486

154. 155. Forms of Apparatus used in Methods of Folin and Associates

for Determination of Total Nitrogen, Urea and Ammonia . . . 487

156. Bock and Benedict Apparatus 489

157. Gulick Micro-oxidation Flask. 490

158. Van Slyke and Cullen Apparatus 492

159. Folin's Urea Apparatus 496

160. Doremus-Hinds Ureometer 497

161. Marshall's Urea Apparatus 498

162. Hiifner's Urea Apparatus 498

163. Folin's Ammonia Apparatus 499

164. Folin Improved Absorption Tube 500

165. Ruhemann's Uricometer 513

166. Hall's Purinometer 517

167. Esbach's Albuminometer 532

168. Scott- Wilson Apparatus 536

169. Blood Sugar as Influenced by Diet 566

170. Influence of Protein Ingestion on Endogenous Uric Acid Output 573

171. The Endogenous Uric Acid Output during Fasting 573

172. Berthelot-Atwater Bomb Calorimeter 586

PHYSIOLOGICAL CHEMISTRY

CHAPTER I

ENZYMES AND THEIR ACTION

According to the old classiti cation ferments were divided into two
classes, the organized ferments and the unorganized ferments. As organ-
ized ferments or true ferments there were grouped such substances as
yeast and certain bacteria which were supposed to act by virtue of vital
processes, whereas the unorganized ferments included salivary amylase
(ptyalin), gastric protease (pepsin), pancreatic protease (trypsin), etc.,
which were described as ''non-Hving unorganized substances of a
chemical nature." Kiihne designated this latter class of substances as
enzymes i^v ^vfirj — in yeast). This division into organized ferments
(^true ferments) and unorganized ferments (enzymes) was generally
accepted and was practically unquestioned until Buchner overthrew
it in the year 1897 by his epoch-making investigations on zymase.
Previous to this time many writers had expressed the opinion that the
action of the ferment organisms was similar to that of the unorganized
ferments or enzymes and that therefore the activity of the former was
possibly due to the production of a substance in the cell, which was in
nature similar to an enzyme. Investigation after investigation, how-
ever, failed to isolate any such principle from an active cell and the
exponents of the "vital" theory became strengthened in their belief that
certain fermentative processes brought about by living cells could not
occur apart from the biological activity of such cells. However, as
early as 1858, Traube had enunciated, in substance, the principles
which were destined to be fundamental in our modern theory of fermen-
tation. He expressed the belief that the yeast cell produced a product
in its metabolic activities which had the property of reacting with sugar
with the production of carbon dio.xide and alcohol, and further that this
reaction between the product of the metabolism of the yeast cell and the
sugar occurred without aid from the original cell. It was not until 1897,
however, that this theory was placed upon a firm experimental basis.
This was brought about through the efforts of Buchner, who succeeded in
isolating from the living yeast cells a substance (zymase) which, when
freed from the last trace of organized cellular material, was able to bring

2 PHYSIOLOGICAL CHEMISTRY

about the identical fermentative processes which, up to this time, had
been deemed possible only in the presence of the active, living yeast cell.

Buchner's manipulation of the yeast cells consisted in first grind-
ing them with sand and infusorial earth, after which the finely divided
material was subjected to great pressure (300 atmospheres) and yielded
a liquid which possessed the fermentative activity of the unchanged
yeast cell.^ This Hquid contained zymase, the principal enzyme of
the yeast cell. Later the lactic-acid- and acetic-acid-producing bac-
teria were subjected by Buchner to treatment similar to that accorded
the yeast cells, and the active intracellular enzymes were obtained.
Many other instances are on record in which a soluble, active agent has
been isolated from ferment cells, with the result that it is pretty well
estabhshed that all the so-called organized ferments elaborate sub-
stances of this character.

Enzymes act by catalysis and hence may be termed catalyzers or
catalysts. A simple rough definition of a catalyst is "a substance
which alters the velpcity of a chemical reaction without undergoing
any apparent physical or chemical change itself and without becoming
a part of the product formed." It is a well-known fact that the veloc-
ity of the greater number of chemical reactions may be changed
through the presence of some catalyst. For example, take the case of
hydrogen peroxide. It spontaneously decomposes slowly into water
and oxygen. In the presence of colloidal platinum, ^ however, the de-
composition is much accelerated and ceases only when the destruction
of the hydrogen peroxide is complete. Without multiplying instances,
sufl&ce it to say that there is a close analogy between inorganic catalysts
and enzymes, the main point of difference between the enzymes and most
of the inorganic catalysts being that the enzymes are colloids. The
great majority of enzymes are hydrolytic in character.

We may define an enzyme as an organic catalyst which is elaborated
by an animal or vegetable cell and whose activity is entirely independent
of any of the life processes of such a cell. According to this definition
the enzyme zymase elaborated by the yeast cell is entirely comparable
to the enzyme pepsin elaborated by the cells of the stomach mucosa.
One is derived from a vegetable cell, the other from an animal cell, yet
the activity of neither is dependent upon the integrity of the cell.

Inasmuch as each of the enzymes has an action which is more or less
specific in character, and since it is a fairly simple matter, ordinarily, to
determine the character of that action, the classification of the enzymes

* In later investigations the process was improved by freezing the ground cells with
liquid air and finely pulverizing them before applying the pressure.

2 Produced by the passage of electric sparks between two platinum terminals immersed
in distilled water, thus liberating ultra-microscopic particles.

ENZYMES AND THEIR ACTION 3

is not attended with very great difficulties. They are ordinarily classi-
fied according to the nature of the substrate^ or according to the type
of reaction they bring about. Thus we have various classes of enz}-mes,
such as amylolytic,'^ proteolytic, lipolytic, glycolytic, uricolytic, autolytic,
oxidizing, reducing, inverting, protein-coagulating, deamidizing, etc. In
every instance the class name indicates the individual type of enzy-
matic activity which the enzymes included in that class are capable of
accomplishing. For example, amylolytic enzymes facilitate the hydro-
lysis of starch (amylum) and related substances, lipolytic enzymes
facihtate the hydrolysis of fats (Xittos), whereas through the agency of
uricolytic enzymes uric acid is broken down. There is a tendency,
at the present time, to harmonize the nomenclature of the enzymes by
the use of the termination -ase. According to this system of nomen-
clature, all starch-transforming enzymes, or so-called amylolytic en-
zymes, are called amylases; all fat-splitting enz3'mes are called lipases,
etc. Thus ptyalin, the amylolytic enzyme of the saliva, would be
termed salivary amylase in order to distinguish it from pancreatic amy-
lase (amylopsin) and vegetable amylases (diastase, etc.). According
to the same system, the fat-splitting enzyme of the gastric juice would
be termed gastric lipase to differentiate it fro-^n t>ancreatic lipase (steap-
sin), the fat-splitting enzyme of the pancreatic juice.

Defensive (protective) enzymes are those believed to be manufac-
tured by certain cells (perhaps the leucocytes) and passed into the
circulating blood in order to digest any foreign material of endogenous
or exogenous origin that may have found its way into the circulation.
The most important defensive enzymes are proteolytic enzymes.
Abderhalden^ claims that the parenteral introduction of any foreign
protein into the animal body will be followed by the appearance in the
blood of a defensive enzyme capable of digesting that protein. He also
claims that in pregnancy the passage into the blood of protein material
in the form of cells and fragments of chorionic villi will cause the
appearance in the blood of a defensive proteolytic enzyme capable of
digesting placenta protein. The AbderJialden reaction for pregnancy
is based upon this hypothesis. The reaction has been widely employed
and much has been said both for and against its accuracy.^ Modifications
of the reaction have been employed as an aid in the diagnosis of various
disorders, e.g., cancer, tuberculosis, dementia pra^cox, etc. Taylor^

^ Substance acted upon. See Lippmann: Ber. d. Deutsch. Chcm. Ges., 36, 331, 1903.

2 Armstrong suggests the use of the termination "clastic" instead of "lytic." He calls
attention to the fact that amylolytic, in analogy with electrolytic, means "decomposition by
means of starch" and is therefore a misnomer. He suggests the use of aniyloclastic,
proleoclaslic, etc.

^ Abwelirfennentc dcs tierischcn Organismus, 5th Ed., Berlin, 1915, Springer.

^Bronfenbrenner: Jour. Am. Med. Assn., 65, 1268, 1915. Van Slyke: Neiu York Med.
Jour., 103, 219, 1916.

^ Taylor: Jour. Biol. Chcm., 22, 59, 191 5.

4 PHYSIOLOGICAL CHEMISTRY

has very recently shown that "the rabbit does not form a protective
ferment in response to the injection of the protamine of the salmon. "
He, however, points out the fact that this does not prove that a de-
fensive enz}Tne is not formed in response to the passage of placental
protein into the blood.

Our knowledge regarding the distribution of enzymes has been
wonderfully broadened in recent years. Up to within a few years,
the real scientihc information as to the enzymes of the animal organism,
for example, was limited, in the main, to a rather crude understanding
of the enzymes intimately connected with the main digestive func-
tions of the organism. We now have occasion to beheve that enzymes
are doubtless present in every animal cell and are actively associated
with. all \-ital phenomena. As a preeminent example of such cellular
acti\-ity may be cited the liver cell with its reputed complement of 15-20
or more enzymes.

A list of the more important enz}-mes together with their class, dis-
tribution, substrate and end-products is given below.

CLASSIFICATION OF ENZYMES

Name and Class Distribution Substrate End-products

Carbohydrases "-^ i Carbohydrates j

I. Amylases Starch, dextrin, etc

(a) Pancreatic. . . . Pancreatic juice Starch, dextrin, etc Maltose.

(amylopsin')

(b) Salivary Saliva Starch, dextrin, etc Maltose.

(ptyalin)

(c) Vegetable Malt, rice fungus, etc Starch, dextrin, etc Maltose.

2. Glycogenase. . . .

Liver, muscles ? . . . .

Glycogen

. . . . Dextrin and maltose
(glucose?)

3. Inulase

Fungi, other plants.

Inulin

. . . . Fructose.

4. Lactase

Intestinal juice and

mucosa

Lactose

. . . . Glucose and galactose.

5. Maltase

Blood serum, Uver, saliva,
pancreatic and intestinal
juices and lymph.

Maltose

. . . . Glucose.

6. Sucrase

(invertasei

Intestinal juice and

mucosa.

Sucrose

. . . . Glucose and fructose.

7. Zymase

Yeast

Sugars

. . . . Alcohol, CQj, etc.

Carboxylase

Yeast

COOH group
acids.

of aUphatic Carbon dioxide.

Amino compounds ...

I. Adenase

Adenine

. . . . Hypoxanthine.

2. Arginase

Intestine, liver,
spleen, etc.

kidney,

Arginine

. . . . Ornithine and urea.

3. Guanase

Animal tissues

Guanin

. . . . Xanthine.

4. Urease

Micrococcus ureae, soy
bean, etc.

Urea

. . . . Carbon dioxide and am-
monia.

Glucosidases

1. Emulsin

2. Invertase

Plants

Yeast, etc

Glucosides (amygdalin
others).

/3-glucosides

o-glucosides

and

. . . . Glucose, etc.
. . . . Glucose, etc.

ENZYMES AND THEIR ACTION ;

CLASSIFICATION OF E'SZYMES.— Continued
Name and Class Distribution Substrate End-products

Lipases Fats

1. Autolytic Animal tissues Fats. P'atty acid an^i n.v,_^.-rv.i.

2. Pancreatic Pancreatic juice Fats. Fatty acid and glycerol.

(steapsin) . , , ,

3. Vegetable Castor bean, etc Fats Fatty acid and glycerol.

Nucleases N'ucleicacidand derivatives.

1. Nucleicacidase. . Intestinal mucosa and juice. Nucleic acid N'ucleotides.

other tissues.

2. Nucleotidase.. . . Intestinal mucosa and juice. Nucleotides Phosphoric acid and nu-

other tissues. cleosides.

3. Nucleosidase.. . . Tissues Nucleosides Carbohydrate and bases.

Oxidases.

1. Laccase Lac tree, fungi, etc Polyhydric para-phenols as Oxidation products.

hydroquinol and pyro-
gallol.

2. Peroxidase Plant and animal tissues. . . Organic pero.xides Oxygen or oxidation prod-

ucts.

3. Calalase Plant and animal tissues.. . Hydrogen peroxide Oxygen or oxidation prod-

ucts.

4. Purine-oxidases. Purines.

(a) Hypoxanthine Animal tissues Hypoxanthine. Xanthine.

oxidase.

(b) Uricase Animal tissues Uric acid .V.lantoin.

(c) Xanthine Animal tissues Xanthine Uric acid.

oxidase.

5. Tyrosinase Plant and animal tissues.. . Tyrosine. Homogentisic acid, etc.

Peptases Polypeptids

I . Erepsin Intestinal mucosa and juice. Peptids Simpler peptids and

other tissues. amino acids.

Phytase Rice bran, liver, blood Phytin Inositol and phosphoric

acid.

Proteases. Proteins

1. Coagulases .' Proteins in solution

(a^ Rennin Gastric juice Casein Paracasein.

(gastric)

(b) Rennin Pancreatic juice Casein Paracasein.

(pancreatic)

(c) Thrombin Blood ■ Fibrinogen. . . . Fibrin.

2. Pepsin Gastric juice Proteins Proteoses, peptones, and

(acid-protease) peptides.

3. Trypsin. ./..... Pancreatic juice Proteins Proteoses, peptones, pep-

(alkali-protease) ; tides, amino-acids.

4. Vegetable pro-j
teases.

(a) Bromelin Pineapple Proteins.. Proteoses, peptones, etc.

(b) Papain. Pawpaw Proteins.. Proteoses, peptones, etc.

(papayotin)

Purinases(see Purine
Oxidases and Pur-
ine Deaminases).

In text-book discussions of the enzymes it is customary to say that
very little is known regarding the chemical characteristics of these sub-
stances since no member of the enzyme group has, up to the present
time, been prepared in an absolutely pure condition. Apparently, how-
ever, from the nature of the facts in the case, it would be much more
accurate to say that we absolutely do not know whether a specific enzyme
has, or has not, been prepared in a pure state. (Some authors, like
Arthus, have assumed that enzymes are not chemical individuals, but
properties conferred upon bodies.) The enzymes are very difticult to
prepare in anything like a condition approximating purity, since they
are very prone to change their nature during the process by which the

O PHYSIOLOGICAL CHEMISTRY

investigator is attempting to isolate them. For this reason we have
absolutely no proof that the final product obtained is, or is not, in the
same state of purity it possessed in the original cell. Some of the en-
zymes are more or less closely associated with the proteins from the fact
that they are both formed in every cell as the result of the cellular ac-
tivity, both may be removed from solution by *' salting-out," both are
for the most part non-diffusible and are probably very similar as re-
gards elementary composition. Hence in the preparation of some
enzymes it is extremely difficult to make an absolute separation from
the protein. Most of the evidence points to the protein character of
enzymes.^ Under certain conditions enzymes are readily adsorbed by
shredded protein material, such as fibrin, and may successfully resist
the most prolonged attempts at washing them free. We may sum-
marize some of the properties of the great body of enzymes as follows :
Enzymes are soluble in dilute glycerol, sodium chloride solution,
dilute alcohol and water, and precipitable by ammonium sulphate
and strong alcohol. Their presence may be proven froin the nature
of the end-products of their action and not through the agency of any
chemical test. They are colloidal and non-diffusible, and occur closely
associated with protein material with which they generally possess many
properties in common. Each enzyme shows the greatest activity at a
certain temperature called the optimum temperature; there is also a
minimum and a maximum temperature for each specific enzyme. Their
action is inhibited by sufficiently lowering the temperature, although
some activity may be shown at o° or even at lower temperatures
and freezing does not, in most cases, permanently injure enzymes.
Most enzymes, if in solution, are entirely destroyed by subjecting
them to a temperature of 70-1 oo°C. The best known enzymes, whether
derived from warm-blooded or cold-blooded animals, are most active
between 35°-45°C. The nature of the surrounding media alters the
velocity of the enzymatic action, some enzymes being more active in
acid solution whereas others require an alkahne fluid.

Many of the more important enzymes do not occur preformed
within the cell, but are present in the form of a zymogen or mother-
substance. In order to yield the active enzyme this zymogen must be
transformed in a certain specific manner and by a certain specific sub-
stance. This transformation of the inactive zymogen into the active
enzyme is termed activation. For instance, the zymogen of the enzyme
pepsin of the gastric juice, termed pepsinogen, is activated by the hydro-
chloric acid secreted by the gastric cells (see page 141), whereas the actir
vation of the trypsinogen of the pancreatic juice is brought about by a

^ Others seem to be like the substrate on which they act, e.g., carbohydrate.

ENZYMES AND THEIR ACTION 7

substance termed enterokinase^ (see page 196). These are examples of
many well-known activation processes going on continually within the
animal organism. The agency which is instrumental in activating a
zymogen is generally termed a zymo-exciter or a kinase. In the cases
cited hydrochloric acid would be termed a zymo-exciter and entero-
kinase would be termed a kinase.

After filtering yeast juice, prepared by the Buchner process (see page
2), through a Martin gelatin filter, Harden and Young showed that
the colloids left behind and the filtrate were both inactive fermenta-
tively. Upon treating the colloid material (enz>Tne) with some of the
filtrate, however, the mixture was shown to be able to bring about pro-
nounced fermentation. It is believed that a co-enzyme present in the
filtrate was the efficient agent in the transformation of the inactive
enzyme. It is necessary to make frequent renewals of the co-enzyme
in order to maintain continuous fermentation. It was further shown
that this co-enzyme, in addition to being diffusible, was not destroyed
by boiling and that it disappeared from yeast juice when this latter
was fermented or allowed to undergo autolysis. The exact nature of
this co-enzyme of zymase is unknown. The co-enzyme action, in this
case, is probably dependent upon the presence of two individual
agencies, one of which is phosphates.

It has been shown by Loevenhart that the property of acting as a
pancreatic lipase co-enzyme is vested in hile salts, and ]VIagnus has
further shown that the synthetic salts are as efficient in this regard as
the natural ones. A few other instances of co-enzyme demonstrations
have been reported.

Electrolytes are very important factors in facilitating or inhibiting
enzyme action.^ For example, the CI ion in proper amount facihtates
the action of amylases.^ In fact the presence of the CI or Br ion is
apparently absolutely essential to the activity of pancreatic amylase,
inasmuch as dialysis renders this enzyme inactive, the activity return-
ing on the addition of sodium chloride.^ The acidity or hydrogen ion
concentration of the solution also exerts much influence on the activity
of enzymes. It has been demonstrated in the case of certain enz>Tnes,
at least, that the continuous vibration or shaking of their solutions tends
to produce a destruction of the enzyme. Ultraviolet light also has a
destructive action on enzymes.

The so-called "specificity" of enzyme action is an interesting and
important fact. That enzymes are very specific as to the character of

1 According to Delezenne, trypsinogen may be rapidly activated by soluble calcium salts.
- For literature, see Kendall and Sherman: Jour. Am. Client. Soc, 32, 1087, 1910.
' Wohlgemuth: Biochemisclte Zeilschrifl, q, 10, 1908.
* Bierry: Ibid., 40, 357, 191 2.

8 PHYSIOLOGICAL CHEMISTRY

the substrate, or substance acted upon, is well known. Emil Fischer
investigated this problem of specificity extensively in connection with
the fermentation of sugars and reached the conclusion that enzymes,
with the possible exception of certain oxidases, can act only upon such
substances as have a specific stereo-isomeric relationship to themselves.
He considers that the enzyme and its substrate must have an inter-
relation, such as the key has to the lock, or the reaction does not occur.
Fischer was able to predict, in certain definite cases, from a knowledge
of the constitution and stereo-chemical relationships of a substance,
whether or not it would be acted upon by a certain enzyme. An appli-
cation of this specificity of enzyme action may be seen in the well-known
facts that certain enzymes act on carbohydrates, others on fats, and
others on protein; and, moreover, that the group of those which trans-
form carbohydrates, for example, is further subdivided into specific en-
zymes each of which has the power of acting alone upon some one sugar.

It has been conclusively shown, in the case of certain enzymes,^
at least, that their action is a reversible one and is, in all its main fea-
tures, directly analogous to the reversible reactions produced by chem-
ical means. For instance, in the saponification of ethyl-butyrate by
means of pancreatic lipase, it has been shown that upon the formation
of the end-products of the reaction, i.e., butyric acid and ethyl alcohol,
there is reversion^ and the reaction is stationary. This does not mean
there are no chemical changes going on, but simply indicates that
chemical equilibrium has been established, and that the change in one
direction is counterbalanced by the change in the opposite direction.
Pancreatic lipase was one of the first enzymes to have the reversibility
of its reaction clearly demonstrated.^ A knowledge of the fact that
lipase possesses this reversibility of action is of extreme physiological
importance and aids us materially in the explanation of the processes
involved in the digestion, absorption, and deposition of fats in the
animal organism (see page 178).

Euler^ claims that enzymatic cleavage and synthesis are often brought
about by two different components of an enzyme preparation. He
would indicate this fact by giving the termination -ese to those enzymes
exerting a synthetic function. For example, the enzyme which catalyzes
the formation of nitriles Euler would call nitrile^e in distinction from
nitrila^e which splits nitriles. He would further designate as phos-

' This is probably a general condition.

^ The re-synthesis of ethyl-butyrate from its hydrolysis products. This may be indi-
cated thus:

C3H7COO.C2H5+H20fc>C3H7COOH+C2H50H.

Elhyl-biUyrale. Butyric acid. Ethyl alcohol.
3 This principle was first demonstrated in connection with the enzyme maltase (seep. 57).
* Euler: Zcilschrijljiir physiologische chemie, 74, 13, 191 1.

ENZYMES AND THEIR ACTION 9

phatese the enzyme which builds up phosphoric acid esters of carbo-
hydrates in distinction from phosphatase which causes their cleavage.
In the same way he would differentiate the lipolytic enzymes into lipases
and lipeses.

In respect to many enzymes it has been found that the law govern-
ing the action of inorganic catalyzers is directly applicable, i.e., that
the intensity is almost directly proportional to the concentration of the
enzyme. In the case of enzymes, however, there is a difference in that a
maximum intensity is soon reached and that subsequent concentration
of the enzyme is productive of no further increase in intensity. The en-
zymes which have been shown to obey this linear law are lipase, sucrase,
rennin, and tr\'psin. In certain instances, where this law of direct
proportionality betweien the intensity of action and the concentration
of enzymes does not hold, it has been found that the Schutz-Borissow
law, first experimentally demonstrated by E. Schiitz, was applicable.
This is to the effect that the intensity is directly proportional to the
square root of the concentration, or conversely, that the relative con-
centrations of enzyme preparations are directly proportional to the squares
of the intensities}

It has been shown that there are certain substances which possess
the property of directly inhibiting or preventing the action of a cata-
lyzer. These are called anti-catalyzers or paralyzers and have been com-
pared to the anti-toxins. Related to this class of anti-catalytic agents
stand the anti-enzymes. The first anti-enzyme to be reported was the
antirennin of Morgenroth. This was produced by injecting into an
animal increasing doses of rennet solution, whereupon an "anti"
substance was subsequently found both in the serum and in the milk,
which prevented the enzyme rennin from exerting its normal activity
in the presence of casein. In other words, anti-rennin had been
formed in the serum of the animal,- through the repeated injections of
rennet solution. Since the discovery of this anti-enz)Tne, anti-bodies
have been demonstrated for pepsin, trypsin, lipase, urease, amylase,
laccase, tyrosinase, emulsin, papain, and thrombin. According to
Weinland, the reason why the stomach does not digest itself is. that
during life there is present in the mucous membrane of the stomach an
anti-enzyme (anti-pepsin) which has the property of inhibiting the action
of pepsin. A similar substance (anti-trypsin) is present in the intestinal
mucosa as well as in the tissues of various intestinal worms. Some in-
vestigators are not inclined to accept the enzyme nature of these
inhibitory agents as proven.

^ This Schutz-Borissow law is not generally applicable.
* Serum is normally anti-lryplic.

lO PHYSIOLOGICAL CHEMISTRY

The investigations of Ehrlich^ and of Neuberg^ have served to cause
a complete revision of our ideas regarding yeast fermentation. EhrKch,
for example, has shown that yeast will liberate ammonia from amino acids
and leave behind a non-nitrogenous complex. Among these complexes
amyl alcohol, succinic acid and others may be mentioned. Thus, amyl
alcohol results from the fermentation of leucine, whereas ethyl alcohol
results from the fermentation of sugar. Neuberg has demonstrated the
presence in the yeast of an enzyme termed carboxylase which has the
property of splitting of carbon dioxide from the carboxyl group of amino
and other aliphatic acids. The findings mentioned above constitute the
basis for much important work on so-called "sugar-free fermentation."

For a more extended consideration of enzymes the student is referred
to the following sources:

Bayliss. — The Nature of Enzyme Action, Third Edition, Long-
mans, Green and Co., New York and London.

CoHNHEiM. — Enzymes, Wiley and Sons, New York, 191 2.

DucLAUX. — Traite de Microbiologic, Masson and Co., Paris.

Effront. — Enzymes and their Applications, Translated by Pres-
cott, Wiley and Sons, New York.

EuLER. — (a) Allgemeine Chemie der Enzyme, Bergmann, Wies-
baden, 1910. (b) Ergebnisse der Physiologic, 1909-10. (c) General
Chemistry of the Enzym.es, Translated by Pope, Wiley and Sons,
1912.

Oppenheimer. — Die Fermente und Ihre Wirkungen, Vierte Auflage,
Vogel, Leipzig.

Samuely. — Handbuch der Biochemie des Menschen und der Thiere
(Oppenheimer), Gustav Fischer, Jena, 1910-11.

Wohlgemuth. — Grundriss der Fermentmethoden, 1913, Berlin,
Springer.

EXPERIMENTS ON ENZYMES AND ANTI-ENZYMES
A. Experiments on Enzymes^

I. AMYLASES

I. Demonstration of Salivary Amylase.* — ^To 25 c.c. of a i per cent starch
paste in a small beaker, add 5 drops of saliva and stir thoroughly. At intervals
of a minute remove a drop of the solution to one of the depressions of a test-tablet

' Ehrlich: Biochemische Zeitschrifl, 36, 477, 191 1.

* Neuberg and Collaborators: Biochemische Zeitschrifl, 31, 170; 32, 323; 36 (60, 68, and
76). 1911.

2 If it is deemed advisable by the instructor to give all the practical work upon enzymes
at this point in the course, additional experiments will be found in Chapters III, VI, VII,
X and XI.

* For a discussion of this enzyme see p. 55.

ENZYMES AND THEIR ACTION II

and test by the iodine test.^ If the blue color with iodine still forms after five
minutes, add another 5 drops of saliva.

The opalescence of the starch solution should soon disappear,
indicating the formation of sohible starch {amidtilin) which gives a blue
color with iodine. This body should soon be transformed into erythro-
dextrin which gives a red color with iodine, and this, in turn, should
pass into achroodextrin which gives no color with iodine. This point is
called the achromic point. When this point is reached test by Fehling's
test^ to show the production of a reducing substance (maltose). A
positive Fehling's test may be obtained while the solution still reacts red
with iodine, inasmuch as some sugar is formed from the soluble starch
coincidently with the formation of the erythrodextrin. For further
discussion of the transformation of starch see page 56.

2. Demonstration of Pancreatic Amylase.^ — Proceed exactly as indicated above
in the Demonstration of Salivary Amylase except that the saliva is replaced by 5 c.c.
of pancreatic extract prepared as described on p. 189.'* Pancreatic amylase trans-
forms the starch in a manner entirely analogous to the transformation resulting
from the action of salivary amylase.

3. Preparation of Vegetable Amylase. — Extract finely ground malt with water,
filter and subject the filtrate to alcohoUc fermentation by means of yeast. When
fermentation is complete filter off the yeast and precipitate the amylase from the
filtrate by the addition of alcohol. The precipitate may be filtered off and ob-
tained in the form of a fine white powder.

A purer preparation^ is obtained if the solution is dialyzed against
water at about io°C. (in the ice-box) for 24 hours, filtered and pre-
cipitated with alcohol or acetone. First alcohol or acetone to make a 50
per cent solution is added, the precipitate thus formed being rejected,
while the precipitate formed on the addition of sufficient alcohol or
acetone to make a final concentration of 65-70 per cent is preserved, and
dried in a vacuum desiccator at a low temperature.

4. Demonstration of Vegetable Amylase. — This enzyme may be demon-
strated according to the directions given under Demonstration of SaUvary Amylase,
page 10, with the exception that the sahva used in that experiment is replaced by
an aqueous solution of the vegetable amylase powder prepared as described
above. ^

^ See p. 45.

* See p. 26.

^ For a discussion of this enzyme see p. 187.

* Commercial preparations of pancreatic amylase may be substituted for the pancreatic
extract.

'Sherman and Schlesinger: /. Am. Ch. Soc, 35, 1617, 1915.

^ If desired the first aqueous extract of the original malt may be used in this demonstra-
tion. Commercial taka-diaslase may also be employed.

12 PHYSIOLOGICAL CHEMISTRY

n. PROTEASES

1. Preparation of Gastric Protease. ^ — Treat the finely comminuted mucosa of
a pig's stomach with 0.4 per cent hydrochloric acid and extract at 38°C. for
24-48 hours. The filtrate from this mixture constitutes a very satisfactory acid
extract of gastric protease (see page 144).

2. Demonstration of Gastric Protease. — Introduce some protein material
(fibrin, coagulated egg-white, or washed lean beef) into the acid extract of gastric
protease prepared as above described,'- add an equal volimie of 0.4 per cent
hydrochloric acid and place the mixture at 38°C. for 2-3 days. Identify the
products of digestion according to directions given on page 144.

Carmine- fibrin may also be used in this test. This is prepared
by running fibrin through a meat chopper washing carefully and placing
in a }4 per cent ammoniacal carmine solution (very little excess am-
monia should be present) until the maximum coloration of the fibrin
(a dark red) is obtained. The fibrin is then washed in water and water
acidified with acetic acid. It is preserved under glycerol.

To 15 c.c. of the solution to be tested add a small amount of the
carmine fibrin and allow to digest at room temperature. Digestion will
be shown by the setting free of carmine with coloration of the solution.
This is a delicate test for pepsin. A control should be run using acid of
same strength as that of enzyme solution tested.

3. Preparation of Pancreatic Protease.^ — A satisfactory extract of this
enzyme may be made from the pancreas of a pig or sheep according to the direc-
tions given on page 189.

4. Demonstration of Pancreatic Protease. — Into an aUcaUne extract of pan-
creatic protease,^ prepared as directed on page 189, introduce some fibrin, coagu-
lated egg-white or lean beef and place the mixture at 38°C. for 2-5 days.* At
the end of that period separate and identify the end-products of the action of pan-
creatic protease according to the directions given on page 189.

Congo-red fibrin may be used in this test. This may be prepared
by placing fibrin in faintly alkaline congo-red solution and heating to
8o°C. The fibrin is then washed. A small amount of this colored
fibrin is placed in the slightly alkaline solution of the enzyme. Diges-
tion is shown by a red coloration of the solution due to setting free of
Congo red.

' Also called pepsin, pepsase, gastric protease and acid protease. For a discussion of this
enzyme see p. 141.

^ If so desired, a solution of commercial pepsin powder in 0.2 per cent hydrochloric acid
may be substituted.

^ .\lso called trypsin, irypsase, pancreatic protease and alkali protease. For a discussion
of this enzyme see p. 186.

^ A 0.25 per cent sodium carbonate solution of commercial trypsin or pancreatin may be
substituted.

. 5 A few c.c. of toluol or an alcoholic solution of thymol should be added to prevent putre-
faction.

ENZYMES AND THEIR ACTION 1 3

5. Demonstration of a Vegetable Protease. — A commercial preparation of
papain {papayotin, carase or papase), the protease of the fruit of the pawpaw (carica
papaya), may be used in this connection. Follow the same procedure as that de-
scribed under Gastric Protease (see p. 12).

It has been demonstrated by IMendel and Blood' that the presence of HCN
will accelerate the proteolytic activity of papain. It is suggested that the HCN
acts as a so-called co-enzyme (see page 7).

Vines- believes that "papain" consists of a mixture of two enzymes, a pepsin
and an erepsin. Mendel and Blood do not consider the evidence on this point as
conclusive.

m. LIPASES

1. Preparation of Pancreatic Lipase.* — An extract of this enzyme may be
prepared from the pancreas of the pig or sheep according to the directions given
on page 189.'

2. Demonstration of Pancreatic Lipase. — Into each of two test-tubes intro-
duce 10 c.c. of milk and a small amount of litmus powder. To the contents of one
tube add 3 c.c. of a neutral extract of pancreatic lipase and to the contents of the
other tube add 3 c.c. of a boiled neutral extract of pancreatic lipase. Keep the
tubes at 38°C. and watch for color changes.

The blue color of the litmus powder will gradually give place to a
red. This change in color of the litmus from blue to red has been
brought about by the fatty acid which has been produced through the
lipolytic action exercised by the lipase upon the milk fats.

3. Preparation of Vegetable Lipase. — This enzyme may be readily prepared
from castor beans, several months' old, by the following procedure:* Grind the
shelled beans very fine^ and extract for twenty-four-hour periods with alcohol-ether
and ether, in turn. Reduce the semi-fat-free material to the finest possible consist-
ency by means of mortar and pestle and pass this material through a sieve of very
fine mesh. Place this material in a Soxhlet extractor and extract for one week.
This fat-free powder may then be used to demonstrate the action of vegetable
lipase. Powder prepared as described may be used in quantitative tests. For
ordinary qualitative tests it is not necessary to remove the last traces of fat and
therefore the extraction period in the Soxhlet apparatus may be much shortened.

4. Demonstration of Vegetable Lipase. — The lipolytic action of the lipase pre-
pared from the castor bean, as just described, may be demonstrated in a manner
entirely analogous to that used in the Demonstration of Pancreatic Lipase, see
above. Proceed as indicated in that experiment and substitute the vegetable
lipase powder for the neutral extract of pancreatic lipase. The type of action is
entirely analogous in the two instances.

^ Mendel and Blood: Journal of Biological Chemistry, 8, 177, 1910.

''Vines: Annals of Botany, 19, 174, 1905.

' Also called steapsin. P'or a discussion of the enzyme see p. 188. .V very active lipo-
lytic extract may also be prepared from the liver.

* If preferred, a glycerol extract may be prepared according to the directions given by
Kanitz {Zeitschrift fiir physiologische Chemie, 1906, 46, p. 482) or commercial pancrealin
may be employed.

^ A. E. Taylor: On Fermentation; University of California Publications, igo-;.

^ The shells should be removed without the use of water. These beans are poisonous,
due to their content of ricin.

14 PHYSIOLOGICAL CHEMISTRY

An experiment similar to Experiment 2, page 193, may also be tried if desired.
In this experiment 0.2 c.c. of either ethyl buiyrate or aniyl acetate may be employed.

IV. INVERTASESi

1. Preparation of Vegetable Sucrase.- — Thoroughly grind about 100 grains of
brewer's yeast in a mortar with sand. Spread the ground yeast in thin layers on
glass or porous plates and dry it rapidly in a current of dry, warm air. Powder
this dry yeast, extract it with distilled water and filter. Pour the filtrate into
acetone, stir and after permitting the acetone mixture to stand for a few minutes
filter on a Buchner funnel. The resulting precipitate, after drying and pulver-
izing, may be used to demonstrate vegetable sucrase.

2. Demonstration of Vegetable Sucrase. — To about 5 c.c. of a i per cent
solution of sucrose in a test-tube add a small amount of the sucrase powder pre-
pared as directed above. Place the tube at 38°C. for 24-72 hours and at the end
of that period test the solution by Fehling's test. Reduction indicates that the
active sucrase powder has transformed the non-reducing sucrose into glucose
and fructose, and these sugars, in turn, have reduced the Fehling solution.

For other experiments on Invertases, see Chapter XI.

V. OXIDASES 3

I. Demonstration of Oxidase.- — Oxidases or oxidizing enzymes con-
stitute a very important group of intracellular enzymes. They are
intimately connected with the oxidation processes in the plant and ani-
mal organisms.

1. Cut a thin slice from a freshly pared potato, place it on a watch glass and
examine at intervals during the laboratory exercise. Note that the colorless
potato gradually becomes brown.

This is due to the oxidation of para-oxyphenyl substances such as
tyrosin, in the cells and in the intracellular juice of the potato. Two
oxidases which have the power of accelerating the oxidation of para-
oxyphenyl compounds are called tyrosinase and laccase.

2. Preparation of Potato Extract. — Scrape a pared potato by means of a knife
or scalpel or comminute the potato substance by means of a grater. Extract the
macerated potato substance by means of water. Strain through cheese cloth and
filter the extract. Make an iodine test on the solid substance (see Starch, page
45), and save the water extract for use in the following experiments.

3. Oxidation of Para-oxyphenyl Compounds by Potato Oxidases. — Introduce
5 c.c. of filtered potato extract prepared as indicated above, into each of six test-
tubes. Introduce additional reagents into the tubes according to the following
series :

(a) Potato extract + 5 drops of toluol (control).

(b) Potato extract + 5 drops of ether (control).

* The inverting enzymes of the alimentary tract; Mendel and Mitchell: American Journal
of Physiology, 20, 81, 1907-08.

2 For a discussion of this enzyme see p. 195.

2 These experiments have been adapted from directions contained in the Laboratory
Notes of Professor Gies of the College of Physicians and Surgeons, New York.

ENZYMES AND THEIR ACTION 1 5

(c) Potato extract + 5 drops of i per cent phenol solution.

(d) Potato extract + 5 drops of i per cent '* tri-cresol " solution.

(e) Potato extract (boiled and cooled) + 5 drops of i per cent phenol solution,

(f) Potato extract (boiled and cooled) -f- 5 drops of i per cent "tri-cresol"
solution.

Shake the contents of the six tubes thoroughly. Are there any immediate
color changes? Place the tubes in your rack, and examine them at the next
laboratory exercise.

4. Experiments with Typical Oxidase Reagents. — Introduce 5 c.c. of filtered
potato extract into each of four test-tubes. Add oxidase reagents as follows :

(a) Potato extract + 10 drops of guaiac solution.^

(b) Potato extract + 10 drops of a-naphthol solution. -

(c) Potato extract +10 drops of para-phenylenediamine hydrochloride
solution.^

(d) Potato extract + 5 drops of a-naphthol solution + 5 drops of para-
phenylenediamine hydrochloride solution + 5 drops of 10 per cent sodium
carbonate (Indophenol Test).

Shake the contents of each tube thoroughly and note immediate color
changes. Place the tubes in the rack and leave them undisturbed until the
end of the laboratory exercise. Note any changes or pecuUarities in the color-
ation efifects, especially at the surface of the liquid.

In tube (a) the guaiaconic acid of the guaiac resin has been oxidized
and formed guaiac blue.

In tube (b) a violet coloration due to the production of di-naphthol
appears. The oxidase has oxidized the a-naphthol.

In tube (c) we have a change whose chemistry is not well known.

In tube (d) we have the production of indophenol from the a-naph-
thol and the para-phenylenediamine hydrochloride under the influence of
oxidase. The indophenol is soluble in the alkaline solution. The color
gradually changes from red to purple as the indophenol accumulates.

The production of the above colors does not possess any biological
significance. These colors simply serve to indicate that certain reac-
tions are taking place which occur normally in living cells, although
in the latter case they are of course unaccompanied by any color
change. Intracellular oxidase favors the utilization of oxygen by a
cell, just as the potato oxidase has facilitated the oxidation of the
chromogens in the above tests.

VI. CATALASE

Demonstration of Catalase. — The various animal tissues as liver,

kidney, blood, lung, muscle and brain contain an enzyme called catalase

or peroxidase which possesses the property of decomposing hydrogen

1 Made by dissolving 0.5 gram of guaiac resin in 30 c.c. of 95 per cent alcohol.
^ Made by dissolving i gram of a-naphthol in 100 c.c. of 95 per cent alcohol.
^ Dissolve I gram of para-phenylene diamine hydrochloride in 100 c.c. of water.

1 6 PHYSIOLOGICAL CHEMISTRY

peroxide as well as certain biological peroxides with the liberation of
oxygen. Catalase is an indirect oxidizing enzyme, that is, it brings about
oxidations only in the presence of a peroxide. Catalase is also found in
many plant tissues and an extract of it may be prepared from potatoes.

1. Vegetable Catalase. — Into each of four test-tubes place 5 c.c. of filtered
potato extract prepared as in Experiment 2, page 14. Prepare a second
series of four tubes (see 4, p. 15), but use a boiled potato extract. Prepare
also a third series using water instead of potato extract. Now add to each
of the twelve tubes 5 drops of a 3 per cent solution of hydrogen peroxide. While
the resultant Uvely effervescence is in progress add to each series the four
"Typical Oxidase Reagents" in the order and quantities specified in the preceding
experiment (4). Allow the tubes to remain undisturbed and carefully note com-
parative effects during the remainder of the laboratory exercise.^

2. Animal Catalase. — The presence of this enzyme may also be demonstrated
as follows: Introduce into a low, broad, wide-mouthed bottle some pulped liver
tissue and a porcelain crucible containing neutral hydrogen peroxide.^ Connect the
bottle with a eudiometer filled with water, upset the crucible of hydrogen peroxide
upon the liver pulp and note the collection of gas in the eudiometer. This gas is
oxygen which has been liberated from the hydrogen peroxide through the action of
the catalase of the liver tissue.

See next experiment for a method for the quantitative determination of catalase
based on the above principle.

3. Quantitative Determination of Catalase.^ — In the determination of the
catalase values of tissues weighed portions of the tissue under examination should
be ground with sand in a mortar then treated with four volumes of chloroform water
and permitted to extract for 24 hours at room temperature. An apparatus such
as that shown in Fig. i may be employed in determining the catalase values. The
main features of the apparatus are based upon those of a dehvery funnel for intro-
ducing liquids under increased or diminished pressure.

In making a determination introduce a measured volume (1-4 c.c.) of the filtered
extract^ into the small flask and insert the modified Johnson burette graduated to
5 c.c. and containing 50 c.c. of hydrogen peroxide (Oakland dioxygen neutral^ to
Congo red) into the neck of the flask. Fill the eudiometer with water and place in
position. Close cocks A and C and open cocks B and D thus permitting 5 c.c. of
the peroxide to flow into the flask. Shake the contents of the flask briskly^ and
record the volume of oxygen evolved in a two-minute period taking readings at
intervals of fifteen seconds.

Calculation. — When a series of comparative tests are made on different tissues
or on the same tissue under different conditions it is considered satisfactory to make
a comparison of the catalase values upon the basis of the volume of oxygen evolved

^ This experiment has been adapted from one contained in the Laboratory Notes of '
Professor Gies of the College of Physicians and Surgeons, New York.

^ Mendel and Leavenworth: American Journal of Physiology, 21, 85, 1908.
^ Hawk: Journal of American Chemical Society, 33, 425, igii.

* If less than 4 c.c. of extract are used the volume should be made up to 4 c.c. bj' the
addition of distilled water.

^ An acid reactioji modifies the rate of the oxygen evolution. (See Mendel and Leaven-
worth, American Journal of Physiology, 21, 85, 1908.)

* In making a series of comparative tests it is essential that the shaking process should be
uniform from determination to determination.

ENZYMES AND THEIR ACTION

17

in a period of two minutes from 5 c.c. of neutral hydrogen peroxide by means of i c.c.
of a I : 4. chloroform-water extract of the tissue.

B. Experiments on Anti-Enzymes

I, F>reparation of an Extract of Anti -Pepsin. ' — Grind up a number of intestinal
worms (ascaris)- with quartz sand in a rnortar. Subject this mass to high pressure,
filter the resultant juice and treat it with alcohol until a concentration of 60 per
cent is reached. If any precipitate forms it should be filtered off^ and alcohol
added to the filtrate until the concentration of alcohol is 85 per cent, or over. The
anti-enzyme is precipitated by this concentration. Permit this precipitate to stand

Fig. I. — .\i>PARATUs for QuANTixAxrvE Determination of Catalase.

for twenty-four hours, then filter it off, wash it with 95 per cent alcohol, absolute
alcohol, and ether, in turn, and finally dry the substance over sulphuric acid. The
sticky powder which results may be used in this form or may be dissolved in water as
desired and the aqueous solution used.''

2. Demonstration of Anti-Pepsin.^ — Introduce into a test-tube a few fibrin
shreds and equal volumes of pepsin-hydrochloric acid® and ascaris extract made as
indicated above. Prepare a control tube in which the ascaris extract is replaced by
water. Place the tubes at 38°C. Ordinarily in one hour the fibrin in the control
tube will be completely digested. The fibrin in the tube containing the ascaris
extract may, however, remain unchanged for days, thus indicating the inhibitory
influence exerted by the anti-enzyme present in this extract.

^ Anti-gastric-protease or anti-acid-protease.

* These may be readily obtained from pigs at a slaughter house.

^ This precipitate consists of impurities, the anti-enzyme not being precipitated until a
higher concentration of alcohol is reached.

* The original ascaris extract possesses much greater activity than either the powder or
the aqueous solution.

^ ^lartin H. Kischer: Physiology of Alitmntalion. 1007, p. 134.

* Made by bringing 0.015 gram of pepsin into solution in 7 c.c. of water and 0.23 gram
of concentrated hvdrochloric acid.

1 8 PHYSIOLOGICAL CHEMISTRY

3. Preparation of an Extract of Anti -Trypsin.' — The extract may be prepared
from the intestinal worm, ascaris, according to the directions given on page 17.

4. Demonstration of Anti-Trypsin. — Introduce into a test-tube a few shreds
of fibrin and equal volumes of an artificial tryptic solution^ and the ascaris extract
made as described on page 17. Prepare a control tube in which the ascaris
extract is replaced by water. Place the two tubes at 38°C.

Ordinarily the fibrin in the control tube will be completely digested
in two hours. The fibrin in the tube containing the ascaris extract may,
however, remain unchanged for days, thus indicating the inhibitory
influence of the anti-enzyme.

Blood serum also contains anti-try psin. This may be demonstrated
as follows: Introduce equal volumes of serum and artificial tryptic
solution (prepared as described above) into a test-tube and add a few
shreds of fibrin. Prepare a control tube containing boiled serum. Place
the two tubes at 38°C. It will be observed that the fibrin in the tube
containing the boiled serum digests, whereas that in the other tube does
not digest. The anti-trypsin present in the unboiled serum has exerted
an inhibitory influence upon the action of the trypsin.

C. Quantitative Applications

Methods for the quantitative determination of various enzymes
will be found in the following chapters: Amylase (Chapter X);
Erepsin (Chapter XI) ; Pepsin (Chapter VIII) ; Trypsin (Chapter X) ;
Urease (Chapter XXVI).

^ Anti-pancreatic-protease or anti-alkali-protease.

^Made by dissolving 0.04 gram of sodium carbonate and 0.015 pram of trypsin in 8
c.c. of water.

CHAPTER II
CARBOHYDRATES

The name carbohydrates is given to a class of bodies which are an
especially prominent constituent of plants and which are found also in
the animal body either free or as an integral part of various proteins.
They are called carbohydrates because they contain the elements C, H
and O; the H and 0 being present in the proportion to form w^ater. The
term is not strictly appropriate inasmuch as there are bodies, such as
acetic acid, lactic acid and inositol, which have H and O present in the
proportion to form water, but which are not carbohydrates, and there
are also true carbohydrates which do not have H and O present in this
proportion, e.g., rhamnose, C6H12O5.

Chemically considered, the carbohydrates are aldehyde or ketone
derivatives of complex alcohols. Treated from this standpoint, the
aldehyde derivatives are spoken of as aldoses, and the ketone derivatives
are spoken of as ketoses. The carbohydrates are also frequently named
according to the number of oxygen atoms present in the molecule, e.g.,
trioses, pentoses, and hexoses.

The more common carbohydrates may be classified as follows:

I. Monosaccharides.

1. Pentoses, C5H10O5.

{a) Arabinose.

(b) Xylose.

(c) Rhamnose (Methyl-pentose), CeHioOs-

2. Hexoses, CeH^Oe.

(a) Glucose.

(b) Fructose.

(c) Galactose.

II. Disaccharides, CisHooOu-

1. Maltose.

2. Lactose.

3. Iso-Maltose.

4. Sucrose.

, III. Trisaccharides, C18H32O16.
I. Raffinose.

19

20 PHYSIOLOGICAL CHEMISTRY

IV. Polysaccharides, (C6Hio05)x-

1. Gum and Vegetable Mucilage Group.

(a) Dextrin.

(b) Vegetable Gums.

2. Starch Group.

(a) Starch.
{b) Inulin.

(c) Glycogen.

(d) Lichenin.

3. Cellulose Group.

{a) Cellulose.

(b) Hemicelluloses.

(i) Pentosans.

Gum Arabic.
(2) Hexosans.

Galactans.
Agar-agar.

Each member of the above carbohydrate classes, except the members
of the pentose group, may be supposed to contain the group CeHioOs,
called the saccharide group. The polysaccharides consist of this group
alone taken a large number of times, whereas the disaccharides may be
supposed to contain two such groups plus a molecule of water, and the
monosaccharides to contain one such group plus a molecule of water.
Thus, (CeHioOs).^ = polysaccharide, (CeHioOsji + HoO — ^ disacchar-
ide, CeHioOs + H2O -^ monosaccharide. In a general way the solu-
bility of the carbohydrates varies with the number of saccharide groups
present, the substances containing the largest number of these groups
being the least soluble. This means simply that, as a class, the mono-
saccharides (hexoses) are the most soluble and the polysaccharides
(starches and cellulose) are the least soluble.

MONOSACCHARIDES

Hexoses, CeHiiOe

The hexoses are monosaccharides containing six oxygen atoms in a
molecule. They are the most important of the simple sugars, and two
of the principal hexoses, glucose and fructose, occur widely distributed
in plants and fruits. Of these two hexoses, glucose results from the
hydrolysis of starch, whereas both glucose and fructose are formed in
the hydrolysis of sucrose. Galactose, which with glucose results from
the hydrolysis of lactose, is also an important hexose. These three
hexoses are fermentable by yeast, and yield levulinic acid upon heating

CARBOHYDRATES 2 1

with dilute mineral acids. They reduce metallic oxides in alkaline
solution, are optically active and extremely soluble. With phenyl-
hydrazine they form characteristic osazones.

CH2OH

GLUCOSE (CH0H)4

j
CHO

Glucose, also called dextrose or grape sugar, is present in the blood
in small amount and also occurs in traces in normal urine. ^ After
the ingestion of large amounts of sucrose, lactose or glucose, causing
the assimilation limit to be exceeded, an ahmentary glycosuria may
arise. In diabetes mellitus very large amounts of glucose are excreted
in the urine. The following structural formula has been suggested by
Victor Meyer for (/-glucose:

CHO

H— C— OH

HO— C— H

I
H— C— OH

I
H— C— OH

CH2OH

(For further discussion of glucose see section on Hexoses, page 20.)

Experiments on Glucose

The following tests are made on glucose as a typical carbohydrate
and are not specific for this sugar. A specific test for glucose is the
Phenylhydrazine Reaction (3) in the absence of a positive Resorcinol-
Hydrochloric Acid Reaction (see page 35).

1. Solubility. — Test the solubility of glucose in the "ordinary solvents" and
in alcohol. (In the solubility test throughout the book we shall designate the
following solvents as the "ordinary solvents:" H2O; 10 per cent NaCl; 0.5 per
cent Na^COs; 0.2 per cent HCl; concentrated KOH; concentrated HCl. '

2. a-Naphthol Reaction (Mohsch). Place approximately 5 c.c. of concen-
trated HoSO.) in a test-tube. Incline the tube and slowly pour down the inner
side of it approximately 5 c.c. of the sugar solution to which 2 drops of Mo-
lisch's reagent (a 15 per cent alcoholic solution of a-naphthol) has been added,
so that the sugar solution will not mix with the acid. A reddish-violet zone
is produced at the point of contact.

' See Folin's test for sugar in normal urine [Jour. Biol. Cheni., 22, 327, 1915).

22 PHYSIOLOGICAL CHEMISTRY

The reaction is due to the formation of furfural.^

HC— CH

il II
HC CCHO,

\/

o

by the acid. The test is given by all bodies containing a carbohydrate
group and is therefore not specific and, in consequence, of very little
practical importance.

3. Phenylhydrazine Reaction. — Test according to one of the following
methods : (a) To a small amoimt of phenylhydrazine mixture (enough to fill the
rounded portion of a small test-tube) fiunished by the instructor, ^ add 5 c.c.
of the sugar solution, shake well and heat on a boiling water-bath for one -half to
three-quarters of an hour. Allow the tube to cool slowly (not under the tap)
and examine the crystals microscopically (Plate III, opposite) .

If the solution has become too concentrated in the boiling process it
will be light red in color and no crystals will separate until it is diluted
with water.

Yellow crystalline bodies called osazones are formed from certain
sugars under these conditions, in general each individual sugar giving
rise to an osazone of a definite crystalline form which is typical for that
sugar. It is important to remember in this connection that of the
simple sugars of interest in physiological chemistry, glucose and fructose
yield the same osazone. Each osazone has a definite melting-point
and as a further and more accurate means of identification it may be
recrystallized and identified by the determination of its melting-point
and nitrogen content. The reaction taking place in the formation of
phenylglucosazone is as follows :

CH2OH

I
(CHOH)3

CHOH

+C6H5NH-NH2

CHoOH

(CH0H)3
I +C6H5NH-NH2-

CHOH
I ^N-NHCeHs+HzO

\H

Glucose

Phenylhydrazine

\H

Phenylhyd razone

' According to v. Ekenstein and Blanksma {Ber. d. d. chem. GeselL, 43, 2358, 1910),
oxymethylfurfural is formed.

2 This mixture is prepared by combining one part of phenylhydrazine hydrochloride and
two parts of sodium acetate by weight. These are thoroughly mixed in a mortar.

PLATE III.

OSAZONES.

Upper form, dextrosazone; central form, maltosazone; lower form, lactosazone.

CARBOHYDRATES 23

CH2OH CH2OH

(CH0H)3 (CH0H)3

I +C6H5NH-XH2^ I

C = 0 C = N-NHC6H5+H20
I ^N-NHC6H5+C6H5NH2+NH3 ^X-NHCsHb

C C

Aniline Glucosazone

(b) Place 5 c.c. of the sugar solution in a test-tube, add i c.c. of the phenyl-
hydrazine-acetate solution furnished by the instructor/ and heat on a boiling
water-bath for one -half to three-quarters of an hour. Allow the Uquid to cool
slowly and examine the crystals microscopically (Plate III, opposite p. 22).

The phenylhydrazine test has been so modified by Cipollina as to
be of use as a rapid clinical test. The directions for this test are given
in the next experiment.

4. Cipollina's Test. — Thoroughly mix 4 c.c. of dextrose solution, 5 drops of
phenylhydrazine (the base) and J^ c.c. of glacial acetic acid in a test-tube. Heat
the mixture for about one minute over a low flame, shaking the tube continually to
prevent loss of fluid by bumping. Add 4-5 drogs of sodium hydroxide (sp. gr. 1.16),
being certain that the fluid in the test-tube remains acid, heat the mixture again for
a moment and then cool the contents of the tube. Ordinarily the crystals form at
once, especially if the sugar solution possesses a low specific gravity. If they do
not appear immediately allow the tube to stand at least 20 minutes before deciding
upon the absence of sugar.

Examine the crystals under the microscope and compare them with those shown
in Plate III, opposite page 22.

5. Riegler's Reaction. ^ — Introduce o.i gram of phenylhydrazine-hydrochloride
and 0.25 gram of sodium acetate into a test-tube, add 20 drops of the solution under
examination and heat the mixture to boiling. Now introduce 10 c.c. of a 3 per cent
solution of potassium hydroxide and gently shake the tube and contents. If the
solution under e.Kamination contains dextrose the liquid in the tube will assume a
red color.

One per cent dextrose yields an immediate color, whereas 0.05 per cent yields
the color only after the lapse of a period of one-half hour from the time the alkali is
added. In urinary examination if the color appears after the thirty-minute interval
the color change is without significance, inasmuch as sugar-free urine will respond
thus. The reaction is given by all aldehydes and therefore the test cannot be safely
employed in testing urines preserved by formaldehyde. Albumin does not interfere
with the test.

6. Bottu's Test. 3— To 8 c.c. of Bottu's reagent^ in a test-tube add i c.c. of the

' This solution is prepared by mixlDg one part by volume, in each case, of glacial acetic
acid, one part of water and two parts of phenylhydrazine (the base).

^ Riegler: Compl. rend. soc. biol., 66, p. 795.

' Bottu: Compt. rend. soc. biol., 66, p. 972.

* This reagent contains 3.5 grams of o-nitrophenylpropiolic acid and 5 c.c. of a freshly
prepared 10 per cent solution of sodium hydroxide per liter.

24

PHYSIOLOGICAL CHEMISTRY

solution under examination and mix the liquids by gentle shaking. Now heat the
upper portion of the mixture to boiling, add an additional i c.c. of the solution and
heat the mixture again immediately. The appearance of a blue color accompanied
by the precipitation of small particles of indigo blue indicates the presence of dex-
trose in the solution under examination. The test will serve to detect the presence
of O.I per cent of dextrose.

7. Precipitation by Alcohol. — To 10 c.c. of 05 per cent alcohol add about 2 c.c.
of dextrose solution. Compare the result with that obtained under Dextrin, 5,
page 48.

8. Iodine Test. — Make the regular iodine test as given under Starch, 5, page 45,
and keep this result in mind for comparison with the results obtained later with
starch and with dextrin.

9. Diffusibility of Glucose. — Test the diffusibility of glucose solution through
animal membrane or parchment paper, making a dialyzer hke one of the models
shown in Fig. 2.

Fig. 2. — DiALYziNG Apparatus for Students' Use.

A most satisfactory dialyzing bag may be made of collodion as follows:
Pour a solution of collodion into a clean dry Erlenmeyer flask or test-tube.
While rotating the vessel on its longitudinal axis, gradually pour out the collodion,
at the same time being careful that the interior surface of the flask is completely
coated with the solution. Continue the rotation in the inverted position until
the collodion ceases to flow. After the solution has evaporated such that the
collodion skin on the rim is dry and stiff, cut or loosen it around the edge of the
rim. With a pipette or wash bottle run in a few cubic centimeters of water be-
tween the membrane and the wall of the flask or test-tube. Shake the incUned
vessel while rotating on its longitudinal axis, thus detaching the membrane.
Now withdraw the detached bag and fill with water, to determine whether or not
it contains defects.'

All monosaccharides and disaccharides are diffusible, but many polysac-
charides are not.

10. Moore's Test. — To 2-3 c.c. of sugar solution in a test-tube add an equal
volume of concentrated KOH or NaOH, and boil. The solution darkens and finally
assumes a brown color. . At this point the odor of caramel may be detected.

This is an exceedingly crude test and is of little practical value. The alkali
brings about condensation and decomposition. The brown color is due to the
formation of condensation products. Among the decomposition products are the
potassium or sodium salts of certain organic acids.

^ Gies: Quoted by Clark. Bioch. Bull., i, 198, 1911.

CARBOHYDRATES 25

II. Reduction Tests. — To their aldehyde or ketone structure many
sugars owe the property of readily reducing alkaline solutions of the
oxides of metals like copper, bismuth and mercury; they also possess
the property of reducing ammoniacal silver solutions with the separa-
tion of metallic silver. Upon this property of reduction the most
widely used tests for sugars are based. When whitish-blue cupric
hydroxide in suspension in an alkaline liquid is heated it is converted
into insoluble black cupric oxide, but if a reducing agent like certain
sugars be present the cupric hydroxide is reduced to insoluble yellow
cuprous hydroxide, which in turn, on further heating, may be converted
into brownish-red or red cuprous oxide. These changes are indicated
as follows:

OH

/
Cu ^Cu = 0+H20.

\ Cupric o-Tide

\ (black).

OH

Cupric hydroxide
(whitish-blue).

Cu

OH

OH

OH

-^ 2Cu-OH-t-H20+0.

Cuprous hydroxide
(yellow).

Cu

OH

Cu

Cu— OH

\

1 -s

0-hHoO

Cu— OH

/

Cu

Cuprous hydroxide
(yellow).

Cuprous oxide
(brownish-red) .

The chemical equations here discussed are exemplified in Trommer's
and Fehling's tests.

(c) Trommer's Test. — To 5 c.c. of sugar solution in a test-tube add one-half it.s
volume of KOH or NaOH. Mix thoroughly and add, drop by drop, a very dilute
solution of copper sulphate. Continue the addition until there is a slight permanent
precipitate of cupric hydroxide and in consequence the solution is slightly turbid.
Heat, and the cupric hydroxide is reduced to yellow cuprous hydroxide or to brown-
ish-red cuprous o.xide.

If the solution of copper sulphate used is too strong a small brownish-red pre-
cipitate produced in a weak sugar solution may be entirely masked. On the other

26 PHYSIOLOGICAL CHEMISTRY

hand, particularly in testing for sugar in the urine, if too little copper sulphate is
used a light-colored precipitate formed by uric acid and purine bases may obscure
the brownish-red precipitate of cuprous oxide. The action of KOH or NaOH in the
presence of an excess of sugar and insufficient copper will produce a brownish color.
Phosphates of the alkaline earths may also be precipitated in the alkaline solution
and be mistaken for cuprous hydroxide. Trommer's test is not very satisfactory.

Salkowski^ has proposed a modification of the Trommer procedure which he
claims is a very accurate sugar test.

(b) Fehling's Test. — To about i c.c. of Fehling's solution^ in a test-tube add
about 4 c.c. of water, and boil.^ [The cupric hydroxide is held in solution by the
sodium potassium tartrate (Rochelle salt).] This is done to determine whether
the solution will of itself cause the formation of a precipitate of brownish-red
cuprous oxide. If such a precipitate forms, the Fehling's solution must not be
used. Add sugar solution to the warm Fehling's solution a few drops at a time
and heat the mixture after each addition. The production of yellow cuprous hy-
droxide or brownish-red cuprous oxide indicates that reduction has taken place.
The yellowish precipitate is more likely to occur if the sugar solution is added
rapidly and in large amount, whereas with a less rapid addition of smaller
amounts of sugar solution the brownish-red precipitate is generally formed.

This is a much more satisfactory test than Trommer's, but even this
test is not entirely reliable when tfsed to detect sugar in the urine. Such
bodies as conjugate glycuronates, uric acid, nucleoprotein and homogen-
tisic acid when present in sufficient amount may produce a result simi-
lar to that produced by sugar. Phosphates of the alkaline earths may
be precipitated by the alkali of the Fehling's solution and in appearance
may be mistaken for cuprous hydroxide. Cupric hydroxide may also
be reduced to cuprous oxide and this in turn be dissolved by creatinine,
a normal urinary constituent. This will give the urine under examina-
tion a greenish tinge and may obscure the sugar reaction even when a
considerable amount of sugar is present. According to Laird, "* even
small amounts of creatinine will retard the reaction velocity of reducing
sugars with Fehling's solution.

In testing urine preserved by chloroform a positive test may be ob-
tained in the absence of sugar. This is due to the fact that the hot
alkali produces formic acid (a reducing fatty acid) from the chloroform.

' Salkowski: Zeit. physiol. Chem., 79, 164, 1912.

2 Fehling's solution is composed of two definite solutions — a copper sulphate solution
and an alkaline tartrate solution — which may be prepared as follows:

Copper sulphate solution = 54.6$ grams of copper sulphate dissolved in water and made
up to 500 c.c.

Alkaline tartrate solution = i2S grams of potassium hydroxide and 173 grams of Rochelle
salt dissolved in water and made up to 500 c.c.

These solutions should be preserved separately in rubber-stoppered bottles and mixed
in equal volumes when needed for use. This is done to prevent deterioration.

* More dilute Fehling's solution should be used in testing very dilute sugar solutions.
In case of concentrated sugar solutions it may sometimes be desirable to use a larger volume
of the Fehling's solution.

'' Laird: Journal of Pathology and Bacteriology, 16, 398, 1912.

CARBOHYDRATES 2 7

Ammonium salts also interfere with Fehling's test. If present in
excess the solution {e.g., urine) should be made alkaline and boiled in
order to decompose the ammonium salts.

If the solution under examination by Fehling's test is acid in re-
action it must be neutralized or made alkaline before applying the test.

(c) Benedict's Modifications of Fehling's Test. — First Modification. — To 2 c.c.
of Benedict's solution' in a test-tube add 6 c.c. of distilled water and 79 drops
(not morej of the solution under examination. Boil the mixture vigorously for
about 15-30 seconds and permit it to cool to room temperature spontaneously.

If sugar is present in the solution a precipitate will form which is
often bluish-green or green at first, especially if the percentage of sugar is
low, and which usually becomes yellowish upon standing. If the sugar
present exceeds 0.06 per cent this precipitate generally forms at or below
the boiling-point, whereas if less than 0.06 per cent of sugar is present the
precipitate forms more slowly and generally only after the solution has
cooled.

Benedict claims, whereas the original Fehling test will not serve
to detect sugar when present in a concentration of less than o.i per
cent, that the above modification will serve to detect sugar when
present in as small quantity as 0.015-0.02 per cent. Corroboration
of this claim of increased delicacy has recently been submitted by
Harrison. -

The modified Fehling solution used in the above test differs from
the original Fehling solution in that 100 grams of sodium carbonate is
substituted for the 125 grams of potassium hydroxide ordinarily used,
thus forming a Fehling solution which is considerably less alkaline
than the original. This alteration in the composition of the Fehling
solution is of advantage in the detection of sugar in the urine inasmuch
as the strong alkalinity of the ordinary Fehling solution has a tendency,
when the reagent is boiled with a urine containing a small amount of
dextrose, to decompose sufficient of the sugar to render the detection of
the remaining portion exceedingly difficult by the usual technic. Bene-
dict claims that for this reason the use of this modified solution permits
the detection of much smaller amounts of sugar than does the use of the
ordinarily Fehling solution.

' Benedict's modified Fehling solution consists of two definite solutions — a copper sul-
phate solution and an alkaline tartrate solution, which may be prepared as follows:

Copper sulphate solution = 24-(>5 grams of copper sulphate dissolved in water and made
up to 500 c.c.

Alkaline tartrate solution = ioo grams of anhydrous sodium carbonate and 173 grams of
Rochelle salt dissolved in water and made up to 500 c.c.

These solutions should be preserved separately in rubber-stoppered bottles and mi.xed
in equal volumes when needed for use. This is done to prevent deterioration.

* Harrison: Fliarm. Jour., 87, 746, 1911.

28 PHYSIOLOGICAL CHEMISTRY

Second Modification. ^ — Benedict has fvirther modified his solution and has
succeeded in obtaining one which does not deteriorate upon long standing. ^
The following is the procedure for the detection of glucose in solution : To 5 c.c.
of the reagent in a test-tube add 8 (not more) drops of the solution under exam-
ination. Boil the mixture vigorously for from one to two minutes and then allow
the fluid to cool spontaneously. In the presence of dextrose the entire body of
the solution will be filled with a precipitate, which may be red, yellow or green in
color, depending upon the amount of sugar present. If no glucose is present, the
solution will remain perfectly clear. (If urine is being tested, it may show a very
faint turbidity, due to precipitated urates.)

Even very small quantities of glucose (o.i per cent) yield precipitates
of surprising bulk with this reagent, and the positive reaction for glucose
is the filling of the entire body of the solution with a precipitate, so that
the solution becomes opaque. Since amount rather than color of the
precipitate is made the basis of this test, it may be applied even for the
detection of small quantities of glucose, as readily in artificial light as in
daylight. Chloroform does not interfere with this test nor do uric acid
or creatinine interfere to such an extent as in the case of Fehling's test.

Mercuric Oxide Reduction Test (Cramer).^ — This test depends on
the reduction of mercuric oxide in a weakly alkaline solution, with the
formation of metallic mercury. The degree of alkalinity is an important
factor, as the test becomes more sensitive but less specific the greater
the alkalinity of the reagent.

For the detection of reducing sugar in aqueous solution proceed as follows :
Introduce 3 c.c. of Cramer's "2.5 reagent" into a test-tube^ and heat to boiling.
The solution remains clear, but turns sUghtly yellow. Add 3 c.c. of the sugar
solution and again heat to boiling. Remove the tube from the flame and note
that the mixture becomes turbid, darkens, and that on standing a precipitate
of finely divided mercury settles to the bottom of the tube.

^ Benedict: Jour. Am. Med. Ass'n, 57, 1193, 1911.

^ Benedict's new solution has the following composition:

Copper sulphate i7-3 grams.

Sodium citrate 1730 grams.

Sodium carbonate (anhydrous) 100. o grams.

Distilled water to make i liter.

With the aid of heat dissolve the sodium citrate and carbonate in about 600 c.c of water.
Pour (through a folded filter paper if necessary) into a glass graduate and make up to 850 c.c.
Dissolve the copper sulphate in about 100 c.c. of water and make up to 150 c.c. Pour the
carbonate-citrate solution into a large beaker or casserole and add the copper sulphate solu-
tion slowly, with constant stirring. The mixed solution is ready for use and does not dete-
riorate upon long standing.

^ Cramer: Bioch. Jour., 9, 156, 1915.

* Cramer's "2.5 Reagent." — 0.4 gram mercuric oxide (red or yellow) and 6 grams potas-
sium iodide are dissolved in 100 c.c. water. This solution is weakly alkaline. The alka-
linity must now be adjusted so that 10 c.c. of the reagent are neutralized by 2.5 c.c. of
N/io acid, using phenolphthalein as indicator. This is done by titrating 10 c.c. of the
reagent with X/io acid and, after the alkalinity of the reagent has thus been determined,
adding the requisite amount of X/io acid or alkali to the bulk of the reagent. The reagent
is a clear colorless solution which turns slightly yellow on heating and becomes colorless
again on cooling. It must rernain clear on boiling.

CARBOHYDRATES 29

This test is positive with such sugars as give other reduction tests,
e.g., glucose, fructose, lactose, maltose, arabinose, etc. If the reducing
sugar be present in aqueous solution a slight reduction may be obtained
with I mg. of glucose. If the reagent be made strongly alkaline, it
ceases to be specific for reducing sugars and chemically allied sub-
stances and is reduced by other organic substances, e.g., creatinine.

It is claimed that this test is free from fallacies inherent in Fehling's
test as the result of the reducing action of uric acid and creatinine.

The test is more sensitive than the Fehling's or Xylander's reac-
tions, and is particularly suitable for the examination of urines in which
the amount of sugar present exceeds the normal amount only slightly.

(e) Bismuth Reduction Test (Boettger). — To 5 c.c. of sugar solution in a test-tube
add I c.c. of KOH or NaOH and a very small amount of bismuth subnitrate, and
boil. The solution will gradually darken and finally assume a black color due to
reduced bismuth. If the test is made on urine containing albumin this must be
removed, by boiling and filtering, before applying the test, since with albumin a
similar change of color is produced (bismuth sulphide).

(f) Bismuth Reduction Test (Nylander). — To 5 c.c. of sugar solution in a test-
tube add one-tenth its volume of Nylander's reagent' and heat for fi.ve minutes
in a boiling water-bath.- The solution will darken if reducing sugar is present,
and upon standing for a few moments a black color wiU appear.

This color is due to the precipitation of bismuth. If the testis made
on urine containing albumin this must be removed, by boiling and
filtering, before applying the test, since with albumin a similar change of
color is produced. Glucose when present to the extent of 0.08 per cent
may be easily detected by this reaction (Rabe^ claims that o.oi per cent
sugar may be so detected). Uric acid and creatinine which interfere
with the Fehling's test do not interfere with the Xylander test. It
is claimed by Bechold that the bismuth reduction tests give a nega-
tive reaction \vith solutions containing sugar when mercuric chloride or
chloroform is present. Other observers^ have failed to verify the
inhibitory action of mercuric chloride and have shown that the in-
hibitory influence of chloroform may be overcome by raising the tem-
perature of the urine to the boiling-point for a period of live minutes
previous to making the test. Urines rich in indican. urochromc, urocry-
thrin or hemato porphyrin, as well as urines excreted after the ingestion of
large amounts of certain medicinal substances, may give a darkening of

^ Nylander's reagent is prepared by digesting 2 grams of bismuth subnitrate and 4 grams
of Rochelle salt in 100 c.c. of a 10 per cent potassium hydroxide solution. The reagent is
then cooled and filtered.

- Hammarsten suggests that the mi.xture should be boiled 2-5 minutes (according to the
sugar content) over a free flame and the tube then permitted to stand 5 minutes before
drawing conclusions.

^Rabe: Apotlt. Ztg., 29, 554, 1Q14.

^ Rehfusp and Hawk: Journal of Biological Chemistry; 7, 267, igio; also Zeidlitz:
U psala Lakarcforen Fork., N. F., ii, 1906.

30 PHYSIOLOGICAL CHEMISTRY

Nylander's reagent similar to that of a true sugar reaction. It is a dis-
puted point whether the urine after the administration of urotropin
will reduce Nylander's reagent.^ Strausz^ has recently shown that the
urine of diabetics to whom "lothion" (diiodohydroxypropane) has
been administered will give a negative Nylander-Almen reaction and
respond positively to the Fehling and polariscopic tests. "lothion"
also interferes with the Nylander-Almen test in vitro whereas KI and
I do not.

According to Rustin and Otto, the addition of PtCU increases the
delicacy of Nylander-Almen reaction. Theyclaim that this procedure
causes the sugar to be converted quantitatively. No quantitative
method has yet been devised, however, based upon this principle.

Bohmansson^ before testing the urine under examination treats
it (lo c.c.) with J-^ volume of 25 per cent hydrochloric acid and about
}4 volume of boneblack. This mixture is shaken one minute, then
filtered and the neutralized filtrate tested by Nylander-Almen reaction.
Bohmansson claims that this procedure removes certain interfering
substances, in particular urochrome.

A positive bismuth reduction test is probably due to the following
reactions:

(a) Bi(OH)2N03 + K0H-^Bi(0H)3 + KNO3.

(b) 2Bi(OH)3— 30->Bi2 + 3H2O.

(g). Barfoed's Test. — Place about 5 c.c. of Barfoed's solution* in a test-tube
and heat to boiling. Add glucose solution slowly, a few drops at a time, heating
after each addition. Reduction is indicated by the formation of a red precipitate
of cuprous oxide. If the precipitate does not form upon continued boiling allow
the tube to stand a few minutes and examine.

According to Welker^ chlorides interfere pronouncedly with the
reaction causing the formation of a green precipitate.

Barfoed's test is not a specific test for glucose as is frequently stated,
but simply serves to detect monosaccharides. Disaccharides will also
respond to the test, under proper conditions of acidity.^ Also if the
sugar solution is boiled sufficiently long, in contact with the reagent, to
hydrolyze the disaccharide through the action of the acetic acid present
in the Barfoed's solution a positive test results.'' Barfoed's is a copper

^Abt: Archives of Pediatrics, 24, 275, 1907; also Weitbrecht: Schiveiz. Wochschr., 47,
577. 1909-

* Strausz: Munch, med. Woch., 59, 85, 191 2.
' Bohmansson: Biochem. Zeit., 19, p. 281.

* Barfoed's solution is prepared as follows: Dissolve 4.5 grams of neutral crystallized
copper acetate in 100 c.c. of water and add 1.2 c.c. of 50 per cent acetic acid. This solu-
tion should be freshly made.

* Welker: Jour. Am. Chem. Soc, 37, 2227, 1915.

* Mathews and McGuigan: Am. Jour. Physiol., 19, 175, 1907.

' Hinkle and Sherman: Jour. Am. Chem. Soc, 29, 1744, 1907.

CARBOHYDRATES 3 1

reduction test, but differs from Fehling's and other reduction tests in
that the reduction is brought about in an acid solution. It is unsuited
for the detection of sugar in urine.

12. Fermentation Test. — "Rub up" in a mortar about 20 c.c. of the sugar solu-
tion with a small piece of compressed yeast. Transfer the mixture to a sacchar-
ometer (shown in Fig. 3) and stand it aside in a warm place for about twelve
hours. If the sugar is fermentable, alcoholic fermentation will occur and carbon
dioxide will collect as a gas in the upper portion of the tube (see Fig. 4;.
On the completion of fermentation introduce a Uttle potassium hydroxide solu-
tion into the graduated portion by means of a bent pipette, place the thumb
tightly over the opening in the apparatus and invert the saccharometer. Re-
membering that KOH has the power to absorb
CO 2 how do you explain the result?'

13. Formation of Caramel. — Gently heat a
small amount of pulverized dextrose in a test-tube.
After the sugar has melted and turned brown, allow
the tube to cool, add water and warm. The color-
ing matter produced is known as caramel.

s^Vk

Fig. 3. — EixHORN Saccharometer.

Fig. 4. — Illustrating Different Stages
IN Fermentation.

14. Demonstration of Optical Activity. — A demonstration of the use of the
polariscope, by the instructor, each student being required to take readings and
compute the "specific rotation."

Use of the Polariscope

For a detailed description of the different forms of polariscopes, the
method of manipulation and the principles involved, the student is
referred to any standard text-book of physics. A brief description fol-
lov^^s: An ordinary ray of light vibrates in every direction. If such a

1 The findings of Neuberg and associates- indicate that the liberation of carbon di-
oxide by yeast is not necessarily a criterion of the presence of sugar. The presence of
an enzyme called carftovy/fl^e has been demonstrated in yeast which has the power of
splitting off C02 from the carboxyl group of amino- and other aliphatic acids.

^ Neuberg and .Associates: Biochcm. Zcitscli., 31, 170; 32, T,2y, 36, (60, 68, 76), 1911.

32

PHYSIOLOGICAL CHEMISTRY

ray is caused to pass through a "polarizing" Nicol prism it is resolved
into tivo rays, one of which \dbrates in every direction as before and a
second ray which vibrates in one plane only. This latter ray is said to
be polarized. Many organic substances (sugar, proteins, etc.) have the
power of twisting or rotating this plane of polarized light, the extent to
which the plane is rotated depending upon the number of molecules
which the polarized light passes. Substances which possess this power
are said to be "optically active." The specific rotation of a substance is
the rotation expressed in degrees which is afforded by i gram of sub-

FiG. 5- — One Form or Laurent Polariscope.

B, ^Microscope for reading the scale; C, a vernier; E, position of the analyzing Nicol prism;
H, polarizing Nicol prism in the tube below this point.

Stance dissolved in i c.c. of water in a tube one decimeter in length.
The specific rotation, (Q:)n, may be calculated by means of the following
formula:

Wz,=

p.i'

in which

J) = sodium light.
a = observed rotation in degrees.
p — grams of substance dissolved in i c.c. of liquid.
/ = length of the tube in decimeters.

If the specific rotation has been determined and it is desired to ascer-
tain the per cent of the substance in solution, this may be obtained by
the use of the following formula,

P =

{a)D I

The value of p multiplied by loo will be the percentage of the sub-
stance in solution.

CARBOHYDRATES 33

SPECIFIC ROTATIONS OF MORE COMMON CARBOHYDRATES i

</-Glucose + 52.5° Sucrose + 66.5'

(i-Fructose — 92.3° Lactose + 52.5°

<f-Galactose +81.5° Maltose +137.0°

£j-Mannose +14.2° Raffinose +104.0"

/-Arabinose +104.5° Dextrin +195.0°

/-Xylose + 19.0° Starch (soluble) +196.0°

Rhamnose + 9.0° Glycogen +197.0°

An instrument by means of which the extent of the rotation may be
determined is called a polariscope or polarimeter. Such an instru-
ment designed especially for the examination of sugar solutions is
termed a saccharimeter or polarizing saccharimeler. The form of polari-
scope in Fig. 5, page 32, consists essentially of along barrel pro\-ided
with a Nicol prism at either end (Fig. 6,). The solution under exami-
nation is contained in a tube which is placed between these two prisms.

Fig. 6. — Diagr.xmmatic Representation of the Course of the Light through the
Laurent Polariscope. (The direction is reversed from that of Fig. 5, p. 32.)

a, Bichromate plate to purify the light; h, the polarizing Nicol prism; c, a thin quartz
plate covering one-half the field and essential in producing a second polarized plane; d,
tube to contain the liquid under examination; e, the analyzing Nicol prism; /and g, ocular
lenses.

At the front end of the instrument is an adjusting eyepiece for focusing
and a large recording disc which registers in degrees and fractions of a
degree. The light is admitted into the far end of the instrument and is
polarized by passing through a Nicol prism. This polarized ray then
traverses the column of liquid within the tube mentioned above and
if the substance is optically active the plane of the polarized ray is
rotated to the right or left. Bodies rotating the ray to the right are
called dextro-rotatory and those rotating it to the left levo-rotalorv.

Within the apparatus is a disc which is so arranged as to be without
lines and uniformly light at zero. Upon placing the optically active
substance in position, however, the plane of polarized light is rotated
or turned and it is necessary to rotate the disc through a certain number
of degree in order to secure the normal conditions, i.e., "without lines

1 The specific rotation varies with the temperature and concentration of the solution.
The figures here given are for concentrations of about 10 per cent and temperatures of about
20°C. Fresh solutions may give markedly different values due to mutarotation, the figures
here given representing the constant values obtained on standing.

3

34

PHYSIOLOGICAL CHEMISTRY

and uniformly light." The difference between this reading and the
zero is a or the observed rotation in degrees.

Polarizing saccharimeters are also constructed by which the per-
centage of sugar in solution is determined by making an observation
and multiplying the value of each division on a horizontal sliding scale
by the value of the division expressed in terms of dextrose. This
factor may vary according to the instrument.

Fig. 7. — PoLAEiscoPE (Schmidt and Hansch Model).

"Optical" raethods embracing the determination of the optical
activity are being utilized in recent years in many "quantitative"
connections.^

CH2OH

FRUCTOSE (CH0H)3

CO

CH20H

' Abderhalden and Schmidt: "Determination of blood content by means of the optical
method," Zeit. physiol. Chem., 66, 120, 1910; also C. Neuberg: "Determination of nucleic
acid cleavage by polarization," Biochemische Zeiischrift, 30, 505, 191 1.

CARBOHYDRATES 35

As already stated, fructose, sometimes called levulose or fruit sugar,
occurs widely disseminated throughout the plant kingdom in company
with glucose. Its reducing power is somewhat weaker than that of
dextrose. Fructose does not ordinarily occur in the urine in diabetes
mellitus, but has been found in exceptional cases. With phenylhydra-
zine it forms the same osazone as glucose. With methylphenyUiy-
drazine, levulose forms a characteristic methylphenylfructosazone.

(For a further discussion of fructose see the section on Hexoses,
page 20.)

Experiments on Fructose

1-6. Repeat Solubility, Fehling's, Phenylhydrazine, Barfoed's, Nylander's,
and Fermentation tests as given under Glucose, pages 21-31.

7. Resorcinol-Hydrochloric Acid Reaction (Seliwanoff). — To 5 c.c. of Seli-
wanoff's reagent^ in a test-tube add a few drops of a fructose solution and heat the
mixture to boiling. A positive reaction is indicated by the production of a red
color and the separation of a brown-red precipitate. The latter may be dissolved
in alcohol to which it will impart a striking red color.

If the boiling be prolonged a similar reaction may be obtained with
solutions of glucose or maltose. This has been explained- in the case
of glucose as due to the transformation of the glucose into fructose
by the catalytic action of the hydrochloric acid. The precautions neces-
sary for a positive test for levulose are as follows: The concentration
of the hydrochloric acid must not be more than 12 per cent. The reac-
tion (red color) and the precipitate must be observed after not more
than 20-30 seconds boiling. Glucose must not be present in amounts
exceeding 2 per cent. The precipitate must be soluble in alcohol with
a bright red color.

8. Borchardt's Reaction. — To about 5 c.c. of a solution of fructose in a test-
tube add an equal volume of 25 per cent hydrochloric acid and a few crystals of
resorcinol. Heat to boiling and after the production of a red color, cool the tube
under running water and transfer to an evaporating dish or beaker. Make the
mixture slightly alkaline with solid potassium hydroxide, return it to a test-tube,
add 2-3 c.c. .of acetic ether and shake the tube vigorously. In the presence of
levulose, the acetic ether is colored yellow. (For further discussion of the test see
Chapter XXIII.)

9. Formation of Methylphenylfructosazone. — To a solution of i.S grams of
levulose in 10 c.c. of water add 4 grams' of methylphenylhydrazine and enough
alcohol to clarify the solution. Introduce 4 c.c. of 50 per cent acetic acid and heat
the mixture for 5-10 minutes on a boiling water-bath.* On standing 15 minutes

^ Seliwanoff's reagent may be prepared by dissolving 0.05 gram of resorcinol in 100 c.c.
of dilute (1:2) hydrochloric acid.

* Koenigsfeld: Bioch. Zcil., 38, 311, 1912.
' 3.66 grams if absolutely pure.

* Longer heating is to be avoided.

36 PHYSIOLOGICAL CHEMISTRY

at room temperature, crystallization begins and is complete in two hours. By
scratching the sides of the flask or by inoculation, the solution quickly congeals to
form a thick paste of reddish-yellow silky needles. These are the crystals of methyl-
phenyljructosazone. They may be recrystallized from hot 95 per cent alcohol and
melt at i53°C.

CHoOH

GALACTOSE, (CH0H)4

!

CHO

Galactose occurs with glucose as one of the products of the hydro-
lysis of lactose. It is dextro-rotatory, forms an osazone with phenyl-
hydrazine and ferments slowly with yeast. Upon oxidation with nitric
acid galactose yields mucic acid, thus differentiating this monosac-
charide from glucose and fructose. Lactose also yields mucic acid
under these conditions. The mucic acid test may be used in urine
examination to differentiate lactose and galactose from other reducing
sugars.

Experiments on Galactose

1 . Phloroglucinol-Hydrochloric Acid Reaction (Tollens) . — To equal volumes of
galactose solution and hydrochloric acid (sp. gr. 1.09) add a little phloroglucinol,
and heat the mixture on a boiling water-bath. Galactose, pentose and glycuronic
acid will be indicated by the appearance of a red color. Galactose may be
differentiated from the two latter substances in that its solutions exhibit no
absorption bands upon spectroscopical examination.

2. Mucic Acid Test. — Treat 100 c.c. of the solution containing galactose with
20 c.c. of concentrated nitric acid (sp. gr. 1.4) and evaporate the mixture in a broad,
shallow glass vessel on a boiUng water-bath until the volume of the mixture has
been reduced to about 20 c.c. At this point the fluid should be clear, and a fine
white precipitate of mucic acid should form.

If the percentage of galactose present is low it may be necessary to
cool the solution and permit it to stand for some time before the
precipitate will form. It is impossible to differentiate between galactose
and lactose by this test, but the reaction serves to differentiate these
two sugars from all other reducing sugars. Differentiate lactose from
galactose by means of Barfoed's test (page 30).

3. Phenylhydrazine Reaction. — Make the test according to directions given
under Glucose, 3 or 4, pages 22 and 23.

Pentoses, CsHioOs

In plants, and more particularly in certain gums, very complex car-
bohydrates, called pentosans (see page 50), occur. These pentosans

CARBOHYDRATES 37

through hydrolysis by acids may be transformed into pentoses. Pento-
ses do not ordinarily occur in the animal organism, but have been found
in the urine of morphine habitues and others, their occurrence some-
times being a persistent condition without known cause. They may be
obtained from the hydrolysis of nucleoproteins being present in the
nucleic acid complex of the molecule. Pentoses are non-fermentable,
have strong reducing power and form osazones with phenylhydrazine.
Pentoses are an important constituent of the dietary of herbivorous
animals. Glycogen is said to be formed after the ingestion of these
sugars containing five oxygen atoms. This, however, has not been
conclusively proven. On distillation with strong hydrochloric acid
pentoses and pentosans yield furfurol, which can be detected by its
characteristic red reaction with aniline-acetate paper.

CHoOH

ARABINOSE, rCH0H)3

I

CHO

Arabinose is one of the most important of the pentoses. The
^arabinose may be obtained from gum arable, plum or cherry gum by
boiling for 10 minutes with concentrated hydrochloric acid. This
pentose is dextro-rotatory, forms an osazone and has reducing power,
but does not ferment. The i-arabinose has been isolated from the
urine and yields an osazone which melts at i66°-i68°C.

Experiments on Arabinose

I. Orcinol-Hydrochloric Acid Reaction (Bial).' — To 5 c.c. of Bial's reagent- in
a test-tube add 2-3 c.c. of the arabinose solution and heat the mixture gently until
the first bubbles rise to the surface. Immediately or upon cooUng the solution
becomes green and a fiocculent precipitate of the same color may form. (For
further discussion see Chapter XXIII.) The test may also be performed by
adding the pentose to the hot reagent.

It is claimed that this test is more delicate than the original orcinol
test (see 3) and more accurate, since menthol, kreosotal, etc., respond
to the original orcinol test but not to Bial's. Sachs^ has offered
suggestions as to modification of the test in order to avoid confusion
with glycuronic acid.

iBial: Dent. mcd. Woch., 28, 252, 1902, and Bcrl. kliii. U'lnli., No. 18, 1903.
- Orcinol 1.5 gram.

Fuming HCl 500 grams.

Ferric chloride (10 per cent) 20-30 drops.
^ Sachs: Block. Zc'U., i, 383, 1906, and 2, 245, 1906.

38 PHYSIOLOGICAL CHEMISTRY

2. Phloroglucinol-Hydrochloric Acid Reaction (Tollens). — To equal volumes of
arabinose solution and hydrochloric acid (sp. gr. 1.09) add a little phloroglucinol
and heat the mixture on a boiling water-bath. Galactose, pentose or glycuronic
acid will be indicated by the appearance of a red color. To differentiate between
these bodies make a spectroscopic examination and look for the absorption band
between D and E given by pentoses and glycuronic acid. Differentiate between
the two latter bodies by the melting-points of their osazones.

Compare the reaction with that obtained with galactose (page 36).

3. Orcinol Test. — Repeat 2, using orcinol instead of phloroglucinol. A suc-
cession of colors from red through reddish blue to green is produced. A green pre-
cipitate is formed which is soluble in amyl alcohol and has absorption bands be-
tween C and D.

4. Phenylhydrazine Reaction. — Make this test on the arabinose solution
according to directions given under Glucose, 3 or 4, pages 22 and 23.

CH2OH
XYLOSE, (CH0H)3

CHO

Xylose, or wood sugar, is obtained by boiling wood gums with dilute
acids as explained under Arabinose, page 37. It is dextro-rotatory,
forms an osazone and has reducing power, but does not ferment.

Experiments on Xylose
1-4. Same as for arabinose (see above).

RHAMNOSE, C6H12O5

Rhamnose or methyl-pentose is an example of a true carbohydrate
which does not have the H and 0 atoms present in the proportion to
form water. Its formula is C6H12O5. It has been found that rham-
nose when ingested by rabbits or hens has a positive influence upon the
formation of glycogen in those organisms.

DISACCHAKCDES, C12H22O11

The disaccharides as a class may be divided into two rather dis-
tinct groups. The first group would include those disaccharides which
are found in nature as such, e.g., sucrose and lactose, and the second
group would include those disaccharides formed in the hydrolysis of
more complex carbohydrates, e.g., maltose and iso-maltose.

The disaccharides have the general formula C12H22O11, to which,
in the process of hydrolysis, a molecule of water is added causing the

CARBOHYDRATES 39

single disaccharide molecule to split into two monosaccharide (hexose)
molecules. The products of the hydrolysis of the more common di-
saccharides are as follows:

Maltose = glucose+glucose.
Lactose = glucose+galactose.
Sucrose = glucose+f ructose.

All of the more common disaccharides except sucrose have the power
of reducing certain metallic oxides in alkaline solution, notably those
of copper and bismuth. This reducing power is due to the presence
of the aldehyde group (^ — CHO) in the sugar molecule.

MALTOSE, Ci2H220n

Maltose or malt sugar is formed in the hydrolysis of starch through
the action of an enzyme, vegetable amylase {diastase), contained in sprout-
ing barley or malt. Certain enzymes in the saliva and in the pancreatic
juice may also cause a similar hydrolysis. Maltose is also an intermedi-
ate product of the action of dilute mineral acids upon starch. It is
strongly dextro-rotatory, reduces metallic oxides in alkaline solution
and is fermentable by yeast after being inverted (see Polysaccharides,
page 43) by the enzyme maltase of the yeast. In common wdth the other
disaccharides, maltose may be hydrolyzed with the formation of two
molecules of monosaccharide. In this instance the products are two
molecules of glucose. With phenylhydrazine maltose forms an osa-
zone, maltosazone. The following formula represents the probable
structure of maltose:

CH2OH CHO

CHOH CHOH

I !

CHO CHOH

I I

CHOH CHOH

CHOH CHOH

I , I

C C CHo

\

H

Maltose.

Experiments on Maltose

1-6. Repeat Solubility, Fehling's, Nylander's, Phenylhydrazine, Barfoed's
and Fermentation tests as given under Glucose, pages 21-31.

40 PHYSIOLOGICAL CHEMISTRY

ISO-MALTOSE, C12H22O11

Iso-maltose, an isomeric form of maltose, is formed, along with mal-
tose by the action of diastase upon starch paste, and also by the action
of hydrochloric acid upon glucose. It also occurs with maltose as one
of the products of salivary digestion. It is dextro-rotatory and with
phenylhydrazine gives an osazone which is characteristic. Iso-maltose
is very soluble and reduces the oxides of bismuth and copper in alkaline
solution. Pure iso-maltose is probably only slightly fermentable.

LACTOSE, C12H22O11

Lactose or milk sugar occurs ordinarily only in milk, but has often
been found in the urine of women during pregnancy and lactation. It
may also occur in the urine of normal persons after the ingestion of
unusually large amounts of lactose in the food. It has a strong reducing
power, is dextro-rotatory and forms an osazone with phenylhydrazine.
Upon hydrolysis lactose yields one molecule of glucose and one molecule
of galactose.

In the souring of milk the bacterium lactis and certain other micro-
organisms bring about lactic acid fermentation by transforming the lac-
tose of the milk into lactic acid,

H OH
H— C— C— COOH,

H H

and alcohol. This same reaction may occur in the alimentary canal as
the result of the action of putrefactive bacteria. In the preparation
of kephyr and koumyss the lactose of the milk undergoes alcoholic
fermentation, through the action of ferments other than yeast, and at
the same time lactic acid is produced. Lactose and galactose yield
mucic acid on oxidation with nitric acid. This fact is made use of in
urine analysis to facihtate the differentiation of these sugars from other
reducing sugars.

Lactose is not fermentable by pure yeast.

Experiments on Lactose

1-6. Repeat Solubility, Fehling's, Phenylhydrazine, Barfoed's, Nylander's
and Fermentation tests as given under Glucose, pages 21-31.

7. Mucic Acid Test. — Treat 100 c.c. of the solution containing lactose with
20 c.c. of concentrated nitric acid (sp. gr. 1.4) and evaporate the mixture in a
broad, shallow glass vessel on a boiUng water-bath, until the volume of the mix-
ture has been reduced to about 20 c.c. At this point the fluid should be clear,
and a fine white precipitate of mucic acid should form.

CARBOHYDRATES 4 1

If the percentage of lactose present is low it may be necessary to
cool the solution and permit it to stand for some time before the
precipitate will appear. It is impossible to differentiate between lactose
and galactose by this test, but the reaction serves to differentiate these
two sugars from all other reducing sugars.

Differentiate lactose from galactose by means of Barfoed's test,
page 30.

SUCROSE, C12H22O11

Sucrose, also called saccharose or cane sugar, is one of the most
important of the sugars and occurs very extensively distributed in
plants, particularly in the sugar cane, sugar beet, sugar millet and in
certain palms and maples.

Sucrose is dextro-rotatory and upon hydrolysis, as before mentioned,
the molecule of sucrose takes on a molecule of water and breaks down
into two molecules of monosaccharide. The monosaccharides formed in
this instance are glucose and fructose. This is the reaction:

C12H22O11-I-H2O — >C6Hi206-l-C6Hi206.

Sucrose Glucose Fructose

This process is called inversion and may be produced by bacteria, en-
zymes, and certain weak acids. After this inversion the previously
strongly dextro-rotatory solution becomes levo-rotatory. This is due
to the fact that the fructose molecule is more strongly levo-rotatory
than the glucose molecule is dextro-rotatory. The product of this
inversion is called iiivert sugar.

Sucrose does not reduce metalHc oxides in alkahne solution and forms
no osazone with phenylhydrazine. It is not fermentable directly by
yeast, but must first be inverted by the enzyme sucrose {invertase or
invertin) contained in the yeast. The probable structure of sucrose
may be represented by the following formula. Note the absence of
any free ketone or aldehyde group.

CH2OH CH2OH

I I

CHOH CHO

CHO CHOH

CHOH CHOH

I I

CHOH C

C ' O CH2OH

\
\

H

Sucrose.

42

PHYSIOLOGICAL CHEMISTRY

Experiments on Sucrose

1-6. Repeat Solubility, Fehling's, Nylander's, Barfoed's, Phenylhydrazine
and Fermentation tests according to the directions given under Glucose, pages
21-31.

7. Inversion of Sucrose. — To 25 c.c. of sucrose solution in a beaker add 5
drops of concentrated H2SO4 and boil one minute- Cool the solution and render
neutral with saturated barium hydroxide. Filter off the precipitate of baiiimi
sulphate and upon the resulting fluid repeat the phenylhydrazine, Fehling,
Nylander's and Barfoed's reactions as given under Glucose, pp. 26, 29 and 30 ;
the Resorcinol-Hydrochloric Acid Reaction (Seliwanoff), as given under Fruc-
tose, page 35. Explain the results.

8. Alcoholic Fermentation. — Prepare 500 c.c. of a concentrated (10-20 per
cent) solution of sucrose, add a small amount of egg albumin or commercial

peptone and introduce the mixture into a liter flask.
Add yeast, and by means of a bent tube connect this
flask with a second flask containing a solution of
barium hydroxide protected from the air by a soda-
lime tube in the stopper. Place the flasks in a
warm place and note the passage of gas bubbles
into the barium hydroxide solution. As these gas
bubbles (CO 2) enter, a white precipitate of barium
carbonate will form. The sucrase has been changed
to glucose and fructose and these sugars have been
fermented according to the following equation :

Fig. 8.-I0DOFORM. {Aulenrieth.) C6Hi20^^2C2H60H+C02

When the activity of yeast has practically ceased, connect the fermentation
flask with a condenser and distil the mixture. Catch the first portion of the dis-
tillate separately and test for alcohol by one of the following reactions :

(a) Iodoform Test. — Render 2-3 c.c. of the distillate alkaline wtih potassivun
hydroxide solution and add a few drops of iodine solution. Heat gently and note
the formation of iodoform crystals. Examine these crystals under the microscope
and compare them with those in Fig. 8.

(b) Aldehyde Test. — Place 5 c.c. of the distillate in a test-tube, add a few
drops of potassium dichromate solution, K2Cr207, and render it acid with dilute
sulphuric acid. Boil the acid solution and note the odor of aldehyde changing
to that of acetic acid.

TRISACCHARIDES, C18H32O16

RAFFINOSE

This trisaccharide, also called meKtose, or melitriose occurs in cotton
seed, Australian manna, and in the molasses from the preparation of
beet sugar. It is dextro-rotatory, does not reduce Fehling's solution,
and is only partly fermentable by yeast.

Raflfinose may be hydrolyzed by weak acids the same as the poly-

CARBOHYDRATES . 43

saccharides are hydrolyzed, the products being fructose and mehbiose;
further hydrolysis of the mehbiose yields glucose and galactose.

POLYSACCHARIDES, (CeHioOg),

In general the polysaccharides are amorphous bodies, a few, how-
ever, are crystallizable. Through the action of certain enzjnnes or
weak acids the polysaccharides may be hydrolyzed with the formation
of monosaccharides. As a class the polysaccharides are quite insoluble
and are non-fermentable until inverted. By inversion is meant the
hydrolysis of disaccharide or polysaccharide sugars to form monosacchar-
ides, as indicated in the following equations:

(a) Ci2H220ii + H20-^2(G6Hi206).

(b) CeHioOs+H.O-^CeHisOe.

STARCH, (CeHioOis)^

Starch is widely distributed throughout the vegetable kingdom,
occuriing in grains, fruits, and tubers. It occurs in granular form, the
microscopical appearance being t}^ical for each individual starch.
The granules, which differ in size according to the source, are composed
of alternating concentric rings of granulose and cellulose. Ordinary
starch is insoluble in cold water, but if boiled with water the cell walls
are ruptured and starch paste results. In general starch gives a blue
color with iodine.

Starch is acted upon by amylases, e.g., salivary amylase (ptyalin)
and pancreatic amylase (amylopsin), with the formation of soluble
starch, erythro-dextrin, achroo-dextrins and maltose (see Salivary Diges-
tion, page 56). Maltose is the principal end-product of this enzyme
action. Upon boiling a starch solution with a dilute mineral acid a
series of similar bodies is formed, but under these conditions glucose
is the principal end-product.

Soluble starch may be prepared by the action of dilute hydro-
chloric acid on ordinary starch for several weeks, or at higher tem-
peratures for a shorter period. By precipitation with alcohol this may
be obtained in a dry form readily soluble in cold water.^

Experiments on Starch

I. Preparation of Potato Starch. — ^Pare a raw potato, comminute it upon a fine
grater, mix with water, and "whip up" the pulped material vigorously before
straining it through cheese cloth or gauze to remove the coarse particles. The

^ Fernbach: Proceedings St/i Int. Cong. Appl. Chcin., 13, 131, 1912.
Chapin: Jour. Ind. and Eng. Chem., 6, 649, 1914.

44

PHYSIOLOGICAL CHEMISTRY

Fig. 9. — Potato.

Fig. 10. — Bean. Fig. ii. — Arrowroot.

Fig. 12. — Rye.

Fig. 13. — Barley.

Fig. 14. — Oat.

Fig. 15. — Buckwheat. Fig. 16.^ — ^Maize.

Fig. 17. — Rice.

Fig. 18.— Pea.

Fig. 19. — Wheat.

Starch Granules from Various Sources. {Lcffmann and Beam.)

CARBOHYDRATES 45

starch rapidly settles to the bottom and can be washed by repeated decantation.
Allow the compact mass of starch to drain thoroughly and spread it out on a watch
glass to dry in the air. If so desired this preparation may be used in the experi-
ments which follow.

2. Microscopical Examination. Examine microscopically the granules of the
various starches submitted and compare them with those shown in Figs. 9-19,
page 44. The suspension of the granules in a drop of water will faciUtate the
microscopical examination.

3. Solubility. — Try the solubiUty of one form of starch in each of the ordinary
solvents (see page 21). If uncertain regarding the solubility in any reagent,
filter and test the filtrate with iodine solution as given under 5 below. The pro-
duction of a blue color would indicate that the starch had been dissolved by the
solvent. J

4. Iodine Test. — Place a few granules of starch in one of the depressions of a
porcelain test-tablet and treat with a drop of a dilute solution of iodine in potas-
sium iodide. The granules are colored blue due to the formation of so-called
iodide of starch. The cellulose of the granule is not stained as may be seen by
examining microscopically.

5. Iodine Test on Starch Paste. ^ — Repeat the iodine test using the starch
paste. Place 2-3 c.c. of starch paste- in a test-tube, add a drop of the dilute
iodine solution and observe the production of a blue color. Heat the tube and
note the disappearance of the color. It reappears on cooling.

In similar tests note the influence of alcohol and of alkali upon the so-called
iodide of starch.

The composition of the iodide of starch is not definitely known. In per-
forming this test the solution must always be neutral or acid in reaction.

6. Fehling's Test. — On starch paste (see page 26).

7. Hydrolysis of Starch. — Place about 25 c.c. of starch paste in a small
beaker, add 10 drops of concentrated HCl, and boil. By means of a small pipette,
at the end of each minute', remove a drop of the solution to the test-tablet and
make the regular iodine test. As the testing proceeds the blue color should
gradually fade and finally disappear. At this point, after cooUng and neutraUz-
ing with soUd KOH, FehUng's test (see page 26) should give a positive result
due to the formation of a reducing sugar from the starch. Make the phenyl-
hydrazine test upon some of the hydrolyzed starch. What sugar has been
formed?

8. Influence of Tannic Acid. — Add an excess of tannic acid solution to a small
amount of starch paste in a test-tube. The liquid will become strongly opaque
and ordinarily a yellowish-white precipitate is produced. Compare this result with
the result of the similar experiment on dextrin (page 48).

9. Diffusibility of Starch Paste. — -Test the diffusibility of starch paste through
animal memljrane, parchment paper or collodion, making a dialyzer like one of the
models shown in Fig. 2, page 24.

^ Preparation of Starch Paste. — Grind 2 grams of starch powder in a mortar with a small
amount of cold water. Bring 200 c.c. of water to the boiling-point and add the starch m\x-
ture from the mortar with continuous stirring. Bring again to the boiling-point and allow
it to cool. This makes an approximate i per cent starch paste which is a very satisfactory
strength for general use.

- For this particular test a starch paste of very satisfactory strength may be made by
mixing i c.c. of a i per cent starch paste with 100 c.c. of water.

46 PHYSIOLOGICAL CHEMISTRY

INULm, (C6Hio05)x

Inulin is a polysaccharide which may be obtained as a white, odor-
less, tasteless powder from the tubers of the artichoke, elecampane, or
dahlia. It has also been prepared from the roots of chicory, dandelion,
and burdock. It is very slightly soluble in cold water and quite easily
soluble in hot water. In cold alcohol of 60 per cent or over it is prac-
tically insoluble. Inulin gives a negative reaction with iodine solution.
The "yellow" color reaction with iodine mentioned in many books is
doubtless merely the normal color of the iodine solution. It is very
difl&cult to prepare inulin which does not reduce Fehling's solution
slightly. This reducing power may be due to an impurity. Prac-
tically all commercial preparations of inulin possess considerable
reducing power.

Inulin is levo-rotatory and upon hydrolysis by acids or by the
enzyme inulase it yields the monosaccharide fructose which readily
reduces Fehling's solution. The ordinary amylolytic enzymes occur-
ring in the animal body do not digest inulin. A small part of the
ingested inulin may be hydrolyzed by the acid gastric juice, but Lewis^
has recently shown that "the value of inulin as a significant source of
energy in human dietaries must be questioned."

Experiments on Inulin

1. Solubility. — Try the solubility of inulin powder in hot and cold water and
alcohol. If uncertain regarding the solubiUty in any reagent, filter and neutralize
the filtrate if it is alkaline in reaction. Add a drop of concentrated hydrochloric
acid to the filtrate and boil it for one minute. Render the solution neutral or
slightly alkaline with solid potassium hydroxide and try Fehling's test. What
is the significance of a positive Fehling's test in this connection?

2. Iodine Test. — (a) Place 2-3 c.c. of the inuHn solution in a test-tube and
add a drop of dilute iodine solution. What do you observe ?

(b) Place a small amount of inulin powder in one of the depressions of a test-
tablet and add a drop of dilute iodine solution. Is the effect any different from
that observed above?

3. MoUsch's Reaction. — Repeat this test according to directions given under
Glucose, 2, page 21.

4. Fehhng's Test, — Make this test on the inuUn solution according to the
instructions given under Glucose, page 26. Is there any reduction? ^

5. Hydrolysis of Inulin. — Place 5 c.c. of inulin solution in a test-tube, add a
drop of concentrated hydrochloric acid and boil it for one minute. Now cool
the solution, neutralize it with concentrated KOH and test the reducing action
of I c.c. of the solution upon i c.c. of diluted (1:4) Fehhng's solution. Also

^ Lewis: Journal American Medical Ass'n., 58, 1176, 1912.
^ See the discussion of the properties of inulin, above.

CARBOHYDRATES 47

try the Resorcinol-Hydrochloric Acid reaction as given on p. 35. Explain the
result.'

GLYCOGEN, (CeHioO^)^

(For discussion and experiments see Muscular Tissue, Chapter XIX.)

LICHENIN, (CeHioOs)

Lichenin may be obtained from Cetraria islandica (Iceland moss).
It forms a difficultly soluble jelly in cold water and an opalescent solu-
tion in hot water. It is optically inactive and gives no color with
iodine. Upon hydrolysis with dilute mineral acids lichenin yields dex-
trins and glucose. It is said to be most nearly related chemically to
starch. Saliva, pancreatic juice, malt diastase and gastric juice have
no noticeable action on lichenin.

DEXTRIN, (CeHioOs)^

The dextrins are the bodies formed midway in the stages of the
hydrolysis of starch by weak acids or an enzyme. They are amorphous
bodies which are easily soluble in water, acids, and alkalis, but are in-
soluble in alcohol or ether. Dextrins are dextro-rotatory and are not
fermentable by yeast.

The dextrins may be hydrolyzed by dilute acids to form glucose
and by amylases to form maltose. With iodine one form of dextrin
(erythro-dextrin) gives a red color. Their power to reduce Fehling's
solution is questioned. The lower members of the dextrin series prob-
ably reduce.

Experiments on Dextrin

1. SolubiHty. — Test the solubiUty of pulverized dextrin in hot and cold water.
Dextrin forms a clear solution in hot water, distinguishing it from glycogen which
gives an opalescent solution.

2. Iodine Test. — Place a drop of dextrin solution in one of the depressions
of the test-tablet and add a dilute solution of iodine in potassiimi iodide. A red
color results due to the formation of the red iodide of dextrin. Ordinary dextrin
preparations contain some starch and in the presence of starch it is necessary to
have an excess of iodine present. If the reaction is not sufficiently pronounced
make a stronger solution from pulverized dextrin and repeat the test. The
solution should be slightly acid to secure the best results.

Make proper tests to show that the red iodide of dextrin is influenced by

^ If the inulin solution gave a positive Fehling test in the last experiment it will be neces-
sary to check the hydrolysis experiment as follows: To 5 c.c. of the inulin solution in a test-
tube add one drop of concentrated hj'drochloric acid, neutralize with concentrated KOH
solution and test the reducing action of i c.c. of the resulting solution upon i c.c. of diluted
(i :4) Fehling's solution. This will show the normal reducing power of the inulin solution.
In case the inulin was hydrolyzed, the Fehling's test in the hydrolysis experiment should
show a more pronounced reduction than that observed in the check experiment.

48 PHYSIOLOGICAL CHEMISTRY

heat, alkali, and alcohol in a similar manner to the blue iodide of starch (see
page 45).

The color in the case of dextrin does not reappear as readily on cooling as
in the case of starch.

3. Fehhng's Test. — See if the dextrin solution will reduce Fehling's solution.

4. Hydrolysis of Dextrin. — Take 25 c.c. of dextrin solution in a small beaker,
add 5 drops of dilute hydrochloric acid, and boil. By means of a small pipette,
at the end of each minute, remove a drop of the solution to one of the depressions
of the test-tablet and make the iodine test. The power of the solution to produce
a color with iodine should rapidly disappear. When a negative reaction is ob-
tained cool the solution and neutraUze it with concentrated potassium hydroxide.
Try Fehhng's test (see page 26). This reaction is now strongly positive, due to
the formation of a reducing sugar. Determine the nature of the sugar by means
of the phenylhydrazine test (see pages 22 and 23).

5. Precipitation by Alcohol. — To about 50 c.c. of 95 per cent alcohol in a small
beaker add about 10 c.c. of a concentrated dextrin solution. Dextrin is thrown
out of solution as a gummy white precipitate. Compare the result with that
obtained under Glucose, 7, page 24.

6. Influence of Tannic Acid. — Add an excess of tannic acid solution to a
small amount of dextrin solution in a test-tube. No precipitate forms. This
result differs from the result of the similar experiment upon starch (see Starch, 8,

page 45)-

7. Diflfusibility of Dextrin. — (See Starch, 9, page 45.)

CELLULOSE, (CsHioOs)^

This complex polysarcharide forms a large portion of the cell wall
of plants. It is extremely insoluble and its molecule is much more com-
plex than the starch molecule. The best quality of filter paper and
the ordinary absorbent cotton are good types of cellulose.

At one time there was but a single known solvent for cellulose.
Recent investigation has, however, revealed a long list of cellulose
solvents. (See Experiment 7.)

Cellulose is not hydrolyzed by boiling with dilute mineral acids. It
may be hydrolyzed, however, by treating with concentrated sulphuric
acid then subsequently diluting the solution with water and boiling.
The product of this hydrolysis is glucose.

There is some difference of opinion as to the exact extent to which
cellulose is utilized in the animal organism. It is no doubt, more effi-
ciently utilized by herbivora than by carnivora or by man. It is claimed
that about 25 per cent may be utilized by herbivora, less than 5 per cent
by dogs whereas the quantity utilized by man is " too small for it to play
a role of importance in the diet of a normal individual."^ In neither
man nor the lower animals has there been demonstrated any formation

' Swartz: Transactions of the Connecticut Academy of Arts and Sciences, 16, 247, 1911.

CARBOHYDRATES 49

of sugar or glycogen from cellulose.^ It is probable that the cellulose
which disappears from the intestine is transformed for the most part into
fatty acids. -

Experiments on Cellulose

1 . Solubility. — Test the solubility of cellulose in water, dilute and concentrated
acid and alkali.

2. Iodine Test. — ^Add a drop of dilute iodine solution to a few shreds of cotton
on a test-tablet. Cellulose differs from starch and dextrin in giving no color
with iodine.

3. Formation of Amyloid.'' — Add 10 c.c. of dilute and 5 c.c. of concentrated
H2SO4 to some absorbent cotton in a test-tube. When entirely dissolved fwith-
out heating I pour one-half of the solution into another test-tube, cool it and dilute
with water. Amyloid forms as a gxmimy precipitate and gives a brown or blue
coloration with iodine.

After allowing the second portion of the acid solution of cotton to stand about
10 minutes, dilute it with water in a small beaker and boil for 15-30 minutes.
Now cool, neutraUze with soUd KOH and test with Fehhng's solution. Glucose
has been formed from the cellulose by the action of the acid.

4. Ammoniacal Cupric Hydroxide SolubiHty Test (Schweitzer). — Place a
little absorbent cotton in a test-tube, add Schweitzer's reagent,^ and stir the
cellulose with a glass rod. When completely dissolved acidify the solution with
acetic acid. An amorphous precipitate of cellulose is produced.

5. Hydrochloric Acid — Zinc Chloride SolubiUty Test (Cross and Bevan).^ —
Place a Uttle absorbent cotton in a test-tube, add Cross and Sevan's reagent,^
and stir the cellulose with a glass rod. When solution is complete reprecipitate
the cellulose with 95 per cent alcohol.

6. Iodine-Zinc Chloride Reaction. — Place a little absorbent cotton or quantita-
tive filter paper in a test-tube and treat it with the iodine-zinc chloride reagent."
A blue color forms on standing. Amyloid has been formed from the cellulose
through the action of the ZnClo and the iodine solution has stained the amyloid
blue.

7. Other Cellulose Solvents. — It has recently been demonstrated by Deming'
that there are many excellent solvents for cellulose (filter paper). For example,
the concentrated aqueous solutions of certain salts such as antimony trichloride,

'Lusk: American Journal of Physiology, 27, 467, 1911; also Hoffmann, Inaugural dis-
sertation, Halle-Wittenberg, 19 10.

- Tappeiner: Zeitschrijt fiir Biologic, 24, 105, 1888.

^ This body derives its name from amylum (starch) and is not to be confounded with
amyloid, the glycoprotein.

* Schweitzer's reagent is made by adding potassium hydroxide to a solution of , copper
sulphate which contains some ammonium chloride. A precipitate of cupric hydroxide
forms and this is filtered off, washed, and 3 grams of the moist cupric hydroxide brought
into solution in a liter of 20 per cent ammonium hydroxide.

^ Cross and Bevan: Chemical Xcus, 63, p. 06.

* Cross and Bevan's reagent may be prepared by combining two parts of concentrated
hydrochloric acid and one part of zinc chloride, by weight.

' The iodine-zinc chloride reagent as suggested by Xowopokrowsky (Beihefte Botan.
Ccnlr., 28, 90, 191 2) may be made b)' dissolving 20 grams ZnCl; in 8.5 c.c. water and when
cool introducing the iodine solution (3 grams KI + i-S gram I in Oo c.c. water) drop by drop
until iodine begins to precipitate.

8 Deming: Journal American Chemical Society, 33, 1515, 191 1.

50 PHYSIOLOGICAL CHEMISTRY

stannous chloride and zinc bromide. In hydrochloric acid solution the solvent action
of the above salts is increased. The following salts are also good solvents in hydro-
chloric acid solution: mercuric chloride, bismuth chloride, antimony pentachloride,
tin tetrachloride and titanium tetrachloride. In the case of the last-mentioned salt
the swollen, transparent character of the cellulose fibers preliminary to solution
can be seen very nicely.

Try selected solvents suggested by the instructor.

HEMICELLULOSES

The hemicelluloses differ from cellulose in that they may be hydro-
lyzed upon boiling with dilute mineral acids. They differ from other
polysaccharides in not being readily digested by amylases. Hemi-
cellulose may yield pentosans, or hexosans upon hydrolysis.

Pentosans. — Pentosans yield pentoses upon hydrolysis. So far as is
known they do not occur in the animal kingdom. They have, however,
a very wide distribution in the vegetable kingdom, being present
in leaves, roots, seeds and stems of all forms of plants, many times in
intimate association or even chemical combination with galactans. In
herbivora, pentosans are 40-80 per cent utilized. '^ The few tests on
record as to the pentosan utilization by man^ indicate that 80-95
per cent disappear from the intestine. According to Cramer,^ bacteria
are efficient hemicellulose transformers. It has not yet been dem-
onstrated that pentosans form glycogen in man, and for this reason
they must be considered as playing an unimportant part in human
nutrition. Gum arable an important pentosan may be hydrolyzed
by concentrated hydrochloric acid if boiled for a short time. The
pentose arabinose results from such hydrolysis.

Galactans. — In common with the pentosans the galactans have a very
wide distribution in the vegetable kingdom. The pure galactans yield
galactose upon hydrolysis. One of the most important members of
the galactan group is agar-agar, a product prepared from certain types
of Asiatic sea-weed. This galactan is about 50 per cent utilizable by
herbivora^ and 8-27 per cent utilizable by man.^ Agar ingestion has
been shown to be a very efficient therapeutic aid in cases of chronic
constipation.^'' This is particularly true when the constipation is due
to the formation of dry, hard, fecal masses (scybala), a type of fecal
formation which frequently follows the ingestion of a diet which is

^ Swartz: Transactions of the Connecticut Academy of Arts and Sciences, 16, 247, 1911.

2 Konig and Reinhardt: Zeit.f. Untersuchung der Nahrwtgs u. Genussmittel, 5, no, 1902.

2 Cramer: Inaug. Diss., Halle, 1910.

*Lohrisch: Zeit.f. exper. Path. u. Pharm., 5, 478, 1908.

^ Saiki: Jour. Biol. Chem., 2, 251, 1906.

^ Mendel: Zentralblatf. d. gesammte Phys. u. Path, des Stoffw., No. 17, i, 1908.

'Schmidt: Miinch. nied. Woch., 52, 1970, 1905.

CARBOHYDRATES 5 1

very thoroughly digested and absorbed. The agar, because of its
relative indigestibility and its property of absorbing water yields a
bulky fecal mass which is sufficiently soft to permit of easy evacua-
tion. Agar has been used with good results in the treatment of con-
stipation in children.^ The function of agar is not limited to its use
in connection with constipation, it may. serve in other capacities as an
aid to intestinal therapeutics. ^

Experiments on a Pentosan

1. Solubility. — Test the solubility of gum arabic in hot and cold water and
alcohol.

2. Iodine Test. — ^Add a drop of dilute iodine solution to a Uttle gum arabic
on a test-tablet. It resembles cellulose in giving no color with iodine.

3. Hydrolysis of Gum Arabic. — Introduce a little gum arabic into a test-tube,
add 5-10 c.c. of strong hydrochloric acid (cone. HCl and water 1:1) and heat to
boiling for 5-10 minutes. Cool, neutralize with potassium hydroxide and test
by the Fehling or some other reduction test. A positive reaction should be ob-
tained indicating that the gum arabic has been hydrolyzed by the acid with the
production of a reducing substance. What is this reducing substance? How
would you identify it?

Experiments on a Galactan

1. SolubiUty. — Test the solubility of agar-agar in hot and cold water. Ob-
serve its marked property of imbibing water (see above).

2. Iodine Test. — ^Add a drop of dilute iodine solution to a little agar-agar on a
test-tablet. It resembles cellulose in giving no color with iodine.

3. Hydrolysis of Agar-agar.^ — Introduce a few pieces of agar-agar into a test-
tube, add 5-10 c.c. of strong hydrochloric acid (cone. HCl and water 1:1) and
heat to boiling for 5-10 minutes. Cool, neutralize with potassium hydroxide and
test by the Fehhng or some other reduction test. A positive reaction should be
obtained indicating that the agar-agar has been hydrolyzed by the acid with the
production of a reducing substance. What is this reducing substance? How
would you identify it?

REVIEW OF CARBOHYDRATES

In order to facilitate the student's review of tlie carbohydrates, the
preparation of a chart similar to the appended model is recommended.
The signs + and — may be conveniently used to indicate positive
and negative reaction. Only those carbohydrates which are of greatest
importance from the standpoint of physiological chemistry have been
included in the chart.

* Morse: Journal American Medical Ass'n., 55, 934 1910.
^Einhorn: Bcrl. klin. Woch., 49, 113, 1912.

52

PHYSIOLOGICAL CHEMISTRY

MODEL CHART FOR REVIEW PURPOSES

Carbo-
hydrate

Solubility

a-Naphthol Reaction
(Molisch)

Moore's Test .
Fehling's Test
Nylander-Alm6n Test
Barfoed's Test

Iodine Test

Resorcinol-Hydrochloric
Acid Reaction (SeliwanofI)

Orcinol-H ydrochloric
Acid Reaction (Bial)

Mucic Acid Test

Precipitation by
Alcohol

a

a
o

N

0

a

o

1

DifEusiblility

Fermentation

Products of Hydrolysis

1

a
Pi.

Glucose.

i i

1

1

1 Fructose.

t

\

1 1

Pentose.

i

!

[

i

Maltose.

1 1 -

i

' '

Lactose. j

I

j \ ■ \ i ^ : 1 i

Sucrose. |

i ' 1

'■'■ \ \

Starch.

Invdin.

1

; i ;

Glycogen.

'

1

Dextrin. ,

Cellulose. ~ |

1 ' ' ^

1 !

Gum Arabic.

1

1

Agar-agar. '

"Unknown" Solutions of Carbohydrates

At this point the student will be given several "unknown" solutions,
each solution containing one or more of the carbohydrates studied.
He will be required to detect, by means of the tests on the preceding
pages, each carbohydrate constituent of the several "unknown" solu-
tions and hand in, to the instructor, a written report of his findings, on
slips furnished by the laboratory.

The scheme given on page 53 may be of use in this connection.

CARBOHYDRATES

53

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CHAPTER III
SALIVARY DIGESTION

The saliva is secreted by three pairs of glands, the submaxillary,
sublingual, and parotid, reinforced by numerous small glands called
buccal glands. The saliva secreted by each pair of glands possesses
certain definite characteristics peculiar to itself. For instance, in man
the parotid glands ordinarily secrete a thin, watery fluid, the submaxil-
lary glands secrete a somewhat thicker fluid containing mucin, while the
product of the sublingual glands has a more mucilaginous character.
The saliva as collected from the mouth is the combined product of all
the glands mentioned. The fact that there are pronounced variations
in the composition of different fractions of saliva secreted by the same
normal individual on a uniform diet has been emphasized by Lothrop
and Gies.^

The saliva may be induced to flow by many forms of stimuli, such as
chemical, mechanical, electrical, thermal, and psychical, the nature and
amount of the secretion depending, to a limited degree, upon the par-
ticular class of stimuli employed as well as upon the character of the
individual stimulus. For example, in experiments upon dogs it has been
found that the mechanical stimulus afforded by dropping several pebbles
into the animal's mouth caused the flow of but one or two drops of
saliva, whereas the mechanical stimulus afforded by sand thrown into
the mouth induced a copious flow of thin watery fluid. Again, when
ice-water or snow was placed in the animal's mouth no saliva was seen,
while an acid or anything possessing a bitter taste, which the dog wished
to reject, caused a free flow of the thin saliva. On the other hand, when
articles of food were placed in the dog's mouth the animal secreted a
thicker saliva having a higher mucin content — a fluid which would lubri-
cate the food and assist in the passage of the bolus through the esopha-
gus. It was further found that by simply drawing the attention of the
animal to any of the substances named above, results were obtained
similar to those secured when the substances were actually placed in the
animal's mouth. For example, when a pretense was made of throw-
ing sand into the dog's mouth, a watery saliva was secreted, whereas
food under the same conditions excited a thicker and more slimy
secretion. The exhibition of dry food, in which the dog had no par-

1 Lothrop and Gies: Journal of I he Allied {Dental) Societies, 6, 65, 191 1.

54

SALIVARY DIGESTION 55

ticular interest (dry bread), caused the secretion of a large amount of
watery saliva, while the presentation of moist food, which was eagerly
desired by the animal, called forth a much smaller secretion, slimy in
character. These experiments show it to be rather difficult to dif-
ferentiate between the influence of physiological and psychical stimuli.

The amount of saliva secreted by an adult in 24 hours has been vari-
ously placed, as the result of experiment and observation, between looo
'and 1500 c.c, the exact amount depending, among other conditions,
upon the character of the food.

The saliva of adults ordinarily has a weak, alkaline reaction to litmus,
but becomes acid, in some instances, 2-3 hours after a meal or during
fasting. The saliva of the newborn is generally neutral to litmus,
whereas that of infants, especially those breast-fed, is generally acid.^
The alkalinity of saliva is due principally to di-sodium hydrogen phos-
phate (Na2HP04) and its average alkalinity may be said to be equiva-
lent to 0.08-0. 1 per cent sodium carbonate. The saliva is the most dilute
of all the digestive secretions, having an average specific gravity of 1.005
and containing only 0.5 per cent of solid matter. Among the solids are
found albumin, globulin, mucin, urea, the enzymes salivary amylase
(ptyalin), maltase, and pep tide-splitting enzymes, phosphates, and
other inorganic constituents. Potassium thiocyanate, KSCN, is also
generally present in the saliva. It has been claimed that this sub-
stance is present in greatest amount in the saliva of habitual smokers.
The significance of thiocyanate in the saliva is not known; it probably
comes from the ingested thiocyanates and from the breaking down of
protein material. The attempts to show some relationship between
tooth decay and the thiocyanate content of the saliva secreted into
the mouth cavity have met with failure. The most recent experiments-
indicate a virtual absence of such relationship.

The so-called tartar formation on the teeth is composed almost
entirely of calcium phosphate with some calcium carbonate, mucin,
epithelial cells, and organic debris derived from the food. The calcium
salts are held in solution as acid salts, and are probably precipitated by
the ammonia of the breath. The various organic substances just men-
tioned are carried down in the precipitation of the calcium salts.

The suggestion has been made that mucin is the salivary constituent
*' which is particularly influential in the development of local conditions
favoring the onset of dental decay. "^

The principal enzyme of the saliva is known as salivary amylase or
ptyalin. This is an amylolytic enzyme (see page 4), so called because it

^ AUaria: Monalsschr fiir Kinderhcilkmide, to, 179, igii.

''Lothrop and Gies: Journal of lite Allied {Dental) Societies, 6, 65, 19U.

' Id.: Ibid., 5, No. 4, 1910.

56 PHYSIOLOGICAL CHEMISTRY

possesses the property of transforming complex carbohydrates such as
starch and dextrin into simpler bodies. The action of salivary amylase
is one of hydrolysis and through this action a series of simpler bodies are
formed from the complex starch. The first product of the action of the
ptyalin of the sahva upon starch paste is soluble starch (amidulin) and its
formation is indicated by the disappearance of the opalescence of the
starch solution. This body resembles true starch in giving a blue color
with iodine. Next follows the formation, in succession, of a series of
dextrins, called erythro-dextrin, a-achroo-dextrin, ^-achroo-dextrin, and
y-achroo-dextrin, the erythro-dextrin being formed directly from soluble
starch and later being itself transformed into a-achroo-dextrin from which
in turn are produced j3-achroo-dextrin, y-achroo-dextrin and perhaps other
dextrins. Accompanying each dextrin a small amount of maltose is
formed, the quantity of maltose growing gradually larger as the proc-
ess of transformation progresses. (Erythro-dextrin gives a red color
with iodine, the other dextrins give no color.) The next stage is the
transformation of the final dextrin into maltose, the latter being the prin-
cipal end-product of the salivary digestion of starch. At this point
a small amount of glucose is formed from the maltose through the ac-
tion of the enzyme maltase. The above changes may be represented
graphically as follows:

Starch

I

Soluble starch

Erythro-dextrin Maltose

a-Achroo-dextrin Maltose

I

l3-Achroo-dextrin Maltose

7-Achroo-dextrin Maltose

I I

I

Maltose

Salivary amylase acts in alkaline, neutral, or combined acid solu-
tions. It will act in the presence of relatively strong combined HCl (see
page 140), whereas a trace (0.003 P^^^ cent to 0.0006 per cent) of ordinary

SALIVARY DIGESTION 57

free hydrochloric acid will not only prevent the action but will destroy
the enzyme. By sufficiently increasing the alkalinity of the saliva to
litmus, the action of the salivary amylase is inhibited.

It has been shown by Cannon that salivary digestion may proceed
for a considerable period after the food reaches the stomach, owing
to the slowness with which the contents are thoroughly mixed with
the acid gastric juice and the consequent tardy destruction of the
enzyme. Food in the pyloric end of the stomach is soon mixed with the
gastric secretion, but food in the cardiac end is not mixed with the acid
gastric juice for a considerable period of time, and in this region during
that time sahvary digestion may proceed undisturbed.

It has been found that salivary amylase acts more efficiently when
the saliva is diluted from 4 to 7 times. '^

Water softened by lime- inhibits the action of salivary amylase due
to the presence of magnesium hydroxide in this water. ^ Electrolytes
have an important influence upon the action of amjdases. The CI ion
has a pronounced facilitating action (see Pancreatic Amylase).

The question of the adaptation of the salivary secretion to diet is one
which has received considerable attention in recent years. It has been
claimed, on the basis of experimental evidence/ that the continued
feeding of a carbohydrate diet causes the secretion of a saliva which
contains a higher concentration of salivary amylase and one which is
therefore able to more efficiently digest the carbohydrate fed. On the
other hand, strong evidence^ has been submitted that the amylase con-
tent of the saliva is not increased through the continued feeding of a
carbohydrate diet. In general the consensus of opinion is opposed
to the adaptation of digestive secretions to diet.

Maltose, sometimes called glucase, is the second enzyme of the saliva.
The principal function of maltase is the splitting of maltose into glucose.
Besides occurring in the saliva it is also present in the pancreatic and
intestinal juices. For experimental purposes the enzyme is ordinarily
prepared from corn. The principles of the "reversibility" of enzyme
action were first demonstrated in connection with maltase by Croft Hill.

It is claimed that the saliva contains dipeptide- and tripeptidc-
spHtting enzymes.^ Leucyl-glycyl-alanine was the tripeptide split,

^ Bergeim and Hawk: Jour. Am. Clicm. Soc, 35, 461, 1913.

^ Prepared by treating tap water with one-sixth its volume of saturated lime water,
allowing to stand 24 hours and filtering.

' Bergeim and Hawk: Jottr. Am. Chem. Soc, 35, 1049, 1913.

* Neilson and Terry: American Journal of Physiology, 15,406,1905; Neilson and Lewis:
Journal of Biological Chemistry, 4, 501, 1908.

^ Mendel: American Journal of the Medical Sciences, Oct., 1909; Mendel and UnderhiU:
Journal of Biological Chemistry, 3, 135, 1907; Mendel, Chapman and Blood: Medical
Record, Aug. 27, igio.

8 Koelker: Zeitschrift fur physiol. Chem., 76, 27, 191 1,

58 PHYSIOLOGICAL CHEMISTRY

whereas the cleavage of several dipeptids was brought about. The
action is similar to that of intestinal erepsin (see Chapter XI). Later
investigations (see page 199), apparently have demonstrated that the
peptoly tic power of saliva, at least in some cases, is due to bacteria.

Microscopical examination of the saliva reveals salivary corpuscles,
bacteria, food debris, epithelial cells, mucus, and fungi. In certain
pathological conditions of the mouth, pus cells and blood corpuscles
may be found in the saliva.

Experiments on Saliva

A satisfactory method of obtaining the saliva necessary for the ex-
periments which follow is to chew a small piece of pure paraffin wax,
thus stimulating the flow of the secretion, which may be collected in a
small beaker. Filtered saliva is to be used in every experiment except
for the microscopical examination.

I. Microscopical Examination. — Examine a drop of unfiltered saliva micro-
scopically, after staining with methylene blue, and compare with Fig. 19 below.

Fig. 20. — Microscopical Constituents of Saliva.

a, Epithelial cells; b, salivary corpuscles; c, fat drops; d, leucocytes; e, f and g, bacteria;

h, i, and k, fission-fungi.

2. Reaction. — ^Test the reaction to litmus, phenolphthalein and Congo red.

3. Specific Gravity. — Partially fill a urinometer cylinder with saliva, introduce
the urinometer, and observe the reading.

4. Test for Mucin.— To a small amount of saliva in a test-tube add 1-2 drops
of dilute acetic acid. Mucin is precipitated.

5. Biuret Test.^ — ^Render a Uttle saliva alkaline with an equal volmne of KOH
and add a few drops of a very dilute (2-5 drops in a test-tube of water) copper
sulphate solution. The formation of a purplish-violet color is due to mucin.

This reaction is given by protein material and simply indicates that mucin is
a protein.

6. Millon's Reaction. 2 — Add a few drops of Millon's reagent to a little saliva.
A light yellow precipitate formed by the mucin gradually turns red upon being
gently heated.

This reaction indicates the presence of protein (mucin).

^ The significance of this reaction is pointed out on p. 98.
* The significance of this reaction is pointed out on p. 97.

I

SALIVARY DIGESTION 59

7. Preparation of Mucin. — Pour 25 c.c. of saliva into 100 c.c. of 95 per cent
alcohol, stirring constantly. Cover the vessel and allow the precipitate to stand
at least 12 hours. Pour off the supernatant liquid, collect the precipitate on a
filter and wash it, in turn, with alcohol and ether. Finally dry the precipitate,
remove it from the paper and make the following tests on the mucin : faj Test
its solubiUty in the ordinary solvents (see page 21); (b) Millon's reaction; (c)
dissolve a small amount in KOH, and try the biuret test on the solution; (d) boil
the remainder, with 10-25 c.c. of water to which 5 c.c. of dilute HCl has been
added, until the solution becomes brownish. Cool, render alkaline with solid
KOH, and test by Fehling's solution. A reduction should take place.

Mucin is what is known as a conjugated protein or glycoprotein
(see page 112) and upon boiling with the acid the carbohydrate group
in the molecule has been split off from the protein portion and its
presence is indicated by the reduction of Fehling's solution.

8. Inorganic Matter.- — Test for chlorides, phosphates, sulphates, and cal-
cium. For chlorides, acidify with HNO3 and add AgNOs. For phosphates,
acidify with HNO3, heat and add molybdate solution. ^ For sulphates, acidify
with HCl and add BaCl2 and warm. For calcium, acidify with acetic acid, CH3-
COOH, and add ammonium oxalate, (NH4)2C204.

9. Viscosity Test. — Place filter papers in two funnels, and to each add an equal
quantity of starch paste (5 c.c). Add a few drops of saUva to one lot of paste and
an equivalent amount of water to the other. Note the progress of filtration in
each case. Why does one solution filter more rapidly than the other?

10. Test for Nitrites. — Add 1-2 drops of dilute H2SO4 to a little saliva and
thoroughly stir. Now add a few drops of a potassium iodide solution and some
starch paste. Nitrous acid is formed which liberates iodine, causing the formation
of the blue iodide of starch.

11. Thiocyanate Tests. — (a) Ferric Chloride Test. — To a little sahva in a
small porcelain crucible, or dish, add a few drops of dilute ferric chloride and
acidify slightly with HCl. Red ferric thiocyanate Fe(SCN)3 forms. To show
that the red coloration is not due to iron phosphate add a drop of HgCl2 when
colorless mercuric thiocyanate forms.

{b) Solera's Reaction. — This test depends upon the Uberation of iodine through
the action of thiocyanate upon iodic acid. Moisten a strip of starch pastc-iodic acid
test paper- with a little saliva. If thiocyanate be present the test paper will assume
a blue color, due to the liberation of iodine and the subsequent formation of the so-
called iodide of starch.

12. Digestion of Starch Paste. — To 25 c.c. of starch paste in a small beaker,
add 5 drops of saliva and stir thoroughly. At intervals of a minute remove a
drop of the solution to one of the depressions in a test-tablet and test by the io-
dine test. If the blue color with iodine still forms after five minutes, add another
5 drops of saUva. The opalescence of the starch solution should soon disappear,
indicating the formation of soluble starch which gives a blue color with iodine.

^ See "Reagents and Solutions."

^ This test paper is prepared as follows: Saturate a good quality of filter paper with 0.5
per cent starch paste to which has been added sufficient iodic acid to make a i per cent
solution of iodic acid and allow the paper to dry in the air. Cut it in strips of suitable size
and preserve for use.

6o PHYSIOLOGICAL CHEMISTRY

This body should soon be transformed into erythro-dextrin which gives a red
color with iodine, and this in turn should pass into achroo-dextrin which gives no
color with iodine. This is called the achromic point. When this point is reached
test by Fehling's test to show the production of a reducing body. A positive
Fehling's test may be obtained while the solution still reacts red with iodine
inasmuch as some maltose is formed from the soluble starch coincidently with
the formation of the erythro-dextrin. How long did it take for a complete trans-
formation of the starch? For a graphic representation of the above changes see
page 56.

13. Separation of the Products of Salivary Digestion. — To 25 c.c. of starch
paste in a small beaker add i c.c. of saliva and stir thoroughly. At intervals of
one minute test a drop of the mixture by the iodine test. If the blue color per-
sists after five minutes add another i c.c. of saUva. When the mixture reacts
red with iodine, indicating that erythrodextrin has been formed, add 100 c.c. of
95 per cent alcohol. Allow to stand until the white precipitate has settled.
Filter, evaporate the filtrate to dryness, dissolve the residue in 5-10 c.c. of water
and try Fehling's test (page 26) and the phenylhydrazine reaction (see Glucose, 3,
page 22). On the dextrin precipitate try the iodine test (page 45). Also
hydrolyze the dextrin as given under Dextrin, 4, page 48.

14. Digestion of Dry Starch. — In a test-tube shake up a small amount of dry
starch with a little water. Add a few drops of saUva, mix well, and allow to
stand. After 10-20 minutes filter and test the filtrate by FehUng's test. What
is the result and why?

Dry starch is very slowly digested by salivary amylase.

15. Digestion of Inulin.— To 5 c.c. of inulin solution in a test-tube add 10 drops
of saliva and place the tube in the incubator or water-bath at 4o°C. After one-
half hour test the solution by Fehling's test.^ Is any reducing substance present?
What do you conclude regarding the salivar>^ digestion of inulin?

16. Influence of Temperature. — In each of four tubes place about 5 c.c. of
starch paste. Immerse one tube in cold water from the faucet, keep a second at
room temperature, and place a third in the incubator or the water-bath at 40°C.
(If the temperature of the bath or incubator is allowed to rise to 7o°C. or over the
enzyme is destroyed and no digestion takes place.) Now add to the contents of
each of these three tubes two drops of saliva and shake well; to the contents of
the fourth tube add two drops of boiled saUva. Test frequently by the iodine
test, using the test-tablet, and note in which tube the most rapid digestion occurs.
Explain the results.

17. Influence of Dilution.- — Take a series of six test-tubes each containing
9 c.c. of water. Add i c.c. of saUva to tube i and shake thoroughly. Remove
I c.c. of the solution from tube i to tube 2 and after mixing thoroughly remove
I c.c. from tube 2 to tube 3. Continue in this manner until you have 6 saliva
solutions of gradually decreasing strength. Now add starch paste in equal
amounts to each tube, ttiiy very thoroughly, and place in the incubator or water-

1 If the inulin solution gives a reduction before being acted upon by the saliva it will be
necessary to determine the extent of the original reduction by means of a "check" test (see

p. 47)-

'^ The technic of Wohlgemuth's method (see Chapter X) may be employed in this test
if so desired.

SALIVARY DIGESTIOX 6 1

bath at 40'C. After 10-20 minutes test by both the iodine and Fehhng's tests.
In how great dilution does your saliva act?

18. Influence of Acids and Alkalis. — (a) Influence of Free Acid. — Prepare a
series of six tubes in each of which is placed 4 c.c. of one of the following strengths
of free HCl : 0.2 per cent, o.i per cent, 0.05 per cent, 0.025 per cent, 0.0125 per
cent and 0.006 per cent. Now add 2 c.c. of starch paste to each tube and shake
them thoroughly. Complete the solutions by adding 2 c.c. of saUva to each and
repeat the shaking. The total acidity of this series would be as follows : o.i per
cent, 0.05 per cent, 0.025 per cent, 0.0125 P^r cent, 0.006 per cent and 0.003 P^r
cent. Place these tubes on the water-bath at 40°C. for 10 20 minutes. Divide
the contents of each tube into two parts, testing one part by the iodine test and
testing the other, after neutraUzation, by Fehhng's test. What do you find?

(b,) Influence of Combined Acid (Protein Salti. -Repeat the first three ex-
periments of the above series using combined hydrochloric acid (see page 140)
instead of the free acid. How does the action of the combined acid differ from
that of the free acid? (For a discussion of combined acid see page 140. 1

(c) Influence of AlkaU— Repeat the first four experiments under (ai replac-
ing the HCl by 2 per cent, i per cent, 0.5 per cent and 0.25 per cent NajCOs.
Neutralize the alkalinity before trying the iodine test (see Starch, 5, page 45),

(d) Nature of the Action of Acid and AlkaU. — Place 2 c.c. of sahva and 2 c.c,
of 0.2 per cent HCl in a test-tube and leave for 15 minutes. NeutraUze the
solution, add 4 c.c. of starch paste and place the tube in the incubator or water-
bath at 40'C. In 10 minutes test by the iodine and Fehhng's tests and explain
the result. Repeat the experiment, replacing the 0.2 per cent HCl by 2 per cent
NaoCOs. What do you deduce from these two experiments?

19. Influence of MetaUic Salts, etc. — In each of a series of tubes place 4 c.c.
of starch paste and J^ c.c. of one of the solutions named below. Shake well, add
^2 c.c. of saliva to each tube, thoroughly mix, arid place in the incubator or water-
bath at 40°C. for 10-20 minutes. Show the progress of digestion by means of the
iodine and Fehling tests. Use the following chemicals: MetaUic sails, 10 per cent
lead acetate, 2 per cent copper sulphate, 5 per cent ferric chloride, 8 per cent mer-
curic chloride; Neutral salts, 10 per cent sodium chloride, 10 per cent magnesium
sulphate, 3 per cent barium chloride, 10 per cent Rochelle salt. Also tr\' the influ-
ence of 2 per cent carbolic acid, 95 per cent alcohol, and ether and chloroform.
What are your conclusions?

Antiseptics do not necessarily inhibil enzyme action.

20. Excretion of Potassium Iodide. — Ingest a small dose of potassiimi iodide
(0.2 gram) contained in a gelatin capsule, quickly rinse out the mouth with
water, and then test the saUva at once for iodine. This test should be negative.
Make additional tests for iodine at two-minute intervals. The test for iodine is
made as follows: Take i c.c. of NaNO. and i c.c. of dilute HjSOi' in a test-
tube, add a little saliva directly from the mouth, and a small amount of starch
paste. The formation of a blue color signifies that the potassium iodide is being
excreted through the salivary glands. Note the length of time elapsing between
the ingestion of the potassium iodide and the appearance of the first traces of the
substance in the saliva. If convenient, the urine may also be tested. The

' Instead of this mixture a lew drops of HXO3 possessing a yellowish or brownish color
due to the presence of HXO.; may be employed.

62 PHYSIOLOGICAL CHEMISTRY

chemical reactions taking place in this experiment are indicated in the following
equations :

(a) 2NaN02+H2S04-^2HN02+Na2S04.

(b) 2KI + H2S04^2HI + K2S04.

(C) 2HNO2+ 2HI-^l2 + 2H20 + 2NO.

CHAPTER IV
PROTEINS :i THEIR DECOMPOSITION AND SYNTHESIS

The proteins are a class of substances, which in the light of our pres-
ent knowledge, consist, in the main, of combinations of a-amino acids or
their derivatives. These protein substances form the chief constituents
of many of the fluids of the body, constitute the organic basis of animal
tissue, and at the same time occupy a decidedly preeminent position
among our organic food-stuffs. They are absolutely necessary to the
uses of the animal organism for the continuance of life and they cannot
be satisfactorily replaced in the diet of such an organism by any other
dietary constituent either organic or inorganic. Such an organism may
exist without protein food for a period of time, the length of the period
varying according to the specific organism and the nature of the substi-
tution offered for the protein portion of the diet. Such a period is, how-
ever, distinctly one of existence rather than one of normal life and one
which is consequently not accompanied by such a full and free exercise
of the various functions of the organism as would be possible upon an
evenly balanced ration, i.e., one containing the requisite amount of
protein food. These protein substances are, furthermore, essential
constituents of all living cells and therefore without them vegetable life
as well as animal life is impossible.

The proteins, which constitute such an important group of sub-
stances, differ from carbohydrates and fats very decidedly in elementary
composition. In addition to containing carbon, hydrogen, and oxygen,
which are present in fats and carbohydrates, the proteins invariably
contain nitrogen in their molecule and generally sulphur also. Pro-
teins have also been described which contain phosphorus, iron, copper,
iodine, manganese, and zinc. The percentage composition of the more im-
portant members of the group of protein substances would fall within
the following limits: C = 50-55 per cent, H = 6-7.3 P^r cent, 0 =
19-24 per cent, N= 15-19 per cent, 8 = 0.3-2.5 per cent, P = o.4-
0.8 per cent ivhen present. WHien iron, copper, iodine, manganese, or
zinc are present in the protein molecule they are practically without

^ The term proleid has been very widely used by English-speaking scientists to signify
the class of substances we have called proteins.

63

64 PHYSIOLOGICAL CHEMISTRY

exception present only in traces and with the exception of iodine are
probably not constituents of the protein molecule.^

Of all the various elements of the protein molecule, nitrogen is by far
the most important. The human body needs nitrogen for the continua-
tion of life, but it cannot use the nitrogen of the air or that in various
other combinations as we find it in nitrates, nitrites, etc. However, in
the protein molecule the nitrogen is present in a form which is utilizable
by the body. The nitrogen in the protein molecule occurs in at least
four different forms as follows :

I. Monamino acid nitrogen.
11. Diamino acid nitrogen or basic nitrogen.

III. Amide nitrogen.

IV. A guanidine residue.

The actual structure of the protein molecule is still unknown, and we
have as yet no means by which its molecular weight can be even approxi-
mately established. The many attempts which have been made to
determine this have led to very different results, some of which are given
in the following table:

Globin =15000—16086

Oxyhemoglobin = 14800— 15000 — 16655 — 16730

Of these figures, those given for oxyhemoglobin deserve the most
consideration, for these are based on the atomic ratios of the sulphur
and iron contained in this substance. The simplest formula that can
be calculated from analyses of oxyhemoglobin, namely,

C658Hii8lN207S2FeO210

serves to show the great complexity of this substance.

The decomposition- of protein substances may be brought about by
oxidation or hydrolysis, but inasmuch as the hydrolytic procedure has
been productive of the more satisfactory results, that type of decomposi-
tion procedure alone is used at present. This hydrolysis of the protein
molecule may be accomplished by acids, alkalis, or superheated steam,
and in digestion by the action of the proteolytic enzymes. The char-
acter of the decomposition products varies according to the method
utilized in tearing the molecule apart. Bearing this in mind, we may
say that the decomposition products of proteins include proteoses, pep-
tones, peptides, carbon dioxide, ammonia, hydrogen sulphide, and amino

1 Some investigators regard these elements as contaminations, or constituents of some
non-protein substance combined with the protein.

2 The terms "degradation," "dissociation," and "cleavage," are often used in this con-
nection.

PROTEINS 65

acids. These amino acids' constitute a long list of important substances
which contain nuclei belonging either to the aliphatic, carbocyclic, or
heterocyclic series. The list includes glycocoll, alanine, serine, phenyl-
alanine, tyrosine, cystine, tryptophane, histidine, valine, arginine, leucine,
isoleucine, lysine, aspartic acid, glutamic acid, proline, oxyproline, and
diaminotrihydroxydodecanoic acid. Of these amino acids, tyrosine and
phenylalanine contain carbocyclic nuclei: histidine, proline, and trypto-
phane contain heterocyclic nuclei: and the remaining members of the
list, as given, contain aliphatic nuclei. The amino acids are preemi-
nently the most important class of protein decomposition products.
These amino acids are all a-amino acids, and, with the exception of
glycocoll, are all optically active. Furthermore, they are amphoteric
substances and consequently are able to form salts with both bases and
acids. These properties are inherent in the NH2 and COOH groups of
the amino acids.

The decomposition products of protein may be grouped as pri-
mary and secondary decomposition products. By primary products are
meant those which exist as radicals within the protein molecule and
which are hberated, upon cleavage of this molecule, with their carbon
chains intact and the position of their nitrogen unaltered. The second-
ary products are those which result from the disintegration of the
primary cleavage products. No matter what method is used to de-
compose a given protein molecule, the primary products are largely the
same under all conditions.^

In the process of hydrolysis the protein molecule is gradually broken
down and less complicated aggregates than the original molecule are
formed, which are known as proteoses, peptones, and peptides, and which
still possess true protein characteristics. Further hydrolysis causes the
ultimate transformation of these substances, of a protein nature, into the
amino acids of known chemical structure. In this decomposition the
protein molecule is not broken down in a regular manner into }/^, ^,
^i portions and the amino acids formed in a group at the termination of
the hydrolysis. On the contrary, certain amino acids are formed very
early in the process, in fact while the main hydrolytic action has pro-
ceeded no further than the proteose stage. Gradually the complexity
of the protein portion undergoing decomposition is simplified by the
splitting off of the amino acids and finally it is so far decomposed
through previous cleavages that it yields only amino acids at the
succeeding cleavage. In short, the general plan of the hydrolysis of
the protein molecule is similar to the hydrolysis of starch. In the case

^For a discussion of amino acids see Underhill's "Plij'siology of Amino Acids,'' Yale
University Press, Nov., 1915.

* Alkaline hydrolysis yields urea and brrttVAtwc which result iiom arginine, the product of
acid hj'drolysis.

66 PHYSIOLOGICAL CHEMISTRY

of starch there is formed a series of dextrins of gradually decreasing
complexity and coincidently with the formation of each dextrin a small
amount of sugar is split off and finally nothing but sugar remains. In
the case of protein hydrolysis there is a series of proteins of gradually
decreasing complexity produced and coincidently with the formation of
each new protein substance amino acids are split oft" and finally the sole
products remaining are amino acids.

Inasmuch as diversity in the method of decomposing a given protein
does not result in an equally diversified line of decomposition products,
but, on the other hand, yields products which are quite comparable in
character, it may be argued that there are probably well-defined Hnes of
cleavage in the individual protein molecule and that no matter what the
force brought to bear to tear such a molecule apart, the disintegration,
when it comes, will yield in every case certain definite fragments.
These fragments may be called the "building stones" of the protein
molecule, a term used by some of the German investigators. Take, for
example, the decomposition of protein which may be brought about
through the action of the enzyme trypsin of the pancreatic juice.
When this enzyme is allowed to act upon a given protein, the latter is
disintegrated in a series of definite cleavages, resulting in the formation
of proteoses, peptones, and peptides in regular order, the peptides being
the last of the decomposition products which possess protein character-
istics. They are all built up from amino acids and are therefore closely
related to these acids on the one side and to peptones on the other.
We have di-, tri-, tetra-, penta-, dec a-, and poly-peptides which are
named according to the number of amino acids included in the peptide
molecule. Following the peptides there are a diverse assortment of
monamino and diamino acids which constitute the final products of
the protein decomposition. These acids are devoid of any protein
characteristics and are therefore decidedly different from the original
substance from which they were derived. From a protein of huge
molecular weight, a typical colloid, perhaps but slightly soluble, and
entirely non-dift'usible, we have passed by way of proteoses, peptones,
and peptides to a class of simpler crystalline substances which are, for
the most part, readily soluble and diffusible.

These amino acids after their production in the process of digestion,
as just indicated, are synthesized within the cells of the organism to
form protein material which goes to build up the tissues of the body.
It is thus seen that the amino acids are of prime importance in the
animal economy. It was formerly believed that these essential factors
in metabolism and nutrition could not be produced within the animal
organism from their elements, but were only yielded upon the hydrol-

PROTEINS

67

ysis of ingested protein of animal or vegetable origin. Experi-
ments, however, by Abderhalden and by Grafe and Schlapfer and
others indicate that the nitrogen of food protein may in part be re-
placed by ammonium salts. Experiments by Osborne and others
also indicate amino acid synthesis by animals.

Important data regarding the decomposition products of the protein
molecule are given in the tables which follow.

COMPARISON OF THE DECOMPOSITION PRODUCTS OF PROTAMINES,

AND

OTHER PROTEINS.

Protamines.!

Other Proteins.

(Per cent of total nitrogen of

(Per cent of amino acids in

amino acid.)

proteins.)

Decomposition

o5
a
■c

6

G .

•c

c

a
'a

V

c

■5

6

c

"d

'c

i

d

"d

Product.

.a
B

1

0
3

u

6

a

u

0

E

.2.S

XI

0

0

13
0

5

•

GlycocoU ....

1

0

3-8

0

16. S

0

0

Alanine .

3.6

1.5 0.8 4.2 9.79

Valine.

+ I + I + |l.6s| 3-34

6.2

7.2

Leucine I +

14-5

9.4 2.1 :29.o 19. SS

Proline I 3-

+ 4.3

4.1 I 6.7 S-2 ! 2.3 9-04

Phenylalanine.

2.3s

6.SS

Aspartic acid 0.58

4-S

1.4 0.56. 4.4 1. 71

Glutamic acid ■ 43-66 I18.74 !ii-0 l.88j 1.7 26.17

Serine.

+ 3-25 0.13 0.33 I o.s 0.4 0.6

Tyrosine.

i-s:

45

1.3 3.SS

Arginine 88.8 67 .7J63.5 8.7:28.0 88.0 89.2 j 3.16 I14.2 4.84 7-62} 5-4 ' ^SS

Lysine

1 8.4 30.3! 6.6 . . . .

. . . . 0

;v

S-95 2.7S| 4.3

0

Histidine

II. 8

. . . . 0.61

2.2

2.50 0.40 II. 0

0.82

Tryptophane

....| +

+

i.. ..!....'

+

1.5 0 +

0

. . . . ' 0 .45

1 .00

0.06s 0 0.3

?

?

2.0

1 0.23 6.4

I .0

?

^^ , 1

'0.75 • • •

?

decanoic acid. ' ' 1 1

5.33

2.3

i.6i

3 64

i 1 1 I ■

When we examine the formulas of the principal members of the
crystalline end-products of protein decomposition we note that they are

■ ''Kossel: Zeit. physiol. Chem., 44, 347, 1905.
^Osborne and Guest: Jour. Biol. Chcm., 0, 425, 19 11.
^.\bderhalden, Kossel and others.

* Abderhalden, Fischer, Morner and others.

'Fischer, Levene and Aders: Zeil. physiol. Chem., 35, 70, 1902; also Lcvene and
Beatty: Ibid., 49, 252, 1906.

"Abderhalden: Zcit. physiol. Chem., 37, 4S4, 1903.
'Osborne and Liddle, .\m. Jour. Physiol., 26, 295, 1910.

* This unique and important protein has probably been more carefully analyzed
than any other.

68

PHYSIOLOGICAL CHEMISTRY

W

H
O
P<

Ah
«

o
o

•6
E

s

'x

From decom-
position of

en J3

(0

'S

•E

U

4.
C

c
'Z

1.

c
X

c

■4
tr

c

£

4

c

s

0

Casein.

4J 1 VO

Q 1 "

o

On

o
o

o

HI

0

0

o>

HI

8v

M

0

M

Ov

^ c -
C i4^

f ^

tn -^

tn cd

c n

CO (u

O ^
« 3

T3

C

go

<U
t/

Spq

CT3

g 4.^

1— I

u -a
.S2.0

"o

oo

O

q

O

00

oo"
PI

O

M

to

fO

10

'I-

vd

q

10 1
6

Discovered.

ni
C

00
OO

00
00

\o
o-

00

HI

w

0

Ov

M

0

w

<o
0

0

0

1 -a
c
a

i ^

:S O

ja pq

"a
tr

Xi
u

p

■4

1^

u

03
d
ni

tn

.S
)5 4>

4J

u
a

cl'cS .

4) 4> -;

Optical
activity.

d

"tt

"tt

-

-

-.

-

-a

-

in

1.1

in O

u
'tn

-^ 2

0 c

u

03 •>-•

-i= E

0 rt

n

c!j

_>

'1.4

4)

73
PL,

>

■c

"o «■

>

•c

"2 4i

0

'tn 0

d.S

0 rt

0

1 j

0 !

1

o

d
u

•
d

o

d

Is

u

d

d

6
ffi

u

d

to

u

to

^ i

CJ

Nuc-
leus.*

<

<

<

^

<

<

i

u
3

c
1>

E

o
5

3 >

SO ,

■J 'is

e

6

c

'e

.ft C

c

c

'i

o
"3

a

N

1
a

0

"c

.2

c
c

<i

0

c .

"c

>

0.

0

.5 a

0

0

>^^

°|
^ T3 .

i. u "5
^ >. (J

gva;3
0

^^

?o •

^ >— < rt
ft ^ tj

■^ E c
>^

•-"I

K

PROTEINS

69

i-s

1.1

S '«

0 2

■:; a.

T3

b

11

>•

oS

Xi

c

o3

c

g

XI

3

a

0

2 -5
o rt !:;

■5 pa

M

t^

-2 5

«

a

3
o

O

C

U

6^

N3

T3

C

rt.-
u

uP3

o

o u

<U "tn 0*

a o 5

3 *- C

CO O o

en O

2: «

§2

■^ S

o °

•- O u-

^ c -^

u

o
ed
II

lu

u

"r ■>..y 5

-*! I

c
o

s

o

Is

=? u

3

0-3
' n .

^ ^ C

■3 >

1:^

>,-a

a a.

to

u — '

a c rt

3

1 o

.S.5

yo PHYSIOLOGICAL CHEMISTRY

invariably acids, as has already been mentioned, and contain an NH2
group in the a position. This relation of the NHo group to the acid radi-
cal is constant, no matter what other groups or radicals are present. We
may have straight chains as in alanine and glutamic acid, the benzene
ring as in phenylalanine, or we may have sulphurized bodies as in cystine
and still the formula is always of the same type, i.e.,

NH2

R— CH— COOH

•

It is seen that this characteristic grouping in the amino acid provides
each one of these ultimate fragments of the protein molecule with both a
strong acid and a strong basic group. For this reason it is theoretically
possible for a large number of these amino acids to combine and the re-
sulting combinations may be very great in number, since there is such
a varied assortment of the acids. The protein molecule, which is of
such mammoth proportions, is probably constructed on a foundation of
this sort. Much valuable data have been collected regarding the syn-
thetic production of protein substances, the leaders in this line of in-
vestigation being Fischer and Abderhalden. After having gathered a
mass of data regarding the final products of the protein decomposition
and demonstrating that amino acids were the ultimate results of the
various forms of decomposition, these investigators, and notably
Fischer, set about in an effort to form, from these amino acids, by
synthetic means, substances which should possess protein character-
istics. The simplest of these bodies formed in this way was synthesized
from two molecules of glycocoll with the liberation of water, thus:

CH2-(NH2)-CO OH H HN-CH2-COOH.

The body thus formed is a dipeptide, called glycyl-glycine. In an analo-
gous manner may be produced leucyl-leucine, through the synthesis of
two molecules of leucine or leucyl-alanyl-glycine through the union of one
molecule of leucine, one of alanine, and one of glycocoll. By this pro-
cedure Fischer and his pupils have been able to make a large number of
peptides containing varied numbers of amino acid radicals, the name
polypeptides being given to the whole group of synthetic substances thus
formed. One of the most complex polypeptides yet produced is one
containing fifteen glycocoll and three leucine residues.

Notwithstanding the fact that most synthetic polypeptides are pro-
duced through a union of amino acids by means of their imide bonds, it
must not be imagined that the protein molecule is constructed from

PROTEINS 7 1

amino acids linked together in straight chains in a manner analogous to
the formation of simple peptides, such as glycyl-glycine. The molecular
structure of the proteins is much too complex to be explained upon any
such simple formation as that. There must be a variety of linkings,
since there is a varied assortment of decomposition products of totally
different structure.

]\Iany of these synthetic bodies respond to the biuret test, are pre-
cipitated by phosphotungstic acid, and behave, in other ways, as to
leave no doubt as to their protein characteristics. For instance, a
number of amino acids each possessing a sweet taste have been syn-
thesized in such a manner as to yield a polypeptide of bitter taste, a
well-known characteristic of peptones. From the fact that the poly-
peptides formed in the manner indicated have free acidic and basic
radicals we gather the explanation of the amphoteric character of true
proteins.

For the benefit of those especially interested in such matters a photo-
graph of the Fischer apparatus (Fig. 24, page 75) used in the fractional
distillation, in vacuo, of the esters of the decomposition products of the
proteins, as well as micro-photographs and drawings of preparations of
several of these decomposition products (Figs. 21 to 33, pages 72 to 84)
are introduced. For the preparations and the photograph of the appa-
ratus the author is indebted to Dr. T. B. Osborne, of New Haven, Conn.,
who has made many important observations upon the hydrolysis of
proteins. The reproduction of the crystalline form of some of the more
recent of the products may be of interest to those viewing the field of
physiological chemistry from other than the student's aspect.

An extended discussion of the various decomposition products being
out of place in a book of this character, we will simply make a few general
statements in connection with the primary decomposition products.

DISCUSSION OF THE PRODUCTS

Ammonia, XH3. — Ammonia is an important decomposition product
of all proteins and probably arises from an amide group combined
with a carboxyl group of some of the amino acids. It is possible that the
dibasic acids, aspartic and glutamic, furnish most of these carboxyl
groups. This is indicated by the more or less close relationship which
exists between the amount of ammonia and that of the dibasic acids
which the several proteins yield upon decomposition. The elimination
of the ammonia from proteins under the action of acids and alkaUs is
very similar to that from amides like asparagine.

Glycocoll, CH2-(XH2)-COOH.— Glycocoll, or amino acetic acid, is

72 PHYSIOLOGICAL CHEMISTRY

the simplest of the amino acids which occurs as a protein decomposition
product^ and has the following formula:

NH2
H— C— COOH.

H

Glycocoll, as the formula shows, contains no asymmetric carbon atom,
and is the only amino acid yielded by protein decomposition which is
optically inactive. Glycocoll and leucine were among the first decom-
position products of proteins to be discovered. Upon administering
benzoic acid to man or lower animals the output of hippuric acid in the

Fig. 21. — ^Glycocoll Ester Hydrochloride.

urine is greatly increased, thus showing a synthesis of benzoic acid and
glycocoll in the organism (see page 585, Chapter XXVII). Glycocoll,
ingested in small amount, is excreted in the urine as urea, whereas if
administered in excess it appears in part unchanged in the urine. It is
usually separated from the mixture of protein decomposition products
as the hydrochloride of the ester. The crystalHne form of this com-
pound is shown in Fig. 21.

Alanine, CH3-CH(NH2)-COOH.-^Alanine is a-amino-propionic acid,
and as such it may be represented structurally as follows:

H NH2
H— C— C— COOH.
H H

^ Amino formic acid (carbamic acid), NH2COOH, is the simplest amino acid.

PROTEINS

73

Obtained from protein substances, alanine is dextro-rotatory, is very
soluble in water, and possesses a sweet taste. Tyrosine, phenylalanine,
cystine, and serine are derivatives of alanine. This amino acid has been
obtained from nearly all proteins examined. Its absence from those
proteins from which it has not been obtained has not been proven.
Most proteins yield relatively small amounts of alanine.

Serine, CH2(OH)CH(NH2)-COOH. — Serine is a-amino-^-hydroxy-
propionic acid and possesses the following structural formula:

OHNH2
H— C— C— COOH.

H H

Serine obtained from proteins is levo-rotatory, possesses a sweet taste,
and is quite soluble in water. Serine is not obtained in quantity from

Fig. 22. — Serine.

most proteins, but is yielded abundantly by silk glue. Owing to the

diflSculty of separating serine it has not been found in a number of

proteins in which it probably occurs. Serine crystals are shown in Fig.

22.

Phenylalanine, C6H6CH2-CH(NHo) COOH.— This product is ^-

phenyl-a-amino-propionic acid, and may be represented graphically as

follows :

H NH2

I I
C— C— COOH.

H H

74

PHYSIOLOGICAL CHEMISTRY

The levo-rotatory form is obtained from proteins. Phenylalanine has
been obtained from all the proteins examined except from the pro-
tamines and some of the albuminoids. The yield of this body from the
decomposition of proteins is frequently greater than the yield of tyrosine.
The crystalline form of phenylalanine is shown in Fig. 23.

Tyrosine, C6H5(.OH)CH2CH(NH2)COOH.— Tyrosine, one of the
first discovered end-products of protein decomposition, is the amino
acid, p-hydroxy-^-phenyl-a-amino-propionic acid or hydroxy phenylala-
nine. It has the following formula:

H NH2

C— C— COOH.

H H

OH

The tyrosine which results from protein decomposition is usually levo-
rotatory. Tyrosine is one of the end-products of tryptic digestion and
usually separates in conspicuous amount early in the process of diges-

FiG. 23. — Phenylalanine.

tion. It does not occur, however, as an end-product of the decomposi-
tion of gelatin.

Tyrosine is found in old cheese, and derives its name from this fact.
It crystallizes in tufts, sheaves, or balls of fine needles, which decompose
at 295°C. and are sparingly soluble in cold (1-2454) water, but much
more so in boiling (1-154) water. Tyrosine forms soluble salts with
alkalis, ammonia, or mineral acids, and is soluble with difficulty in
acetic acid. It responds to Millon's reaction, thus showing the presence

PROTEINS

75

of the hydroxyphenyl group, but gives no other protein test. The aro-
matic groups present in tyrosine, phenylalanine, and tryptophane cause
proteins to yield a positive xanthoproteic reaction. In severe cases of
typhoid fever and smallpox, in acute yellow atrophy of the liver, and in

Fig. 24. — Fischer Apparatus.

Reproduced from a photograph made by Prof. E. T. Reichert, of the University of Penn-
sylvania. The negative was furnished by Dr. T. B. Osborne, of New Haven, Conn.

A, Tank into which freezing mixture is pumped and from which it flows through the
condenser, B; C, flask from which the esters are distilled, the distillate being collected in D;
E, a Dewar flask containing liquid air serving as a cooler for condensing tube F; G and G',
tubes leading to the Geryck pump by which the vacuum is maintained; /, tube leading to a
McLeod gauge (not shown in figure); J, a bath containing freezing mixture in which the
receiver I) is immersed; A', a bath of water during the first part of the distillation and of
oil during the last part of the process; 1-5, stop cocks which permit the cutting out of
different parts of the apparatus as the procedure demands.

acute phosphorus poisoning, tyrosine has been found in the urine.
Tyrosine crystals are shown in Fig. 25, page 76.

Cystine, C6Hio04NoS2.^Friedmann has shown cystine to be
a-diamino-^-dithiolactyl acid and to possess the following structural
formula :

76

PHYSIOLOGICAL CHEMISTRY

CH2 ■ S — S • CH2

I I

CHNH2 CHNH,.

I I

COOH COOH

Fig. 25. — Tyrosine.

Cystine is the principal sulphur-containing body obtained from the
decomposition of protein substances. It is obtained in greatest amount
as a decomposition product of keratin-containing tissues as horn, hoof,

Fig. 26. — Cystine.

and hair. Cystine occurs in small amount in normal urine and is
greatly increased in quantity under certain pathological conditions. It
crystallizes in thin, colorless, hexagonal plates which are shown in Fig.

PROTEINS 77

26. Cystine is very slightly soluble in water but its salts, with both
bases and acids, are readily soluble in water. It is levo-rotator}- .

It was formerly claimed that cystine occurred in two forms, i.e.^
stone-cysdne and protein-cystine, and that these two forms are distinct
in their properties. This view is incorrect.

For the preparation of cystine from wool or hair see page 87.

For a discussion of cystine sediments in urine see Chapter XXIV.

Tryptophane, C8H6N-CH2CH(NH2)-COOH.— Recently Ellinger
and Flamand have shown that tryptophane possesses the following
formula :

CCH2CH(NH2)COOH

It is therefore ^-indol-a-amino-propionic acid. Tyrophane is the
mot Jier-subs lance of indole, skatole, skatole acetic acid and skatole carhoxylic
acid, all of which are formed as secondary decomposition products of
proteins (see Chapter XIII on Putrefaction Products). Its presence
in protein substances may be shown by means of the Hopkins-Cole
reaction (see page 98) . It may be detected in a tryptic digestion mix-
ture through its property of giving a \dolet color reaction with bromine
water. ^ Tryptophane is \delded by nearly all proteins, but has been
shown to be entirely absent from zein, the prolamin (alcohol-soluble pro-
tein) of maize and also from gelatin.

According to Osborne and jMendel,^ tryptophane is present in maxi-
mum amount in lactalhumin. Upon being heated to 285°C. trytophane
decomposes with the evolution of gas.

Histidine, C3H3N2-CH2-CH(XH2)-COOH.— Histidine is a-amino-

.^-imidazol-propionic acid or ^-imidazol-alaniuc with the following

structural formula:

H NH2

1 I
HC C— C— C— COOH.

I I
H H
HN N

\/
CH

The histidine obtained from proteins is levo-rotatory. It has been
obtained from all the proteins thus far examined, the majority of them
3'ielding about 2.5 per cent of the amino acid. However, about 11 per

^ Kurajeff: Zeit. physiol. Client., 36, 501, 1898-99.

* Osborne and Mendel: Joitr. Biol. Chem., 20, 357, 1915.

78 PHYSIOLOGICAL CHEMISTRY

cent was obtained by Abderhalden from globin, the protein constituent
of oxyhemoglobin, and about 13 per cent by Kossel and Kutscher from
the protamine stiirine.

Crystals of histidine dichloride are shown in Fig. 27.

Knoop's Color Reaction for Histidine. — To an aqueous solution of histidine
or a histidine salt in a test-tube add a little bromine water. A yellow coloration
develops in the cold and upon further addition of bromine water becomes perma-
nent. If the tube be heated/ the color will disappear and will shortly be re-
placed by a faint red coloration which gradually passes into a deep wine red.
Usually black, amorphous particles separate out and the solution becomes
turbid.

The reaction cannot be obtained in solutions containing free alkali.
It is best to use such an amount of bromine as will produce a permanent

■V C^

Fig. 27. — Histidine Dichloride.

yellow color in the cold. The use of a less amount of bromine than this
produces a weak coloration, whereas an excess of bromine prevents the
reaction. The test is not very delicate, but a characteristic reaction
may always be obtained in i : 1000 solutions. The only histidine de-
rivative which yields a similar coloration is imidazolethylamine, and
the reaction in this case is rather weak as compared with the color ob-
tained with histidine or histidine salts.

Valine, C5H11NO2. — The amino-valerianic acid obtained from
proteins is a-amino-isovalerianic acid, and as such bears the following
formula :

CH3 NH2

H— C C— COOH.

CH3 H

^ The same reaction will take place in the cold more slowly.

PROTEINS 79

It closely resembles leucine in many of its properties, but is more soluble
in water. It is a difficult matter to identify valine in the presence of
leucine and isoleucine inasmuch as these amino acids crystallize together
in such a way that the combination persists even after repeated recrys-
tallizations. Valine is dextro-rotatory.

Arginine, C6H14N4O2. — Arginine is 8-guanidine-a-amino-valerianic
acid and possesses the following structural formula :

H H H NH2
NH— C— C— C— C— COOH.
NH=C H H H H

NH2

It has been obtained from every protein so far subjected to decomposi-
tion. The arginine obtained from proteins is dextro-rotatory, and has
pronounced basic properties, reacts strongly alkaline toHtmus, and forms
stable carbonates. Because of these facts, Kossel considers arginine to
be the nucleus of the protein molecule. It is obtained in widely different
amounts from different proteins, over 85 per cent of certain protamines
having been obtained in the form of this amino acid. It is claimed that
in the ordinary metabolic activities of the animal body arginine gives
rise to urea. \Miile this claim is probably true, it should, at the same
time, be borne in mind that the greater part of the protein nitrogen is
eliminated as urea and that, therefore, but a very small part can arise
from arginine.

Leucine, CeHisNOa. — Leucine is an abundant end-product of the
decomposition of protein material, and was one of the first of these
products to be discovered. It is a-amino-isohulyl-acetic acid, and
therefore has the following formula:

CH3 NH2

I 1

H— CCH2C— COOH.

I 1

CH3 H

The leucine which results from protein decomposition is /-leucine.
Leucine is present normally in the pancreas, thymus, thyroid, spleen,
brain, liver, kidneys, and salivary glands. It has been found patliolog-
ically in the urine (in acute yellow atrophy of the liver, in acute phos-
phorus poisoning, and in severe cases of typhoid fever and smallpox),
and in the liver, blood, and pus.

Pure leucine crystallizes in thin, white, hexagonal plates. Crystals

8o

PHYSIOLOGICAL CHEMISTRY

of pure leucine are reproduced in Fig. 28. It is rather easily soluble in
water (46 parts), alkalis, ammonia, and acids. On rapid heating to
295°C., leucine decomposes with the formation of carbon dioxide, ammo-
nia, and amylamine. Aqueous solutions of leucine obtained from pro-
teins are levo-rotatory, but its acid or alkaline solutions are dextro-
rotatory. So-called impure leucine^ is a slightly refractive substance,
which generally crystallizes in balls having a radial structure, or in
aggregations of spherical bodies. Fig. 139, Chapter XXIV.

Isoleucine, C6H13NO2. — Isoleucine is a-amino-^-methyl-^-ethyl-pro-
■pionic acid, and possesses the following structural formula*

CH3 NHo

H— C

C— COOH.

C2H5 H

Fig. 28. — Leucine.

This amino acid was discovered by Ehrlich in 1903. Its presence has
been established among the decomposition products of only a few pro-
teins, although it probably occurs among those of many or most of them.
Ehrlich has shown that the J-amyl alcohol which is produced by yeast
fermentation originates from isoleucine and the isoamylalcohol origi-
nates from leucine. Isoleucine is dextro-rotatory.

Lysine, CH2 (NH2) ■ CH2 • CH2 • CH2 • CH (NH2) • COOH.— The three
bodies, lysine, arginine, and histidine, are frequently classed together
as the hexone bases. Lysine was the first of the bases discovered. It
is a-e-diammo-caproic acid and hence possesses the following structure :

^ These balls of so-called impure leucine do contain considerable leucine, but inasmuch
as they may contain many other things it is a bad practice to allude to them as leucine.

PROTEINS

NH2H H H XHo
H— C— C— C— C— C— COOH
H H H H H

81

Fig. 29. — ^Lysine Picrate.

It is dextro-rotatory and is found in relatively large amount in casein
and gelatin. Lysine is obtained from nearly all proteins, but is absent
from the vegetable proteins which are soluble in strong alcohol. It is

Fig. 30. — AsPARTic Acid.

the mother-substance of cadaverin and has never been obtained in
crystalline form. Lysine is usually obtained as the picrate which is
sparingly soluble in water and crystallizes readily. These crystals are
shown in Fig. 29.
6

82 PHYSIOLOGICAL CHEMISTRY

Aspartic Acid, C4H7NO4. — Aspartic acid is amino-succinic acid and
has the following structural formula:

NH2
H— CCOOH .

H— CCOOH.

I
H

The amide of aspartic acid, asparagine, is very widely distributed
in the vegetable kingdom. Asparagine has the following formula.

NH2

H— CCOOH

I

H— CC0(NH2).

H

The crystalline form of aspartic acid is exhibited in Fig. 30.

Aspartic acid has been found among the decomposition products of
all the proteins examined, except the protamines. It has not been ob-
tained, however, in very large proportion from any of them. The
aspartic acid obtained from protein is levo-rotatory.

Glutamic Acid, C5H9NO4. — This acid is a-amino-normal-glutaric
acid and as such bears the following graphic formula:

NH2

I
H— CCOOH

H— C— H

I
H— CCOOH.

H

Glutamic acid is yielded by all the proteins thus far examined,
except the protamines, and by most of these in larger amount than
any other of their decomposition products. It is yielded in especially
large proportion by most of the proteins of seeds, 43.66 per cent having
been obtained by Osborne and Guest ^ by the hydrolysis of gliadin, the
prolamin of wheat. This is the largest amount of any single decompo-
sition product yet obtained from any protein except the protamines.

^ Osborne and Guest: Jour. Biol. Chcm. 9, 425, 191 1.

PROTEINS

83

Glutamic acid and aspartic acid arc the only dibasic acids which
have thus far been obtained as decomposition products of proteins. As
there is an apparent relation between the proportion of these acids
and that of ammonia which the different proteins yield it is possible
that one of the carboxyl groups of these acids is united with XHo as
an amide, the other carboxyl group being united in polypeptide union
(see page 32) with some other amino acid. This might be represented
by the following formula:

R— CHNH— COOH

/

CO— CHNHo— CH2— CH2— COXH.2.

It has been shown by Thierfelder and Sherwin^ that the amide,
glutamine, is a product of normal metabolism and hence this substance
rather than glutamic acid is present in the protein molecule.

Fig. 31. — Glutamic Acid.

Reproduced from a micro-photograph made by Prof. E. T. Reichert, of the University

of Pennsylvania.

The glutamic acid, yielded by proteins upon hydrolysis, is dextro-
rotatory. Crystals of glutamic acid are reproduced in Fig. 31.

Proline, C5H9XO2. — Proline is a-pyrro\idinc-carhoxyUc acid and
possesses the following graphic structure:

H2C CH2

HoC

CHCnOH.

NH

Proline was llrst obtained as a decomposition product of casein. Pro-
* Thierfelder and Sherwin: Zeil. Physiol. Chcmic, 94, 1, 1915.

84

PHYSIOLOGICAL CHEMISTRY

line obtained from proteins is levo-rotatory and is the only protein de-
composition product which is readily soluble in alcohol. It is also one of
the few heterocyclic compounds obtained from proteins. Proline has
been found among the decomposition products of all proteins except the

Fig. 32. — LEVo-a-PROLiNE.

protamines. The maximum yield reported is 13.73 P^^ cent obtained
by Osborne and Clapp from the hydrolysis of hordein. Fischer and
Boehner^ have obtained 7.7 per cent from the hydrolysis of gelatin.

Fig. ^s. — Copper Salt of Proline.
Reproduced from a micro-photograph made by Prof. E. T. Reichert, of the University of

Pennsylvania.

The crystalline form of levo-a-proline is shown in Fig. 32 and the
copper salt of prohne is represented by a micro-photograph in Fig. 7,2).
The crystals of the copper salt have a deep blue color, but when they
^ Fischer and Boehner: Zeit. phys. chem., 65, 118, 1910.

PROTEINS 85

lose their water of crystallization they assume a characteristic violet
color.

Oxyproline, C5H9NO3. — Oxyproline was discovered by Fischer.
It has as yet been obtained from only a few proteins, but this may be
due to the fact that only a few have been examined for its presence.
The position of the hydroxyl group has not yet been established.

Diaminotrihydroxydodecanoic Acid, C12H26N2O6. — This amino acid
was discovered by Fischer and Abderhalden as a product of the hydro-
lysis of casein. It has thus far been obtained from no other source.
It is levo-rotatory and its constitution has not been determined.

Experiments

Protein Decomposition. — While the ordinary courses in physiological
chemistry preclude any extended study of the decomposition products
of proteins, the manipulation of a simple decomposition and the sub-
sequent isolation and study of a few of the products most easily and
quickly obtained will not be without interest.^ To this end the student
may use the following decomposition procedure.

Treat the protein (coagulated egg albumin) in a large flask with water con-
taining 3-5 per cent of H2SO4 and place it on a water-bath until the protein ma-
terial has been decomposed and there remains a fine, fluffy, insoluble residue.
Filter off this residue and neutralize the filtrate with Ba(0H)2 and BaCOs*
Filter off the precipitate of BaS04 which forms and when certain that the fluid is
neutral or faintly acid,- concentrate (first on a wire gauze and later on a water-
bath) to a syrup. This syrup contains the end-products of the decomposition of
the protein, among which are proteoses, peptones, tyrosine, leucine, etc. Add
95 per cent alcohol slowly to the warm syrup until no more precipitate forms,
stirring continuously with a glass rod. This precipitate consists of proteoses and
peptones. Gather the sticky precipitate on the rod or the sides of the dish and,
after warming the solution gently for a few moments, filter it through a filter
paper which has not been previously moistened. After dissolving the precipi-
tate of proteoses and peptones in water^ the solution may be treated according to
the method of separation given on page 120.

The leucine and tyrosine, etc., are in solution in the warm alcoholic filtrate.
Concentrate this filtrate on the water-bath to a thin syrup, transfer it to a beaker,
and allow it to stand over night in a cool place for crystaUization. The tyrosine
first crystallizes (Fig. 25, page 76), followed later by the formation of characteristic

1 The procedure here set forth has nothing in common with the procedure by means
of which the long line of decomposition products just enumerated are obtained. This
latter process is an exceedingly comphcated one which is entirely outside the province of
any course in physiological chemistry.

^ If the solution is alkaline in reaction at this point, the amino acids will be broken
down and ammonia will be evolved.

' At this point the aqueous solution of the proteoses and peptones may be filtered to
remove any BaS04 which may still remain. Tyrosine crystals will also be found here,
since it is less soluble than the leucine and may adhere to the proteose-peptone precipitate.
Add the crystals of tyrosine to the warm alcohol filtrate.

86 PHYSIOLOGICAL CHEMISTRY

crystals of impure leucine (see Fig. 139, Chapter XXIV). After examining these
crystals under the microscope, strain ofif the crystalline material through fine
muslin, heat it gently in a little water to dissolve the leucine (the tyrosine will be
practically insoluble) and filter. Concentrate the filtrate and allow it to stand in a
cool place over night for the crude leucine to crystallize. Filter off the crystals
and use them in the tests for leucine given on page 87. The crystals of tyrosine
remaining on the paper from the first filtration may be used in the tests for tyro-
sine as given below. If desired, the tyrosine and leucine may be purified by
recrystallizing in the usual manner. Habermann has suggested a method of
separating leucine and tyrosine by means of glacial acetic acid.

Experiments on Tyrosine

Make the following tests with the tyrosine crystals prepared in
the above experiments, or upon those obtained during the preparation
of cystine (see page 87), or upon some pure tyrosine furnished by the
instructor.

1. Microscopical Examination. — Place a minute crystal of tyrosine on a slide,
add a drop of water, cover with a cover-glass, and examine microscopically.
Now run more water under the cover-glass and warm in a Bunsen flame until the
tyrosine has dissolved. Allow the solution to cool slowly, then examine again
microscopically, and compare the crystals with those shown in Fig. 25, page 76.

2. Solubility. — Try the solubility of very small amounts of tyrosine in cold and
hot water, cold and hot 95 per cent alcohol, dilute NH4OH, dilute KOH and dilute
HCl.

3. Sublimation. — Place a little tyrosine in a dry test-tube, heat gently and
notice that the material does not sublime. How does this compare with the
result of Experiment 3 under Leucine?

4. Hoffman's Reaction. — This is the name given to Millon's reaction when
employed to detect tyrosine. Add about 3 c.c. of water and a few drops of Mil-
lon's reagent to a little tyrosine in a test-tube. Upon dissolving the tyrosine by
heat the solution gradually darkens and may assume a dark red color. What
group does this test show to be present in tyrosine?

5. Sulphuric Acid Test (Piria). — Warm a little tyrosine on a watch glass on a
boiling water-bath for 20 minutes with 3-5 drops of cone. H2SO4. Tyrosine-
sulphuric acid is formed in the process. Cool the solution and wash it into a
small beaker with water. Now add CaCOs in substance slowly with stirring,
until the reaction of the solution is no longer acid. Filter, concentrate the
filtrate, and add it to a few drops (avoid an excess) of very dilute neutral ferric
chloride. A purple or violet color, due to the formation of the ferric salt of
tyrosine-sulphuric acid, is produced. This is one of the most satisfactory tests
for the identification of tyrosine.

6. Formaldehyde -Sulphuric Acid Test (Momer). — ^Add about 3 c.c. of
M timer's reagent' to a little tyrosine in a test-tube, and gently raise the tempera-
ture to the boiling-point. A green color results.

^ Morner's reagent is prepared by thoroughly mixing i volume of formalin, 45 volumes
of distilled water, and 55 volumes of concentrated sulphuric acid.

PROTEINS 87

7. Folin and Denis's Test.'^ — To 12 c.c. of the solution to be tested add an
equal volume of a special reagent (containing 10 per cent sodium tungstate, 2
per cent phosphomolybdic acid and 10 per cent phosphoric acid) and 3-10 c.c.
of a saturated solution of sodium carbonate. A blue color indicates tyrosine.
It is said to detect i part in one million.

Abderhalden- claims the reagent also reacts with tryptophane,
oxytryptophane and /-oxyproline.

Experiments on Leucine

Make the following tests upon the leucine crystals already prepared
or upon some pure leucine furnished by the instructor.

I, 2 and 3. Repeat these experiments according to the directions given
under Tyrosine (pages 86 and 87 j.

Preparation of Cystine^

From 50 to 500 grams of wool or hair is pushed into a (Jena) flask and con-
centrated hydrochloric acid (200 c.c. to each 100 grams of wool) is added. In
order to get a part of the acid quickly to the bottom of the flask a part of the acid
may be put in first, then the wool, and finally the remaining acid. A condenser
consisting only of a glass tube 2 to 3 ft. long is inserted and the mixture is boiled
until the biuret reaction is entirely negative. The wool dissolves in a few min-
utes and if much cystine is desired more wool and acid can then be introduced.
After three to five hours' boiling with moderate quantities of wool the biuret
reaction has usually disappeared.

To the hot acid solution of amino acids so obtained is added at once an excess
of solid sodium acetate, i.e., until the Congo red reaction for mineral acids is
entirely negative. A dark, heavy precipitate containing practically all the cystine
is obtained. After a few hours' standing at room temperature the liquid is filtered
off and the precipitate is washed with cold water. (From the mother liquor
diluted with the wash water is usually obtained on long standing a second pre-
cipitate consisting chiefly of tyrosine.)

The crude cystine is then dissolved in boiUng 3-5 per cent hydrochloric acid
and the solution is decolorized with good boneblack which should have been
previously thoroughly digested with hot, dilute hydrochloric acid and then washed
with water in order to remove the calcium phosphate. The hot filtrate from the
boneblack should be as clear as water. If it is not perfectly colorless the bone-
black treatment should be repeated and if a colorless solution is not then ob-
tained the fault lies with the quaUty of the boneblack. The last filtrate is heated
to boiUng and the cystine precipitated by a slow addition of concentrated hot
sodium acetate solution.

Large amounts of colorless cystine consisting of tjrpical hexagonal plates can
thus be prepared without difficulty and with very little labor. Compare the
microscopical appearance of these crystals with those shown in Fig. 26, page 76.

' Folin and Denis: Jour. Biol. C/icm., 12, 245, IQ12.
* Abderhalden: Zeit. Physiol. CItem., 85, 91, 1913.
' Folin: Jour. Biol. Cliem., 8, 9, 1910.

PHYSIOLOGICAL CHEMISTRY

THE QUANTITATIVE DETERMINATION OF ALIPHATIC
AMINO GROUPS

Method of Van Slyke.^ — Principle. — This method for the determination of
ahphatic amino nitrogen is based on the measurement of the nitrogen gas evolved
in the reaction,

RNH2+HN02 = ROH+N2+HoO.

During the process the following reaction also takes place, the nitrous acid solution
decomposing spontaneously with the formation of nitric oxide,

2HN02 = HN03+NO.

Fig. 34.

-Van Slyke Amino Nitrogen
Apparatus.

Fig. 35. — Section of Van Slyke
Apparatus.

This latter reaction is utiUzed in displacing all the air of the apparatus with nitric
oxide. The amino solution is then introduced, evolution of nitrogen mixed with
nitric oxide resulting. The oxide is absorbed with alkaline permanganate solution
and the pure nitrogen measured in a special gas burette shown in the figure.
Procedure. — The determination is carried out in three stages:
I. Displacement of Air by Nitric Oxide. — Water f rom F (see Figs. 34 and 35),
fills the capillary leading to the Hempel pipette and also the other capillary
as far as c. Into A one pours a volume of glacial acetic acid sufficient to fill

^ Van Slyke: Jour. Biol. Chem., 12, 275, 1912; 61, 121 and 125, 1913.

PROTEINS 89

one-fifth of D. For convenience, A is etched with a mark to measure this amount. .
The acid is run into D cock c being turned so as to let the air escape from D.
Through A one now pours sodium nitrite solution (30 grams NaNOa to 100 c.c.
H2O) until D is full of solution and enough excess is present to rise a little above
the cock into A. It is convenient to mark A for measuring off this amount also.
The gas exit from D is now closed at c, and, a being open, D is shaken for a few
seconds. The nitric oxide, which instantly collects, is let out at c, and the shaking
repeated. The second crop of nitric oxide which washes out the last portions of air,
is also let out at c. D is now connected with the motor and shaken till all but 20 c.c.
of the solution have been displaced by nitric oxide and driven back into A . A naark
on D indicates the 20 c.c. point. One then closes a and turns c and /so that D and
F are connected. The above manipulations require between one and two minutes.

2. Decomposition of the Amino Substance. — Of the amino solution to be analyzed
10 c.c. or less, as the case may be, are measured off in B. Any excess added above
the mark can be run off through the outflow tube. The desired amount is then run
into D, which is already connected with the motor, as shown in Fig. 34. It
is shaken when a-amino acids are being analyzed for a period of three to five
minutes. With a-amino acids, proteins or partially or completely hydrolyzed
proteins, we find that at the most five minutes vigorous shaking completes the
reaction. Only in the case of some native proteins which, when deaminized form
unwieldy coagula that mechanically interfere with the thorough agitation of the
mixture, a longer time may be required. In case a viscous solution is being analyzed
and the liquid threatens to foam over into F, B is rinsed out and a little caprylic
alcohol is added through it. For amino substances such as amino purins, requiring
a longer time than five minutes to react, one merely mixes the reacting solutions
and lets them stand the required length of time, then shakes about two minutes to
drive the nitrogen completely out of solution.

When it is known that the solution to be analyzed is likely to foam violently,
it is advisable to add caprylic alcohol through B before the amino solution. B is
then rinsed with alcohol and dried with ether or a roll of filter paper before it
receives the amino solution.

3. Absorption of Nitric Oxide and Measurement of Nitrogen. — The reaction being
completed, all the gas in D is displaced into F by liquid from A and the mixture of
nitrogen and nitric oxide is driven from F into the absorption pipette.^ The driving
rod is then connected with the pipette by lifting the hook from the shoulder of d and
placing the other hook, on the opposite side of the driving rod, over the horizontal
lower tube of the pipette. The latter is then shaken by the motor for a minute,
which, with any but almost completely exhausted permanganate solutions, com-
pletes the absorption of nitric oxide. The pure nitrogen is then measured in F.
During the above operations a is left open, to permit displacement of liquid from D
as nitric oxide forms in D.

Blank determinations, performed as above except that 10 c.c. of distilled water
replaces the solution of amino substance, must be performed on every fresh lot
of nitrite used. Nitrite giving a much larger correction than 0.3 to 0.4 c.c. should
be rejected.

The room temperature and the barometric pressure must be noted. The

*The solution in the absorption pipette is 40 grams KMNO4 and 25 grams KOH in a
liter.

90

PHYSIOLOGICAL CHEMISTRY

MILLIGRAMS OF AMINO NITROGEN CORRESPONDING TO i C.C. OF NITRO-
GEN GAS AT ii°-3o°C.; 728-772 MM. PRESSURE

13°
14°
15°

728

732

734

736 I 738

0.s68o|o.s69S O.SSio 0.5725

0.565s 0.56700.5685 0.S700

o". 5630 o . 5645 o . 5660 o. 567s

0.5605 0.56200.5635 0.5650I0. 5665 0.5680

0.55800.5595,0.5610 0.5625^0. s640|0. 5655

0.574SI0.5760I0.5775

0.5720 0.5735 0.5750

0.5695 0.57100.5725

0.5700

0.5670

0.S790
0.5765
0.5740

744

0.5805
0.5780
0.5755

0.5715 0.5730

746

748

750

0.5685 0.570s 0.5720b. 5735 !o.S7SO

0.5820 0.5840 0.5855
0.57950.58150.5830
0.5770|o.5785|o.5805
0.5745:0.5760, .05775

13"
14°
is"

16° 0.555s 0.55700.5585 0.56000.5615 0.5630
17° 0.552s|o. 55400. 5555 0.5575J0. 55900. 560s
18° 0.55000.5515 0.55300.55450. 5560 0.5580
19° [0.5475:0.5490 0.5505 6.5520 0.5535 0.5550
o. 5445 0.54600.5475 0.54950. 5510 0.5525

0.5645
0.5620
0.5595

0.5660 0.5675
0.5635:0.5650
0.56100. 562s

0.5690b. 571010.5725
o . 566s o . 56800 . 5695
0.5640 0.5655 0.5670

0.5565 0.5580b. 5595 0.5610 o.5630jO. 5645
0.5540 0.5555 0.55700.5585 0.56000.5615

16"
17°
18°
19°

23°
24°
25°

0.54200.5435
0.53950.5410

0.54500.5465 0.54800.5495 0.55100.5525 0.5540
0. 542510. 5440j0. 5455 0.5470 0.548s 0.5500 o.SSiS
0. 5365^0. 5380b. 53950. 5410,0.5425 0.5440
0.5335 o.S350|0. 5365 0.53800.54000.541510.543010.5445 0.5460
0.5310I0.5325 0.5340 0.5355,0.53700.5385 0.5400 0.5415 0.5430

0.555s 0.5575JO. 5590
o. 5530,0. 554SJO. 5560
0.5500b. 5515 0.5530
o. 5475 ;o.5490|0. 550s
0.5445:0.54600.5475

23

24°

25°

26"

27"

28°

29°

130°

0.52600.5295 0.53100.5325 0.53400.5355
0.5250b. 5265(0. 5280 0.5295 0.53100.532s
0.5220 0.523s o. 5250 0.5265I0. 5280:0. 5295
0.5195 o. 52 lojo. 5220 0.523510.52500.5265
0.5160 0.517s 0.51900.520510.522010.5235

0.5370
0.5340
0.5310
0.5280

0.5365 0.5400
0.5355b. 5370

0.5325 0.5340 0.535s 0.5370
0.5295 0.5310 0.53250. 5340

0.54IS 0.5430 0.544s
0.538510.54000.5415
0.5385

0.5355

0.52500.5265 0.5280 0.5295 0.5310

0.532s

260

2 7"

28°
29"
30°

t

728

730

732

734 736 I 738

740

742

746

748

754 I 7S6

7S8

.5870
■ 584s
.5820
.5790
.5765

o. 5885 |o. 59000.

o. 5860b. 5875 o,

o.s835j0.58sojo,

0.580S 0.582s o,

576510. 57950,

760

5915 o.
5890 o.

58650.
5840:0.
581010.

762

764 766 768

770

5935 O.595O1O
S90S 0.5925 O
58800.5895:0

S8S5
S830

o.5870|0
0.58450

59650.
59400.
5910 o.
5885'o.
,5860 o.

59800.
S9S5|o,
S930JO.
59000,
58750.

599Sb
597o!o
594sjo
59150
5890I0

6010

5985
5960
5935
5905

0.6030
O . 6000
0.597S
O.S9SO
0.5920

772

13"
14°
IS"

5740
S7IO
568s
5660
5630

0.57S5b.S770JO
57300.5745 O
o. 5700b. 5715 O
0.567s 0.5690 O
0.5645 0.5660 o

5785 o.
576o'o.
5730|0.
S705:o,
.56750,

I i

5800b. 58150.

S77SjO.S790 0.
S74s|o.576sjo.
5720|0.5735 O.
569O1O.570S O.

58300.
5805 O,
5780 O.
5750 O.
5725 O.

58500.
5820 O.
579510.
57650.
574oio.

I
5865JO.
S82s'o.
5810J0.
5780 O.
575510.

5880
5850
582s
5795
5770

0.589s
0.586s
0.5840
0.5810
0.578s

16°
17°
18°
19°

23°
24°
25°

0.560s
O.SS7S
O.S545
0.5520
0.S490

0.5620 0.5635 0.56so]o.s665 0.5680,0.5695 0.57IOJO. 5725 |o. 5740
o.5S90io. 5605 0.5620 0.5635 0.5650 0.5665 0.5680(0.5695 0.5715

0.55600.5575 0.5595
0.5535 0.55500.5565
0.5505 0.5520 O.SS3S

0.5610b. 5625 0.5640 0.56ssb.567ob.5685
0.55800.5595 0.56100.5625 0.56400.5655
0.55500.5565 0.558010. 5595(0. 5610 0.5625

0.S7SS
0.5730
0.5700
0.5670
o . 5640

23°
24°
2S°

26°
27°
28°
29°
30»

0.5460
0.5430
0.5400
0.5370
0.5340

0.5475:0.54900.5505 0.55200.5535 0.5550(0.5565 0.55800.5595
0. 544Sb.5460|0. 5475 jo. 5490J0. 5505 0.5520 0.5535(0. 555o|o. 5565
0.5415 0.54300.5445,0.5460,0.5475 0.5490, 0.5505 0.5520

0.538510.5400
0.53550.5370

0.5415
5385

0.543o|o. 5445,0.5460 0.5475 0.5490
0.5400 0.541 5 0.5430 0. 5445 '0.5460

5535
0.550s
5475

0.5610
0.5580
0.5550
0.5520
0.5490

26°
27°
28°
29°
30°

752

754

756

7S8

760

762 I 764

766 I 768

770

772

Journal of Biological Chemistry,
mination of Amino Groups.

12, 27s, 1Q12. Van Slyke: The Quantitative Deter-

PROTEINS 91

calculation of the weight of nitrogen gas corresponding to the volume obtained is
most readily made with the aid of the tables (see page 90) devised for this purpose.^

The Van Slyke Micro-apparatus. ^ — In later work. \an Slyke has used to a large
extent an ai)paratus which differs from the one described above only in being con-
siderabl}- smaller. More accurate measurements can be made with this and
smaller amounts of amino nitrogen determined. In using this only 10 c.c. of
nitrite solution and 2.5 c.c. of acetic acid are required for an analysis. One-fifth
the amount of substance may be analyzed with the same degree of accuracy as
with the larger apparatus. Practically the only alteration from the mode of opera-
tion already detailed above, is in the speeds at which the deaminizing bulb and the
Hempel pipette are shaken. During the first stage of the analysis the deaminizing
bulb should be shaken by the motor at a very high rate of speed, about as fast as
the eye can follow or an unnecessary amount of time is lost in freeing the apparatus
from air. This stage is also much accelerated by warming the nitrite solution to
30° before it is used, in case a low room temperature has reduced the temperature
of the solutions below 20°. In the third stage when the nitric oxide is being ab-
sorbed by the permanganate, the Hempel pipette should be shaken not faster than
twice per second. This is to prevent the breaking off of small gas bubbles.

It is especially necessary that in the first stage the removal of air be complete.
This is assured by shaking the solution in the deaminizing bulb back each time,
in this stage, until the bulb is two-thirds filled w-ith nitric oxide.

For the determination of total and free amino acid nitrogen in the urine by
this method see chapter on Quantitative Analysis of Urine.

ESTIMATION OF AMINO -ACED ^-NITROGEN

Method of Harding and MacLean.' — Principle. — Amino-acid mixtures when
treated with triketohydrindene hydrate give a colored solution which may be com-
pared colorimetrically with a standard.

Procedure. — One c.c. of the solution to be estimated (containing not more than
0.05 mg. of amino-acid a- nitrogen and neutral to phenolphthalein, is mixed with
I c.c. of a ID per cent aqueous solution of pure pyridine and i c.c. of a freshly pre-
pared 2 per cent solution of triketohydrindene hydrate and heated in a rapidly
boiling constant-level water-bath for 20 minutes. At the end of that time the test
tube is removed, cooled and diluted to a suitable volume, usually 100 c.c, but if the
amino-acid a-nitrogen is very small in amount a correspondingly smaller dilution
can be used. The solution is compared with a standard in a Duboscq colorimeter.
The standard solution is prepared by dissolving 0.3178 gm. of pure, freshly crystal-
lized alanine in a liter of distilled water. The solution contains 0.05 mg. of N per
c.c. Treat i c.c. of this standard just as above, except that only i c.c. of trike-
tohydrindene is required. The standard solution is stable for three months.
Amounts of amino nitrogen from 0.005 to 0.05 mg. may be determined. The
method is inaccurate for cystine and has not yet been adapted for use with biolog-
ical fluids other than solutions of protein hydrolysis products.

1 See \'an Slyke: Jour. Biol. Client.. 12, 275, 191 2 or Gatterniann: Pra.\is dcs organis-
clien Cliritiikir.K. ninth edition. In using the tables in the latter work or similar tables it
should be borne in mind that the volume of nitrogen gas must be divided by two, inasmuch
as only one-half of the nitrogen collected comes from the amino groups.

° Either of these apparatus may be obtained from Kmil (ireiner, 45 Cliff Street, New
York, or from Robert Goetze, Leipzig. Van Slyke has recently described a third form of
his apparatus about half of the size of the earlier micro-apparatus. This has a more
accurate burette so that the gas volumes can be read to 0.00 1 c.c. (,\'an Slyke: Jot4r. Biol.
Cheni., 2;^, 407, 1915.)

^Harding and ^lacLean: Jour. Biol. Chem., 20, 217, 1915.

CHAPTER V

PROTEINS: THEIR CLASSIFICATION AND
PROPERTIES

From what has already been said in Chapter IV regarding the
protein substances it will be recognized that the grouping of the diverse
forms of this class of substances in a logical manner is not an easy
task. The fats and carbohydrates may be classified upon the funda-
mental principles of their stereo-chemical relationships, whereas such a
system of classification in the case of the proteins is absolutely im-
possible since, as we have already stated, the molecular structure of
these complex substances is unknown. Because of the diversity of
standpoint from which the proteins may be viewed, relative to their
grouping in the form of a logically classified series, it is obvious that
there is an opportunity for the presentation of classifications of a widely
divergent character. The fact that there were until recent years at
least a dozen different classifications which were recognized by various
groups of English-speaking investigators emphasizes the dififlculties in
the way of the individual or individuals who would offer a classification
which should merit universal adoption. ReaHzing the great handi-
cap and disadvantage which the great diversity of the protein classifi-
cations was forcing upon the workers in this field, the Chemical and
Physiological Societies of England drafted a classification which ap-
pealed to these groups of scientists as fulfilling all requirements and
presented it for the consideration of the American Physiological Society
and the American Society of Biological Chemists. The outcome of
this has been that there are now only two protein classifications which
are recognized by Enghsh-speaking scientists, one the British Classi-
fication, the other the American Classification. These classifications
are very similar and doubtless will ultimately be merged into a single
classification. In our consideration of the proteins we shall conform
in all details to the American Classification. In this connection we
will say, however, that we fell that the English Societies have strong
grounds for preferring the use of the term scleroproteins for albu-
minoids and chromoproteins for hemoglobins. The two classifications
are as follows:

92

PROTEINS 93

CLASSIFICATION OF PROTEINS ADOPTED BY THE AMERI-
CAN PHYSIOLOGICAL SOCIETY AND THE AMERICAN
SOCIETY OF BIOLOGICAL CHEMISTS

I. SIMPLE PROTEINS

Protein substances which yield only a-amino acids or their deriva-
tives on hydrolysis.

{a) Albumins. — Soluble in pure water and coagulable by heat,
e.g., ovalbumin from egg white, serum albumin from blood serum,
lactalbumin from milk, vegetable albumins.

(b) Globulins. — Insoluble in pure water but soluble in neutral
solutions of salts of strong bases with strong acids, ^ e.g., serum globulin,
ovoglobulin from egg yolk, edestin from hemp seed, amandin from almond
and peach kernel, and other vegetable globulins.

(c) Glutelins. — Simple proteins insoluble in all neutral solvents, but
readily soluble in very dilute acids and alkalis,^ ^.g., glutenin from wheat.

(d) Alcohol-soluble Proteins (Prolamins).^ — Simple proteins sol-
uble in 70-So per cent alcohol, insoluble in water, absolute alcohol, and
other neutral solvents,"^ e.g., zein from corn, gliadin from wheat and
rye, hordein from barley, and bynin from malt.

(e) Albiuninoids.— Simple proteins possessing a similar structure to
those already mentioned, but characterized by a pronounced insolubihty
in all neutral solvents,^ e.g., elastin from ligament, collagen from tendon,
keratin from horn and hoof.

(/) Histones. — Soluble in water and insoluble in very dilute ammor
nia, and, in the absence of ammonium salts, insoluble even in excess of
ammonia; yield precipitates with solutions of other proteins and acoagu-
lum on heating which is easily soluble in very dilute acids. On hydroly-
sis they yield a large number of amino acids among which the basic
ones predominate. In short, histones are basic proteins which stand
between protamines and true proteins, e.g., globin from hemoglobin,
scombronc from mackerel sperm, thymus Jrislonc.

ig) Protamines.— Simpler polypeptides than the proteins included
in the preceding groups. They are soluble in water, uncoagulable by

^ The precipitation limits with ammonium sulphate should not be made a basis for dis-
tinguishing the albumins from the globulins.

2 Such substances occur in abundance in the seeds of cereals and doubtless represent a
weU-defined natural group of simple proteins.

' The name proliimins has been suggested for these alcohol-soluble proteins by Dr.
Thomas B. Osborne {Science, 190S, xxviii, p. 417). It is a very fitting term inasmuch as
upon hydrolysis they yield particularly large amounts of proline and ammonia.

* The subclasses defined (a, b, c, d,) are exemplified by proteins obtained from both
plants and animals. The use of appropriate prefixes will sufiice to indicate the origin of
the compounds, e.g., owglobulin, /jiValbuniin, etc.

* These form the principal organic constituents of the skeletal structure of animals and
also their external covering and its appendages. This definition does not provide for
gelatin which is, however, an artificial derivative of collagen.

94 PHYSIOLOGICAL CHEMISTRY

heat, have the property of precipitating aqueous solutions of other pro-
teins, possess strong basic properties and form stable salts with strong
mineral acids. They yield comparatively few amino acids, among
which the basic ones predominate. They are the simplest natural
proteins, e.g., salmine from salmon sperm, sturine from sturgeon sperm,
cln peine irom. herring s per 711, scombrine from mackerel sperm.

II. CONJUGATED PROTEINS

Substances which contain the protein molecule united to some other
molecule or molecules otherwise than as a salt.

(a) Nucleoproteins. — Compounds of one or more protein molecules
with nucleic acid, e.g., cytoglohulin from cytoplasm. niicIcoJiistone from
nucleus.

(b) Glycoproteins. — Compounds of the protein molecule with a
substance or substances containing a carbohydrate group other than a
nucleic acid, e.g., mucins and mucoids {osseomucoid from bone, tendomu-
coid from tendon, ichtlmlin from carp eggs, helico protein from snail).

(c) Phosphoproteins. — Compounds of the protein molecule with
some, as yet undefined, phosphorus-containing substances other than a
nucleic acid or lecithin,^ e.g., casein from milk, ovovitellin from egg
yolk.

(d) Hemoglobins.^ — Compounds of the protein molecule with
hematin, or some similar substance, e.g., hemoglobin from red blood
cells, hemocyanin from blood of invertebrates.

(e) Lecithoproteins. — Compounds of the protein molecule with
lecithins.

III. DERIVED PROTEINS

I. Primary Protein Derivatives

Derivatives of the protein molecule apparently formed through
hydrolytic changes which involve only slight alteration of the protein
molecule.

{a) Proteans. — Insoluble products which apparently result from
the incipient action of water, very dilute acids or enzymes, e.g., myosan
from myosin, edestan from edestin.

(b) Metaproteins. — Products of the further action of acids and alka-
lis whereby the molecule is so far altered as to form products soluble in

^ The accumulated chemical evidence distinctly points to the propriety of classifying
the phosphoproteins as conjugated compounds, i.e., they are possibly esters of some phos-
phoric acid or acids and protein.

PROTEINS 95

very weak acids and alkalis but insoluble in neutral fluids, e.g., acid
metaprotein (acid albnmiuale), alkali mela protein (alkali albuminate).

(c) Coagulated Proteins. — Insoluble products which result from
(i) the action of heat on their solutions, or (2) the action of alcohol on
the protein.

2. Secondary Protein Derivatives^

Products of the further hydrolytic cleavage of the protein molecule.

(0) Proteoses. — Soluble in water, non-coagulable by heat, and
precipitated by saturating their solutions with ammonium — or zinc
sulphate,^ e.g., proto proteose, deutero proteose.

(b) Peptones. — Soluble in water, non-coagulable by heat, but not
precipitated by saturating their solutions with ammonium sulphate,^
e.g., antipcptone, amphopeptone.

(c) Peptides. — Definitely characterized combinations of two or more
amino acids, the carboxyl group of one being united with the amino
group of the other with the elimination of a molecule of water,^ e.g.,
dipeptides , tripeptides, tetrapeptides, penta peptides.

CLASSIFICATION OF PROTEINS ADOPTED BY THE CHEM-
ICAL AND PHYSIOLOGICAL SOCIETIES
OF ENGLAND

I. Simple Proteins
«

1. Protamines, e.g., salmine, clupeine.

2. Histones, e.g., globin, scombrone.

3. Albumins, e.g., ovalbumin, serum albumin, vegetable albumins.

4. Globulins, e.g., serum globulin, ovoglobulin, vegetable globulins.

5. Glutelins, e.g., glutenin.

6. Alcohol-soluble proteins, e.g., zein, gliadin.

7. Scleroproteins, e.g., elastin, keratin.

8. Phosphoproteins, e.g., casein, vitellin.

II. Conjugated Proteins

1. Glucoproteins, e.g., mucins, mucoids.

2. Nucleoproteins, e.g., nucleohistone, cytoglobuUn.

3. Chromoproteins, e.g., hemoglobin, hemocyanin.

^ The term secondary protein derivatives is used because the formation of the primary
derivatives usually precedes the formation of the secondary derivatives.

2 As thus dctinecl, this terna does not strictly cover all the protein derivatives com-
monly called i)roleoses, c.t^., hcteroprt)leose and dysproteose.

^ in this KTouji the kyrines may be included. I-'or the present it is believed that it will
be helpful to retain this term as dciined, reserving the expression peptide for the simpler
compounds of delinite structure, such as dipeptides, etc.

■• The peptones are undoubtedly peptides or mixtures of peptides, the latter term being
at present used to designate those of definite structure.

96 PHYSIOLOGICAL CHEMISTRY

III. Products of Protein Hydrolysis

1. Infraproteins, e.g., acid infraprotein {acid albuminate), alkali
infraprotein {alkali albuminate).

2. Proteoses, e.g., protoproteose, hetero proteose, deutero proteose.

3. Peptones, e.g., amphopeptone, antipeptone.

4. Polypeptides, e.g., dipeptides, tripeptides, tetrapeptides.

CONSIDERATIONS OF THE VARIOUS CLASSES
OF PROTEINS

SIMPLE PROTEINS

The simple proteins are true protein substances which, upon hy-
drolysis, yield only a-amino acids or their derivatives. "Although
no means are at present available whereby the chemical individuality of
any protein can be established, a number of simple proteins have been
isolated from animal and vegetable tissues which have been so well
characterized by constancy of ultimate composition and uniformity of
physical properties that they may be treated as chemical individuals
until further knowledge makes it possible to characterize them more
definitely." Under simple proteins we may class albumins, globulins,
gluteHns, prolamins, albuminoids, histones and protamines.

ALBUMINS

Albumins constitute the first class of simple proteins and may be
defined as simple proteins which are coagulable by heat and soluble
in pure (salt-free) water. Those of animal origin are not precipitated
upon saturating their neutral solutions at 30°C. with sodium chloride
or magnesium sulphate, but if a saturated solution of this character
be acidified with acetic acid the albumin precipitates. All albumins
of animal origin may be precipitated by saturating their solutions with
ammonium sulphate.^ They may be thrown out of solution by the
addition of a sufi&cient quantity of a mineral acid, whereas a weak
acidity produces a slight precipitate which dissolves upon agitating the
solution. MetaUic salts also possess the property of precipitating al-
bumins, some of the precipitates being soluble in excess of the reagent,
whereas others are insoluble in such an excess. Of those proteins
which occur native the albumins contain the highest percentage of sul-
phur, ranging from 1.6 to 2.5 per cent. Some albumins have been

' In this connection, Osborne's observation that there are certain vegetable albumins
which are precipitated by saturating their solutions with sodium chloride or magnesium
sulphate or by half-saturating with ammonium sulphate, is of interest.

PROTEINS 97

obtained in crystalline form, notably egg albumin, serum albumin, and
lactalbumin, but the fact that they may be obtained in crystalline form
does not necessarily prove them to be chemical individuals.

GENERAL COLOR REACTIONS OF PROTEINS

These color reactions are due to a reaction between some one or
more of the constituent radicals or groups of the complex protein mole-
cule and the chemical reagent or reagents used in any given test. Not
all proteins contain the same groups and for this reason the various color
tests will yield reactions varying in intensity of color according to the
nature of the groups contained in the particular protein under examina-
tion. Various substances not proteins respond to certain of these color
reactions, and it is therefore essential to submit the material under ex-
amination to several tests before concluding definitely regarding its
nature.

TECHNIC OF THE COLOR REACTIONS

I. Millon's Reaction. — To 5 c.c. of a dilute solution of egg albumin^ in a test-
tube add a few drops of Millon's reagent. A white precipitate forms which turns
red when heated.

This test is a particularly satisfactory one for use on solid proteins,
in which case the reagent is added directly to the solid substance and
heat applied, which causes the substance to assume a red color. Such
proteins as are not precipitated by mineral acids, for example certain
of the proteoses and peptones, yield a red solution instead of a red
precipitate.

The reaction is due to the presence of the hydroxy-phenyl group,
— C6H4OH, in the protein molecule and certain non-proteins such as
tyrosine, phenol (carbolic acid) and thymol also respond to the reaction.
Inasmuch as the tyrosine grouping is the only hydroxyphenyl grouping
which has definitely been proven to be present in the protein molecule it
is evident that protein substances respond to Millon's reaction because
of the presence of this tyrosine complex. The test is not a very satis-
factory one for use in solutions containing inorganic salts in large
amount, since the mercury of the Millon's reagent- is thus precipitated
and the reagent rendered inert. This reagent is therefore never used
for the detection of protein material in the urine. If the solution under

1 This egg albumin solution may be prepared by beating egg-white with 6-10 volumes of
water. The precipitate of ovoglobulin is hltered off and the filtrate used in the tests.

2 Millon's reagent consists of mercury dissolved in nitric acid containing some nitrous
acid. It is prepared by digesting one part (by weight) of mercury with two parts (by
weight) of HXO3 (sp. gr. 1.42) and diluting the resulting solution with two volumes of
water.

98 PHYSIOLOGICAL CHEiUSTRY

examination is strongly alkaline it should be neutralized inasmuch as
the alkali will precipitate yellow or black oxides of mercury.

2. Xanthoproteic Reaction. — To 2-3 c.c. of egg albtimin solution in a test-tube
add concentrated nitric acid. A white precipitate forms, which upon heating
turns yellow and finally dissolves, imparting to the solution a yeUow color.
Cool the solution and carefully add ammonium hydroxide, potassium hydroxide,
or sodiimi hydroxide in excess. Note that the yellow color deepens into an
orange.

This reaction is due to the presence in the protein molecule of the
phenyl group — CeHs, with which the nitric acid forms certain nitro
modifications. The particular complexes of the protein molecule
which are of especial importance in this connection are those of tyrosine,
phenylalanine, and tryptophane. The test is not a satisfactory one for
use in urinary examination because of the color of the end-reaction.

3. GlyoxyUc Acid Reaction (Hopkins-Cole).^ — Place 1-2 c.c. of egg albumin
solution and 3 c.c. of glyoxyhc acid, CHO.COOH + H2O or CH(0H)2C00H,
solution (Hopkins-Cole reagent") in a test-tube and mix thoroughly. In a second
tube place 5 c.c. of concentrated sulphuric acid. Incline the tube containing sul-
phuric acid and by means of a pipette allow the albvunin-glyoxyUc acid solution
to flow carefully down the side. When stratified in this manner a reddish -violet
color forms at the zone of contact of the two fluids.

This color is due to the presence of the tryptophane group. Gelatin
does not respond to this test. For formula of tryptophane see page
77. Benedict^ has suggested a new reagent for use in carrying out
the Hopkins-Cole reaction.'^ Nitrates (XaXOs and KXO3) entirely
prevent the reaction whereas formaldehyde or nitric acid interfere
somewhat.^

4. Biuret Test. — To 2-3 c.c. of egg albximin solution in a test-tube add an
eqiial volmne of concentrated potassium hydroxide solution, mix thoroughly,
and add slowly a very dilute (2-5 drops in a test-tube of water) copper siilphate
solution until a purplish-violet or pinkish-violet color is produced. The depth

1 Hopkins and Cole: Journal of Physiology, 27, 418, 1902.

- Hopkins- Cole reagent is prepared as follows: To one liter of a saturated solution of
oxalic acid add 60 grams of sodium amalgam and allow the mixture to stand until the
evolution of gas ceases. Filter and dilute with 2-3 volumes of water.

^ Benedict: Journal of Biological Chemistry, 6, 51, 1909.

* Benedict's modified Hopkins-Cole reagent is prepared as follows: Ten grams of pow-
dered magnesium are placed in a large Erlenmeyer flask and shaken up \\ith enough dis-
tilled water to liberally cover the magnesium. Two hundred and fifty c.c. of a cold, satur-
ated solution of oxalic acid is now added slowly. The reaction proceeds very rapidly and
with the liberation of much heat, so that the flask should be cooled under running water
during the addition of the acid. The contents of the flask are shaken after the addition of
the last portion of the acid and then poured upon a filter, to remove the insoluble magnesium
oxalate. A little wash water is poured through the filter, the filtrate acidified with acetic
acid to prevent the partial precipitation of the magnesium on long standing, and made up to
a liter with distilled water. This solution contains only the magnesium salt of glyoxylic
acid.

* Mathewson: Dissertation (Columbia Univ.), Eschenbach Publishing Co., Easton, Pa.,
1912.

PROTEINS 99

of the color depends upon the nature of the protein; proteoses, and peptones
giving a decided pink, while the color produced with gelatin is not far removed
from a blue.

This reaction is given by those substances which contain two amino
groups in their molecule, these groups either being joined directly
together or through a single atom of nitrogen or carbon. The amino
groups mentioned must either be two CONH2 groups or one CONH2
group and one CSXHo, C(NH)XH2 or CH2XH2 group. It follows
from this fact that substances which are non-protein in character but
which contain the necessary groups will respond to the biuret test.
As examples of such substances may be cited oxamide,

CONH2

CONH2

and biuret,

CONH2

\
NH.

/
COXH2

The test derives its name from the fact that this latter substance which
is formed on heating urea to i8o°C (see page 375) will respond to the
test. Protein material responds positively since there are two COXH2
groups in the protein molecule.

According to Schiff the end-reaction of the biuret test is dependent
upon the formation of a copper-potassium-biuret compound (cupri-
potassium biuret or biuret potassium cupric hydroxide). This sub-
stance was obtained by Schiff in the form of long red needles. It has
the following formula:

OH OH

CO XHa Cu XH2CO

\ /

NH HX

/ \ .

CO •XH2— K K— NH2CO

I I

OH OH

Testing Colored Solutions by Biuret Test. — If the color of the solu-
tion is such as to interfere with the end-reaction of the biuret test,
proceed as follows: Make the solution strongly alkaline with potassium
hydroxide and add a solution of copper sulphate. Shake up the mixture
with alcohol and if protein is present the alcohol will assume the typical

lOO PHYSIOLOGICAL CHEMISTRY

biuret coloration. This procedure is not applicable in case the pigment
of the original solution is soluble in alcohol. Excess of the copper salt
need not be avoided in this test.

Gies's Biuret Reagent.'^ — Gies has devised a reagent for use in the biuret test.
This reagent consists of lo per cent KOH solution, to which 25 c.c of 3 per cent
CuSOi solution per liter has been added. This imparts a slight though distinct
blue color to the clear liquid. This reagent is of material assistance in performing
the biuret test.

Biuret Paper of Kantor and Gies. — According to Kantor and Gies- when
filter paper is immersed in the above reagent and subsequently dried it forms a
very' satisfactory- "biuret paper" which may be used in a manner analogous to
indicator papers. Moist papers may be used in the examination of powders which
are neutral or alkaline in reaction. In preparing the "biuret paper," if the filter
paper is left for a sufficient length of time in the reagent all traces of the copper
sulphate will be removed from the solution.

5. 'Ring Biuret Test (Posner). — This test is particularly satisfactory for use on
dilute protein solutions, and is carried out as follows. To some dilute egg albumin
in a test-tube- add one-half its volume of potassium hydroxide solution. Now hold
the tube in an inclined position and allow some very dilute copper sulphate solution,
made as suggested on page 98 to flow down the side, being especially careful to
prevent the fluids from mixing. At the juncture of the two solutions the typical
end-reaction of the biuret test should appear as a colored zone (see Biuret Test,
page 98).

6. Liebermann's Reaction. — Add about 10 drops of concentrated egg albumin
solution (or a little dry egg albumin) to about 5 c.c. of concentrated HCl in a test-
tube. Boil the mixture until a pinkish-violet color results. This color was origi-
nally supposed to indicate the presence of a carbohydrate group in the protein
molecule, the furfural formed through the action of the acid upon the protein react-
ing with the hydroxyphenyi group of the protein producing the pinkish-violet color.
It is now considered uncertain whether the carbohydrate group enters into the reac-
tion. Cole has called attention to the fact that a blue color results if protein mate-
rial which has been boiled with alcohol and subsequently washed with ether be used
in making the test. He believes the blue color to be due to an interaction between
the glyoxylic acid, which was present as an impurity in the ether used in washing
the protein, and the tryptophane group of the protein molecule which was split off
through the action of the acid.

7. Acree-Rosenheim Formaldehyde Reaction. — Add a few drops of a dilute
(i : 5000) solution of formaldehj-de to 2-3 c.c. of egg albumin solution in a test-tube.
Mix thoroughly and after two to three minutes carefully introduce a httle concen-
trated sulphuric acid into the tube in such a manner that the two solutions do not
mix. A violet zone will be observed at the point of juncture of the two solutions,
especially if the mixture is slightly agitated. This color probably results through
the union of the protein and the formaldehyde. If the sulphuric acid is added to the
protein before the formaldehyde is added the typical end-reaction is not obtained.
So far as is known this is a specific test for proteins. The reaction cannot be applied
satisfactorily with concentrated formaldehyde.

1 Gies: Proceedings of Society of Biological Chemists, Journal of Biological Chemistry,
7, 60, 1910.

2 Kantor and Gies: Proc. Sac. Biol. Chem., p. 11, 1910.

PROTEINS lOI

Rosenheim claims the reaction is due to the presence of oxidizing material in
the sulphuric acid and that when pure sulphuric acid is used no reaction is obtained.
He advises the use of a slight amount of an oxidizing agent, e.g., ferric chloride or
potassium nitrate (0.005 gram per 100 cc. of sulphuric acid) in order to facilitate
the reaction. Rosenheim further states that proteins respond to the formaldehyde
reaction because of the presence of the tryptophane group, a statement \Yhich Acree
does not accept as proven.

8. Bardach's Reaction.^ — This is one of the most recent tests which have been
described for the detection of protein material. The test depends upon the property
possessed by protein substances of preventing the formation of typical iodoform
crystals through the interaction of an alkaline acetone solution with iodopotassium
iodide. Instead of the typical hexagonal plates or stellar formations of iodoform
there are produced, under the conditions of the test, fine yelloiv needles which are
apparently some iodine compound other than iodoform. The technic of the test
is as follows: Place about 5 cc. of the protein solution- under examination in a test-
tube, add 2-3 drops of a 0.5 per cent solution of acetone and sufficient Lugol's solu-
tion' to supply a moderate excess of iodine and produce a red-brown coloration.
(The amount of Lugol's solution necessary will depend upon the content of protein,
sugar, and other iodine-reacting substances in the solution under examination and
may vary from one drop to several cubic centimeters.) Add an excess (ordinarily
about 3 CO.) of concentrated ammonium hydroxide and thoroughly mix the solu-
tion. Place the tube in the test-tube rack, examine the contents at intervals of
five minutes, and when it is evident that crystals have formed, place a drop of the
mixture upon a microscopic slide, put a cover-glass in position, and examine the
mixture under the microscope. The formation of canary yellow crystals indicates
the presence of protein material in the solution examined. The crystals are ordi-
narily needle-like in appearance and show a tendency to assume rosette or bundle-
like formations, but under certain conditions they may show knobbed (nail-like)
and branching variations.

If a moderate excess of iodine is used in making the test, a black precipitate
of iodonitro compounds is at once formed upon the addition of the ammonium
hydroxide, and yellow needles are subsequently deposited upon it. In case just the
proper amount of iodine is used, the solution soon assumes a yellow color and the
black precipitate formed upon the addition of the ammonium hydroxide is gradually
transformed more or less completely into the yellow cr>'stals. In either case the
needles ordinarily form within an hour, and frequently in a much shorter time.
If too great an excess of iodine is employed the heavy black precipitate may obscure
or even prevent the reaction. The presence of insufficient iodine or excess protein
may likewise prevent the reaction. In tests in which a concentrated protein solu-
tion and an excess of iodine are used, the addition of ammonium hydroxide im-
mediately produces a grayish-green precipitate. In such instances, if the propor-
tions are favorable and the mixture be stirred with a glass rod for a few minutes,
the precipitate is gradually transformed into the crystals before mentioned.

It is probable that all soluble proteins will respond to Bardach's reaction, but
the relative delicacy of the reaction as well as the value of the test as compared with

^Bardach: Zeilschrifl fiir Pliysiologisclic Chcmic, 54, 355, 1908; also Seaman and Gies:
Proceedings of the Society for Experinictital Biology and Medicine, 5, 125, 190S.
- The solution should not contain more than 5 per cent of protein material.
^ Dissolve 4 grams of iodine and 6 grams of potassium iodide in 100 cc. of distilled water.

I02 PHYSIOLOGICAL CHEMISTRY

other protein tests remain to be determined. The only disturbing factor noted
thus far is the presence of earthy phosphates in the solution under examination.

PRECIPITATION REACTIONS AND OTHER PROTEIN TESTS

There are three forms in which proteins may be precipitated, i.e.,
unaltered, as an albuminate, and as an insoluble salt. An instance of the
precipitation in a native or unaltered condition is seen in the so-called
salting-out experiments. Various salts, notably (NH4)2S04, ZnS04,
MgS04, Na2S04 and NaCl, possess the power, when added in solid form to
certain definite protein solutions, of rendering the menstruum incapable
of holding the protein in solution, thereby causing the protein to be
precipitated or salted-out, to use the common term. Mineral acids and
alcohol also precipitate proteins unaltered. In the case of concentrated
acids the protein is dissolved in the presence of an excess of acid with
the formation of a protein salt. Proteins are precipitated as albu-
minates when treated with certain metallic salts, and precipitated as
insoluble salts when weak organic acids such as certain of the alkaloidal
reagents are added to their solutions.

If certain acids (picric, phosphotungstic, phosphomolybdic, tannic, or
chromic) be added to a neutral albumin solution a precipitate of an
insoluble protein salt occurs. If, however, the salts of these acids be
added no precipitate occurs. The addition of a small amount of acid,
as acetic acid, to such a solution will cause a precipitate to form.^

The effect of the addition of the salts of the heavy'metals is in the
first instance to cause a precipitation of the protein. In many cases,
however, the addition of an excess of such salts causes the solution of
the precipitate while a further excess may cause a reprecipitation. The
precipitate which is first formed in a protein solution by the addition
of the salts of the heavy metals may be redissolved not only by an
excess of such salts but by an. excess of protein as well.^

It is generally stated that globulins are precipitated from their solu-
tions upon half saturation with ammonium sulphate and that albumins
are precipitated upon complete saturation by this salt. Comparatively
few exceptions were found to this rule until proteins of vegetable origin
came to be more extensively studied. These studies, furthered es-
pecially by Osborne and associates, have demonstrated very clearly
that the characterization of a globulin as a protein which is precipitated
by half saturation with ammonium sulphate, can no longer hold.
Certain vegetable globuHns have been isolated which are not precipi-

1 Mathews: Amer. Jour, of Physiology, i, 445, 1898.

^Pauli: Hojmeisler's Beitrage, 6,233, ^9°A~°S'> Robertson: Ergehnisse der Physiologic,
ro, 290, 1910.

PROTEINS 103

tated by this salt until a concentration is reached greater than that
secured by half-saturation. As an example of an albumin which does
not conform to the definition of an albumin as regards its precipitation
by ammonium sulphate may be mentioned the leucosin of the wheat
germ, which is precipitated from its solution upon /?o//-saturation with
ammonium sulphate. The limits of precipitation by ammonium
sulphate, therefore, do not furnish a sufficiently accurate basis for the
differentiation of globuUns from albumins. It has further been deter-
mined that a given protein which is precipitable by ammonium sulphate
cannot be ''salted-out" by the same concentration of the salt under all

conditions.

Experiments

1. Influence of Concentrated Mineral Acids, Alkalis and Organic Acids. —
Prepare five test-tubes each containing 5 c.c. of concentrated egg albumin solu-
tion. To the first add concentrated HjS04, drop by drop, until an excess of the
acid has been added. Note any changes which may occur in the solution. AUow
the tube to stand for 24 hours and at the end of that period observe any altera-
tion which may have taken place. Heat the tube and note any further change
which may occur. Repeat the experiment in the four remaining tubes with
concentrated hydrochloric acid, concentrated nitric acid, concentrated potassium
hydroxide and acetic acid. How do strong mineral acids, strong alkalis, and
strong organic acids differ in their action toward protein solutions?

2. Precipitation by Metallic Salts. — Prepare four tubes each containing 2-3
c.c. of dilute egg albumin solution. To the first add mercuric chloride, drop by
drop slowly, until an excess of the reagent has been added, noting any changes
which may occur. If not added very gradually the formation of the precipitate
may not be noted, due to its solubiUty in excess of the reagent. Repeat the ex-
periment with lead acetate, silver nitrate, copper sulphate, ferric chloride, and
bariimi chloride, using very dilute solutions.

Egg albumin is used as an antidote for lead or mercury poisoning.
Why ? Is it an equally good antidote for the other metalUc salts tested ?

3. Precipitation by Alkaloidal Reagents. — Prepare six tubes each containing
2-3 c.c. of dilute egg albumin solution. To the first add picric acid drop by drop
imtil an excess of the reagent has been added, noting any changes which may
occur. Repeat the experiment with trichloracetic acid, tannic acid, phospho-
timgstic acid, phosphomolybdic acid, and potassio-mercuric iodide. Are these
precipitates soluble in excess of the reagent? Acidify with hydrochloric acid
before testing with the last three reagents.

4. Nitric Acid Test (Heller).— Place 5 c.c. of concentrated nitric acid in a
test-tube, incline the tube, and by means of a pipette allow the dilute albimiin
solution to flow slowly down the side. The Uquids should stratify with the
formation of a white zone of precipitated albxmiin at the point of juncture. This
is a very delicate test and is further discussed on page 423.

An apparatus called the albttmoscope or Itorismoscope has been devised for use
in the tests of this character and has met with considerable favor. The method of
using the albumoscope is described on p. 104. The instrument is shown in Fig.
130, p. 424.

I04 PHYSIOLOGICAL CHEMISTRY

Use of the Alhumoscope. — This instrument is intended to facilitate the making of
"ring" tests such as Heller's and Roberts'. In making a test about $ c.c. of the
solution under examination is first introduced into the apparatus through the larger
arm and the reagent used in the particular test is then introduced through the capil-
lary arm and allowed to flow down underneath the solution under examination.
If a reasonable amount of care is taken there is no possibility of mixing the two solu-
tions and a definitely defined white "ring" is easily obtained at the zone of contact.

5. Nitric Acid — MgS04 Test (Roberts). — Place 5 c.c. of Roberts' reagent^ in
a test-tube, incline the tube, and by means of a pipette allow the albumin solu-
tion to flow slowly down the side. The liquids should stratify with the formation
of a white zone of precipitated albumin at the point of juncture. This test is a
modification of Heller's ring test and is rather more satisfactory. The alhumo-
scope may also be used in making this test (see Fig. 130, page 424).

6. Spiegler's Ring Test. — Place 5 c.c. of Spiegler's reagent^ in a test-tube, in-
cline the tube, and by means of a pipette allow 5 c.c. of albumin solution, acidified
with acetic acid, to flow slowly down the side. A white zone will form at the point
of contact. This is an exceedingly delicate test, in fact too delicate for ordinary
clinical purposes, since it serves to detect albumin when present in the merest trace
(i : 250,000). This test is further discussed on page 424.

7. Tanret's Test. — To 5 c.c. of albumin solution in a test-tube add Tanret's
reagent,' drop by drop, until a turbidity or precipitate forms. This is an exceed-
ingly delicate test. Sometimes the albumin solution is stratified upon the reagent
as in Heller's or Roberts' ring tests. In urine examination it is claimed by Repiton
that the presence of urates lowers the delicacy of the test. Tanret claims that the
removal of urates is not necessary inasmuch as the urate precipitate will disappear
on warming and the albumin precipitate will not. He says, however, that mucin
interferes with the delicacy of his test and should be removed by acidification with
acetic acid and filtration before testing for albumin.

8. Sodium Chloride and Acetic Acid Test.^ — Mix 2 volumes of albumin solu-
tion and I volume of a saturated solution of sodium chloride in a test-tube, acidify
with acetic acid, and heat to boihng. The production of a cloudiness or the
formation of a precipitate indicates the presence of albumin.

9. Acetic Acid and Potassium Ferrocyanide Test. — To 5 c.c. of dilute egg
albumin solution in a test-tube add 5-10 drops of acetic acid. Mix well and
add potassium ferrocyanide, drop by drop, until a precipitate forms. This test
is very delicate.

Schmiedl claims that a precipitate of Fe(Cn)6K2Zn or Fe(Cn)6-
Zn2, is formed when solutions containing zinc are subjected to this test,
and that this precipitate resembles the precipitate secured with protein

1 Roberts' reagent is composed of i volume of concentrated HNO3 and 5 volumes of a
saturated solution of MgS04.

2 Spiegler's reagent has the following composition:

Tartaric acid 20 grams.

Mercuric chloride 40 grams.

Sodium chloride.. 50 grams.

Glycerol 100 grams.

Distilled water 1000 grams.

' Tanret's reagent is prepared as follows: Dissolve 1.35 grams of mercuric chloride in 25
c.c. of water, add to this solution 3.32 grams of potassium iodide dissolved in 25 c.c. of
water, then make the total solution up to 60 c.c. with water and add 20 c.c. of glacial acetic
acid to the combined solutions.

PROTEINS 105

solutions. In the case of human urine a reaction was obtained when
0.000022 gram of zinc per cubic centimeter was present. Schmiedl
further found that the urine collected from rabbits housed in zinc-lined
cages possessed a zinc content which was sufficient to yield a ready re-
sponse to the test. Zinc is the only interfering substance so far
reported.

10. Salting-out Experiments. — (a) To 25 c.c. of egg albumin solution in a
small beaker add solid ammonium sulphate to the point of saturation, keeping
the temperature of the solution below 40°C. Filter, test the precipitate by
Millon's reaction and the filtrate by the biuret test. What are your conclu-
sions? (b) Repeat the above experiment, making the saturation with solid
sodium chloride. How does this result differ from the result of the saturation
with ammonium sulphate? Add 2-3 drops of acetic acid. What occurs?

All proteins except peptones are precipitated by saturating their
solutions with ammonium sulphate. Globulins are the only proteins
precipitated by saturating with sodium chloride (see Globulins, page
108), unless the saturated solution is subsequently acidified, in which
event all proteins except peptones are precipitated.

Soaps may be salted-out in a similar manner (see page 181).

11. Coagulation or Boiling Test. — Heat 25 c.c. of dilute egg albumin solution
to the boiling-point in a small evaporating dish. The albumin coagulates. Com-
plete coagulation may be obtained by acidifying the solution with 3-5 drops of
acetic acid^ at the boiling-point. Test the coagulimi by Millon's reaction.

The acid is added to neutralize any possible alkalinity of the solu-
tion, to dissolve any substances which are not albumin and to facilitate
coagulation (see further discussion on pages 117 and 424).

12. Coagulation Temperature. — Prepare four test-tubes each containing 5 c.c
of neutral egg albumin solution. To the first add i drop of 0.2 per cent hydro-
chloric acid, to the second add i drop of 0.5 per cent sodivmi carbonate solution,
to the third add i drop of 10 per cent sodium chloride solution and leave the
fourth neutral in reaction. Partly fill a beaker of medium size with water and
place it within a second larger beaker which also contains water, the two vessels
being separated by pieces of cork. Fasten the four test-tubes compactly together
by means of a rubber band, lower them into the water of the inner beaker and
suspend them, by means of a clamp attached to one of the tubes, in such a manner
that the albumin solutions shall be midway between the upper and lower sur-
faces of the water. In one of the tubes place a thermometer with its bulb entirely
beneath the surface of the albumin solution (Fig. 36). Gently heat the water in
the beakers, noting carefully any changes which may occur in the albumin solu-
tions and record the exact temperature at which these changes occur. The
first appearance of an opacity in an albimiin solution indicates the commencement
of coagulation and the temperature at which this occurs should be recorded as
the coagulation temperature for that particular albumin solution.

1 Nitric acid is often used in place of acetic acid in this test. In case nitric acid is used,
ordinarily 1-2 drops are sutlicient.

io6

PHYSIOLOGICAL CHEMISTRY

What is the order in which the four solutions coagulate?
Repeat the experiment, adding to the first tube i drop of acetic acid, to the
second i drop of concentrated potassium hydroxide solution, to the third 2 drops
of a 10 per cent sodium chloride solution and leave the fourth neutral as before.
What is the order of coagulation here? Why? See page 116.
13. Precipitation by Alcohol. — Prepare three test-tubes each containing
about 10 c.c. of 95 per cent alcohol. To the first add i drop of 0.2 per cent

hydrochloric acid, to the second i drop of potas-
siiun hydroxide solution and leave the third
neutral in reaction. Add to each tube a few
drops of egg albmnin solution and note the re-
sults. What do you conclude from this experi-
ment?

OB

If in acid or neutral solution alcohol
precipitates proteins unaltered, but if al-
lowed to remain under alcohol the protein is
transformed. The "fixing" of tissues for
histological examination by means of al-
cohol is an illustration of the application
of this transformation produced by alcohol.
It apparently is a process of dehydration.

14. CrystaUization of Egg Albmnin. ^ — Care-
fully remove the egg-white from a number of
absolutely fresh eggs.^ Measure the volume of
the egg-white and add an equal volume of satur-
ated ammonium sulphate a small portion at a
time, beating the mixture vigorously after each
addition.^ Filter the mixture through a large
pleated filter paper.* Measure the volume of
the filtrate. To 100 c.c. of the filtrate add very
carefully a 10 per cent solution of acetic acid from
a burette being certain to note the exact volume
of the acid used. The acid should be added drop
by drop, the albumin mixture being gently shaken
during the process. Add acid until the precipi-
tate_ which forms at each addition is no longer dissolved when the albumin is
shaken, and an opalescent mixture is secured. (It is generally rather difiicult
to determine this point, inasmuch as suspended air bubbles may simulate a
precipitate.) As soon as the solution is milky, indicating that a permanent pre-
cipitate has formed, run in from the burette i cc. of the acetic acid. This should
produce a heavy white precipitate. Now ^ake the burette reading to determine
the exact volume of acid used in the treatment of 100 c.c of the albumin mixture.

^ Hopkins and Pinkus: Jour. Physiol., 23.
2 If not perfectly fresh the albumin will not crystallize.
^ Note the odor of ammonia. What causes it?

* Sometimes better results are obtained by permitting the mixture to stand several
hours before filtering.

Fig. 36. — Coagulation Tempera-
ture Apparatus.

PROTEINS 107

Calculate the exact volume of acid necessary to precipitate the remaining portion
of the original albumin mixture and add this calculated quantity. Mix the two
portions of albumin and allow to stand over night. Remove a drop of the suspended
material to a slide and examine microscopically. Crystals in the form of fine
needles will be observed. This is the crystallized egg albumin. To recrystallize,
filter off the crystals and dissolve them in the smallest possible volume of water.
Filter, and to the filtrate carefuUy add saturated ammonium sulphate until a faint,
permanent precipitate is formed. Allow the mixture to stand several hours and
examine as before. The crystals of albumin should be somewhat larger than when
first examined.

The above method may also be used for crystallizing serum albumin from the
fresh blood serum of the horse, mule or ass.

15. Preparation of Powdered Egg Albumin. — This may be prepared as follows:
Ordinary egg-white finely divided by means of scissors or a beater is treated with
4 volumes of water and filtered. The filtrate is evaporated on a water-bath at
about 5o°C. and the residue powdered in a mortar.

16. Tests on Powdered Egg Albumin. — ^With powdered albumin prepared as
described above (by yourself or furnished by the instructor), try the following
tests :

(a) Solubility .^ — Test the solubility of the albumin in water, sodium chloride,
dilute acid and alkali.

(b) Millon's Reaction.

(c) Glyoxylic Acid Reaction (Hopkins-Cole). — ^When used to detect the
presence of protein in solid form this reaction should be conducted as follows :
Place 5 c.c. of concentrated sulphuric acid in a test-tube and add carefiilly, by
means of a pipette, 3-5 c.c. of HopMns-Cole reagent. Introduce a small amount
of the solid substance to be tested, agitate the tube sUghtly, and note that the
suspended pieces assimie a reddish-violet color, which is the characteristic end-
reaction of the Hopkins-Cole test ; later the solution will also assume the reddish-
violet color.

(d) Composition Test. — Heat some of the dry powder in a dry test-tube in
which is suspended a strip of moistened red Utmus paper and across the mouth of
which is placed a piece of filter paper moistened with lead acetate solution.
As the powder is heated it chars, indicating the presence of carbon; the fimies of
ammonia are evolved, tiurning the red litmus paper blue and indicating the pres-
ence of nitrogen and hydrogen; the lead acetate paper is blackened, indicating
the presence of sulphur, and the deposition of moisture on the side of the tube
indicates the presence of hydrogen. Moisture indicates hydrogen only in case
both powder and test-tube used in the test are absolutely dry.

(e) Coagulation Test. — Immerse a dry test-tube containing a Uttle powdered
egg albumin in boiling water for a few moments. Remove and test the solubUity
of the albvmiin according to the directions given under (ai above. It is still
soluble. Why has it not been coagulated? Repeat the above experiments
with powdered serimi albumin and see how the results compare with those
just obtained.

SULPHUR IX PROTEIN

Sulphur is believed to be present in two different forms in the pro-
tein molecule. The first form, which is present in greatest amount,

Io8 PHYSIOLOGICAL CHEMISTRY

is that loosely combined wdth carbon and hydrogen. An example of
this combination is shown in cystine,

CH2"S — SCH2

I I

CHXH2 CHNH2

I I

COOH COOH

Sulphur in this form is variously termed unoxidized, loosely combined,
mercaptan, and lead-hlackening sulphur. The second form is combined
in a more stable manner with carbon and oxygen and is known as
oxidized or acid sulphur. The protamines are the only class of sulphur-
free proteins.

Tests for Sulphur

1. Tests for Unoxidized Sulphur. — (a) To equal volumes of KOH and egg
albumin solutions in a test-tube add 1-2 drops of lead acetate solution and boil the
mixture. Unoxidized sulphur is indicated by a darkening of the solution, the
color deepening into a black if sufficient sulphur is present. Add hydrochloric
acid and note the characteristic odor evolved from the solution. Write the reac-
tions for this test, (b) Place equal volxmies of KOH and egg albximin solutions
in a test-tube and boil the mixture vigorously. Cool, make acid with glacial
acetic acid and add 1-2 drops of lead acetate. A darkening indicates the pres-
ence of vmoxidized sulphur.

2. Test for Total Sulphur (Unoxidized and Oxidized). — Place the substance
to be examined (powdered egg albmnin) in a small porcelain crucible, add a suit-
able amount of soUd fusion mixture (sodiimi carbonate and potassium nitrate
mixed in the proportion 2:1) and heat carefully until a colorless mixture results.
(Sodium peroxide may be used in place of this fusion mixture if desired.) Cool,
dissolve the cake in a Uttle warm water and filter. Acidify the filtrate with hydro-
chloric acid, heat it to the boiUng-point and add a small amount of barium chlor-
ide solution. A white precipitate forms if sulphur is present. What is this
precipitate?

GLOBULINS

Globulins are simple proteins especially predominant in the vege-
table kingdom. They are closely related to the albumins and in com-
mon with them give all the ordinary protein tests. Globulins dififer
from the albumins in being insoluble in pure (salt-free) water. They
are, however, soluble in neutral solutions of salts of strong bases with
strong acids. Most globulins are precipitated from their solutions by
saturation with solid sodium chloride or magnesium sulphate. As a
class they are much less stable than the albumins, a fact shown by the
increasing difl&culty with which a globulin dissolves during the course of
successive reprecipitations.

We have used an albumin of animal origin (egg albumin), for all

PROTEINS 109

the protein tests thus far, whereas the globuHn to be studied will be
prepared from a vegetable source. There being no essential difiference
between animal and vegetable proteins, the vegetable globulin we shall
study may be taken as a true type of all globulins, both animal and
vegetable.

Experiments on Globulin

Preparation of the Globulin.^ — Extract 20-30 grams fa handful) of crushed
hemp seed with a 5 per cent solution of sodium chloride for one-half hour at
6o°C. Filter while hot through a paper moistened with 5 per cent sodium chloride
solution. Place the filtrate in the water-bath at 6o'C. and allow it to stand for
24 hours in order that the globuUn may crystaUize slowly. In case the filtrate is
cloudy it should be warmed to 6o'C. in order to produce a clear solution. The
globuUn is soluble in hot 5 per cent sodium chloride solution and is thus extracted

Fig. 37. — Edestix.

from the hemp seed, but upon cooling this solution much of the globulin separates
in crystalline form. This particular globulin is called edestin. It crystaUizes
in several different forms, chiefly octahedra isee Fig. 37, above). (The crystal-
line form of excelsin, a protein obtained from the Brazil nut, is shown in Fig. 38,
p. no. This vegetable protein crystaUizes in the form of hexagonal plates.)
Filter off the edestin and make the following tests on the crystaUine body and on
the filtrate which still contains some of the extracted globulin.

Tests on Crystallized Edestin. — Microscopical examination (see Fig. 37.

(2) SolubiUty. — Try the solubihty in the ordinary solvents i.see page 21).
Keep these solubiUties in mind for comparison with those of edestan, to be made
later (see page 115).

(3) Millon's Reaction.

(4) Coagiilation Test. — Place a small amount of the globuhn in a test-tube, add
a little water and boil. Now add dilute hydrochloric acid and note that the pro-
tein no longer dissolves. It has been coagiilated.

no

PHYSIOLOGICAL CHEMISTRY

(5) Dissolve the remainder of the edestin in 0.2 per cent hydrochloric acid
and preserve this acid solution for use in the experiments on proteans (see page

115)-

Tests on Edestin Filtrate. — (i) Influence of Protein Precipitants. — ^Try a
few protein precipitants such as nitric acid, tannic acid, picric acid, and mercuric
chloride.

(2) Biuret Test.

(3) Coagulation Test. — ^Boil some of the filtrate in a test-tube. What
happens?

(4) Saturation with Sodium Chloride.^Saturate some of the filtrate with
solid sodium chloride. How does this result differ from that obtained upon
saturating egg albumin solution with solid sodium chloride?

Fig. 38. — ExcELSiN, The Protein of the Brazil Nut.
(Drawn from crystals furnished by Dr. Thomas B; Osborne, New Haven, Conn.)

(5) Precipitation by Dilution. — Dilute some of the filtrate with 10-15 volumes
of water. Why does the globuhn precipitate?

Glutelins

It has been repeatedly shown, particularly by Osborne, that after
extracting the seeds of cereals with water, neutral salt solution, and
strong alcohol, there still remains a residue which contains protein
material which may be extracted by very dilute acid or alkali. These
proteins which are insoluble in all neutral solvents, but readily soluble
in very dilute acids and alkalis are called glutelins. The only member
of the group which has yet received a name is the glutenin of wheat,
a protein which constitutes nearly 50 per cent of the gluten, the re-
mainder being principally gliadin. It is not definitely known whether
glutelins occur as constituents of all seeds.

PROTEINS III

Gluten: Preparation and Tests. ^ — To about 50 grams of wheat flour in a
casserole or evaporating dish, add a little water and mix thoroughly until a stiff
dough results. Knead this dough thoroughly and permit it to stand for about a
half hour. This is done in order that the maximum quantity of gluten may be
obtained. Treat the dough with about 200 c.c. of water and knead it thoroughly.
Note the yellowish color of the dough and the milky appearance of the water due
to suspended starch granules. (Place a drop of the suspension on a slide, cover
with a cover sUp, run underneath the slip a drop of iodine solution and observe
the stained starch granules under the microscope.) Filter and apply a protein
color reaction (see page 97) to the filtrate. It should be positive indicating
that water-soluble proteins were present in the flovu". Add fresh water to the
dough and repeat the kneading process. Continue this procedure with fresh
addition of water until practically no starch granules are noted in suspension.
To a small piece of the yellow, fibrous gluten apply Millon's Reaction (page 97).
This test shows gluten to be protein material, Utihze the remainder of the
gluten in the preparation of gliadin (page 112).

Glutenin : Preparation and Tests. — ^(In the preparation of gliadin (page 112)
it is customary to remove this prolamin from the crude gluten by extracting with
70 per cent alcohol. Inasmuch as gluten consists chiefly of gliadin and glutenin
the portion of the gluten remaining after the extraction of the alcohol-soluble
protein gliadin may be utilized for the preparation of glutenin.)

To the finely divided residue from the preparation of gliadin (page 112) in a
flask or bottle add about 250 c.c. of 70 per cent alcohol. Allow to stand for about
48 hours with repeated shaking. This alcohol treatment will remove the gliadin
and leave crude glutenin. To purify the glutenin treat it in a mortar, with suffi-
cient 0.2 per cent NaOH to dissolve it, and filter the liquid through a wet pleated
filter. NeutraUze the filtrate carefully, with 0.2 per cent HCl adding the acid
drop by drop with thorough mixture after each addition. (The glutenin is sol-
uble in excess of acid.) Filter off the glutenin precipitate and wash several
times with 70 per cent, alcohol and finally with water. Apply the following tests :

1. Solubility in water, salt solution, 0.2 per cent HCl and 0.5 per cent Na2C03.

2. Millon's Reaction.

Prolamins (Alcohol-soluble Proteins)

The term prolamin has been proposed by Osborne for the group of
proteins formerly termed "alcohol-soluble proteins." The name is
very appropriate inasmuch as these proteins yield, upon hydrolysis,
especially large amounts of proline and ammonia. The prolamins are
simple proteins which are insoluble in water, absolute alcohol and other
neutral solvents, but are soluble in 70 to 80 per cent alcohol and in dilute
acids and alkalis. They occur widely distributed, particularly in the
vegetable kingdom. The only prolamins yet described are the zein of
maize, the hordein of barley, the gliadin of wheat and rye, and the hynin
of malt. They yield relatively large amounts of glutamic acid on hy-

1 This experiment as well as those on glutenin and gliadin which follow have been
adapted from directions given in Laboratory Notes of Professor Gies, College of Physicians
and Surgeons, New York.

112 PHYSIOLOGICAL CHEMISTRY

drolysis but no lysin. The largest percentage of glutamic acid (43.66
per cent) ever obtained as a decomposition product of a protein sub-
stance has very recently been obtained by Osborne and Guest from the
hydrolysis of the prolamin gliadin} This yield of glutamic acid is also
the largest amount of any single decomposition product yet obtained
from any protein except protamines.

Gliadin : Preparation and Tests. — Introduce the finely divided crude gluten
as prepared on page 1 1 1 into a flask or bottle, add about 250 c.c. of 70 per cent
alcohol- and allow the mixture to stand 24 hoixrs with occasional shaking. Filter
(retaining the undissolved portion for preparation of glutenin, page in), evaporate
the filtrate to drjmess in a porcelain dish over a water -bath. Pulverize the dry
material. Apply the following tests to this gUadin powder :

Solubility and Protein Tests. — Test the solubihty in alcohol (30 per cent,
50 per cent and 70 per cent), water, 0.9 per cent NaCl, 0.2 per cent HCl and 0.5
per cent Na2C03. Shake each test repeatedly and filter. To the filtrate apply
Coagulation test (page 105) and Biuret test (page 98).

Albuminoids (Scleroproteins)

The albuminoids yield similar hydrolytic products to those obtained
from the other simple proteins already considered, thus indicating that
they possess essentially the same chemical structure. They differ from
all other proteins, whether simple, conjugated, or derived, in that they
are insoluble in all neutral solvents. The albuminoids include "the
principal organic constituents of the skeletal structure of animals as
well as their external covering and its appendages." Some of the princi-
pal albuminoids are keratin, elastin, collagen, reticulin, spongin, and
fibroin. Gelatin cannot be classed as an albuminoid although it is a
transformation product of collagen. The various albuminoids differ
from each other in certain fundamental characteristics which will be
considered in detail under Epithelial and Connective Tissue (sec
Chapter XVIII).

CONJUGATED PROTEINS

Conjugated proteins consist of a protein molecule united to some
other molecule or molecules otherwise than as a salt. We have glyco-
proteins, nude 0 proteins, hemoglobins (chromoproteins), phosphoproteins
and lecithoproteins as the five classes of conjugated proteins.

Glycoproteins may be considered as compounds of the protein mole-

1 Osborne and Guest: Jour. Biol. Chem., 9, 425, 1911. Up to this time the yield of
41.32 per cent obtained by Kleinschmitt from hordein was the maximum yield.

2 Bailey and Blish claim that 50 per cent alcohol is more satisfactory {Jour. Biol.
Chem., 23, 345, 1915).

s.

C.

H.

0.

2-33

48.76

6.53

30.60

2.32

47-43

6.63

31-40

PROTEINS 113

cule with a substance or substances containing a carbohydrate group
other than a nucleic acid. The glycoproteins yield, upon decomposition,
protein and carbohydrate derivatives, notably glucosamine, CH2OH.-
(CHOH)3.CH(NH2).CHO, and galactosamine, OHCHs.fCHOHjg.CH-
(NH2).CH0. The principal glycoproteins are mucoids, mucins, and
chondroprotcins. By the term mucoid we may in general designate
those glycoproteins which occur in tissues, such as tendomucoid from
tendinous tissue and osseomucoid from bone. (For the preparation of
tendomucoid see Chapter XVIII.) The elementary composition of
these typical mucoids is as follows:

N.

Tendomucoid^ ii-75

Osseomucoid- 12.22

The term mucins may be said in general to include those forms of glyco-
proteins which occur in the secretions and fluids of the body (For the
preparation of salivary mucin see Chapter III.) Chondroproteins are
so named because chondrom>ucoid, the principal member of the group,
is derived from cartilage (chondrigen) . A myloid,^ which appears patho-
logically in the spleen, liver, and kidneys, is also a chondroprotein.

The phospho proteins are considered to be "compounds of the
protein molecule and some, as yet undefined, phosphorus-containing
substances other than a nucleic acid or lecithin." The percentage of
phosphorus in phosphoproteins is very similar to that in nucleoproteins,
but they differ from this latter class of proteins in that they do not
yield any purine bases upon hydrolytic cleavage. Two of the common
phosphoproteins are the casein of milk and the ovoviteUin of the egg-
yolk. The phosphorus in these, as in all proteins, exists in phosphoric
acid radicals. For the preparation of a typical phosphoprotein (casein)
see Chapter XVII.

The hemoglobins (chromoproteins) are compounds of the protein
molecule with hematin or some similar substance. The principal mem-
ber of the group is the hemoglobin of the blood. Upon hydrolytic cleav-
age this hemoglobin yields a protein termed glohin and a coloring matter
termed hcmochromogcn. The latter substance contains iron and upon
coming into contact with oxygen is oxidized to form hematin. Hemo-
cyanin, another member of the class of hemoglobins, occurs in the blood
of certain invertebrates, notably ccphalopods, gastcropods, and

' Chittenden and Gies: Jour. Exp. Med., i, 1S6, 1S96.
■^ Hawk and Oies: Anier. Jour. Physiol., 5, 387, 1901.

^ Not to be confused \vitl\ tlie suVjstance awyloid which may be formed from cellulose
(see p. 49).

114 PHYSIOLOGICAL CHEMISTRY

Crustacea. Hemocyanin generally contains either copper, manganese,
or zinc in place of the iron of the hemoglobin molecule. For the prepa-
ration of hemoglobin in crystaUine form see Chapter XV.

The lecithoproteins consist of a protein molecule joined to lecithin.
They have been comparatively little studied and may possibly be
mixtures of protein and lecithin.

For consideration of nucleoproteins see Chapter VL

DERIVED PROTEINS

These substances are derivatives which are formed through hydro-
lytic changes of the original protein molecule. They may be di\'ided
into two groups, the primary protein derivatives and the secondary
protein derivatives. The term secondary derivatives is made use of
in this connection since the formation of the primary derivatives gener-
ally precedes the formation of these secondary derivatives. These
derived proteins are obtained from native simple proteins by hy-
drolyses of various kinds, e.g.. through the action of acids, alkalis,
heat, or enz}Tnes. The particular class of derived protein desired
regulates the method of treatment to which the native protein is
subjected.

Primary Protein Derivatives

The primary protein derivatives are "apparently formed through
hydrolytic changes which involve only sHght alterations of the protein
molecule.'" This class includes proteans, metaproteins and coagulated
proteins.

PROTEANS

Proteans are those insoluble protein substances which are produced
from proteins originally soluble through the incipient action of water,
enz}Tnes, or very dilute acids. It is well known that globulins become
insoluble upon repeated reprecipitation and it may possibly be found that
the greater number of the proteans are transformed globulins. Osborne,
however, beUeves that nearly all proteins may give rise to proteans.
This investigator who has so very thoroughly investigated many of
the vegetable proteins claims that the hydrogen ion is the active agent
in the transformation. The protein produced from the transformation
of edestin is called edestan, that produced from myosin is called myosan,
etc. The name protean was first given to this class of proteins by Os-
borne in 1900 in connection with his studies of edestin.

PROTEINS I I

Experiments on Proteans

Preparation and Study of Edestan. — Prepare edestin according to the direc-
tions given on page log. Bring the edestin into solution in 0.2 per cent hydro-
chloric acid and permit the acid solution to stand for about one-half hour.^ Neutral-
ize with a 0.5 per cent, solution of sodium carbonate, filter off the precipitate of
edestan and make the following tests:

1. Solubility. — Try the solubility in water, sodium chloride, dilute acid and
alkali. Note the altered solubility of the edestan as compared with that of edestin
(see page 109).

2. Millon's Reaction.

3. Coagulation Test. — Place a small amount of the protean in a test-tube,
add a little water and boil. Now add dilute hydrochloric acid and note that
the protein no longer dissolves. It has been coagulated.

4. Tests on Edestan Solution. — Dissolve the remainder of the edestan pre-
cipitate in 0.2 per cent hydrochloric acid and make the following tests:

(a) Biuret Test.

(b) Influence of Protein Precipitants. — Try a few protein precipitants such as
picric acid and mercuric chloride.

METAPROTEINS

The metaproteins are formed from the native simple proteins
through an action similar to that by which proteans are formed. In
the case of the metaproteins, however, the changes in the original pro-
tein molecule are more profound. These derived proteins are char-
acterized by being soluble in very weak acids and alkalis, but insoluble
in neutral fluids. The metaproteins were formerly termed albuminates,
but inasmuch as the termination ate signifies a salt it has always been
somewhat of a misnomer.

Two of the principal metaproteins are the acid metaprotein or so-
called acid albuminate and the alkali metaprotein or so-called alkali
albuminate. They differ from the native simple proteins principally in
being insoluble in sodium chloride solution and in not being coagulated
except when suspended in neutral fluids. Both forms of metaprotein
are precipitated upon the approximate neutralization of their solutions.
They are precipitated by saturating their solutions with ammonium sul-
phate, and by sodium chloride also, provided they are dissolved in
an acid solution. Acid metaprotein contains a higher percentage of
nitrogen and sulphur than the alkali metaprotein from the same source,
since some of the nitrogen and sulphur of the original protein is liberated
in the formation of the latter. Because of this fact, it is impossible
to transform an alkali metaprotein into an acid metaprotein, while it
is possible to reverse the process and transform the acid metaprotein
into the alkali modification.

^ The edestan solution preserved from experiment (5), p. no, may be used.

il6 physiological chemistry

Experiments on Metaproteins

AGED METAPROTEIN (ACID ALBUMINATE)

Preparation and Study. — Take 25 grams of hashed lean beef washed free
from the major portion of blood and inorganic matter, and place it in a medium-
sized beaker with 100 c.c. of 0.2 per cent HCl. Place it on a boiUng water-bath
for one -half hour, filter, cool, and divide the filtrate into two parts. Neutralize
the first part with dilute KOH solution, filter off the precipitate of acid metapro-
tein and make the following tests :

(i) Solubility. — SolubiUty in the ordinary solvents (see page 21).

(2) Millon's Reaction.

(3) Coagulation Test— Suspend a little of the metaprotein in water (neutral
solution) and heat to boiUng for a few moments. Now add 1-2 drops of KOH
solution to the water and see if the metaprotein is still soluble in dilute alkali.
What is the result and why?

(4) Test for Unoxidized Sulphur (see page 108).

Subject the second part of the original solution to the following tests :

(5) Coagulation Test. — Heat some of the solution to boiling in a test-tube.
Does it coagulate?

(6) Biuret Test.

(7) Influence of Protein Precipitants. — Try a few protein precipitants such as
picric acid and mercuric chloride. How do the results obtained compare with
those from the experiments on egg albumin? (See page 103.)

ALKALI METAPROTEIN (ALKALI ALBUMINATE)

Preparation and Study. — Carefully separate the white from the yolk of a
hen's egg and place the former in an evaporating dish. Add concentrated potas-
sium hydroxide solution, drop by drop, stirring continuously. The mass gradu-
ally thickens and finally assumes the consistency of jelly. This is solid alkali
metaprotein or "Lieberkiihn's jelly." Do not add an excess of potassium hydrox-
ide or the jelly will dissolve. Cut it into small pieces, place a cloth or wire gauze
over the dish, and by means of running water wash the pieces free from adherent
alkaU. Now add a small amount of water, which forms a weak alkahne solution
with the alkaU within the pieces, and dissolve the jelly by gentle heat. Cool the
solution and divide it into two parts. Proceed as follows with the first part:
Neutralize with dilute hydrochloric acid, noting the odor of the Uberated hydro-
gen sulphide as the alkaH metaprotein precipitates. Filter off the precipitate
and test as for acid metaprotein (tests i, 2, 3 and 4), above, noting particularly
the sulphur test. How does this test compare with that given by the acid meta-
protein? Make tests on the second part of the solution the same as for acid
metaprotein (tests 5, 6 and 7) above.

Coagulated Proteins

These derived proteins are produced from unaltered protein mate-
rials by heat, by long standing under alcohol, or by the continuous
movement of their solutions such as that produced by rapid stirring or
shaking. In particular instances, such as the formation of fibrin from

PROTEINS I I 7

fibrinogen (see page 256), the coagulation may be produced by enzyme
action. Ordinary soluble proteins after having been transformed into
the coagulated modification are no longer soluble in the ordinary sol-
vents. Upon being heated in the presence of strong acids or alkalis,
coagulated proteins are converted into metaproteins.

Many proteins coagulate at an approximately fixed temperature
under defim'te conditions (see pages 105 and 339). This characteristic
may be applied to separate difierent coagulable proteins from the same
solution by fractional coagulation. The coagulation temperature fre-
quently may serve in a measure to identify proteins in a manner similar
to the melting-point or boiling-point of many other organic substances.
The separation of proteins by fractional coagulation is thus analogous
to the separation of volatile substances by means ol fractional distillation.
This method of separating proteins is not a satisfactory one, however,
inasmuch as proteins in solution have difierent eft'ects upon one another
and also because of the fact that the nature of the solvent causes a
variation in the temperature at which a given protein coagulates. The
nature of the process involved in the coagulation of proteins by heat
is not well understood, but it is probable that in addition to the altered
arrangement of the component atoms in the molecule, there is a mild
hydrolysis which is accompanied by the liberation of minute amounts
of hydrogen, nitrogen, and sulphur. The presence of a neutral salt
or a trace of a mineral acid may facilitate the coagulation of a protein
solution (see page 105), whereas any appreciable amount of acid or
alkali will retard or entirely prevent such coagulation.

It has been shown that the coagulation of proteins by heat pro-
ceeds in two stages:^ first, a reaction between the protein and the hot
water (denaturation), and second, an agglutination or separation of the
altered protein in particulate form. The concentration of acid, or
hydrogen ion, in the solution influences the coagulation of proteins, such
that the original protein is acted upon less readily by hot water alone
than in the presence of acid. The formation of the coagulum is ac-
companied by the disappearance of the free acid from the solution,
indicating the formation of a protein salt. A disturbance of the equi-
librium between the hydrolyzed and unhydrolyzed portions of the pro-
tein salt, due to the greater rapidity with which the unhydrolyzed
portion is precipitated, results in the gradual removal of both pro-
tein and acid from the solution. This has been offered as an explana-
tion of the decreasing acidity.

According to Chick and Martin, the addition of neutral salts to the
acid solution of the salt-free protein to be coagulated results in a decreased

^ Chick and Martin: Journal of Physiology, 43, i, 191 1.

Il8 PHYSIOLOGICAL CHEMISTRY

rate of coagulation. This is due in part to the decrease in the concen-
tration of the free acid, which results from the disturbance of the equilib-
rium between the protein and acid and also in part to the direct influence
which the salts exert upon the protein. The presence of neutral salts
may under certain circumstances facilitate the coagulation of proteins
by heat.

The temperature at which egg-white is coagulated causes a difference
in the appearance of the coagulum.^ Coagulated egg-white which has
been immersed in water at a low temperature and then gradually heated
to the coagulating temperature is more translucent and has a bluish
color, whereas egg-white which has been immersed in water heated to a
temperature above the coagulating temperature is creamy white in
color. They also possess different digestibilities.

Experiments on Coagulated Protein

Ordinary coagxilated egg-white may be used in the following tests :

1. Solubility. — Try the solubiUty of small pieces of the coagulated protein in
each of the ordinary solvents (see page 21).

2. Millon's Reaction.

3. Xanthoproteic Reaction. — Partly dissolve a medium-sized piece of the
protein in concentrated nitric acid. Cool the solution and add an excess of
ammonium hydroxide. Both the protein solution and the undissolved protein
will be colored orange.

4. Biuret Test. — Partly dissolve a mediiun-sized piece of the protein in con-
centrated potassium hydroxide solution. If the proper dilution of copper sul-
phate solution is now added the white coagulated protein, as well as the protein
solution, will assume the characteristic purphsh-violet color.

5. Glyoxylic Acid Reaction (HopkLns-Cole). — Conduct this test according to
the modification given on page 107.

Secondary Protein Derivatives

These derivatives result from a more prof ound cleavage of the protein
molecule than that which occurs in the formation of the primary deriva-
tives. The class includes proteoses, peptones, and peptides.

PROTEOSES AND PEPTONES

Proteoses are intermediate products in the digestion of proteins by
proteolytic enzymes, as well as in the decomposition of proteins by hy-
drolysis and the putrefaction of proteins through the action of bacteria.
Proteoses are called albumoses by some writers, but it seems more logical
to reserve the term albumose for the proteose of albumin.

Peptones are formed after the proteoses and it has been customary to

* Frank: Journal of Biological Chemistry, 9, 463, 191 1.

PROTEINS 119

consider them as the last product of the processes before mentioned
which still possess true protein characteristics. In other words, ithas
been considered that the protein nature of the end-products of the
cleavage of the protein molecule ceased with the peptones, and that the
simpler bodies formed from peptones were substances of a different
nature (see page 65). However, as the end-products have been more
carefully studied, it has been found to be no easy matter to designate
the exact character of a peptone or to indicate the exact point at
which the peptone characteristic ends and the peptide characteristic
begins. The situation regarding the proteoses, peptones and peptides
is at present a most unsatisfactory one because of the unsettled state
of our knowledge regarding them. The exact differences between
certain members of the peptone and peptide groups remain to be more
accurately established. It has been quite well established that the
peptones are peptides or mixtures of peptides, but the term peptide is
used at present to designate only those possessing a definite structure.
There are several proteoses (protoproteose, heteroproteose and
deuteroproteose), and at least two peptones (amphopeptone and anti-
peptone), which result from proteolysis. The differentiation of the
various proteoses and peptones at present in use is rather unsatisfactory.
These compounds are classified according to their varying solubilities,
especially in ammonium sulphate solutions of diff"erent strengths. The
exact differences in composition between the various members of the
group remain to be more accurately established. Because of the
diflSculty attending the separation of these bodies, pure proteose and
peptone are not easy to procure. The so-called peptones sold com-
mercially contain a large amount of proteose. As a class the proteoses
and peptones are very soluble, dift'usible bodies which are non-coagu-
lable by heat. Peptones differ from proteoses in being more diffusible,
non-precipitable by (NH4)2S04, and by their failure to give any reaction
with potassium ferrocyanide and acetic acid, potassio-mercuric iodide
and HCl, picric acid, and trichloracetic acid. Peptones may be pre-
cipitated by phosphotungstic acid, phosphomolybdic acid, absolute
alcohol and tannic acid, but an excess of the precipitant may dissolve
the precipitate. The so-called primary proteoses are precipitated by
HNO3 and are the only members of the proteose-peptone group which
are so precipitated.

Some of the more general characteristics of the proteose-peptone group may
be noted by making the following simple tests on a proteose-peptone powder:
(i ) Solubility. — SolubiUty in hot and cold water and sodium chloride solution.
(2) Millon's Reaction.
Dissolve a little of the powder in water and test the solution as follows :

I20 PHYSIOLOGICAL CHEMISTRY

(i) Precipitation by Picric Acid. — To 5 c.c. of proteose -peptone solution in a
test-tube add picric acid until a permanent precipitate forms. The precipitate
disappears on heating and returns on cooling.

(2) Precipitation by a Mineral Acid. — Try the precipitation by nitric acid.

(3) Coagxilation Test. — Heat a littie proteose-peptone solution to boiling.
Does it coagulate Uke the other simple proteins studied?

SEPARATION OF PROTEOSES AND PEPTONES^

Place 50 c.c. of proteose-peptone solution in an evaporating dish or casserole,
and half-saturate it with ammoniimi sulphate solution, which may be accom-
plished by adding an equal volvune of saturated ammonivun sulphate solution.
At this point note the appearance of a precipitate of the primary proteoses
(protoproteose and hetero-proteose). Now heat the half -saturated solution and
its suspended precipitate to boihng and saturate the solution with solid am-
monium sulphate. At full saturation the secondary proteoses (deuteroproteoses)
are precipitated. The peptones remain in solution.

Proceed as follows with the precipitate of proteoses: Collect the sticky
precipitate on a rubber-tipped stirring rod or remove it by means of a watch
glass to a small evaporating dish and dissolve it in a littie water. To remove the
ammonium sulphate, which adhered to the precipitate and is now in solution,
add barium carbonate, boil, and filter off the precipitate of barium sulphate.
Concentrate the proteose solution to a small volume ^ and make the follow-
ing tests :

(i) Biuret Test.

(2) Precipitation by Nitric Acid. — ^What would a precipitate at this point
indicate?

(3) Precipitation by Trichloracetic Acid. — This precipitate dissolves on heating
and returns on cooling.

(4) Precipitation by Picric Acid. — This precipitate also disappears on heat-
ing and returns on cooling.

(5) Precipitation by Potassio-mercuric Iodide and Hydrochloric Acid.

(6) Coagulation Test. — Boil a littie in a test-tube. Does it coagulate?

(7) Acetic Acid and Potassium Ferrocyanide Test.

The solution containing the peptones should be cooled and filtered, and the
ammonium sulphate in solution removed by boiling with barium carbonate as
described above. After filtering off the barium sulphate precipitate, concentrate
the peptone filtrate to a small volume and repeat the tests as given under the
proteose solution, above. Also try the precipitation by phosphotungstic acid
and by tannic acid. In the biuret test the solution should be made very strongly
alkaUne with solid potassium hydroxide.

PEPTIDES

The peptides are "definitely characterized combinations of two or
more amino acids, the carboxyl (COOH) group of one being united

^ The separation of proteoses and peptones by means of fractional precipitation with,
ammonium sulphate does not possess the significance it was once supposed to possess inas-
much as the boundary between these substances and peptides is not well defined (see p. 119).

^ If the proteoses are desired in powder form, this concentrated proteose solution may
now be precipitated by alcohol, and this precipitate, after being washed with absolute
alcohol and with ether, may be dried and powdered.

PROTEINS

with the amino (NH2) group of the other with the elimination of a mole-
cule of water." These peptides are more fully discussed on pages 70
and 119.

REVIEW OF PROTEINS

In order to facilitate the student's review of the proteins, the prepara-
tion of a chart similar to the model given is recommended. The signs -4-
and — may be conveniently used to indicate positive and negative
reactions.

MODEL CHART FOR REVIEW PURPOSES

Solubility

s

"3
O
e
'S

S

Salting-
Precipitation Tests out

Tests

-

Protein
f

Water
10% NaCl

O

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u
5

6

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(NH4)2S04

0

2

Diffusion
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Albumin
Globulin

--• —

-

Nucleoprotein

1 : ,

Phosphoprotein

1

i

Glucoprotein

Acid metaprotein

Alkali metaprotein

i Proteose

J_

1 Peptone i I

•

; Coagulated protein | i 1

1

"Unknown" Mixtures and Solutions of Proteins

At this point the student's knowledge of the characteristics of the
various proteins studied will be tested by requiring him to examine several
"unknown" protein mixtures or solutions and make full report upon the
same. The scheme given on page 122 may be used in this examination.

122

PHYSIOLOGICAL CHEMISTRY

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CHAPTER VI
NUCLEIC ACIDS AND NUCLEOPROTEINS^

The Nucleoproteins. — The nucleoproteins occur widely distributed
in the animal and plant kingdoms, being found in nearly all cells and
particularly in the nuclei of cells. They are found in especially large
amounts in glandular tissues such as those of the thymus, pancreas and
spleen. The nucleoproteins are combinations of protein with a phos-
phorus-containing substance known as nucleic acid. As different nu-
cleic acids exist and are found in combination with different proteins,
a variety of nucleoproteins exist. The protein combined with the
nucleic acid is in certain cases a histone, the conjugated protein in
this case being called a nucleohistone.

The nucleoproteins give the ordinary protein color reactions.
They are acidic in character and insoluble in water. They are readily
soluble in weak alkali but are precipitated from such solution on the
addition of acetic acid in excess of which they dissolve with more or
less difficulty although readily soluble in very dilute hydrochloric acid.
We distinguish them from mucins, which are likewise precipitated by
acetic acid through the fact that the latter give no tests for phosphorus
on decomposition.

The nucleoproteins are very complex and unstable substances
and one has probably never been prepared in a pure form. Under the
action of the gastric juice or of weak acid nucleoproteins lose a portion
of their protein content and are transformed into a rather ill-defined
class of substances known as micleins w'hich still possess some protein
in combination with the nucleic acid molecule. In most cases the
decomposition does not proceed further in gastric digestion. Through
the action of the pancreatic juice, however, the remainder of the
protein is split off and the nucleic acid set free. The decomposition
of nucleoprotein may be diagramatically expressed thus, although
the course of decomposition is probably not quite so simple as indicated.

^ For review of the literature on nucleic acids and nucleases see Monograph on "Nucleic
Acids" by Walter Jones, New York, 19 14, Longmans Green & Co.

123J

124 PHYSIOLOGICAL CHEMISTRY

NTJCLEOPROTEIN

. I.

(gastric digestion)

Protein Nuclein

I

(pancreatic digestion)

Protein Nucleic Acid

The Nucleic Acids. — The nucleic acids of the animal body occur
mainly in combination with protein material in the so-called nucleo-
proteins of which they form the characteristic radicals (see page 123).
The amount and character of the protein with which the nucleic acid
molecule is combined varies and the acid may in certain cases be found
in cells in a free form. Naturally those tissues are richest in nucleic
acid which contain the largest amount of nuclear material and of
nucleoprotein. Such are the glandular tissues of the body as the
thymus, spleen, pancreas, liver, etc. The heads of the spermatozoa
consist almost entirely of nucleic acid in combination with protamine.

The nucleic acids are a distinct class of substances, characterized
by their decomposition products. They are strongly acid in reaction
and contain considerable phosphorus. They may be divided into two
main groups, the animal and the plant nucleic acids. The two
classes differ in certain respects but all of the true animal nucleic acids
appear to be practically identical in composition. Animal nucleic
acid is most readily prepared from the thymus while plant nucleic
acid is most readily obtained from yeast.

The nucleic acids are difficultly soluble in cold water, more readily
in hot water, insoluble in alcohol, but readily soluble in weak alkali
with the formation of the alkali salt. If pure they do not give the
protein color reactions. They are optically active. They are pre-
cipitated from their alkaline solutions by HCl, but only the plant nu-
cleic acid is precipitated by acetic acid. In weak acid solution they are
precipitated by protein the combination being considered a "nuclein."
They form insoluble salts with alkaline earth and heavy metals.
The sodium salt of animal nucleic acid in 4 per cent solution is liquid
while warm but solidifies to a gelatinous mass on cooling. Plant
nucleic acid does not do this.

The nucleic acids on hydrolysis yield phosphoric acid, purine and
pyrimidine bases, and a carbohydrate or carbohydrate derivative. The
composition varies slightly with the type of nucleic acid. Plant nucleic
acids contain a pentose group while animal nucleic acids contain a

NUCLEIC ACIDS AND NUCLEOPROTEINS 1 25

hexose group. Both types contain the purine bases, guanine and
adenine and the pyrimidine base cytosine. Plant nucleic acid contains
also the pyrimidine base uracil, which in the animal nucleic acid is sub-
stituted by the base thymine. The nucleic acids are not, however,
simple substances whose molecules contain a single phosphoric acid or
carbohydrate group. They are apparently combinations of several
radicals known as nucleotides each of which contains one car-
bohydrate group combined with a single base and a single phosphoric
acid molecule. Thus the following structural formula has been given
to yeast nucleic acid by Levene and Jacobs^ indicating that it contains
four nucleotide radicals and may hence be called a tetranucleotide.

HO

\

0 = POC5H803C5H4N50

/ Guanine group

o

\

0-POC5H803C5H4N5

/ Adenine group

0

\

0=POC5H803C4H3N202

/ Uracil group

o

\

0 = POC5H803C4H4N30

/ Cytosine group

HO

Yeast nucleic acid (tetranucleotide)

The cleavage of the nucleic acid molecule into its corresponding
nucleotides is brought about during digestion by enzymes present in
the intestinal juice and intestinal mucosa. Enzymes of similar origin
act further on the nucleotides thus formed and split off the phosphoric
acid radicals together with carbohydrate-base compounds which are
called nucleosides. The decomposition prior to absorption does
not probably proceed further than to the formation of nucleotides
and nucleosides. ]\Iany tissues however contain enzymes capable of
completing the decomposition with liberation of the carbohydrate
and basic radicals. The purine bases may also be deaminized while
still in combination as nucleosides and further hydrolysis would then
lead to the direct liberation of the oxypurines instead of their precursors,
the amino-purines.

^Levene and Jacobs: Bcr. d. dcitlsch. Clicm. Gcs., 43, 3151. iQio; 44, 1027, loii

126 PHYSIOLOGICAL CHEMISTRY

Jones^ has suggested a method by which the course of the decom-
position of the nucleic acid molecule can be followed. By this means
it is readily shown that phosphoric acid is liberated at very different
rates from the different nucleotides.

The following outline will indicate the course of decomposition of/a
nucleic acid and the enzymes involved in the process.

DECOMPOSITION OF NUCLEIC ACID
NUCLEIC ACID

(nucleicacidase of intestinal mucosa and juice)

I I

Purine Nucleotides Pyrimidine Nucleotides

I . I

(nucleotidase of intestinal (tissue nucleases)

mucosa and juice) I

Phosphoric Acid Purine Nucleosides 55^^^?!,°"^ 4"*^

I Pjrrimidme Bases

I Cytosine and Thjrmine

(nucleosidase of tissues) or Uracil

Sugar Piu-ine Bases

(pentose or hexose) Adenine

Guanine

With regard to the fate of the various radicals of the nucleic acids
in the body a;fter absorption little is definitely known. The phosphoric
acid may of course be built up into phosphorus-containing cell con-
stituents such as nucleoproteins, phosphoproteins or phosphatides, or
be eliminated as phosphate in the urine. The carbohydrate portion
may undergo the usual transformations of intermediary carbohydrate
metabolism. The nucleosides appear to be ordinarily absorbed un-
changed from the intestine and may be to a certain extent directly re-
synthesized in the animal body to nucleoprotein. The excess over body
requirement must, however, be decomposed, although a certain portion
may possibly be stored up in the individual cells or in certain organs.
Enzymes capable of decomposing nucleic acids are found in most of the
cells of the body.

The Purine Bases. — As has been indicated the basic substances
present in nucleic acid belong to two classes the purine and pyrimi-
dine bases. The purine bases set free on the decomposition of nucleic
acid are adenine and guanine belonging to the class of amino purines.

^ Jones: Presidential address before the Society of Biological Chemists, Boston, Dec.
27, iQiS-

NUCLEIC ACIDS AND NUCLEOPROTEINS

127

The fate of the amino purines in the animal body is of considerable
interest. It has been shown that certain tissues contain enzymes
which transform these amino purines first to corresponding oxypurines
known as hypoxanthine and xanthine and finally to uric acid. It is
probable that different enzymes enter into the various steps of these
transformations leading to the formation of uric acid. Still another
enzyme carries the oxidation further with the formation of the com-
pound allantoin. This enzyme is known as uricase. The [purine
enzymes are widely distributed in tissues. The transformations
brought about are indicated in the following diagrams.

N=CNH2

HN— CO

HC C— NH +H2O— NHa-^ HC C— NH

Adenase

//

CH

N— C— N

Adenine
6-aniino purine

N— C— N'

Hypoxan'.hxnt
6-oxypurine

/

CH

+0

Hypoxanthine
oxidase

HN— CO

r I

H2NC C— NH

HN— CO

I I
OC C— NH

CH;+H20 — NH3-> CH

// Ciianase /^

N— C— N HN— C— N

Guanine
2-amino-6-oxypurine

Xanthine
2-6-dioxypurine

+0

Xanthine
oxidase

NH2

CO CO— NH O

I I \ Uricase

CO

HN— CO

I I
OC C— NH

CO

NH— CH— NH

Allantcin

HN— C— NH

Uric acid
2-6-8-trioxypurine

128 PHYSIOLOGICAL CHEMISTRY

All of the physiologically important purine bodies are precipitated
by ammoniacal silver nitrate solution in the cold and by copper sul-
phate and sodium bisulphite in boiling solutions. Some of them are
readily identified by their crystalline forms or the crystalline forms of
certain of their salts. Uric acid differs from the other purines in being
insoluble in dilute sulphuric acid. The purine bodies may be distin-
guished to a certain extent also by the reactions which they give when
their solutions are evaporated with nitric acid and the residue treated
with ammonia. Uric acid gives the characteristic formation of the
purple murexide (ammonium purpurate) . Potassium hydroxide changes
this to a bluish-violet color which disappears on heating. Xanthine
and guanine form yellow compounds with nitric acid which turn
purple or violet on treating with potassium hydroxide. The color in
this case is not lost by heating. Adenine and hypoxanthine do not
give a color reaction with nitric acid.

The Pyrimidine Bases. — The pyrimidine bases entering into the
composition of nucleic acid are thymine, cytosine and uracil. Cytosine
is found in both types of nucleic acid, while thymine is found only
in animal nucleic acid and uracil only in plant nucleic acid. They
possess the following formulas.

NH— C=0 NH— C=0 N=C— NH2

O-C CH 0=C C— CH3 0=C CH

NH— CH NH— CH NH— CH

Uracil Thymine Cytosine

2-6-dioxypyrimidine 5-methyl- 6-amino-

2-6-dioxypyrimidine 2-dioxy pyrimidine

With regard to the fate of pyrimidine bases in metabolism very
little is known. When the bases as such are fed they reappear un-
changed in the urine. ^ If nucleic acid is fed this does not occur which
indicates that the pyrimidine bases may undergo certain alterations
in the animal body while still existing in combination.

Experiments

I. Preparation of Nucleoprotein from Yeast. ^ — Place two small cakes of ordi-
nary compressed yeast in a mortar. Sprinkle a small horn-spoonful of sand over
the yeast, add 5 c.c. of ether and 10 c.c. of water and thoroughly triturate the
mixture, grinding vigorously. The ether kills the yeast, in which condition the
comminution of the cells with sand is more thoroughly affected. Occasionally
during the trituration process add i or 2 c.c. of water until the mixture is
comparatively fluid. The whole process of maceration can be completed in five

1 Mendel and Myers: Am. J. Physiol., 26, 77, 1910.

^ All experiments on nucleoprotein of yeast have been taken from Laboratory Notes of
Professor W. J. Gies, of College of Physicians and Surgeons, New York.

NUCLEIC ACIDS AND XUCLEOPROTEINS 1 29

minutes. Pour the thick liquid into a bottle aiding the transfer with enough
0.4 per cent NaOH to make a final volume of about 125 c.c. The alkaU extracts
the nucleoprotein along with the water-soluble proteins of the yeast. Add a little
toluol and allow to stand with frequent shaking for 1224 hours. Filter through
a wet, fluted filter. While thoroughly stirring add i drop at a time of 10 per cent
HCl cautiously continuing the addition as long as the milkiness of the mixture can
be increased. Continue until the protein completely separates and the Uquid is
practically clear. Note that the solution is now acid in reaction. Excess of acid
causes resolution. Filter on a wet, fluted filter. Retain the precipitate on the
filter for nucleoprotein tests.

2. Tests on Nucleoprotein. — Try the following tests on the nucleoprotein
prepared as above.

(a) Try the xanthoproteic and Millon's tests.

(b) Test the solubiUty in water, 10 per cent NaCl, 10 per cent HCl, dilute
KOH, and alcohol.

(c) Test for organically combined phosphorus by one of the following
methods.

Tests for Phosphorus in Organic Matter. — i. Fusion Test. — To a small
amount of the substance in a crucible add about five times its bulk of fusion mix-
ture (2 parts of sodiiun carbonate to i of potassium nitrate). Heat carefully until
the resulting mixture is colorless. Cool, dissolve the mass in a little warm water,
acidify with nitric acid, heat nearly to boiling and add a few cubic centimeters of
molybdate solution. In the presence of phosphorus a yellow precipitate of phos-
phomolybdate is formed.

Instead of acidifying with nitric acid, the aqueous solution may be approxi-
mately neutralized with hydrochloric acid, a few cubic centimeters of magnesia
mixture added and then excess of ammonium hydroxide solution. A white pre-
cipitate of magnesium ammoniiun phosphate is formed.

2. Moist Ashing Procedure. — Treat a small amount of the substance in a
large test-tube with about i c.c. of concentrated sulphuric acid. Then add drop by
drop an equal volume of concentrated nitric acid, and warm gently until a clear
solution is obtained. A few more drops of nitric acid may be added if necessary.
This treatment with sulphuric and nitric acids must be carried out with the
greatest caution particiilarly when fatty substances are present ; otherwise an
explosive reaction may take place. Dilute the acid solution with a Uttle water,
make sUghtly alkaline with ammonia and then acid with nitric acid. Add
molybdate solution and warm. A yellow precipitate is formed.

(d) Dissolve a little of the precipitate in very dilute KOH and then make
slightly acid with acetic acid.

(e) Mix a small portion of the nucleoprotein with 10 c.c. of alcohol. Filter
and wash free from HCl with more alcohol. (Freedom from HCl is indicated by
absence of AgNOa-chloride reaction in the filtrate.) Wash free from alcohol
with a httle water. Transfer small particles of the precipitate to moistened red
and blue litmus paper on a microscopic slide. What is the reaction of nucleo-
protein thus freed from adherent acid?

3. To Show the Presence of Purine Base Radicals in Nucleoprotein. The
nucleic acid portion of the protein molecule contains phosphoric acid, carbohy-
drate, and purin base radicals (see page 126). Hence on the complete acid hydro-
lysis of nucleoprotein material these substances will be Uberated as well as the
decomposition products of the protein part of the molecule. To show their pres-

9

130 PHYSIOLOGICAL CHEMISTRY

ence proceed as follows: Transfer the precipitate of nucleoprotein remaining
from the previous experiment to a small flask and add 25-50 c.c. of 5 per cent
H2SO4. Boil for an hour or more to decompose. Maintain the original volume
by adding water. The solution becomes brown due to formation of melanin-
like substances. The purine bases are set free. Retain one-fourth of the solu-
tion for the next experiment. Transfer the remainder to a casserole and add
anmionia with thorough mixing, a Uttle at a time, until the fimd is nearly neutral.
Then make sUghtly alkahne with dilute ammonia and filter if not clear. Transfer
to a beaker and add about 10 c.c. of 5 per cent ammoniacal silver nitrate solution.
Purine bases if present will yield a brown fiocculent precipitate of their silver
compounds. If a precipitate does not appear immediately, examine the solution
after it has been allowed to stand for some time undisturbed.

4. To Show the Presence of Protein, Carbohydrate, and Phosphoric Acid
Radicals in Nucleoprotein.— Filter the greater portion of the acid liquid which was
reserved from the preceding experiment. Apply the following tests to portions of
it: (a) The biuret test, (b) The xanthoproteic test, (c) Molisch test, (d)
Fehling's test, (e) Test for phosphate.

5. Preparation of Thymus Nucleoprotein. — About 100 grams of fresh thymus
gland (lymphatic glands may also be used) freed as nearly as possible from adherent
fat are run through a meat chopper. To this material in a flask add 300 c.c. of 0.9
per cent NaCl and allow to stand 24-48 hours in the cold. A little chloroform and
toluol should be added as preservatives, and the mixture shaken occasionally during
this period. Filter. A milk white liquid is obtained. Precipitate the nucleo-
protein from solution by the careful addition of dilute acetic acid. Excess of the
acid should be avoided. Ordinarily acetic acid to make a i per cent solution is
sufiicient. Filter off the precipitate. Wash with alcohol and then with ether and
dry.

6. Experiments on Thymus Nucleoprotein. — Repeat the experiments given
under Yeast Nucleoprotein (page 129).

7. Preparation of Yeast Nucleic Acid. — Dilute 50 c.c. of i per cent NaOH
with 250 c.c. of water in a casserole and add to this solution 100 grams of com-
pressed yeast cut in small pieces. Heat on the water-bath for half an hour with
occasional stirring. Remove from the bath and filter at once through a folded
filter. To the cooled filtrate add acetic acid until faintly acid to Utmus. Filter
again. Evaporate the solution to 100 c.c. or less and filter if necessary. Allow
to cool to 40°C. or below, then pour with vigorous stirring into 200 c.c. of 95 per
cent alcohol containing 2 c.c. of concentrated HCl. Allow to settle and wash the
precipitate by decantation in a tall vessel, twice with 95 per cent, alcohol and
twice with ether. Transfer to a filter paper. Allow to drain and dry at room
temperature.

8. Tests on Nucleic Acid from Yeast.' — i. Test the solubility of nucleic acid
in cold and hot water, in alcohol, and in dilute acid and alkali. To the solution in
alkali add dilute HCl drop by drop until the solution is acid, then add excess of
concentrated HCl.

Does nucleic acid coagulate on boiUng? Does the solution in hot water
gelatinize on cooling?

2. Try xanthoproteic reaction and biuret test.

3. Dissolve a little nucleic acid in water with the aid of heat. Test the re-

1 A satisfactory preparation of yeast nucleic acid may be obtained from Merck and Co.

NUCLEIC ACIDS AND NUCLEOPROTEINS I3I

action of different portions of tiie solution with litmus, alizarin, and Congo red
solution.

4. Boil a small portion of the nucleic acid with about 10 c.c. of 10 per cent
sulphuric acid for one to two minutes. Divide into three portions.

(a) To one portion apply carbohydrate tests, e.g., the a-naphthol fMolisch;
reaction and Bial's test. What do these indicate?

(b) To a second portion apply a test for purine bases. Add an excess of
ammonia and then a Uttle silver nitrate solution.

(c) To the third portion apply test for phosphate, adding ammonia in slight
excess, then making acid with nitric acid, adding molybdic solution and warming.

9. Preparation of Thymus Nucleic Acid.^ — "To a boiling mi.xture of 200 c.c. of
water, 10 grams of sodium acetate and 3.3 grams of NaOH, is added in small suc-
cessive portions 100 grams of trimmed and finely ground thymus gland. The tissue
usually dissolves completely forming a pale brown liquid, but any resistant portions
are either removed or gotten into solution by heating for a short time over a small
flame. The vessel containing the products is now immersed in a briskly boiling
water-bath where it is allowed to remain with occasional stirring for two hours,
when the product is diluted with one-third its volume of water and made faintly
but distinctly acid to litmus with 50 per cent acetic acid. The amount of acid
required is about 10 c.c. but the final additions must be made with care because the
fluid will not filter unless the proper condition of acidity is reached. Any difficulty
met at this point may be easily overcome by the alternate addition of acetic acid and
sodium hydroxide and testing a small portion of the material after each addition on
a small flat filter that has been heated with boiling water. When the acidity has
finally been obtained which is favorable to rapid filtration, the material is heated to
vigorous boiling and filtered with a hot water funnel. Under proper conditions the
filtration proceeds with considerable rapidity and continuously leaves a green slime
on the filter and gives a pale yellow filtrate which gelatinizes upon cooling. The
filtrate and washings are evaporated on a water-bath to about 75 c.c and while warm
the concentrated solution is poured slowly into 100 c.c. of 95 per cent alcohol. On
standing over night the precipitated sodium nucleate settles sharply to a spongy
white mass from which the bulk of brown alcoholic fluid can be sharply decanted
and the remainder pressed out with a spatula leaving the material in one cohesive
mass. The substance is washed by decantation in turn with 80 per cent and 95 per
cent alcohol and, after pressing out the last wash fluid as far as possible is transferred
to a flask with 30 c.c of hot water and heated on a water-bath. In half an hour or
less, insoluble phosphates will collect leaving a perfectly transparent interstitial
fluid which is treated with i c.c. of 20 per cent NaOH to lower the viscosity and
filtered with a hot water funnel. The perfectly transparent yellow filtrate is acidi-
fied with acetic acid and poured into 70 c.c. of 95 per cent alcohol when sodium
nucleate wUl be precipitated which can be washed by decantation as before with
alcohol of increasing strength and ground in a mortar with absolute alcohol until
it has crumbled to a fine white powder. If necessary the absolute alcohol may be
decanted and renewed once or twice but not oftener because the nucleate emulsifies
with alcohol after the last traces of acetic acid and sodium acetate have been washed
away. The material is finally .washed on a filter with absolute alcohol and allowed
to dry in a sulphuric acid desiccator. The yield of nucleic acid is about ^.^ grams
from 100 grams of gland. The product is a fine white non-hygroscopic powder

^ From Monograph on "Nucleic Acids" by Waiter Jones: Longmans, Green & Co.

132 PHYSIOLOGICAL CHEMISTRY

that can scarcely be improved by any method of purification. It is a soluble
sodium salt of thymus nucleic acid but is generally referred to simply as thymus
nucleic acid. Very similar or identical substances may be prepared by the same
procedure from other animal tissues, rich in cell nuclei such as the pancreas and
spleen."

10. Tests on Thymus Nucleic Acid. — 1-4. Repeat the experiments as given
under yeast nucleic acid, page 130. 5. Make a 4 per cent solution of thymus nucleic
acid in hot water {% gram to 10 c.c). Allow to cool. What happens? Divide
into two portions. To one add a little NaOH solution; to the other add acetic acid.
Then neutralize carefully in each case.

Both acetic acid and NaOH decrease the viscosity of the nucleate solution. It
may be changed back and forth from the gelatinous to the fluid condition by the
alternate addition of acid and alkali.

11. Tests on Purine Bases and Derivatives. — (a) Xanthine. — i. Silver
Nitrate Reaction. — Dissolve a little xanthine in ammonia and add silver nitrate
solution. Examine a little of the precipitate microscopically. (See page 351.)

2. Copper Sulphate Reaction. — Dissolve a little of the substance in dilute
alkali, make faintly acid with acetic acid. Heat to boiling. Add i c.c. 10
per cent CuSO 4 and then a few drops at a time of sodium bisulphite (saturated
solution) until the precipitate becomes yellowish. All of the purines give this
reaction.

3. Nitric Acid Test. — Place a small amount of the substance in a small
evaporating dish, add a few drops of concentrated nitric acid, and evaporate to
dryness very carefully on a water-bath. The yellow residue upon moistening
with caustic potash becomes red in color and upon further heating assvmies a
purplish-red hue. Now add a few drops of water and warm. A yellow solution
results which yields a red residue upon evaporation. Compare with similar
reaction on other purine bases and uric acid. (See Murexide test, Chapter XXII. )

4. Weidel's Reaction. — Bring a small amount of the substance into solution in
bromine water. Evaporate to dryness on a water-bath. Remove the stopper
from an ammonia bottle and by blowing across the mouth of the bottle direct the
fumes of ammonia so that they come into contact with the dry residue. Under
these conditions the presence of xanthine is shown by the residue assuming a red
color. A somewhat brighter color may be obtained by using a trace of nitric acid
with the bromine water. By the use of this modification, however, we may get a
positive reaction with bodies other than xanthine.

(b) Hypoxanthine. — i. Repeat Experiments i and 3 under Xanthine. Ex-
amine the crystals of hypoxanthine silver nitrate under the microscope. (See
page 351. J

2. Dissolve a little of the substance in a very small amount of hot 6 per cent
nitric acid and allow to cool. Characteristic whetstone crystals of hypoxanthine
nitrate should be formed. Examine under the microscope. (See Fig. 40, page
136.)

(c) Adenine. — i. Warm a few crystals of adenine in a test-tube with a little
water. They should become cloudy at 53°C.

2. Dissolve a httle adenine in hot water and add a few drops of picric acid.
Examine the pale yellow crystals under the microscope. The picrate crystal-
lizes as needle clusters.

3. Repeat Experiment 3 under Xanthine.

NUCLEIC ACIDS AND NUCLEOPROTEINS 1 33

(d) Guanine. — i. Dissolve a little substance in 20 25 times its weight of
boiling 5 per cent alcohol. Allow to cool and examine crystals microscopically.

3. Dissolve a little guanine in 20-25 times its weight of boiling 5 per cent
hydrochloric acid. Allow to cool and examine crystals under microscope.
(See Fig. 39, page 135.)

3. Perform Experiment 3 under Xanthine.

(e) Uric Acid. — i. On a small amount of uric acid try the test as given under
Xanthine number 3. This test on uric acid is called the Murexide test.

2. For other tests on uric acid see Chapter XXII on Urine.

12. Isolation of Guanine and Adenine from Nucleic Acid (Method of Wal-
ter Jones). ^ — The amino purines ma}- be isolated from yeasL or thymus nucleic acid
or from glandular tissue (such as the pancreas) after hydrolysis of the material with
sulphuric acid.

In the case of yeast nucleic acid, heat 10 grams of the substance with 50 c.c. of
10 per cent sulphuric acid on a boiling water-bath for about two hours, replacing
any water lost, or using a condenser tube. To the hot solution add concentrated
ammonia slowly until approximately neutral. Then add enough excess of ammonia
to make about a 2 per cent solution. Filter off the precipitate of guanine and wash
it with I per cent ammonia. Dissolve in as small an amount of 20 per cent sul-
phuric acid as possible, add a little animal charcoal and boil. Filter, heat to boiling
and precipitate with excess of ammonia. Filter, dry the precipitate at 40°C. and
dissolve it in about 20 parts of boiling 5 per cent hydrochloric acid. As the solu-
tion cools guanine chloride separates out as needle-shaped crystals. Filter off,
wash with very dilute hydrochloric acid and dry in the air (do not put in desiccator).
Perform the nitric acid test on the product.

Combine the ammoniacal filtrates obtained in the isolation and purification of
guanine. Filter if necessary. The ammonia may then be boiled off and an excess
of picric acid added in which case a yellow precipitate of adenine picrate is produced
which is filtered off and dried. It is better, however, to neutralize the ammonia of
the combined filtrates and make faintly acid with sulphuric acid. Then precipitate
the adenine as its copper compound (see directions under experiment on Demonstra-
tion of Nucleases B) decomposing this with hydrogen sulphide and evaporating the
filtrate from the copper sulphide to dryness on the water-bath. Dissolve the residue
in hot 5 per cent sulphuric acid and allow to crystallize out. If necessary dissolve
in hot water decolorize with a little charcoal and allow to crystallize out again.
The compound has the formula (C5H5N5)2.HnS04.2H20. Apply the picric acid
and nitric acid tests as given under adenine (page 132).

13. The Pyrimidine Derivatives. The pyrimidine derivatives,
cytosine, thymine, and uracil, are separated from nucleic acid witli
some difficulty. 'J1ie following test may be made on a solution of
cytosine or uracil. Thymine does not give the test.

Wheeler-Johnson Reaction for Uracil and Cytosine. To about 5 c.c. of the
solution under examination add bromine water until the color is permanent.
Avoid the addition of a large excess as this will interfere with the test. In
case the solution contains only small quantities of cytosine or uracil it is advis-
able to remove any excess of bromine by passing a stream of air through the

1 See Walter Jones: Alonograph on " Xucleic .\cids," 1914, Longmans, Circen &. Co.

134 PHYSIOLOGICAL CHEMISTRY

solution. Now add an excess of an aqueous solution of barium hydroxide
and note the appearance of a purple color.

Very dilute solutions do not give the test. Under these conditions
the solution should be evaporated to dryness, the residue dissolved in a
little bromine water and the excess of bromine removed. Then upon
adding an excess of barium hydroxide a decided bluish-pink or lavender
color will appear in the presence of as small an amount as o.ooi gram of
uracil.

In testing solutions for cytosine it is preferable to warm or boil the
solution with bromine water, and after cooling the solution to apply
the test as suggested above, being careful to have a slight excess of
bromine present before adding barium hydroxide.

14. Demonstration of Nucleases and Purinases in Tissues.' — All
glandular tissues contain nucleic acids and enzymes capable of their
hydrolysis as well as the transformation of liberated purine bodies.
By allowing autolysis (self-digestion) to take place in such a tissue and
studying the products formed it is possible to determine what enzymes
were present in the tissue under examination. Typical results may be
obtained by using ox and pig spleens, which differ in the purine enzymes
which they contain. The two experiments should be run in parallel.

A. Preparation of the Material for Digestion. — Run the gland once or tmce
through a meat chopper. Introduce about 650 grams into a two liter bottle, fill
about three-quarters full of water, add 20 c.c. of chloroform, and allow to remain
at room temperature for 12-36 hours with occasional agitation. Strain through
linen and replace the turbid extract in the bottle with 10 c.c. of chloroform. This
solution contains the enzymes and nucleic acid of the tissue. (Reserve 50 c.c.
of one of the extracts for the experiment on phosphonuclease (E), which should
also be started at this time.) The bottle is tightly closed and allowed to remain
in the thermostat 4-5 days.

B. Separation of Purine Derivatives from Other Substances. — Introduce
the products into a saucepan or large evaporating dish, heat to brisk boiling,
make faintly alkaUne with caustic soda, boil a few minutes, make faintly acid with
acetic acid, boil vigorously and filter hot. (If desired one-half of the filtrate may
be treated with 100 c.c. of 20 per cent sulphuric acid per liter and boiled for one
hour, keeping at constant volume. At the end of the hydrolysis the sulphuric acid
is nearly neutralized with caustic soda and the purine bases of the solution
determined as in the other half of the filtrate. This will give information as to
the presence of deaminases acting upon the amino purines remaining in combina-
tion). To the boiUng filtrate add 100 c.c. of 10 per cent copper sulphate and small
successive portions (2-5 c.c.) of sodium bisulphite (commercial saturated solution)
until the precipitate takes on a decided yellow color due to precipitation of cuprous
oxide. Filter, wash the precipitate with boiUng water, pierce the filter and wash
the precipitate into a flask. Add i per cent sodium sulphide solution to decom-

1 From Monograph on "Nucleic Acids" and Laboratory Notes in Physiological Chem-
stry by Professor Walter Jones of Johns Hopkins University, with additions.

NUCLEIC ACIDS AND NUCLEOPROTEINS

135

pose the copper compound continuing the addition until the precipitate becomes
uniformly black and then in small successive portions, testing a drop of the prod-
uct after each addition by bringing it into contact with a drop of lead acetate
on a filter paper. To the boiUng fluid add acetic acid (in the case of the extract
of pig's spleen and other solutions containing guanine the acetic acid should be
replaced by dilute sulphuric) until the insoluble copper sulphide collects and filter
the hot fluid as quickly as possible.

C. Treatment of the Filtrate from Pig's Spleen. — When the filtrate from the
copper sulphide is cold make strongly alkaUne with ammonia and precipitate the
purine compounds with a sUght excess of ammoniacal silver nitrate. Filter, wash
thoroughly with cold water. Pierce the paper, wash the precipitate into a flask
with boihng water and decompose the silver precipitate with hydrochloric acid.
When enough acid has been added the silver chloride will settle as a heavy case-
ous precipitate leaving clear interstitial fluid. Filter and heat the filtrate to
boiling. Treat with an excess of ammonia (enough to make about 1-2 per cent).

Fig. 39. — Guanine Chloride.
(Reproduced from crystals furnished by Professor Walter Jones.)

Allow to cool and filter off the guanine which precipitates. Wash the guanine
with I per cent ammonia and then suspend it in a Uttle hot water and add a few
drops of 20 per cent sulphuric acid to dissolve it. At the boihng point add a Uttle
animal charcoal, boil and filter. Make strongly alkaline with ammonia. Snow
white guanine is precipitated. Dissolve the precipitate in 20 volumes of boiling

5 per cent hydrochloric acid. Upon cooUng beautiful needle-shaped crystals of
guanine chloride separate. (See Fig. 39.)

Evaporate the filtrate from the guanine to dryness on the water-bath to expel
ammonia. Moisten with hydrochloric acid and again evaporate. Treat the
residue with warm water. Does it dissolve almost completely indicating the
absence of xanthine and uric acid? Test a drop of the solution with picric acid.
If no precipitate is obtained adenine is absent. Evaporate to dryness, moisten
with alcohol and again evaporate. Dissolve the residue in about 30 parts of hot

6 per cent nitric acid. On cooUng, characteristic whetstone crystals of hypo-
xanthine nitrate form. ((See Fig. 40, page 136.) The xanthine nitric acid
color test should be practically negative on this product.

136

PHYSIOLOGICAL CHEMISTRY

What does the finding of guanine and hypoxanthine but not adenine or xan-
thine indicate as to the type of purine deaminase present in the pig's spleen?

D. Treatment of Filtrate from Ox Spleen. — The filtrate from the copper sul-
phide should be evaporated to dryness on the water-bath. Extract with cold
water. Test a part of this aqueous solution with picric acid. A lack of precipi-
tate indicates the absence of adenine. To another portion add anmionia (a
lack of precipitate indicates the absence of guanine), and then a Uttle ammo-
niacal silver nitrate solution (lack of appreciable precipitate indicates absence of
purines of any kind in more than traces). Dissolve half of the residue, which
should consist mainly of uric acid and xanthine, in as few drops of concentrated
sulphuric acid as possible and dilute with 4 volumes of water. Stir until the
uric acid begins to separate and then let stand for about three hours. The uric
acid is completely precipitated. Apply the murexide test. To the remainder
of the xanthine-uric acid residue add a Uttle 4 per cent potassiimi hydroxide solu-
tion. Warm and add an equal volume of 30 per cent nitric acid. Allow to cool.

Fig. 40. — Hypoxanthine Chloride.^
(Reproduced from crystals furnished by Professor Walter Jones.)

Xanthine nitrate separates out in a granular form, showing characteristic crystals

under the microscope. Apply the nitric acid test.

What does the presence of uric acid and xanthine and the absence of guanine
and adenine indicate as to the purine enzymes of ox spleen?

E. Demonstration of Nucleotidase (Phosphonuclease). — In this experiment
use the 50 c.c. portion of enzyme solution retained from Experiment A preceding.
Prepare a 2 per cent solution of yeast nucleic acid aiding the solution by the slow
addition of KOH solution until the reaction, as indicated by a few drops of Utmus
added, is neutral. Prepare a series of three large test-tubes as follows : In No. i
place 10 c.c. of enzyme solution and 5 c.c. of nucleic acid. In No. 2 place 10 c.c.
of enzyme solution and 5 c.c. of water. In No. 3 place 10 c.c. of enzyme solution,
boiled and 5 c.c. of nucleic acid. To each tube add 2-3 c.c. each of CHCI3 and
toluol as preservatives. Place the tubes at 37°C. for 24 hours. Add i c.c. of
litmus solution to each tube and note whether any changes in reaction have taken
place. Put the tubes in boihng water for a few minutes to coagulate proteins
Then add 5 c.c. of 5 per cent HCl and let stand for an hour. This precipitates.

^Hypoxanthine nitrate crystallizes in similar form.

NUCLEIC ACIDS AND NUCLEOPROTEINS 1 37

any unaltered nucleic acid which may be present. Filter and take an aliquot
portion of each filtrate (15 c.c). Add magnesia mixture and a few cubic centi-
meters of strong ammonia. Let stand over night. Any phosphoric acid present
will be precipitated as magnesium ammonium phosphate. Observe the relative
amounts of phosphate in each case. Has any phosphate been set free from the
nucleic acid added? From the nucleic acid of the gland extract?

15. Experiments on Uricase (Uricolytic Enzyme). — A. Preparation of Extract
Containing Uricase. — Extract about 50 grams of pulped kidney tissue of the ox
with 200 c.c. of toluol or chloroform water at 38°C. for 24 hours, with occasional
shaking. Filter and use the filtrate in the following experiment.

B. Demonstration of Uricase. — Add about o.i gram of uric acid to 10 c.c.
of water and bring the uric acid into solution by the addition of the minimal quan-
tity of KOH. To 5 c.c. of this uric acid solution in a test-tube add 50 c.c. of the
uricoljrtic enzjrme extract prepared as described above. Prepare a second tube
containing a like amount of the uric acid solution but boil the extract before
it is introduced. Place the two tubes at 38°C. for two days. The vessels should
be open to the air and the contents stirred occasionally, or much better, a con-
tinuous current of air which has gone through a chloroform wash bottle is passed
through the mixture. Make both mixtures faintly acid with acetic acid and
boil. Filter and take an aUquot of each filtrate. Evaporate to low volume, make
faintly alkaUne with ammonia and filter. Add a few cubic centimeters of
ammoniacal silver nitrate solution. Any uric acid will be precipitated as silver
urate. The control should give a heavy precipitate while the test should show
no precipitate or one much lighter than the control, due to uric acid destruction in
the latter case.

If it is desired to separate out the pure uric acid the silver-purine precipitate
may then be filtered off. It is washed with water and transferred to a beaker with
the aid of a httle water. To the mixture add a few cubic centimeters of hydrogen
sulphide solution and a few drops of HCl and allow to stand over night. The uric
acid should separate out in crystaUine form and should be found in less amount
in the test than in the control experiment. The uric acid may also be titrated
with permanganate as in the FoUn-Shaflfer method for uric acid in urine. See
Chapter XXVI on Quantitative Analysis of Urine.) This will enable us to
determine exactly how much of the uric acid was destroyed through the action
of the enzyme extract.

CHAPTER VII
GASTRIC DIGESTION

Gastric digestion takes place in the stomach and is promoted by
the gastric juice, which is secreted by the glands of the stomach mucosa.
These glands are of two kinds, fundus glands and pyloric glands which
are situated, as their names imply, in the regions of the fundus and
pylorus. The principal foods acted upon in gastric digestion are the
proteins which are so changed by its processes as to become better pre-
pared for further digestion in the intestine and for their final absorption.

From reliable experiments made upon lower animals it is evident
that the gastric juice is secreted as the result of stimuli of two forms,
i.e., psychical stimuli and chemical stimuli. The psychical form of
stimuli may be produced by the sight, thought, or taste of food, and the
chemical stimuli may be produced by certain substances, such as water,
milk, the extractives of meat, etc., when coming in contact with the
stomach mucosa. The stimulatory power of water has been very
strikingly demonstrated.^ The claim that the drinking of water with
meals is harmful because such a procedure causes a dilution of the gastric
juice, has no basis in fact. The drinking of water with meals by normal
individuals has been found to be accompanied by a more economical
utilization of the ingested proteins, fats and carbohydrates. Various
other desirable and no undesirable features have been demonstrated
as accompanying or following such a dietary procedure.^ No experi-
mental evidence has been submitted which can justly be interpreted as
showing any harmful influence to accompany or follow the drinking,
by normal persons, of large quantities of water at meal time.

The volume of gastric juice secreted during any given period of
digestion varies with the quantity and kind of the food. These con-
clusions were deduced principally from a series of so-called delusive
feeding experiments. A dog was prepared with two esophageal open-
ings and a gastric fistula. When thus prepared and fed foods of various

^ Foster and Lambert: Journ. Exper. Med., lo, 820, 1908.

Bergeim, Rehfuss and Hawk: Jour. Biol. Chem., 19, 345, 1914.
2 Hawk: University of Pennsylvania Medical Bulletin, 18, i, 1905.

Fowler and Hawk: Jour. Exper. Med., 12, 388, 1910.

Hattrem and Hawk: Arch. Int. Med., 7, 610, 1911.

Mattill and Hawk: Jour. Am. Chem. Soc, 33, pp. 1978, 1999, and 2019, 1911.

Hawk: Arch. Int. Med., 8, 382, 191 1.

Hawk: Proceedings Soc. Exp. Biol, and Med., 8, 36, 1910.

Fairhall and Hawk: Jour. Am. Chem. Soc, 34, 546, 1912.

Howe and Hawk: Jour. Biol. Chem., 11, 129, 1912.

Hawk: Biochem. Bull., 3, 420, 1914.

138

GASTRIC DIGESTION 1 39

kinds such as meat and bread, the material instead of passing to the
stomach, would invariably find its way out of the animal's body at the
upper esophageal opening. Through the medium of the gastric fistula
the course of the secretion of gastric juice could be carefully followed.
It was found that when the dog ate meat, for example, there was a large
secretion of gastric juice notwithstanding no portion of the food eaten
had reached the stomach. Further experiments made through the
medium of a cul-de-sac formed from the stomach wall have given us
many valuable conclusions, among others those regarding the influence
of the chemical stimuli. The method followed was to feed the animal
certain substances and note the secretion of gastric juice in the miniature
stomach while the real process of digestion was taking place in the
stomach proper.

Normal gastric juice is a thin, light colored fluid which is acid in
reaction and has a specific gravity varying between i.ooi and i.oio.
It contains only 2-3 per cent of solid matter which is made up prin-
cipally of hydrochloric acid, sodium chloride, potassium chloride, earthy
phosphates, mucin and the enzymes pepsin, gastric rennin, and gastric
lipase; the hydrochloric acid and the enzymes are of the greatest impor-
tance. The acidity of the gastric juice is due to /ree hydrochloric acid.
It was formerly believed that this acid was secreted by the parietal cells
of the fundus as well as by the chief cells of both the fundus and pyloric
glands. It has been claimed,^ however, that the parietal cell is the
seat oj the formation of the hydrochloric acid. This conclusion is based
upon the formation of Prussian blue after the subcutaneous injection of
potassium ferrocyanide and ammonium ferric citrate (rabbits and
guinea-pigs) and the subsequent (3 to 30 hours) microscopical examina-
tion of the gastric mucosa. The acid was shown to be present in the
lumina of the gland tubules and in the canaliculi of the parietal cells;
traces were also apparently present in the cytoplasm. Later Bensley
and Harvey- showed by means of dyes which act as vital stains and
as indicators very sensitive to alkali that the secretion in the parietal
cells is slightly alkaline whereas that in the lumen of the gland proper
is very nearly neutral. Therefore, the acid is formed entirely above the
level of the gland proper, i.e., in the foveolae and on the surface. Ham-
met^ and still more recently Macallum and Collip'* have confirmed Miss
Fitzgerald's claim that the acid is formed in the parietal cells.

It was believed that hydrochloric acid was generally present in the
gastric juice of man to the extent of about 0.2 per cent. Wlien the

^ Fitzgerald: Proceedings Royal Society (B), 83, 56, 1910.

- Bensley and Harvey: Biological Bulletin, 23, 225, 1912.

' Hammett: Anatomical Record, g, 21, 1915.

* Reported before Society of Biological Chemists, Boston, Dec. 27, 1915.

I40 PHYSIOLOGICAL CHEMISTRY

amount of hydrochloric acid varied to any considerable degree from this
value a condition of hypoacidity or hyperacidity was said to be es-
tablished. On the basis of more recent experiments/ however, it
appears that the actual acidity of the gastric juice of man as secreted
by the glands is 0.4 to 0.5 per cent hydrochloric acid. Boldyreff be-
lieves that this acidity is lowered to about 0.2 per cent by regurgitation
of alkaline fluid from the intestine (Chapter VIII on Gastric Analysis).
Hydrochloric acid has the power of combining with protein substances
taken in the food, thus forming so-called combined hydrochloric acid.
This combined acid is a less potent germicide than free hydrochloric
acid and has less power to destroy the amylolytic enzyme salivary
amylase (ptyalin) of the saliva. This last fact explains to a degree the
possibility of the continuance of salivary digestion in the stomach.

The term combined hydrochloric acid is really a misnomer. WTien
free hydrochloric acid is treated with a protein the latter functions as
a base and a salt is formed. Therefore, instead of having ''com-
bined hydrochloric acid" we have a protein salt of hydrochloric acid.
This salt ionizes differently from the free acid. This fact explains the
variation in the germicidal properties of the two solutions as well as
their different action toward enz\'mes, such, for example, as salivary
amylase (see page 61).

The hydrochloric acid of the gastric juice forms a medium in which
the pepsin can most satisfactorily digest the protein food, and at the
same time it acts as an antiseptic or germicide which prevents putre-
factive processes in the stomach. It also possesses the power of inverting
cane sugar, this property being due to the hydrogen ion. When the
hydrochloric acid of the gastric juice is diminished in quantity (hypoacid-
ity) or absent, as it may be in many cases of functional or organic dis-
ease, there is no check to the growth of micro-organisms in the stomach.
There are, however, certain of the more resistant spores which even the
normal acidity of the gastric juice \\\\\ not destroy. A condition of
hypoacidity may also give rise to fermentation with the formation of
comparatively large amounts of such substances as lactic acid and
butyric acid.

The question of the origin of the hydrochloric acid of the gastric
juice is a problem to whose solution many investigators have given
much attention. Many theories have been proposed, among them the
interaction of sodium chloride with carbonic acid,^ with acid phosphate^

^ Babkin: Die iiussere Sekretion der Verdauungsdriisen, Berlin, 1914, p. 113.

Boldyreff: Quart. Jour. Exper. Physiol., 8, i, 1914.

Carlson: Am. Jour. Physiol., 38, 248, 19 15.
^ Bunge: Physiologic and Pathologic Chemistry, 2nd. Eng. Ed., Philadelphia, 1902, p. 135.
^Maly: Zeit. f. physiol. Chem., i, 174, 1877. ]Macallum and Collip: Reported before
the Society of Biological Chemists, Boston, Dec. 27, 1915.

GASTRIC DIGESTION 141

or with organic acids. On the other hand, it is possible that hydro-
chloric acid is set free from* combination with some weak base as
ammonia^ or that free phosphoric acid valences may be set free by the
enzymic hydrolysis of organic phosphoric acid esters.- We cannot go
into a discussion of these various theories. That the hydrochloric
acid arises from the chlorides of the blood appears to be well established
but the same cannot be said with regard to the immediate or ultimate
origin of the hydrogen ions involved in the reaction.

The most important of the enzymes of the gastric juice is the pro-
teolytic enzyme pepsin. The pepsin does not originate as such in the
gastric cells but is formed from its precursor, the z\ mogen or mother-
substance pepsinogen, which is apparently produced by the parietal
cells of the fundus as well as by the chief cells of the fundus and pyloric
glands. Pepsinogen may be differentiated from pepsin from the fact
that it is more resistant to alkali.'^ Upon coming into contact with the
hydrochloric acid of the secretion this pepsinogen is immediately trans-
formed into pepsin. Pepsin is not active in alkaline or neutral solutions,
but requires at least a faint acidity before it can exert its power to dis-
solve and digest proteins. The percentage of hydrochloric acid facili-
tating the most rapid peptic action varies with the character of the
protein acted upon, e.g., 0.08 per cent to o.i per cent for the digestion of
fibrin and 0.25 per cent for the digestion of coagulated egg-white.
While hydrochloric acid is the acid usually employed to promote arti-
ficial peptic proteolysis, other acids, organic and inorganic, will serve the
same purpose. Acidity of the liquid is necessary to promote the
activity of the pepsin, but the acidity need not necessarily be confined
to hydrochloric acid.

In common with many other enzymes pepsin acts best at about
38°-4o°C. and its digestive power decreases as the temperature is low-
ered, the enzyme being only slightly active at o°C. Its power is only
temporarily inhibited by the appHcation of such low temperatures,
however, and the enzyme regains its full proteolytic power upon rais-
ing the temperature to 40°C. As the temperature of a digestive mix-
ture is raised above 4o°C. the pepsin gradually loses its activity
until at about 8o°-ioo°C. its proteolytic power is permanently
destroyed.

Our ideas regarding the nature of the products formed in the course
of peptic proteolysis have undergone considerable revision in recent
years. The former view that these products included only acid albu-
minate (acid metaprotein), proteoses, peptones and peptides is no

^Mathews: Physiological Chemistry, New York, 1915, p. 374.
- Bergeim: Proc. Soc. Exp. Biol, and ^led., 12, 21, 1914.
^Langley: Jour, of Physiol., 3, 246.

142 PHYSIOLOGICAL CHEMISTRY

longer tenable. From the investigations of numerous observers we
have learned that artificial gastric digestion if permitted to proceed for a
sufficiently long period will yield, in addition to proteoses, peptones and
peptides, a long list of protein cleavage products which are crystalline
in character, including leucine, tyrosine, alanine, phenylalanine, aspartic
acid, glutamic acid, proline, leucinimide, valine, and lysine. A similar
group of substances may result from the action of the enzyme trypsin
(see page i86). The relative amounts of proteoses, peptones, and crys-
talline substances formed depends to a great extent upon the character
of the protein undergoing digestion, e.g., a greater proportion of pro-
teoses results from the digestion of fibrin than from the digestion of
coagulated egg-white. We must not be led into the error of thinking
that the large number of protein cleavage products just mentioned are
formed in the course of normal gastric digestion within the animal
organism. They are formed only after comparatively long-continued
hydrolysis. In pancreatic digestion, however, there are formed even
under normal conditions the large number of cleavage products to
which reference has been made. Peptic proteolysis, therefore, within
the animal organism differs from tryptic proteolysis (see page i86)
in that the former yields larger amounts of proteoses, smaller amounts
of peptones and no considerable quantity of crystalline bodies as end-
products in the brief period during which proteins are ordinarily sub-
jected to gastric digestion. Prolonged hydrolysis with gastric juice
does, however, yield considerable quantities of the non-protein end-
products. In cases of cancer of the stomach a peptide-splitting
enzyme (erepsin) is said to be present in the stomach contents. This
enzyme is believed to be elaborated by the cancer tissue and its identi-
fication is of importance in connection with the diagnosis of gastric
cancer. The glycyl-trytophane test^ is sometimes used for this
purpose. This test has been very severely criticized (see page 199).
Abderhalden and Meyer^ have shown active pepsin to be present
in the contents of all parts of the small intestine. It is suggested that
pepsin may be adsorbed in the stomach by such protein substances
as pass into the intestine in solid form and that the pepsin thus pro-
tected may bring about gastric digestion whenever the reaction of the
surrounding intestinal contents is favorable. This fact may be of
importance in connection with the profound proteolysis taking place
in the intestine. Heretofore, this process was believed to be furthered
alone by trypsin and erepsin. The passage of adsorbed pepsin into the
intestine may be an efficient aid to the proper digestion of solid proteins

^ Neubauer and Fischer: Dent. Arch.f. klin. Med., 97, 499, 1909.
'^Abderhalden and Meyer: Zeit. fur physiol. Chem., 74, 67, 191 1.

GASTRIC DIGESTION 1 43

which are ingested without sufficient mastication (" bolted ") ^ and which
consequently, at times, pass into the intestine in rather large pieces
(see Chapter XIV on Feces).

Gastric rennin, the second enzyme of the gastric juice, is what is
known as a milk curdling or protein coagulating enzyme. Rennin acts
upon the casein of the milk, splitting it into a peptone-like body and
soluble paracasein. This soluble body, in the presence of calcium
salts, combines with calcium, forming calcium paracasein which is
insoluble and precipitates. There is some uncertainty regarding
the reaction to litmus in which gastric rennin shows the greatest
activity. It is, however, said to be active in neutral, alkaline, or acid
solution. However, it probably possesses its greatest activity in the
presence of a sUght acid reaction, as would naturally be expected. It
is especially abundant in the gastric mucosa of the calf, and is used
to curdle the milk used in cheese making. Gastric rennin is always
present normally in the gastric juice, but in certain pathological con-
ditions such as atrophy of the mucosa, chronic catarrh of the stomach,
or in carcinoma it may be absent.

The theory that the proteolytic activity and the milk curdling prop-
erty of the gastric juice reside in a single substance is causing much
controversy at the present time. The theory was originally advanced
by the Pawlow school.^ According to Xencki and Sieber,^ the milk
curdling and protein hydrolyzing activities reside in definite and distinct
side chains of a single mammoth molecule. The view which has rather
the strongest support, however, is to the eft'ect that there are two entirely
distinct enzymes. Important evidence has been advanced in favor of
this view by Hammarsten,^ Taylor,^ and Hemmeter.^ Burge^ has re-
ported experiments upon the influence of a direct electric current upon
solutions possessing typical rennin and peptic activities. By this
means he was able to prepare a solution possessing strong rennin
activity but entirely devoid of peptic activity. This furnishes strong
evidence against the identity of the two enzymes but does not neces-
sarily deny the accuracy of the side-chain theory.

Gastric lipase, the third enzyme of the gastric juice, is a fat-splitting
enzyme. It possesses but slight activity when the gastric juice is of
normal acidity, but evinces its action principally at such times as a

^ Foster and Hawk: Proceedings of the Eighth International Congress of Applied Chem-
istry, New York, September, 191 2.

^ Pawlow and Parastschuk: Zeitschrift fiir Physiologische Chemie, 42, 415, 1904.
' Nencki and Sieber: Zeilschrift fiir Physiologische Chemie, 23, 191, 1901.
*Hammarsten: Zeilschrift fiir Physiologische Chemie, 56, 18, 1908; 94, 291, 1915.

* Taylor: Journal of Biological Chemistry, 5, 399, 1909.

• Hemmeter: Berliner klinischc Wochenschrtft, Ewald Festnummer, 44, 1905.
^ Burge: American Journal of Physiology, 29, 191 2.

144 PHYSIOLOGICAL CHEMISTRY

gastric juice of low acidity is secreted either from physiological or patho-
logical cause. The digestion of fat in the stomach is, however, at
most, of but slight importance as compared with the digestion of fat in
the intestine through the action of the lipase of the pancreatic juice
(see page i88).

Boldyreff^ has shown trypsin to be present in stomach contents, due
to regurgitation of intestinal contents through the pylorus. This claim
has been verified by others- (see Chapter VIII on Gastric Analysis) .

PREPARATION OF AN ARTIFICIAL GASTRIC JIHCE

Dissect the mucous membrane of a pig's stomach from the muscular portion
and discard the latter. Divide the mucous membrane into two parts (4/5 and
1/5). Cut up the larger portion, place it in a large-sized beaker with 0.4 per cent
hydrochloric acid and keep at 38°-40°C. for at least 24 hours. Filter ofif the
residue, consisting of nuclein and other substances, and use the filtrate as
an artificial gastric juice. This filtrate contains pepsin, rennin, and the prod-
ucts of the digestion of the stomach tissue, i.e., acid metaprotein (acid albu-
minate), proteoses, peptones, etc.

Preparation of a Glycerol Extract of Pig's Stomach

Take the one-fifth portion of the mucous membrane of the pig's stomach not
used in the preparation of the artificial gastric juice, cut it up very finely, place it
in a small-sized beaker and cover the membrane with glycerol. Stir frequently
and allow to stand at room temperature for at least 24 hours. The glycerol will
extract the pepsinogen. Separate, with a pipette or by other means, the glycerol
from the pieces of mucous membrane and use the glycerol extract as required in
the later experiments.

Products of Gastric Digestion

Into the artificial gastric juice, prepared as above described, place the protein
material (fibrin, coagulated egg-white, or lean beef) provided for you by the
instructor, add 0.4 per cent hydrochloric acid as suggested by the instructor and
keep the digestion mixture at 40°C. for two to three days. Stir frequently and
keep free hydrochloric acid present in the solution (for tests for free hydro-
chloric acid see page 152).

The original protein has been digested and the solution now contains the
products of peptic proteolysis, i.e., acid metaprotein (acid albuminate), proteoses,
peptones, etc. The insoluble residue may include nuclein and other substances.
Filter the digestion mixture and after testing for free hydrochloric acid neutralize
the filtrate with potassium hydroxide solution. If any of the acid metaprotein
(acid albuminate) is still untransformed into proteoses it will precipitate upon
neutraUzation. If any precipitate forms heat the mixture to boiling, and filter.
If no precipitate forms proceed without filtering.

1 Boldj'reff: Quart. Jour. Exper, Physiol., 8, i, 1914.

^ Spencer, Meyer, Rehfuss and Hawk: Am. Jour. Physiol, 39, 459, 1916.

GASTRIC DIGESTION 145

We now have a solution containing a mixture consisting principally of proteo-
ses and peptones. Separate and identify the proteoses and peptones according
to the directions given on pages 119 and 120.

GENERAL EXPERIMENTS ON GASTRIC DIGESTION

1. Conditions Essential for the Action of Pepsin. — Prepare four test-tubes as
follows :

(a) Five c.c. of pepsin solution.

(b) Five c.c. of 0.4 per cent hydrochloric acid.

(c) Five c.c. of pepsin-hydrochloric acid solution.

(d) Two or 3 c.c. of pepsin solution and 2-3 c.c. of 0.5 per cent sodium car-
bonate solution.

Introduce into each tube a small piece of fibrin and place them in the incu-
bator or water-bath at 40°C. for one-half hour, carefully noting any changes which
occur. ^ (Carmine-fibrin may be used to advantage in this and the following tests
under Gastric Digestion. In this case, however, the experiments should be con-
ducted at room temperature. For directions as to the preparation of carmine-
fibrin see Chapter I.) Now combine the contents of tubes (a) and fb) and
see if any further change occurs after standing at 40°C. for 15-20 minutes. Ex-
plain the results obtained from these five experiments.

2. Influence of Different Temperatures. — In each of four test-tubes place 5
c.c. of pepsin-hydrochloric acid solution. Immerse one tube in cold water from
the faucet, keep a second tube at room temperature and place a third in the
incubator or water-bath at 40°C. Boil the contents of the fourth tube for a few
moments, then cool and also keep it at 40°C. Into each tube introduce a small
piece of fibrin and note the progress of digestion. In which tube does the most
rapid digestion occur? Explain this.

3. The Most Favorable Acidity. — Prepare three tubes as follows :

(a) Five c.c. of 0.2 per cent pepsin-hydrochloric acid solution.

(b) Two or 3 c.c. of 0.2 per cent hydrochloric acid + i c.c. of concentrated
hydrochloric acid + 5 c.c. pepsin solution.

(c) One c.c. of 0.2 per cent pepsin-hydrochloric acid solution + 5 c.c. of
water.

Introduce a small piece of fibrin into each tube, keep them at 40'C., and note
the progress of digestion. In which degree of acidity does the fibrin digest the
most rapidly?

4. Differentiation between Pepsin and Pepsinogen. — Prepare five tubes as
follows :

(a) Few drops of glycerol extract of pepsinogen + 2-3 c.c. of water.

(b) Few drops of glycerol extract of pepsinogen + 5 c.c. of 0.2 per cent hydro-
chloric acid.

(c) Few drops of glycerol extract of pepsinogen + 5 c.c. of 0.5 per cent sodium
carbonate.

^ Digestion of fibrin in a pepsin-hydrochloric acid solution is indicated first by a swelling
of the protein due to the action of the acid, and later by a disinlegration and dissolving of
the fibrin due to the action of the pepsin-hydrocliloric acid. If uncertain at any time
whether digestion has taken place, the solution under examination may be filtered and the
biuret test applied to the filtrate. A positive reaction will signify tlie presence of acid
metaprotein (acid albuminate), proteoses (albumoses), or peptones, the presence of any
one of which would indicate that digestion has taken place.

146 PHYSIOLOGICAL CHEMISTRY

(d) Two or 3 c.c. of pepsin solution + 2-3 c.c. of i per cent sodium carbonate.

(e) Few drops of glycerol extract of pepsinogen + 5 c.c. of i per cent sodium
carbonate.

Add a small piece of fibrin to the contents of each tube, keep the five tubes at
40°C. for one-half hour and observe any changes which may have occurred. To
(a) add an equal volume of 0.4 per cent hydrochloric acid, neutraUze (c), (d) and
(e) with hydrochloric acid and add an equal volume of 0.4 per cent hydrochloric
acid. Place these tubes at 4o°C. again and note any further changes which may
occur. What contrast do we find in the results from the last three tubes?
On the basis of these tests what is the relative resistance of pepsin and pepsinogen
to alkaUs?

5. Comparative Digestive Power of Pepsin with Different Acids. — Prepare a
series of tubes each containing a N/io solution of one of the following acids:
hydrochloric, sulphuric, nitric, combined hydrochloric, acetic, lactic and oxalic.
To each acid add a few drops of the glycerol extract of pig's stomach and a small
piece of fibrin. Shake well, place at 40°C., and note the progress of digestion.
In which tubes does the most rapid digestion occur?

6. Influence of MetaUic Salts, etc. — Prepare a series of tubes and into each
tube introduce 4 c.c. of pepsin-hydrochloric acid solution and 3-^ c.c. of one of the
chemicals listed in Experiment 18 under Salivary Digestion, page 61. Introduce a
small piece of fibrin into each of the tubes and keep them at 40°C. for one-half hour.
Note the variations in the progress of digestion. Where has the least rapid diges-
tion occurred?

7. Sahli's Desmoid Reaction. — This is a method for testing gastric function
without using the stomach tube. The underlying principle of the test is the fact
that raw cagtut may be digested in gastric juice but is entirely indigestible in
pancreatic juice. The test is made as follows : A methylene -blue pill is intro-
duced into a small rubber bag and the mouth of the bag subsequently tied with
catgut. 1 The small bag is then ingested immediately after the mid-day meal and
the urine examined 5, 7, 9 and 18-20 hours later for methylene blue. If methyl-
ene blue is present in appreciable quantity, it will impart to the urine a greenish-
blue color. If not present in sufficient amount to impart this color the urine should
be boiled with one-fifth its volume of glacial acetic acid, whereupon a greenish-
blue color results if the chromogen of methylene blue is present. This contin-
gency seldom arises, however, inasmuch as in most cases of uncolored urine it will
be found that the rubber bag has passed through the stomach unopened. If the
methylene blue is found in the urine inside of 18-20 hours a satisfactory gastric
function is indicated.

For Einhorn's bead method for the study of digestive function see chapter on
Feces.

8. Testing the Motor and Functional Activities of the Stomach. — This
test is performed the same as Experiment 19 under Salivary Digestion, page 61.
If the experiment was carried out under salivary digestion it will not be neces-
sary to repeat it here.

' About 0.05 gram of methylene blue is mixed with sufficient ext. glycyrrhiza to form
a pill about 3-4 mm. in diameter. The pill is then placed in the center of a square
piece of thin rubber dam and a little bag-like receptacle constructed by a twisting
movement. The neck of the bag is then closed by wrapping three turns of catgut about
it. The most satisfactory catgut to use is number 00 raw catgut which has previously
been soaked in water until soft. When ready for use the bag should sink instantly when
placed in water and be water-tight.

GASTRIC DIGESTION 1 47

9. Influence of Bile. — Prepare three tubes as follows :

(a) Five cc. of pepsin-hydrochloric acid solution -r 1/2-1 c.c. of bile.

(b) Five c.c. of pepsin-hydrochloric acid solution -f- 5 c.c. of bile.

(c) Five c.c. of pepsin-hydrochloric acid solution.

Introduce into each tube a small piece of fibrin. Keep the tubes
at 40°C. and note the progress of digestion. Does the bile exert any
appreciable influence?-' How?

10. Influence of Gastric Rennin on Milk. — Prepare a series of five tubes as
follows :

(a) Five c.c. of fresh milk — 0.2 per cent hydrochloric acid add slowly until
precipitate forms .

(b) Five c.c. of fresh milk — 5 drops of rennin solution.^

(c) Five c.c. of fresh milk — 10 drops of 0.5 per cent sodium carbonate solu-
tion.

(d) Five c.c. of fresh milk — 10 drops of a saturated solution of ammonium
oxalate.

(e) Five c.c. of fresh milk — 5 drops of 0.2 percent hydrochloric acid. Now to
eachof the tubes c , d ,and 'e; adds drops of rennin solution. Place the whole
series of five tubes at 40^C. and after 10-15 minutes note what is occurring in the
different tubes. Give a reason for each partictilar result. How do ammonium
oxalate and sodium carbonate prevent coagulation?

^ Any good commercial rennin or rennet preparation may be used in preparing this
solution.

CHAPTER VIII

GASTRIC ANALYSIS

The method of gastric analysis which has been in vogue clinically
for years (see page 174) entails the feeding of a standard test meal,
the removal of the complete stomach contents at the end of a one-
hour period, and the analysis of the material so removed. That this
method is inaccurate has been repeatedly demonstrated in the author's
laboratory^ and elsewhere.^ Furthermore, owing to the bulk of the
old form of stomach tube and the discomfort occasioned by its use, it
is impossible to follow the whole cycle of digestion and estimate, step

Time

Ihr.

2hr.

Fig. 41. — Normal and Pathological Curves after an Ewald Meal.

I. normal curve; 2 delayed digestion with late hyperacidity; 3, larval hyperacidity;
4, tardive hyperacidity; 5, marked continued secretion from obstruction.

by step, the exact changes which take place in the stomach after the
introduction of definite food mixtures into that organ.

Realizing the inadequacy of the procedure entailed in the old
method of gastric analysis, a new procedure has been developed by Dr.
Martin E. Rehfuss in the author's laboratory. This so-called "Frac-
tional Method" entails the analysis of samples of material withdrawn
from the stomach (by syringe) at short intervals for a period of two
hours or more (until stomach is empty) after the ingestion of the test
meal. By this means the observer is able to follow the entire cycle of

' Rehfuss: Jour. Am. Med. Ass'n, 64, 569, 1914.

Rehfuss, Bergeim and Hawk: Jour. Am. Med. Ass^n, 63, 909, 1914.

Bergeim, Rehfuss and Hawk: Jour. Am. Med. Ass^n, 63, 11, 1914.
* Harmer and Dodd: Arch. Int. Med., Nov. 13, 1913, p. 488.

148

GASTRIC ANALYSIS

149

gastric digestion and is not limited, as in the old method, to information
derived from the analysis of a single sample of stomach contents with-
drawn at the end of one hour. That the acid values obtained by the
old method may be grossly misinterpreted and lead to an incorrect
diagnosis is indicated by the foregoing diagram (Fig. 41):

It is set forth in the above diagram that various t>'pes of abnormal
gastric secretion would be considered normal on the basis of a single
examination at the end of one hour whereas the application of the
fractional method reveals the abnormality of the secretion and enables
a rapid and correct diagnosis. The removal of samples of gastric
contents at short intervals, for a period of two hours or more after a
test meal, is made possible by the use of a modified stomach tube^ of
small diameter (No. 12 French tubing) and fitted with a metal tip.

Fig. 42. — Rehtuss Stomach Tube.

The tip is slotted ^^'ith large perforations, the diameter of each being
equivalent to the maximum bore of the tubing. Such a tube can be
left in the stomach through the entire cycle of gastric digestion \Nithout
inconvenience to the patient.- A cut of the Rehfuss stomach tube
(Fig. 42) is shown above. ^

The idea of making a fractional examination of gastric contents is
not new. Most of such attempts have been made, however, by using
the old t^-pe of stomach tube and removing the entire stomach contents
at different intervals on successive days, e.g., after fifteen minutes the
first day, thirty minutes the second day, forty-five minutes the third
day, etc. Hayem* was the first to employ this method and later

1 Rehfuss: Am. Jour. Med. ScL, June, 1914.

^ McClendon has recently suggested the introduction of an electrode into the stomach in
an attempt to follow the consecutive changes in the hydrogen ion concentration of the
stomach contents (see .4w. Jour. Physiol., 38. 180, 1915).

' This tube is manufactured by Charles Lentz & Sons, Philadelphia.

* Hayem: Brouardel & Gilbert's, Traitc dc Mcdcciue, 4, 236, 1905.

I50

PHYSIOLOGICAL CHEMISTRY

Ewald and Boas/ Reichmann,- v. Jaksch,^ Kornemann,^ Schule^ and
Gregersen^ followed a similar procedure. The first report of data from
the entire gastric cycle obtained by means of a small bore tube were
made by Ehrenreich.'^ This investigator used a Nelaton catheter.
Skaller^ has reported a few experiments in which a small bore stomach
tube with a metal tip was employed and the stomach contents
subjected to fractional analysis.

Until recent years, the concensus of opinion based principally upon
the work of the Pawlow schooP was to the effect that the gastric juice

Total additij

Frceacufity

Trgpsln

I20niinates

Diet. 100cx:.o^ 0.542 7oHCl at23X

F G, 43. — Influence of Acid Introduced into the Normal Human Stomach.
{Spencer, Meyer, Rehfiiss and Hawk: American Journal of Physiology, March, 1916.)

of normal man had an average acid concentration of 0.2 per cent
hydrochloric acid, whereas the gastric juice of the dog and cat had an
average acid concentration of 0.4-0.5 per cent hydrochloric acid.
These experiments were based principally upon the examination of
the pure gastric juice of the lower animals as compared with the stomach

' Ewald & Boas: Virchow's Arch., loi, 325, 1885.
2 Reichmann: Zeit. f. klin. Med., 24, 565, 1885.
* V. Jaksch: Zeit. f. klin. Med., 19, 383, 1890.
*Kornemann: Arch. f. Verdauungskr., p. 369, 1912.
'Schule: Zeit. f. klin. Med., 27, 461, 1895.
*Gregersen: Arch. f. Verdauungskr., 19, 263, 1913.
^ Ehrenreich: Zeit.f. klin. Med., p. 231, 1912.
^Skaller: Berl. klin. Woch., 50, No. 47, 1913.

» Pawlow: The Work of the Digestive Glands. Translated by Thompson, Second Edition,
1910.

GASTRIC ANALYSIS

151

contents of man. Later experiments' have, however, demonstrated
that the acid concentration of the freshly secreted gastric juice of man
is similar to that of the dog, i.e., 0.4-0.5 per cent. Boldyreff claims
that this initial high acidity of the human gastric juice is normally
lowered to the "optimum acidity" of 0.15-0.2 per cent hydrochloric
acid by regurgitation of alkaline fluids (bile, pancreatic and intestinal
juices) from the intestine. This claim has been substantiated by
experiments made in the author's laboratory- and elsewhere.'^ Both
bile and tr>'psin are easily identified in the stomach contents of man
after the introduction of 0.5 per cent hydrochloric acid into the empty
organ. The above points are illustrated by the chart shown in Fig.
43, page 150."

The composition of human gastric juice and of the residuum (see
page 160) is given in the following table:

COMPOSITION OF HUMAN GASTRIC JUICE.

Constituent

Appetite juice^

Residuum'

Specific gravity

1 .007

1.006

A degrees

-0-55

-0.47

Total acidity, per cent

0.45 0.30

Per 100 CO. of Juice j

1

Total solids, gram

Organic solids, gram

0.55 j 0.98^

0.41

0.53^

Inorganic solids, gram

0.14

0.45^

Total nitrogen, gram

0.060

0.066^

Total phosphorus, gram

0.005^

Total sulphur, gram

0.007^

Ammonia N, gram

0.002-3

Amino-acid N, gram

0 . 003-9

Chlorides, gram

0-5

1

1 Babkin: Die Aussere Sekretion der Verdauungsdriisen, Berlin, 1914.

Boldyreff: Transactions of nth Congress of Physicians, St. Petersburg, 1909.

Boldyreff: Quart. Jour. Exp. Med., 8, i, 19 14.

Carlson: Am. Jour. Physiol., 38, 248, 1915.

Bergeim, Rehfuss & Hawk: Jour. Biol. Client., 19, 345, 19 14.
- Spencer, Meyer, Rehfuss and Hawk: Ai>i. Jour. Physiol., 39, 459, 1916.
*Migai: Diss., St. Petersburg, 1909.

Milosorov: Zent. Physiol., 28, 615, 1914.

Zaitzeff: Russky Vrach., 14, No. 29, 191 5.

* Spencer et al: Loc. cit.

* Carlson: Loc. cit.

* Fowler, Rehfuss and Hawk: Loc. cit.
'Fowler & Buchanan: Unpublished.

152 physiological chemistry

The Use of Indicators in Determining the Reaction of Gastric
Juice and Other Fluids

The reaction of the gastric juice and other body fluids is most
readily tested by means of indicators, so-called because they show
changes of color with differing degrees of acidity or alkalinity of the
solution. They behave as though they were weak acids or bases whose
ions and unionized molecules have different colors. Modern theories
of color in organic compounds however class them as tautomeric
substances.

A neutral solution is one in which there are equal numbers of hy-
drogen and hydroxyl ions. An acid solution has a preponderance of
hydrogen ion and an alkaline solution an excess of hydroxyl ion. All
indicators do not show changes of color at the true neutral point, but
at some fixed degree of acidity (or alkalinity), i.e., at a definite hydrogen
or hydroxyl ion concentration. Indicators which change color at the
approximate true neutral point are litmus and rosolic acid, while phenol-
phthalein changes color in a slightly alkaline solution. Congo red,
sodium alizarin sulphonate and tropaeolin 00 are examples of indicators
which change color in an acid solution.

Organic acids in general are not sufficiently strong; i.e., do not dis-
sociate with the production of enough hydrogen ion to cause color
changes in dilute solution with indicators of the last-mentioned class.
Litmus, rosolic acid and phenolphthalein, however, change at so
low a hydrogen ion concentration that they are affected by dilute
solutions of organic acids and may be used for their titration. Even
very dilute solutions of mineral acids are sufficiently acid to produce
color changes with Congo red, alizarin, etc., and hence these indicators
may be used in the titration of mineral acid. Phenolphthalein which
changes color in a weakly alkaline solution indicates the presence of acid
combined with weakly alkaline substances (as protein) as well as other
types of acid such as acid salts, and hence, is used in the titration of
solutions for their total acidity.

The hydrogen ion concentration of pure water or a neutral solution
is approximately iXio~^, being expressed as approximate moles of
hydrogen ion per liter. That is water is a 1/10,000,000 N solution of
hydrogen ions. The concentration of hydroxyl ions in pure water or a
neutral solution is exactly equal to that of the hydrogen ions, so that
water may be considered to be an N/ 10,000,000 alkali as well as an
N/io,ooo,ooo acid. Hydrogen ion concentrations are often ex-
pressed for the sake of brevity as their logarithms with the sign re-
versed. For example the logarithm of iXio~^ would be -7.0 and

GASTRIC ANALYSIS I 53

according to this notation the H ion concentration would be expressed
as Ph = 7-o. The product of the hydrogen ion concentration (H"^)
by the hydroxyl ion concentration (OH") is constant at about iXio~^*
so that as (H"^) increases from iXio"^ (Ph = 7-o) to iXio"'*
(Ph = 4.0) the (0H~) falls to iXio~^°, and vice versa. It must be
borne in mind that higher figures for the logarithmic notation indicate
lower figures for (H"^). The hydrogen ion concentrations at which
certain indicators commonly used in titration work change color, are
indicated below.

True nature
Indicator Hydrogen ion concentration ., .,

color changes

Phenolphthalein Between iXio~* and iXio"^ Alkaline.

Neutral red i X io~^ Xeutral.

Rosolic acid i X lo"' Xeutral.

Litmus Between iXio"^ and iXio"^ Xeutral.

Sodium alizarin sulphonate Between iXio~* and iXio~^ Acid.

Congo red Between i X lo"^ and i X io~^ .\cid.

Dimethyl-amino-azobenzene Between iXio"^ and iXio"'' Acid.

Methyl orange Between iXio"^ and iXio~^ Acid.

Tropajolin 00 iXio~- Acid.

Tests with Indicators. — Prepare a series of solutions of varying acidities as
outlined in the following table, page 154. Introduce 5 or 10 c.c. portions of each
of these into a series of test-tubes and add to each a few drops of a solution of
Tropaeolin 00. Make a note of the colors produced, in the spaces left for this
purpose. In the same way test out the other indicators mentioned, in order,
using in each case a few drops of the indicator solution. The tests using the last
three mentioned indicators: Giinzberg's, Boas' and TropaeoUn (evaporation
test) are carried out differently as indicated on page 155.

Are the following assumptions on which the use of certain of these
indicators in gastric analysis is based borne out by your findings :

1. That Topfer's reagent (Dimethyl-amino-azo-benzene) gives its
characteristic pinkish-red color only in the presence of free HCl.

2. That a blue color with Congo red indicates free hydrochloric (or
other mineral acid), a violet color indicates an organic acid, and a brown
color indicates combined hydrochloric acid.

3. That Tropaeolin 00 and methyl orange are indicators for free
mineral acid.

4. That alizarin reacts to free mineral acid, organic acids and acid
salts but not to combined HCl.

5. That phenolphthalein can be used in titrating total acidity, that
is, acidity due to mineral and organic acids, acid salts and combined
acid.

6. That iodine is liberated from KI-KIO3 to a relatively slight ex-
tent by other than free mineral acid.

154

PHYSIOLOGICAL CHEMISTRY

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GASTRIC ANALYSIS I 55

7. That Giinzberg's test is the most satisfactory one for free HCl
and that Boas' reagent and Tropa^olin 00 are also delicate reagents for
free mineral acid.

Special Tests for Free HCl. Perform the following tests on the solutions as
outhned on page 154 and tabulate the results.

1. Giinzberg's Reagent.' — Place 1-2 drops of the reagent in a small porcelain
evaporating dish and carefully evaporate to dryness over a low flame. Insert
a glass stirring rod into the mixture to be tested and draw the moist end of the
rod through the dried reagent. Warm again gently and note the production of a
purphsh-red color in the presence of free hydrochloric acid.

2. Boas' Reagent.- — Perform this test in the same manner as i, above.
Free hydrochloric acid is indicated by the production of a rose-red color which
becomes less pronounced on cooling.

3. Tropaeolin OO,'

NH (CeHs) _C6H4-N = N-C6H4-S03Na.

Place 2 drops of the solution to be tested and i drop of the indicator in an evapo-
rating dish and evaporate to dryness over a low flame. The formation of a red-
dish-violet color indicates free hydrochloric acid.

This test may also be conducted in the same manner as i, above.

Hydrogen Ion Concentration and Titratable Acidity

The acidity of a solution may be determined in two different ways
by means of indicators. One method is by titration with standard
alkali using the indicator to determine the end point of the titration.
For this purpose the indicator should be one which gives a sharp color
change which is sensitive to the form of acidity which is to be deter-
mined, and which is not destroyed by any substance contained in the
titration mixture. Thus phenolphthalein can be used for the titration
of strong bases and nearly all weak acids, but cannot be used for weak
bases, and is unsatisfactory in the presence of ammonium salts. Methyl
orange on the other hand is useful for strong acids and weak bases such
as ammonia and for the soluble carbonates but cannot be used for weak
acids such as carbonic acid or the organic acids. Almost any indicator
may be used in the titration of mineral acids against strong bases such
as KOH inasmuch as under these conditions i drop of the standard
solution will throw the hydrogen ion concentration so far beyond that of
neutrality that the turning point of any common indicator ^v'ill be
passed.

Titration does not, however, enable us to determine in all cases the

* Giinzberg's reagent is prepared by dissolving 2 grams of phloroglucinol and i gram of
vanillin in loo c.c. of 95 per cent alcohol.

^ Boas' reagent is prepared by dissolving 5 grams of resorcinol and 3 grams of sucrose in
100 c.c. of 50 per cent alcohol.

^ Prepared by dissolving 0.05 gram of tropsolin 00 in 100 c.c. of 50 per cent alcohol.

156 PHYSIOLOGICAL CHEMISTRY

true acidity of a solution, that is, its hydrogen ion concentration. In the
case of strong acids and bases very accurate results for the true acidity
may be obtained in this way. In the case of weak acids or bases the
titration values may give but slight information as to the true acidity.
Thus in the case of a slightly dissociated acid, such as acetic acid, as
fast as the acidity due to its dissociated hydrogen ions is neutralized
the undissociated acid ionizes further and the titration value finally
obtained represents the total acid present at the beginning both ionized
and unionized. Salts of strong acids and very weak bases and vice
versa also hydrolyze during the course of the titration and the values
obtained in no sense represent the true acidity.

Hydrogen ion concentrations may be determined through a certain
range by means of indicators. The unknown solution is treated with
a few drops of indicator and the color obtained compared with that
produced with the same amount of indicator and a solution of known
hydrogen ion concentration. If the same tint is produced in both
cases the two acidities are the same. This is of course only true when
the indicator chosen is a suitable one, that is, one that shows definite
color changes in hydrogen ion concentrations in the neighborhood of
that of the unknown. The choice of indicators for this purpose is
somewhat different than that for titration purposes. For use in the
determination of the hydrogen ion concentration of a solution we need
an indicator showing a very gradual change in color through a given
range, one which is not readily affected by the presence of neutral salts
or other substances likely to be present, and the color of which does
not fade too rapidly. The ranges through which a number of indicators
may be used with satisfactory results for the determination of hydrogen
ion concentrations is indicated in the chart (Fig. 44, page 157). Those
surrounded by the heavy lines are the most satisfactory.

The chart also indicates how standard solutions of definite hydrogen
ion concentrations may be made up from a series of stocK. solutions,
by mixing in various proportions. The stock solutions indicated on the
chart were suggested by Sorensen and are as follows: o.ioNHCl;
o.ioNNaOH; 7.505 g. glycocoll plus 5.85 gm. NaCl per liter; 11.876
g. Na2HP04.2H20 per liter; 9.078 g. KH2PO4 per liter; 21.008 g.
citric acid in i liter of 0.20 N NaOH; 12.404 g. boric acid in i liter of
o.io N NaOH. The other solutions are 0.20 N sodium acetate and
0.20 N acetic acid. Solutions of known hydrogen ion concentration are
prepared from these by mixing in the proportions indicated on the
chart, the abscissae representing parts of the more alkaline or less acid
constituent. Thus a mixture of seven volumes of the sodium acetate
stock solution with three volumes of the stock acetic acid solution

GASTRIC ANALYSIS

157

p

X

I

7

5

X

I

J
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158

PHYSIOLOGICAL CHEMISTRY

gives a mixture with an hydrogen ion concentration of i X io~^
(exponent: 5.0). The mixtures are most satisfactory through the
ranges where the hydrogen ion concentration changes most gradually,
that is, through the flatter portions of the curves.

The amounts of indicator solutions and their strengths to be used
in the determinations of hydrogen ion concentrations in 10 c.c. portions
of unknown solution are indicated below.

I.

Alizarin yellow R (p-
nitrobenzene-azo-salic-

2.

3-

ylic acid)

Azolitmin (litmus)
Cochineal

lo-s

4-
5-

2, 5-dinitro-hydroquinone
Mauvein

5-2
8-1

6.

Methyl orange

5-3

7-
8.

9-

Methyl red
Methyl violet
Neutral red

4-2

8-1

20-10

10.
II.
12.

p-Nitrophenol
Phenolphthalein
Rosolic acid

20-3
20-3
15-6

13-
14.

IS-

Thymolphthalein
Tropaeolin 0
Tropaeolin 00

10-3
10-5
S-3

16. Tropaeolin 000

INDICATOR SOLUTIONS

Drops Preparation of solution

o. I gram to 1000 c.c. water.

Aqueous solution.

Alcoholic solution.

I gram to 1000 c.c. alcohol.

o. 5 gram to looo c.c. water.

0.1 gram recrystallized salt to 1000 c.c.

water.
Saturated solution in 50 per cent, alcohol.
0.5 gram to 1000 c.c. water,
o. I gram in 500 c.c. alcohol, and 500 c.c. water
0.4 gram to 60 c.c. alcohol, 940 c.c. water.
0.5 gram to 500 c.c. alcohol, 500 c.c. water,
o . 4 gram to 400 c.c. alcohol, 600 c.c. water.
0.4 gram to 500 c.c. alcohol, 500 c.c. water,
o. I gram to 1000 c.c. water.
Of recrystallized salt, o.i gram to 1000 c.c.

water.
10-4 0.1 gram to 1000 c.c. water.

Determination of Hydrogen Ion Concentration. — Introduce 10 c.c. portions
of the unknown solution into a series of test-tubes of similar diameter and of
clear glass. Test first with Utmus paper which changes at about the neutral
point. According to whether the reaction is acid or basic to litmus test other indi-
cators on the acid side such as p-nitrophenol, methyl orange and tropaeolin 00,
or on the basic side as phenolphthalein. Select an indicator which gives with the
solution neither its maximum acid or maximum basic color. Note from the chart
through what range this indicator exhibits its characteristic change of color.
Then to 10 c.c. portions of standard solutions of known hydrogen ion concentra-
tion (furnished by the instructor), which cover approximately the same range as
the indicator add exactly the same number of drops of indicator solution as was
added to the standard. Compare colors of unknown and standards until one is
found which matches and which consequently possesses the same hydrogen ion
concentration. If the unknown is so strongly acid or basic that none of the indi-
cators mentioned can be used directly it will be necessary to dilute it with 10 or a
greater number of volumes of water before testing further.

In case the unknown solution is slightly colored the standards should like-
wise be brought to the same tint by the addition of some coloring agent as Bis-
marck brown, methyl orange, methyl violet, etc., before making the comparison.

For appUcations of the indicator method for the determination of hydrogen ion
concentration to biological fluids see chapters on the quantitative analysis of
blood (XVI) and urine (XXVI).

Comparison of H Ion Concentration and Titratable Acidity. — i. Determine

GASTRIC ANALYSIS 1 59

colorimetrically the H ion concentration of an N/ioo solution of hydrochloric acid
using tropaeolin 00 as an indicator and of an N/ 100 acetic acid using methyl
orange as an indicator. Note the great difference between the true acidities of
the two solutions.

Titrate 10 c.c. portions of N 100 hydrochloric acid and of N/ioo acetic acid
with N/ioo KOH using phenolphthalein as an indicator. Note that identical
results are obtained for the titratable acidities of the two.

2. Determine colorimetrically the H ion concentration of an N;ioo KOH
solution using tropagolin O as an indicator, and of an N/ioo ammonia solution
using phenolphthalein as an indicator. Note the results and then titrate 10 c.c.
portions of both solutions with N/ioo HCl using alizarin as an indicator.

3. Mix equal portions of M 15 potassium dihydrogen phosphate and M 15
disodium phosphate (see chart). Note that the mixture is practically neutral to
litiDius. Titrate one 10 c.c. portion of this mixture with N/io KOH, using phe-
nolphthalein as an indicator. Titrate another portion with N/'io HCl solution,
using methyl orange as an indicator.

4. Mix equal volumes of N/5 sodiiun acetate solution and N/5 acetic acid.
Note that the mixture is acid to litmus. Titrate one 10 c.c. portion with N 10
HCl using tropaeolin 00 as an indicator. Titrate another portion with N 10
KOH using phenolphthalein as an indicator.

THE FRACTIONAL METHOD OF GASTRIC ANALYSIS

Procedure in Gastric Analysis by the Fractional Method

1. Introduction of the stomach tube (see pages 159 and 160).

2. Removal of the residuum (see pages 160 and 161).

3. Feeding the test meal (see page 161).

4. Feeding the retention meal (in special cases), see page i6i.

5. Removing samples of stomach contents for analysis (see page i6i).

6. Examination of the samples for:

(a) Total acidity (see page 162).

(b) Free acidity (see page 164).

(c) Pepsin (see page 165).

(d) Tripsin (not a routine procedure), see page 169.

(e) Lactic acid (see page 170).
(/) Occult blood (see page 171).
{g) Bile (see page 171).

(/;) Microscopical constituents (sec page 173).
I. Introduction of the Stomach Tube. — Whereas the large tube is
directly inserted by propulsion, the Rehfuss tube is swallowed in the
natural manner and aided by gravity. The tube may be passed in one
of three ways, i.e.: (i) lubricated; (2) with aid of lluid; (3) after throat is
cocainized. When passed by the first method the tip of the tube, after
thorough lubrication with glycerol or liquid petrolatum, is seized between

l6o PHYSIOLOGICAL CHEMISTRY

the thumb and forefinger and placed on the tongue. Then with the
aid of the forefinger the tip is pushed forward until it reaches the root of
the tongue and is engaged in the oropharynx. Then the patient is
encouraged to swallow persistently while the tube is slowly fed into the
mouth. After slight discomfort in the pharynx and its passage past the
level of the cricoid cartilage, practically no discomfort is felt. This
method is used when it is essential that the pure gastric secretion or
residuum be obtained. Ordinarily, however, it is much easier to swallow
the tube by the second method. This method consists in placing
the tip in the oropharynx and then giving the patient a measured
quantity of water or tea to swallow. The movements induced by the
swallowing carry the tube rapidly to the stomach with a minimum of
discomfort. When an Ewald meal (see below) is given, part of the tea
can be reserved for swallowing the tube. This procedure makes it
scarcely more arduous than the swallowing of food. Should the patient,
however, be extremely neurotic or the unfortunate possessor of marked
pharyngeal hyperesthesia, cocain hydrochloride in 2 per cent aqueous
solution can be applied to the throat rendering the passage of the tube
practically insensitive. When the tube has entered the stomach, as-
piration of the material shows the characteristic gastric contents.
Should the tip remain in the esophagus through transient cardiospasm
or other cause, aspiration results in the removal of only a very small
specimen having all the characteristics of the pharyngeal and esoph-
ageal secretions.

2. Removal of Residuum. — If the so-called "empty" stomach is
examined in the morning before any food or drink has been taken it
will be found to contain considerable material. This is termed res-
iduum. Before a test meal is introduced into the stomach, this organ
should be emptied. If this is not done we cannot consider the samples
withdrawn after the test meal is eaten as representing the secretory
activity of the gastric cells under the influence of the stimulation of the
test meal. It has been generally recognized, clinically, that a residuum
above 20 c.c. is pathological.^ Such a volume has been considered as
indicative of hypersecretion, and this in turn in many cases indicates an
organic lesion. The observations indicating that a residuum of over
20 c.c. was pathological, were made upon residuums removed by means
of the old type of stomach tube which does not completely empty the
stomach.- When the residuum is completely removed by means of

* Loeper: Leqons de pathologie digestive, 191 2, Series 2, pp. 17-19.

Zweig: Magen- und Darmkrankheiten, p. 459.

Kemp: Diseases of the Stomach, Intestines and Pancreas, 191 2, p. 133.

Wolff: Taschenbuch der Magen- und Darmkrankheiten, p. 22.
^ Harmer and Dodd: Loc. cit.

GASTRIC ANALYSIS l6l

the Rehfuss tube it has been demonstrated that the normal residuum
is practically always over 20 c.c. and that the average is about 50 c.c.^
The normal residuum has been found to possess all the qualities of a
physiologically active gastric juice with an average total acidity of 30
and an average free acidity of 18.5. The residuum is often colored by
bile. This is particularly true if the fluid has a relatively high acidity.
Trypsin is also generally present. These findings indicate regurgita-
tion (see page 151). A residuum of large volume possessing a total
acidity value of 70 or over may indicate ulcer.

Analysis of Residuum. — Remove the residuum as directed under (^5), below,
and analyze the fluid according to methods outlined on page 162.

3. The Test Meal. — Before making an analysis of the stomach
contents it is customary to introduce something into the stomach which
will stimulate the gastric cells. The response to this stimulation is
then measured clinically by the determination of total acidity, free
acidity and pepsin in the stomach contents. ]\Iany forms of test meal
have been used.

The test meal most widely employed is the Ewald test meal. This consists
of 2 pieces (35 grams) of toast and 8 ounces (250 c.c.) of tea.

Inasmuch as it was demonstrated in the author's laboratory^ that
water gave a similar gastric stimulation to that produced by the Ewald
meal it was suggested that a simple water meal might be substituted
for the Ewald meal. This water meal also has the added advantage
of enabling one to determine the presence of food rests and to test more
accurately for lactic acid, blood and bile.

4. The Retention Meal. — In order to obtain more information
regarding gastric motility than is furnished by the ordinary test meal
described above the patient may be fed a so-called retention meal. This
meal is fed in place of the regular evening meal and contains substances
readily detected. In the morning before breakfast (7-8 a. m.) remove
the stomach contents (residuum, see page 1 60) by aspiration and examine
for food rests. The normal stomach should give no eA-idences of food
retention. A satisfactory retention meal consists of 4 ounces each of
boiled string beans and rice.^ Diets containing prunes, raspberry mar-
malade, lycopodium powder, etc., have also been employed. In many
instances an ordinary mixed diet \\\\\ serve the purpose.

5. Removal of Samples for Analysis. — At intervals of exactly 15
minutes from the time the test meal is eaten until the stomach is empty

^ Rehfuss, Bergeim and Hawk: Jour. Am. Med. Ass'n, 63, 11, 1914.

Fowler, Rehfuss and Hawk: Jour. Am. Med. Ass'n, 65, 1021, 1915.
- Bergeim, Rehfuss, and Hawk: Jour. Biol. Cfiem., 19, 345, 1914-

Rehfuss, Bergeim and Hawk: Jour. Am. Med. Ass'n, 63, 11, 1914.
' Myers and Fine: Essentials of Pathological Chcmislry, 1913.
II

l62 PHYSIOLOGICAL CHEMISTRY

5-6 c.c. samples of gastric contents are withdrawn from the stomach
by means of aspiration.

In the removal of samples from the stomach, it is essential that very-
little traction be employed. To completely empty the stomach, aspira-
tion is practised in four positions : (a) on the back ; (b) on the stomach ;
(c) on right side, {(t) on left side. This results in complete evacuation
of the stomach. Three tests may be employed to determine whether
the stomach is empty: (i) No more material can be aspirated in any
position; (2) injection of air and auscultation over the stomach with a
stethoscope reveals a sticky rale and not a series of gurgling rales
such as is heard when there is material in the stomach; (3) lavage or
irrigation through the tube which shows the absence of all food in the
stomach.

6. Examination of the Samples.- — The old methods of gastric analy-
sis involved the collection (by analysis and calculation) of data regard-
ing several types of acidity (see Topfer's method, page 174). The
modern tendency among clinicians is to lay particular emphasis upon
the values for total acidity and free acidity. The determination of the
peptic activity is also important as well as the demonstration of the
presence or absence of occult blood, lactic acid, mucus, food rests, etc.

Procedixre. — Strain each sample through a fine-mesh cheese cloth. ^ Examine
the residue for mucus, blood and food rests. Use the strained stomach contents
for the determination of total acidity, free acidity and peptic activity by methods
which follow.

(a) Determination of Total Acidity. — Pririciple. — The indicator
used is phenolphthalein. Since the indicator reacts with mineral
acid, organic acid, combined acid and acid salts the values obtained
represent the total acidity of the solution.

Procedure.— Measure i c.c. of the strained stomach contents by means of an
Ostwald pipette and introduce it into a low-form 60 c.c. porcelain evaporating
dish. Dilute with 15 c.c. of distilled water. Add 2 drops of a i per cent alcoholic
solution of phenolphthalein and titrate with N/ioo sodium hydroxide until a
faint pink color is obtained and persists for about two minutes. ^ Take the burette
reading and calculate the total acidity.

* The examination for microscopical constituents (see {h) p. 173) should be made on the
original (unstrained) gastric contents. Tests for occult blood may be made on the sedi-
ment if desired.

"^ Procedure for Serial Titrations. — When a series of titrations are to be made the following
procedure may be used: Arrange the numbered evaporating dishes in rows on a tray. In-
troduce I c.c. of the proper sample into each dish, dilute with 10 c.c. of water and add the
indicator. Add the N/ioo NaOH to contents of dish No. i at a definite rate until a point is
reached at which a faint pink color is obtained, as described above. Return dish No. i to
its place in the tray and place dish No. 2 under the burette. Take the burette reading of
No. I. Then titrate No. 2 in the same way. Continue the series. This procedure has the
advantage of being speedy and accurate. There is a slight error made by the rapid addition
of the NaOH but it is uniform and the results (titrations) are therefore comparable.

GASTRIC ANALYSIS

163

Calculation. — Note the number of cubic centimeters of N/ 100 NaOH required
to neutralize i c.c. of stomach contents, and multiply it by 10 to obtain the number
of cubic centimeters N/io NaOH necessary to neutralize 100 c.c. of stomach
contents. This is the method of calculation most widely used. For other forms
of expressing total acidity see page 174. Plot your results in a form similar to
those shown in Figs. 45 and 46.

Curves Obtained by the Fractional Method. — When an Ewald test meal
is given to normal individuals a curve such as indicated below is usu-
ally obtained. The curve may vary within certain limits depending on
individual idiosyncrasies, but is usually found to follow the curve
depicted, and the meal normally leaves the stomach in two and one-

iOO

20 40 60 60 100 120

Fig. 45. — Acidity Curves of XoRiiAL Human Stomach.

half hours. Pathologically every variation occurs, both in time of
evacuation as well as the character of the curve and the quantity of the
secretion elaborated. Fig. 41 represents some of the possibilities of
pathological cases, but a consideration of their interpretation is outside
the purpose of the present volume. It will be evident, however, from
a consideration of the figure that the cycle of gastric digestion is a con-
stantly changing one, and no information concerning the trend of
digestion can be obtained by an examination of only a single stage of
digestion. Marked changes may precede or follow that stage and the
possibilities suggested in Fig. 41 are all observed clinically and are of
varying significance. Typical curves from cases of hyperacidity,
gastric carcinoma and achylia are shown in Figs. 46, 47 and 48
respectively.

164

PHYSIOLOGICAL CHEMISTRY

(b) Determination of Free Acidity. — The reagent most widely used,
clinically, for the determination of free hydrochloric acid in stomach

100

Total acidih|

x:
o

to

o

Free acidity

'A V/z IV4. 2 hours

Fig. 46. — Acidity Curves From a Case of Hyperacidity.

contents is Topfer's reagent (see page 175). It has been found, however,
that this reagent gives rather inaccurate results due to the uncertain

c

I

1

1120
960

800^

u

640§
to
z

480^

320 80

60

160 40

1

1

i

(7a.
Cat

<itric
cinon

a

i

i

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/

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y'

y'

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Fig. 47. — Acidity and Protein Curves in Gastric Carcinoma.
Jour. Am. Med. Ass'n, 64, 1737, 1915-)

(Clarke and Rehfuss:

end point. For this reason we have employed Sahli's reagent.^ This
reagent contains KI and KIO3 and liberates iodine in the presence of

^ A mixture of equal parts of a 48 per cent solution of potassium iodide and an 8 per cent
solution of potassium iodate.

GASTRIC ANALYSIS

165

free hydrochloric acid. The liberated iodine is titrated by thiosulphate
using starch as an indicator. It gives values similar to Topfer's re-
agent in average acidities.^ Acidities other than free hydrochloric re-
act to a certain extent with Sahli's reagent.

Procedure. — Measure i c.c. of the strained stomach contents by means of an
Ostwald pipette and introduce it into a 60 c.c. porcelain evaporating dish. Dilute
with ID c.c. of distilled water, and add i c.c. of Sahli's reagent (a. mixture of
equal parts of 48 per cent KI and 8 per cent KIO3). Allow the stomach contents
thus treated to stand for five minutes and then titrate with N/ioo sodium thio-
sulphate imtil only a faint yellow color remains. Now add 5-10 drops of a i
per cent solution of soluble starch and continue the titration until the blue color
disappears. In serial titrations the same procedure may be employed as de-
scribed on page 162, note 2.

Calculation. — Note the number of cubic centimeters of N/ioo sodium thio-
sulphate required to titrate i c.c. of stomach contents to the total disappearance
of blue color in the presence of starch. Inasmuch as N/ioo thiosulphate is
equivalent to N/ioo alkaU, this value indicates the number of cubic centimeters
of N/ioo sodiimi hydroxide necessary to neutralize the free hydrochloric acid in

"p ^0

80
40

,

-^

. — ' "

Hours

V4

V2

3/4

I IV4

V/z

1%.

Fig. 48. — Total Acidity and Protein Curves in Benign Achylia (Solid Line
Represents Acidity). {Clarke and Rehfuss: Jour. Am. Med. Ass'n., 64, 1737, 1915.)

I c.c. of the stomach contents. Multiply the value by 10 to obtain the number of
cubic centimeters of N/io NaOH necessary to neutrahze 100 c.c. of stomach
contents. This is the method of calculation most widely used. For other forms
of expressing free acidity see page 174. Plot your results in a curve similar
to those shown in Figs. 43, 45, and 46, pages 150, 163 and 164.

(c) Determination of Peptic Activity. — (i) Method of Mett- as
Modified by Nirenstein and Scln&.^—Frinicplc. — Small glass tubes
filled with coagulated egg albumin are introduced into tlie solution to
be tested, and kept for a definite length of time in the incubator. The
protein column is digested at both ends of the tube to an extent depend-
ing upon the amount of pepsin present. The method is not strictly
accurate but is the most satisfactory for clinical purposes on account
of its simpUcity. Nirenstein and Schiff showed that human gastric
juice contained inhibiting substances the effect of which is overcome by
the dilution recommended.

1 Fowler, Bergeim and Hawk: Unpublished data.

2 Mett: Arch. f. Anal. u. Physiol., 1804. 68.

^Nirenstein and Schiff: Arch. f. Vcrdauungskraukhcilen, 8, 559, 1902.

1 66 PHYSIOLOGICAL CHEMISTRY

Procedure. — Introduce into a small Erlemneyer flask i c.c. of gastric juice
and 15 c.c. of N/20 HCl ( = 0.18 per cent HCl). Add two Mett tubes prepared
as indicated below, stopper the flask to prevent evaporation and place in an in-
cubator at 37°C. for 24 hours. By means of a low power microscope and a milli-
meter scale (graduated to half millimeters) determine accurately the length of
the column of albumin digested at each end of the tubes. It is well to run the
determination in dupUcate in which case the result is the average of the eight
figures obtained. Ordinarily from 2-4 mm. of albumin are digested by normal
human gastric juice.

Calculation. — The peptic power is expressed as the square of the nxmiber of
millimeters of albumin digested. This is based on the Schiitz-Borissow law that
the amount of proteolytic enzyme present in a digestion mixture is proportional
to the square of the number of millimeters of albumin digested. Therefore a
gastric juice which digests 2 mm. of albumin contains four times as much pepsin
as one which digests only i mm. of albvunin.

Example. — If the microscopic reading gives on an average 2.2 mm. of albumin
digested the pepsin value for the diluted juice would be 2.2 - = 4.84, and for the
pure undiluted juice, 4.84X16 = 77.44.

Preparation of Mett Tubes {Christiansen's Method).^ — The liquid portions of
the whites of several eggs are mixed and strained through cheese cloth. The mix-
ture should be homogeneous and free from air bubbles. A number of thin-walled
glass tubes of 1-2 mm. internal diameter are thoroughly cleaned and dried and cut
into lengths of about 10 inches. These are sucked full of the egg-white and kept
in a horizontal position. Into a large evaporating dish or basin 5-10 liters of water
are introduced and heated to boiling. The vessel is then removed from the fire
and stirred with a thermometer until the temperature sinks to exactly 85°C. The
tubes filled with egg-white are immediately introduced and left in the water until
it has cooled. The tubes thus prepared are soft boiled, more easUy digested than
hard boiled tubes, and free from air bubbles. The ends are sealed by dipping in
melted parafifin or sealing wax (preferably the latter), and the tubes can be kept thus
for a long time. When ready for use mark with a file and break into pieces about
^ inch long. After cutting, the tubes should be immediately introduced into the
digestion mixture or may be kept a short time under water. Tubes whose ends are
not squarely broken off must be rejected.

The digestibility of different egg-whites varies widely. Hence in making up
a new set of. tubes if we wish our results to be comparable these tubes must be
standardized against those first prepared. This may be done by running simul-
taneous tests with tubes from the two series, using the same gastric juice and com-
paring the lengths of the columns digested in each case. Christiansen's method of
preparing tubes of the same digestibility is to be preferred. He proceeds as in
the original preparation of the tubes except that as the water cools from 90°-8o°C.
a single tube containing the new egg-white is dropped in at each degree change of
temperature, that is at 90°, 89°, etc. Pieces of each of these tubes as well as of the
original standard tubes are then allowed to digest simultaneously in portions of the
same gastric juice. One of these tubes should show a digestibility equal to that
of the standard tubes. For example the tube coagulated at 88°C. may show the
proper digestibility. Then the new series of tubes should be made in the same man-
ner as this one, that is introduced at 88°C. The tubes thus prepared should be
again checked up with the standard to see that no mistake has been made.
^ Christiansen: Biochem. Zeit., 46, 257, 1912.

GASTRIC ANALYSIS 1 67

(2) Fuld and Levison's Method. — This test is founded upon the fact, shown by
Osborne, that edestin when brought into solution in dilute acid will change in its
solubility, due to the contact with the acid, and that a protean called edes tan, v>'h\ch
is insoluble in neutral fluid, will be formed. The procedure is as follows: Dilute
the gastric juice under examination with 20 volumes of water and introduce gradu-
ally decreasing volumes of the diluted juice into a series^ of narrow test-tubes about
I cm. in diameter. The measurements of gastric juice may conveniently be made
with a I c.c. pipette which is accurately graduated in Hoo c-c. Into the first tube
in the series may be introduced i c.c. of gastric juice, and the tubes which follow in
the series may receive volumes which differ, in each instance, from the volume intro-
duced into the preceding tube by Koo; Ho; Mo; or Ho o^ ^ cubic centimeter.
Now rapidly introduce into each tube the same volume {e.g., 2 c.c.) of a i : 1000
solution of edestin- and place the tubes at 4o°C. for one-half hour. At the end of
this time stratify ammonium hydroxide upon the contents of each tube,-' place the
tubes in position before a black background and examine them carefully. The
ammonium hydroxide, by diffusing into the acid fluid, forms a neutral zone and in
this zone will be precipitated any undigested edestan which is present. Select the
tube in the series which contains the least amount of gastric juice and which exhibits
no ring, signifying that the edestan has been completely digested, and calculate the
peptic activity of the gastric juice under examination on the basis of the volume of
gastric juice used in this particular tube.

Calculation. — Multiply the number of cubic centimeters of edestin solution used
by the dilution to which the gastric juice was originally subjected and divide the
volume of gastric juice necessary to completely digest the edestan by this product.
For example, if 2 c.c. of the edestin solution was completely digested by 0.25 c.c.
of a I : 20 gastric juice we would have the following expression : o.25-i-(2oX2) or
I : 160. This peptic activity may be expressed in several ways, e.g., (a) i : 160 pep-
sin; (b) 160 pepsin content; (c) 160 parts.

(3) Rose's Modification^ of the Jacoby-Solms Method.^ — Dissolve 0.25 gram of
the globulin of the ordinary garden pea,^ Pisiim sativum, in 100 c.c. of 10 per cent

1 The longer the series, the more accurate the deductions which maj" be drawn.

2 This edestin should be prepared in the usual way (seep. 109), and brought into solution
in a dilute hydrochloric acid of approximately the same strength as that which occurs nor-
mally in the human stomach. This may be conveniently made by adding 30 c.c. of X^ 10
hydrochloric acid to 70 c.c. of water. Ordinarily it should not take longer than one minute
to introduce the edestin solution into the entire series of tubes. However, if the edestin is
added to the tubes in the same order as the ammonium hydroxide is afterward stratified, no
appreciable error is introduced.

^ Making the stratification in the same order as the edestin solution was added.

* Rose: Archives of Internal Medicine, 5, 459, 1910.

* Solms: Zeitschrifl JUr klinische Medizin, 64, 159, 1907.

' The globulin may be prepared as follows: "The finelj' ground peas, freed as much as
possible from the outer coating, are repeatedly extracted with large quantities of 10 per cent
sodium chloride solution, the extracts combined, strained through fine bolting-cloth, and
allowed to stand over night in large cyhnders to deposit insoluble matter. The supernatant
fluid is siphoned off and saturated with ammonium sulphate. The precipitate of albumin
and globuHn is filtered off, suspended in a httle water, and dialyzed in running water for
three days, until the salt has been removed, and the albumins have been dissolved. The
globulins are filtered off and washed two or three times to remove the last trace of albumins.
To purify further, the precipitate is extracted with 10 per cent sodium chloride solution, and
filtered until perfectly clear. The resulting solution is neutrahzed to litmus paper by the
cautious addition of dilute sodium hydroxide, and again dialyzed in running water for three
days to remove the salts completely. The precipitated globulins are then filtered off and
dried on a water-bath at 40°C. During the entire process of separation the proteins should
be preserved with a mixture of alcoholic thymol and toluol." This dried globulin is used in
the clinical procedure.

1 68 PHYSIOLOGICAL CHEMISTRY

sodium chloride solution, warming slightly if necessary.^ FUter and introduce i c.c.
of the clear filtrate into each of a series of six^ test-tubes about i cm. in diameter.
Introduce into each tube i c.c. of 0.6 per cent hydrochloric acid and permit a period
of about five minutes to elapse for the development of the turbidity. Make a
known volume of the gastric juice (5-10 c.c. is sufficient) exactly neutral to litmus
paper with dilute alkali; and record the volume of the alkali so used. If acid
metaprotein precipitates, filter it off; if there is no precipitate proceed without
filtration. Dilute the clear neutral solution with a known quantity of distUled
water (usually 5 volumes) making proper allowance for the volume of alkali used in
the neutralization. Boil 5-10 c.c. of the diluted juice, filter and add the following
decreasing volumes (c.c.) to the series of six tubes: i.o, 0.9, 0.7, 0.5, 0.2, 0.0. Make
the measurements by means of a i c.c. pipette graduated in o.oi c.c. Now rapidly
introduce the unboiled, diluted juice in the following increasing volumes (c.c.) in
order: 0.0, o.i, 0.3, 0.5, 0.8, 1.0. Each tube now contains a total volume of 3 c.c.
and a total acidity of 0.2 per cent hydrochloric acid. Shake each tube thoroughly
and place them at 5o-52°C. for 15 minutes or at 35-36°C. for one hour. Examine
the series of tubes at the end of the digestion period and select that tube which
contains the smallest quantity of gastric juice and which shows no turbidity. The
volume of the juice used in this tube is taken as the basis for the calculation of the
peptic activity.

Calculation. — The peptic activity is expressed in terms of i c.c. of the undiluted
juice. For example, if it requires 0.5 c.c. of the diluted juice (five-fold dilution) to
clear up the turbidity in i c.c. of the globulin solution in the proper experimental
time interval (15 minutes or one hour according to temperature) the peptic activity
would be expressed as follows:

(i-r-o.5)X5 = io (peptic activity).

According to this scale of pepsin units 10 may be considered as "normal" peptic
activity. These units are about Ko as large as those expressed by the Jacoby-
Solms scale.

Inasmuch as it has been shown' that blood serum contains an antipepsin it is
advisable to test the gastric juice for blood before determining its proteolytic power.

(4) Given's Modification of Rose's Method.^ — The gastric contents are
strained through cheese cloth. Two c.c are measured by means of an Ostwald pipette
into a 25 c.c stoppered volumetric cylinder, and dUuted to the mark with dis-
tUled water. Into each of seven small test-tubes (i X 10 cm.) is measured, with
an Ostwald pipette, i cc of a 0.25 per cent filtered pea globulin in 10 per cent
sodium chloride solution. To each tube is added i c.c of 0.6 per cent hydro-
chloric acid, also by means of an Ostwald pipette. The tubes are allowed
to stand about five minutes, untU the maximum turbidity develops. To the
first five, distilled water is added as follows: To the first, 0.9 c.c; to the second,
0.8 cc; to the third, 0.7 c.c; to the fourth, 0.6 c.c; and to the fifth, 0.2 c.c; to
the sixth and seventh, none. Then there are rapidly added to each test-tube
the following amounts of the diluted (i :i2.5) gastric juice; to thefirst, o.i c.c.;to
the second, 0.2 cc; to the third, 0.3 c.c; to the fourth, 0.5 c.c; to the fifth, 0.8 cc;

^ This solution may be preserved at least two months under toluene.
^ A longer series of tubes may be used if desired. However, experience has shown that
a series of six ordinarily affords sufficient range for all diagnostic purposes.
'Oguro: Biochemische Zeitschrift, 22, 266, 1909.
* Givens: Hygienic Lab. Bull. loi, p. 71, August, 1915.

GASTRIC ANALYSIS 1 69

to the sixth, i.o c.c; and to the seventh, i.o c.c. of the diluted juice boiled. These
measurements can be accurately made with a i c.c. pipette graduated in o.oi c.c.
All tubes are then immersed for 15 minutes in a water-bath at 50° to S2°C. At the
end of this time, the tube is selected which is clear and contains the least amount of
diluted gastric juice. Upon this basis, the peptic activity is calculated as the num-
ber of cubic centimeters of 0.25 per cent globulin digested by i c.c. of undiluted
gastric juice. For example, if tube 2 containing 0.3 c.c. of a 12.5 times diluted
juice be clear, then the result would be expressed:

Peptic activity= (i-j-o.3)Xi2.5 = 4i.2.

Ordinarily this scheme of seven tubes is used, though it is not a rule. If the
free acidity be high, sometimes a dilution of 3^5 is made. The number of tubes
used will depend upon the accuracy desired.

(d) Determination of Tryptic Activity. — Trypsin is not a gastric
enzyme but occurs in the pancreatic juice (see page i88). In case of
regurgitation of intestinal contents through the pylorus trypsin would
be passed into the stomach. This regurgitation is doubtless of frequent
occurrence and may even be a normal mechanism by which gastric
acidity is regulated (see page 151). Trypsin is, therefore, generally
present in the contents of the normal human stomach.

Spencer's Method.' — (a) Prepare five reagent tubes, Nos. i, 2,3,4, and 5; more
if desired.

To tubes I and 2 add 0.5 c.c. of gastric contents (filter if cloudy).

(b) To tubes 2, 3, 4, and 5 add 0.5 c.c. of distilled water.

(c) From tube 2 remove 0.5 c.c. of its mixed contents and add to tube 3. Mix
thoroughly and add 0.5 c.c. from tube 3 to tube 4. Repeat for tube 5.

We now have dilutions of gastric contents of i, 3^, 3^, 3^, and 3^6-

(d) To each tube add one drop of phenolphthalein solution (phenolphthalein
I gram; alcohol (95 per cent) 100 c.c); then add drop by drop a 2 per cent sodium
bicarbonate solution until a light pink color is produced.

(e) To tubes i, 2, 3, and 4 add 0.5 c.c. of casein solution. Tube 5 must receive
I c.c. of casein solution, since it contains i c.c. of the diluted gastric contents. For
the casein solution, dissolve 0.4 gram of casein in 40 cc. of N/io NaOH. Add 130
c.c. of distilled water, then 30 c.c. of N/io HCl. This leaves the solution alkaline
to the extent of 10 c.c. of N/io NaOH, minus about 3 cc neutralized by the
casein.

(J) Incubate for five hours at 4o°C.

(g) Precipitate the undigested casein by dropwise addition of a solution of the
following composition: glacial acetic acid i c.c, alcohol (95 per cent) 50 c.c, dis-
tilled water 50 cc. The tubes in which digestion has been complete remain clear;
others become turbid.

(h) The tryptic values are expressed in terms of dilution. Thus, complete
digestion in tube 3 (a dilution of Ji) shows four times the tryptic power of un-
diluted gastric juice; taken as a standard as i, therefore, its tryptic value is 4.

^Elaborated by Dr. W. H. Spencer {Jour. Biol. Chem., 21, 165, 1915) in the author's
laboratory for the specific purpose of determining trypsin in gastric juice. For other trjp-
sin methods see Chapter X.

lyo PHYSIOLOGICAL CHEMISTRY

(z) Controls of boiled gastric contents plus casein solution, and of distilled water
plus casein solution, treated as above stated, must show no digestion, and become
turbid on addition of the precipitating solution.

(e) Detection of Lactic Acid. — WTien the acidity of the stomach
contents is reduced to a low value there may occur considerable fermen-
tation of carbohydrates which have been introduced into the stomach
in the ingested food. This fermentation yields various organic acids
among which lactic acid is particularly prominent. It is important,
therefore, in case of low gastric acidity that the stomach contents be
examined for lactic acid.

Tests. I. Ether -Ferric Chloride Test (Strauss).— A satisfactory
deduction regarding the presence of lactic acid can only be made by
removing the lactic acid from disturbing factors {e.g., hydrochloric acid,
protein digestion products, etc.) present in the stomach contents.
Lactic acid may be extracted from the stomach contents by ether.
The following technic not only serves to detect lactic acid but also gives
an approximate idea as to the amount of the acid present.

Procedure. — Introduce 5 c.c. of strained stomach contents into a small grad-
uated separatory funnel, add 20 c.c. of ether and shake the mixture thoroughly.
Permit the ether to separate, then allow all the fluid to run out of the separatory
funnel except the upper 5 c.c. of ether. To this ether extract add 20 c.c. distilled
water and 2 drops of a 10 per cent solution of ferric chloride and shake the mix-
ture gently. A slight green color is obtained in the presence of 0.05 per cent lac-
tic acid whereas o. i per cent lactic acid yields a very intense yellowish -green color.

2. Ferric Chloride Test (Kelling). — Fill a test-tube with water, add 1-2
drops of a 10 per cent solution of ferric chloride and mix thoroughly to form a
liquid which is very faintly colored. Divide the solution into two parts and keep
one part as a control. To the other part add a small amount of the strained
gastric contents and to the control tube add a similar volimie of water. Lactic
acid is indicated by the immediate development of a distinct yellow color in the
tube containing the gastric contents.

The color in this test is due to the formation of ferric lactate.

3. Uffelmann's Reaction. — To 5 c.c. of Uffelmann's reagent^ in a test-tube
add an equal volume of strained gastric juice. A canary yellow or greenish-
yellow color develops if lactic acid be present to the extent of o.oi per cent or over.

Other organic acid gives a similar reaction. Mineral acids such as
hydrochloric acid discharge the blue coloration leaving a colorless
solution. In other words, the color of the reagent is weakened in the
presence of an acid reaction.

^ Uffelmann's reagent is prepared by adding ferric chloride solution to a i per cent solu-
tion of carbolic acid until an amethyst-blue color is obtained, due in part to the formation of
a ferric salt of carbolic acid and in part to the reduction of some of the iron.

GASTRIC ANALYSIS 171

4. Hopkins' Thiophene Reaction.— Place about 5 cc. of concentrated sulphuric
acid in a test-tube and add i drop of a saturated solution of copper sulphate.^
Introduce a few drops of the gastric contents, shake the tube well, and immerse it
in the boiling water of a beaker-water-bath for one or two minutes. Now remove
the tube, cool it under running water, add 2-3 drops of a dilute alcoholic solution-
of thiophene, C4H4S, from a pipette, replace the tube in the beaker and carefully
observe any color change which may occur. Lactic acid is indicated by the ap-
pearance of a bright cherry-red color which forms rapidly. This color may be made
more or less permanent by cooling the tube as soon as the color is produced. Ex-
cess of thiophene produces a deep yellow or brown color with sulphuric acid. The
test is not wholly specific though the author claims it to be more so than Uffelmann's
reaction.

(f) Detection of Occult Blood. ^~i. Ortho-toli din Test (RuttanandHardisty)."
— To I cc. of a 4 per cent glacial acetic acid solution of o-tolidin4na test-tube add
I cc. of the gastric juice under examination and i cc. of 3 per cent hydrogen
peroxide. In the presence of blood a bluish color develops (sometimes rather
slowly) and persists for some time (several hours in some instances).

This test is said to be as sensitive for the detection of occult blood in
feces and stomach contents as is the benzidine reaction. It is also
claimed to be more satisfactory for urine than any other blood test.
The acetic acid solution may be kept for one month with no reduction in
delicacy.

2. Benzidine Reaction. — This is one of the most delicate of the reactions for the
detection of blood. Different benzidine preparations vary greatly in their sensi-
tiveness, however. Inasmuch as benzidine solutions change readily upon contact
with Ught it is essential that they be kept in a dark place. The test is per-
formed as follows : To a saturated solution of benzidine in alcohol or glacial acetic
acid add an equal volume of 3 per cent hydrogen peroxide and i cc of the gastric
contents under examination. If the mixture is not already acid render it so with
acetic acid, and note the appearance of a blue color. A control test should be
made substituting water for the solution under examination.

The sensitiveness of the benzidine reaction is greater when applied
to aqueous solutions than when applied to the urine. According to
Ascarelli the benzidine reaction serves to detect blood when present in
a dilution of 1:300,000. (For further discussion of this test see
chapter on Blood.)

(g) Detection of Bile in Stomach Contents. — If we accept Boldyreff's
theory as to the automatic regulation of gastric acidity^ under normal

' This is added to catalyze the oxidation which follows.
-About 10-20 drops in 100 cc. af 95 per cent alcohol.

' These tests maybe made upon the strained stomach contents or upon the sohd residue.
* Ruttan and Hardisty: Canadian Medicine Ass'n Journal, Nov., 1912; also Biochem.
Bull., 2, 225, 1913.

5 XHov yXH.,

/CeH^ — C6H4\

CH3/ \CH,

•Boldyreff: Quart. Jour. Exp. Med., 8, i, 1914.

172

PHYSIOLOGICAL CHEMISTRY

conditions by the regurgitation of alkaline material from the intestine,
then the presence of bile in the gastric juice does not possess the clinical
significance it has been accorded. However, if an ordinary Ewald meal
be fed, and bile in any considerable quantity be found throughout the
entire course of digestion it may indicate, pathologically, a stenosis
below the level of the common bile duct. Frequently samples of
gastric contents are encountered which are uncolored and which never-
theless contain bile. It is also true that bile may be adsorbed from
stomach contents by mucus and food rests. The regulation technic for
bile testing is often inadequate to demonstrate the presence of this

Fig. 49. — Microscopical Constituents of the Gastric Contents.

A, Starch cells; B, yeast cells; C, Oppler-Boas bacilli; D, staphylococci; E, streptococci;
F, sarcinae; G, muscle iibre; H, mucus; /, red blood cells; /, leucocytes; K, snail-like mucus
formations; L, squamous epithelial cell; Af, cellulose.

fluid in gastric contents. The following procedure based upon the
oxidation of the bilirubin with nitric acid forming green biliverdin is
delicate and easy of application.

Procedure. — Saturate 10 c.c. of the fluid portion of the stomach contents with
powdered ammonium sulphate. This may be accomplished by shaking for one
to two minutes. It generally requires about i inch of powdered sulphate in
the bottom of an ordinary test-tube to obtain full saturation. When the fluid is
saturated add 1-3 c.c. of acetone and thoroughly mix the contents of the tube by
inverting the tube five or six times. (It is better not to shake.) Permit
the tube to stand and allow the acetone to rise to the surface. This acetone con-

GASTRIC ANALYSIS 1 73

tains the bile pigment if any is present in the stomach contents. Allow a drop
of yellow nitric acid to flow down the side of the tube and note the green color in
the acetone.

This green color is biliverdin which has been produced from the
bilirubin by oxidation with nitric acid. If too much acid is added
the green color will be oxidized to a purple or red. If the acetone does
not rise to the surface promptly the liquid has not been completely
saturated with ammonium sulphate.

If the stomach contents contains large amounts of bile as indicated
by a deep green color 4-5 drops of the fluid may be diluted with 10 c.c.
water and the above test applied.

(h) Microscopy of the Gastric Contents. — A microscopical exami-
nation of the gastric contents is a routine clinical procedure.

When an Ewald meal is given the starch granules in various stages
of digestion are observed together with epithelia from the pharynx,
esophagus, and occasionally the stomach. Gastric and salivar>'
mucus are seen and readily recognized by their ropy appearance.
Pathologically various bacteria are seen, sarcinae, Oppler-Boas bacilli,
streptococci, leptothrix, etc. Retained food from previous meals is
readily recognized by its histological appearance; meat fibers, vegetable
cells, and cellulose may all occur in pathological retention. In certain
pathological processes such as. ulcer and cancer, red blood cells, pus,
and even the cancer cells themselves may be found. For illustrations
of the microscopical constituents of gastric contents, see Fig. 49.

Procedure.— Examine a drop of the original (mixed) stomach contents un-
stained under the low and high powers of the microscope. Compare your find-
ings with the microscopical views shown in Fig. 49.

Wolff Technic for the Protein Concentration of the Gastric Contents.' —
Owing to the diagnostic importance of the protein concentration of the gastric
secretion, a short note of this test is given here. Under normal conditions the
protein concentration follows that of acidity rather closely. In certain cases, how-
ever, such as carcinoma (Fig. 47), there is an actual increase in the protein concen-
tration of the gastric juice out of ail proportion to the acidity. The test may be
made as follows: The regular Ewald test meal is fed and specimens of the gastric
contents are obtained at is-minute intervals by means of the Rehfuss tube. One
c.c. of the filtered juice is then diluted with 9 c.c. of water representing a dilution
of I :io; 5 c.c. of this mixture is again added to 5 c.c. of water and a dilution of i :2o
obtained; this is again repeated using 5 c.c. of the mi.xturc last obtained and 5 c.c.
of distilled water and the dilutions are kept up until a scries is obtained representing
1 : 10, 1 : 20. 1 : 40, i : 80, i : 160, i : 320, and if necessarj^ i : 640 or more. They are

1 Wolff: Magen- und Darmkrankh., Berlin, 1912, p. 217; also Berl. klin. Woch., May 29,
1911, and March i8, 1912.

Rolph: Ued. Rec, 19 13, p. 848.

Clarke and Rehfuss: Jour. Am. Med. Ass'n, 64, 1737, 191 5.

174 PHYSIOLOGICAL CHEMISTRY

then stratified with approximately i c.c. of Wolff's reagent/ care being taken that
the liquids do not mix. The tubes should be read immediately against a dark
background and the tube giving a protein ring at the greatest dilution of gastric
juice recorded. A glance at Fig. 47 will show a pronounced case of gastric carci-
noma. With normal acid figures the protein concentration evolves proportionally
to the acidity. A case of achylia is shown in Fig. 48.

Topfer's Method of Gastric Analysis

This method is much less elaborate than many others but is sufl&ciently ac-
curate for ordinary clinical purposes. The method embraces the volumetric de-
termination of (i) total acidity, (2) free acidity {organic and inorganic),^ and {3) free
hydrochloric acid, and the subsequent calculation of (4) combined acidity and (5)
acidity due to organic acids and acid salts, from the data thus obtained.

Procedure. — Feed the Ewald test meal as directed on page 161. At the end of
one hour remove the entire stomach contents and analyze as directed below. This
method of procedure is less accurate than the Fractional Method (see page 148).
Measure the volume of the gastric contents, strain it through cheese cloth and intro-
duce 10 cc of the strained material into each of three small beakers or porcelain
dishes^ Label the vessels A, B, and C, respectively, and proceed with the analysis
according to the directions given below. The volume of fluid present in the stomach
one hour after an Ewald meal varies under normal conditions between 50 and 100
c.c. In cases of hypersecretion or defective motility 200-300 c.c. may be found.
Very excessive volumes, e.g., 500-3000 c.c, are indicative of dilatation of the stomach
and suggest pyloric stenosis, either benign or malignant.

I. Total Acidity.'* — Add 3 drops of a i per cent alcoholic solution of phenol-
phthalein^ to the contents of vessel A and titrate with N/io sodium hydroxide solu-
tion until a faint pink color is produced and persists for almost two minutes. Take
the burette reading and calculate the total acidity.

Calculation. — The total acidity may be expressed in the following ways:

I. The number of cubic centimeters of N/io sodium hydroxide solution neces-
sary to neutralize 100 c.c. of gastric juice.

2; The weight (in grams) of sodium hydroxide necessary to neutralize 100 c.c.
of gastric juice.

3. The weight (in grams) of hydrochloric acid which the total acidity of 100
c.c. of gastric juice represents, i.e., percentage of hydrochloric acid.

The forms of expression most frequently employed are i and 3, preference being
given to the former, particularly in clinical work.

In making the calculation note the number of cubic centimeters of N/io sodium
hydroxide required to neutralize 10 c.c. of the gastric juice and multiply it by 10 to
obtain the number of cubic centimeters necessary to neutralize 100 c.c. of the fluid.

^ Phosphotungstic acid 0.3 c.c.

Concentrated hydrochloric acid i . o c.c.

Alcohol 95 per cent 20.0 c.c.

Distilled water sufficient to make 100. o c.c.

- For a discussion of combined acid see chapter on Gastric Digestion.
3 If sufficient gastric juice is not available it may be diluted with water or a smaller
amount, e.g., 5 c.c, taken for each determination.

* This includes free and combined acid and acid salts.

^ One gram of phenolphthalein dissolved in 100 cc. of 95 per cent alcohol.

GASTRIC ANALYSIS 1 75

If it is desired to express the acidity of 100 cc. of gastric juice in terms of hydro-
chloric acid, by weight, multiply the value just obtained by 0.00365.^

2. Free Acidity (Organic and Inorganic). — Add 3 drops of sodium alizarin
sulphonate solution- to the contents of vessel B and titrate with X/io sodium hy-
droxide solution until a violet color is produced. In this titration the red color,
which appears after the tinge of yellow due to the addition of the indicator has
disappeared, must be entirely replaced by a distinct violet color. Take the burette
reading and calculate the free acidity due to organic and inorganic acids.

Calculation. — Since the indicator used reacts to both organic and inorganic
acids, the number of cubic centimeters of N/io sodium hydroxide used indicates
the free acidity of 10 cc. of gastric juice. The data for 100 cc. of gastric juice may
be calculated according to the directions given under Total Acidity, page 174.

3. Free Hydrochloric Acid.^ — Add 4 drops of di-methyl-amino-azobenzene
(Topfer's reagent) solution'* to the contents of the vessel C and titrate with X/io
sodium hydroxide solution until the initial red color is replaced by orange yellow.^
Take the burette reading and calculate the free acidity.

Calculation.— T\it indicator used reacts only to free hydrochloric acid, hence the
number of cubic centimeters of N/io sodium hydroxide used indicates the volume
necessary to neutralize the free hydrochloric acid of 10 cc. of gastric juice. To
determine the data for 100 cc of gastric juice proceed according to the directions
given under Total Acidity, page 174.

4. Combined Acidity. — This value may be obtained by subtracting the number
of cubic centimeters of N/io sodium hydroxide used in neutralizing the contents of
vessel B from the number of cubic centimeters of N/io sodium hydroxide used in
neutralizing A. The data for 100 cc of gastric juice may be calculated according
to directions given under Total Acidity, page 174.

5. Acidity Due to Organic Acids and Acid Salts. — This value may be conven-
iently calculated by subtracting the number of cubic centimeters of N/io sodium
hydroxide used in neutralizing the contents of vessel C from the number of cubic
centimeters of N/io sodium hydroxide solution used in neutralizing the contents of
vessel B. The remainder indicates the number of cubic centimeters of N/io
sodium hydroxide solution necessary to neutralize the acidity due to organic acids
and acid salts present in 10 cc. of gastric juice. The data for 100 cc of gastric
juice may be calculated according to directions given under Total Acidity, page 174.

^ One CO. of N/io hydrochloric acid contains 0.00365 gram of hydrochloric acid.
^ One gram of sodium alizarin sulphonate dissolved in 100 cc. of water.
^ Hydrochloric acid not combined with protein material.
* One-half gram dissolved in 100 cc. of 95 per cent alcohol.

^ If the orange yellow color appears as soon as the indicator is added it denotes the ab-
sence of free acid.

CHAPTER IX

FATS

Fats occur very widely distributed in the plant and animal king-
doms, and constitute the third general class of food-stuffs. In plant
organisms they are to be found in the seeds, roots, and fruit while each
individual tissue and organ of an animal organism contains more or less
of the substance. In the animal organism fats are especially abundant
in the bone marrow and adipose tissue. They contain the same ele-
ments as the carbohydrates, i.e., carbon, hydrogen, and oxygen, but
the oxygen is present in smaller percentage than in the carbohydrates

Fig. 50. — Beef Fat. {Long.)

and the hydrogen and oxygen are not present in the proportion to form
water.

Chemically considered the fats are esters^ of the tri-atomic alcohol,
glycerol, and the mono-basic fatty acids. In the formation of these fats
three molecules of water result. This water arises by the replacement
of the H's of the carboxyl groups of the three fatty acid molecules by
the glycerol radical, thus yielding the following type of formula. In
this case the combination is with palmitic acid (C15H31COOH).

CH2— OOCH31C15
I

CH-OOCH31C16.
I
CH2— OOCH31C15

^ An ester is an oxyacid, one of whose acid hydrogens is replaced by an organic radical.

176

FATS 177

The three fatty acid radicals entering into the structure of a neutral
fat may be the radicals of the same fatty acid or they may consist of
the radicals of three different fatty acids.

By hydrolysis of a neutral fat, i.e., by the addition to the molecule
of those elements which are eliminated in the formation of the fat from
glycerol and fatty acid, it may be resolved into its component parts,
i.e., glycerol and fatty acid. In the case of palmitin the following
would be the reaction:

C3H5(OCi5H3iCO)3+3H20-^C3H5(OH)3+3(Ci5H3iCOOH).

Palmitin. Glycerol. Palmitic acid.

This process is called saponification and may be produced by boiling
with alkalis; by the action of steam under pressure; by long-continued
contact with air and light; by the action of certain bacteria and by
fat-splitting enzymes or lipases, e.g., pancreatic lipase (see page 188).
The cells forming the walls of the intestines evidently possess the pecul-
iar property of synthesizing the glycerol and fatty acid thus formed so
that after absorption these bodies appear in the blood not in their
individual form but as neutral fats.

The principal animal fats wdth \\±iich we have to deal are stearin,
palmitin, olein, and butyrin. Such less important forms as laurin and
myristin may occur abundantly in plant organisms. The older system
of nomenclature for these fats was to apply the prefix "tri" in each
case {e.g., /n-palmitin) since three fatty acid radicals are contained in
the neutral fat molecule.

The fatty acids corresponding to the above-mentioned animal fats
are stearic, CH3(CH2)i6COOH; palmitic, CH3(CH2)i4COOH; oleic,
CH3(CH2)7CH = CH(CH2)7COOH; and butyric, CH3(CH2)2COOH.
Stearic, palmitic and butyric acids are saturated fatty acids, whereas
oleic acid belongs to the class of unsaturated acids. Linoleic acid is
also unsaturated. Upon the presence of these unsaturated fatty acids
depends the property which certain fats possess of absorbing or combin-
ing with iodine. The determination of this so-called "iodine absorption
number" is important in the differentiation of fats and oils. Fats
containing the unsaturated acids oleic and linoleic may be transformed
by "hydrogenation"^ into the fats containing the corresponding
saturated acid (stearic) . The oleic acid is changed thus :

C18H34O2 + 2H— ^CisHseOa-

Oleic acid. Stearic acid.

Fats occur ordinarily as mixtures of several individual fats. For
example, the fat found in animal tissues is a mixture of olein, palmitin
* Addition of hydrogen to the molecule, producing a "hydrogenated fat."

lyS PHYSIOLOGICAL CHEMISTRY

and stearin, the percentage of any one of these fats present depending
upon the particular species of animal from whose tissue the fat was
derived. Thus the ordinary mutton fat contains more stearin and less
olein than the pork fat. Human fat contains from 67 per cent to 85 per
cent of olein and, according to Benedict and Osterberg, upon analysis
yields 76.08 per cent of carbon and 11.78 per cent of hydrogen. Butter
consists in large part of olein and palmitin. Stearin, butyrin, caproin
and traces of other fats are also present.

Pure neutral fats are odorless, tasteless, and generally colorless.
They are insoluble in the ordinary protein solvents such as water, salt
solutions, and dilute acids and alkalis, but are very readily soluble in
ether, benzene, chloroform, and boiling alcohol. The neutral fats are
non-volatile substances possessing a neutral reaction. If allowed to
remain in contact with the air for a sufficient length of time they become
yellow in color, assume an acid reaction and are said to be rancid. The
neutral fats may be crystallized, some of them with great facility. The
crystalline forms of some of the more common fats are reproduced in
Figs. 50, 51 and 52 on pages 176, 179 and 181. Each individual fat
possesses a specific melting- or boiling-point (according to whether the
body is solid or fluid in character), and this property of melting or boiling
at a definite temperature may be used as a means of differentiation in
the same way as the coagulation temperature (see page 105) is used for
the differentiation for coagulable proteins. When shaken with water,
or a solution of albumin, soap, or acacia, the liquid fats are finely divided
and assume a condition known as an emulsion. The emulsion with
water is transitory, while the emulsions with soap, acacia, or albumin
are permanent.

The fat ingested continues essentially unaltered until it reaches the
intestine where it is acted upon by pancreatic lipase (steapsin), the fat-
splitting enzyme of the pancreatic juice (see page 188), and glycerol
and fatty acid are formed. The glycerol is absorbed directly. The
fatty acid thus formed unites with the alkalis of the pancreatic juice
and forms soluble soaps. These soaps are readily absorbed. That
bile is of assistance in the absorption of fat is indicated by the
increase of fat in the feces when for any reason bile does not pass
into the intestine. Bloor^ claims that neither petroleum hydrocar-
bons nor nonsaponifiable esters, e.g., wool fat (lanolin), are absorbed.
He believes that saponification is a necessary preliminary to absorption.

The fat distributed throughout the animal body is formed partly
from the ingested fat and partly from carbohydrates and the "carbon

^ Bloor: Jour. Biol. Chem., 15, 105, 1913.

FATS 179

moiety" of protein material. The formation of adipocere^ and the
occurrence of fatty degeneration are sometimes given as proofs of the
formation of fat from protein. This is questioned by many investiga-
tors. Rather more satisfactory and direct proof of the formation of fat
from protein material has been obtained by Hofmann in experimentation
with fly-maggots. The normal content of fat in a number of maggots
was determined and later the fat content of others which had developed
in blood (84 per cent of the solid matter of blood plasma is protein
material) was determined. The fat content was found to have in-
creased 700 to HOC per cent as a result of the diet of blood proteins.

Fig. 51. — Mutton Fat. (Long.)

The celebrated experiments of Pettenkofer and Voit, however, have
furnished what is, perhaps, the most substantial positive e\ddence of
the formation of fat from protein. These investigators fed dogs large
amounts of lean meat, daily, and through examination of urine, feces and
expired air were enabled to account for only part of the ingested carbon,
although obtaining a satisfactory nitrogen balance. The discrepancy
in the carbon balance was explained upon the theory that the protein of
the ingested meat had been split into a nitrogenons and a non-nitroge-
nous portion in the organism, and that the non-nitrogenous portion, the
so-called "carbon moiety" of the protein, had been subsequently trans-
formed into fat and deposited as such in the tissues of the organism.
Later evidence in favor of the formation of fat from protein has
been furnished by the experiments of Weinland. This investigator
worked with the larvae of Calliphorar these larvae being rubbed up
in a mortar^ with Witte's peptone and water to form a homogeneous

' A very complete analysis of adipocere was reported by Ruttan and Marshall before
the Society of Biological Chemists, Boston, Dec. 27, 1915.
^ The ordinary "blow-fly."

l8o PHYSIOLOGICAL CHEMISTRY

mixture. After placing these mixtures at 38°C. for 24 hours the fat
content was found to have increased, as much as 140 per cent in some
instances. The active agency in this transformation of fat is the larval
tissue, since the tissues of both the dead and living larvae possess the
property. Data are given from control tests which show that the action
of bacteria in this transformation of protein was excluded.

Some investigators are not inclined to accept any data regarding the
formation of fat from protein as conclusive.

Experiments on Fats

1. Solubility. — Test the solubility of olive oil in water, dilute acid and alkali
and in cold alcohol, hot alcohol, chloroform, ether, and carbon tetrachloride.

2. Formation of a Transparent Spot on Paper. — Place a drop of olive oil
upon a piece of ordinary writing paper. Note the transparent appearance of the
paper at the point of contact with the fat.

3. Reaction. — ^Try the reaction of fresh olive oil to litmus, Congo red and phe-
nolphthalein. Repeat the test with rancid olive oil.^ What is the reaction of a
fresh fat and how does this reaction change upon allowing the fat to stand for some
time?

4. Formation of Acrolein. — To a Uttle oUve oil in a mortar add some dry potas-
sium bisulphate, EIHSO4, and rub up thoroughly. Transfer to a dry test-tube
and cautiously heat. Note the irritating odor of acrolein. The glycerol of the
fat has been dehydrolyzed and acrylic aldehyde or acrolein has been produced.
This is the reaction which takes place :

CH2OH CHO

CHOH -^ CH+2H2O.

I II

CH2OH CH2

Glycerol. Acrolein.

5. Emulsification. — (a) Shake up a drop of neutral' oUve oil with a little water
in a test-tube. The fat becomes finely divided, forming an emulsion. This
is not a permanent emulsion since the fat separates and rises to the top upon
standing.

(b) To 5 c.c. of water in a test-tube add 2 or 3 drops of 0.5 per cent Na2C03.
Introduce into this faintly alkaline solution a drop of neutral oUve oil and shake.
The emulsion while not permanent is not so transitory as in the caes of water free
from sodium carbonate.

(c) Repeat (b) using rancid olive oil. What sort of an emulsion do you get

' Intact larvae were used in some experiments.

* To prepare rancid olive oil add 5 drops of oleic acid to 10 c.c. of olive oil.

^ Neutral olive oil may be prepared by shaking ordinary olive oil with a lo per cent
solution of sodium carbonate. This mixture should then be extracted with ether and the
ether removed by evaporation. The residue is neutral olive oil.

FATS

I»I

and why? It is impossible to emulsify a highly rancid fat due to the excessive
formation of rather insoluble soaps about the oil drops.

(d) Shake a drop of neutral olive oil with dilute albumin solution. What is
the nature of this emulsion? Examine it under the microscope.

6. Fat Crystals. — Dissolve a small piece of lard in ether in a test-tube, add
an equal volimie of alcohol and allow the alcohol-ether mixture to evaporate
spontaneously. Examine the crystals under the microscope and compare them
with those reproduced in Figs. 50, 51, and 52, on pages 176, 179 and 181.

7. Saponification of Bayberry Tallow.' — Fill a large casserole two-thirds
full of water rendered strongly alkaUne with soUd potassium hydroxide (a. stick
one inch in length). Add about 10 grams of bayberry tallow and boil, keeping
the volume constant by adding water as needed. When saponification is com-

PoRK Fat.

plete^ remove 25 c.c. of the soap solution for use in Experiment 8 and add concen-
trated hydrochloric acid slowly to the remainder until no further precipitate is
produced.' Cool the solution and the precipitate of free fatty acid will rise to the
surface and form a cake. In this instance the fatty acid is principally palmitic
acid. Remove the cake, break it into small pieces, wash it with water by decan-
tation and transfer to a small beaker by means of 95 per cent alcohol. Heat on a
water-bath imtil the palmitic acid is dissolved, then filter through a dry filter
paper and allow the filtrate to cool slowly in order to obtain satisfactory crystals.
Write the reactions which have taken place in this experiment.

When the palmitic acid has completely crystallized filter off the alcohol, dry
the crystals between filter papers and try the tests given in Experiment 10, p. 182.

8. Salting-out Experiments. — To 25 c.c. of soap solution, prepared as de-
scribed above, add soUd sodiimi chloride to the point of saturation, with continual
stirring. A menstruum is thus formed in which the soap is insoluble. This

1 Bayberry tallow is derived from the fatty covering of the berries of the u-ax myrtle. It
is therefore frequently called "myrtle wax" or "bayberry wax."

^ Place 2 or 3 drops in a test-tube full of water. If saponification is complete the prod-
ucts will remain in solution and no oil will separate.

'Under some conditions a purer product is obtained if the soap solution is cooled before
precipitating the fatty acid.

I»2

PHYSIOLOGICAL CHEMISTRY

salting-out process is entirely analogous to the salting-out of proteins (see page
102).

9. Formation of Insoluble Soaps. — Introduce 5 c.c. of soap solution into each
of two test-tubes. To the contents of one tube add a small amount of a solution
of calcium chloride and to the contents of the other tube add a small amount
of a solution of magnesimn sulphate. Note the formation of insoluble soaps of
calcimn and magnesium.

10. Palmitic Acid. — (a) Examine the crystals under the microscope and com-
pare them with those shown in Fig. 53, below.

(b) SolubiUty. — ^Try the solubiUty of palmitic acid in the same solvents as used
on fats (see page 180).

(c) Melting-point. — Determine the melting-point of palmitic acid by one of
the methods given on page 183.

Fig. 53.^ — Palmitic Acid.

(d) Formation of Transparent Spot on Paper. — Melt a httle of the fatty acid
and allow a drop to fall upon a piece of ordinary writing paper. How does this
compare with the action of a fat under similar circumstances?

(e) Acrolein Test. — ^Apply the test as given under 4, page 180. Explain the
result.

(f) Iodine Absorption Test. — For directions see Experiment 13.

11. Saponification of Lard. — To 25 grams of lard in a fiask add 75 c.c. of
alcohoUc -potash solution and warm upon a water-bath until saponification is
complete. (This point is indicated by the complete solubility of a drop of the
solution when allowed to fall into a Uttle water.) Now transfer the solution from
the flask to an evaporating dish containing about 100 c.c. of water and heat on a
water-bath until all the alcohol has been driven off. Precipitate the fatty acid
with hydrochloric acid and cool the solution. Remove the fatty acid which rises
to the surface,^ neutralize the solution with sodiimi carbonate and evaporate to
dryness. Extract the residue with alcohol, remove the alcohol by evaporation
upon a water-bath and on the residue of glycerol thus obtained make the tests
as given below.

12. Glycerol, (a) Taste.— What is the taste of glycerol?

^ After drying the acid make an iodine absorption test as described in Experiment 13.

FATS

183

Oe

(b) Solubility. — Try the solubility of glycerol in water, alcohol and ether.

(c) H5rpochlorite-Orcinol Reaction.' — This is based on the oxida-
tion of glycerol to the corresponding aldose sugar glycerose and the
detection of the latter by means of orcinol. Homologues of glycerol
as well as the corresponding acids and certain sugars as glucose and
mannose give the reaction. The first named occur seldom while the
latter may be removed with baryta.

Two to 3 c.c. of a I per cent or Ko per cent solution of glycerol in water is
treated with exactly 3 drops ( = 0.12 c.c.) normal NaOCl- and boiled for a minute.
To the Uquid while still hot add 3 drops of hydrochloric acid (sp. gr. 1.124) and
boil 30-60 seconds to drive off chlorine, a
colorless solution being obtained. Then add
an equal volume of f xmiing hydrochloric acid and
a small knife -point of orcinol. On boiling the
mixture becomes a beautiful violet or green blue.
The precipitate formed is soluble in amyl alcohol
and may be examined spectroscopically.

(d) Acrolein Test. — Repeat the test as given
under 4, page 180.

(e) Borax Fusion Test. — Fuse a little
glycerol on a platinum wire with some powdered
borax and note the characteristic green flame.
This color is due to the glycerol ester of boric
acid.

(f) Fehling's Test. — ^How does this result
compare with the results on the sugars?

(g) Solution of Cu(OH)2. Form a little
cupric hydroxide by mixing copper sulphate
and potassium hydroxide. Add a little glycerol
to this suspended precipitate and note what
occurs.

13. Iodine Absorption Test. — Dissolve a
small amount of an unsaturated organic acid,
e.g., oleic acid, in chloroform. Add 2-3 drops
of Hiibl's iodine solution^ and shake. The solu-
tion will be decolorized if unsatiirated acids are
present. This is due to the absorption of the
iodine. The test should be controlled by shak-
ing chloroform and iodine solution to which no
acid has been added.

14. Melting-point of Fat.— First Method. —

Insert one of the melting-point tubes, furnished by the instructor, into the
liquid fat and draw up the fat until the bulb of the tube is about one -half full
of the material. Then fuse one end of the tube in the flame of a Bunsen burner

' Mandel and Neuberg: Block. Zcil., 71, 214, 1915.
^ Made according to Raschig: Bcr., 40, 4586, 1907.

' Prepared by dissolving 26 grams of iodine and 30 grams of mercuric chloride in one
liter of 95 per cent alcohol.

OS

Fig. 54. — Melting-point
Apparatus.

184 PHYSIOLOGICAL CHEMISTRY

and fasten the tube to a thermometer by means of a rubber band in such a maimer
that the bottom of the fat col'omn is on a level with the bulb of the thermometer
(Fig. 54, p. 183). Fill a beaker of medium size about two-thirds full of water and
place it within a second larger beaker which also contains water, the two vessels
being separated by pieces of cork. Immerse the bulb of the thermometer and
the attached tube in such a way that the bulb is about midway between the
upper and the lower surfaces of the water of the inner beaker. The upper
end of the tube being open it must extend above the surface of the surround-
ing water. Apply gentle heat, stir the water, and note the temperature at
which the fat first begins to melt. This point is indicated by the initial trans-
parency. For ordinary fats, raise the temperature very cautiously from 30°C.
To determine the congealing-point remove the flame and note the temperature
at which the fat begins to soUdify. Record the melting- and congealing-points
of the various fats submitted by the instructor.

Second Method. — Fill a small evaporating dish about one-half full of mercury
and place it on a water-bath. Put a small drop of the fat under examination on an
ordinary cover-glass and place this upon the surface of the mercury. Raise the
temperature of the water-bath slowly and by means of a thermometer whose bulb
is immersed in the mercury, note the melting-point of the fat. Determine the con-
gealing-point by removing the flame and leaving the fat drop and cover-glass in
position upon the mercury. How do the melting-points as determined by this
method compare with those as determined by the first method? Which method
is the more accurate, and why?

CHAPTER X
' PANCREATIC DIGESTION^

As soon as the food mixture leaves the stomach it comes into inti-
mate contact with the bile and the pancreatic juice. Since these fluids
are alkaline in reaction (see Bile, page 202) there can obviously be no
further peptic activity after they have become intimately mixed with
the chyme and have neutralized the acidity previously imparted to it
by the hydrochloric acid of the gastric juice. The pancreatic juice
reaches the intestine through the duct of Wirsung which opens into the
intestine near the pylorus.

Normally the secretion of pancreatic juice is brought about by the
stimulation produced by the acid chyme as it enters the duodenum.
Therefore, any factor which produces an increased flow of gastric juice
such, for example, as water^ will cause a stimulation of the pancreatic
secretion. The secretion of pancreatic juice is probably not due to a
nervous reflex as was believed by Pawlow but rather, as Bayliss and
Starling have shown, is dependent upon the presence, in the epithelial
cells of the duodenum and jejunum of a body known as prosecretin.
This body is changed into secretin through the hydrolytic action of the
acid present in the chyme. The secretin is then absorbed by the blood,
passes to the pancreas and stimulates the pancreatic cells, causing a
flow of pancreatic juice. The quantity of juice secreted under these
conditions is proportional to the amount of secretin present. The
activity of secretin solutions is not diminished by boiling, hence the
body does not react like an enzyme. Further study of the body may
show it to be a definite chemical individual of relatively low molecular
weight. It has not been possible thus far to obtain secretin from any
tissues except the mucous membrane of the duodenum and jejunum.

This secretin mentioned above belongs to the class of substances
called hormones or chemical messengers. These hormones play a very
important part in the coordination of the activities of certain functions
and glands. Other important hormones are those elaborated by the
thyroids, the adrenals, the pituitary body (hypophysis), the embryo and

^ Under this head we will consider only such digestive processes as are brought about
by enzymes originating in the pancreas. In the following chapter on Intestinal Digestion
will be found a consideration of such enzymes as have a true intestinal origin.

* See chapter on Gastric Digestion.

185

1 86 PHYSIOLOGICAL CHEMISTRY

the reproductive glands. It is claimed by some that all active organs
of the body produce hormones.

The juice as obtained from a permanent fistula differs greatly in
its properties from the juice as obtained from a temporary fistula, and
neither form of fluid possesses the properties of the normal fluid. Pan-
creatic juice collected by Glaessner from a natural fistula has been
found to be a colorless, clear, strongly alkaline fluid which foams readily.
It is "further characterized by containing albumin, globulin, proteose,
and peptone; nucleoprotein is also present in traces.^ The average
daily secretion of pancreatic juice is 650 c.c. and its specific gravity is
1.008. The fluid .contains 1.3 per cent of solid matter and the freezing-
point is — o.47°C. The normal pancreatic secretion contains at least
four distinct enzymes. They are trypsin, a proteolytic enzyme; pan-
creatic amylase (amylopsin), an amylolytic enzyme; pancreatic lipase
(steapsin) , a fat-splitting enzyme ; and pancreatic rennin, a milk-coagu-
lating enzyme.

The most important of the four enzymes of the pancreatic juice is
the proteolytic enzyme trypsin. This enzyme resembles pepsin in so
far as each has the power of breaking down protein material, but the
trypsin has much greater digestive power and is able to cause a more
complete decomposition of the complex protein molecule. In the
process of normal digestion the protein constituents of the diet are for
the most part transformed into proteoses (albumoses) and peptones
before coming in contact with the enzyme trypsin. This is not abso-
lutely essential, however, since trypsin possesses digestive activity suffi-
cient to transform unaltered native proteins and to produce from their
complex molecules comparatively simple fragments. Among the prod-
ucts of tryptic digestion are ^ro/eo5ej, peptones, peptides, leucine, tyrosine,
aspartic acid, glutamic acid, alanine, phenylalanine, glycocoll, cystine,
serine, valine, proline, oxyproline, isoleucine, arginine, lysine, histidine,
and tryptophane. (The crystalline forms of many of these products are
reproduced in Chapter IV.) Trypsin does not occur preformed h^ the
gland, but exists there as a. zymogen called trypsinogen which bears the
same relation to trypsin that pepsinogen does to pepsin. Trypsin has
never been obtained in a pure form and therefore very little can be
stated definitely as to its nature. The enzyme is the most active in
alkaline solution but is also active in neutral or slightly acid solutions.
Trypsin is destroyed by mineral acids and may also be destroyed by
comparatively weak alkali (2 per cent sodium carbonate) if left in con-
tact for a sufficiently long time. Trypsinogen, on the other hand, is
more resistant to the action of alkalis. In pancreatic digestion the pro-

^ Glaessner: Zeitschrift jUr physiologische Cheniie, 40, 476, 1904.

PANCREATIC DIGESTION 1 87

tein does not swell as is the case in gastric digestion, but becomes more
or less "honey-combed" and finally disintegrates.

The presence of active pepsin in the contents of the intestine has
been demonstrated by Abderhalden and Meyer. ^ It may possibly be
that pepsin may play a part in the profound intestinal proteolysis which
has up to this time been assigned to trypsin and erepsin (see chapter on
Gastric Digestion).

The pancreatic juice which is collected by means of a fistula pos-
sesses- practically no power to digest protein matter. A body called
enter okinase occurs in the intestinal juice and has the power of converting
trypsinogen into trypsin. This process is known as the " activation" of
trypsinogen and through it a juice which is incapable of digesting pro-
tein may be made active. (For further discussion of enterokinase
see chapter on Intestinal Digestion.) Mendel and Rettger- and others
have demonstrated that activation of tr^-psinogen into trypsin may be
brought about in the gland as well as in the intestine of the li\'ing
organism. The manner of the activation in the gland and the nature
of the body causing it are unknown at present. Prym'^ denies that
such an activation occurs.

Delezenne claims that trypsinogen may be activated by soluble
calcium salts. He reports experiments which indicate that proteolytic-
ally inactive pancreatic juice, obtained directly from the duct, when
treated \vith salts of this character, assumes the property of digesting
protein material. This process by which the tripsinogen is activated
through the instrumentality of calcium salts is very rapid and is desig-
nated by Delezenne as an "explosion." The suggestion of Mays that
there may possibly be several precursors of tripsin otie of which is
activated by enterokinase and the others by other agents, is of interest
in this connection.

Boldyreff ^ has demonstrated the presence of trypsin in the stomach
due to the regurgitation of duodenal contents through the pylorus
(see Chapters VII and VIII). Others^ have confirmed this finding (see
chapter on Gastric Analysis).

Pancreatic amylase {amylopsin), the second of the pancreatic en-
zymes, is an amylolytic enzyme which possesses somewhat greater diges-
tive power than the salivary amylase (ptyalin) of the saliva. As its
name implies, its acti\Tty is confined to the starches, and the products
of its amylolytic action are dextrins and sugar. The sugar is principally

^Abderhalden and Meyer: Zeit. physiol. C/tem., 74, 67, 191 1.
-Mendel and Rettger: American Journal of Physiology, 7.
' Prym: Pfliiger^s Archiv, 104 and 107.

<Boldyreff: Transactions of the nth Pirogoff's Congress of Physicians, St. Petersburg,
1910.

'Spencer, Meyer, Rehfuss and Hawk: American Jour. Physiol., 39, 459, 1916.

1 88 PHYSIOLOGICAL CHEMISTRY

maltose and this by the further action of an inverting enzyme (maltase)
is transformed into glucose.

It is possible that the saliva as a digestive fluid is not absolutely
essential. The salivary amylase (ptyalin) is destroyed by the hydro-
chloric acid of the gastric juice and is therefore inactive when the chyme
reaches the intestine. Should undigested starch be present at this
point, however, it would be quickly transformed by the active pancreatic
amylase. This enzyme is not present in the pancreatic juice of infants
during the first few weeks of life, thus showing very clearly that a starchy
diet is not normal for this period.

The pronounced influence of electrolytes upon the action of pancrea-
tic amylase and other amylases has been demonstrated many times. ^
In fact the removal of electrolytes from pancreatic juice by dialysis
yields a juice which possesses no power to split starch. It also appears
that the CI or Br ion is absolutely essential to the activity of animal
amylases.^

It has been claimed that pancreatic amylase has a slight digestive
action upon unboiled starch.

The extent to which amylase is present in the feces has been taken as
the index of pancreatic activity.

The third enzyme of the pancreatic juice is called pancreatic lipase
{steapsin) and is a fat-splitting enzyme. It has the power of splitting
the neutral fats of the food by hydrolysis, into fatty acid and glycerol.
A typical reaction would be as follows:

C3H5(OCi5H3iCO)3+3H20^3(Ci5H3iCOOH)+C3H5(OH)3.

Palmitin. Palmitic acid. Glycerol.

Recent researches make it probable that fats undergo saponifica-
tion to a certain extent prior to their absorption. The fatty acids
formed unite with the alkalis of the pancreatic juice and intestinal
secretion to form soluble soaps which are readily absorbed. It was
formerly believed that the fats could also be absorbed in emulsion —
a condition promoted by the presence of the soluble soaps. After ab-
sorption the fatty acids are resynthesized to form neutral fats with
glycerol.

Bloor^ has reported experiments which "make it extremely probable
that fats can be absorbed only in water-soluble form and that saponi-
fication is a necessary preliminary to absorption." Petroleum hydro-
carbons and non-saponifiable esters, e.g., wool fat (lanolin) were un-

^ For the literature see Kendall and Sherman: Jour. Am. Cheni. Soc, 32, 1087, 1910.
* Wohlgemuth: Biochem. Zeit., 9, 10, 1908; and Kendall and Sherman: Jour. Am. Chem.
Soc, 32, 1087 1910. Bierry: Biochem. Zeit., 40, 357, 1912.
' Bloor: Jour. Biol. Chem., 15, 105, 1913.

PANCREATIC DIGESTION 1 89

absorbed. Bloor further claims^ that in the absorption of fats there is
a tendency toward the formation of a uniform chyle fat, presumably the
characteristic body fat of the animal.

Pancreatic lipase is very unstable and is easily rendered inert by the
action of acid. For this reason it is not possible to prepare an extract
having a satisfactory fat-splitting power from a pancreas which has
been removed from the organism for a sufficiently long time to have
become acid in reaction.

The fourth enzyme of the pancreatic juice is called pancreatic rennin.
It is a milk-coagulating enzyme whose action is very similar to that
of the gastric rennin found in the gastric juice. It is supposed to show
its greatest activity at a temperature varying from 60° to 65°C.

PREPARATION OF AN ARTIFICIAL PANCREATIC JUICE^

After removing the fat from the pancreas of a pig or sheep, finely divide the
organ by means of scissors and grind it in a mortar. If convenient, the use of an
ordinary meat chopper is a very satisfactory means of preparing the pancreas.

When finely divided as above the pancreas should be placed in a 500 c.c.
flask, about 150 c.c. of 30 per cent alcohol added and the flask and contents shaken
frequently for 24 hours. (What is the reaction of this alcoholic extract at the end
of this period, and why?) Strain the alcohoUc extract through cheese cloth,
filter, nearly neutraUze with potassiimi hydroxide solution and then exactly
neutrahze it with 0.5 per cent sodium carbonate.

Products of Tryptic Digestion

Take about 200 grams of lean beef which has been freed from fat and finely
ground and place it in a large-sized beaker. Introduce equal volumes of the pan-
creatic extract prepared as above and 0.5 per cent sodium carbonate, add 5 c.c.
of an alcohoUc solution of thymol to prevent putrefaction, and place the beaker in
an incubator at 40°C. Stir the contents of the beaker frequently and add more
thymol if it becomes necessary. Allow digestion to proceed for from two to five
days and then separate the products formed as follows: Strain off the undis-
solved residue through cheese cloth, nearly neutralize the solution with dilute
hydrochloric acid and then exactly neutraUze it with 0.2 per cent hydrochloric acid.
A precipitate at this point would indicate alkaU metaprotein (alkali albiuninate).
Filter off any precipitate and divide the filtrate into two parts, a one-fourth and a
three-fourth portion.

Transfer the one-fourth portion to an evaporating dish and make the sepa-
ration of proteoses and peptones as weU as the final tests upon these bodies
according to the directions given on page 120.

Place about 5 c.c. of the three -fourth portion in a test-tube and add about
I c.c. of bromine water. A violet coloration^ indicates the presence of trypto-

' Bloor: Jonr. Biol. Cliem., 16, 517, 1914.

- For other methods of preparation see Karl ^lays: Zeitschrift fur physiologische Chetnie,
38, 428, 1903.

*Kurajefif: Zeit. physiol. Chetn., 36,. 501, 1898-99.

190 PHYSIOLOGICAL CHEMISTRY

phane (see page 77. Also see glycyl-tryptophane reaction in chapter on Intes-
tinal Digestion). To another 5 c.c. add 10 drops of concentrated sulphuric acid
and 10 c.c. of a 10 per cent solution of mercuric sulphate in 5 per cent sulphuric
acid. Shake the tube and allow to stand five minutes. A yellow precipitate of a
mercury compound of trjrptophane forms. ^ Concentrate- the remainder of the
three-fourths portion to a thin syrup and make the separation of leucine and tyro-
sine according to the directions given on page 85.

GENERAL EXPERIMENTS ON PANCREATIC DIGESTION

Experiments on Trypsin^

1. The Most Favorable Reaction for Tryptic Digestion. — Prepare seven tubes
as follows :

(a) 2-3 c.c. of neutral pancreatic extract +2-3 c.c. of water.

(b) 2-3 c.c. of neutral pancreatic extract+2-3 c.c. of i per cent sodium car-
bonate.

(c) 2-3 c.c. of neutral pancreatic extract+2-3 c.c. of 0.5 per cent sodium
carbonate.

(d) 2-3 c.c. of neutral pancreatic extract+2-3 c.c. of 0.2 per cent hydro-
chloric acid.

(e) 2-3 c.c. of neutral pancreatic extract+2-3 c.c. of 0.2 per cent combined
hydrochloric acid.

(f) 2-3 c.c. of neutral pancreatic extract+2-3 c.c. of 0.4 per cent boric acid.

(g) 2-3 c.c. of neutral pancreatic extract+2-3 c.c. of 0.4 per cent acetic acid.
Add a small piece of fibrin^ to the contents of each tube and keep them at 40°C.

noting the progress of digestion. In which tube do we find the most satisfactory
digestion, and why? How do the indications of the digestion of fibrin by trypsin
differ from the indications of the digestion of fibrin by pepsin?

2. The Most Favorable Temperature. — (For this and the following series of
experiments under tryptic digestion use the neutral extract plus an equal volume
of 0.5 per cent sodium carbonate.) In each of four tubes place 5 c.c. of alkaline
pancreatic extract. Immerse one tube in cold water from the faucet, keep a
second at room temperature and place a third in the incubator or water-bath at
40°C. Boil the contents of the fourth for a few moments, then cool and also keep
it at 40°C. Into each tube introduce a small piece of fibrin and note the progress
of digestion. In which tube does the most rapid digestion occur? What is the
reason?

3. Influence of Bile. — Prepare three tubes as follows :

(a) 5 c.c. of pancreatic extract+i/2-1 c.c. of bile.

(b) 5 c.c. of pancreatic extract+5 c.c. of bile.

' It has been claimed that a similar yellow precipitate forms in the presence of tyrosine,
cystine and polypeptides. For quantitative estimation of tryptophane see Homer: Jour.
Biol. Chetn., 22, 369, 1915.

2 If the solution is alkaline in reaction, while it is being concentrated, the amino acids
will be broken down and ammonia will be liberated.

' For these experiments as well as for those on the other pancreatic enzymes commer-
cial preparations of trypsin and pancreatin may be employed.

^ Congo red fibrin may be used in this and the following tests on tryptic digestion. If
used the experiments should be made at room temperature. For preparation of this
fibrin see Chapter I.

PANCREATIC DIGESTION IQI

(c) 5 c.c. of pancreatic extract.

Introduce into each tube a small piece of fibrin and keep them at 40'C.
Shake the tubes frequently and note the -progress of digestion. Does the pres-
ence of bile retard tryptic digestion? How do these results agree with those
obtained under gastric digestion?

4. Quantitative Determination of Tryptic Activity.^ — Gross' Method. — This
method is based upon the principle that faintly alkahne solutions of casein are
precipitated upon the addition of dilute ( 1 per cent j acetic acid whereas its digestion
products are not so precipitated. The method follows : Prepare a series of tubes
each containing 10 c.c. of a o.i per cent solution of pure, fat-free casein,- which
has been heated to a temperature of 4o''C. Add to the contents of the series of
tubes increasing amounts of the trypsin solution under examination,- and place
them at 40^0. for fifteen minutes. At the end of this time remove the tubes and
acidify the contents of each with a few drops of dilute (i per centj acetic acid.
The tubes in which the casein is completely digested will remain clear when
acidified, while those tubes which contain undigested casein will become more
or less txirbid under these conditions. Select the first tube in the series which
exhibits no turbidity upon acidification, thus indicating complete digestion of
the casein, and calculate the tryptic activity of the enzyme solution under ex-
amination.

Calcxilation. — The unit of tryptic activity is an expression of the power of i
c.c. of the fluid under examination exerted for a period of fifteen minutes on 10
c.c. of a 0.1 per cent casein solution. For example, if 0.5 c.c. of a trypsin solu-
tion completely digests 10 c.c. of a o.i per cent solution of casein in fifteen
minutes the activity of that solution would be expressed as follows :

Tryptic activity = 1 -^ 0.5 = 2.

Such a trypsin solution would be said to possess an activity of 2. If 0.3 c.c
of the trypsin solution had been required the solution would be said to possess an
activity of 3.3 ; i.e., i -T-0.3 =3.3.

Experiments on Pancreatic Amylase

I. The Most Favorable Reaction. — ^Prepare seven tubes as follows:

(a) I c.c. of neutral pancreatic extract + 1 c.c. of starch paste -1-2 c.c. of
water.

(b) I c.c. of neutral pancreatic extract+i c.c. of starch paste + 2 c.c. of
I per cent sodiimi carbonate.

(c) I c.c. of neutral pancreatic extract +i c.c. of starch paste + 2 c.c. of
0.5 per cent sodium carbonate.

(d) I c.c. of neutral pancreatic extract+i c.c. of starch paste +2 c.c. of
0.2 per cent hydrochloric acid.

Shake each tube thoroughly and place them in the incubator or water-bath
at 40°C. At the end of a half -hour divide the contents of each tube into two parts
and test one part by the iodine test and the other part by Fehhng's test. Where

' For a discussion of Spencer's method for the quantitative determination of tr\-psin
in stomach contents see chapter on Gastric Anal^'sis.

* Made by dissolving 1 gram of Griibler's casein in a liter of 0.1 per cent sodium car-
bonate. A little chloroform may be added to prevent bacterial action.

'The amount of solution used may vary from 0.1- 1 c.c. The measurements may
conveniently be made by means of a i c.c. graduated pipette.

192 PHYSIOLOGICAL CHEMISTRY

do you find the most satisfactory digestion? How do the results compare with
those obtained from the similar series under Trypsin, page 190?

2. The Most Favorable Temperature. — (For this and the following series of
experiments upon pancreatic amylase use the neutral extract plus an equal vol-
imie of 0.5 per cent soditun carbonate.) In each of fovu: tubes place 2-3 c.c. of
alkaline pancreatic extract. Immerse one tube in cold water from the faucet,
keep a second at room temperature, and place a third on the water-bath at 40°C.
Boil the contents of the fourth for a few moments, then cool and also keep it at
40°C. Into each tube introduce 2-3 c.c. of starch paste and note the progress of
digestion. At the end of one-half hoiu' divide the contents of each tube into two
parts and test one part by the iodine test and the other part by Fehling's test.
In which tube do you find the most satisfactory digestion? How does this result
compare with the result obtained in the similar series of experiments under
Trypsin (see page 190)?

3. Influence of Bile. — ^Prepare three tubes as follows :

(a) 2-3 c.c. of pancreatic extract+2-3 c.c. of starch paste + i/2-1 c.c. of
bUe.

(b) 2-3 c.c. of pancreatic extract+2-3 c.c. of starch paste+5 c.c. of bile.

(c) 2-3 c.c. of pancreatic extract+2-3 c.c. of starch paste.

Shake the tubes thoroughly and place them in the incubator or water-bath
at 40°C. Note the progress of digestion frequently and at the end of a half -hour
divide the contents of each tube into two parts and test one part by the iodine
test and the other part by Fehling's test. What are yoiu* conclusions regarding
the influence of bile upon the action of pancreatic amylase?

4. Digestion of Dry Starch. — To a little dry starch in a test-tube add about
5 c.c. of pancreatic extract and place the tube in the incubator or water-bath at
40°C. At the end of a half-hour filter and test separate portions of the filtrate
by the iodine and Fehling tests. What do you conclude regarding the action of
pancreatic amylase upon dry starch? Compare this result with that obtained in
the similar experiment under Salivary Digestion (page 60).

5. Digestion of Inulin.— To 5 c.c. of inulin solution in a test-tube add 10 drops
of pancreatic extract and place the tube in the incubator or water-bath at 40°C.
After one-half hour test the solution by Fehling's test.^ Is any reducing substance
present? What do you conclude regarding the digestion of inulin by pancreatic
amylase?

6. Quantitative Determination of Amylolytic Activity. — ^Wohlgemuth's
Method.- Arrange a series of test-tubes with diminishing quantities of the
enzyme solution under examination, introduce into each tube 5 c.c. of i per cent
solution of soluble starch^ and place each tube at once in a bath of ice-water.*

^ If the inulin solution gives a reduction before being acted upon by the pancreatic juice
it will be necessary to determine the extent of the original reduction by means of a "check"
test (see p. 47).

^ Wohlgemuth: Biochemische Zeitschrift, 9, i, 1908.

' Kahlbaum's soluble starch is satisfactory. In preparing the i per cent solution, the
weighed starch powder should be dissolved in cold distilled water in a casserole and stirred
until a homogeneous suspension is obtained. The mixture should then be heated, with con-
stant stirring, untU it is clear. This ordinarily takes about 8-10 minutes. A slightly opaque
solution is thus obtained which should be cooled and made up to the proper volume before
using.

* Ordinarily a series of six tubes is satisfactory, the volumes of the enzyme solution used
ranging from 1 c.c. to o.i c.c. and the measurements being made by means of a i c.c. gradu-
ated pipette Each tube should be placed in the ice-water bath as soon as the starch solu-
tion is introduced. It will be found convenient to use a small wire basket to hold the tubes.

PANCREATIC DIGESTION 1 93

When all the tubes have been prepared in this way and placed in the ice-water
bath they are transferred to a water-bath or incubator and kept at 38'C. for from
30 minutes to an hour.' At the end of this digestion period the tubes are again
removed to the bath of ice-water in order that the action of the enzyme may
be stopped.

Dilute the contents of each tube, to within about i 2 inch of the top, with
water, add one drop of a N / 10 solution of iodine and shake the tube and contents
thoroughly. A series of colors ranging from dark blue through bluish violet and
reddish yellow to yellow, will be formed. - The dark blue color shows the presence
of unchanged starch, the bluish-violet indicates a mixture of starch and erythro-
dextrin, whereas the reddish-yellow signifies that erythro dextrin and maltose are
present and the yellow solution denotes the complete transformation of starch
into maltose. Examine the tubes carefully before a white background and select
the last tube in the series which shows the entire absence of all blue color, thus
indicating that the starch has been completely transformed into dextrins and
sugar. In case of indecision between two tubes, add an extra drop of the iodine
solution, and observe them again, after shaking.

Calculation. — The amylolytic activity' of a given solution is expressed in terms
of the activity of i c.c. of such a solution. For example, if it is found that 0.02
CO. of an amylolytic solution, acting at 38'C., completely transformed the starch
in 5 c.c. of a I per cent starch solution in 30 minutes, the amylolytic activity of
such a solution would be expressed as follows :

I>3o'=250

This indicates that i c.c. of the solution under examination possesses the power
of completely digesting 250 c.c. of i per cent starch solution in 30 minutes at
38X.

"Wohlgemuth has suggested a slight alteration in the above procedure for use
in the determination of the amylase content of the feces. ^ A modification of the
Wohlgemuth procedure'' for this purpose is given in the chapter on Feces.

Experiments on Pancreatic Lipase

1. "Litmus-milk" Test. — Into each of two test-tubes introduce 10 c.c. of milk
and a small amount of htmus solution. To the contents of one tube add 3 c.c.
of neutral pancreatic extract"^ and to the contents of the other tube add 3 c.c. of
water or of boiled neutral pancreatic extract. Keep the tubes at 40'C. and note
any changes which may occur. What is the result and how do you explain it?

2. Ethyl Butyrate Test. — Into each of two test-tubes introduce 4 c.c. of water,
2 c.c. of ethyl butyrate, C3H7COO.C H,, and a small amount of Utmus powder.
To the contents of one tube add 4 c.c. of neutral pancreatic extract and to the
contents of the other tube add 4 c.c. of water or of boiled neutral pancreatic ex-

' Longer digestion periods may be used where it is deemed advisable. If exceedingly
weak solutions are being investigated, it may be most satisfactory to permit the digestion to
extend over a period of 24 hours.

* See p. 56.

' Designated by "D" the first letter of "diastatic."

* Wohlgemuth : Berliner klinische Wochcnschrijt, 47, 92, 1910.
^ Hawk: Archives of Internal Medicine, 8, 552, 191 1.

^ Commercial pancreatin may be used in this test if desired.

194 PHYSIOLOGICAL CHEMISTRY

tract. Keep the tubes at 40°C. and observe any change which may occur.
What is the result and how do you explain it? Write the equation for the reac-
tion which has taken place.

Experiments on Pancreatic Rennin

Prepare four test-tubes as follows :

(a) 5 c.c. of milk+io drops of neutral pancreatic extract.

(b) 5 c.c. of milk +20 drops of neutral pancreatic extract.

(c) 5 c.c. of milk+io drops of alkaline pancreatic extract.

(d) 5 c.c. of milk+20 drops of alkaline pancreatic extract.

Place the tubes at 6o°-65°C. for a half hour without shaking. Note the
formation of a clot.^ How does the action of pancreatic rennin compare with the
action of the gastric rennin?

* This reaction will not always succeed, owing to conditions which are not well under-
stood.

CHAPTER XI
INTESTINAL DIGESTION

Strictly speaking, all digestive processes which take place in the
intestine may be classed under Intestinal Digestion. However, we will
consider under Intestinal Digestion only those digestive processes
which are brought about by enzymes which have their origin in the intes-
tine. The activities of those enzymes which originate in the pancreas
we have considered in Chapter X under Pancreatic Digestion,

The enzymes of the intestinal juice {succus entericus) are of great
importance to the animal organism. These enzymes include erepsin,
sucrose, maltase, lactase, nucleases, and enterokinase.

Erepsin is a proteolytic enzyme which has the property of acting
upon the proteoses, peptones, and peptides which are formed through the
action of trypsin, and further splitting them into amino-acids. Erepsin
has no power of digesting any native proteins except caseinogen. his-
tones, and protamines. It possesses its greatest activity in an alkaline
solution, although it is slightly active in acid solution. An extract of the
intestinal erepsin may be prepared by treating the finely divided intes-
tine of a cat, dog, or pig with toluol- or chloroform-water and permitting
the mixture to stand with occasional shaking for 24-72 hours. Enzymes
similar to erepsin occur in various tissues of the organism.

In cases of gastric cancer a peptide-splitting enzyme is claimed to
be present in the stomach contents. The glycyl-tryptophane test is
sometimes used for its detection. Some investigators claim that the
peptide-splitting power of gastric juice in cancer is generally due to the
regurgitation of trypsin or erepsin from the intestine or to the presence
in the gastric contents of swallowed saliva which possesses peptolytic
power. The peptide-splitting power of saliva may be due to a specific
enzyme or to the presence of bacteria (see Glycyltryptophane Reaction,
page 199).

The three invertases sucrase, maltase, and lactase are also important
enzymes of the intestinal mucosa. The sucrase acts upon sucrose
and inverts it with the formation of invert sugar (glucose and fructose).
Some investigators claim that sucrase is also present in saliva and
gastric juice. It probably docs not exist normally in either of these

195

196 PHYSIOLOGICAL CHEMISTRY

digestive juices, however, and if found owes its presence to the excretory
processes of certain bacteria. Sucrases may also be obtained from
several vegetable sources. For investigational purposes it is ordinarily
obtained from yeast (see page 14). It exhibits its greatest activity
in the presence of a slight acidity, but if the acidity be increased to any
extent the reaction is inhibited.

Lactase is an enzyme which inverts lactose with the consequent
formation of glucose and galactose. Its action is entirely analogous,
in type, to that of sucrase. It has apparently been proven that lactase
occurs in the intestinal mucosa of the young of all animals which suckle
their offspring.^ It may also occur in the intestinal mucosa of certain
adult animals if such animals be maintained upon a ration containing
more or less lactose. Fischer and Armstrong have demonstrated the
reversible action^ of lactase.

Maltase possesses the power of splitting maltose, the end-product
of the digestion of starch, into glucose. It was first discovered in the
urine and shortly after this time its presence was noted in the small
intestine and the saliva. Corn is sometimes used as the medium for
the preparation of the enzyme for experimental purposes. It occurs
in corn in a very active state. It was in connection with maltase that
the principles of the "reversibility of enzyme action" were first
demonstrated.

Enierokinase possesses the power of "activating" trypsinogen see
Chapters I and X). In other words, trypsinogen as formed by the
pancreas has no proteolytic power, but when this inactive trypsino-
gen reaches the intestine and comes into contact with enterokinase the
latter transforms it into active trypsin. Enterokinase is not always
present in the intestinal juice since it is secreted only after the pan-
creatic juice reaches the intestine. It resembles the enzymes in that
its activity is destroyed by heat, but differs materially from this class
of bodies in that a certain quantity is capable of activating only a
definite quantity of trypsinogen. It is, however, generally classified
as an enzyme. Enterokinase has been detected in the higher animals,
and a kinase possessing similar properties has been shown to be present
in bacteria, fungi, impure fibrin, lymph glands, and snake-venom.

The intestinal juice and the epithelium of the intestinal wall con-
tain enzymes capable of hydrolyzing nucleic acids and as these acids
are not acted upon by the gastric juice and probably not to any great
extent by pure pancreatic juice, the intestine apparently plays the chief
role in decomposition or digestion of these substances. At least two

1 Mendel and Mitchell: American Journal of Physiology, 20, 81, 1907.

2 See p. 8.

PANCREATIC DIGESTION 1 97

enzymes take part in this digestion process, one decomposing the
nucleic acid with formation of simple nucleotides containing a single
radical each of phosphoric acid, carbohydrate and base (see chapter
on Nucleic Acids). This enzyme may be called nudeicacidase. An-
other enzyme present in the intestine and intestinal juice decomposes
these nucleotides with the liberation of phosphoric acid. This enzyme
may be called ■nucleotidase or phosplwnuclcase. The intestinal mucosa
also decomposes many other organic phosphorus compounds with libera-
tion of their phosphoric acid.^ Thus glycero-phosphoric acid and
hexose-phosphoric acid as well as phosphoproteins are split in a similar
manner, the phosphoric acid they contain thus being absorbed in the
free form.

General Experiments on Intestinal Digestion

Demonstration of Enterokinase. — Trypsinogen may be activated
by enterokinase. This activation occurs normally in the intestine.
Calcium salts also bring about a similar activation of the trypsinogen.

Procedure. — Prepare an extract of trypsinogen by grinding 10 grams of the
fresh, fat-free pancreas of the pig with a Uttle sand. Gradually add 100 c.c.
of water during the grinding process. Strain through cheese cloth.

Prepare an extract of enterokinase by grinding 5 grams of fresh, fat-free
duodenal mucosa- of the pig with a Uttle sand. Gradually add 50 c.c. of water
during the grinding process. Strain through cheese cloth.

Prepare the following series of tubes :

(a) 10 c.c. pancreas extract+5 c.c. water.

(b) 10 c.c. pancreas extract+5 c.c. duodenal extract.

(c) 5 c.c. duodenal extract +10 c.c. water.

(d) 10 c.c. pancreas extract+5 cc. duodenal extract.

(e) 10 c.c. pancreas extract+5 c.c. duodenal extract (boiled^*.

(f) 10 c.c. pancreas extract+5 c.c. of 4 per cent calcium chloride.

Boil the contents of tube (d) for five minutes and cool to 40°C. Keep all six tubes
at 40°C. for 20 minutes.

To each tube add 5 c.c. of 10 per cent sodium carbonate and mix the contents
thoroughly and immediately. Introduce into each tube the same quantity (size
of a pea) of fresh fibrin. Shake the tubes and place them at 40°C. Observe the
tubes frequently for one hour to note digestive changes. Tubes (b) and (f)
should show most rapid digestion. Why?

Experiments on Intestinal Nucleases

I. Preparation of Intestinal Extract. — Wash thoroughly 100 grams of pig's
intestine and run through a meat chopper several times. Introduce into a 500
c.c. mixing cyUnder and add normal salt solution to make 500 c.c. Allow to

^ Plimmer: Biochem. J., 7, 43, 1913.

^ The dried mucosa may be substituted if desired.

198 PHYSIOLOGICAL CHEMISTRY

stand for 6-24 hours at room temperatxire, shaking occasionally, toluol being
added as a preservative. Strain and filter.

2. Demonstration of Intestinal Nucleases. — Prepare a 2 per cent solution
of yeast nucleic acid put in solution with the aid of just sufficient NaOH solution
to make the resulting mixture neutral to Utmus. To each of two large test-tubes
add 20 c.c. of the intestinal extract prepared as above. Boil one for one to two
minutes. To each tube then add 10 c.c. of the 2 per cent nucleic acid solution.
Add 2-3 c.c. each of toluol and chloroform to each mixture. Keep at 38°C. for
24 hours.

Heat the tubes to boiling in a water-bath to coagulate protein. Add 5 c.c. of
5 per cent HCl and allow to stand for one hour. This precipitates any unchanged
nucleic acid. Filter and take aUquots of the filtrate (about 20 c.c). Precipitate
the phosphate from each mixture by adding 5 c.c. of magnesia mixture and 5 c.c.
of ammonia. Allow to stand over night. A heavy precipitate of magnesium
ammonium phosphate should be found in the test experiment indicating that the
phosphoric acid of the nucleic acid had been Uberated by the nucleotidase of the
intestinal extract. The control should show only a sUght precipitate.

If desired the phosphorus of the precipitates may be determined quantitatively
by dissolving in 2 per cent HNO3, precipitating as the phosphomolybdate and
determining volumetrically according to the Neumann procedure (see 554).

Experiments on Erepsin

1. Preparation of Erepsin. — Grind the mucous membrane of the small intes-
tine of a cat, dog, or pig with sand in a mortar. Treat the finely divided membrane
with toluol- or chloroform-water and permit the mixture to stand, with occasional
shaking, for 24-72 hours. ^ Filter the extract thus prepared through cotton and
use the filtrate in the following experiment.

2. Demonstration of Erepsin. — To about 5 c.c. of a i per cent solution of
Witte's peptone in a test-tube add about i c.c. of the erepsin extract prepared as
described above and make the mixture slightly alkaUne (o.i per cent) with sodiimi
carbonate. Prepare a second tube containing a like amount of peptone solution
but boil the erepsin extract before introducing it. Place the two tubes at 38°C.
for two to three days. At the end of that period heat the contents of each tube
to boiling, filter and try the biuret test on each filtrate. In making these tests
care should be taken to use Uke amounts of filtrate, potassium hydroxide and
copper sulphate in each test in order that the drawing of correct conclusions may
be faciUtated. The contents of the tube which contained the boiled extract
should show a deep pink color with the biuret test, due to the peptone still present.
On the other hand, the biuret test upon the contents of the tube containing the
unboiled extract should be negative or exhibit, at the most, a faint pink or blue
color, signifying that the peptone, through the influence of the erepsin, has been
transformed, in great part at least, into amino-acids which do not respond to the
biuret test-

1 The enzyme may also be extracted by means of glycerol or alkaline "physiological" salt
solution if desired.

^ Strictly speaking, this erepsin demonstration is not adequate unless a control test
is made with native protein (except casein, histones and protamines) to show that the
extract is trypsin-free and digests peptone but not native protein.

INTESTINAL DIGESTION 1 99

3. The Glycyl-tryptophane Reaction. — The dipeptide glycyl -tryptophane 1
may be used in place of the peptone solution for the demonstration of erepsin.
It is claimed to be of service in the diagnosis of gastric cancer. It is claimed that
a peptide -spUtting enzyme (erepsin) is present in the stomach contents of indi-
viduals suffering from cancer of the stomach, whereas the stomach contents of
normal individuals contains no such enzyme. The glycyl-tryptophane test, there-
fore, may sometimes furnish a means of aiding in the diagnosis of this disorder.
As applied to stomach contents, the test is as follows :- Introduce about 10 c.c. of
the filtrate from the stomach contents into a test-tube, add a little glycyl-trypto-
phane and a layer of toluol, and place the tube in an incubator at 38'C. for 24
hours. At the end of this time by means of a pipette transfer 2-3 c.c. of the fluid
from beneath the toluol to a test-tube, add a few drops of 3 per cent acetic acid
and carefully introduce bromine vapors. Shake the tube and note the production
of a red color if tryptophane is present. The tryptophane has, of course, been
liberated from the peptide through the action of the peptide -spUtting enzyme
(erepsin) elaborated by the cancer tissue.

If an excess of bromine is added the color will vanish. If no rose color is
noted, add more bromine vapors carefully with shaking until further addition of
the vapors causes the production of a yellowish color. This indicates an excess
of bromine and constitutes a negative test. Occasionally the rose color indicating
a positive test is so transitory as to escape detection unless the test be very care-
fully performed.

Several fallacies have been pointed out in connection with this test.
In the first place the regurgitation of duodenal contents through the
pylorus might insure the presence in the stomach of erepsin and trypsin
either of which possesses peptide-splitting power. It has also been
claimed that saliva contains an enzyme capable of splitting glycyl-
tryptophane. Doubt has, however, been cast upon the dipeptide-
splitting agent of the saliva by Smithies^ and by Jacque and Woodyatt,^
who point to bacteria as the peptolytic agents. In any event saliva
contains something which is capable of splitting the glycyltryptophan,
thus making the entrance of saliva into the stomach an important
source of error, so far as the utility of this test is concerned, as a diagnos-
tic aid. Bacteria may, of course, be removed from the gastric juice by
passing the fluid through an efTective filter.

Experiments on Invert ases^

I. Preparation of an Extract of Sucrase. — Treat the finely divided epi-
thelium of the small intestine of a dog, pig, rat, rabbit, or hen with about 3
voltimes of a 2 per cent solution of sodium fluoride and permit the mixture to

^ This dipeptide is sold commercially under the name "Ferment Diagnosticon."
- Neubauer and Fischer: Deulsclies Archiv f. klinische Medizin, 97, 499, 1909.
^ Smithies: Arch. Int. Med., 10, 521, 191 2.

* Jacque and Woodyatt: Arch. Int. Med., Dec, 191 2, p. 560.

* "The Inverting Enzymes of the Alimentary Tract," Mendel and Mitchell: American
Journal of Physiology, 20, 81, 1907-08.

200 PHYSIOLOGICAL CHEMISTRY

stand at room temperature for 24 hours. Strain the extract through cloth or
absorbent cotton and use the strained material in the following demonstration.

2. Demonstration of Sucrase. — To about 5 c.c. of a i per cent solution of
sucrose, in a test-tube, add about i c.c. of a 2 per cent sodium fluoride intes-
tinal extract, prepared as described above. Prepare a control tube in which the
intestinal extract is boiled before being added to the sugar solution. Place the
two tubes at 38°C. for two hours. ^ Heat the mixture to boiUng to coagulate the
protein material, filter, and test the filtrate by Fehling's test (see page 26).
The tube containing the boiled extract should give no response to Fehling's test,
whereas the tube containing the unboiled extract should reduce the Fehling's
solution. This reduction is due to the formation of invert sugar (see page 41 )
from the sucrose through the action of the enzyme sucrase which is present in
the intestinal epithelium.

For preparation and demonstration of Vegetable Sucrase see Chapter I.

3. Preparation of an Extract of Lactase. — Treat the finely divided epithelium
of the small intestine of a kitten, puppy, or pig embryo with about 3 volumes of a
2 per cent solution of sodium fluoride and permit the mixture to stand at room
temperature for 24 hours. Strain the extract through cloth or absorbent cotton
and use the strained material in the following demonstration.

4. Demonstration of Lactase. ^ — To about 5 c.c. of a i per cent solution of
lactose in a test-tube add about i c.c. of a toluol-water or a 2 per cent sodium
fluoride extract of the first part of the small intestine^ of a kitten, puppy, or pig
embryo prepared as described above. Prepare a control tube in which the
intestinal extract is boiled before being added to the sugar solution. Place the
two tubes at 38°C. for 24 hours. At the end of this period add i c.c. of the diges-
tion mixture to 5 c.c. of Barfoed's reagent* and place the tubes in a boiUng water-
bath.^ Examine the tubes at the end of three minutes against a black back-
ground in a good Ught. If no cuprous oxide is visible replace the tubes and
repeat the examination at the end of the fourth and fifth minutes. If no reduc-
tion is then observed permit the tubes to stand at room temperature for 5-10
minutes and examine again. "^

It has been determined that disaccharide solutions will not reduce Barfoed's
reagent until after they have been heated for 9-10 minutes on a boiUng water-
bath in contact with the reagent.^ Therefore in the above test, if the tube con-
taining the unboiled extract exhibits any reduction after being heated as indicated,
for a period of five minutes or less, and the control tube containing boiled extract
shows no reduction, it may be concluded that lactase was present in the intestinal
extract. **

^ If a positive result is not obtained in this time permit the digestion to proceed for a
longer period.

- Roaf: Bio-Chemical Journal, 3, 182, 1908.
' Duodenum and first part of jejunum.

* To 4.5 grams of neutral crystallized copper acetate in 900 c.c. of water add 0.6 c.c. of
glacial acetic acid and make the total volume of the solution i liter.

^ Care should be taken to see that the water in the bath reaches at least to the upper
level of the contents of the tubes.

* Sometimes the drawing of conclusions is facilitated by pouring the mixture from the
tube and examining the bottom of the tube for adherent cuprous oxide.

' The heating for 9-10 minutes is sufficient to transform the disaccharide into mono-
saccharide.

8 The reduction would, of course, be due to the action of the glucose and galactose
which had been formed from the lactose through the action of the enzyme lactase.

INTESTINAL DIGESTION 20I

5. Preparation of an Extract of Maltase.- Treat the finely divided epithelium
of the small intestine of a cat, kitten, or pig fembryo or adult) with about 3
volumes of a 2 per cent solution of sodium fluoride and permit the mixture to
stand at room temperature for 24 hours. Strain the extract through cloth and
use the strained material in the following demonstration.

6. Demonstration of Maltase. — Proceed exactly as indicated in the demon-
stration of lactase, p. 200, except that a i per cent solution of maltose is sub-
stituted for the lactose solution. The extract used may be prepared from the
upper part of the intestine of a cat, kitten, or pig (embryo or adult). In the case
of lactase, as indicated, the intestine used should be that of a kitten, puppy, or
pig (embryo).

CHAPTER XII
BILE

The bile is secreted continuously by the liver and passes into the
intestine through the common bile duct which opens near the pylorus.
Bile is not secreted continuously into the intestine. In a fasting animal
no bile enters the intestine, but when food is taken the bile begins to
flow; the length of time elapsing between the ingestion of the food and
the secretion of the bile as well as the qualitative and quantitative char-
acteristics of the secretion depending upon the nature of the food ingested.
Fats, the extractives of meat and the protein end-products of gas-
tric digestion (proteoses and peptones), cause a copious secretion of bile,
whereas such substances as water, acids and boiled starch paste fail
to do so. In general a rich protein diet is supposed to increase the
amount of bile secreted, whereas a carbohydrate diet would cause a
much less decided increase and might even tend to decrease the amount.
It has been demonstrated by Bayliss and Starling that the secretion of
bile is under the control of the same mechanism that regulates the flow
of pancreatic juice (see page 185). In other words, the hydrochloric
acid of the chyme, as it enters the duodenum transforms prosecretin
into secretin and this in turn enters the circulation, is carried to the
liver, and stimulates the bile-forming mechanism to increased activity.

We may look upon the bile as an excretion as well as a secretion. In
the fulfillment of its excretory function it passes such bodies as lecithin,
metallic substances, cholesterol, and the decomposition products of
hemoglobin into the intestine and in this way aids in removing them
from the organism. The bile assists materially in the absorption of
fats from the intestine by its solvent action on the fatty acids formed
by the action of the pancreatic juice.

The bile is a ropy, viscid substance which is usually alkaline in reac-
tion to litmus, ^ and ordinarily possesses a decidedly bitter taste. It varies
in color in the different animals, the principal variations being yellow,
brown and green. Fresh human bile from the living organism ordi-
narily has a green or golden-yellow color. Post-mortem bile is variable
in color. It is very difficult to determine accurately the amount of
normal bile secreted during any given period. For an adult man it

* It does not contain more than a slight excess of hydroxyl ions, however.

202

BILE

203

has been variously estimated at from 500 c.c. to iioo c.c. for 24 hours.
The specific gravity of the bile varies between i.oio and 1.040, and
the freezing-point is about — o.56°C. As secreted by the liver, the
bile is a clear, limpid fluid which contains a relatively low content of
solid matter. Such bile would have a specific gravity of approximately
I.OIO. After it reaches the gall-bladder, however, it becomes mixed
with mucous material from the walls of the gall-bladder,* and this proc-
ess coupled with the continuous absorption of water from the bile has
a tendency to concentrate the secretion. Therefore the bile as we find it
in the gall-bladder ordinarily possesses a higher specific gravity than
that of the freshly secreted fluid. The specific gravity under these
conditions may run as high as 1.040.

The principal constituents of the bile are the salts of the bile acids,
bile pigments, neutral fats, lecithin, phosphatides, nucleo protein, mucin,
and cholesterol, besides the salts of iron, copper, calcium, and magnesium.
Zinc has also frequently been found in traces.

The quantitative composition of bile varies according to the source
of the bile, i.e., whether the bile for analysis is obtained from the gall-

QUANTITATIVE COMPOSITION OF BILEi
(Parts per 1000)

Constituent

Bladder bile,
Hammartsen-

Biliary fistula,
Rosenbloom'

Water

Solids

' 829.7

170.3

970.2
39-8

Bile salts

Q7 0

10 I

Mucin and pigments

J.I . 0

4.86

Cholesterol

9-9

2.6l5

Fat

I 1-9

6.85

Soaps

II. 2*

1

2.6

Lecithin

' 2.2 '

6.42

Inorganic matter

S.I

9.2

Fatty acids

Included under "soaps"

1.2

* For other analyses see Czylharz, Fuchs and v. Fiirth: Block. Zeit., 49, 120, 1913.

*Hammarsten: Pincussohn's Med.-Chem. Lab. Hilfsbuch, Leipzig, 191 2, p. 388.
'Rosenbloom: Jour. Biol. Chcin., 14, 241, 1913.

* Includes fatty acids.

* Includes cholesterol esters.

204 PHYSIOLOGICAL CHEMISTRY

bladder or by means of a fistula before it reaches the gall-bladder.
The variation in the composition of these two types of bile is shown in
the preceding selected analyses:

The bile acids, which are elaborated exclusively by the hepatic
cells, may be divided into two groups, the glycocholic acid group and
the taurocholic acid group. In human bile glycocholic acid predomi-
nates, while taurocholic acid is the more abundant in the bile of car-
nivora. The bile acids are conjugate amino-acids, the glycocholic
acid yielding glycocoll,

CH2NH2

COOH,

and cholic acid upon decomposition, whereas taurocholic acid give
rise to taurine,

CH2NH2

CH2SO2OH,

and cholic acid under like conditions. Glycocholic acid contains some
nitrogen but no sulphur, whereas taurocholic acid contains both these
elements. The sulphur of the taurocholic acid is present in the taurine
(amino-ethyl-sulphonic-acid) , of which it is a characteristic constituent.
There are several varieties of cholic acid and therefore we have several
forms of glycocholic and taurocholic acids, the variation in constitution
depending upon the nature of the cholic acid which enters into the com-
bination. The bile acids are present in the bile as salts of one of the
alkalis, generally sodium. The sodium glycocholate and sodium tau-
rocholate may be isolated in crystalline form, either as balls or rosettes
of fine needles or in the form of prisms having ordinarily four or six
sides (Fig. 55, page 205) . The salts of the bile acids are dextro-rotatory.
Among other properties these salts have the power of holding the
cholesterol and lecithin of the bile in solution.

Hammarsten has demonstrated a third group of bile acids in the
bile of the shark. This same group very probably occurs in certain
other animals also. These acids are very rich in sulphur and resemble
etheral sulphuric acids inasmuch as upon treatment with boiling hydro-
chloric acid they yield sulphuric acid.

The bile pigments are important and interesting biliary constitu-
ents. The following have been isolated: bilirubin, biliverdin, bili-
fuscin, biliprasin, bilihumin, bilicyanin, choleprasin, and choletelin. Of
these, bilirubin and biliverdin are the most important and predominate
in normal bile. The colors possessed by the various varieties of normal
bile are due almost entirely to these two pigments, the biliverdin being

BILE

20:

the predominant pigment in greenish bile and the bilirubin being the
principal pigment in lighter colored bile. The pigments, other than
the two just mentioned, have been found almost exclusively in biliary
calculi or in altered bile obtained at post-mortem examinations.

Bilirubin, which is perhaps the most important of the bile pigments,
is apparently derived from the blood pigment, the iron freed in the

Fig. 55. — Bile Salts.

process being held in the liver. Bilirubin has the same percentage com-
position as hematoporphyrin, which may be produced from hematin.
It is a specific product of the liver cells, but may also be formed in other
parts of the body. The pigment may be isolated in the form of a
reddish-yellow powder or may be obtained in part, in the form of reddish-

#

t

Fig. 56. — Bilirubin (Hzmatoidin). (Ogden.)

yellow rhombic plates (Fig. 56) upon the spontaneous evaporation
of its chloroform solution. The crystalline form of bilirubin is
practically the same as that of hematoidin. It is easily soluble in
chloroform, somewhat less soluble in alcohol and only slightly soluble
in ether and benzene. Bilirubin has the power of combining with

206 PHYSIOLOGICAL CHEMISTRY

certain metals, particularly calcium, to form combinations which are no
longer soluble in the solvents of the unaltered pigment. Upon long
standing in contact with the air, the reddish-yellow bilirubin is oxidized
with the formation of the green biliverdin. Bilirubin occurs in animal
fluids as soluble bilirubin-alkali.

Solutions of bilirubin exhibit no absorption bands. If an ammonia-
cal solution of bilirubin-alkali in water is treated with a solution of zinc
chloride, however, it shows bands similar to those of bilicyanin (Absorp-
tion Spectra, Plate II), the two bands between C and D being rather
well defined.

Biliverdin is particularly abundant in the bile of herbivora. It is
soluble in alcohol and glacial acetic acid and insoluble in water, chloro-
form, and ether. Biliverdin in formed from bilirubin upon oxidation.
It is an amorphous substance, and in this differs from bilirubin which
may be at least partly crystallized under proper conditions. Biliverdin
may be obtained in the form of a green powder. In common with
bilirubin, it may be converted into hydrobilirubin by nascent hydrogen.

The neutral solution of bilicyanin or cholecyanin is bluish green or
steel blue and possesses a blue fluorescence, the alkaline solution is
green with no appreciable fluorescence, and the strongly acid solution is
violet blue. The alkaline solution exhibits three absorption bands, the
first a dark, well-defined band between C and D, somewhat nearer C;
the second a less sharply defined band extending across D and the third
a rather faint band between E and F, near E (Absorption Spectra, Plate
II). The strongly acid solution exhibits two absorption bands, both
lying between C and E and separated by a narrow space near D. A
third band, exceedingly faint, may ordinarily be seen between b and F.

Bile pigments are converted into urobilinogen (urobilin) in the intes-
tine. This is absorbed, carried to the liver and reconverted into bile
pigment. In diseases of the liver the liver cell loses the capacity to
convert the urobilinogen and this is then excreted in the urine. The
presence of urobilinogen in urine, therefore, may be considered as an
index oi functional liver incapacity.^

Biliary calculi, otherwise designated as biliary concretions or gall
stones, are frequently formed in the gall-bladder. These deposits may
be divided into three classes, cholesterol calculi, pigment calculi, and
calculi made up almost entirely of inorganic material. This last class
of calculus is formed principally of the carbonate and phosphate of
calcium and is rarely found in man although quite common to cattle.
The pigment calculus is also found in cattle, but is more common to
man than the inorganic calculus. This pigment calculus ordinarily

1 Rowntree, Hurwitz and Bloomfield: Johns Hopkins Hospital Bulletin, Nov., 1913.

BILE 207

consists principally of bilirubin in combination with calcium; biliverdin
is sometimes found in small amount. The cholesterol calculus is the one
found most frequently in man. These may be formed almost entirely
of cholesterol, in which event the color of the calculus is very light, or
they may contain more or less pigment and inorganic matter mixed
with the cholesterol, which tends to give us calculi of various colors.
For discussion of cholesterol see page 355.

Experiments on Bile

1. Reaction. — Test the reaction of fresh ox bile to litmus, phenolphthalein and
Congo red.

2. Nucleprotein. — Acidify a small amount of bile with dilute acetic acid. A
precipitate of nucleoprotein forms. Bile acids will also precipitate here under
proper conditions of acidity.

3. Inorganic Constituents. — Test for chlorides, sulphates, and phosphates
(see page 59).

4. Tests for Bile Pigments.— Practically all of these tests for bile
pigments are based on the oxidation of the pigment, by a variety of
reagents, with the formation of a series of colored derivatives, e.g.,
biliverdin (green), bilicyanin (blue), choletelin (yellow).

(a) Gmelin's Test. — To about 5 c.c. of concentrated nitric acid in a test-tube
add 2-3 c.c. of diluted bile carefully so that the two fluids do not mix. At the
point of contact note the various colored rings, green, blue, violet, red and reddish
yellow. Repeat this test with different dilutions of bile and observe its deUcacy.

(b) Rosenbach's Modification of Gmelin's Test. — Filter 5 c.c. of diluted bile
through a small filter paper. Introduce a drop of concentrated nitric acid into
the cone of the paper and note the succession of colors as given in Gmelin's test.

(a) Nakayama's Reaction. — To 5 c.c. of diluted bile in a test-tube add an equal
volume of a 10 per cent solution of barium chloride, centrifugate the mixture, pour
off the supernatant fluid, and heat the precipitate with 2 c.c. of Nakayama's reagent.^
In the presence of bile pigments the solution assumes a blue or green color.

(d) Huppert's Reaction.^ — Thoroughly shake equal volumes of undiluted bile
and milk of lime in a test-tube. The pigments unite with the calcium and are pre-
cipitated. Filter off the precipitate, wash it with water, and transfer to a small
beaker. Add alcohol acidified slightly with hydrochloric acid and warm upon a
water-bath until the solution becomes colored an emerald green.

In examining urine for bile pigments, according to Steensma, this procedure
may give negative results even in the presence of the pigments, owing to the fact
that the acid-alcohol is not a sufllciently strong oxidizing agent. He therefore
suggests the addition of a drop of a 0.5 per cent solution of sodium nitrite to the
acid-alcohol mixture before warming on the water-bath. Try this modification also.

(e) Hammarsten's Reaction.— To about 5 cc. of Hammarsten's reagent- in a

1 Prepared by combining 99 c.c. of alcohol and i c.c. of fuming hydrochloric acid con-
taining 4 grams of ferric chloride per liter.

^ Hammarsten's reagent is made by mi.\ing i volume of 25 per cent nitric acid and 19
volumes of 25 per cent hydrochloric acid and then adding i volume of this acid mbtture
to 4 volumes of 95 per cent alcohol.

2o8 PHYSIOLOGICAL CHEMISTRY

small evaporating dish add a few drops of diluted bile. A green color is produced.
If more of the reagent is now added the play of colors as observed in Gmelin's test
may be obtained.

(f) Smith's Test. — To 2-3 c.c. of diluted bile in a test-tube add carefully about
5 c.c. of dilute tincture of iodine (i : 10) so that the fluids do not mix. A play of
colors, green, blue and violet, is observed. In making this test upon the urine ordin-
arily only the green color is observed.

(g) Salkowski-Schipper's Reaction. — To 10 c.c. of diluted bile in a test-tube
add 5 drops of a 20 per cent solution of sodium carbonate and 10 drops of a 20 per
cent solution of calcium chloride. Filter off the resultant precipitate upon a
hardened filter paper and wash it with water. Remove the precipitate to a small
porcelain dish, add 3 c.c. of an acid-alcohol mixture^ and a few drops of a dilute
solution of sodium nitrite and heat. The production of a green color indicates
the presence of bile pigments.

(h) Bonanno's Reaction.- — Place 5-10 c.c. of diluted bile in a small porcelain
evaporating dish and add a few drops of Bonanno's reagent.^ An emerald-green
color will develop.

5. Tests for Bile Acids. — (a) Sucrose-HoSO^ Test (Pettenkofer). — To 5 c.c
of diluted bile in a test-tube add 5 drops of a 5 per cent solution of sucrose. Now
run about 2-3 c.c. of concentrated sulphuric acid carefully down the side of the
tube and note the red ring at the point of contact. Upon slightly agitating the
contents of the tube the whole solution gradually assumes a reddish color. As
the tube becomes warm, it should be cooled in rurming water in order that the
temperature of the solution may not rise above 7o°C.

It is claimed that this test is not satisfactory in the presence of
protein and chromogenic substances which yield interfering colors
with sulphuric acid.

(b) Furfural-H2S04 Test.— Mylius's Modification of Pettenkofer's Test.—
To approximately 5 c.c. of diluted bile in a test-tube add 3 drops of a very dilute
(i : 1000) aqueous solution of furfural,

HC— CH

II II
HC CCHO.

O

Now run about 23 c.c. of concentrated sulphuric acid carefully down the side of
the tube and note the red ring as above. In this case, also, upon shaking the
tube the whole solution is colored red. Keep the temperature of the solution be-
low 7o°C. as before.

(c) Foam Test (v. Udransky). — ^To 5 c.c. of diluted bile in a test-tube add 3-4
drops of a very dilute (i : 1000) aqueous solution of furfural. Place the thtunb
over the top of the tube and shake the tube until a thick foam is formed. By
means of a small pipette add 2-3 drops of concentrated sulphuric acid to the foam
and note the dark pink coloration produced.

^ Made by adding 5 c.c. of concentrated hj'drochloric acid to 95 c.c. of 96 percent
alcohol.

^11 Tommasi, 2, No. 21.

^ This reagent may be prepared by dissolving 2 grams of sodium nitrite in 100 c.c. of
concentrated hydrochloric acid.

BILE

209

fd) Surface Tension Test (Hay). — This test is based upon the principle that
bile acids have the property of reducing the surface tension of fluids in which they
are contained. The test is performed as follows: Cool about 10 c.c. of diluted
bile in a test-tube to 17 'C. or lower and sprinkle a Uttle finely pulverized sulphur
upon the surface of the fluid. The presence of bile acids is indicated if the
sulphur sinks to the bottom of the Uquid, the rapidity with which the sulphur sinks
depending upon the quantity of bile acids present in the mixture. The test is said
to react with bile acids when they are present in the ratio of i : 120,000.

(e) Neukomm's Modification of Pettenkofer's Test. — To a few drops of
diluted bile in an evaporating dish add a trace of a dilute sucrose solution and one
or more drops of dilute sulphuric acid. Evaporate on a water-bath and note the
development of a violet color at the edge of the evaporating mixture. Discontinue
the evaporation as soon as the color is observed.

(f) Peptone Test (Oliver). — To 5 cc of diluted bile add 2-3 drops of acetic
acid, filtering if necessary. Add an equal volume of a i per cent solution of
Witte's peptone to the acid solution. A precipitate is produced which is insoluble
in excess of acetic acid. This precipitate is a compound of protein and bile acids.

6. CrystaUization of Bile Salts. — To 25 c.c. of undiluted bile in an evaporating
dish add enough animal charcoal to form a paste and evaporate to dryness on a
water-bath. Remove the residue, grind it in a mortar, and transfer it to a small
fiask. Add about 50 c.c. of 95 per cent alcohol and boil on a water-bath for 20
minutes. Filter, and add ether to the filtrate until there is a shght permanent
cloudiness. Cover the vessel and stand it away until crystallization is complete.
Examine the crystals under the microscope and compare them with those shown in
Fig- 55) page 205. Try one of the tests for bile acids upon some of the crystals.

7. Analysis of BiUary Calcuh. — Grind the calculus in a mortar with 10 c.c.
of ether. Filter.

Filtrate I.

I

Add an equal volume of 95 per cent alco-
hol^ to the ether extract, allow the mix-
ture to evaporate and examine for choles-
terol crystals (Fig. 57, page 210). (For
further tests see Experiment 8, p. 210.)

Residue I.
(On paper and in mortar.)

.1

Treat with dilute hydrochloric acid and
filter.

FUtrate U.

Test for calcium, phosphates, and iro>i.
Evaporate remainder of filtrate to dry-
ness in porcelain crucible and ignite.
Dissolve residue in dilute hydrochloric
acid and make alkaline with ammonium
hydroxide. Blue color indicates copper.

Residue n.
(On paper and in mortar.)
Wash with a little water. Dry the filter paper.

Treat with ^ c.c. chloroform and filter.

Filtrate m.
Bilirubin.
(Apply test for
bile pigments.)

Residue III.
(On paper and in mortar.)

Treat with 5
alcohol.

of hot

Bilivcrdin.
* The alcohol is added because of the fact that it is often found that crystallization from
pure ether does not yield typical cholesterol crystals.

14

2IO

PHYSIOLOGICAL CHEMISTRY

8. Tests for Cholesterol.

(a) Microscopical Examination. — Examine the crystals under the microscope
and compare them with those shown in Fig. 57, below.

(b) Sulphuric Acid Test (Salkowski). — Dissolve a few crystals of cholesterol
in a Uttle chloroform and add an equal volxmie of concentrated sulphuric acid.
A play of colors from bluish-red to cherry-red and purple is noted in the chloro-
form while the acid assmnes a marked green fluorescence.

(c) Acetic Anhydride-H2S04 Test (Liebermann-Burchard). — Dissolve a
few crystals of cholesterol in 2 c.c. of chloroform in a dry test-tube. Now add 10
drops of acetic anhydride and 1-3 drops of concentrated sulphuric acid. The
solution becomes red, then blue, and finally bluish-green in color. This reaction
is used in the quantitative determination of cholesterol (see Chapter XVI).

(d) Iodine -sulphuric Acid Test. — Place a few crystals of cholesterol in one of
the depressions of a test-tablet and treat with a drop of concentrated sulphuric acid
and a drop of a very dilute solution of iodine. A play of colors consisting of violet,
blue, green, and red results.

Fig. 57. — Cholesterol.

(e) Schiff's Reaction. — To a little cholesterol in an evaporating dish add a few
drops of a reagent made by adding i volume of 10 per cent ferric chloride to 3 vol-
umes of concentrated sulphuric acid. Evaporate to dryness over a low flame and
observe the reddish-violet residue which changes to a bluish-violet.

9. Preparation of Taurine. — To 300 c.c. of bile in a casserole add 100 c.c. of
hydrochloric acid and heat until a sticky mass (dyslysin) is formed. This point
may be determined by drawing out a thread-like portion of the mass by means of a
glass rod, and if it solidifies immediately and assumes a brittle character we may
conclude that all the taurocholic and glycoholic acid has been decomposed. Decant
the solution and concentrate it to a small volume on the water-bath. Filter the
hot solution to remove sodium chloride and other substances which may have sepa-
rated, and evaporate the filtrate to dryness. Dissolve the residue in 5 per cent
hydrochloric acid and precipitate with 10 volumes of 95 per cent alcohol. Filter
off the taurine and recrystallize it from hot water. (Save the alcoholic filtrate for
the preparation of glycocoll, p. 211.) Make the following tests upon the taurine
crystals.

BILE

211

(a) Examine them under the microscope and compare with Fig. 58.

(b) Heat a crj'stal upon platinum foil. The taurine at first melts, then turns
brown, and finally carbonizes as the temperature is raised. Note the suflfocating
odor. What is it?

Fig. 58. — Taurine.

(c) Test the solubility of the crystals in water and in alcohol.

(d) Grind up a crystal with four times its volume of dry sodium carbonate and
fuse on platinum foil. Cool the residue, transfer it to a test-tube, and dissolve it in
water. Add a little dilute sulphuric acid and note the odor of hydrogen sulphide.
Hold a piece of filter paper, moistened with a small amount of lead acetate, over
the opening of the test-tube and observe the formation of lead sulphide.

'Js>'

■M»
%>-

Fig. 59. — Glycocoll.

10. Preparation of Glycocoll.— Concentrate the alcoholic filtrate from the last
experiment (g) until no more alcohol remains. The glycocoll is present here in the
form of an hydrochloride and may be liberated from this combination by the addi-
tion of freshly precipitated lead hydroxide or by lead hydroxide solution. Remove
the lead by hydrogen sulphide. Filler and decolorize the filtrate by animal char-
coal. Filter again, concentrate the filtrate, and set it aside for crystallization.
Glycocoll separates as colorless crystals (Fig. 50).

CHAPTER XIII
PUTREFACTION PRODUCTS

The putrefactive processes in the intestine are the result of the
action of bacteria upon the protein material present. This bacterial
action which is the combined effort of many forms of micro-organisms
is confined almost exclusively to the large intestine. Some of the prod-
ucts of the putrefaction of proteins are identical with those formed
in tryptic digestion, although the decomposition of the protein material
is much more extensive when subjected to putrefaction. Some of the
more important of the putrefaction products are the following: Indole,
skatole, paracresol, phenol, para-oxy phenylpro pionic acid, para-oxyphen-
ylacetic acid, volatile fatty acids, hydrogen sulphide, methane, methyl
mercaptan, hydrogen, and carbon dioxide, besides proteoses, peptones,
peptides, ammonia, and amino-acids. Basic substances such as choline,
neurine, putrescine and cadaverine are present under certain conditions.
Of the putrefaction products the indole, skatole, phenol, and paracresol
appear in part in the urine as ethereal sulphuric acids, whereas the
oxyacids mentioned pass unchanged into the urine. The potassium
indoxyl sulphate (page 386) content of the urine is a rough indicator
of the extent of the putrefaction within the intestine.

The portion of the indole which is excreted in the urine is first sub-
jected to a series of changes within the organism and is subsequently
eliminated as indican. These changes may be represented thus:

/\ CH /\ C(OH)

I II +0-^ 1 y

CH \/\/CH

NH NH

Indole. Indoxyl.

/\ C(OH) /\ C(0-S03H)

+H2SO4 — I I II +H2O

\/\/CH \/\/CH

NH NH

Indoxyl. Indoxyl sulphuric acid.

In the presence of potassium salts the indoxyl sulphuric acid is then
transformed into indoxyl potassium sulphate (or indican),

^-X C(0-S03K),

I IJ
\/\/CH

NH

and eliminated as such in the urine.

212

PUTREFACTION PRODUCTS 213

Indican may be decomposed by treatment with concentrated hydro-
chloric acid (see tests on page 387) into sulphuric acid and indoxyl.
The latter body may then be oxidized to form indigo-bluc thus:

/\ C(OH) /\ COOC /\v

2 I II +20->| I I , +2H2O

\/CH \/\xc.A.c\/\y

NH NH NH

Indoxyl. Indigo-blue.

This same reaction may also occur under pathological conditions
within the organism, thus giving rise to the appearance of crystals of
indigo-blue in the urine.

Skatole or methyl indole possesses the following structure:

_C(CH3)

\/\/CH
NH

In common with indole it is changed within the organism and eliminated
in the form of a chromogenic substance. Skatole is, however, of less
importance as a putrefaction product than indole and ordinarily occurs
in much smaller amount. The tryptophane group of the protein mole-
cule yields the indole and skatole formed in intestinal putrefaction, but
the reasons for the transformation of the major portion of this trypto-
phane into indole and the minor portion into skatole are not well under-
stood. Indole is more toxic than skatole.

Phenol occurs in fairly large amount in certain abnormal conditions
of the organism, but ordinarily the amount is very small. It is probably
derived from the tyrosine group of the protein molecule. Phenol is
conjugated in the liver to form phenyl potassium sulphate and appears
in the urine in this form (Baumann, and Herter). Para-cresol occurs
in the urine as cresyl potassium sulphate.

Regarding the claim of Nencki that methyl mercaptan is formed
as a gas during intestinal putrefaction it is an important fact that
Herter^ was unable to detect the mercaptan in fresh feces. He was,
therefore, not inclined to accept the theory that methyl mercaptan is
formed in ordinary intestinal putrefaction but believed that it may be
formed in exceptional cases. Hydrogen sulphide is, however, formed in
all cases of intestinal putrefaction.

It has been demonstrated that putrefaction processes in the human
intestine may be retarded by the ingestion of a carbohydrate diet.'^ The
putrefactive organisms are facultative organistfis and prefer a carbo-

1 Herter: "Bacterial Infections of the Digestive Tract, p. 227."

^Kendall: Jour. Med. Res., 24, 411, 1911; also Pediatrics, 23, No. 9, 1910.

214 PHYSIOLOGICAL CHEMISTRY

hydrate medium if it is available. These organisms are also unable to
exert their maximum activity in an acid medium and therefore the
acids resulting from the carbohydrate fermentation would tend to lessen
their activity.

It has been shown by Kutscher and his associates^ that many acids
and bases formed in putrefaction and which have been considered as
originating alone from bacterial action, may also be formed in certain
phases of metabohsm in both the plant and animal kingdoms. These
transformation products of amino-acids have been termed "apor-
rhegmas." The following aporrhegmas may result from putrefaction
processes:

Aporrhegma Atnino-acid source

Iminazolethylamine. .^ \ Histidine.

Iminazolpropionic acid )

Ornithine ]

Tetramethylendiamine [ Arginine.

Aminovalerianic acid J

Pentamethylendiamine Lysine.

Amino-butyric acid Glutamic acid.

^^'^P?---., ) Aspartic acid.

Succinic acid J ^

Isovalerianic acid Leucine.

Phenylethylamine 1

Phenylacetic acid \ Phenylalanine.

Phenylpropionic acid J

/>-Oxyphenylacetic acid. \ Xyj-osine

/>-0.xj^henylpropionic acid J

Indole 1

Skatole. 1 Tryptophane.

indolacetic acid

Indolpropionic acid •. J .

Experiments on Putrefaction Products

In many courses in physiological chemistry the instructors are so
limited for time that no extended study of the products of putrefaction
can very well be attempted. Under such conditions the scheme here
submitted may be used profitably in the way of demonstration. Where
the number of students is not too great, a single large putrefaction vaky
be started, and, after the initial distillation, both the resulting distillate
and residue may be distributed to the members of the class for individual
manipulation.

Preparation of Putrefaction Mixture. — Place a weighed mixture of coagulated
egg albumin and ground lean meat in a flask or bottle and add approximately
2 liters of water for every kilogram of protein used. Sterilize the vessel and con-
tents, inoculate with the colon bacillus, and keep at 40°C. for two or three weeks.
If cultures of the colon bacillus are not available, add 6o c.c. of a cold saturated

1 Ackermann and Kutscher: Zeil. physiol. Cliem., 69, 265, 1910.
Ackermann: Ibid., 273.
Engeland and Kutscher: Ibid., 282.

PUTREFACTION PRODUCTS

21:;

solution of sodium carbonate for every liter of water previously added and
inoculate with some putrescent material (pancreas or feces).' Mix the putre-
faction mixture very thoroughly by shaking and insert a cork furnished with a
glass tube to which is attached a wash bottle containing a 3 per cent solution of
mercuric cyanide.' This device is for the purpose of collecting the methyl
mercaptan, a gas formed during the process of putrefaction. It also serves to
diminish the odor arising from the putrefying material. Place the putrefaction
mixture at 40°C. for two or three weeks and at the end of that time make a sepa-
ration of the products of putrefaction according to the following directions :

Subject the mixture to distillation until the distillate and residue are approxi-
mately equal in volume.

PART I
MANIPULATION OF THE DISTILLATE

Acidify with hydrochloric acid ahd extract with ether.

Ether Extract No. i.

Add an equal \'olume of water, make alka-
line with potassium hj-droxide, and shake
thoroughly. I

Residue No. i.
Allow the ether to volatilize,
rate and detect ammonium
crystals (Fig. 60, page 216).

Evapo-
chloride

Ether Extract No. 2.
Evaporate spontaneously. Indole and
skatol remain. Try proper reactions (see
pages 218 and 219).

Alkaline Solution No. i.
Acidify with hydrochloric acid, add
sodium carbonate, and extract with ether.

Ether Extract No. 3.
Evaporate. Detect phenol
(paracresol). See page 219.

Alkaline Solution No. 2.

and cresol .\cidify with hydrochloric acid,

extract with ether.

and

Ether Extract No. 4.

Evaporate. Volatile folly acids remain.

Final Residue.

( Discard. 1

DETAILED DIRECTIONS FOR MAKING THE SEPARATIONS
INDICATED IN THE SCHEME

Preliminary Ether Extraction. — This extraction may be conveniently conducted
in a separatory funnel. Mix the fluids for extraction in the ratio of two volumes
of ether to three volumes of the distillate. Shake very thoroughly for a few mo-
ments, then draw off the extracted fluid and add a new portion of the distillate.
Repeat the process until the entire distillate has been extracted. Add a small
amount of fresh ether at each extraction lo replace that dissolved by the water in
the preceding extraction.

' Putrefying pri)lein may be prepared 1)\- treating 10 grams of tinely ground lean meat
with 100 c.c. of water and 2 c.c. of a saturated solution of sodium carbonate and keeping
the mixture at 40°C. for 24 hours.

*l$ - Concentrated sulphuric acid containing a small amount of /,<.<;//;/ may be used as a
substitute for mercuric cyanide. When this modilicalion is employed it is necessary to
use calcium chloride tubes to exclude moisture from the isatin solution.

2l6

PHYSIOLOGICAL CHEMISTRY

■• Residue No. i. — Unite the portions of the distillate extracted as above and allow
the ether to volatilize spontaneously. Evaporate until crystallization begins.
Examine the crystals under the microscope. Ammonium chloride predominates.
Explain its presence.

Ether Extract No. i. — Add equal volume of water, render the mixture alkaline
with potassium hydroxide, and shake thoroughly by means of a separatory funnel
as before. The volatile fatty acids, contained among the putrefaction products,
would be dissolved by the alkaline solution (No. i) whereas any indole or skatole
would remain in the ethereal solution (No. 2).

Alkaline Solution No. i. — Acidify with hydrochloric acid and add sodium
carbonate solution until the fluid is neutral or slightly acid from the presence of
carbonic acid. At this point a portion of the solution, after being heated for a few
moments, should possess an alkaline reaction on cooling. Extract the whole mix-
ture with ether in the usual way, using care in the manipulation of the stop cock to

Fig. 60. — Ammonium Chloride.

relieve the pressure due to the evolution of carbon dioxide. The ether (Ether
Extract No. 3) removes any phenol or crcsol which may be present while the volatile
fatty acids will remain in the alkaline solution (No. 2) as alkali salts.

Ether Extract No. 2. — Drive off the major portion of the ether at a low tempera-
ture on a water-bath and allow the residue to evaporate spontaneously. Indole
and skatole should be present here. Prove the presence of these bodies. For
tests for indole and skatole seepages 218 and 219.

Alkaline Solution No. 2. — Make strongly acid with hydrochloric acid and ex-
tract with a small amount of ether, using a separatory funnel. As carbon dioxide is
liberated here, care must be used in the manipulation of the stop cock of the funnel
in relieving the pressure within the vessel. The volatile fatty acids are dissolved
by the ether (Ether Extract No. 4).

Ether Extract No. 3. — Evaporate this ethereal solution on a water-bath. The
oily residue contains phenol and cresol. The cresol is present for the most part as
paracresol. Add some water to the oUy residue and heat it in a flask. Cool and
prove the presence of phenol and cresol. For tests for these bodies see page 219.

Ether Extract No. 4. — Evaporate on a water-bath. The volatile fatty acids
remain in the residue.

PUTREFACTION PRODUCTS

217

PART II

MANIPULATION OF THE RESIDUE

Evaporate, filter, and extract with ether.

Ether Extract.
Evaporate, extract the residue with
warm water, and filter.

Aqueous Solution.
Evaporate until crj'Stals begin to
form. Stand in a cold place until
crystallization is complete. Filter.

Crystalline Deposit.
Consists of a mixture of
leucine and tyrosine crystals
(Figs. 25, 28 and 139, pages
76, 80 and 463.)

Filtrate No. 2.

Contains oxyacids and
skatole-carbonic acid.

Residue.

Contains non-volatile
fatty acids.

Filtrate No. i.
Contains proteose, peptone,
aromatic acids, and tryptophane.

DETAILED DIRECTIONS FOR MAKING THE

SEPARATIONS INDICATED IN

THE SCHEME

Preliminary Ether Extraction. — This extraction may be conducted in a separatory
funnel. In order to make a satisfactory extraction the mixture should be shaken
thoroughly. Separate the ethereal solution from the aqueous portion and treat
them according to the directions given on page 215.

Ether Extract. — Evaporate this solution on a safety water-bath until the ether
has been entirely removed. Extract the residue with warm water and filter.

Aqueous Solution. — Evaporate this solution until crystallization begins. Stand
the solution in a cold place until no more crystals form. This crystalline mass con-
sists of impure leucine and tyrosine. Filter off the crystals.

Crystalline Deposit. — Examine the crystals under the microscope and compare
them with those reproduced in Figs. 25, 28, and 139, pages 76, 80, and 463. Do the
forms of the crj'stals of leucine and tyrosine resemble those previously examined?
Make a separation of the leucine and tyrosine and apply typical tests according to
directions given on pages 85 and 86.

Filtrate No. i. — Make a test for tryptophane with bromine water (see page 189) ,
and also with the Hopkins-Cole reagent (see page 98). Use the remainder of the
filtrate for the separation of proteoses and peptones. Make the separation ac-
cording to the directions given on page 120.

Filtrate No. 2. — This solution contains para-o.xyphenylacetic acid, para-oxy-
phenylpropionic acid and skatole-carbonic acid. Prove the presence of these
bodies by appropriate tests. Tests for o.xyacids and skatole-carbonic acid are
given on page 220.

2l8 PHYSIOLOGICAL CHEMISTRY

TESTS FOR VARIOUS PUTREFACTION PRODUCTS

Tests for Indole

The various tests for indole ond skatole may be carried out upon an
aqueous solution ot these products or upon an aqueous solution of
the residue from Ether Extract No. 2 (see page 172). A distillate
secured by distilling a putrefaction mixture first in alkaline and then
in acid reaction may also be employed.

1. Herter's j5-Naphthaquinone Reaction. — (a) To a dilute aqueous solution
of indole (i : 500,000) add i drop of a 2 per cent solution of /i-naphthaquinone-
sodiiun-monosulphonate. No reaction occurs. Add a drop of a 10 per cent
solution of potassium hydroxide and note the gradual development of a blue
or blue-green color which fades to green if an excess of the alkali is added.
Render the green or blue-green solution acid and note the appearance of a
pink color. Heat faciUtates the development of the color reaction.

One part of indole in one million parts of water may be detected by means of
this test if carefully performed.

(b) If the alkah be added to a more concentrated indole solution before the
the introduction of the naphthaquinone the course of the reaction is different,
particularly if the indole solution is somewhat more concentrated than that men-
tioned above and if heat is used. Under these conditions the blue indole com-
pound ultimately forms as fine acicular crystals which rise to the surface.

If we do not wait for the production of the crystalline body but as soon as the
blue color forms, shake the aqueous solution with chloroform, the blue color dis-
appears from the solution and the chloroform assumes a pinkish-red hue.
This is a distinguishing feature of the indole reaction and facilitates the differen-
tiation of indole from other bodies which yield a similar blue color. A very sat-
isfactory method for the quantitative determination of indole is based upon the
principle underlying this test (see chapter on Feces).

2. Formaldehyde Reaction (Konto). — To i c.c. of the material under exami-
nation in a test-tube add 3 drops of a 40 per cent solution of formaldehyde and i
c.c. of concentrated sulphuric acid. Now agitate the mixture and note the appear-
ance of a violet-red color if a trace of indole is present. The test is said to serve
for the detection of indole when present in a dilution of i : 700,000.

Skatole gives a yellow or brown color under the above conditions.

3. Cholera-red Reaction. — To a little of the material under examination in a
test-tube add one-tenth its voliune of a 0.02 per cent solution of potassium nitrite
and mix thoroughly. Carefully run concentrated sulphuric acid down the side
of the tube so that it forms a layer at the bottom. Note the purple color. Neu-
tralize with potassium hydroxide and observe the production of a bluish-green
color.

4. Nitroprusside Reaction (Legal). — To a small amount of the material under
examination in a test-tube add a few drops of a freshly prepared solution of sodium
nitroprusside, Na2Fe(CN) 5NO+ 2H2O. Render alkaline with potassium hydroxide
and note the production of a violet color. If the solution is now acidified with
glacial acetic acid the violet is transformed into a blue.

PUTREFACTION PRODUCTS 2ig

5. Pine Wood Test. — Moisten a pine splinter with concentrated hydrochloric
acid and insert it into the material under examination. The wood assumes a
cherr>--red color.

6. Nitroso-indole Nitrate Test. — .\cidify some of the material under examina-
tion with nitric acid, add a few drops of a potassium nitrite solution and note the
production of a red precipitate of nitroso-indole nitrate. If the residue contains
but little indole simply a red coloration will result. Compare this result with the
result of the similar test on skatole.

Tests for Skatole

1. Herter's Para-dimethylaminobenzaldehyde Reaction.' — To 5 c.c. of the
distillate or aqueous solution under examination add i c.c. of an acid solution of
para-dimethylaminobenzaldehyde- and heat the mixture to boiling. A purpUsh-
blue coloration is produced which may be intensified through the addition of a
few drops of concentrated hydrochloric acid. If the solution be cooled under
running water it loses its purpUsh tinge of color and becomes a definite blue.
The solution at this point may be somewhat opalescent through the separation of
uncombined para-dimethylaminobenzaldehyde. Care should be taken not to
add an excess of hydrochloric acid inasmuch as the end-reaction has a tendency
to fade under the influence of a high acidity.

A rough idea regarding the actual quantity of skatole in a mixture may be
obtained by extracting this blue solution with chloroform and subsequentiy
comparing this chloroform solution, by means of a colorimeter Duboscq , ^^"ith
the maximal reaction, obtained with a skatole solution of known strength.

2. Color Reaction with Hydrochloric Acid.— Acidify some of the residue with
concentrated hydrochloric acid. Note the production of a \'iolet color.

3. Acidify some of the residue with nitric acid and add a few drops of a potas-
sium nitrite solution. Xote the white turbidity. Compare this result with the
result of the similar test on indole.

Tests for Phenol and Cresole

1. Color Test. — Test a little of the solution with Millon's reagent. A red
color results. Compare this test with the similar one under Tyrosine see page
86).

2. Ferric Chloride Test. — Add a few drops of neutral ferric chloride solution
to a Uttle of the material under examination. A dirty bluish-gray color is formed.

3. Formation of Bromine Compounds. — Add some bromine water to a little
of the fluid under examination. Note the crystalline precipitate of tribrom-
phenol and tribromcresol. The reaction for phenol is as follows:

CeHoOH+sBro^CeH.BraOH-l-sHBr.

Phenol. Tribromphenol.

'.Herter: Bacterial Injections of the Digestive Tract. 1907, p. 141.

* Made by dissolving 5 grams of para-dimethylaminobenzaldehyde in 100 c.c. of 10
per cent sulphuric acid.

' If the color does not appear add more of the aldehyde solution.

2 20 PHYSIOLOGICAL CHEMISTRY

4. Nitric Acid Test. — ^Add some nitric acid to some of the material under
examination. Heat and note a yellow color due to the production of picric acid
(trinitrophenol) from phenol. This is the reaction :

C6H50H+3HN03^C6H2(N02)30H+3H20.

Phenol. Picric acid.

Tests for Oxyacids

1. Color Test. — Test a little of the solution with Millon's reagent. A red color
results.

2. Bromine Water Test.^ — Add a few drops of bromine water to some of the
filtrate. A turbidity or precipitate is observed.

Test for Skatole -carbonic Acid

Ferric Chloride Test. — Acidify some of the filtrate with hydrochloric acid, add
a few drops of ferric chloride solution, and heat. Compare the end-reaction with
that given by phenol.

CHAPTER XIV
FECES

The feces are the residual mass of material remaining in the intes-
tine after the full and complete exercise of the digestive and absorptive
functions and are ultimately expelled from the body through the rectum.

They may be said to be composed of the following substances:

1. Food residues: (a) those portions of the food which have escaped
absorption, and (b) that part of the diet either not digested or incapable
of absorption.

2. The remains of the intestinal and digestive secretions not
destroyed or reabsorbed.

3. Substances excreted into the intestinal tract, notably salts of
calcium, iron, and other metals.

4. The bacterial flora of the intestinal tract.

5. Cellular elements to which may be added, under pathological
conditions, blood, pus, mucus, serum, and parasites.

6. Abnormally: enteroliths, gall stones, and pancreatic calculi.
The amount of the fecal discharge varies with the individual and the

diet. Upon an ordinary mixed diet various authorities claim that the
daily excretion by an adult male will aggregate 1 10-170 grams with a
soUd content ranging between 25 and 45 grams; the fecal discharge of
such an individual upon a vegetable diet will.be much greater and may
even be as great as 350 grams and possess a solid content of 75 grams.
In the author's own experience the average daily output of moist feces,
calculated on the basis of data secured from the examination of over
1000 stools, was about 100 grams. The variation in the normal daily
output being so great renders this factor of very little value for diag-
nostic purposes, except where the composition of the diet is accurately
known. Lesions of the digestive tract, a defective absorptive function,
or increased peristalsis as well as an admixture of mucus, pus, blood,
and pathological products of the intestinal wall may cause the total
amount of excrement to be markedly increased. An idea of the varia-
tion of the percentage of dry matter in the feces evacuated after the
ingestion of different diets may be gathered from a consideration of the
following table. ^

'Schmidt & Strasburger: "Die Fazes des Menschen", Berlin iqi5

221

222

PHYSIOLOGICAL CHEMISTRY

INFLUENCE OF DIET ON FECAL DRY MATTER

Diet

Dry Matter Percent.

Nursing infant .
Milk '

[ Adult.

Meat

Bread

Potatoes. . . .
Cabbage ....
Mixed Diet. .

15.0

28.0
29.0
25.0
15-0
4-4
26.0

The fecal pigment of the normal adult is hydrobilirubin This,
pigment originates from the bilirubin which is secreted into the intes-
tine in the bile, the transformation from bilirubin to hydrobilirubin
being brought about through the activity of certain bacteria. Hydro-
bilirubin is sometimes called stercobilin
and bears a close resemblance to urobilin
or may even be identical with that pig-
ment. Neither bilirubin nor biliverdin
occurs normally in the fecal discharge of
adults, although the former may be de-
tected in the excrement of nursing in-
fants. If these pigments are found in
the feces of adults, they indicate an
abnormally rapid transit through the
large bowel thus preventing their trans-
formation into hydrobilirubin. Fre-
quently, in some way as yet unknown,
probably through the agency of certain bacterial processes, color-
less hydrobilirubinogen (leucohydrobilirubin) is formed which after
the passage of the movement and exposure to air is reconverted
into hydrobilirubin. This may explain in some cases the darken-
ing of the stool when exposed to the air. The most important
factor in determining the color of the fecal discharge is the diet. A
mixed diet, for instance, produces stools which vary in color from light
to dark brown, an exclusive meat diet gives rise to a brownish-black
stool, whereas the stool resulting from a milk diet is invariably light
colored. Certain pigmented foods, such as the chlorophyllic vegetables
and various varieties of berries, each afford stools having a characteristic
color. Certain drugs act in a similar way to color the fecal discharge.
This is well illustrated by the occurrence of green stools following the use
of calomel, of black stools after bismuth ingestion, and of yellow stools
following the administration of rhubarb, senna or santonin. The green

Fig. 61. — Hematoidin Crys-

T.A.LS FROM ACHOLIC StOOLS. {v.

Jaksch.)

Color of crystals same as the color
of those in Fig. 56, page 205.

FECES 223

color of the calomel stool is generally believed to be due to biliverdin.
V. Jaksch, however, claims to have proven this view to be incorrect
since he was able to detect hydrobilirubin (or urobilin) but no biliverdin
in stools after the administration of calomel. The bismuth stool was at
one time thought to derive its color from the black sulphide which is
formed from the subnitrate of bismuth. We now know^ that the color
is due to the reduction of the bismuth compound (subnitrate) to bismuth
suboxide. In cases of biliary obstruction the grayish-white acholic
stool is formed.

Under normal conditions the odor of feces is due to skatole and
indole, two bodies formed in the course of putrefactive processes occur-
ring within the intestine (see page 212). Such bodies as methane,
methyl mercaptan, and hydrogen sulphide may also add to the disagree-
able character of the odor. The intensity of the odor depends to a
large degree upon the character of the diet, being very marked in stools
from a meat diet, much less marked in stools from a vegetable diet, and
frequently hardly detectable in stools from a milk diet. Thus the stool
of the infant is ordinarily nearly odorless and any decided odor may
generally be readily traced to some pathological source.

A neutral reaction ordinarily predominates in normal stools, although
slightly alkaline or even acid stools are met with. The acid reaction is
encountered much less frequently than the alkaline, and then commonly
only following a vegetable diet.

Experiments in which the actual hydrogen ion concentration of the
feces was determined indicate that the reaction of the excreta is uni-
formly slightly alkaline.- Pronounced dietary changes, e.g., low protein
diet, high protein diet, fasting, water drinking with meals, produce at
most only minor changes in the reaction of the feces.

The form and consistency of the stool is dependent, in large measure,
upon the nature of the diet. Under normal conditions the consistency
may vary from a thin, pasty discharge to a firmly formed stool. Stools
which are exceedingly thin- and watery ordinarily have a pathological
significance. In general the feces of the carnivorous animals is of a
firmer consistency than that of the herbivora.

The continued ingestion of a diet which is very thoroughly digested
and absorbed is frequently accompanied by the formation of dry. hard
fecal masses (scybala). Constipation generally results, due to the small
bulk of the feces and its lack of moisture. At present the formation of
scybala is considered pathological, as an expression of spastic constipa-
tion. To counteract this tendency toward constipation the ingestion

' Quincke: Miinch. med. Woch., p. 854, 1896.

* Howe and Hawk: Jour. Biol. Chem., 11, 129, 191 2.

2 24 PHYSIOLOGICAL CHEMISTRY

of agar-agar'^ has been suggested." This agar is relatively indigestible
and readily absorbs water (about i6 times its weight), thus forming a
bulky fecal mass which is sufficiently soft to permit of easy evacuation.
The function of agar is not limited to its use in connection with consti-
pation ; it may serve in other capacities as an aid to intestinal therapeu-
tics by serving as a vehicle for certain drugs. ^

It is frequently desirable for clinical or experimental purposes to
make an examination of the fecal output which constitutes the residual
mass from a certain definite diet. Under such conditions, it is custom-
ary to cause the person under observation to ingest some substance, at
the beginning and end of the period in question, which shall sufficiently
differ in color and consistency from the surrounding feces as to render
comparatively easy the differentiation of the feces of that period from
the feces of the immediately preceding and succeeding periods. One
of the most satisfactory methods of making this "separation" is by
means of the ingestion of a gelatin capsule containing about 0.2 gram of
powdered charcoal at the beginning and end of the period under observa-
tion. This procedure causes the appearance of two black zones of char-
coal in the fecal mass and thus renders comparatively simple the
differentiation of the feces of the intermediate period. Carmine (0.3
gram) may be used in a similar manner and forms two dark red zones.
Some similar method for the "separation of feces" is universally
practised in connection with the scientifically accurate type of nutrition
or metabolism experiment which embraces the collection of useful data
regarding the income and outgo of nitrogen and other elements.

Among the macroscopical constituents of the feces may be men-
tioned the following: Intestinal parasites, undigested food particles,
gall stones, pathological products of the intestinal wall, enteroliths,
intestinal sand, and objects which have been accidentally swallowed.

The fecal constituents which at various times and under different
conditions may be detected by the use of the microscope are as follows :
Constituents derived from the food, such as muscle fibers, connective-
tissue shreds, starch granules, and fat; form elements derived from
the intestinal tract, such as epithelium, erythrocytes, and leucocytes;
mucus; pus corpuscles; parasites and bacteria. In addition to the con-
stituents named the following crystalline deposits may be detected:
cholesterol, ko pro sterol, soaps, fatty acid, fat, hematoidin, '^triple phos-

^ Agar-agar is a product prepared from certain types of Asiatic sea-weed. It is a carbo-
hydrate and is classified as a galaclan in the polysaccharide group.

2 Mendel: Zent.f. ges. Physiol, u. Path, des Stofw., No. 17, p. i, 1908; Schmidt: Miinch.
med. Woch., 52, 1970, 1905.

^ Einhorn: Berl. klin. Woch., 49, 113, 1912.

FECES 225

phate," Charcot-Leyden crystals, and the oxalate, carbonate, phosphate,
sulphate, and lactate of calcium. (See Figs. 64 to 69, pp. 230 and 231.)

The koprosterol of the feces is similar to cholesterol, and may be
formed by the reduction of the latter. It responds to cholesterol color
tests and has the same solubility, but possesses a lower melting-point
and crystallizes in fine needles instead of plates such as cholesterol
forms.

The detection of minute quantities of blood in the feces ("occult
blood") has recently become a recognized aid to a correct diagnosis of
certain disorders. In these instances the hemorrhage is ordinarily so
slight that the identification by means of macroscopical characteristics
as well as the microscopical identification through the detection of ery-
throcytes are both unsatisfactory in their results. Of the tests given
for the detection of "occult blood" the benzidine reaction and the
ortho-tolidin and hematein tests (page 233) are probably the most
satisfactory. Since "occult blood" occurs with considerable regularity
and frequency in gastrointestinal cancer and in gastric and duodenal
ulcer, its detection in the feces is of especial value as
an aid to a correct diagnosis of these disorders. Cer-
tain precautions are essential, such as the establish-
ment of a meat-free diet over a period of time before
the specimen is collected. (Feces from a meat diet
will give an occult blood reaction with some of the

most delicate tests.) Bleeding from the bowel such Fig. 62.— Charcot-
, 1 • 1 11 ^1 1 • . r Leydex Crystals.

as IS seen m hemorrhoids, as well as the admixture of

menstrual blood, is to be considered in the interpretation of the result.

It has been quite clearly shown that the intestine of the newly born
is sterile. However, this condition is quickly altered and bacteria may
be present in the feces before or after the first ingestion of food. There
are three possible means of infecting the intestine, i.e., by way of the
mouth or anus or through the blood. The infection by means of the
blood seldom occurs except under pathological conditions, thus limit-
ing the general infection to the mouth and anus.

In infants with pronounced constipation two-thirds of the dry sub-
stance of the stools has been found to consist of bacteria. In the stools
of normal adults probably about one-third of the dry substance is
bacteria.^ The average excretion of dry bacteria in 24 hours for an
adult is about 8 grams. The output of fecal bacteria has been found
to undergo a decrease under the influence of water drinking with meals. -

' Schittenhelm and Tollens found bacteria to comprise 42 per cent of the dry matter.
This value is, however, undoubtedly too high.

- Mattill and Hawk: Jour. Am. Chan. Soc, 33, 1999, 1911; Blatherwick and Hawk:
Bioch. Bull., 3, 28, 1913.^

2 26 PHYSIOLOGICAL CHEMISTRY

There was also a decrease in intestinal putrefaction/ a fact which
indicates that at least a part of the bacterial deficit was made up of
putrefactive organisms. In some cases over 50 per cent of the total
nitrogen of feces has been shown to be bacterial nitrogen.'^

Various enzymes have been detected in the feces. The first one so
demonstrated was pancreatic amylase.^ The amylase content of the
feces is beheved to be an index of the activity of the pancreatic function.^
The excretion of this enzyme has been found to increase under the
influence of water drinking with meals. ^ Other enzymes which have
been found in the feces under various conditions are tripsin, rennin,
maltase, sucrase, lactase, nuclease and lipase.^ In an abnormally rapid
transit of food through the intestinal tract, such as is seen in certain
diarrheas, nearly all of these enzymes may be detected.

Some of the more important organisms met with in the feces are the
following:'^ B. coli, B. lactis aerogenes, Bad. Welchii, B. bifidus, and
coccal forms. Of these the first three types mentioned are gas-forming
organisms. The production of gas by the fecal flora in dextrose-
bouillon is subject to great variations under pathological conditions;
alterations in the diet of normal persons will also cause wide fluctuations.
Data as to the production of gas are of considerable importance in a
diagnostic way, although the exact cause of the variations is not yet
established. It should be borne in mind in this connection that gas
volumes are frequently variable with the same individual. For this
reason it is necessary in every instance to follow the gas production for
a considerable period of time before drawing conclusions.^ While the
question of the study of bacterial flora of the feces is a question beyond
the range of this work, mention may be made here of the character of
the organisms observed by Gram staining of the stool after administra-
tion of different types of diet. It has been shown that when the diet
is markedly protein, the protein type of flora becomes predominant in
the stools. Gram-stained smears show a fairly equal distribution of
Gram-negative and Gram-positive organisms. Among the latter are
largely the subtiloid organisms with some of the Bad. Welchii, together
with a moderate number of diplococci and coccoid forms. Most of the
Gram-negative organisms resemble the B. coli. When the diet is

1 Hattrem and Hawk: Arch. Int. Med., 7, 610, 191 1; Blatherwick, Sherwin and Hawk:
loc. cit.

^MacNeal, Latzer and Kerr: Jour. Inf. Dis., 6, 123, 1909; Mattill and Hawk: Jour.
Exp. Med., 14, 433, 1911; Blatherwick and Hawk: Biochem. Bull., 3, 28, 1913.

^ Wegscheider: Inaug. Diss., Strassburg, 1875.

* Wohlgemuth: Berl. klin. Woch., 47, 3, 92, 1910.

* Hawk: Arch. Int. Med., 8, 382, 191 1.
^Ury: Biochem. Zeit., 23, 152, 1909.

' Herter and Kendall: Journal of Biological Chemistry, 5, 283, 1908.

* Herter and Kendall: loc. cit.

FECES 227

carbohydrate the field is strongly Gram positive and has a more homo-
geneous appearance. The bacteria seen consist chiefly of long slender
Gram-positive rods belonging to the B. acidophilus and B. bifidus
groups.^

The nitrogen present in the feces consists principally of bacteria,
unahsorbed intestinal secretions, epithelial cells, mucus material and food
residues. In the early days of nutrition study the fecal nitrogen was
believed to consist principally of food residues. We now know that
such residues ordinarily make up but a small part of the nitrogen quota
of the stools of normal individuals who exercise normal mastication.^
When meat has been ''bolted," however, from 3^ gram to 16 grams of
macroscopical meat residues has been found in a single stool. ^ The
phrase ''metabolic product nitrogen" is frequently used as a designa-
tion for all fecal nitrogen except that present as food residues and
bacteria. Bacteria cannot logically be classed under "metaboHc"
nitrogen since they doubtless develop at the expense of food nitrogen
as well as at the expense of that in the form of intestinal secretions.
In the accurate study of "protein utilization"^ a correction should be
made for "metabolic nitrogen." Data regarding the output of meta-
bolic nitrogen may be secured by determining the fecal nitrogen excre-
tion on a diet of proper energy value but containing no nitrogen.^
Agar-agar may be utilized advantageously in connection with such a
nitrogen-free diet.

Feces are still excreted from the intestine even when no food is
ingested. Carefully conducted fasting experiments have demonstrated
this. A dog nourished on an ordinary diet to which bone ash has been
added will excrete a grey feces. WTien fasted such an animal will, after
a few days, excrete a small amount of a greenish-brown mass, containing
no bone ash. These are fasting feces. It is of a pitch-like consistency
and turns black on contact with the air.^ Adult fasting men have been
found to excrete 7-8 grams of feces per day, the daily nitrogen value
being about o.i gram.^ Xo separating medium such as charcoal or
carmine (page 238) should be used in differentiating fasting feces.

In recent years the examination of feces for evidences of parasitism
(detection of parasites and their ova) has taken on an added importance.
The investigation of the hookworm has been particularly developed.

^ Cammidge: The Feces of Children and Adults, 1914, p. 126.

- Kermauner: Zeit. fiir Biol., 35, 316, 1897.

' Foster and Hawk: Jour. Am. Chem. Soc, 37, 1347, 191 5.

* The percentage of the ingested protein which is absorbed from the intestine. This
may be calculated by subtracting the metabolic nitrogen from the total fecal nitrogen and
dividing this value by the food nitrogen.

' Tsuboi: Zeit. jUr Biol., 35, 68, 1897; Mendel and Fine: Jour. Biol. Chem., 11, 5, 191^.

* Howe and Hawk: Jour. Am. Chem. Soc, n, 215, 1911.
^ Howe, Mattill and Hawk: Ibid., 33, 568, 191 1.

'2-28 PHYSIOLOGICAL CHEMISTRY

(For methods and discussion see Bulletin 135, Bureau of Animal Indus-
try, U. S. Department of Agriculture, 191 1, M. C. Hall.)

For diagnostic purposes the macroscopical and microscopical exami-
nations of the feces ordinarily }deld much more satisfactory data than
are secured from its chemical examination. Possibly with the excep-
tion of certain examinations for occult blood, the most satisfactory data
for diagnostic purposes are secured by microscopical examination.
This presupposes a knowledge of microscopical technic and the use of
certain microchemical tests, by which much information can be ob-
tained. The principle underhdng this examination consists in the study
of the actual changes which the various food-stuffs have undergone dur-
ing digestion. A knowledge of the changes which occur in normal diges-
tion and which are seen in normal feces enables one to readily detect
pathological variations. One diet widely used for this purpose is the
Schmidt diet which is given below. The modification^ described is
better adapted to American conditions.

The Schmidt intestinal diet is as follows:

In the morning: 0.5 Hter of milk, or if milk does not agree 0.5 liter
of cocoa (prepared from 20 grams of cocoa powder, 10 grams sugar,
400 grams water, and 100 grams milk). To this add 50 grams zwiebach.

In the forenoon: 0.5 Hter oatmeal gruel (made from 40 grams oat-
meal), 10 grams butter, 100 grams milk, 300 grams water, i egg strained.

At noon: 125 grams of chopped beef (raw weight) broiled rare with
20 grams of butter, so that the interior will remain raw. To this add
250 grams potato broth (made of 190 grams mashed potatoes, 100 grams
milk, 10 grams of butter).

In the afternoon: as in the morning.

In the eventing: as in the forenoon.

This diet necessitates five meals a day especially prepared and does
not follow the average American dietary. In simple microscopical
examinations for food digestion, the following diet as more closely
approximating the ordinary dietary regime is suggested. Should
chemical determinations for fat be desired all fat containing foods can
be ehminated except those in which its specific content is known and a
measured amount of fat given. The feces can then be separated by
means of carmine.

Modified Schmidt Diet
Breakfast:

100 grams Cream of wheat or oatmeal
60 grams toast
20 grams butter
250 c.c. milk.

1 Used by Dr. Rehfuss at Jefferson Hospital.

TECES

229

Luncheon:

Rice soup (chicken broth with rice)
100 grams green vegetable (asparagus)
100 grams mashed potato
60 grams toast
20 grams butter
250 c.c. milk.

4 o'clock:

250 c.c. of milk.

Dinner:

150 grams of chopped meat, grilled on the outside and rare in the center
100 grams green vegetable (spinach)
100 grams mashed potatoes

60 grams of toast

20 grams of butter
250 c.c. milk
Stewed fruit.

Experiments on Feces

I. Macroscopical Examination. — If the stool is watery pour it into a shallow
dish and examine directly. If it is firm or pasty it should be treated with water
and carefully stirred before the examination for macroscopical constituents is
attempted. The macroscopical constituents may be collected very satisfactorily
by means of a double layer of cheese cloth.

A Boas sieve (Fig. 63) may also be used to collect the macroscopical
constituents of feces. This sieve is constructed of two easily detachable
hemispheres which are held together by means of a
bayonet catch. In using the apparatus the feces is
spread out upon a very fine sieve contained in the
lower hemisphere and a stream of water is allowed to
play upon it through the medium of an opening in
the upper hemisphere. The apparatus is provided
with an orifice in the upper hemisphere through
w^hich the feces may be -stirred by means of a glass
rod during the washing process. After 1 5-30 minutes
washing nothing but the coarse fecal constituents
remain upon the sieve.

Fig. 63. — Bo.\s

SiF.VF.

2. Microscopical Examination. — After the ingestion of
the test diet (see Schmidt diet above) for several days, a
specimen of the movement is collected. Any gross abnor-
malities are recorded in the form, consistence, and char-
acter of the stool as well as the admixture of certain pathological elements
such as pus, blood, mucus, and parasites. The movement is then rubbed out
on plates and the presence of undigested food-stuffs sought for. Normally the
test diet is almost completely digested and no gross undigested material is
found. Therefore the presence of these macroscopic rests is in itself evidence
of disturbed digestion. Clean slides and cover-glasses are then prepared
and a small representative portion of the movement is placed on each of three
slides. The routine clinical method of examination follows : To the first slide

230 PHYSIOLOGICAL CHEMISTRY

is added a drop of distilled water and it is then examined with low and high
powers.

Meat fibers are readily recognized by their yellowish hyaline ap-
pearance possibly with a few striee still visible in the libers. Should

Fig. 64. — .4, intact undigested meat Fig. 65. — A, neutral fat; B, iatty acid

fibers; B, partially digested meat fibers; liberated by acetic acid; C, soaps; D, fatty

C, almost completely digested meat acid crystals,
fibers.

Fig. 66. — A, elastic tissue; B, white Fig. 67. — .4 , cellulose remains of vege-

fibrous tissue (macroscopic); C, white tables; B, empty potato cells; C, potato

fibrous tissue (microscopic.) cells filled with starch, and stained with

iodine; D. hard cells found in pears; E, spiral
and woody fibers from pith of vegetables;
F, vegetable hairs.

Figs. 64 to 67. — ^Iicroscopic.a.l Constituents of Feces.
meat fibers be found bound together by connective tissue or raw
connective tissue, either white fibrous or yellow elastic, be noted, it
indicates a disturbance of gastric function inasmuch as one of the spe-
cific functions of the gastric juice is to dissolve the intercellular tissue

FECES

231

binding together the fibers. If large numbers of meat fibers are found
after a test diet, particularly if the nuclei are still intact in the fibers,
the inference of poor or low pancreatic function is justifiable. This
is true if it can be demonstrated that the food has been sufficiently
long in its transit through the intestinal tract to permit the pancreatic
enzymes to carry on their work. A dilute solution of methylene blue
will readily show the nuclei if present.

The second slide is examined for fats and then treated with acetic
acid and heated to split any soaps which may be present and form
fatty acid.

Fats are met with in three forms (a) neutral fats readily demonstrated by
Sudan III, Scharlach R or Osmic acid; (b) fatty acids which are usually found in
the form of needle-like crystals soluble in ether, alcohol, and solutions of sodium

Fig. 69. — A, Schmidt test bag for study
of pancreatic function; B, nuclei of meat
fibers digested; C, nuclei of meat fibers
undigested; D, undigested stained thymus
cells.
Figs. 68 and 69.— Microscopical Coxstituents of Feces.

Fig. 68. — .4, calcium sulphate crys-
tals; B, cholesterol crystals; C, char-
coal detritus; D, bismuth sub-oxide
crystals; E, calcum oxalate crystals.

hydrate (these crystals do not stain with Sudan III but form drops on being
warmed) ; (c) soaps are usually found in the feces either as amorphous flakes or
scallop shell-like formations, but may occasionally occur in crystalline form.
The calciiun soaps which compose the bulk of the soaps in the feces can be dis-
tinguished from the potassium and sodiimi compounds because of their insolu-
bility in hot water, alcohol, and ether. On heating with 30 per cent acetic acid,
fatty acids are set free in drops which crystaUize out on cooling.

The estimation of fats is a rather important matter and the trained
observer can usually detect disturbances in fat digestion. Normally
there are fats present in the movement, but abnormally their c}uantity
is relatively increased either in total fat, or in one of its components.

232 PHYSIOLOGICAL CHEMISTRY

While it is true that bacterial activity plays a considerable role in the
digestion of fats, a marked increase in fat usually indicates pancreatic
disease, or a disturbance in pancreatic function. This is, of course, the
case only when the amount of fat ingested is not in excess of that which
can be readily handled under normal conditions. In cases of pure
biliary obstruction without pancreatic involvement, fat-splitting takes
place in a normal way, but the fatty acids and soaps formed are not
absorbed owing to the absence of bile. Such a movement is full of
soaps and fatty acid crystals which on treatment with acetic acid show
a marked increase in total fat over normal. Failure of absorption
owing to extensive disease of the intestinal mucosa can produce a similar
picture but will usually give some cytological evidence of intestinal
disease. Pure pancreatic disease gives a marked increase in total and
neutral fat with the presence of bile.

Undigested starches are readily recognized by their blue reaction with iodine.
This can be studied on the third sUde.

This phenomenon is the least frequent among the different forms of
pathological digestion and usually indicates food bolting, an excessive
ingestion of, or poor preparation of carbohydrate food, or an infection
of the bowel with so-called "garungsdyspepsia" rather than an actual
disturbance of pancreatic function inasmuch as theamylolytic function
of the pancreas is the most persistent and the last to disappear.

Disturbance in cellulose digestion, the presence of blood, leucocytes,
mucus, etc. , can all be demonstrated by appropriate technic and represent
a chapter in the study of the feces ofgreat diagnostic importance, but one
which is beyond the province of this volume. (For further discussion,
see page 228. For cuts of fecal constituents found microscopically,
see pages 230 and 231.)

3. Reaction. — ^Thoroughly mix the feces and apply moist red and blue litmus
papers to the surface. If the stool is hard it should be mixed with water before
the reaction is taken. Examine the stool as soon after defecation as is convenient,
since the reaction may change very rapidly. The reaction of the normal stools of
adult man is ordinarily neutral or faintly alkaline to litmus, but seldom acid.
Infants' stools are generally acid in reaction. Try the reaction to Congo red
paper. Also test the reaction of fecal extract to phenolphthalein.

4. Starch. — If any imperfectly cooked starch-containing food has been
ingested it will be possible to detect starch granules by a microscopical examina-
tion of the feces. If the granules are not detected by a microscopical examination,
the feces should be placed in an evaporating dish or casserole and boiled with
water for a few minutes. Filter and test the filtrate by the iodine test in the usual
way (see page 45).

5. Cholesterol, Koprosterol and Fat. — Introduce about 5 grams of moist
feces into a 100 c.c. glass-stoppered cylinder. Add 30 c.c. of distilled water and

FECES 233

25 c.c. of ether, then stopper the cylinder and shake vigorously for five minutes.
Allow to separate, pour or pipette ofif the ethereal solution. FUter and remove the
ether by evaporation. The residue contains cholesterol and the mixed fats of
the feces. For every gram of fat add about i 12 grams of soUd potassium hy-
droxide and 25 c.c. of 95 per cent alcohol and boil in a flask on a water-bath for
one-half hour, maintaining the volume of alcohol constant. This alcohohc-
potash has saponified the mixed fats and we now have a mixture of soaps,
cholesterol and koprosterol. Add sodium chloride, in substance, to the mixture
and extract with ether to dissolve out the cholesterol and koprosterol. Remove
the ether by evaporation and examine the residue microscopically for cholesterol
and koprosterol crystals. Try any of the other tests for cholesterol as given on
page 210.

6. Blood. — Undecomposed blood may be detected macroscopically.
If uncertain, look for erythrocytes under the microscope, and spectro-
scopically for the spectrum of oxyhemoglobin (see Absorption Spectra,
Plate 1).

In case the blood has been altered or is present in minute amount
("occult blood"), and cannot be detected by the means just mentioned,
the following tests may be tried:

(a) Benzidine Reaction. — Make a thin fecal suspension using about 5 c.c. of
distilled water, and heat it to boiUng to render oxidizing enzymes inactive.
To 2 c.c. of a saturated solution of benzidine in glacial acetic acid add 3 c.c. of
3 per cent hydrogen peroxide and 2-3 drops of the cooled fecal suspension.
A clear blue color appears within one to two minutes in the presence of blood.
If the mixture is not shaken a ring of color will form at the top. Minute traces of
blood are more easily detected by the latter procedure.

Wagner^ has simplified the benzidin test so that it can be applied
much more conveniently.

Slide Modification. — Take up a little of the solid stool on a match, smear it
on an object glass and pour the reagent over it. It turns blue if there is blood
present and there is no misleading green tint from fluid. Make the solution
as follows: Add a knife-tip of benzidine to 2 c.c. of glacial acetic acid, and
add 20 drops of a 3 per cent solution of hydrogen peroxide.

By this dry technic there is no danger of soiling the fingers, and the
test is more sensitive than the usual "wet" benzidine test. , The smear
of stool is either blue or it is not blue. The rapidity of the color change
gives some idea as to the proportion of blood in the stool ; with much
blood present the change to blue is instantaneous.

(b) Ortho-tolidin Test (Ruttan and Hardisty)^ — To i c.c. of a 4 per cent

^Wagner: Zeulbl. fiir Chirurgie, 41, No. 28, 1914.

2 Ruttan and Hardisty: Canadian Medical Ass'n Journal, Nov., 1912, also Biochemical
Bull., 2, 225, 1913.

234 PHYSIOLOGICAL CHEMISTRY

glacial acetic acid solution of o-tolidin^ in a test-tube add i c.c. of the solution
under examination and i c.c. of 3 per cent hydrogen peroxide. In the presence
of blood a bluish color develops (sometimes rather slowly) and persists for
some time (several hours in some instances).

This test is said to be as sensitive for the detection of occult blood in
feces and stomach contents as is the benzidine reaction. It is also
claimed to be more satisfactory for urine than any other blood test.
The acetic acid solution may be kept for one month with no reduction
in delicacy.

(c) Phenol phthalein Test^ — Make a thin fecal suspension using about 5 c.c. of
distilled water. Heat to boiling,^ cool and add 2 c.c. of the suspension to i c.c. of
the phenolphthalein reagent^ and a few drops of hydrogen peroxide. A pink or
red color promptly forms in the presence of blood.

Schirokauer* makes the statement that a mixture of alcohol and glacial acetic
acid will give the phenolphthalein reaction for occult blood. The action of an oxi-
dizing agent will make this reaction more distinct. Von Czylharz and Neustadl®
find that a solution of sodium salicylate added to a blood-free extract of feces will
give a very deceptive reaction, while feces after the administration of sodium
salicylate by mouth gave the same reaction. The same was true of acetyl salicylic
acid and other similar drugs. Their studies in clinical cases likewise indicated that
the phenolphthalein test was unreliable.

{d) Hematein Reaction for Occult Blood. — Couturier" advises the use of
hematein^ in testing for occult blood. It is only slightly soluble in water,
but gives a pronounced red color. In contact with sodium hydroxide
this red solution turns a deep violet blue, giving an insoluble compound
of hematein and sodium. This compound, exposed to the air oxidizes
after several days, and gives brownish or yellowish compounds, depend-
ing on dilution. This change is only hastened a little by the addition
of hydrogen peroxide, but if a trace of blood is added to the hydrogen
peroxide, it takes place almost instantly. To avoid oxidation, the hem-
atein sodium mixture should be prepared just before use. Three fluids

1 NH2 NH2

/C6H4 — V-^6H4y^
CH3 CH3

* Boas: Deul. med. Woch., 37, 62, 1911.

' Boas suggests using an ether extract of the fecal suspension thus eliminating the
necessity of boiling. However, oxidizing enzymes are the main sources of error here and the
action is easily and effectively eliminated by boiling. (See White: Boston Medical and
Surgical Journal, 164, 876, 191 1.)

* Prepared by dissolving 1-2 grams of phenolphthalein and 25 grams of KOH in 100 c.c.
of distilled water. Add 10 grams of powdered zinc and heat gently until the solution is
decolorized. Prepared in this way the solution will not deteriorate on standing.

* Deiitsch. med. Woch., Aug. 6, 1914.
' Wien. med. Woch., Sept. 5, 1914.
''Lyon Med., 46, 313, 1914.

* Hematein is a brownish-red crystalline substance derived from hematoxylin by the
successive action of ammonia and acetic acid. It should not be confused with hematin,
the hemoglobin derivative.

FECES 235

are required: (i) a 0.05 per cent aqueous solution of hematein; (2) a
40 per cent solution of sodium hydroxide and (3) 3 per cent hydrogen
peroxide. These will keep almost indefinitely.

The test may be performed as follows : Take 4-5 c.c. of the liquid specimen in a
tube and in another tube take the same amount of material known not to contain
blood as a control. To each add 4-5 c.c. of the sodium hydroxide solution and
shake. Then to each of the tubes add 2 drops of the hematein solution. A blue
color of about equal intensity will develop in both tubes. Then add 10 drops of
hydrogen peroxide to each tube and compare. If blood is present, the tube con-
taining it will turn very rapidly (in three or four seconds; to violet red, then in
twenty seconds to clear brown, in forty seconds to pale yellow while the second
tube will not show these changes for several minutes. The reaction is said to
detect blood when present in a concentration of i part in 400,000.

(e) Aloin-turpenlive Test. — Mix the stool very thoroughly and take about
5 grams of the mixture for the test. Reduce this sample to a semi-fluid mass by
means of distUled water and extract very thoroughly with an equal volimie of ether
to remove any fat which may be present. Now treat the extracted feces with one-
third its volume of glacial acetic acid and 10 c.c. of ether and extract ver>' thoroughly
as before. The acid-ether extract wUl rise to the top and may be removed.

Introduce 2-3 c.c. of this acid-ether solution into a test-tube, add an equal
volume of a dilute solution of aloin in 70 per cent alcohol and 2-3 c.c. of ozonized
turpentine and shake the tube gently. If blood is present the entire volume of fluid
ordinarily becomes pink and finally cherry red. In some instances the color wiU
be limited to the aloin solution which sinks to the bottom. This color reaction
should occur within 15 minutes in order to indicate a positive test for blood, since
the aloin will turn red of itself if allowed to stand for a longer period. The color is
ordinarily light yellow in a negative test. Hydrogen peroxide is not a satisfactor>-
substitute for turpentine in the test.

(f j Cowie's Guaiac Test. — To i gram of moist feces add 4-5 c.c. of glacial
acetic acid and extract the mixture with 30 c.c. of ether. To 1-2 c.c. of the extract
add an equal volume of water, agitate the mixture, introduce a few granules of
powdered guaiac resin, and after bringing the resin into solution, gradually add
30 drops of old turpentine or hydrogen peroxide. A blue color indicates the
presence of blood. Cowie claims that by means of this test an intestinal hemor-
rhage of I gram can easily be detected by an examination of the feces.

(g) Weber's Guaiac Test. — Mix a little feces with 30 per cent acetic acid to form
a fluid mass. Transfer to a test-tube and extract with ether. If blood is present
the ether will assume a brownish-red color. Filter off the ether extract and to a
portion of the filtrate add an alcoholic solution of guaiac (strength about 1:60),'
drop by drop, until the fluid becomes turbid. Now add hydrogen peroxide or old
turpentine. In the presence of blood a blue color is produced (see page 2 58).

(A) Acid-hematin. — Examine some of the ethereal extract from Experiment (g)
spectroscopically. Note the typical spectrum of acid-hematin (see Absorption
Spectra. Plate II).

7. HydrobiUrubin. Schmidt's Test. Rub up a small amount of feces in a
mortar with a concentrated aqueous solution of mercuric chloride. Transfer to a

^ Buckmaster advises the use of an alcoholic solution of guaiaconic acid instead of an
alcoholic solution of guaiac resin.

236 PHYSIOLOGICAL CHEMISTRY

shallow, flat-bottomed dish and allow to stand 6-24 hours. The presence of
hydrobilirubin will be indicated by a deep red color being imparted to the par-
ticles of feces containing this pigment. This red color is due to the formation
of hydrobihrubin-mercury. If unaltered bihrubin is present in any portion of
the feces that portion will be green in color due to the oxidation of biUrubin to
biUverdin.

Another method for the detection of hydrobilirubin is the following: Treat
the dry feces with absolute alcohol acidified with sulphuric acid and shake
thoroughly. The acidified alcohol extracts the pigment and assumes a reddish
color. Examine a little of this fluid spectroscopically and note the typical
spectrum of hydrobilirubin (Absorption Spectra, Plate II).

8. BiUrubin. 1 (a) Gmelin's Test. — Place a few drops of concentrated
nitric acid in an evaporating dish or on a porcelain test-tablet and allow a few
drops of the feces and water to mix with it. The usual play of colors of Gmelin's
test is produced, i.e., green, blue, violet, red, and yellow. If so desired, this
test may be executed on a slide and observed under a microscope.

(b) Htippert's Test. — Treat the feces with water to form a semi-fluid mass, add
an equal amount of milk of lime, shake thoroughly, and filter. Wash the precipi-
tate with water, then transfer both the paper and the precipitate to a small beaker
or flask, add a small amount of 95 per cent alcohol acidified slightly with sulphuric
acid, and heat to boiling on a water-bath. The presence of bilirubin is indicated
by the alcohol assuming a green color.

Steensma advises the addition of a drop of a 0.5 per cent solution of sodium
nitrite to the acid-alcohol mixture before warming on the water-bath. Try this
modification also.

9. Bile Acids. — Extract a small amount of feces with alcohol and filter.
Evaporate the filtrate on a water-bath to drive off the alcohol and dissolve the
residue in water made sUghtly alkaline with potassixim hydroxide. Upon this
aqueous solution try any of the tests for bile acids given on page 208.

10. Casein. — Extract the fresh feces first with a dilute solution of sodium
chloride, and later with water acidified with dilute acetic acid, to remove soluble
proteins. Now extract the feces with 0.5 per cent sodium carbonate and filter.
Add dilute acetic acid to the filtrate to precipitate the casein, being careful
not to add an excess of the reagent as the casein would dissolve. Filter off the
casein and test it according to directions given on page 321. Casein is found
principally in the feces of children who have been fed a milk diet. Mucin would
also be extracted by the dilute alkali, if present in the feces. What test could
you make on the newly precipitated body to differentiate between mucin and
casein?

11. Nucleoprotein. — Mix the stool thoroughly with water, transfer to a flask,
and add an equal amount of saturated lime water. Shake frequently for a few
hours, filter, and precipitate the nucleoprotein with acetic acid. Filter off this
precipitate and test it as follows:

(o) Phosphorus. — Test for phosphorus by fusion (see page 129).
(ft) Solubility. — Try the solubility in the ordinary solvents.

(c) Protein Color Test. — Try any of the protein color tests.

^ The detection of bilirubin in the feces is comparatively simple provided it is not ac-
companied by other pigments. When other pigments are present, however, it is difficult to
detect the bilirubin and, at times, may be found impossible.

FECES 237

What proof have you that the above body was not mucin? What other test
can you use to differentiate between nucleoprotein and mucin?

12. Albumin and Globulin. — Extract the fresh feces with a dilute solution of
sodium chloride. (The preliminary extract from the preparation of casein (10),
above, may be utilized here.) Filter, and saturate a portion of the filtrate with
sodium chloride in substance. A precipitate signifies globulin. Filter off the pre-
cipitate and acidify the filtrate slightly with dilute acetic acid. A precipitate at
this point signifies albumin. Make a protein color test on each of these bodies.

13. Proteose and Peptone, — Heat to boiling the portion of the sodium chloride
extract not used in the last experiment. Filter oflf the coagulum, if any forms.
Acidify the filtrate slightly with acetic acid and saturate with sodium chloride in
substance. A precipitate here indicates proteose. Filter it ofif and test it according
to directions given on page 120. Test the filtrate for peptone by the biuret test.

14. Inorganic Constituents. — Incinerate a smaU amount of feces in a crucible
and dissolve the ash in a small volume of dilute nitric acid. Dilute with water and
filter. Make the following tests upon the clear filtrate.

(c) Chlorides. — Acidify with nitric acid and add silver nitrate.

{h) Phosphates. — Acidify with nitric acid, add molybdic solution, and warm
gently.

(c) Sulphates. — Acidify with hydrochloric acid, add barium chloride, and warm.

{d) Calcium. — Neutralize with ammonium hydroxide, make slightly acid with
acetic acid and add ammonium oxalate. Let stand.

(e) Magnesium. — Neutralize with ammonium hydroxide, and add Na2HP04
and excess of NH4OH. Let stand.

15. Indole Reactions. — Rub up the stool with water to form a thin paste
and distill first in alkaline and then in acid solution. Test the distillate by
any of the tests for the detection of indole in putrefaction mixtures (see
page 218).

16. Schmidt's Nuclei Test. — This test serves as an aid to the diag-
nosis of pancreatic insufficiency. The test is founded upon the theory
that cell nuclei are digestible only in pancreatic juice, and therefore
that the appearance in the feces of such nuclei indicates insufficiency of
pancreatic secretion.

The procedure is as follows: Cubes of fresh beef about 12 cm. square are
enclosed in small gauze bags and ingested with a test meal. Subsequently
the fecal mass resulting from this test meal is examined, the bag opened, and
the condition of the enclosed residue determined. Under normal conditions the
nuclei would be digested. Therefore if the nuclei are found to be for the most
part undigested, and the intervening period has been sufficient to permit of the
full activity of the pancreatic function (at least six hours), it may be considered a
sign of pancreatic insufficiency (see Fig. 69, p. 231).

It has been claimed by Steele that under certain conditions the non-
digestion of the nuclei may indicate a general lowering of the digestive
power rather than a true pancreatic insufficiency.

Kashiwado^ has suggested the use of stained cell nuclei in this test.
A preparation put out under the name "Gefarbte gewebskerne zur

^ Kashiwado: Deut. Arch. Klin. Med., 104, 584, 191 1.

238

PHYSIOLOGICAL CHEMISTRY

Pankreasfuntionspriifung nach Prof. Dr. Schmidt und Dr. Kashiwado"
consists of a mixed preparation of thymus cells, the nuclei of which
are stained by iron hematoxylin, and lycopodium powder. After
administration, the lycopodium, which is readily recognized, is sought
for in the stool and when found that portion is examined for the stained
thymus cells. Their statement is as follows: If stained nuclei are
not found in the feces after an intestinal transit of sufficient duration
(at least six hours) normal pancreatic function (external) is' indicated.
If, however, all or part of the cells are found, a definite disturbance in
pancreatic function is present.

17. Influence of Drugs upon the Color of the Stool. — Ingest an ordinary
mixed diet, take the indicated dose of one of the following drugs, "separate"
the feces (see page 587) and after the "marker" appears note the color of the
stools evacuated :

Drug

Dose

Color of stool

1 Bismuth subnit'rate, grams

5

Black.

Calomel, mg

130-140

Green.

Reduced iron, mg

65-70 Grayish black turning darker on exposure to air.

1
Methylene blue, mg 130-140, Blue, especially after exposure to air.

Manganese dioxide, mg. . . .

130-1401 Dark brown or black.

Hematoxylin, grams

I

Reddish brown.

Rhubarb, c.c. fluid extract..

1

2 ' Yellow.

Senna, c.c. fluid extract. . .

4 Dark yellow.

Cambogia, mg

130-140 Dark yellow.

Santonin, mg

6';-70 Dark vellow.

1

18. Einhom's Bead Test.* — ^This is a method for testing the digestive func-
tion. In some respects it is similar to SahU's desmoid reaction (see Gastric
Analysis). The procedure consists in wrapping the material under examination
(catgut, fish-bone, raw beef, cooked potatoes, thjrmus gland or mutton fat, etc.)
in gauze to which glass beads of various colors are attached and enclosing gauze
and beads in a gelatine capsule.^ The gelatine capsule is swallowed and the
beads serve to faciUtate the separation of the gauze from the feces. The residue

^ Einhorn: The Post-Graduale, May, 191 2: Boas^ Arch., 12, 26, 1906; 13, 35, 1907; Ibid.,
47S; IS, part 2, 1909.

^ Ordinarily two substances are attached to each bead, three beads tied together and
enclosed in one capsule. Test capsules may be obtained from Eimer and Amend, New York.

FECES 239

within the gauze is then examined. If beads appear in much less than 24 hours
an accelerated motility is indicated, whereas an interval of 48 hours or over
elapsing indicates retarded motihty. If gastric function alone is to be studied
silk threads are attached to the beads and the latter are withdrawn and examined
before they have passed into the intestine.

19. "Separation" of Feces. — In order to become famiUar with the method
ordinarily utihzed in metaboUsm experiments to differentiate the feces which
correspond to the food ingested during any given interval, and at the same time
to secure data as to the length of time necessary for ingested substances to pass
through the alimentary tract proceed as follows: Just before one of the three
meals of the day ingest a gelatine capsule (No. 00) containing 0.2 0.3 of a gram
of carmine or charcoal. Make an Inspection of all stools subsequently dropped
and note the time interval elapsing between the ingestion of the capsule and the
appearance of its contents in the feces. Under normal conditions this period is
ordinarily 24 hours. This test is thus an index of intestinal motiUty.

20. Influence of Foods upon the Color of the Stool. — Ingest a diet which
contains a Uberal quantity of one of the following articles of diet, "separate" the
feces (page 587) and after the "marker" appears note the color of the stools
evacuated :

Article of diet

Color of stool

Milk.

Light yellow or grayish white.

Meat

Brownish black.

Chlorophyllic vegetables, e.g., spinach —

Greenish. |

Non-rhlorophyllic vegetables

Light brown.

Cherries or blackberries

Reddish brown.

Cocoa

Dark red or chocolate brown.

Coffee

Dark brown.

Corn meal

Light colored.

21. Quantitative Determination of Fecal Amylase (The Author's^ Modification
of Wohlgemuth's- Method). — Weigh accurately about 2 grams of fresh feces into
a mortar,' add 8 c.c. of a phosphate-chloride solution (o.i mol dihydrogen sodium
phosphate and 0.2 mol disodium hydrogen phosphate per liter of i per cent sodium
chloride), 2 c.c. at a time, rubbing the feces mixture to a homogeneous consistency
after each addition of the extraction medium. Permit the mixture to stand at
room temperature for a half-hour with frequent stirring. We now have a neutral
fecal suspension. Transfer this suspension to a 15 c.c. graduated centrifuge lube,
being sure to wash the mortar and pestle carefully with the phosphate-chloride
solution and add all washings to the suspension in the centrifuge tube. The sus-
pension is now made up to the 15 c.c. mark with the phosphate-chloride solution

1 Hawk: Arch. Int. Med., 8, 552, 191 1.

^ Wohlgemuth: Bcrl. klin. Wocli., 47, 3, 92, 1910; also see page 192, this book.

' Duplicate determinations should be made.

240 PHYSIOLOGICAL CHEMISTRY

and centrifugated for a 15-niinute period, or longer if necessary, to secure satis-
factory' sedimentation. At this point, read and record the height of the sediment
column. Remove the supernatant liquid by means of a bent pipette, transfer it to
a 50 CO. volumetric flask and dilute it to the 50 c.c. mark with the phosphate-
chloride solution. Mix the fecal extract thoroughly by shaking and determine its
amylolytic activity. For this purpose a series of six graduated tubes is prepared,
containing volumes of the extract ranging from 2.5 c.c. to 0.078 c.c. Each of the
intermediate tubes in this series will thus contain one-half as much fluid as the
preceding tube. Now make the contents of each tube 2.5 c.c. by means of the
phosphate-chloride solution in order to secure a uniform electrolyte concentration.
Introduce 5 c.c. of a i per cent soluble starch solution^ and three drops of toluol
into each tube, thoroughly mix the contents by shaking, close the tubes by means
of stoppers and place them in an incubator at 38°C. for 24 hours. At the end of
this time remove the tubes, fill each to within half an inch of the top with ice-water,
add I drop of tenth-normal iodin solution, thoroughly mix the contents and examine
the tubes carefully with the aid of a strong light. Select the last tube in the series
which shows entire absence of blue color, thus indicating that the starch has been
completely transformed into dextrin and sugar, and calculate the amylolytic activity
on the basis of this dilution. In case of indecision between two tubes, add an extra
drop of the iodin solution and observe them again.^

The amylolytic value, Df, of a given stool, may be expressed in terms of i c.c.
of the sediment obtained by centrifugation as above described. For example, if it
is found that 0.31 c.c. of the phosphate-chloride extract of the stool acting at 38°C.
for 24 hours completely transformed the starch in 5 c.c. of a i per cent starch solu-
tion, then we would have the following proportion:

0.31 :5 (c.c. starch) :: i(c.c. extract) :X

The value of X in this case is 16. i, which means that i c.c. of the fecal extract
possesses the power of completely digesting 16. i c.c. of a i per cent starch solution
in 24 hours at 38°C.

Inasmuch as stools vary so greatly as to water content, it is essential to an
accurate comparison of stools that such comparison be made on the basis of the
solid matter. Supposing, for example, that in the above determination we had
6.2 c.c. of sediment. Since the supernatant fluid was removed and made up to

1 In preparing the i per cent solution, the weighed starch powder should. be dissolved
in cold distUled water in a casserole and stirred untU a homogeneous suspension is obtained.
The mixture should then be heated with constant stirring, unril it is clear. This ordinarily
takes from eight to ten minutes. A slightly opaque solution is thus obtained, which
should be cooled and made up to the proper volume before using.

2 Theoretically we would expect the colors to range from a light yellow to a dark blue,
with red tubes holding an intermediate position in the series. This color sequence does
often occur, but its occurrence is far from universal. Many times the first tubes in the series,
i.e., those containing the largest quantities of the fecal extract, will exhibit a bluish cast of
color which should not be confused with the starch color reaction. When these blue tubes
are present, they are generally followed by yellow, red and blue tubes in order, the final blue
tube, of course, being the regulation starch reaction. Occasionally greenish colors will be
obtained to the left of the red color. It also sometimes happens that it is somewhat dif-
ficult to determine in which tube to the right of the red color the starch blue color is first de-
tected, unless the tube be examined carefully before a strong light. In every instance, how-
ever, \yhen these blue and green colors are observed, it is noted that tubes possessing the
true dextrin red color are always present between these tubes and the tubes possessing the
true starch blue color. It is evident, therefore, that these bluish tints in the tubes to the
left of the dextrin color cannot be due to the presence of starch. The cause of the blue color
reaction in the first tubes of the series has not been ascertained as yet.

PECES 241

50 c.c. before testing its amylolytic value, it is evident that i c.c. of this sediment is
equivalent to 8.1 c.c. of extract. Therefore, in order to derive the amylolytic
value of I c.c. of sediment, we must multiply the value (16. i) as obtained above
for the extract, by 8.1. This yields 130.4 and enables us to express the activity
as follows:

Dl24h = 130-4

The above method of calculation is that suggested by Wohlgemuth. In case time
and facilities permit cf the determination of the moisture content of the feces, it is
much more accurate and satisfactory to place the amylolytic values of the stools
on a "gram of dry matter" basis. The amylolytic values of the stools are expressed
as the number of cubic centimeters of i per cent starch solution which the amylase
content of i gram of dry feces is capable of digesting.

22. Quantitative Determination of Fecal Bacteria.^ — The method is a simpli-
fication of MacXeal's adaptation of the Strasburger procedure. ^ About 2 grams of
feces are accurately weighed and placed in a 50 c.c. centrifuge tube. To the feces
in the tube a few drops of 0.2 per cent hydrochloric acid are added, and the material
is mixed to a smooth paste by means of a glass rod. Further amounts of the acid
are added with continued crushing and stirring until the material is thoroughly
suspended. The tube is then whirled in the centrifuge at high speed for one-half
to one minute. The suspension is found sedimented into more or less definite
layers, the uppermost of which is fairly free from the larger particles. The upper
and more liquid portion of the suspension is now drawn off by means of a pipette
and transferred to a beaker.^ The sediment remaining in the tube is again rubbed
up with the glass rod with the addition of further amounts of dilute acid, and again
centrifugalized for one-half to one minute. The supernatant liquid is pipetted off
and added to the first, the same pipette being used for the one determination through-
out.'* A third portion of the dilute acid is then added to the sediment, which is
again mixed by stirring and again centrifugalized. All the washings are added to
the first one, and during the process care is taken to wash the material from the
walls and mouth of the centrifuge tube down into it. Finally, when the sediment
is sufficiently free from bacteria, the various remaining particles are visibly clean,
and the supernatant liquid after centrifugalization remains almost clear. This is
removed to the beaker in which are now practically all the bacteria present in the
original portion of feces, together with some solid matter not yet separated. In the
centrifuge tubes there is a considerable amount of bacferia-free solid matter.

The suspension is now transferred to the same centrifuge tube, centrifugalized
for a minute, and the supernatant liquid transferred to a clean beaker by means of
the same pipette. The tube is then refilled from the first beaker and thus all the
suspension centrifugalized a second time. The beaker is finally carefully washed
with the aid of a rubber-tipped glass rod, the second sediment in the centrifuge
tube is washed free of bacteria by means of this wash water and by successive por-
tions of the dilute acid, and the supernatant liquid after centrifugalization is added
to the contents of the second beaker. The second clean sediment is added to the

^ Mattill and Hawk: Jour. Exp. Med., 14, 433, 191 1.

^ MacNeal, Latzer and Kerr, Joiir. Inf. Dis., 6, 123, 1909.

' A 25 c.c. pipette is the most satisfactory size; to facilitate observation, the delivery tube
is bent near the bulb to an angle of about 120 degrees.

^ A convenient support for the pipettes is a wire spring on a glass base, such as is used on
a desk for pen-holders. The delivery tube, just where it is bent, is inserted between the
wires, and any hquid not delivered collects in the bend of the tube.
16

242 PHYSIOLOGICAL CHEMISTRY

first. The bacterial suspension now in the second beaker is again centrifugalized
in the same way and a third portion of bacteria-free sediment is separated. Fre-
quently a fourth serial centrifugalization is performed — always if the third sediment
is of appreciable quantity. At all stages of the separation, small portions of the
dilute hydrochloric acid are used, so that the final suspension shall not be too vo-
luminous. Ordinarily it amounts to 125 to 200 c.c. At the same time, the final
amount of fluid should not be too small, as shown by Ehrenpfordt,^ because the
viscosity accompanying increased concentration prevents proper and complete
sedimentation.

To the final bacterial suspension an equal volume of alcohol is added and the
beaker set aside to concentrate. A water-bath at 50° to 6o°C. is very satisfactory.
After two or three days, when the liquid is concentrated to about 50 c.c, the beaker
is removed and about 200 c.c. of alcohol are added. The beaker is covered and
allowed to stand at room temperature for 24 hours. At the end of this time the
bacterial substance is generally settled, so that most of the clear supernatant liquid,
of dark brown color, can be directly siphoned off without loss of solid matter. The
remainder is then transferred to centrifuge tubes, centrifugalized, and the remaining
clear liquid pipetted off." The sediment consists of the bodies of the bacteria, and
is transferred to a Kjeldahl flask for nitrogen determination. This is the bacterial
nitrogen. Where a determination of bacterial dry substance is desired, the sedi-
ment of bacteria is extracted by absolute alcohol and ether in succession, trans-
ferred to a weighed porcelain crucible, and dried at io2°C. to constant weight.
This dried sample is then used in the nitrogen determination. Our procedure
differs from that of MacNeal in that the bacterial dry matter is not determined.
A saving of about seven days' time and of considerable labor is accomplished by
this omission.

Inasmuch as it has been shown by various investigators that such bacteria as
are present in the feces contain on the average about 11 per cent of nitrogen, the
values for bacterial nitrogen as determined by our method may conveniently serve
as a basis for the calculation of the actual output of bacterial substance.

23. Quantitative Deterinination of Indol in Feces. Bergeim's Modification of the
Herter -Foster Method.' — Principle. — The feces is distilled from alkaline solution
to remove phenols. This distillate are again distilled from acid solution to remove
ammonia. The indol in the final distillate is treated with /3-naphthaquinone sodium
monosulphonate and alkali and the blue compound formed extracted with chloro-
form and determined colorimetrically.

Procedure. — Rub 30-50 grams of the fresh, well-mixed feces in a mortar with
water to a uniform consistency. Transfer to a wide mouth Kjeldahl flask of about
1000 c.c. capacity, rinsing mortar and neck of flask with distilled water to make
about 400 c.c. Add 5 c.c. of 10 per cent KOH solution and about 2 c.c. of paraffin
to decrease foaming. Distill with steam using ordinary Kjeldahl distillation ap-
paratus with good stream of water in the condenser. Heat carefully for a few
minutes until danger of foaming is past and then allow to boil vigorously. Distill
over 500 c.c. of liquid, bringing the volume of the fecal suspension down to about
100 c.c. toward the end of the distillation.

^ Ehrenpfordt: Zeii. cxp. Path. Thcr., 7, 455, 1909.

2 In later work (see Blatherwick and Hawk: Biochem. Bull., 3, 28, 1913) it was
found advantageous to centrifugalize with alcohol and ether in succession before trans-
ferring the bacterial cells to Kjeldahl flasks.

3 Herter and Foster: Jour. Biol. Chcm., i, 257, 1906. Bergeim, Fishback, and Hawk:
Unpublished data.

FECES

243

Transfer the distillate to a clean Kjeldahl flask, add 2 drops of phenolphthalein
as an indicator. Make neutral with N sulphuric acid and add i c.c. excess. Dis-
till with steam as before, collecting the first 500 c.c. of distillate and bringing the
residue finally to about 100 c.c. Mix distillate well by shaking.

Take an aliquot portion of the distillate (100 c.c); add i c.c. of a 2 per cent
solution of /3-naphthaquinone sodium monosulphonate solution. Then add 2 c.c.
of 10 per cent KOH. Shake and let stand for 15 minutes. This is best carried out
in a 150 c.c. Squibb shape separatory funnel. Extract with chloroform, shaking
vigorously, using a 10 c.c. and a 7 c.c. portion which will bring the total volume of
the extract to the mark of a 15 c.c. graduated tube. Mix thoroughly. Run at
the same time and in the same way a standard using i c.c. of a solution of indol o.i
mg. of indol per c.c. Compare the extract with this standard in a colorimeter,
using the standard ordinarily at the .30-mm. mark. Calculate the indol to the
basis of milligrams of indol per gram of moist feces.

Indol. and naphthaquinone solutions should be freshly prepared or may be
kept in the ice-box for some days. Indol distillates should be kept in the ice-box
if not used at once, especially in hot weather. The feces must be fresh.

24. Quantitative Determination of Fat in Feces. — Principle. — The
determination of fat in dried feces is a more or less tedious process, and
one which is somewhat dangerous if applied to pathological feces. Most
of the methods for the determination of fat in the moist feces are accurate,
but require a long time. Saxon^ has proposed a method for the deter-
mination of fat in moist feces, which is speedy, convenient, and accur-
ate. The soaps of the feces are converted into free fatty acids by
means of hydrochloric acid, and the material is then extracted by shak-
ing with ether. The ether removes the neutral fat. the fatty acids
which were present as such, the fatty acids derived from the soaps, and
the cholesterol. The ether is removed by distillation, the crude fat
purified by means of petroleum ether, and the weight of the total fat
obtained. The fat is then dissolved in benzol and titrated with tenth-
normal sodium alcoholate solution, using phenolphthalein as an indi-
cator. The fatty acid is calculated, from the titration, to stearic acid.

Procedure. — Place about 5 grams (accurately weighed > of the thoroughly
mixed feces in a 100 c.c. glass-stoppered graduated cylinder. -

Add 20 c.c. of distilled water, i to 2.5 c.c. of concentrated hydrochloric acid
(depending upon the amount of the sample) and again, suflBcient distilled water
to make a total bulk of 30 c.c. Add exactly 20 c.c. of ether, stopper, and shake
vigorously for five minutes. Allow to stand for a few seconds, remove the stopper,
add exactly 20 c.c. of 95 per cent alcohol, and again shake for five minutes.

Stand the cylinder aside. The ether, containing practically all of the fat,
will come to the top as a colored transparent layer. Blow the ether layer ofif into

^ Saxon: J. Biol. CItem., 17, gg, 19 14.

^ Care must be taken not to smear the neck of the cylinder. This may be avoided by
removing the feces from the weighing bottle by means of a glass rod, the end of which is
flattened, and bent in the shape of a hoe, and transferring small bits of the feces from the hoe
to the cylinder, using short pieces of glass rod, which are dropped into the cylinder together
with the feces.

244 PHYSIOLOGICAL CHEMISTRY

a tall 150-200 c.c. beaker. ^ The thin layer of ether which remains is diluted with
5 c.c. of ether, the tube slightly agitated, and the ether blown ofif. This is done
in all five times, care being taken each time to wash down the sides of the cylinder.
The stopper should also be washed.

Twenty c.c. of ether are again added, and the cylinder shaken for five minutes
and set aside. When the ether has nearly stratified, blow it off and wash as
before. During the second washing stratification will complete itself.

Evaporate the ether- until no trace of the alcohol, which has been carried
over with it, remains. To the residue add 30 c.c. of low-boiling petrolevmi ether
(should boil below 6o°C.), and allow to stand over night. Petroleimi for this
work should be frequently tested for a residue on evaporation. If a residue is
left, the ether shoxild be redistilled.

Filter the petroleum ether solution of the fat, catch the filtrate and washings
in a tall, weighed, 100 c.c. beaker, evaporate off the solvent, dry the beaker at
90°C., desiccate and weigh.

After weighing, dissolve the contents of the beaker in 50 c.c. of benzol, heat
almost to the boiUng -point, add 2 drops of a 0.5 per cent solution of phenolphthalein,
and titrate with a decinormal solution of sodiimi alcoholate.^

Calculations.- — The weight of total fat is obtained by subtracting the
weight of the empty beaker from the weight of the beaker plus the dried
fat. The weight of fatty acids (in terms of milligrams of stearic acid)
is obtained by multiplying the number of cubic centimeters of deci-
normal sodium alcoholate solution by the factor 28.4. The difference
between the weight of total fat and the weight of fatty acids is the
weight of neutral fat in the sample extracted.

A separate determination without the addition of hydrochloric acid
may be run upon the sample, for the purpose of determining the weight
of neutral fat and free fatty acids. The difference between this weight
and the weight of total fat is the weight of fatty acid present in the
original sample in the form of soaps.

^ This is accomplished in the same manner that water is blown from a wash bottle.
The submerged end of the delivery tube is bent upward, as in the apparatus used for the
determination of fat in milk by Meig's method (see Milk). This avoids upward currents
which would disturb the subjacent alcohol-ether-feces layer.

^ Erlenmeyer flasks of about 200 c.c. capacity may be used, instead of beakers, for the
collection of the ether blown from the cylinders. The ether may then be distilled and re-
covered. The same procedure may be followed in removing the petroleum ether.

^ In the preparation of the sodium alcoholate solution, absolute alcohol and freshly cut,
bright, metallic sodium are used; otherwise the procedure is the same as that for the stand-
ardization and preparation of any alkali solution.

CHAPTER XV
BLOOD AND LYMPH

Blood is composed of four types of form-elements (erythrocytes or
red blood corpuscles, leucocytes or white blood corpuscles, blood plates
or plaques and blood dust or hemoconein) held in suspension in a fluid
called hlood plasma. These form-elements compose about 60 per cent of
the blood, by weight. Ordinarily blood is a dark red opaque fluid due to
the presence of the red blood corpuscles, but through the action of
certain substances, such as water, ether, or chloroform, it may be
rendered transparent. Blood so altered was formerly said to be laked.
The term hemolysis is now used in this connection and substances which
cause such action are spoken of as hemolytic agents. The hemolj^tic
process is simply a liberation of the hemoglobin from the stroma of
the red blood corpuscle. Normal blood is alkaline in reaction to
litmus, the alkalinity being due principally to sodium carbonate.
When examined according to physico-chemical methods the blood is
found to be neutral, i.e., it does not contain an excess of hydroxyl
ions. Even in cases of the most pronounced acidosis the reaction of the
blood is but slightly altered. The specific gravity of the blood of adults
ordinarily varies between 1.045 ^^^ i-075- It varies somewhat with
the sex, the blood of males having a rather higher specific gravity than
that of females of the same species. Under pathological conditions
also the density of the blood may be very greatly altered. The freezing-
point (a) of normal blood is about — o.56°C. Variations between
— 0.51° and — o.62°C. may be due entirely to dietary conditions, but if
any marked variation is noted it can in most cases be traced to a
disordered kidney function. The total amount of blood in the body has
been variously estimated at from one-twelfth to one-fourteenth of the
body weight. Perhaps 1/13.5 is the most satisfactory figure. Abder-
halden and Schmidt^ have suggested a unique method for the deter-
mination of this value. It is based upon the change in the optical
activity of the blood upon injection of a body of known optical activity,
such, for example, as dextrin. Keith, Rowntree and Geraght>- have
recently made use of a dye in the determination of blood \olumc.
. Among the most important constituents of blood plasma are the four

1 Abderhalden and Schmidt: Zeit. physiol. chetn., 66, 120, 1910.
* Keith, Rowntree and Geraghty: Arch. Int. Med., 16, 509, 1915.

245

246 PHYSIOLOGICAL CHEMISTRY

protein bodies, fibrinogen, nucleoprotein, serum globulin (euglobulin and
pseudo-globulin) and serum albumin. Plasma contains about 8.2 per
cent of solids of which the protein constituents named above constitute
approximately 84 per cent and the inorganic constituents (mainly
chlorides, phosphates and carbonates) approximately 10 per cent.
Among the inorganic constituents sodium chloride predominates. To
prevent coagulation, blood plasma is ordinarily studied in the form of
an oxalated or salted plasma. The former may be obtained by allowing
the blood to flow from an opened artery into an equal volume of 0.2 per
cent ammonium oxalate solution, whereas in the preparation of a salted
plasma 10 per cent sodium chloride solution may be used as the diluting
fluid.

Fibrinogen is perhaps the most important of the protein constituents
of the plasma. It is also found in lymph and chyle as well as in certain,
exudates and transudates. Fibrinogen possesses the general properties
of the globulins, but differs from serum globulin in being precipitated
upon half-saturation with sodium chloride. In the process of coagula-
tion of the blood the fibrinogen is transformed into fibrin. This fibrin is
one of the principal constituents of the ordinary blood clot.

The nucleoprotein of blood possesses many of the characteristics of
serum globulin. In common with this body it is easily soluble in sodium
chloride, and is completely precipitated from its solutions upon satura-
tion with magnesium sulphate. It is much less soluble in dilute acetic
acid than serum globulin, and its solutions coagulate at 65°-69°C.

The body formerly called serum globulin is probably not an indi-
vidual substance. Recent investigations seem to indicate that it
may be resolved into two individual bodies called euglobulin and pseudo-
globulin. The euglobulin is practically insoluble in water and may be
precipitated in the presence of 28-36 per cent of saturated ammonium
sulphate solution. The pseudo-globulin, on the contrary, is soluble in
water and is only precipitated by ammonium sulphate in the presence of
from 36 to 44 per cent of saturated ammonium sulphate solution.

In common with serum globulin the body known as serum albumin
seems also to consist of more than a single individual substance. The
so-called serum albumin may be separated into at least two distinct
bodies, one capable of crystallization, the other an amorphous body.
The solution of either of these bodies in water gives the ordinary albu-
min reactions. The coagulation temperature of the serum albumin mix-
ture as it occurs in serum or plasma varies from 70° to 85°C. according to
the reaction of the solution and its content of inorganic material.
Serum albumin differs from egg albumin in being more levorotatory,
in being rendered less insoluble by alcohol, and in the fact that when

BLOOD AND LYMPH 247

precipitated by hydrochloric acid it is more easily soluble in an excess of
the reagent.

When blood coagulates and the usual clot forms, a light yellow fluid
exudes. This is blood serum. It differs from blood plasma in contain-
ing a large amount oi fibrin ferment, a body of great importance in the
coagulation of the blood, and also in possessing a lower protein content.
The protein material present in plasma and not found in serum is the
fibrinogen which is transformed into fibrin in the process of coagulation
and removed. The specific gravnty of the serum of human blood
varies between 1.026 and 1.032. If blood be drawn into a vessel and
allowed to remain without stirring or agitation of any sort the major
portion of the red corpuscles will sink away from the upper surface,
causing this portion of the clot to assume a lighter color due to the
predominance of leucocytes- This light-colored portion of the clot is
called the '' buffy coat."

Beside the protein constituents already mentioned, other bodies
which are found in both the plasma and serum are the following: Sugar
{glucose), uric acid (urates), urea. fat. amino-acids. enzymes, lecithin,
creatine, carbamic acid, cholesterol and its esters, nucleoprotein. acetone
bodies, paralactic acid, gases, ammonia, coloring-matter (lutein or lipo-
chrome) and mineral substances. In addition to the substances just
named the blood doubtless contains a class of substances called hor-
manes of which adrenaline is the only one thus far definitely identified.
Some of the pathological constituents of blood are proteoses, biliary con-
stituents and purine bodies. In many pathological conditions certain
normal constituents are present in increased amount.

Normal human blood contains slightly less than o.i per cent of
glucose on the average. Strouse^ in a very recent series of tests places
the average glucose content at 0.084 per cent. That the diet influences
the sugar content is shown by the fact that two and one-half to four
hours after a meal the sugar content has been found to equal 0.18 per
cent.- In case of glycosuria the blood sugar may increase (hypergly-
cemia) to 0.3-1.0 per cent. For the quantitative determination of
blood sugar see page 279.

The determination of the cholesterol content of the blood is assuming
clinical importance. Normal blood contains 140-180 mg. per 100
grams of blood, or about 0.15 per cent. This value has been found to
be increased (hypercholesterolemia) in gall stones, pregnancy, nephritis,
diabetes, and arteriosclerosis and syphilis. (See page 285 for quantitative
methods.)

' Strouse: Bull. Johns Hop. Hasp., 26, 211. 1915.
^Hirsch: Zeil. physiol. Client., 93. 355, 1915.

248 PHYSIOLOGICAL CHEMISTRY

Uric acid is present in normal blood to the extent of about 1-2 mg.
per 100 grams of blood. In gout this value may be increased to 4-6
mg. The quantitative determination of the uric acid content of blood
is of importance as an aid in differentiating gout and certain other
disorders exhibiting similar clinical symptoms (for method see page
274).

The non-protein nitrogen of normal blood amounts to about 25-35
mg. per 100 grams of blood. The urea forms about 50 per cent of this,
creatinine 2 per cent, uric acid 2 per cent, ammonia 0.3 per cent, and
amino-acids, etc., about 46 per cent. In nephritis the non-protein
nitrogen of the blood is much increased. Myers and Fine^ report a
fatal case of uremia in which the non-protein nitrogen reached 300 mg.

Amino-acids are always present in the blood. They result for the
most part from the digestion of protein material in the intestine.

Creatinine occurs in normal blood to the extent of about 1-2 mg.
per 100 c.c. of blood. In uremia the amount is increased.^ Various
investigators report the values as ranging from 5 to 33 mg. per
100 c.c.

The creatine content of normal blood ranges from 5 to 10 mg. per
100 c.c. of blood. The creatine values have no important pathological
significance at the present time.

The acetone (acetone and acetoacetic acid) content of normal blood
ranges from o to i mg. per 100 c.c. of blood. In mild diabetes mellitus
the value rises to 5-12 mg., whereas in severe diabetes mellitus (coma)
as much as 20-45 ^g- P^^ 1°° c.c. of blood serum has been found.

Normal blood contains about 20 per cent of solids and 3 per cent of
total nitrogen, whereas chlorides are present to the extent of about 0.65
per cent. In severe diabetes the chlorides are decreased because of the
accompanying diuresis.

AbeP and associates have devised a method by which diffusible
substances may be removed from the blood of a living animal. The
process is termed vividifusion and is brought about by permitting the
blood from an artery to flow through collodion tubes surrounded by
physiological salt solution. The dialyzable substances, except sodium
chloride, are removed and the dialyzed blood is returned to the body of
the animal by means of a vein. The apparatus has been modified by
McGuigan and von Hess."*

1 Myers and Fine: Chemical Composition of the Blood in Health and Disease, 1915.
^ Folin and Denis; Jour. Biol. Chcm., 17, 487, 1914.
Myers and Fine: Jour. Biol. Chcm., 20, 391, 191 5.
3 Abel, Rowntree and Turner: Transactions of the Ass'n of American Physicians, 1913;
also Jour, of P harm, and Exp. Therap., 5, 275, 1914.

* McGuigan and Von Hess: Jour. Pharm. and E.xp. Therap., vol. 6, 1914'.

PLATE IV.

Normal Erythrocytes and Leucocytes.

BLOOD AND LYMPH 249

In the application of blood-letting or venesection it has been cus-
tomary to discard both the corpuscles and plasma of the withdrawn
blood. AbeP and associates have found it possible to separate the
corpuscles from the removed blood by centrifugation and to return
them to the body suspended in Locke's solution. They name the pro-
cedure plasma phcBresis. By this means blood-letting can be carried
out repeatedly during a short interval of time without endangering the
life of the animal.

There has been considerable controversy regarding the form of the
erythrocytes or red blood corpuscles of human blood. It is claimed by
some investigators that the cells are hell-shaped or cup-shaped. As the
erythrocytes occur normally in the circulation, however, they are prob-
ably thin, non-nucleated, biconcave discs.-

The blood of most mammals contains erythrocytes similar in form
to those of human blood. In the blood of birds, fishes, amphibians and
reptiles the erythrocytes are ordinarily more or less elliptical, biconvex
and possess a nucleus. The erythrocytes vary in size with the different
animals. The average diameter of the erythrocytes of blood from
various species is given in the following table :^

Elephant . -V, ,f of an inch.

Guinea-pig .,-2^3- of an inch.

Man jji. jj of an inch.

Monkey ,~'j^ of an inch.

Dog .,,ig j^ of an inch.

Rat. ._ j^ij ., of an inch.

Rabbit ^gijj of an inch.

Mouse ^>.V3 of an inch.

Lion 5^-ji^^ of an inch.

Ox :i2 r? of an inch.

Horse -j-^^ of an inch.

Pig 3^^5 of an inch.

Cat -i^^ of an inch.

Sheep ;, j,Jy; of an inch.

Goat T,-^^, of an inch.

Musk-deer i , j i ^ of an inch.

The erythrocytes, from whatever source obtained, consist essentially
of two parts, the stroma or protoplasmic tissue and its enclosed pigment,
hemoglobin. For human blood the number of erythrocytes present in
the fluid as obtained from well-developed males in good physical condi-
tion is about 5,500,000 per cubic millimeter."* The normal content of
the blood of adult females is from 4,000,000 to 4,500,000 per cubic

^Abel, Rowntree, Turner, Marshall and Lamson (see Abel's Mellon Lecture," 1915):
also Abel: Science, 42, 135, 1915.

* When examined singly under the microscope, they possess a pale greenish-yellow
color (see Plate IV, opposite), whereas when grouped in large masses a reddish tint is
noted.

' Wormley's Micro-Chemistry of Poisons, second edition, p. 733.

* This statement is based upon observations made upon the blood of athletes in training.
See Hawk: Amer. Jour. Physiol., 10, 384, 1904. It is generally stated in text-books that
the blood of males contains about 5,000,000, per cubic millimeter.

250 PHYSIOLOGICAL CHEMISTRY

millimeter. The number of erythrocytes varies greatly under different
conditions. For instance, the number may be increased after the trans-
fusion of blood of the same species of animal; by residing in a high
altitude; or as a result of strenuous physical exercise continued over a
short period of time. An increase is also noted in starvation; after
partaking of food; after cold or hot baths; after massage, as well as
after the administration of certain drugs and accompanying certain
diseases, such as cholera, diarrhea, dysentery and yellow atrophy of the
liver. A decrease in the number occurs in the different forms of anemia.
The number has been known to increase to 7,040,000 per cubic milli-
meter as a result of physical exercise, while 11,000,000 per cubic milli-
meter have been noted in cases of polycythemia and increases nearly as
great in cyanosis. The number has been known to decrease to 500,000
per cubic millimeter or lower in pernicious anemia.

Erythrocytes possess the property, when properly treated, of
"clumping" together in masses and precipitating, producing so-called
agglutination. Cells other than erythrocytes {e.g., bacteria) possess
this property. When spoken of in connection with the blood such
action is termed hemagglutination. A substance which will bring about
hemagglutination is said to contain hemagglutinins. These hem-
agglutinins are particularly abundant in the vegetable kingdom.^ For
a demonstration of hemagglutination see page 261.

Oxyhemoglobin, the coloring matter of the blood, is a conjugated
protein. Through treatment with hydrochloric acid it may be split into
a protein body called globin, and hemochromogen, an iron-containing
pigment. The latter body is rapidly transformed into hematin in the
presence of oxygen, and this in turn gives place to hematin-hydrochlo-
ride or hemin (Figs. 78 and 79, page 265). The pigment of arterial blood
is for the most part loosely combined with oxygen and is termed oxy-
hemoglobin, whereas the pigment of venous blood is principally hemo-
globin (so-called reduced hemoglobin) . Oxyhemoglobin is the oxygen
carrier of the body and belongs to the class of bodies known as respira-
tory pigments. It is held within the stroma of the erythrocyte. The re-
duction of oxyhemoglobin to form hemoglobin (so-called reduced hemo-
globin) occurs in the capillaries. Oxyhemoglobin may be crystallized
and a specific form of crystal obtained from the blood of each individual
species (see Figs. 70 to 76, pages 251 to 254). This fact seems to indi-
cate that there are many varieties of oxyhemoglobin. The interesting
findings of Reichert and Brown are of great value in this connection.
These investigators prepared oxyhemoglobin crystals from the blood

^Mendel: Archivio di fisiologia, 7, 168, 1909; also Schneider: Journal of Biological
Chem., II, 47, 1912.

BLOOD AND LYMPH

2qi

Fig. 70. — Oxyhemoglobin Crystals from Blood of the Guinea-pig.
Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the University

of Pennsylvania.

^x'^

\

< h

1

^-/

4k

Fig. 71. — Oxyhemoglobin Crystals from Blood of the Rat.
Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the University

of Pennsvlvania.

252

PHYSIOLOGICAL CHEMISTRY

Fig. 72. — Oxyhemoglobin Crystals from Blood of the Horse.
Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the University

of Pennsylvania.

#

Fig. 73. — Oxyhemoglobin Crystals from Blood of the Squirrel.
Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the University

of Pennsylvania.

BLOOD AND LYMPH

253

Fig. 74. — OxYHEiioGLOBix Crystals from Blood of the Dog.
Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the University

of Pennsylvania.

Fig. 75. — Oxyhemoglobin' Crystals from Blood or the C.\t.
Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the University

of Pennsvlvania.

254

PHYSIOLOGICAL CHEMISTRY

of over one hundred species of animal and subsequently studied the
characteristics of the crystals very minutely from the standpoint of
crystallography. Their findings may prove of importance from the
standpoint of heredity and the origin of species.

Fig. 76. — Oxyhemoglobin Crystals from Blood of the Necturus.
Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the University

of Pennsylvania. 1

HEMOGLOBIN

Carbon monoxide hemoglobin

Acid hematin (+ globin)

■fi"

0

•X3

CO

ei

^— s

■^

■^

'p

X

0^

^

v^

Oxyhemoglobin

Hemin ^/)J

(Hematin hydrochloride) N . _ .

Acid hematoporph3rrin (+ iron)

Hemochromogen
Methemoglobin

3 .

ra t-r'

\^e

Alkaline hematin (+ globin)

Hemin

(Hematin hydrochloride)

Alkaline hematoporph3^in

* The micro-photographs of oxyhemoglobin (see pages 251-254) and hemin (see page
(265) are reproduced through the courtesj^ of Professors E. T. Reichert and Amos P. Brown,
of the University of Pennsylvania, who have investigated the crystalline forms of
biochemic substances.

BLOOD AND LYMPH 255

The following bodies may be derived from hemoglobin, and each
possesses a specific spectrum which serves as an aid in its detection
and identification: Oxyhemoglobin, methemoglobin, carbon-monox-
ide hemoglobin, nitric-oxide hemoglobin, hemochromogen, hematin,
acid-hematin, alkali-hematin and hematoporphyrin (see Absorption
Spectra, Plates I and II).

The relationship between hemoglobin and its derivatives may be
represented by the scheme shown on page 254.

The chemical transformations which occur in the blood duringrespira-
tion are complicated and of great importance. In brief the exchange of
oxygen and carbon dioxide may be described as follows: Oxygen from
the air passes through the lungs into the blood where it is appropriated
for the most part by the red blood corpuscles. The hemoglobin of
these corpuscles possesses the property of uniting with oxygen, forming
oxyhemoglobin. This oxyhemoglobin possesses a red color and imparts
to the arterial blood its bright appearance. The oxygen is thus borne
by these blood cells in the circulating blood to all parts of the body.
As the blood passes through the capillaries it gives up the major part of
its oxygen which is used by the tissues in their varied activities. As the
blood loses its oxygen it becomes darker in color due to the fact that
the oxyhemoglobin has been transformed into hemoglobin (or reduced
hemoglobin). At the same time in the tissue capillaries the blood takes
up excretory products from the tissues, the chief of which is carbon
dioxide. This carbon dioxide is present in the blood mainly as sodium
carbonate and sodium acid carbonate; a small amount is probably com-
bined with the proteins of the plasma. We now have so-called venous
blood. This is, in turn, carried to the lungs where the carbon dioxide is
exchanged for oxygen and the cycle is repeated.

The white corpuscles (or leucocytes) of human blood differ from
the red corpuscles (or erythrocytes) in many particulars, such as being
somewhat larger in size, in containing at least a single nucleus and in
possessing ameboid movement (see Plate IV, opposite page 249).
They are typical animal cells and therefore contain the following bodies
which are customarily present in such cells: Proteins, fats, glycogen,
purine bodies, enzymes, phosphatides, lecithin, cholesterol, inorganic salts
and water. Compound proteins make up the chief part of the protein
quota of leucocytes, the nucleoproteins predominating. Of the en-
zymes present the proteolytic are the most important. It is claimed^
that there are two proteolytic enzymes in leucocytes, one active in
alkaline solution and present in the polynuclear cells,- and the other

*Opie: Jour, of Ex peri menial Med., 8; Opie and Barker: Ibid., 9.
2 For discussion of different types of leucocytes see "Da Costa's Clinical Hematology"
or some similar volume.

256 PHYSIOLOGICAL CHEMISTRY

active in acid medium and present in mononuclear cells. It is claimed
that the granular leucocytes originate in the bone marrow, whereas
the non-granular leucocytes (lymphocytes) have a lymphatic origin
(lymph glands or lymphoid tissue) ; this matter of origin is uncertain.
The normal number of leucocytes in human blood varies between 5000
and 10,000 per cubic millimeter. The ratio between the leucocytes and
erythrocytes is about 1:350-500. A leucocytosis is said to exist when
the number of leucocytoses is increased for any reason. Leucocytoses
may be divided into two general classes, the physiological *and the
pathological. Under the physiological form would be classed those
leucocytoses accompanying pregnancy, parturition and digestion, as well
as those due to mechanical and thermal influences. The leucocytoses
spoken of as pathological are the inflammatory, infectious, post-hemor-
rhagic, toxic and experimental forms, as well as the type of leucocytosis
which accompanies malignant disease.

The blood plates (platelets or plaques) are round or oval colorless
discs which possess a diameter about one-third as great as that of the
erythrocytes. Upon treatment with certain reagents, e.g., artificial
gastric juice, they may be separated into a homogeneous, non-refractive
portion and a granular, refractive portion. The blood plates are
associated with the coagulation of the blood. This relationship is not
completely understood at present.

The hemoconein or so-called "blood dust" is made up of round
granules which usually have a diameter somewhat less than i micron.
The serum of normal as well as of pathological blood contains these
granules. They were first described by Miiller to whom they appeared
as highly refractile granules possessed of Brownian movement. The
"blood dust" is apparently not concerned with the coagulation of the
blood. The granules are insoluble in alcohol, ether and acetic acid
and are not blackened by osmic acid. According to Miiller, the gran-
ules making up the so-called "blood dust" constitute a new organized
constituent of the blood, whereas other investigators believe them to be
merely free granules from certain of the forms of leucocytes. They
appear to possess no clinical significance.

The processes involved in the coagulation of the blood are not fully
understood. Several theories have been advanced and each has its
adherents. The theory which appears to be fully as firmly founded
upon experimental evidence as any is the following: Blood contains a
zymogen called prothrombin which combines with the calcium salts
present to form an enzyme known as thrombin or fibrin-ferment. When
freshly drawn blood comes into contact with the air the fibrin-ferment
at once acts upon the fibrinogen present and gives rise to the formation

BLOOD AND LYMPH 257

oi fibrin. This fibrin forms in shreds throughout the blood mass and,
holding the form elements of the blood within its meshes, serves to
produce the typical blood clot. The fibrin shreds gradually contract,
the whole clot assumes a jelly-like appearance and the yellowish serum
exudes. If, immediately upon the withdrawal of blood from the body,
the fluid be rapidly stirred or thoroughly "whipped" with a bundle of
coarse strings, twigs or a specially constructed beater, the fibrin shreds
will not form in a network throughout the blood mass but instead will
cling to the device used in beating. In this way the fibrin may be
removed and the remaining fluid is termed defibrinated blood. The
above theory of the coagulation of the blood may be stated briefly as
follows :

I. Prothrombin + Calcium Salts = Thrombin (or Fibrin-ferment).

II. Thrombin (or Fibrin-ferment) -f Fibrinogen = Fibrin.
HowelP has suggested an ingenious modification of the above theory.

He says: "In the circulating blood we find as constant constituents
fibrinogen, prothrombin, calcium salts and antithrombin. The last-named
substance holds the prothrombin in combination and thus prevents its
conversion or activation to thrombin. When the blood is shed, the
disintegration of the corpuscles (platelets) furnishes material (throm-
boplastin) which combines with the antithrombin and liberates the
prothrombin; the latter is then activated by the calcium and acts on
the fibrinogen. According to this view the actual process of coagula-
tion involves only three factors, fibrinogen, prothrombin and calcium.
These three factors exist normally in the circulating blood but are
prevented from reacting by the presence of antithrombin."

The question as to whether menstrual blood coagulates has caused
much discussion. The most recent investigations seem to show that it
does not coagulate because of the removal of fibrin-ferment and fibrinogen
from such blood by the endometrium or lining membrane of the uterus.^

Among the medico-legal tests for blood are the following: (i)
Microscopical identification of the erythrocytes, (2) spectroscopic iden-
tification of blood solutions, (3) the guaiac test, (4) the benzidine reac-
tion, (5) preparation of hemin crystals. Of these five tests the last
two named are generally considered to be the most satisfactory. Tliey
give equally reliable results with fresh blood and ^^ith blood from clots
or stains of long standing, provided the latter have not been exposed to
a high temperature or to the rays of the sun for a long period. The
technic of the tests is simple and the formation of the dark brown or
chocolate-colored crystals of hemin or the production of the green or

' Howell: American Journal of Physiology, 29, 187, 191 1.
* Bell: Jour. Path, and Bad., 18, No. 4, 1914.

17

258 PHYSIOLOGICAL CHEMISTRY

blue color with benzidine is indisputable proof of the presence of blood
in the fluid, clot or stain examined. The weak point of the tests,
medico-legally, lies in the fact that they do not differentiate between
human blood and that of certain other species of animal.

The guaiac test (see page 262), although generally considered less
accurate than the hemin test, is held by some to be a more delicate test
than the hemin test if properly performed. One of the most common
mistakes in the manipulation of this test is the use of a guaiac solution
which is too concentrated and which, when brought into contact with
the aqueous blood solution, causes the separation of a voluminous
precipitate of a resinous material which may obscure the blue colora-
tion; this is particularly true of the test when used for the examination
of blood stains. A solution of guaiac made by dissolving i gram of the
resin in 60 c.c. of 95 per cent alcohol is very satisfactory for general use.
The test is frequently objected to upon the ground that various other
substances, e.g., milk, pus, saliva, etc., respond to the test and that it
cannot therefore be considered a specific test for blood and is of value
only in a negative sense. We have demonstrated to our own satisfac-
tion, however, that many samples of milk give the blue color upon the
addition of an alcoholic solution of guaiac resin without the addition of
hydrogen peroxide or old turpentine. It has also been shown^ that
those milks which respond positively, fail to do so after boiling. In the
case of blood the test is positive both before and after boiling the blood
for 15-20 seconds. Pus does not respond after boiling. Old, partly
putrilied pus gives the test even without the addition of hydrogen
peroxide or old turpentine, whereas fresh pus responds upon the addi-
tion of hydrogen peroxide. Saliva gives a positive reaction only in
case blood or pus is present. Certain plant extracts give the test before
but not after boiling for 15-20 seconds. Buckmaster has advocated
the use of an alcoholic solution of guaiaconic acid instead of an alcoholic
solution of guaiac resin. He claims that he was able to produce the
blue color upon the addition of the guaiaconic acid to milk only when
the sample of milk tested was brought from the country in sterile bottles,
and further, that no sample of London milk which he examined responded
to the test. In the application of the guaiac test to the detection of
blood, he states that he was able to detect laked blood when present in
the ratio i : 5,000,000 and unlaked blood when present in the ratio
I : 1,000,000. This author considers the guaiac test to be far more
trustworthy than is generally believed.

Up to within recent times it has been impossible to make an absolute
differentiation of human blood. The so-called "biological" blood test

^Leary: Private communication.

BLOOD AND LYilPH 259

has, however, made such a differentiation possible. ITiis test, known as
the Bordet reaction, is founded upon the fact that the blood serum of an
animal into which has been injected the blood of another animal of
different species develops the property of agglutinating and dissoK-ing
erythrocytes ' 5/w//ar to those injected, but exerts this influence upon
the blood from no other species. The antiserum used in this test is
prepared by injecting rabbits with 5-10 c.c. of human defibrinated
blood, at intervals of about four days, until a total of between 50 and 80
c.c. has been injected. After a lapse of one or two- weeks the animal is
bled, the serum collected, placed in sterile tubes and preserved for use as
needed. In examining any specific solution for human blood it is simply
necessary to combine the antiserum and the solution under examination
in the proportion of 1:100 and place the mixture at 37°C. If human
blood is present in the solution a turbidity wdll be noted and this will
change within three hours to a distinctly flocculent precipitate. This
antiserum will react thus with no other known substance.

Lymph may be considered as the "middle man" in the transactions
between blood and tissues. It is the medium by which the nutritive
material and oxygen transported by the blood for the tissues is brought
into intimate contact with those tissues and thus utilized. In the
further fulfillment of its function, the lymph bears from the tissues
water, salts and the products of the acti\dty and catabolism of the
tissues and passes these into the blood. Lymph, therefore, exercises
the function of a "go-between" for blood and tissues. It bathes every
active tissue of the animal body, and is believed to have its origin partly
in the blood and partly in the tissues.

In chemical characteristics, lymph resembles blood plasma. In fact,
it has been termed "blood without its red corpuscles." L>Tnph from
the thoracic duct of a fasting animal or from a large lymphatic vessel of
a well-nourished animal is of a variable color (colorless, yellowish or
slightly reddish) and alkaline in reaction to litmus. It contains
fibrinogen, fibrin-ferment and leucocytes and coagulates slowly, the clot
being less firm and bulky than the blood clot. Serum albumin and
serum globulin are both present in lymph, the albumin predominating
in a ratio of about 3 or 4:1. The principal inorganic salts are sodium
salts (chloride and carbonate), whereas the phosphates of potassium,
calcium, magnesium and iron are present in smaller amount.

Substances which stimulate the flow of lymph are termed lympha-
gogiies. Such substances as sugar, urea, certain salts (especially
sodium chloride), peptone, egg albumin, extracts of dogs' liver and
intestine, crab muscles and blood leeches are included in this class.

In a fasting animal, the lymph coming from the intestine is a clear,

26o PHYSIOLOGICAL CHEMISTRY

transparent fluid possessing the characteristics already outlined. After
a meal containing fat has been ingested, this intestinal lymph is white
or " milky." This is termed chyle and is essentially lymph possessing an
abnormally high (5-15 per cent) content of emulsified fat. This chyle
is absorbed by the lacteals of the intestine and transported to the lower
portion of the thoracic duct. Apart from the fat value, the composition
of lymph and chyle are similar.

Experiments on Blood

I. Defibrinated Ox-blood

1. Reaction. — Moisten red and blue litmus papers with 10 per cent sodium
chloride solution and test the reaction of the defibrinated blood. Test by Congo
red paper also.

2. Microscopical Examination. — ^Examine a drop of defibrinated blood under
the microscope. Compare the objects you observe with Plate IV, opposite page
249. Repeat the test with a drop of yoxxr own blood.

3. Specific Gravity. — ^Determine the specific gravity of defibrinated blood
by means of an ordinary specific gravity spindle. Compare this result with
the specific gravity as determined by Hammerschlag's method in the next
experiment.

4. Specific Gravity by Hammerschlag's Method. — Fill an ordinary urinom-
eter cylinder about one-half full of a mixture of chloroform and benzene, having
a specific gravity of approximately 1.050. Into this mixture allow a drop of the
blood under examination to fall from a pipette or directly from the finger in case
fresh blood is being examined. Care must be taken not to use too large a drop
of blood and to keep the drop from coming into contact with the walls of the cyl-
inder. If the blood drop sinks to the bottom of the vessel, thus showing it to be
of higher specific gravity than the surroimding fluid, add chloroform until the
blood drop remains suspended in the mixture. Stir carefully with a glass rod
after adding the chloroform. If the blood drop rises to the surface upon being
introduced into the mixture, thus showing it to be of lower specific gravity than the
surrounding fluid, add benzene until the blood drop remains suspended in the
mixtiu-e. Stir with a glass rod after the benzene is added. After the blood
drop has been brought to a suspended position in the mixture by means of one or
more additions of chloroform and benzene this final mixture should be filtered
through muslin and its specific gravity accurately determined. What is the
specific gravity of the blood under examination?

5. Tests for Various Constituents. — ^Place 10 c.c. of defibrinated blood in an
evaporating dish, dilute with 100 c.c. of water and heat to boiling. Is there any
coagulation, and if so what bodies form the coagxilum? At the boiUng-point
acidulate slightly with dilute acetic acid. Filter. The filtrate should be clear
and the coagulum dark brown. Reserve this coagulum. What body gives the
coagulum this color? Evaporate the filtrate to about 25 c.c, filtering off any
precipitate which may form in the process. Make the following tests upon the
filtrate :

(a) Fehling's Test. — To 5 c.c. of theneutraUzed filtrate add 5 drops of Fehhng's
solution and boil one minute.

BLOOD AND LYMPH 26 I

(b) Chlorides. — ^To a small amount of the filtrate in a test-tube add a few-
drops of nitric acid and a Uttle silver nitrate. In the presence of chloride, a white
precipitate of silver chloride will form.

(c) Phosphates. — Test for phosphates by nitric acid and molybdate solution
according to directions given on page 59.

(d) Proteose and Peptone. — Test a small amount of the solution for pro-
teose and peptone by saturating with ammonium sulphate according to directions
given on page 120.

(e) Crystallization of Sodium Chloride. — Place the remainder of the filtrate
in a watch glass and evaporate it on a water-bath. Examine the crystals under
the microscope and compare them with those in Fig. 80, page 267.

6. Test for Iron. — Incinerate a small portion of the coagulum from the last
experiment (5) in a porcelain crucible. Cool, dissolve the residue in dilute hy-
drochloric acid and test for iron by potassiimi ferrocyanide or ammonium thio-
cyanate. Which of the constituents of the blood contains the iron?

Fig. 77. — Efffxt of Water on Erythrocytes.

7. Hemolysis ("Laky Blood"). — Note the opacity of ordinary defibrinated
blood. Place a few cubic centimeters of this blood in a test-tube and add water,
a httle at a time, until the blood is rendered transparent. Hemolysis has taken
place. How does the water act in causing this transparency? Examine a drop
of hemolyzed blood under the microscope. How does its microscopical appear-
ance differ from that of unaltered blood? What other agents may be used to
bring about hemolysis?

8. Osmotic Pressure. — Place a few cubic centimeters of blood in each of
three test-tubes. Hemolyze the blood in the first tube according to directions
given in the last experiment (7) : add an equal volimie of isotonic (0.9 per cent)
sodium chloride to the blood in the second tube, and an equal volume of 10 per
cent sodium chloride to the blood in the third tube. Mix thoroughly by shaking
and after a few moments examine a drop from each of the three tubes under the
microscope (see Figs. 77 and 150, page 473). What do you find and what is
your explanation from the standpoint of osmotic pressure?

262 PHYSIOLOGICAL CHEMISTRY

9. Hemagglutination. — The common garden bean, such as the
Scarlet Runner/ contains a protein substance which exhibits the
interesting property of causing a clumping or agglutination of red
blood corpuscles.^

Dilute defibrinated blood^ ten times with physiological sodium chloride solu-
tion (0.9 per cent) and place i c.c. in each of three small test-tubes.

Grind three beans in a coffee mill, or with mortar and pestle to a fine meal
and extract for a few minutes with 0.9 per cent sodium chloride solution. Filter
and add 0.05 c.c. (about 2-3 drops) of the filtered extract to the first of the blood
tubes ; o.oi c.c. to the second ; and 0.05 of 0.9 per cent sodium chloride to the third.

Invert each tube to mix the contents thoroughly, and note the rapid agglutina-
tion and precipitation of the blood corpuscles in the first tube, a less rapid aggluti-
nation in the second, while the third or control tube remains unaltered. In
one-half hour the corpuscles in the first tube often are packed soUd and one is
able to pour off perfectly clear senmi.

If the remainder of the bean extract is boiled for a few minutes, the coagulmn
filtered out and 0.05 c.c. of the filtrate added to the control tube, still no agglutina-
tion occurs, indicating that the hemagglutinin has been destroyed or removed
by the boihng.

10. Diffusion of Hemoglobin. — ^Prepare some hemolyzed ("laky") blood,
thus hberating the hemoglobin from the erythrocytes. Test the diffusion of the
hemoglobin by preparing a dialyzer Uke one of the models shown in Fig. 2, page
24. How does hemoglobin differ from other well-known crystalUzable bodies?

11. Guaiac Test. — To 5 c.c. of water in a test-tube add 2 drops of blood.
By means of a pipette drop an alcohoUc solution of guaiac 'strength about i : 60)*
into the resulting mixture xmtil a turbidity is observed and add old turpentine
or hydrogen peroxide, drop by drop, until a blue color is obtained.

In the detection of small amounts of blood the quantity of guaiac
used should also be decreased. Do any other substances respond in a
similar manner to this test? Is a positive guaiac test a sure indication
of the presence of blood? (See discussion on page 258.)

12. Schumm's Modification of the Guaiac Test. — To about 5 c.c. of the
solution under examination^ in a test-tube add about 10 drops of freshly prepared
alcoholic solution of guaiac. Agitate the tube gently, add about 20 drops of old
turpentine, subject the tube to a thorough shaking and permit it to stand for about
two to three minutes. A blue color indicates the presence of blood in the solution
under examination. In case there is insufficient blood to yield a blue color under

^ The Scarlet Runner is a familiar variety purchasable in every seed store. It occurs in
two varieties, the zc'/n'/e and the red. Ricin, a protein constituent of the castor bean, also
possesses pronounced agglutinating properties. Because of its poisonous nature it is, how-
ever, not suitable for use in class experiments.

-Mendel: Archivio di fisiologia, 7, 168, 1909; Schneider: Journal Biol. Chem., 11, 47,
1912.

' Rabbit's blood is especially desirable (Mendel: loc. cil.) and may be obtained for the
purpose by bleeding from a small cut on the animal's ear and detibrinating.

* Buckmaster advises the use of an alcoholic solution of guaiaconic acid instead of an
alcoholic solution of guaiac resin.

* Alkaline solutions should be made slightly acid with acetic acid, as the blue end-
reaction is very sensitive to alkali.

BLOOD AND LYMPH 263

these conditions, a few cubic centimeters of alcohol shovild be added and the tube
gently shaken, whereupon a blue coloration will appear in the upper alcohol-
turpentine layer.

A control test should always be made, using water in place of the solution under
examination. In the detection of very minute traces of blood only 3-5 drops of
the guaiac solution should be employed.

13. Ortho-tolidin Test (Ruttan and Hardisty).' — To i c.c. of a 4 per cent
glacial acetic acid solution of o-tolidin- in a test-tube add i c.c. of the solution
under examination and i c.c. of 3 per cent hydrogen peroxide. In the presence
of blood a bluish color develops (sometimes rather slowly) and persists for some
time (several hours in some instances).

This test is said to be as sensitive for the detection of occult blood
in feces and stomach contents as is the benzidine reaction. It is also
claimed to be more satisfactory for urine than any other blood test.
The acetic acid solution may be kept for one month with no reduction
in delicacy.

14. Benzidine Reaction.— This is one of the most delicate of the
reactions for the detection of blood. Dififerent benzidine prepara-
tions vary greatly in their sensitiveness, however. Inasmuch as ben-
zidine solutions change readily upon contact with light it is essential
that they be kept in a dark place.

The test is performed as follows : To a saturated solution of benzidine in
alcohol or glacial acetic acid add an equal volxmie of 3 per cent hydrogen peroxide
and I c.c. of the solution vmder examination. If the mixture is not already acid
render it so with acetic acid, and note the appearance of a green or blue color.
A control test should be made substituting water for the solution under
examination.

The hemoglobin decomposes the hydrogen peroxide (catalysis) and
the liberated oxygen oxidizes the benzidine. The sensitiveness of the
benzidine reaction is greater when applied to aqueous solutions than
when applied to the urine. According to Ascarelli^ the benzidine reac-
tion serves to detect blood when present in a dilution of i : 3,000,000.
Walter^ has also shown the test to be very delicate, and claims it to be
more satisfactory than the guaiac test.

Lyle, Curtman and Marshall have investigated the benzidine

^ Rattan and Hardisty: Canadian Medical Ass'n Journal, Nov., 1912; also Biochemical
Bull., 2, 225, 1913.

2 NHo NHo

\ , / ■

CoH* — C0H4.

/ \

CH3 CH3

^ Ascarelli: II policlin sez. prat., 1909.
■• Walter: Detit. vied. Woclt., 36, p. 309.
*Lyle, Curtman and Marshall: Jour. Biol. C//f»;., iq. 445, 19x4.

264 PHYSIOLOGICAL CHEMISTRY

reaction very carefully. They suggest a new procedure in preparing the
reagent^ and in conducting the test.

The test follows: Into a perfectly clean dry test-tube introduce 1.4 c.c.
benzidine solution, ^ add 0.2 c.c. of water or glacial acetic acid, then i c.c. of the
fluid to be tested and finally 0.4 c.c. of 3 per cent hydrogen peroxide. Note the
appearance of a blue color, which reaches its maximum in five to six minutes.

The acetic acid keeps the benzidine in solution. An excess dimin-
ishes the delicacy of the reagent.

Hydrogen peroxide supplies oxygen for the reaction and also bleaches
the blue color. An excess of peroxide interferes with the reaction by
destroying the catalytic power of the blood and by reacting with the
benzidine itself, with the formation of products which appear to have
an inhibitory action. It is very essential that the peroxide be added
last.

The benzidine solution should be dilute. Such solutions are exceed-
ingly sensitive and permit the detection of blood when present in ratio
I : 5,000,000.

15. Hem in Test. — (a) Teichmann's Method. — ^Place a very small drop of
blood on a microscopic shde, add a minute grain of sodiixm chloride^ and care-
fully evaporate to dryness over a low flame. Put a cover-glass in place, nm
imdemeath it a drop of glacial acetic acid and warm gently until the formation of
gas bubbles is noted. Add another drop of glacial acetic acid, cool the prepara-
tion, examine under the microscope and compare the crystals with those shown in
Figs. 78 and 79.

The hemin crystals result from the decomposition of the hemoglobin
of the blood. What are the steps involved in this process? The hemin
crystals are also called Teichmann's crystals. Is this an absolute test
for blood? Is it possible to differentiate between human blood and the
blood of other species by means of the hemin test?

(b) Nippe's Method. 3 — Spread a small drop of blood on a sUde in the form of
a film and evaporate to dryness over a low flame. Now add 2 drops of a solution
containing o.i gram each of potassixim chloride, iodide and bromide in 100 c.c.
of glacial acetic acid. Place a cover-glass in position and heat gently over a low
flame until gas bubbles form and the solution boils. Run 1-2 drops of the
reagent underneath the cover-glass and examine under a microscope. Compare
the crystals with those shown in Figs. 78 and 79.

This method is more rapid than Teichmann's method and crystals

1 Benzidine solution may be prepared as follows: Place 4.33 c.c. of glacial acetic acid in
a small Erlenmeyer flask, warm to 50° and add 0.5 gram of benzidine. Heat the flask for
eight to ten minutes in water at 50°. To the resultant solution add 19 c.c. of distilled
water. This solution may be kept for several days without deterioration.

2 Buckmaster considers the use of potassium chloride preferable.
^Nippe: Dent. nied. Woch., 38, 2222, 1912.

BLOOD AND LYMPH 265

-^^ "^ ^ ^

^e:^"**^

Fig. 78. — Heshn Crystals from Human Blood.

Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the University

of Pennsylvania.

Fig. 79. — Hemin Crystals from Sheep Blood.

Reproduced from a micro-photograph furnished by Prof. E. T. Reichert, of the
University of Pennsylvania.

266 PHYSIOLOGICAL CHEMISTRY

of inorganic chlorides are not formed. In Teichmann's method crystals
of sodium chloride often obscure the hemin crystals.

(c) Atkinson aiid KendalVs Method. — Introduce a small amount of the solution
under examination into a tube closed at one end, add sodium chloride and glacial
acetic acid as in Teichmann's method, ^ fuse or tightly plug the open end of the tube
and heat for fifteen minutes in a boiling water-bath. ^ Remove the tube and permit
it to cool to room temperature spontaneously. When the tube has cooled, break
it open, transfer the contents to a watch glass or small evaporating dish and con-
centrate on a water-bath until the volume of the fluid in the watch glass or dish
has been reduced to a few drops. Transfer a drop of this fluid to a slide, cover
with a cover slip, allow the slide to stand for a few minutes and examine it under a
microscope. Compare the crystals with those shown in Figs. 78 and 79, page 265.
In case crystals of sodium chloride (see Fig. 80) obstruct the view of the hemin
crystals, dissolve the sodium chloride crj'stals by running a drop of water under
the cover slip.

((f) V. Zeynek and Nencki's Method. — To 10 c.c. of defibrinated blood add acetone
until no more precipitate forms. Filter off the precipitated protein and extract it
with 10 c.c. of acetone made acid with 2-3 drops of hydrochloric acid. Place a
drop of the resulting colored extract on a slide, immediately place a cover-glass in
position and examine under the microscope. Upon the evaporation of the acetone,
crj'stals of hemin will form. Larger crystals may be obtained by evaporating the
acetone extract about one-half, transferring it to a stoppered vessel and allowing it
to remain overnight.

(e) Schalfijew's Method. — Place 20 c.c. of glacial acetic acid in a small beaker
and heat to 8o°C. Add 5 c.c. of strained defibrinated blood, again bring the
temperature to 8o°C., remove the flame and allow the mixture to cool. Examine
the crystals under the microscope and compare them with those reproduced in
Figs. 78 and 79, page 265.

16. Catalytic Action. — To about 10 drops of blood in a test-tube add twice the
volume of hydrogen peroxide, without shaking. The mixture foams. What is
the cause of this phenomenon?

17. CrystaUization of Oxyhemoglobin. Reichert's Method. — Add to 5 c.c.
of the blood of the dog, horse, guinea-pig, or rat, before or after laking, or de-
fibrinating, from i to 5 per cent of ammonium oxalate in substance. Place a
drop of this oxalated blood on a sHde and examine under the microscope. The
crystals of oxyhemoglobin wiU be seen to form at once near the margin of the
drop, and in a few minutes the entire drop may be a soUd mass of crystals.
Compare the crystals with those shown in Figs. 70 to 76, pages 251 to 254.

18. Preparation of Hematin. — Place 100 c.c. of hcmolyzed ilaked) blood in a
beaker and add 95 per cent alcohol until precipitation ceases. What bodies are
precipitated? Transfer the precipitate to a flask and boil with 95 per cent alcohol
previously acidulated with sulphuric acid. Through the action of the acid the
hemoglobin is spUt into hematin and a protein body called globin. Later the
"sulphuric acid ester of hematin" is formed, which is soluble in the alcohol. Con-
tinue heating until the precipitate is no longer colored, then filter. Partly saturate
the filtrate with sodium chloride and warm. In this process the "hydrochloric acid

1 Care should be taken not to add too great an excess of these reagents.
- This process insures constancy of temperature and strength of reagents.

BLOOD AND LYMPH

267

ester of hematin" is formed. Filter and dissolve on the filter paper by sodivim
carbonate. Save this alkaline solution of hematin and make a spectroscopic ex-
amination later after becoming familiar with the use of the spectroscope. How
does the spectrum of oxyhemoglobin differ from that of the derived alkali hematin ?
19. Preparation of Thrombin fHowell).' — Prepare fibrin from pig's blood
according to directions given on page 268. Wash the fibrin thoroughly in water
to remove hemoglobin. Squeeze out the water, mince the fibrin and cover with
an 8 per cent sodium chloride solution and allow to stand in the cold for 48 hours.
Filter. Precipitate the thrombin fand other proteins j from the filtrate by adding
an equal volume of acetone. Filter the mixture rapidly through a nximber of
small (25-50 c.c.) filters. Spread out filter papers and precipitate and dry rapidly
in a current of cold air. Cut the dried papers into small pieces and treat with a
volume of water eqmvalent to 66 per cent of the 8 per cent NaCl previously used.
Allow to stand one -half hour and filter. Shake the filtrate with chloroform
(10-15 c.c. per 100 c.c. filtrate) until on settling no opalescence'is developed by

Fig. 80. — SiiDir-M Chloride.

heating a portion of the supernatant fluid. Decant the Uquid and evaporate
on watch glasses (2 c.c. to a watch glass) in a current of air. Thrombin so pre-
pared may be kept indefinitely in a desiccator.

20. Variation in Size of Erythrocytes. — Prepare two small funnels with filter
papers such as are used in quantitative analysis. Moisten each paper with physio-
logical (isotonic) salt solution. Into one funnel introduce a small amount of
defibrinated ox blood and into the other funnel allow blood to drop directly from a
decapitated frog. Note that the filtrate from the ox blood is colored, whereas that
from the frog blood is colorless. What deduction do you make regarding the
relative size of the erythrocytes in ox and frog blood? Does either filtrate clot?
Why?

n. Blood Serum-

I. Coagulation Temperature. — Place 5 c.c. of undiluted serum in a test-tube
and determine its temperature of coagulation according to the method described

1 Howell: Am. Jour. Physiol., 32, 264. igi3.

* For directions as to preparation of serum, see "Reagents and Solutions." (Page 593.)

268 PHYSIOLOGICAL CHEMISTRY

on page 105. Note the temperature at which a cloudiness occurs as well as the
temperature at which coagulation is complete.

2. Precipitation by Alcohol. — To 5 c.c. of senun in a test-tube add twice the
amount of 95 per cent alcohol and thoroughly mix by shaking. What is this pre-
cipitate? Make a confirmatory test. Test the alcohoUc filtrate for protein.
Explain the result.

3. Proteins of Blood Serum. — ^Place about 10 c.c. of serum in a small evapo-
rating dish, dilute with 5 c.c. of water and heat to boihng. At the boiUng-point
acidify sUghtly with dilute acetic acid. Of what does this coagulum consist?
Filter off the coagulum (reserve the filtrate) and test it as follows :

(a) Millon's Reaction. — Make the test according to directions given on page

97.

(b) Hopkins-Cole Reaction. — Make the test according to directions given on
page 98.

4. Sugar in Serum. — To 5 c.c. of the neutralized filtrate from Experiment 3
add 5 drops of Fehling's solution and boil one minute. What do you conclude?

5. Detection of Sodium Chloride. — (a) Test a little of the filtrate from Ex-
periment 3 for chlorides, by the use of nitric acid and silver nitrate, (b) Evapo-
orate 5 c.c. of the filtrate from Experiment 3 in a watch glass on a water-bath.
Examine the crystals and compare them with those reproduced in Fig. 80, p. 267.

6. Separation of Serum Globulin and Senun Albvunin. — Place 10 c.c. of
blood serum in a small beaker and saturate with magnesimn sulphate. What is
this precipitate? Filter it off and acidify the filtrate sUghtly with acetic acid.
What is this second precipitate? Filter this precipitate off and test the filtrate
by the biuret test. What do you conclude?

III. Blood Plasma

1. Preparation of Oxalated Plasma. — Allow arterial blood to run into an equal
volume of 0.2 per cent ammonium oxalate solution.

2. Preparation of Fibrinogen. — To 25 c.c. of oxalated plasma add an equal
volume of saturated sodiiun chloride solution. Note the precipitation of fibrin-
ogen. Filter off the precipitate (reserve the filtrate) and test it by a protein color
test (see page 97).

3. Effect of Calcium Salts. — Place a small amount of oxalated plasma in a
test-tube and add a few drops of a 2 per cent calciiim chloride solution. What
occurs? Explain it.

4. Preparation of Salted Plasma. — Allow arterial blood to run into an equal
volume of a saturated solution of sodium sulphate or a 10 per cent solution of
sodium chloride. Keep the mixture in a cool place for about 24 hours.

5. Effect of Dilution. — Place a few drops of salted plasma in a test-tube and
dilute it with 10-15 volumes of water. What do you observe? Explain it.

rV. Fibrin

I. Preparation of Fibrin. — Allow blood to flow directly from the animal into
a vessel and rapidly whip it by means of a bundle of twigs, a mass of strong cords,
or a specially constructed beater. If a pure fibrin is desired it is not best to
attempt to manipulate a large volmne of blood at one time. After the fibrin has
been collected it shoxild be freed from any adhering blood clots and washed in
water to remove further traces of blood. The piure product should be very Ught
in color. It may be preserved under glycerol, dilute alcohol, or chloroform water.

BLOOD AND LYMPH 269

2. Solubility.— ^Try the solubility of small shreds of freshly prepared fibrin
in water, dilute acid and alkali.

3. Millon's Reaction. — Make the test according to directions given on page

97-

4. GlyoxyUc Acid Reaction CHopkins-Colej. — Make the test according to
directions given on page 98.

5. Biuret Test. — Make the test according to directions given on page 98.

V. Detection of Blood in Stains on Cloth, Etc.

1. Identification of Corpuscles. — ^If the stain under examination is on cloth
a portion should be extracted with a few drops of glycerol or physiological ^0.9 per
cent) soditim chloride solution. A drop of this solution should then be examined
under the microscope to determine if corpuscles are present.

2. Tests on Aqueous Extract. — A second portion of the stain should be
extracted with a small amount of water and the following tests made upon the
aqueous extract :

(a) Hemochromogen. — Make a small amount of the extract alkaline by
potassiimi hydroxide or sodiimi hydroxide, and heat imtil a brownish-green color
results. Cool and add a few drops of ammoniimi sulphide or Stokes' reagent
(see page 296) and make a spectroscopic examination. Compare the spectnmi
with that of hemochromogen (see Absorption Spectra, Plate 11). Hankin^ has
suggested a test based upon the formation of cyanhemochromogen and the
microspectroscopical demonstration of the spectrum of this compoimd.

(b) Hemin Test. — Make this test upon a small drop of the aqueous extract
according to the directions given on page 264.

(c) Guaiac Test. — Make this test on the aqueous extract according to the
directions given on page 262. The guaiac solution may also be appUed directly
to the staia without previous extraction in the following manner : Moisten the
stain with water, and after allowing it to stand several minutes, add an alcohoUc
solution of guaiac (strength about i : 60) and a httle hydrogen peroxide or old
tvirpentine. The customary blue color will be observed in the presence of blood.

(d) Benzidine Reaction. — Make this test according to directions given on
page 263.

(e) Acid Hematin. — If the stain fails to dissolve in water extract with acid
alcohol and examine the spectrum for absorption bands of acid hematin (see
Absorption Spectra, Plate II).

' Hankin: Brit. Med. Jour., p. 1261, 1906.
Sutherland and Mitra: Biochemical Journal, 8, 128, 191 4.

CHAPTER XVI

BLOOD ANALYSIS

The study of the composition of the blood under various normal and
pathological conditions has received great impetus from the development
of methods for blood analysis which require but small amounts of
material and yet give accurate results. Many facts of physiological
as well as clinical importance have thus been made available. Some
t)^ical examples of data obtained in this way are given in the following
table:

COMPOSITION OF NORMAL BLOOD AND OF THE BLOOD IN CERTAIN
PATHOLOGICAL CONDITIONS^

Normal

Chronic
nephritis

Uremia

Early
diabetes

Severe
diabetes

Gout

Lipemia

Cholelith-
iasis

Ar-
thritis

Total solids.

13-19

12-18

17-20

19-21

pel CCUt *■-<■ . w

Total N, per t
cent 30

2.5-3-0

1.7-2.7

I . 8-2 . 9

Non-protein 1
N i. 25-35

35-90

90-350

25—35

Urea N ; 12-23

16-70 70^300

Uric acid

1-3

1-4

4-27

3-6

3-8

Creatinine.. . .

1-2

1-3

4-33

Creatine 5-9

S-30

Amino-acidN. 4-5

6-16.0!

Ammonia N. 0.1-0.2

0.1-0.2

0.2-1.0

Sugar, percent

Acetone +
Acetoacetic

0.06-0. II

0.1-0.2

0.15-0.30

0.3-0.8

2-25

I. 5-12

10-40

^-hydroxy-
butyric acid 1 0-3 . 0

5-25

5-15

lO-SO

Cholesterol,

0.17-0. 35

o.is-0.30

o.S-3.6

0.28-0.95

Chlorides as
NaCl, percent 0.65

0. 55-0. 75

0 . 4S-0 . 65

0.60

•

Acid soluble]
phosphorus..: 2-6

3-7

7-21

Lipoid phos-
phorus 6-12

8-13

8-30

!

3-18

3-29

' Results are expressed as milligrams per 100 grams of blood unless otherwise indicated.
Some of the figures given are based upon but few analyses and may not be entirely charac-
teristic. The data here tabulated have been compiled from the work of many observers.
The following may be particularly mentioned: Myers and Fine: Jour. Biol. Chem., 20,
391, xgi 5; Post-Graduate, 1914-15; reprinted as "Chemical Composition of the Blood in
Health and Disease," New York, 1915; Folin and Denis: Jour. Biol. Chem., 14, 29, 1913;
13, 469, 1913; 17, 487, 1914; Arch. Int. Med., 16, 33, 1915; Christian, Frothingham and
Wood: Am. J. Med. Sci., 150, 655, 1915; Greenwald: Jour. Biol. Chem., 21, 29, 1915; Van
Slyke and Meyer: Jour. Biol. Chem., 12, 399, 1912; Bloor: Jour. Biol. Chem., 23, 317, 1915;
Marriott: Jour. Biol. Chem., 16, 293, 1913; 18, 507, 1914.

2 A short time after a meal rich in fat the blood may contain considerably more fat.

270

BLOOD ANALYSIS 27 I

It will be noted that in chronic nephritis the principal change is in
the urea and non-protein nitrogen of the blood which may increase
considerably. In severe cases associated with uremia the retention of
these forms of nitrogen may be very great and there is a consequent
rise in the blood content which may amount to looo per cent or more.
In uremia there is likewise a great increase in other individual nitroge-
neous components of the blood such as uric acid, creatinine, creatine,
amino-acid nitrogen, and even of ammonia. The increase in creatinine
has been shown by Myers and Fine and others to be significant, inas-
much as this increase does not appear to occur in other types of nephritis.
Uric acid is greatly increased in uremia and may be very much higher
than in gout. Associated with uremia there is ordinarily an acidosis.
There may be an increase in the sugar of the blood and a very great
increase of the acetone bodies present. An increase is also generally
found in cholesterol and in the various forms of phosphorus of the blood.

In diabetes the most noteworthy changes are in the content of glucose
and of acetone bodies. Glucose may be increased above the normal
(about 0.1 per cent) to 0.15-0.80 per cent. The increase in acetone,
diacetic acid and hydroxybutyric acid is very marked in comparison
with the minute amounts found in normal blood. There may also be
an increase in fat and other lipoids in severe diabetes.

In gout the characteristic change is in the uric acid content which is
almost always considerably increased. Other forms of nitrogen are
affected but little. In arthritis the blood may also be high in uric acid
but in this case ordinarily there is a rise in non-protein nitrogen also.

Lipemia is usually associated with an increased sugar content of the
blood. The fat content in this condition has been found as high as 29
per cent. There is a correspondingly large increase in the cholesterol
of the blood.

In cholelithiasis there appears generally to be a fairly marked
increase in the cholesterol content of the blood and this determination
is thus of diagnostic aid. Some increase may also be found in other
disorders as in nephritis, severe diabetes, pregnancy, alteriosclerosis
and syphilis.

Methods

Non -protein Nitrogen.— (a) Colorimetric Method of Folin and Denis .^
— Principle. — This method, which is simple and convenient, depends
upon the removal of the proteins from a sample of blood by precipita-
tion with methyl alcohol, and the estimation of nitrogen in the methyl

* Folin and Denis: /. Biol. Client., 11, 527, 191 2.

272 PHYSIOLOGICAL CHEMISTRY

alcohol solution (after the removal of the proteins) by means of oxi-
dation and Nesslerization. The details of the procedure are carried
out in the following manner:

Method of Drawing Blood. — ^Attach, by means of a short piece of pure gum
tubing, an hypodermic needle about i mm. in diameter and 25 mm. in length
(previously sterilized and paraflined) to the tip of a 2 or 5 c.c. pipette. Introduce
into the upper end of the pipette (which must be perfectly clean and dry) a small
pinch of powdered potassium oxalate, and allow it to run down into the tip and the
needle. Attach a piece of rubber tubing to the upper end of the pipette, and to this
a mouthpiece consisting of a short tapering glass tube. Place a pinchcock over
the rubber tube near the top of the pipette. To draw the blood, insert the needle
into the vein or artery and regulate the flow by means of the pinchcock and suc-
tion. The exact quantity of blood desired is thus obtained without any waste or
clotting.

Method of Isolating Non-protein Nitrogen Constituents. — Methyl alcohol and
zinc chloride are employed as precipitants for the protein materials of the blood,
and the determination of the non-protein nitrogen is then carried out upon a
portion of the methyl alcohol extract. The procedure is as follows: Transfer
the blood, as soon as drawn, to a measuring flask which is half filled with pure
methyl alcohol (must be acetone free). Fill to the mark with methyl alcohol
and shake thoroughly. (If 2 c.c. of blood are taken, 25 c.c. flasks are used for the
precipitation, while for 5 c.c. of blood 50 c.c. flasks are used.) Allow the flask
to stand for at least two hours and at the end of that time, or later, filter the con-
tents through dry filter paper. Add 2-3 drops of a saturated alcoholic solution of
zinc chloride to the filtrate and filter again through a dry filter paper after a few
minutes. The zinc chloride brings down an appreciable precipitate and the last
traces of coloring matter, so that the second filtrate obtained is perfectly colorless
and clear. This filtrate is used for the determination of non-protein nitrogen.

Trichloracetic Acid Modification. — Greenwald^ has suggested the
use of trichloracetic acid as the precipitant for the proteins of the blood,
as being more satisfactory than the methyl alcohol and zinc chloride.
The objection to the methyl alcohol is that some of the amino-acids
(creatine, asparagine, and tyrosine) are insoluble in it and hence pre-
cipitated along with the proteins. These acids are not removed by the
trichloracetic acid. Certain nitrogenous lipoid substances are precipi-
tated by the trichloracetic acid and not by the methyl alcohol. Green-
wald suggests that these substances, even though non-protein in char-
acter, should not be included with the non-protein nitrogen of the
amino-acids and urea.

Procedure. — ^Dilute the blood to ten times its original volume with 2.5 per
cent trichloracetic acid solution. Let stand 30 minutes and then filter. Shake
the filtrate with about 4 grams of kaolin per 100 c.c. and filter again. An aliquot
of this final filtrate is taken, digested with sulphuric acid and nitrogen deter-
mined in the usual way.

^ Greenwald: /. Biol. Chem., 21, 61, 1915.

BLOOD AXALYSIS 273

Determination of Total Non -protein Nitrogen. — Transfer 5 c.c. of the alcoholic
filtrate to a large Jena test-tube of the same kind as is used in urine analysis
(see page 485). Add i drop of concentrated sulphuric acid, i drop of kerosene,
and a small pebble or glass bead to prevent bimiping. Immerse the test-tube
in a beaker of boiUng water for five or ten minutes to drive off the methyl alcohol.
When the alcohol is removed add i c.c. of concentrated sulphuric acid, i gram of
potassium sulphate and i drop of copper sulphate solution. Boil, cool, dilute and
aerate the solution as described in the determination of total nitrogen in urine
(see page 485), except that the ammonia is collected in a large test-tube instead
of the 100 c.c. flask. Nesslerize the solution, using 7 to 8 c.c. of diluted Nessler
reagent (dilution i :5), dilute to 25 or 50 c.c. according to the amount of color,
and compare with a standard solution containing i mg. of ammonia nitrogen,
Nesslerized and diluted to 100 c.c. and the colorimeter prism set at 20 mm.

Calculations. — If 5 c.c. of blood are diluted to 50 c.c. and 10 c.c. of the alcohoUc
extract (equivalent to i c.c. of blood) are used for the determination, the amount
of non-protein nitrogen (as milligrams per 100 c.c. of the blood) can be obtained

20

by use of the formula p X D, in which R stands for the reading of the unknown

and D represents the volimie to which its ammonia has been diluted. If the
equivalent of 0.4 c.c. of blood has been taken for the determination the formula

P X D is used, and if the equivalent of 0.5 c.c. of blood has been taken the

40
formula becomes ^ X D.

(b) Colorimelric Method for Finger Blood. — Principle. — Taylor and
Hulton^ have suggested a modification for the determination of non-
protein nitrogen using from 4 to 8 drops of blood. It is based upon the
observation of Gulick^ that the presence of small amounts of potassium
sulphate does not appreciably interfere \\dth the Nesslerization of solu-
tions containing ammonium salts. The Nesslerization is accordingly
carried out directly upon the oxidized material without removal of the
ammonia by aspiration or distillation. The authors use a mixture of
ether and alcohol for the precipitation of proteins. The authors claim
only approximate accuracy for the method and the small amount of
lipoid nitrogen included with the other non-protein nitrogen may be
disregarded.

Procedure. — Place 10 c.c. of a mixture of absolute alcohol and ether (3 :i)

in a small Erlenmeyer flask. Stopper and weigh the flask with its contents.

Remove the stopper and allow from 4 to 8 drops of blood (depending upon the

amount of non-protein nitrogen) to drop from the finger which has been cleaned

and pricked with a sharp lance. The blood should drop freely when the hand is

held down. Insert the stopper and weigh the flask and contents. The increase

in weight is of course the weight of blood. Within a half-hour filter the mixture

into the digestion flask and wash the filter with 5 c.c. of alcohol-ether. The

filtrate is clear and practically free from protein, although it probably contains

traces of nitrogen-containing Upoids. The Kjeldahl digestion is carried out in a

^ A. E. Taylor and F. Hulton: /. Biol. Chan., 22, 63, 1915.
*Gulick: /. Biol. Clicm., 18, 541, 1914.

iS

2 74 PHYSIOLOGICAL CHEMISTRY

25 c.c. long-necked, round-bottomed Kjeldahl flask, the neck of which has a
crook near the top. Add a small piece of acid potassiimi sulphate, several glass
beads, and drive off the alcohol-ether by heating on a hot plate. When the flask
is nearly dry add i c.c. of concentrated sulphuric acid and not more than 300 or
400 mg. of potassium sulphate. Then place the flask over the direct flame of a
micro-burner (resting the bottom of the flask upon an asbestos board which has a
circular perforation a Uttle smaller than the circle of i c.c. of sulphuric acid in the
digestion flask) and heat until the mixture is colorless. Transfer the digestion
mixture to a 100 c.c. flask, neutraUze the sulphuric acid with about 3 c.c. of a 30
per cent solution of sodium hydroxide, fiU the flask to over three-quarters full
with ammonia-free water, and add 5 c.c. of Winkler's modification of Nessler's
solution (see page 603). Dilute to mark with water and compare the color in the
Duboscq colorimeter (see Fig. 153, p. 486) against a standard solution of ammo-
nium sulphate.

2. Urea. — The Urease Method. — Van Slyke and Cullen's^ Modification of
Marshall's Method.-

Principle. — See Urease Method, Chapter XXVI.

Procedure. — Run 3 c.c. of fresh blood (carefully measured with an accurate
pipette) into a 100 c.c. test-tube containing i c.c. of a 3 per cent solution of potas-
sium citrate (to prevent clotting). Add 0.5 c.c. of the urease solution^ and 2 or 3
drops of capryUc alcohol (to prevent foaming). After ten minutes add 15 c.c.
of a saturated solution of potassium carbonate, and drive off the ammonia by
aspiration into another tube containing 15 c.c. of hundredth -normal hydrochloric
or sulphuric acid. Titrate the excess of acid with hundredth-normal sodium
hydroxide or potassium hydroxide,* using methyl red or ahzarin as indicator.

Calculations. — Each cubic centimeter of acid neutralized indicates o.oi gram
of urea per 100 c.c. of blood, or 0.0467 gram of urea nitrogen per 100 c. c. of blood.
In case the blood should be one of the rare samples containing over o .15 per cent
of urea, all the acid will be neutraUzed, and it will be necessary to repeat the
determinations, using in the determination only i c.c. of blood. Fresh blood
contains so little ammonia that it may be disregarded. For further discussion of
the urease method see Chapter XXVI.

3. Uric Acid. — Colorimetric Microchemical Method. — Principle. —
Folin and Denis^ were the first to apply the technic of their method
for the determination of small quantities of uric acid to the quan-
titative estimation of uric acid in blood. (For a discussion of the
principle of the color reaction see the determination of uric acid in urine,
page 510.) The procedure necessary for the determination in blood is
somewhat different from that used for the determination in urine because
of the presence of proteins in the blood. These must be removed first,
and then the uric acid may be determined in the protein-free extract,
according to the procedure used for the determination in urine. The

^ Van Slyke and CuUen: J. Am. Med. Ass'n, 62, 1558, 1914.
-Marshall: Jour. Biol. Chem., 15, 487, 1913.

^ The enzyme solution is prepared as described under "Reagents and Solutions," p. 594.
* Rose and Coleman (Biochem. Bull., 3, 411, 1914) suggest the colorimetric determina-
tion of the ammonia (see page 492).

' Folin and Denis: /. Biol. Chem., 13, 469, 1913.

BLOOD ANALYSIS 275

proteins are removed from the blood by precipitation with hot dilute
acetic acid in the following manner:

(a) Folin-Denis Procedure. — The blood is drawn into small, wide-mouthed
bottles previously weighed and containing a small amount (about o.i gram 1 of
finely powdered potassium oxalate. From the subsequent weight of each bottle
is obtained the weight of the blood. Five times this weight of N 100 acetic acid
solution' is transferred to an ordinary 1000 c.c. fiask and heated to boiling. The
oxalated blood is then poured into this boiUng acetic acid solution, stirring con-
stantly, and the heating is continued until the solution has again begun to boil.
The mixture is filtered while stiU hot. The coagulated material on the filter paper
is transferred back into the flask (by means of a small spoon or a spatula 1, about
200 c.c. of boiUng water- are poured over it and it is allowed to stand for five
minutes. This mixture is then filtered through the same filter as was used for the
first filtration. The filtrate in the receiving flask should be very nearly as clear
as water, and will be found to be so if the original blood was promptly shaken
with the oxalate, so that no clotting has taken place.

If clotting has occurred, the coagulation and washing of the blood is a Uttle
more complicated. The clot leads to so much bumping in the boiling acetic acid
solution that it is not practical or safe to try to heat the mixture to boiUng.
.The filtration is, therefore, made earUer. The partially coagulated clot is then
broken up with a glass rod, transferred to a mortar and there ground into a paste
in the presence of hot water. This suspension is then poured on the filter. The
protein material on the filter is then washed, as before, with about 200 c.c. of hot
water. In this case the combined filtrates are, however, never colorless but more
or less reddish. On being heated to boiling a second small coagulum will be
obtained and the filtrate will then be practically as clear as water.

The combined filtrate and washings, containing the uric acid and other solu-
ble materials, is further acidified by the addition of 5 c.c. of 50 per cent acetic
acid and is evaporated, over a free flame in a suitable dish," to a very small
volume (about 3 c.c. ). The Uquid is then poured into an ordinary centrifuge tube
and the dish washed with two successive portions of o.i per cent lithium car-
bonate solution, using about 2 c.c. for each rinsing. Any solid material adhering
to the sides of the dish is removed by rubbing with a rubber-tipped stirring rod.
This solid material can be removed by centrifuging and pouring the superna-
tant Hquid into another tube, washing the sediment with lithium carbonate solu-
tion (Smith).

The liquid in the centrifuge tube, which at this stage should not be
more than lo c.c. in volume, is then treated as in the method for urine.

(b) Benedict Procedure. — Benedict^ has suggested that the pre-
cipitation of proteins by the method of Folin and Denis is incomplete,
and proposes the use of colloidal iron for the completion of precipitation

' Prepared by diluting 0.6 c.c. of glacial acetic acid to i liter.

- For this washing, water is used rather than .V/ioo acetic acid, because if the latter is
used the coagulum will give off more or less of the blood pigment and the filtrates are less
clear.

' Deep (half globular) dishes 10 cm. in diameter and having a capacity of 250 c.c. are
very good for this purpose. While free flames are the most convenient for concentrating
the uric acid solutions, care must, of course, be taken not to char the contents toward the
end of the operation. Unless the solution can be watched carefully at this stage, it is safer
to linish the concentration on the water-bath.

* Benedict: /. Biol. Clicm., 20, 629, 1915.

276 PHYSIOLOGICAL CHEMISTRY

after coagulation in dilute acetic acid. Myers and Fine^ suggest the
use of aluminium cream for this purpose. Benedict's procedure is as
follows:

To 20 C.C.2 of oxalated blood are added 100 c.c. of boiling N/ioo acetic acid
in a casserole, and the mixture is heated to boiling for a moment. Remove the
casserole from the flame and add 200 c.c. of boiling distilled water. Povir the
mixture upon a folded filter and wash the residue with 50 c.c. of boiling water
(heated in the same casserole in which the original coagulation took place).
Transfer the whole filtrate to a casserole and boil down rapidly to a volimie of
about 25 c.c. Pour this solution into a small flask roughly marked to indicate a
volume of 50 c.c. Transfer the contents of the casserole to the flask quantita-
tively, with the help of two or three portions of water, heating vigorously to
boiling and rubbing the sides of the casserole with a rubber-tipped stirring rod
each time. The total volume in the flask should not exceed 50 c.c. after the ad-
dition of the washings. Thoroughly cool the tixrbid solution in the flask imder
running water, and add 2 c.c.^ of colloidal iron solution (Merck's "Dialyzed Iron,"
5 per cent solution) while the flask is being gently rotated. Filter the mix-
ture through a small folded filter into a 100 c.c. Jena Florence flask, and wash
the residue twice with distilled water. The filtrate obtained here should be as
clear and colorless as distilled water. Boil the solution down to a volume of from
I to 2 c.c. (care being taken in the early stages to prevent bimiping), then care-
fully pour into a small centrifuge tube and wash out the flask with three portions
of water (i or 2 c.c. each), heating each to boiling in the flask and shaking thor-
oughly prior to transferring it to the centrifuge tube. The volume of liqmd in the
tube at this point should be from 5 to 10 c.c. Cool the Uquid, add 20 drops of the
ammoniacal sUver magnesium solution and proceed with the determination as
described under Urine (Chapter XXVI). If the amoimt of uric acid present is
very small the addition of i drop of cyanide solution, 1 c.c. of uric acid re-
agent, 5 c.c. of 20 per cent sodivun carbonate solution, and dilution to 25 c.c.
are carried out rather than using the larger quantities given for the determina-
tion in the urine.

4. Creatine and Creatinine. Methods oJFolin* — Preformed Creatinine. — Meas-
ure 10 c.c. of blood into a 50 c.c. volumetric flask or, better, into a 50 c.c. shaking
cylinder which can be closed with a glass stopper. Fill to the 50 c.c. mark with satu-
rated picric acid solution and shake a few times. Add about i gram of dry picric
acid to the mixture and shake for five minutes. Transfer the mixture to centrifuge
tubes, throw down the sediment and precipitate and pour the supernatant liquid
through a filter. This is the most economical process where but little blood is avail-
able. If desired, however, double quantities of blood and reagents may be taken and
filtration carried out without preliminary centrifugation. This process removes the
protein materials and leaves the creatine and creatinine in the filtrate which is a satu-

1 Myers and Fine: "Blood in Health and Disease," 1915, p. 14.

^ Smaller amounts of blood may be employed, and the quantity of acetic acid and
water correspondingly reduced. Unless the quantity of uric acid present is very large,
the results are far more accurate when 20 c.c. of blood are used.

* With old samples of blood it may be necessary to add 3 or 4 c.c. of the iron solution
and a little 10 per cent sodium chloride solution. When the precipitate separates in large
flocculent masses the right amount of iron has been added. Any excess of iron must be
avoided, as it would oxidize some of the uric acid later on in the process.

* Folin: Jour. Biol. Chetn.. 17, 475, 1914.

BLOOD ANALYSIS 277

rated picric acid solution. The preformed creatinine is then determined colorimet-
rically. For this purpose a standard solution of creatinine for comparison is
necessary. Prepare this from the standard creatinine stock solution as used in the
analysis of urine (see chapter on Quantitative Analysis of Urine) by diluting an
amount of this solution equivalent to i mg. of creatinine to 500 c.c. with saturated
picric acid solution. We have then a standard solution containing 0.2 mg. of
creatinine in 100 c.c- of saturated picric acid solution.

Take 20 c.c. portions each of the filtrate and of the standard solution. To each
solution then add exactly i c.c. of 10 per cent NaOH from a burette. (If the blood
filtrate becomes turbid on addition of alkali it must be centrifuged or filtered.)
Allow to stand for 10 minutes and compare the colors directly in the colorimeter
without further dilution. The standard creatinine solution may be set advantage-
ously at 20 mm., although this is not necessary.

• Calculation. — Since the blood was diluted five times in the precipitation pro-
cedure and as the standard for comparison contains 0.2 mg. of creatinine per 100 c.c,
it is merely necessary to divide the reading of the standard by the reading of the
unknown to obtain without further calculation the number of milligram'; of creatin-
ine in 100 c.c. of blood.

Creatine Plus Creatinine. — For determining the total creatinine plus creatine
in the blood carry out the preliminary precipitation with picric acid just as in the
determination of creatinine above. Take 10 c.c. of this filtrate for the determina-
tion. Transfer it to a small Erlenmeyer flask or large test-tube. Cover the flask
or test-tube with tin foil, transfer to an autoclave and heat to about i2o°C. for
about 20 minutes. The autoclave should not be opened until the temperature has
fallen below ioo°C. Cool the solution to room temperature, rinse into a 25 c.c.
volumetric flask with saturated picric acid solution. Add 1.25 c.c. of 10 per cent
NaOH for the development of the color.

On account of the variations in the creatine content of normal blood two
standard creatinine solutions are used. In working on pathological cases a third
standard is desirable. These standards contain 0.5, i, and 2 mg. of creatinine
respectively per 100 c.c. of saturated picric acid solution. To 20 c.c. of each of
these solutions in measuring cylinders add i c.c. of 10 per cent NaOH and allow
to stand for 10 minutes. By inspection determine which standard corresponds
most nearly in color with the unknown and use this for comparison. The standard
is usually set at 10 mm. in the Duboscq colorimeter.

Calculation. — Multiply the reading of the standard by 125 and by 0.5, i, or 2,
according to which standard is used, and divide by the reading of the unknown in
millimeters. The result gives the number of milligrams of creatine + creatinine
in 100 c.c. of the blood examined.

5. Amino-acid Nitrogen, (o) Method of Van Slyke and Meyer.^ — Principle. —
The protein of the blood is removed by precipitation with alcohol and the amino-
acid nitrogen determined in the filtrate by the nitrous acid method.

Procedure. — Thirty to 50 c.c. of freshly drawn blood are mixed with 9 or 10
volumes of 95 per cent alcohol to precipitate the proteins. The volume of the
alcohol-blood mixture must be known, but in case it is not convenient to use a
graduated cylinder for the mixture, its volume can be taken as the sum of the
volumes of the alcohol and blood without essentially affecting the results. The
alcohol and blood are thoroughly mixed, the vessel containing them is dosed and

' Van Slyke and Meyer: Jour. Biol. Client., 12, 399, 1912.

278 PHYSIOLOGICAL CHEMISTRY

24 hours are allowed for precipitation of the proteins to become complete. The
solution is filtered through a dry folded filter into a measuring cylinder without
washing the precipitate. The volume of filtrate is noted and is taken for analysis
as an aliquot part of the total blood-alcohol mixture. The filtrate is then con-
centrated to a volume of 3-5 c.c. and used for determination of amino nitrogen by
the Van Slyke nitrous acid method (see Chapter IV on Proteins). The use of a
few drops of caprylic alcohol to prevent foaming is advisable.

(b) Method of Cotistantino. ^^This is based on the formol titration procedure.
One hundred c.c. of blood or serum is mixed with a measured (500 c.c.) volume of 2
per cent mercuric chloride solution containing 0.8 per cent hydrochloric acid. The
mixture is shaken vigorously in a stoppered flask and allowed to stand a few hours.
Centrifugate for 10 minutes, pour the supernatant liquid through a dry filter into a
graduated cylinder. An aliquot of the filtrate is taken, the mercury is removed
with hydrogen sulphide and the latter by a current of air. The liquid is exactly
neutralized and concentrated on the water-bath, or better, at 50° in a vacuum,
MgO added, and the mixture distilled in a vacuum at 45° to get rid of ammonia.
The volume should now be about 30 c.c. A little solid barium chloride and barium
hydroxide are added and 1.5 c.c. of 0.5 per cent solution of phenolphthalein.
Filter. Neutralize accurately to sensitive litmus paper. Add neutral formalin
solution and titrate with N/5 NaOH as described in the chapter on quantitative
analysis of urine (page 504).

6. Ammonia. — Method of Folin and Denis. — The determination of ammonia in
blood is attended with considerable difficulty because of the fact that it is present
only in very small amounts, and to the fact that blood very readily and quickly
undergoes changes which are accompanied by the formation of ammonia from the
nitrogenous compounds present in the fresh blood.

Of the methods proposed for its quantitative estimation that of Folin and Denis^
is perhaps least unsatisfactory.

Principle. — The method is based upon the liberation of the ammonia from fresh
blood by aspiration after adding sodium carbonate solution, and the Nesslerization
of the solution into which the ammonia is aspirated.

Procedure. — Place 10 c.c. of systemic blood or 5 c.c. of portal or mesenteric blood^
in a large Jena test-tube. Add 2 or 3 c.c. of a solution composed of 15 per cent
potassium oxalate and 10 per cent sodium carbonate, and about 5 c.c. of toluene.
Connect the tube for aspiration as in the method for urea in blood; start the air
current, and run as fast as the apparatus wUl stand for 20 to 30 minutes. Collect
the ammonia in another test-tube containing i c.c. of water and 5 or 6 drops of
tenth-normal acid.

At the end of the aspiration Nesslerize in the usual manner (see method for non-
protein nitrogen, page 273) but more cautiously, adding in all not over i c.c. of the
previously diluted Nessler reagent (dilution 1:5). Transfer the contents of the
receiver to a 10 c.c. volumetric flask, fill to the mark with ammonia-free water, and
mix. Fill a 100 mm. polariscope tube with the mixture and close as for ordinary
polariscopic work.

Prepare two standard solutions, one containing 0.5 mg. and the other i.o mg.

of nitrogen, these being Nesslerized simultaneously with the unknown solution and

made up to volume (100 c.c). Use the standard possessing a tint most similar to

that of the unknown. Compare in a Duboscq colorimeter, using the ordinary

^ Constantino: Bioch. Zeit., 55, 419, 1913.

* Folin and Denis: J. Biol. Client., 11, 532, 1915.

^The blood must ht freshly drawn. For method of obtaining blood, see page 272.

BLOOD ANALYSIS 279

cylinder for the standard and replacing the other cylinder and prism by the polari-
scope tube, containing the unknown, which usually fits properly in place in the
colorimeter.

The unknown solution remains stationary (100 mm.) and the standard is
adjusted until the colors match. An iris diaphragm, such as is used in microscopical
work, must be attached to the side of the colorimeter holding the standard to reduce
the light passing through the standard solution. This is necessary in order to
obtain two fields of the same tint. The calculation is made in the usual manner for
colorimetric determinations, the amount of ammonia in the unknown being directly
proportional to the reading of the standard and its concentration.

7. Total Nitrogen. — The total nitrogen of the blood may be readily determined
by the regular Kjeldahl method (see Chapter XXVI). One c.c. of the blood ac-
curately measured is used in this method. The microchemical method of Folin
and Farmer, as outlined in the same chapter, may also be employed. In this case
transfer i c.c. of the well-mixed blood to a 25 c.c. flask, make to the mark with
distilled water, mix thoroughly and take i c.c. of this diluted blood for the digestion
and determination as there given.

8. Sugar, (a) Method of Lewis and Benedict. '—Principle. — The red
color obtained by heating a glucose solution with picric acid and sodium
carbonate is employed as the basis of the colorimetric determination.
The blood protein is removed by precipitation with picric acid.

Procedure. — Two c.c. of blood are aspirated through a hjrpodermic needle*
and a piece of rubber tubing into an Ostwald pipette, a little powdered potassium
oxalate in the tip of the pipette preventing clotting. The blood is drawn up a
Httle above the mark and the end of the pipette is closed with the finger. After
the rubber tubing and needle are disconnected, the blood is allowed to flow back
to the mark and is discharged at once into a 25 c.c. volumetric flask containing

5 c.c. of water. The contents of the flask are shaken to insure thorough mixing
and the consequent hemolysis of the blood. Then 15 c.c. of saturated aqueous
solution of picric acid are added, as well as a drop or two of alcohol to dispel any
foam, and the contents of the flask are made up to the mark with water and then
shaken. After filtration 8 c.c. ahquots are measiu-ed out into large Jena test-
tubes for duplicate determinations. Two c.c. of saturated picric acid solution and
exactly i c.c. of 10 per cent sodivmi carbonate are added (as well as two glass
beads and 2 or 3 drops of mineral oilj, and the contents of the tube are evaporated
rapidly over a direct flame imtil precipitation occurs. About 3 c.c. of water are
added, the tube is again heated to boiling to dissolve the precipitate, the contents
of the tube are transferred quantitatively to a 10 c.c. volumetric flask, ^ cooled,
made up to the mark, shaken, and then filtered through cotton into the chamber
of a Duboscq colorimeter (see Fig. 153, p. 486). The color is compared at once
with that obtained from 0.64 mg. of glucose, 5 c.c. of satiu-ated picric acid, and i
c.c. of 19 per cent sodium carbonate, when evaporated to precipitation over a free

1 Lewis and Benedict: Jour. Biol. Chem., 20, 61, 1915. For modilication see Myers

6 Bailey: Jour. Biol. Chem., 24, 147, 1916.

* It may be more convenient to draw about 5 c.c. of blood directly into a test-tube
containing a little finely powdered potassium oxalate and removing 2 c.c. portions of this
with the Ostwald pipette.

* In case of hyperglycemia the final volume of the reaction fluid is made 25 c.c. or 50
c.c, and the results are accordingly multiplied by 2.5 or 5.0.

28o PHYSIOLOGICAL CHEMISTRY

flame and diluted to lo c.c. as was the unknown, or against the picramic acid
standard mentioned below. ^

Calculation. — If directions are followed exactly the calculation is as follows :

reading of standard
Milligrams glucose m unknown = ,. * u X milhgrams of glucose

in standard.

(b) Pearce's Modification of Lewis-Benedict Method. ^ — ^This modification
entails the use of an autoclave instead of the free flame and has the advantages
of decreasing danger of loss and making it possible to carry out a large number
of estimations at one time. Proceed exactly as in the Lewis-Benedict, but use
6 c.c. of the the picric acid filtrate instead of 8 c.c. and instead of heating over the
free flame introduce into an autoclave for 15-30 minutes at about 20 pounds
pressure to the square inch. Compare with standard in a colorimeter. The
standard recommended by Lewis and Benedict may be diluted one-fourth or
allowed for by calculation, since 6 c.c. of filtrate are used in place of 8 c.c.

(c) Micro -method of Bang. — Principle. — Two or 3 drops of blood
are transferred to a small weighed piece of blotting paper and the
paper again weighed to determine the amount of blood. The paper
is then treated with boiling acidified KCl solution which coagulates
the protein and allows the sugar to diffuse out. The sugar solution
thus obtained is boiled with alkaline cupric chloride solution. The
amount of cuprous chloride formed by the reducing action of the
sugar is determined by titration with standard iodine solution.

Procedure. — Small pieces of good absorbent paper, about 16X28 mm. in
size,' weighing about 100 mg. and held by a small spring cUp, are used. To one
of these previously weighed* transfer 2-3 drops (about 120 mg.) of blood obtained
by piercing the cleansed finger. "Weigh again immediately and determine by
subtraction the weight of blood taken.

^ Permanent Standard. — A solution of picramic acid makes a very satisfactory permanent
standard. The color is identical in quality with that formed in the method above and its
solution keeps perfectly. The formula of the permanent standard is:

Picramic acid o . 064 gram

Sodium carbonate (anhydrous) o. 100 gram

Water to make 1000. o c.c.

Dissolve the picramic acid with the aid of heat in 25 to 50 c.c. of distilled water which
has been made alkaUne with sodium carbonate. Cool and dilute to i liter. This solu-
tion has the same intensity of color as that obtained by the proposed method with 0.64
mg. of sugar when the final volume of the reaction fluid is made 10 c.c. The solution shoidd
be standardized against pure glucose.

A satisfactory preparation of picramic acid may be obtained from the J. T. Baker
Chemical Co., Phillipsburg, N. J.

^Pearce: Jour. Biol. C/iem., 22, 525, 1915.

* Suitable pieces of paper, weighed, ready for use, and with clip attached, may be ob-
tained from Warmbrunn and Quilitz, Berlin. A suitable paper may also be obtained from
Griffin and Sons, London, or Grave of Stockholm. Unless specially prepared, the paper
should be repeatedly washed with large volumes of hot water acidified with acetic acid to
remove impurities.

* The weighing is preferably made on a special torsion micro-balance which, as well as
the other apparatus used in this method, may be obtained from either of the firms mentioned
in Note 3. The weighing must be made in a few seconds and with an accuracy of about
I mg.

BLOOD ANALYSIS 28 1

Coagulation of Blood Protein. — Transfer the piece of paper to a test-tube and
add 6.5 c.c. of boiling acid-potassium chloride solution^ and let stand half an hour.
The clear solution containing the sugar is poured into a 50 c.c. Jena flask the
flange of which has been removed. Wash the paper and tube again with 6.5 c.c.
of hot salt solution and transfer washings to the flask. Cool.

Reduction of Cupric Chloride. ^ — Attach to the mouth of the flask a piece of
tight-fitting rubber tubing about 2 inches long (see Fig. 81 j, provided with a
clamp which permits of shutting off the contents of the flask from the outside air.
Now add to the flask i c.c. of the cupric chloride solution. ^ Heat so that the
solution is brought to a boil in one minute and 30 seconds ''an error of five seconds
may be disregarded). Allow to boil for exactly two minutes; at the end of this
time tighten the clamp over the mouth of the flask. At the
same time remove from the flame and cool at once under the
tap for about a minute.

Titration of Cuprous Chloride Formed. — The titration is
made with N/200 iodine solution^ run in from a very accurate
burette (preferably a 2 c.c. burette graduated in 1/50 c.c).
Two or 3 drops of starch solution (preferably soluble starch^;
are added as an indicator. During the titration air must be
excluded to prevent re-oxidation. This is done by running a
slow stream of carbon dioxide from a generating bottle through
a small tube which extends nearly to the bottom of the flask.
The titration should be carried out against a white backgrovmd
and the end point taken when the blue color persists for 20-30 Baxg Rzduc-
seconds. tion Flask.

Calculation. — The copper and other solutions used in the
test bind about 0.12 c.c. of the iodine solution. This amount must hence be
subtracted from the reading. The corrected reading is then divided by 4 to
obtain the number of milligrams of glucose in the sample.

Example. — If 0.68 c.c. of N/200 I solution were required, * ' — = 0.14

4
mg. glucose in the amount of blood used. If 140 mg. of blood were taken for

analysis the per cent of glucose in the blood would be X0.14 mg. = 0.1 per

140

cent glucose.

The results obtained by this method are a httle higher than those obtained
by other reUable methods due to the presence of certain I-bindLng substances in
blood. As these appear to be nearly constant in amount a correction may be
appUed. To obtain true values for glucose of the blood therefore subtract
0.015 per cent from the value obtained as above, o.i per cent — 0.015 per cent
= 0.085 per cent glucose.

^ Consisting of 1360 c.c. of saturated KCl to which is added 640 c.c. of water and 1.5
c.c. of 25 per cent HCL.

* Copper solution. Introduce into a 1000 c.c. flask 700 c.c. of boiled and cooled water.
Warm to about 3o°C. and add i6o grams of pure potassium bicarbonate in powder form.
When dissolved add 66 grams of pure KCl. Cool and then add 100 grams potassium car-
bonate. Finally add 100 c.c. of 4.4 per cent solution of pure crystalline copper sulphate.
Let stand a short time, then make to mark with boiled water. Allow to stand a day or so
before using.

* N/200 I solution, made fresh each day. DUute N/io I solution 20 times, or
make as follows: Introduce into a 100 c.c. flask 2 grams KI, 1-2 c.c. of 2 per cent KIOj
solution and 5 c.c. of N/io HCl. Make to mark with boiled and cooled distilled water.

* A I per cent solution of Kahlbaum's soluble starch in a saturated KCl solution.

252 PHYSIOLOGICAL CHEMISTRY

To secure accurate results the method of Bang must be rigidly con-
trolled, all new solutions and absorbent papers being checked up
against pure 0.2 per cent glucose solutions. Taylor and Hulton^
also suggest the following precautions. A blank check must be made
on the reagents each day an estimation is made. 0.10-0.15 gram of
blood should be taken and must spread smoothly on the paper. The
proteins are best coagulated by heating of the blood-impregnated
papers in the hot air oven at 100° (as recommended by Gardner and
McLean)- for five minutes with corks of flasks inverted. The solu-
tion should be boiled four minutes for complete reduction. The
iodine solution must be fresh each day and checked each day. Deter-
minations should be made in triplicate. Results cannot be depended
upon to be more accurate than to 0.005 gram glucose in 100 c.c. blood.
Other authors have recommended that an hour instead of half an hour
be allowed for the diffusion of the blood sugar, the fluid being brought
to the boiling-point twice during this period or kept in a bath at 4o°C.

Method of Epstein. 2 — Principle. — This method is a modification of the Lewis
and Benedict procedure, being based on the same principle but making possible the
determination of reducing sugar in finger blood (0.1-0.2 c.c.) with a sufficient
degree of accuracy for clinical purposes, and with little expenditure of time. In-
stead of a Duboscq colorimeter the less expensive Sahli-Gower hemoglobin color-
imeter is recommended.

Procedure. — The apparatus* shown in the illustration (Fig. 82) and the fol-
lowing reagents are necessary:

1. Picric acid, saturated solution.

2. Sodium carbonate, 10 per cent solution.

3. Sodium fluorid or potassium oxalate, 2 per cent solution.

Put one or two drops of the fluorid or oxalate solution into the graduated test-
tube (see illustration). By means of the blood pipette, 3, 0.2 c.c. of blood is
obtained from the tip of the finger or the lobe of the ear and is discharged into the
tube containing the fluorid solution. The pipette is rinsed two or three times
with distilled water and the washings added to the blood in the tube. Distilled
water is then added to the i.o c.c. mark. After laking of the blood has taken place,
picric acid is added to this (a few drops at a time) up to the 2.5 c.c. mark, shaking
the tube gently with each addition of the acid. Precipitation of the blood-proteins
takes place; the sugar, together with an excess of picric acid sufficient for the

^Taylor and Hulton: Jour. Biol. Chem., 22, 63, 1915.

2 Gardner and McLean: Biochem. J., 8, 391, 1914.

^ Epstein: /. Am. Med. Assn., 63, 1667, 1914.

* The tubes belonging to this hemoglobinometer are not all equally calibrated. With
some the 50 per cent mark represents a volume of i.o c.c; with others, i.o c.c. of fluid
reaches up to the 43, 45, 46 or 47 per cent mark. The error in the caUbration is generally
below the 10 per cent mark; the graduations above this mark are usually correct. By
means of the standard 1.0 c.c. pipette one can readily determine whether or not a given
tube is properly calibrated. In order to facilitate a direct reading of the percentage
of sugar on these hemoglobinometer tubes, it is essential to have 1.0 c.c. of fluid stand at
mark 50. To overcome a discrepancy (if any exists) in the calibration of a given tube,
one may put one, two or three small glass beads in the bottom of the tube, of such size
as to raise the meniscus of 1.0 c.c. of fluid up to the 50 per cent mark.

BLOOD ANALYSIS

283

reaction, stays in solution. The tube is finally shaken vigorously (covering the
end of the tube with the finger) and the contents filtered through a small filter, or,
better still, centrifuged for one or two minutes.

One c.c. of the filtrate or the clear supernatant fluid obtained on centrifugal-
ization is withdrawn, put into the plain test-tube, and heated carefully over the
naked flame. The contents of the tube are boiled until all but 2 or 3 drops of the
solution is evaporated. One-half c.c. of the 10 per cent sodium carbonate solution
is then added and the tube heated again until the contents are concentrated to
a small volume equal to about 2 or 3 drops. The color of the fluid changes from
yellow to deep red or reddish brown and the reaction is completed.

Three or 4 drops of distilled water are added and the tube warmed gently. The
contents are then transferred to the graduated tube of the hemoglobinometer.
The boiling tube is rinsed several times with water (using ordy 3 or 4 drops at a
time). The tube is warmed with each rinsing before transferring the contents to
the graduated tube. The volume of fluid is then made up to the mark 50 on the
scale.

Fig. S2. — App.\r.a.tus for Epstein's Sugar Method.

The color of the resulting solution is compared with that of the two standard
tubes, A and B which accompany the instrument. (A solution of picramic acid
of the proper strength, prepared as described on p. 280, may be used as a standard.)
If it is darker than standard A (representing 0.05 per cent of sugar) and lighter
than standard B (representing o.i per cent), the first standard is used for com-
parison. In either case the solution in the graduated tube is diluted gradually
with water (just as is usually done in hemoglobin estimations) untU the colors
match.

The percentage of sugar in the blood is then computed thus: Using the lighter
standard A the figure on the scale, divided by 1000 represents the percentage of
sugar in the blood. For example, the tube reads 86; then the result is

86

=0.086 per cent

1000

When Standard B is used for comparison, the figure on the scale is multiplied
by 2 and divided by 1000. For example, the tube reads 73; then the percentage
of sugar is

73X2
1000

■0.146 per cent

284 PHYSIOLOGICAL CHEMISTRY

With the instructions given, the above formulas may be used for direct com-
putation of the percentage of sugar only, when 0.2 c.c. of blood is used in the
determination. When, however, only o.i c.c. of blood is used, the formulas apply
as well, but the value obtained must be multiplied by 2.

It is better, in cases in which a high sugar content in the blood is suspected (in
diabetes for example) to use only o.i c.c. of blood for the determination. In all
other cases 0.2 c.c. of blood should be used.

8. Acetone Bodies^ (Acetone, Diacetic Acid and /3-Hydroxybutyric Acid). —
Marriott-Scott-Wilson Method. ^^ — (a) Acetone and Diacetic Acid. — Draw 10 c.c.
of blood from a superficial vein by a sterile graduated syringe and run it into about
40 c.c. of 0.5 per cent potassium oxalate solution. Fit up a Kjeldahl distillation
apparatus using an 800 c.c. flask, provided with a dropping funnel, the delivery
tube of the condenser dipping beneath the surface of the water in a receiving
flask. Introduce into the Kjeldahl flask 100 c.c. of water and i c.c. of glacial
acetic acid. Bring the acidified water to a boil and then run the diluted blood
in slowly through the dropping funnel.

Boil for 30 minutes after the last blood is run in. ' To the distillate add a little
dilute sulphuric acid and redistil. To this distillate add 20 c.c. of hydrogen
peroxide solution and a sUght excess of alkali and redistil again. The final dis-
tillate is caught in small Erlenmeyer flasks containing an excess of the Scott-
Wilson "acetone reagent" which has been recently filtered.* The delivery tube
must dip under the surface of the liquid. It is not necessary to distil more than
10 minutes to get off all the acetone. Allow to stand for 10-15 minutes. Filter
through an asbestos mat^ in a separable bottom Gooch crucible. Clear filtrates
are more readily obtained if the pores of the filter have been partly closed by
filtering through it a suspension of talcum powder in water. If the first portions
of the filtrate are turbid, refilter. Wash the precipitate with cold water until
the washings are free from silver.

With the aid of a pointed hooked glass rod transfer the precipitate, mat and
crucible bottom to a 50 c.c. beaker, any adhering particles of precipitate being
washed into the beaker with the aid of about 10 c.c. of "acid mixture."® Add
I c.c. of N/5 potassium permanganate, cover the beaker with a watch glass and
boil until the liqiud is colorless. Add more permanganate, a few drops at a time,
until a persistent brown color is obtained which does not disappear on boiling for a
couple of minutes. The brown color is then discharged by the addition of a few
drops of strong yellow nitric acid. The greater the amount of acetone present
the more permanganate is required, and it is essential to the accuracy of the
method that an excess be added as indicated above, otherwise the residts are
too low.

Cool the beaker under the tap, add 2 c.c. of saturated ferric alum solution,

' For nephelometric method see p. 294.

* Scott- Wilson: Jour, of Physiol.. 42, 444, 1911.
Marriott: Jour. Biol. Client., 16, 295, 1913.

3 If /3-oxybutyric acid is to be determined the residue in the Kjeldahl flask should be
kept and treated as outlined in the latter part of this procedure.

^ The reagent is made up as follows: Mercuric cyanide, 10 grams; sodium hydroxide,
180 grams; water, 1200 c.c. The solution is agitated in a flask and 400 c.c. of a 0.7268
per cent solution of silver nitrate slowly run in. At least 30 c.c. of the reagent must be
taken for each milligram of acetone present.

* Filter paper cannot be used as the strong alkali quickly attacks it.

* "Acid mixture:" Nitric acid 40 parts; sulphuric acid, 5 parts; water 55 parts.

BLOOD ANALYSIS 285

and run in from a burette a standard solution of potassium sulphocyanate (approxi-
mately 0.1 per cent) ^ until a very faint pinkish-brown color is obtained throughout
the solution. The end point which consists in the faintest trace of color, can be
detected only when the titration is performed on a pure white surface. A con-
trol beaker with i drop excess of sulphocyanate should be on hand for compari-
son. A whole cubic centimeter of sulphocyanate may be run in after the end
point is reached without very greatly darkening the shade.

Calculation. — By this procedure acetone preformed and from diacetic acid
are determined together. The amount of acetone and diacetic acid combined,
in terms of acetone, may then be calculated by multiplying the nimiber of cubic
centimeters of the KSCN solution used by the equivalent of i c.c. of this solution
in acetone as determined by standardization. ^ To obtain the amount of acetone
and diacetic acid in 100 c.c. of blood the result must of course be multipUed by 10.

(b) Determination of /3-Hydroxybutyric Acid. — The residue in the Kjeldahl
flask from the above determination is used in the determination of ^-hydroxy-
butyric acid. While still hot, precipitate it with about 8 c.c. of 10 per cent sodium
carbonate, boil a moment, filter on a Biichner fuimel and wash with hot water.
To the clear filtrate add 15 c.c. of basic lead acetate (U.S.P.) and 10 c.c. of strong
ammonia and make to definite volvmie (150 c.c.) with water. Allow the precipi-
tate to settle and then filter off on a dry, folded filter. Take an aUquot of the
clear filtrate (about 125 c.c.) and boil it to expel the greater part of the ammonia.
Cool and add dilute sulphuric acid to precipitate the excess of lead as sulphate
and filter. Add 10 c.c. of 50 per cent sulphuric acid and transfer the whole to a
Kjeldahl flask provided with a dropping funnel. The contents of the flask are
distilled and a solution of potassium bichromate is run in from the dropping funnel
at such a rate that the liquid always retains some yellow color and the volimie
remains at about 100 c.c. It is rarely necessary to add more than about o.i gram
of bichromate and an excess is to be avoided. Slow distUlation is continued for
two hours and about 100 c.c. of distillate is collected. The tip of the deUvery tube
must always remain under the surface of the water in the receiving flask. Add
20 c.c. of hydrogen peroxide, make sUghtly alkaline with NaOH and distil again.
Catch the distillate in small Erlenmeyer flasks containing an excess of the Scott-
Wilson acetone reagent (at least 30 c.c. for each milligram of acetone) and de-
termine the acetone according to the procedure outlined in the preceding method
for acetone and diacetic acid. Calculate the /3-hydroxybutyric acid in terms of
acetone and express as miUigrams of acetone per 100 c.c. of blood.

9. Cholesterol. Method of Autenrieth and Funk} — Principle. —
The blood or serum is boiled with strong alkali to saponify the fats.
The alkaline solution is extracted with chloroform. The chloroform
is dried and clarified by means of anhydrous sodium sulphate and
filtration and then treated with sulphuric acid and acetic anhydride,
and the characteristic color reaction of the Liebermann-Burchard test

' The sulphocj^anate solution should be standardized against pure acetone treated
in the same manner as ihe final tlistillate above. According to Scott-Wilson it may also
be standardized against a pure solution of mercuric nitrate and the equivalent of i c.c. of
the KSCN solution in milligrams of Hg determined. According to this author i mg. of Hg
is equivalent to 0.058 mg. of acetone.

^Autenrieth and Funk: Miinch. mcd. Woch.,()o, 1243, 1913. A slight modification
has been suggested by Bloor {Jour. Biol. Chem., 23, 317, 1915).

286 PHYSIOLOGICAL CHEMISTRY

for cholesterol obtained. The color is compared with a standard in a
colorimeter.

Procedure. — ^With an accurate pipette transfer 2 c.c. of whole blood or serum
to a 100 c.c. Erlenmeyer flask, and add 20 c.c. of a 25 per cent potassium hydroxide
solution. Heat on the water-bath for two hoiirs shaking frequently and adding a
Uttle water if necessary to keep from going to dryness. Pour the undiluted
mixture into a separatory fixnnel and add 25-30 c.c. of chloroform. Shake
vigorously for five minutes and separate. Shake out with four more portions of
20 c.c. each of chloroform. The combined chloroform extracts are turbid and
of a green or brown color and are clarified by shaking with 5-10 grams of anhy-
drous sodium sulphate and filtering. Dilute the filtrate to 100 c.c. with chloroform.
Transfer 5 c.c. of this extract to a small glass-stoppered bottle of about 10 c.c.
capacity, add 2 c.c. of acetic anhydride and o.i c.c. of concentrated sulphuric acid
and shake. Place in a water-bath at 32-35°C. and keep in the dark 15 minutes.
A green color is developed. At the same time a series of standards are prepared
and treated in the same maimer. The color of the test is compared with that
of the most similar standard in a colorimeter (see Fig. 153, p. 486) and its color
strength determined.

Five standards are kept, these being prepared by dissolving in 100 c.c. por-
tions of chloroform: (i) 3.2; (2) 4.8; (3) 6.4; (4) 8.0; (5) 9.6 mg., respectively of
piire cholesterol. In preparing the standards for comparison 5 c.c. portions of
each of the above solutions are taken, placed in small glass-stoppered bottles
and treated as were the unknowns. Each standard then represents a concen-
tration of: 160 mg. ; 240 mg. ; 320 mg. ; 400 mg. ; and 480 mg. respectively of
cholesterol in 100 c.c. of the original blood or sermn.

10. Chlorides. — Method of McLean and Van Slyke.^ — The determination re-
quires two steps: (i) removal of proteins and (2) titration of chlorides.

Coagulation of Proteins. — Removal of the proteins may be accomplished in two
ways, by coagulation or by ignition. Results are identical by both methods, but
coagulation is the simpler. For coagulation 2 c.c. of oxalated plasma (i c.c. may
be used if material is limited) are drawn into a 2 c.c. pipette which has been cali-
brated to contain 2 + 0.005 c.c. From the pipette the plasma is run into a 20 c.c.
stoppered volumetric flask which contains 10 c.c. of a 10 per cent magnesium sul-
phate solution. The pipette is rinsed twice by drawing up into it the solution from
the flask. Two drops of 50 per cent acetic acid are added, the flask is filled to the
mark with water, the contents are mixed by inverting the flask, and heated in a
bath to 100° for ten minutes. By keeping the stopper loosely in place evaporation
is prevented, and when cool the contents return to their original volume. Ten
minutes on the steam bath are sufiicient to coagulate the albumin and to distribute
the chlorides evenly between the fluid and precipitated albumin. The flask is then
allowed to cool, and the contents are poured upon about 0.3 gram of blood char-
coal^ in a small beaker, and mixed. After a few minutes the liquid is filtered
through a dry folded filter, and a water-clear filtrate obtained.

Titration of the Protein-free Filtrate. — In brief, the chlorides are precipitated in
the presence of nitric acid by standard silver nitrate solution, the silver chloride is
removed by filtration, and the excess silver titrated with standard potassium

^ McLean and Van Slyke: Jour. Biol. Chem., 21, 361, 1915.

^Merck's "Blood Charcoal Reagent," purified by acid and freefr cm chloride, is used.
No other form of charcoal has been found to be of serv'ice.

BLOOD ANALYSIS 287

iodide.' The titration is performed in the presence of nitrous acid and starch, so
that the first drop of iodide in excess of the silver present is changed to free iodine
and gives the blue starch-iodine color. The optimum acidity for the end point is
fixed by the addition of trisodium citrate in amount equivalent (J^ mol.) to the
free nitric acid present. Under these conditions i drop of excess N/50 iodide
gives a color preceptible in 150 c.c. of solution.

In detail, the titration of the protein-free plasma filtrate is carried out as
follows: Either 10 c.c. of the filtrate, containing the chlorides of i c.c. of plasma,
are taken in a pipette for titration or the filtrate is collected directly in a certified
25 c.c. graduated cylinder, where it is measured, so that the entire amount may
be taken for titration. In this way 13 to 14 c.c. of filtrate, corresponding to 1.3
to 1.4 c.c. of plasma, may be obtained for titration.

After either measuring 10 c.c. of the filtrate into a 25 c.c. volumetric flask or
recording the amount of filtrate obtained in the cylinder, 5 c.c. of the acidified
Af/29.25 silver nitrate solution (Solution I) are added, and the whole is made to the
25 c.c. mark with water. This will precipitate up to 10 mg. of XaCl. In samples
with high percentage of chloride, only enough filtrate is taken to keep within this
limit of ID mg. Two drops of octyl (caprylic) alcohol are added, and the vessel is
stoppered and shaken gently by inverting it several times. Immediate coagulation
of the silver chloride occurs. After allowing five minutes for complete precipitation
to occur, the solution is filtered through a dry folded filter, and a perfectly clear and
colorless fiJtrate again obtained. An aliquot part of the filtrate (20 c.c.) is now
taken with a pipette for titration.

Just before titration with the potassium iodide solution (Solution II) one adds
a volume of the citrate solution (Solution III) equal to the volume of Solution I
represented in the filtrate to be titrated. If, as is usually the case, one has used
5 c.c. of Solution I diluted to 25 c.c, and taken 20 c.c. of the filtrate for titration
one has the equivalent of 4 c.c. of Solution I present, and must accordingly add

^ The following solutions are required;

I. An acid Af/29.25 solution of silver nitrate, i c.c. of which is equivalent to 2 mg. of
NaCL.

AgNOs 5.812 grams

HNO3 (sp. gr. 1.42) 250 c.c.

Water to 1000 c.c.

II. A solution of ilf/58.5 potassium iodide, i c.c. of which is equivalent to i mg. of
NaCL.

KI 3.0 grams

Water to 1000 c.c.

This solution is standardized against the silver solution by adding 5 c.c. of the latter
to 5 c.c. of Solution III, and titrating with the iodide solution to the blue end-point. The
iodide solution is then diluted to such a degree that 10 c.c. are exactly equivalent to 5 c.c.
of the silver solution.

III. A solution, for use in the final titration, containing sodium citrate, sodium nitrate,
and starch, which substances respectively regulate the acidity, provide an o.xidizing agent
for the iodide, and serve as indicator.

Sodium citrate (NasCsHeOT+S 1/2H2O) 446 grams

Sodium nitrite 20 grams

Soluble starch 2.5 grams

Water to looo c.c.

The starch is first dissolved with the aid of hoat in about 500 c.c. of water. The citrate
and nitrite are then added, and the mixture is heated until all is dissolved. The solution,
while still hot is filtered through cotton, the filter washed with hot water, the tiltrate
allowed to cool, and made up to 1000 c.c. Filtration removes insoluble substances occur-
ring chiefly in the nitrite, and cotton filters more rapidly than filter paper. The solution
keeps indefinitely. It becomes cloudy on standing, but its efficacy is not impaired.

288 PHYSIOLOGICAL CHEMISTRY

4 c.c. of Solution III. On adding Solution III a slight turbidity appears, which in
no way interferes with the end point.

The potassium iodide solution is then run in from a burette until the blue end
point appears. The first definite blue color is taken as the end point, and with
slight practice is unmistakable. An additional drop, which may be used as a control,
causes such a deep blue color that it is impossible to make an error of more than one
drop in titration. Should the end point be accidentally passed, one may add i c.c.
of Solution I, I c.c. of Solution III and retitrate, allowing in the calculation for the
extra sUver nitrate.

The result may be calculated from the following formula, which applies only
when 20 c.c. of the filtrate from silver chloride are titrated:

^ ^^ ^, ,. 12.5 (8 — c.c. KI solution used)

Grams NaCl per liter = r^ — t~zti — I — ^~^ '

*^ c.c. blood filtrate taken

Thus, if 13 c.c. of filtrate are obtained and titrated after precipitation of plasma
protein, and 1.60 c.c. of KI are used in the final titration,

n -KT ^^ r. ^^-SCS - 1.60)
Grams JNaCl per liter = = 6. 1=5.

In case only i c.c. of plasma instead of 2 c.c. has been used, the factor 25 replaces
12.5 in the numerator. The error should be within a limit of i per cent.^

II. Total Solids. — The total solids of the blood are most readily determined by
using a type of weighing bottle differing from the usual form merely in having a
glass loop attached to the under side of the stopper. ^ A block of filter paper is
suspended from this loop by means of a small wire hook. The bottle and filter
block are dried and weighed. From a small pipette 0.3-0.6 gram of the well-mixed
blood is allowed to flow rapidly upon the filter block. The stopper is quickly
inserted and the bottle weighed. The stopper is then tilted and the bottle placed
in the drying oven at 105° over night. When convenient the bottle is cooled and
again weighed. The total solids are calculated from the loss of moisture.

12. Relative Hydrogen Ion Concentration of the Blood. Method
of Levy, Rowntree, and Marriott.^ — Principle. — The blood is dialyzed
against normal salt solution and the H ion concentration of the protein-
free dialyzate is determined by the indicator method, using phenol-
sulphonephthalein.

Procedure. — One to 3 c.c. of clear serum or of blood is run, by means of a
blunt-pointed pipette, into a dialyzing sac* which has been washed outside and

1 The exactness of the method depends directly on the care with which measurements
are made and on the purity of the reagents used. All reagents must, of course, be free
from substances precipitated by silver, and are easily tested. As the volumes measured
are not large, however, small absolute errors in measurement may cause considerable
percentage error in the final result. All glassware must therefore be carefully calibrated
by either the weight of water contained (flasks, cylinders, 2 c.c. pipettes) or the weight de-
livered (other pipettes, burettes), and burettes should be used which are capable of being
read to 0.02 c.c. and which deliver small drops. If these precautions are followed, one
should uniformly obtain results, which are weU within a limit of error of i per cent.

^ Myers and Fine: "Chemical Composition of the Blood in Health and Disease,"
191 5. The weighing bottles may be obtained from Eimer and Amend, N. Y.

^Levy, Rowntree and Marriott, Arch. Int. Med., 16, 389, 1915.

* Preparation of Sacs. — One ounce of celloidin is dissolved in 500 c.c. of a mixture of
equal quantities of ether and ethyl alcohol. The solids swells up and disolves with oc-

BLOOD ANALYSIS

289

inside with salt solution.' The sac is lowered into a small test-tube fiooXio
mm., inside measurements), containing 3 c.c. of salt solution, until the fluid on the
outside of the sac is as high as on the inside. From 5-10 minutes are allowed for
dialysis. The collodion sac is removed and 5 drops of the indicator (o.oi per
cent solution of phenolsulphonephthalein ) are thoroughly mixed with the dialyzate.
The tube is then compared with the standards- until the corresponding color is
found, which indicates the hydrogen ion concentration present in the dialyzate.
Readings should be made immediately against a white background. Results
are expressed in logarithmic notation.

Oxalated blood from normal individuals gives a dialyzate with a Ph varying
from 7.4 to 7.6, while that of serum ranges from 7.6 to 7.8. In cUnical acidosis fig-
ures from 7.55 to 7.2 have been noted by this method for serum and for oxalated
blood from 7.3 to 7.1. A rise in the H ion concentration of the blood is significant
because it indicates a failure on the part of the protective mechanism of the body
to preserve the proper reaction.

casional gentle shakings, in 48 hours. As a small amount of brown sediment separates
out at first, the solution should stand for at least three or four days, after which the clear
supernatant solution is ready for use. A small test-tube (120 by 9 mm., inside measure-
ment) is filled with this mi.xture, inverted, and half the contents poured out. The tube is
then righted, and the collodion allowed to fill the lower half again. A second time it is
inverted and rotated on its axis, the collodion being drained off. Care must be taken to
rotate the tube, in order to secure a uniform thickness throughout. The tube is clamped
in the inverted position and allowed to stand for ten minutes, until the odor of ether finally
disappears. It is filled five or si.x times with cold water, or it is allowed to soak five minutes
in cold water. A knife blade is run around the upper rim, so as to loosen the sac from the
rim of the test-tube, and a few cubic centimeters of water are run down between the sac
and the glass tube. By gentle pulling the tube is e.xtracted, after which it is preserved by
complete immersion in water.

^ The Salt Solution. — The blood or serum is dialyzed against an 0.8 per cent sodium
chloride solution.

Before applying the test, it is necessary to ascertain that the solution is free from acids
other than carbonic. To determine this, a few cubic centimeters of the salt solution are
placed in a Jena test-tube and i or 2 drops of the indicator added, whereupon a yellow color
appears. On boiling, carbon dio.xide is e.xpelled, and the solution loses its lemon color
and takes on a slightly brownish tint. In the absence of this change other acids are
present, and the salt solution is therefore not suitable. If, on the other hand, on adding
the indicator pink at once appears, the solution is alkaline and hence cannot be used.

- Preparation of Standard Colors. — Standard phosphate mi.xtures are prepared according
to Sorensen's directions as follows:

J^5 mol. acid or primary potassium phosphate. 9.07S grams of the pure recrj-stallized
salt (KH2PO4) is dissolved in freshly distilled water and made up to i liter.

Hs mol. alkaline or secondary sodium phosphate. The pure recrystallized salt
(Xa2HP04.i2HoO) is exposed to the air for from ten days to two weeks, protected from
dust. Ten molecules of water of crystallization are given off and a salt of the formula
Na3HP04.2H20 is obtained. 11.876 grams of this is dissolved in freshly distilled water
and made up to i liter. The solution should give a deep rose-red color with phenol-
phthalein. If only a faint pink color is obtained, the salt is not sufficiently pure.

The solutions are mixed in the proportions indicated below to obtain the desired Pii.

TABLE FOR PREPARATION OF STANDARD COLORS

Ph

6.46.6

6.87.0I7.1

7.2

7-3

7.4

7-5

7.6

7-7

7.81 8.0

8.2

8.4

Primary potassium
phosphate c.c

73

63

51 37 32

27

23

19

IS. 8

13-2

II. 0

8.8; 5-6

3.2

2.0

Secondary sodium
phosphate c.c. .....

27

37

49 63 68

73

77

81

84.2

86.8

89.091.2 94.4

96.8

98.0

19

290 PHYSIOLOGICAL CHEMISTRY

13. The Determination of Epinephrin (Adrenalin) in the Adrenal
Glands.^ — Principle. — It has not yet been found possible to determine
adrenalin in the blood by chemical methods. In the adrenals it may be
determined by the method given below.

The method is based upon the quantitative production of blue
color when a solution of adrenalin is treated with phosphotungstic
acid. Uric acid and other substances likewise give the reaction but
can be disregarded when the determination is made upon adrenal
glands.

Procedvire. — Rub the weighed gland thoroughly in a mortar with fine sand
and N/io hydrochloric acid. The mixture is then rinsed into an Erlenmeyer
flask with more N/io acid and water, using in all about 15 c.c. of the acid for each
2 grams of gland and about three times as much water. Heat to boiling to dis-
solve the epinephrine. Then add 5 c.c. of 10 per cent sodium acetate solution for
each 15 c.c. of hydrochloric acid present and heat again to boiling. Transfer
the whole mixture (except the sand) to a volumetric flask (capacity 100 c.c. for
each 2 grams of gland) and make to mark with water. Filter. Pipette 5 c.c. of
the clear extract into a 100 c.c. measuring flask and i c.c. of a fresh uric acid
solution containing i mg. of uric acid into another 100 c.c. flask. To each flask
add 2 c.c. of uric acid reagent (see Folin and Denis' method for uric acid,
page 274) and 20 c.c. of saturated sodiiom carbonate solution. Allow to stand
for two to three minutes, dilute to the mark, shake thoroughly, and compare
in the usual maimer in a Duboscq colorimeter with the uric acid standard set
at 20 mm. Calculate as if the solution contained uric acid, and divide the
result by three to obtain the equivalent in epinephrine which gives three times as
much color as an equal weight of uric acid.

Nephelometric Methods

The Nephelometer. — The nephelometer is an instrument for
measuring the density of precipitates and thus determining the amount
of any substance which can be obtained in the form of a suitable
suspension. It is somewhat similar in form and principle to a color-
imeter. It differs from the latter in that the light which reaches the
eye is not transmitted light, which, on the contrary, is excluded, but
light reflected from the particles of the suspension. The brightness
of the two fields is compared instead of their colors. It is adapted
particularly for the determination of substances that in very dilute
solution may be precipitated in the form of suspensions which do not
agglutinate appreciably in the time required for making readings
(10-20 minutes). The method has been adapted to the determination
of proteins in digestion mixtures, milk, urine, etc.;^ nucleic acids ;^

1 Folin, Cannon, and Denis: Jour. Biol. Chem., 13, 477, 1913.

'^ Kober: Jotir. Biol. Chem., 13, 485, 1913; Jour. Am. Ch. Soc, 35, 1585, 1913; Folin
and Denis: Jour. Biol. Chem., 18, 273, 1914.

2 Kober and Graves: Jour. Am. Chem. Soc, 36, 1304, 1914.

BLOOD ANALYSIS

291

chlorides/ phosphates, and phosphatides in blood, etc.;- fats in milk,
blood, etc.;^ acetone bodies in urine and blood ;^ uric acid and purine
bases ;^ ammonia;^ calcium;^ silver, etc., and is continually finding
new applications. It is possible to determine very minute amounts
of substances, entirely outside of the range of gravimetric methods of
analysis, and hence the procedure may be used where the amount of
material is very limited. If properly carried out the limits of error
of the method are not greater than those
of the colorimetric methods commonly
used. Below will be found descriptions
of and figures representing two satisfac-
tory types of nephelometer.

The Duboscq colorimeter has been
adapted for nephelometric purposes by
Kober^ and by Bloor.^ Bloor's nephelom-
eter is illustrated in Figs. 83 and 84. The
brass plate carrying the colorimeter
plungers is replaced by the plate A with
two slots in which are supported the
nephelometer tubes B with their flanges
resting on the edges of the slots. The slots
are so cut that the center fines of the tubes
are exactly in line with the centers of the
lower openings of the prism case E. If

desired they may be countersunk to re- fig.Ss-bI^ok'sNep^lometer.
ceive the flanges. The colorimeter cups

are replaced by the jackets C which project through the holes in the
cup supports F and are supported on them by the collars D. They
move when the cup supports move. The mirror is turned to the
horizontal position so that it reflects no light. The fight in the nephe-
lometer comes from in front and not from below (see Fig. 84). The
nephelometer tubes are small test-tubes 100X15 mm., preferably
made from the same sample of colorless glass tubing so that they are
of exactly the same bore. The flanges at the top should be well made
so that the tubes rest firmly and evenly in the slots. The glass should

' Richards: Zeilschr. f. anorg. CItem., 7, 269, 1895.

- Greenwald: Jour. Biol. Cliem., 21, 29, 1915; Bloor: Jour. Biol. Chem., 22, 133, 1915;

Kober and Egerer: Jour. Am. Chem. Sac, 37, 2373, 1915.
^ Bloor: Jour. Biol. Client., 17, 377, 1914; /. Am. Chem. Soc, 36, 1300, 1914.
■• Folin and Denis: Jour. Biol. Chem., 18, 263, 1914; Marriott: same, 16, 289, 1913.

* Graves and Kober: Jour. Avi. Chem. Soc, 37, 2430, 1915.
" Graves: /. Am-. Chem. Soc., 37, 1181, 1915.

'Lyman: Jour. Biol. Chem., 21, 551, 1915.

* Kober: Jour. Biol. Chem., 13, 485, 1913; Jour. Am. Chem. Soc., 35, 15S5, 1913.
8 Bloor: Jour. Biol. Chem., 22, 145, 1915.

292

PHYSIOLOGICAL CHEMISTRY

be as free as possible from imperfections and striations. After the
tubes are made and fitted into place the jackets are moved up on
each tube by means of the rack and pinion until the indicator on the
scale is exactly at zero. Marks are made on each tube at the point
reached by the top of the jacket and the portion of the tube above that
point is made opaque by a ring Bl of black paper or paint. Tubes
and jackets are then marked right and left and always used on the
same side. Since it is rare to find two tubes which when filled with the
same solution give exactly the same readings it is necessary to take this
fact into account and correct accordingly.

The jackets C are made of tubing (metal or glass) a little larger
than the tubes and about the same length (they should clear the
mirror when it is turned horizontal), closed at the bottom and made

Path of Light

Partition

Curtain

Fig. 84. — Nephelometer in Position, Showing Relation to Source of Light.

light tight by black paint or paper. The collars D supporting the
jackets may be made of cork or more permanently of metal. A little
cotton wool in the bottom of the jackets will prevent breakage if the
tubes should fall into the jackets.

The openings in the prism case, particularly the lower ones, should
be protected against accidental splashing by thin glass plates (thick
cover slips) which are held in place by a little glue.

Artificial light is necessary and the lamp should be enclosed in
a tight box into one end of which the nephelometer fits snugly. A
partition extending part way up the box as shown in the diagram
(Fig. 84) serves the double purpose of shutting off the light from
the lower part of the instrument and of providing a stop against
which the instrument is pushed, so that its distance from the light

BLOOD ANALYSIS

293

is kept constant. The box is conveniently made without a bottom
and the end closed with a dark curtain after the nephelometer is
pushed into place. The inside of the box should be painted black.
A dark room is desirable but not necessary, as the instrument may
be used satisfactorily in a room darkened by a dark shade or even in a
dark corner of the laboratory.

The relations of the nephelometer and the light source may be
seen in the diagram, Fig. 84. The lamp used is an ordinary 50-
watt tungsten ("Mazda") supported by a bracket about 30 cm. from
the nephelometer and at the height of the nephelometer tubes. The
change from one instrument to the other can be made in one or two

Fig. 85. — Lenzmaxn-Kober Nephelometer.

minutes, since it consists essentially only in unscrewing the brass
plate carrying the plungers and screwing on the plate to carry the
nephelometer tubes. The extra parts needed, plate, tubes, and
jackets, are few and can be made if necessary from material at hand
in any laboratory and by anyone with a sUght degree of mechanical
skill. 1

The above description applies t)nly to the later type of colorime-
ter where the cups move and the prisms are stationary. The changes
required to convert the older type of instrument are more complicated
and scarcely to be advised unless the instrument is to have fairly

* The extra parts necessary for the conversion of the colorimeter into the nephelometer
may be obtained from the International Instrument Co. of Cambridge, Mass.

294 PHYSIOLOGICAL CHEMISTRY

continuous use as a nephelometer. If the change is desired the nephe-
lometer tubes are to be supported in the same way as above, but the
jackets must be carried on special brackets which are made to replace
the brackets carrying the plungers. The nephelometer tubes must be
stationary, the jackets being the movable parts.

Kober has devised^ a combined colorimeter and nephelometer less
expensive than the Duboscq apparatus and which may be obtained
in this country.^ A diagram illustrating the construction of this
Lenzmann-Kober nephelometer is given in Fig. 85, page 293.

Nephelometric Calculations. — The amounts of precipitate in solu-
tions examined nephelometrically is not exactly inversely proportional
to the readings of the scale. When the concentration of the unknown
and of the standard are within 10 per cent of each other (or within
about 20 per cent if the readings are made at depths as great as 50-
60 mm.) accurate results may however be obtained directly. If the
variations are greater than this a correction is necessary. Kober^
has proposed an equation to supply this correction and thus make
possible very accurate work under conditions of moderate variations
of concentration. The equation is as follows:

5 {l—x)sk

y =
X

or

s-\-sk-\-\/{s+sky — ^sky

X =

2y

where y = height of unknown solution, on the left side of the instru-
ment, when standard solution is kept on the right side at a definite
height, s = height of standard solution on the left side and x = the
ratio of the concentrations of the two solutions.

k = where K = a, constant, obtained by substitution of standardi-
zation values of s, y, and x. The instrument should be checked up
for each series of analyses by reading the standard against itself and
determining the potential height of the standard solution by reading
the scale on the left side when the solution on the right side is kept at a
definite height, and the two are matched.

I. Acetone Bodies. — Nephelometric Methods of Marriott ^ — Prin-
ciple.— Acetone in very small amounts forms a cloudy solution with the
Scott-Wilson reagent which may be read nephelometrically. By this

^ Kober: Jour. Ind. and Eng. Chem., 7, 843, 1915.

^ The instrument is manufactured by Lenz and Naumann Pullman Building, 17 Madison
Ave., Xew York City.

* Kober: /. Am. Chem. Soc, 37, 2379, 1915; Jour. Biol. Chem., 13, 485, 1913.

* Marriott: Jour. Biol. Chem., 16, 289 and 293, 1913.

BLOOD ANALYSIS 295

method it is possible to make a complete analysis for acetone and
diacetic acid and hydroxybutyric acid in from 2-5 c.c. of blood.

Procedure.- — Two to 5 c.c. of blood drawn from a superficial arm vein by means
of a sterile syringe are run into a small weighed flask containing 50 c.c. of 0.5
per cent potassium oxalate solution. The flask is reweighed. The diluted blood
is run into 100 c.c. of boiUng water acidified with i c.c. of glacial acetic acid'
contained in an 800 c.c. Kjeldahl distilling flask and the procedure is then carried
out as described in the Marriott-Scott -Wilson methods for (a.) acetone and diac-
etic acid and (b) /3-hydroxybutyric acid as outlined on page 284. The precipitate
in the mercury reagent is however estimated nephelemometrically. In this case
the distillate which should measure 75-100 c.c. is allowed to stand half an hour,
then transferred to a graduated cyUnder and diluted until an opalescence that
can be conveniently read is obtained. The turbidity occasioned by 0.05 mg. of
acetone diluted to 100 c.c. is a convenient strength for this purpose, although
considerably larger or smaller amounts give good results. With heavy opales-
cence it is desirable after diluting to a certain volmne, say 250 c.c. to remove
an aliquot portion with a pipette and dilute this appropriately. A solution con-
taining a known amount of acetone- is distilled into an excess of reagent^ and
this distillate which is to be used as the standard is diluted as above. Read in the
nephelometer against this standard, taking the readings as quickly as possible
after filling the tubes as the suspension settles slowly.

If the unknown suspension is diluted so as to be not more than 20 per cent
different from the standard and if comparisons are made in considerable depths
of solution (50-60 mm.) no corrections are necessary. If the two agree within
10 per cent accurate comparison may be made at less depths. If divergences are
greater and accurate results are desired, Kober's correction equation must be
used (see discussion of nephelometer p. 294).

2. Fat. — Nephelometric Method of Bloor^ — Principle. — The protein is precipi-
tated with alcohol and ether and the fatty acid in the extract determined nephelo-
metrically after saponification.

Procedure. — Extraction. — About 2 c.c. of blood are drawn from the vein with a
graduated syringe and run at once with stirring into a weighed graduated flask
containing about 40 volumes of a mixture of 3 parts alcohol and i part ether.
After again weighing to find the weight of blood added, the solution is raised to
boiling in a water-bath, cooled under the tap, made to volume with alcohol-ether
mixture, mixed and filtered. The filtrate is water clear and almost colorless.

Determination. — From 5-20 c.c. of the extract (containing about 2 mg. of fat)
are measured with a pipette into a small beaker and saponified b)'- evaporating
nearly but not quite to dryness with 2 c.c. of N/i sodium ethylate. The residue is
heated just to boiling after the addition of 5 c.c. of alcohol-ether, and 50 c.c. of
distilled water are added.

A similar solution of the standard is prepared by adding 5 c.c. of the standard

^ Commercial varieties of acetic acid frequently contain substances which behave like
acetone. Blank determinations should always be made and corrections made accordingly.

2 A convenient stock solution contains about 0.03 mg. acetone per c.c. The strength
of such a solution is determined by titration of 200 c.c. bv the Messincer-Huppert method
(see Chapter XXVI).

' The solution cannot be added directly to the reagent as a lower result is obtained than
when distilled.

*Bloor: Jour. Biol. CItcm., 17, 377, 1914; 23. 31;, IQ15.

296 PHYSIOLOGICAL CHEMISTRY

fatty acid solution^ from a pipette with stirring to 50 c.c. of distilled water. To
the standard and to the test solutions are added simultaneously from pipettes and
with stirring 10 c.c. portions of dilute (1:3) hydrochloric acid and the solutions
allowed to stand for five minutes, after which they are transferred to the comparison
tubes of the nephelometer (see Fig. 83, p. 291). Several readings should be taken
and averaged. The standard tube should always be on the same side. See dis-
cussion of nephelometer (page 290) for details as to reading. The results repre-
sent the amount of total fat (fatty acids and cholesterol) in the blood, expressed
as oleic acid. The fat of the corpuscles is not completely extracted, and it should
be borne in mind that other lipoids as cholesterol are included in the results.
Cholesterol may be determined separately and subtracted from the result for total
fat. It may also be determined in a part of the blood extract as prepared above
by a modified Autenrieth-Funk procedure. ^ Methods have also been devised for
the determination of the phosphatides of blood. ^

Instruments Used in the Examination of the Blood

Spectroscope.^ — Either the angular -vision spectroscope (Figs. 87
and 88) or the direct-vision spectroscope (Fig. 86) may be used in
making the spectroscopic examination of the blood. For a complete
description of these instruments the student is referred to any standard
text-book of physics.

I'lG. 8().- — I)iRECT-\isi()N Spectroscope.

1. Oxyhemoglobin. — Examine dilute (1:50) defibrinated blood spectro-
scopically. Note the broad absorption band between D and E. Continue the
dilution until this single broad band gives place to two narrow bands, the one
nearer the D line being the narrower. These are the typical absorption bands
of oxyhemoglobin obtained from dilute solutions of blood. Now dilute the blood
very freely and note that the bands gradually become more narrow and, if the
dilution is sufficiently great, they finally entirely disappear.

2. Hemoglobin (so-called Reduced Hemoglobin). — To blood which has been
diluted sufficiently to show well-defined oxyhemoglobin absorption bands add a
small amount of Stokes' reagent.^ The blood immediately changes in color from

1 The standard solution used is an alcohol-ether solution of pure oleic acid of which
5 c.c. contain about 2 mg. of the acid. The alcohol and ether used for the standard are
freshly redistilled absolute alcohol and pure dry ether.
^Bloor: Jour. Biol. C/tem., 23, 317, 1915.
3 Greenwald: Jour. Biol. Cliem., 21, 29, 1915.
Bloor: Jour. Biol. Chem., 22, 133, 1915, 23, 317, 1915.
Kober and Egerer: J. Am. Chem. Soc, 37, 2373, 1915.
Taylor and Miller: Jour. Biol. Chem., 18, 215, 1914.
For other nephelometric methods see Chapters XVII and XXVI.
■• For Absorption Spectra see Plates I and II.

^ Stokes' reagent is a solution containing 2 per cent ferrous sulphate and 3 per cent tar-
taric acid. When needed for use a small amount should be placed in a test-tube and ammo-
nium hydroxide added until the precipitate which forms on the first addition of the hydrox-
ide has entirely dissolved. This produces ammonium ferrotartrate which is a reducing agent.

BLOOD ANALYSIS

297

a bright red to violet-red. The oxyhemoglobin has been reduced through the
action of Stokes' reagent and hemoglobin (so-called reduced hemoglobin) has
been formed. This has been brought about by the removal of some of the loosely

Fig. 87. — AxouLAR-visioN Spectroscope Arranged for .\bsorptiox Analysis.

combined oxygen from the oxyhemoglobin. Examine this hemoglobin spectro-
scopically. Note that in place of the two absorption bands of oxyhemoglobin we
now have a single broad band lying almost entirely between D and E. This is
the typical spectrum of hemoglobin. If the solution showing this spectrum be

Fig. 88. — Diagram of Angular-vision Spectroscope. (Long.)

The white light F enters the collimator tube through a narrow slit and passes to the
prism, P, which has the power of refracting and dispersing the light. The raj-s then pass to
the double conve.x lens of the ocular tube and arc deflected to the eyepiece E. The dotted
lines show the magnified virtual image which is formed. The third tube contains a scale
whose image is reflected into the ocular and shown with the spectrum. Between the light
F and the collimator slit is placed a cell to hold the solution undergoing examination.

shaken in the air for a few moments it will again assume the bright red color of
oxyhemoglobin and show the characteristic spectrum of that pigment.

3. Carbon Monoxide Hemoglobin. The preparation of this pigment may be
easily accompUshed by passing ordinary illuminating gas' through defibrinated

^ The so-called water gas with which ordinary illuminating gas is diluted contains usu-
ally as much as 20 per cent of carbon monoxide (CO).

298 PHYSIOLOGICAL CHEMISTRY

OX -blood. Blood thus treated assumes a brighter tint (carmine) than that im-
parted by oxyhemoglobin. In very dilute solution oxyhemoglobin appears
yellowish red whereas carbon monoxide hemoglobin under the same conditions
appears bluish red. Examine the carbon monoxide hemoglobin solution spec-
troscopically. Observe that the spectrum of this body resembles the spectnim
of oxyhemoglobin in showing two absorption bands between D and E. The
bands of carbon monoxide hemoglobin, however, are somewhat nearer the violet
end of the spectrimi. Add some Stokes' reagent to the solution and again ex-
amine spectroscopically. Note that the position and intensity of the absorption
bands remain unaltered.

The following is a delicate chemical test^ for the detection of carbon monoxide
hemoglobin :

Tannin Test. — ^Divide the blood to be tested into two portions and dilute each
with 4 volumes of distilled water. Place the diluted blood mixtures in two small
flasks or large test-tubes and add 20 drops of a lo per cent solution of potassiimi
ferricyanide.2 Allow both solutions to stand for a few minutes, then stopper the
vessels and shake one vigorously for 10-15 minutes, occasionally removing the
stopper to permit air to enter the vessel.' Add 5-10 drops of amLmonium svdphide
(yellow) and 10 c.c. of a 10 per cent solution of tannin to each flask. The contents
of the shaken flask will soon exhibit the formation of a dirty oUve-green precipitate,
whereas the flask which was not shaken and which, therefore, still contains car-
bon monoxide hemoglobin, will exhibit a bright red precipitate, characteristic of
carbon monoxide hemoglobin. This test is more deUcate than the spectroscopic
test and serves to detect the presence of as low a content as 5 per cent of carbon
monoxide hemoglobin.

4. Neutral Methemoglobin. — Dilute a Uttle defibrinated blood (i : 10) and
add a few drops of a freshly prepared 10 per cent solution of potassium ferricya-
nide. Shake this mixture and observe that the bright red color of the blood is
displaced by a brownish red. Now dilute a Uttle of this solution and examine it
spectroscopically. Note the single, very dark absorption band lying to the left
of D, and, if the dilution is sufficiently great, also observe the two rather faint
bands lying between D and E in somewhat similar positions to those occupied by
the absorption bands of oxyhemoglobin. Add a few drops of Stokes' reagent to
the methemoglobin solution while it is in position before the spectroscope and note
the immediate appearance of the oxyhemoglobin spectrum which is quickly fol-
lowed by that of hemoglobiti.

5. Alkaline Methemoglobin. — Render a neutral solution of methemoglobin,
such as that used in the last experiment (4), slightly alkaline with a few drops of
ammonia. The solution becomes redder in color, due to the formation of alkaline
methemoglobin and shows a spectrum different from that of the neutral body. In
this case we have a band on either side of D, the one nearer the red end of the
spectrum being much the fainter. A third band, darker than either of those men-
tioned, lies between D and E somewhat nearer E.

6. AlkaU Hematin. — Observe the spectrum of the alkali hcmatin prepared in
Experiment 18 on page 266. Also make a spectroscopic examination of a freshly

^ Sand (Ugeskrifl for Laeger, 76, 1721, 1914; Abst. J. A. M. A., Nov. 21, 1914) proposes
a potassium iodide test for carbon monoxide hemoglobin in blood. He claims 0.125 per
cent may be detected by his test.

^This transforms the oxyhemoglobin into methemoglobin.

' This is done to free the blood from carbon monoxide hemoglobin.

BLOOD ANALYSIS 299

prepared alkali hematin.' The typical spectrum of alkali hematin shows a single
absorption band lying across D and mainly toward the red end of the spectrum.

7. Reduced Alkali Hematin or Hemochromogen. — Dilute the alkali hematin
solution used in the last experiment (6) to such an extent that it shows no absorption
band. Now add a few drops of Stokes' reagent or ammonium sulphide and note
that the greenish-brown color of the alkali hematin solution is displaced by a
bright red color. This is due to the formation of hemochromogen or reduced
alkali hematin. Examine this solution spectroscopically and observe the narrow,
dark absorption band lying midway between D and E. If the dilution is not
too great a faint band may be observed in the green extending across E and b.

8. Acid Hematin. — To some defibrinated blood add half its volume of glacial
acid and an equal volume of ether. Mix thoroughly. The acidified etheral
solution of hematin rises to the top and may be poured off and used for the spectro-
scopic examination. If desired it may be diluted with acidified ether in the ratio
of one part of glacial acetic acid to two parts of ether. A distinct absorption band
will be noted in the red between C and D and lying somewhat nearer C than the
band in the methemoglobin spectrum. Between D and F may be seen a rather
indistinct broad band. Dilute the solution untU this band resolves itself into two
bands. Of these the more prominent is a broad, dark absorption band lying in the
green between b and F. The second, a narrow band of faint outline, lies in the
light green to the red side of E. A fourth very faint band may be observed lying
on the violet side of D.

9. Acid Hematoporphyrin. — To 5 c.c. of concentrated sulphuric acid in a test-
tube add 2 drops of blood, mixing thoroughly by agitation after the addition of
each drop. A wine-red solution is produced. Examine this solution spectroscopic-
ally. Acid hematoporphyrin gives a spectrum with an absorption band on either
side of D, the one nearer the red end of the spectrum being the narrower.

10. Alkaline Hematoporphyrin. — Introduce the acid hematoporphyrin solution
just examined into an excess of distilled water. Cool the solution and add potas-
sium hydroxide slowly until the reaction is but slightly acid. A colored precipitate
forms which includes the principal portion of the hematoporphyrin. The presence
of sodium acetate facilitates the formation of this precipitate. Filter off the
precipitate and dissolve it in a small amount of dilute potassium hydroxide. Alka-
line hematoporphyrin prepared in this way forms a bright red solution and possesses
four absorption-bands. The first is a very faint, narrow band in the red, midway
between C and D ; the second is a broader, darker band lying across D, principally to
the violet side. The third absorption band lies principally between D and E, ex-
tending for a short distance across E to the violet side, and the fourth band is
broad and dark and lies between b and F. The first band mentioned is the faintest
of the four and is the first to disappear when the solution is diluted.

I. Fleischl's Hemometer (Fig. 89, p. 300). — This is an instrument
used quite extensively clinically, for the quantitative determination of
hemoglobin. The instrument consists of a small cylinder which is pro-
vided with a fixed glass bottom and a movable glass cover, and which is

1 Alkali hematin may be prepareil by mixing one volume of a concentrated potassium
hydroxide or sodium hydro.xide solution and two volumes of dilute (i : 5) delibrinated blood.
This mbcture should be heated gradually almost to boiling, then cooled and shaken for
a few moments in the air before examination.

300

PHYSIOLOGICAL CHEMISTRY

Fig.

divided, by means of a metal septum, into two compartments of equal
capacity. This cylinder is supported in a vertical position by means of
a mechanism which resembles the base and stage of an ordinary micro-
scope. Underneath the stage is placed a colored glass wedge (see
Fig. 91), so arranged as to run immediately beneath the glass
bottom of one of the compartments of the cylinder and ground in such a
manner that each part of the wedge corresponds in color to a solution

of hemoglobin of some definite percent-
age. The glass wedge is held in a metal
frame and may be moved backward or
forward by means of a rack and pinion
arrangement. A scale along the side of
this frame indicates the percentage of the
normal amount of hemoglobin which each
particular variation in the depth of color
of the ground wedge represents, taking
the normal hemoglobin content as 100.^
In a position corresponding to the posi-

-Fleischl's Hemometer. tion of the mirror on the ordinary micro-

{Da Costa.) . . ^

scope is attached a light-colored opaque
plate which serves to reflect the light upward through the colored
wedge and the cylinder to the eye of the observer.

In making a determination of the percentage of hemoglobin by this instru-
ment the procedure is as follows: Fill each compartment about three-fourths
full of distilled water. Puncture the finger-tip or lobe of the ear of the subject by
means of a sterile needle or scalpel and, as soon as a drop of blood appears,
place one end of the capillary pipette (Fig. 90), which accompanies the instrument,
against the drop and allow it to fill by capillary attraction. To prevent the blood
from adhering to the exterior of the tube, and so render the determination inac-
curate, it is customary to apply a very thin coating of mutton fat to the outer sur-
face before using or to wrap the tube in a piece of oily chamois when not in use.
As soon as the tube has been accurately filled with blood it should be dipped into
the water of one of the compartments of the cylinder and all traces of the blood
washed out with water by means of a small dropper which accompanies the
instrument. If the blood is not well distributed throughout the compartment and
does not form a homogeneous solution the contents of the compartment should be
mixed thoroughly by means of the metal handle of the capillary measuring pipette.
When this has been done each compartment should be completely filled with dis-
tilled water and the glass cover adjusted, care being taken that the contents of
the two compartments do not mix. Now adjust the cylinder so that the compart-
ment containing the pure distilled water is immediately above the colored glass
wedge. By means of the rack and pinion arrangement manipulate the colored
wedge until a portion of it is found which corresponds in color with the diluted
blood. When this agreement in color has been secured the point on the scale cor-

' The scale of the ordinary instrument is usually too high.

BLOOD ANALYSIS

301

Fig. 90. — Pipette
OF Fleischl's

HEMOiCETER.

responding to this particular color should be read and the actual percentage of
hemoglobin computed. For instance, if the scale reading is 90 it means that the
blood under examination contains 90 per cent of the normal quantity of hemo-
globin, i.e., 90 per cent of 14 per cent.

2. Fleischl-Miescher Hemometer.— The apparatus of Fleischl
has been modihed by Miescher. If all precautions are taken, the
margin of error in the absolute quantity of hemoglobin determined by
this instrument does not exceed 0.15-0.22 per cent by weight of the
blood. Detailed directions for the manipulation of
the Fleischl-Miescher hemometer accompany the in-
strument. In brief Miescher modified the instru-
ment as follows: (i) The scale of each instrument
is supplied with a caliber table of absolute hemo-
globin values, expressed in milligrams: the scale of
Fleischl's hemometer shows the percentage of hemo-
globin in relation to an average selected somewhat
arbitrarily. Thus many errors arising from the irregular coloring of the
glass wedge of the older apparatus are avoided in the instrument as
modified. (2) Each instrument is accompanied by a measuring pip-
ette (melangeur) which allows of a more accurate measurement of the
blood than was possible with the capillary tubes of the older appara-
tus, (jj With the aid of the measuring pipette mentioned above
blood of varying degrees of concentration may be compared. In this
way the indi\ddual examinations are controlled and a check upon the

accuracy of the graduation in the

color of the glass wedge is also
afforded. This wedge is much
more evenly and accurately colored
than in the unmodified apparatus
of Fleischl. (4) Before reading
the percentage as indicated by the
scale, the chamber is covered with
a glass and a diaphragm which sharply define the field on all sides
without the formation of a meniscus.

The measuring pipette is constructed essentially the same as the
pipettes which accompany the Thoma-Zeiss apparatus (see page 305).
The capillary portion, however, is graduated, i, 2/3 and 1/2 which
enables the observer to dilute the blood sample in the proportion of
I :20o, I :3oo or i :40o as he may desire. If there is difficulty in
drawing in the blood exactly to one of the graduations just mentioned
the amount of blood above or below the volume indicated by the gradu-
ation may be determined by means of certain delicate cross-lines which

Fig. 91. — Colored Glass Wedge of
Fleischl's Hemometer. (Da Costa.)

302

PHYSIOLOGICAL CHEMISTRY

are placed directly above and below the graduation. Each cross-line
corresponds to i/ioo of the volume of the capillary tube from the tip
to the I graduation.

A O.I per cent solution of sodium carbonate is used to dissolve the
stroma of the erythrocytes and so render the blood solution perfectly
clear. If this is not done the color of the blood solution invariably ap-
pears darker in tone than that of
the colored glass wedge. A freshly
prepared sodium carbonate solu-
tion should be used in order that
the clearness of the solution may
not be marred by the presence of
sodium bicarbonate.

3. Dare's Hemoglobinometer
(Fig. 92). — This instrument, as
the name signifies, is used for the
determination of hemoglobin. In
using either Fleischl's hemometer
or the instrument as modified by
Miescher the blood is diluted for
examination, whereas with the
Dare instrument no dilution is re-
quired. This probably allows of
rather more accurate determina-
tions than are possible with the
old Fleischl apparatus.

The instrument consists essen-
tially of the following parts: (i)
A capillary observation cell, (2) a
semicircular colored glass wedge,
(3) a milled wheel for manipulat-
ing the wedge, (4) a candle used
to illuminate portions of the capillary observation cell and the colored
wedge, (5) a small telescope used in the examination of the areas illumi-
nated by the candle flame, (6) a scale graduated in percentages of the
normal amount of hemoglobin, (7) a hard-rubber case, (8) a movable
screen attached to the case.

The capillary observation cell is formed of two small, polished
rectangular plates of glass, one being transparent and the other opaque.
When held in position on the instrument, by means of a small metal
bracket, the opaque portion of the cell is nearer the candle and thus
serves to soften the glare of light when an observation is being made.

Fig. 92. — Dare's Hemoglobinometer.
{,Da Costa.)

R, Milled wheel acting by a friction bear-
ing on the rim of the color disc; S, case in-
closing color disc, and provided with a stage
to which the blood chamber is fitted; T,
movable wing which is swung outward dur-
ing the observation, to serve as a screen for
the observer's eyes, and which acts as a
cover to inclose the color disc when the in-
strument is not in use; U, telescoping cam-
era tube, in position for examination; V,
aperture admitting light for illumination of
the color disc; X, capillary blood chamber
adjusted to stage of instrument, the slip of
opaque glass, W, being nearest to the source
of light; Y, detachable candle-holder; Z,
rectangular slot through which the hemo-
globin scale indicated on the rim of the
color disc is read.

BLOOD ANALYSIS

303

The transparent portion of the cell is directly over a circular opening
in the case, through which the blood specimen is viewed by means of
the small telescope.

The semicircular colored glass wedge is so ground that each par-
ticular shade of color corresponds to that possessed by fresh blood which
contains some definite percentage of hemo-
globin. It is mounted upon a disc which
may be manipulated by the milled wheel in
such a manner as to bring successive por-
tions of the wedge in position to be viewed
through a circular opening contiguous to the
opening through which the blood specimen is
viewed. For a further description of the in-
strument see Figs. 92, 93, and 94.

In using the Dare hemoglobinometer proceed as
follows : Puncture the finger-tip or lobe of the ear
of the subject by means of a needle or scalpel and,
after a drop of blood of good proportions has
formed, place the fiat capillary observation cell in
contact with the drop and aUow it to fill by cap-
illary attraction (Fig. 94). Replace the cell in its

proper place on the instnunent. When in position, a portion of this cell may be
observed through a small telescope attached to the apparatus. It is viewed
through a circular opening and near this circle is a second one through which a
portion of a semicircvilar colored glass wedge is visible. These two circles are
illuminated simultaneously by means of the flame of a candle. The colored glass

Fig. 93. — Horizontal Sec-
tion OF Dare's Hemoglobin-
ometer. (Da Cosia.)

Fig. 04. — Method of Filling the Capillary Observatiojsj Cell of Dare's Hemo-
globinometer. (Da Costa.)

may be rotated by means of a milled wheel and the point of agreement of the
color of the adjoining discs may be determined in the same way as in Fleischl's
hemometer. The scale reading gives the percentage of the normal quantity
of hemoglobin which the blood sample imder examination contains. Compute
the actual hemoglobin content in the same manner as from the scale reading of
the Fleischl hemometer (see page 299).

304

PHYSIOLOGICAL CHEMISTRY

4. Tallquist's Hemoglobin Scale. — This consists essentially of a
series of ten colors corresponding to stains produced by blood contain-
ing varying percentages of hemoglobin.

In using this scale a drop of blood is allowed to fall on a small section of
filter paper and the resulting color is compared with the ten colors of the scale.
When the color in the scale is found which corresponds to the color of the blood
stain the accompanying hemoglobin value is read off directly.

This is a very convenient method for determining hemoglobin at the
bedside. There is a possibility of the colors being inaccurately printed,
however, and even if originally correct in tint, under the continued
influence of air and light they must eventually alter somewhat.

5. Thoma-Zeiss Hemoc3rtometer. — This is an instrument used in
"blood counting," i.e., in determining the number of erythrocytes and
leucocytes. The instrument consists of a microscopic slide constructed
of heavy glass and provided with a central counting cell (see Fig. 95,

C'

Fig. 95. — Thoma-Zeiss Counting Chamber. {Da Costa.)

below). This cell, with the cover glass in position, is exactly o.i mm.
deep. The floor of the cell is divided by delicate lines into squares each
of which is 1/400 sq. mm. in area (see Fig. 97, page 306). The volume
of blood, therefore, between any particular square and the cover glass
above must be 1/4000 cu. mm. Accompanying each instrument are
two capillary pipettes (Fig. 96), each constructed with a mixing bulb
in its upper portion. Each bulb is further provided with an enclosed
glass bead which is of great assistance in mixing the contents of the
chamber. The stem of each pipette is graduated in tenths from the
tip to the bulb. The final graduation at the upper end of the bulb is
1 01 on the pipette used in mixing the blood sample in which the ery-
throcytes are counted (erythrocytometer, see Fig. 96), and 11 on
the pipette used in mixing the blood sample for the leucocyte count
(leucocytometer, see Fig. 96). In making "blood counts" with the
hemocytometer it is necessary to use some diluting fluid. Two very
satisfactory forms of fluid for this purpose are Toison's and Sher-

BLOOD ANALYSIS

305

rington's solutions.^ When either of these solutions is used as the dilut-
ing fluid it is possible to make a very satisfactory count of both the
erythrocytes and leucocytes from the same prepara-
tion, since the leucocytes are stained by the meth}l-
violet or methylene-blue.

In counting the erythrocytes by means of the hemo-
cjrtometer, proceed as follows : Thoroughly cleanse the tip
of the finger or lobe of the ear of the subject by the use of
soap and water, alcohol and ether apphed in the sequence
just given. Puncture the skin by means of a needle or
scalpel and allow the blood drop to form without pressure.
Place the tip of the pipette in contact with the blood drop,
being careful to avoid touching the skin, and draw blood into
the pipette up to the point marked 0.5 or i according to
the desired dilution. Rapidly wipe the tip of the pipette
and immediately fill it to the point marked loi with Toison's
or Sherrington's solution. Now thoroughly mix the blood
and diluting fluid within the mixing chamber by tapping
the pipette gently against the finger, or by shaking it while
held securely with the thumb at one end and the middle
finger at the other. After the two fluids have been
thoroughly mixed the diluting fluid contained in the capil-
lary-tube below the bulb should be discarded in order to in-
sure the collection of a drop of the thoroughly mixed blood
and diluting solution for examination. Transfer a drop from
the pipette to the ruled floor of the counting chamber and,
after placing the cover-glass firmly in position,- allow an in-
terval of a few minutes to elapse for the corpuscles to settle
before making the count. Now place the shde under the
microscope and count the number of erythrocytes in a num-
ber of squares, counting the corpuscles which are in con-
tact with the upper and the right-hand boundaries of the

21

w

Fig. 96. — THOiL\-
Zeiss Capillary
Pipettes.

A, Erythrocytometer;
B, Leucocytometer.

Sherrington's solution has the following
formula:

Methylene-blue o. i gram.

Sodium chloride 1.2 gram.

Neutral potassium o.xalate 1.2 gram.

Distilled water 300.0 grams.

^ Toison's solution has the following
formula:

Methyl-violet 0.025 gram.

Sodium chloride i gram.

Sodium sulphate 8 grams.

Glycerol 30 grams.

Distilled water 160 grams.

^ If the cover-glass is in accurate apposition to the counting cell Newton's rings may be
plainly observed. Eustis {Jour. Ant. Med. Ass'n, 61, 1984, 1913) suggests the following
technic: "After the usual shaking of the pipette, and expulsion of a few drops of the
suspension, a good sized drop is placed on the counting chamber, no particular atten-
tion being paid to its size. The cover-glass, which has been previously cleaned, is
then rapidly grasped between the thumb and index-finger of the right hand, while the
slide is steadied on the table with the left hand. While firm pressure is exerted on the
cover-glass it is rapidly slid across the counting chamber, through the drop of suspen-
sion on it. The cover-glass will cut through the drop at exactly o.i mm. The excess
from the drop will rise on top of the cover-glass and jump across the moat. Newton's
rings will be obtained in each instance. The drop on top of the edge of the cover-
glass is wiped or soaked up with the point of a towel or blotting-paper and the preparation
is completed."

3o6

PHYSIOLOGICAL CHEMISTRY

square as belonging to that square. Take the squares in some definite se-
quence in order that the recounting of the same corpuscles may be avoided.
A satisfactory procedure is to begin in the upper right-hand comer and proceed
from left to right counting the cells in each individual square. Take the next
lower row of squares and count from left to right and so on (see Fig. loi, page
311). Of course, all things being equal, the greater the number of squares ex-
amined the more accurate the count. It is considered essential under all cir-
cimistances, where an accurate count is desired, that the counting chamber
shall be filled, at least twice, and the individual counts made in each instance,
as indicated above, before the data are deemed satisfactory. Under no condi-
tions should less than 200 squares be examined.

Fig. 97. — Ordinary Ruling of Thoma-Zeiss Counting Chamber. {Da Costa.)

To calculate the number of erythrocytes per cubic millimeter of
undiluted blood proceed as follows: Determine the number of cor-
puscles in any given number of squares and divide this total by the
number of squares, thus obtaining the average number of erythrocytes
per square. Multiply this average by 4000 to obtain the number of
erythrocytes per cubic millimeter of diluted blood, and multiply this
product by 100 or 200, according to the dilution, to obtain the number of
erythrocytes per cubic millimeter of undiluted blood. Thus:

per

Average number of erythrocytes X4000X 2oo(or loo'
per square ^ ^

_ Number of erythrocytes
~ cubic millimeter.

Great care should be taken to see that the capillary pipette is prop-
erly cleaned. After using, it should be immediately rinsed out with the
diluting fluid, then with water, alcohol, and ether in the sequence given.
Finally dry air should be drawn through the capillary and a horsehair
inserted to prevent the entrance of dust particles.

In counting leucocytes by means of the hemocytometer proceed as follows :
As mentioned above, if the diluting fluid is either Toison's or Sherrington's

BLOOD ANALYSIS

307

solution the leucocytes may be counted in the same specimen of blood in which
the erythrocytes are counted. When this is done it is customary to use a sUde
provided with Zappert's modified niling (Fig. gSj. This method is rather more
accurate than the older one of counting the leucocytes in a separate specimen
of blood. Furthermore, it is obviously preferable to count both the eryth-
rocytes and the leucocytes from the same blood sample. To insure accuracy
the nvunber of leucocytes within the whole ruled region should be determined in
dupUcate blood samples. This includes the examination of an area eighteen
times as great as the old style Thoma-Zeiss central ruUng. This region then
would correspond to 3600 of the small squares and, if duphcate examinations were
» made, the total bumber of small squares examined would aggregate 7200.

The calculation would be as follows :

Number of leucocvtes in 7200 ,, , , . Number of leucocytes per cubic

' X 200X4000 — 7200= •„• .

squares ^ ^-^t 1 millimeter. 1

Fig. 98. — Zappert's Modified Ruling OF Thoma-Zeiss Counting Chamber. iDa Cosla.)

If a Zappert slide is not available, a good plan to follow is to place a
diaphragm in the tube of the ocular of the microscope consisting of a
circle of black cardboard or metaP having a square hole in the center of
such a size as to allow of the examination of exactly 100 squares or one-
fourth of a square millimeter at one time. With this arrangement any
portion of the specimen may be examined and counted whether within
or without the ruled area. In counting by means of this dcNice it is, of
course, helpful if the microscope is provided with a mechanical stage,
but even without this arrangement, if the observer is careful to see that
the leucocytes at the extreme boundary of one field move to the opposite
boundary when the position of the slide is changed, the device may be
very satisfactorily employed. The leucocytes should be counted in 36

' Ehrlich's mechanical eyepiece with iris diaphragm is al--
purpose.

!li-;fart(>r\- for tills

3o8 PHYSIOLOGICAL CHEMISTRY

of the diaphragm-fields in duplicate specimens and the calculation made
• in the same manner as explained above.

If the leucocytes are counted in a separate specimen of blood ordina-
rily the diluting fluid is 0.3-0.5 per cent acetic acid, a fluid in which the
leucocytes alone remain visible. Under these conditions the dilution is
customarily made in the pipette having 1 1 as the final graduation. The
capillary portion is of larger caliber and so requires a greater amount of
blood to fill it to the 0.5 or i mark than is required in the use of the other
form of pipette. In counting the leucocytes according to this method it
is customary to draw blood into the pipette up to the i mark and im-
mediately fill the remaining portion of the apparatus to the 1 1 gradua-
tion with the 0.3-0.5 per cent acetic acid. It then remains to count the
number of leucocytes in the whole central ruled portion of 400 squares.
This should be done in duplicate samples and the calculation made as
follows :

Number of leucocytes in 800 ^ ^ . o Number of leucocytes per cubic

X 4.000 X I o -^ 80c = .,,. - ^

squares ^j,^'^'^^^.^ ow^ millimeter.

6. Biirker's Hemocytometer.^ — This is an improved apparatus^ for the more
accurate counting of erythrocytes than is possible by the Thoma-Zeiss apparatus.
The principles involved are somewhat different from those in force with the latter
apparatus. For example, the blood is diluted in a separate vessel, not in the pipette
with which the sample is drawn, and furthermore the cover-g'ass is applied to the
counting chamber and damped in place before the diluted blood is applied to the
ruled area. Hayem's solution* is used as the diluting fluid. Toison's solution is
not satisfactory for use with the Biirker counting chamber as its viscosity is too
great. The corpuscles settle rapidly in Hayem's fluid as the specific gravity of the
fluid is 1015 whereas that of the erythrocj'tes is 1090.

The pipette for measuring the quantity of blood (Fig. 99, upper pipette) has a
point which is not ground dull but is polished. This allows of better judgment in
deciding whether the column of blood extends to the very tip. The volume of
the pipette between tip and mark is 25 cu. mm. The mark extends all the way
around the tube so that errors of parallax may be avoided.

The pipette for measuring the diluting fluid (Fig. 99, middle pipette) also has
a polished point and circular mark and delivers 4975 cu. mm. This volume of
diluting fluid with 25 cu. mm. of blood gives a dilution of i : 200. Both pipettes
are provided with a piece of rubber tubing and mouthpiece.

For transferring the diluted blood from the diluting flask to the chamber a
plain pipette provided with a rubber cap is used (Fig. 99, lower pipette). It is
filled by pressing the cap slowly with the index-finger, inserting the tip into the
liquid and then releasing the pressure.

* Biirker: Pfliiger's Archiv., 142, 337, 191 1; Miincli. med. Woch., 59, pp. 14 and 89, 1912.

^ Manufactured by C. Zeiss, Jena.

' Hayem's solution has the following formula:

Mercuric chloride o. 25 gram.

Sodium chloride ^ o. 5 gram.

Sodium sulphate 2 . 5 grams.

Distilled water 100 . o grams.

BLOOD ANALYSIS

309

The diluting is done in a small round-boUomed flask as shown in Fig. 99.
Several of these flasks should be kept on hand in a wooden rack which will hold
them in an upright position. Each flask is provided with a paraflined,y)r smooth
cork stopper.

In the older counting chambers the floor of the chamber is circular and the
counting is done in the center of this space. The corpuscles are therefore counted
in the center of a capillary, circular film where on account of surface tension their
number is slightly greater than elsewhere. This source of error is avoided in the
new counting chamber (Fig. 102) in which the floor is represented by the upper
surface of a piece of glass 25 mm. long and 5 mm. wide which is rounded off at both
ends and divided into two portions by a groove 1.5 mm. wide through the center.

Fig. 99. — BiJRKER's Pipettes, Mixing Flasks and Counting Chamber.

At each side of this floor piece, separated from it by a groove is a glass plate
(7.5 mm. X 21 mm.) of such height that the space between the floor of the cell
and a cover-glass placed across the plates is o.ioo mm. A cover-glass 23 mm.
long and 21 mm. wide with rounded polished edges is used so that the rounded
ends of the floor piece project beyond it. The chamber is provided with clamps
to press the cover-glass firmly upon both plates (Fig. 99).

The ruling on each portion of the floor piece is that shown in Fig. 100, which
will be explained below\

Measuring the Diluting Fluid. — Four thousand nine hundred and seventy-five
cu. mm. of diluting fluid {Ilayenis) are measured out into the diluting flask. To
do this the pipette is filled by suction to slightly above the mark and the rubber
tube is carefully clamped off. Then with a soft piece of linen the tip is wiped dr>'.
The meniscus is then accurately adjusted to the mark by lightly touching the point
of the pipette to the cleaned tip of the finger. The pipette is then inserted into

3IO

PHYSIOLOGICAL CHEMISTRY

the diluting flask and with the tip nearly touching the bottom of the flask the fluid
is allowed to run out. The time of the flow should be about forty seconds and is
controlled by placing the tip of the index-finger loosely upon the mouthpiece.
The pipette is emptied completely by alternately blowing through it and touching
it to the wall of the flask slightly above the level of the liquid. The drops clinging
to the wall are united with the bulk of the liquid by a suitable motion of the flask.
The flask is then stoppered, care being taken from now on that none of the liquid
ever touches the neck of the flask or the stopper.

Taking the Blood Sample. — Usually the best time to draw the blood is before
breakfast. For a single determination the author prefers to draw it from the tip
of the fourth finger of the left hand. For repeated determinations it is well to
change off between third, fourth and fifth fingers of left hand. The temperature
of the room should not be below i7°C. to prevent an undue contraction of the
cutaneous vessels. The instrument used to puncture the finger should have a
chisel-shaped point which is preferable to the ordinary lancet-shaped point. The

Fig. ioo. — Ruling of Burker Counting Chamber.

first drop of blood is wiped off. Into the second one the tip of the pipette is in-
serted and blood is drawn in until the meniscus is even with or a little beyond the
mark. The tip is then wiped off without touching the capillary opening and the
observer assures himself that the column of blood extends to the very end of the
capillary. The meniscus is then accurately adjusted to the mark.

Mixing of the Blood and Diluting Fluids. — The tip of the pipette is now dipped
into the diluting fluid which has been measured into the flask and the blood is
slowly blown out. The blood having a much higher specific gravity than the
Hayem's fluid sinks to the bottom. The pipette is then filled with the pure super-
natant diluting fluid and emptied again, care being taken to avoid air bubbles.
This is repeated until the blood is removed as completely as possible. To mix the
blood and diluting fluid the flask is rotated for two minutes in spiral curves of
continually decreasing radius. The motion should be alternately clockwise and
counterclockwise. After complete mixing the pipette is rinsed out several times
with the diluted blood.

BLOOD ANALYSIS

311

Transferral of the Diluted Blood to the Chamber. — The counting chamber which
has been cleaned with distilled water and alcohol-ether and then wiped dry with
a soft cloth as free from lint as possible is placed upon a black surface and carefully
brushed with a camel's hair brush. The cover-glass is now placed over the chamber
by sliding it over the two glass plates with both thumbs while the index-fingers are
pressing it down. By means of the clamps it is held in place firmly so that New-
ton's rings (if possible of the first order: brown and black) may be seen over the
entire area of the plates. The chamber is placed upon the stage of the microscope
and is brought into a horizontal position.

Before transferring the diluted blood to the chamber the flask must be shaken
for two minutes as described before. The liquid shows a cloudy appearance and
must be allowed to stand until the turbidity has become uniform.

One of the plain pipettes described above is now inserted into the diluted blood

I

5

T

9

13

-1

1

— »

--

^

-5

5

-^

-

— *

-9

9

-^

-

— >

-13

13

1

>

T

£

»

1:

J

Fig. ioi. — Schema.

while slight pressure is being exerted on the rubber cap. The pressure is released
slowly and the liquid rises into the pipette. The point of the pipette is now im-
mediately placed upon one of the projecting ends of the floor plate and verj- slight
pressure is exerted on the rubber cap until the liquid coming from the pipette just
reaches the cover-glass when the pressure is released. An instantaneous filling
of the capillary space results. The pipette should be emptied immediately, rinsed
with distilled water and placed in an upright position in a beaker of water. The
other portion of the counting chamber is now filled in the same way with a second
pipette and about one minute is allowed for the settb'ng of the corpuscles. During
this time the pipettes may be washed with distilled water and ether-alcohol and
dried by suction. Occasionally, the pipettes should be cleaned with a horse hair
and with concentrated H2SO4 containing a little KjCraO?,

To see whether the distribution of the corpuscles has been uniform the chamber
is illuminated with a wide-open diaphragm and viewed at an angle. If the opacity

312

PHYSIOLOGICAL CHEMISTRY

is not uniform in either of the portions of the chamber, that one should not be used
for counting. If the counting must be interrupted or requires a long time a moist
chamber^ should be used to prevent evaporation of the diluting fluid. The diluted
blood may be retained in the mixing flasks and duplicate countings obtained after
the lapse of twenty-four hours or more according to Biirker.

Counting and Calculation. — A mechanical stage movable in two directions is
indispensable. With a magnification of 320 diameters the counting is begun in
the left upper corner of the ruling. Proceed from left to right along one row then
move from right to left along the next lower row, and so on. Only the small
squares are used for counting (see Fig. 100) and the figures are recorded in the
schema'^ (see Fig. loi) in which the squares crossed by horizontal or vertical lines
correspond to the small squares used for counting. Usually 80 squares are counted
and by recording the figures in the schema the count may be verified and an idea of

Tiefe

O.lOOmm.

C.Zeiss
Jerva

0

O.Olmm.

Fig. 102. — BtJRKER Counting Chamber.

the uniformity of the distribution may be formed. Half of the counted squares
should be in the one, half in the other portion of the counting chamber. For
more accurate measurements more squares may be counted.

The observer will do well not to attempt counting each individual corpuscle
in a square. After some practice each typical group of corpuscles will immediately
suggest a number. A very common form of grouping is one corpuscle surrounded
by four others. This should immediately suggest the number five. In this way
the counting will become more rapid and also more reliable.

The calculation is very simple. The number of corpuscles in 80 squares
divided by 100 will give the numBer of millions per cubic millimeter. If, for
example, 536 corpuscles have been counted in 80 squares then with a dilution
of I : 200 the number of corpuscles per cubic millimeter is 5,360,000. Thus,

536

Q—X 4000X200= 5,360,000 erythrocytes per cubic miUimeter. More than two

oO

decimal places are without significance.

1 Biirker: Pfliiger's Archiv, 118, 465, 1907.

2 The firm of H. Laupp in Tubingen has put this schema on the market (in packs of 100).

CHAPTER XVII
MILK

Milk is the most satisfactory individual food material elaborated by
nature. It contains the three nutrients, protein, fat, and carbohydrate
and inorganic salts in such proportion as to render it a very acceptable
dietary constituent. It is a specific product of the secretory activity of
the mammary gland. It contains, as the principal solids, olein,
pahnitin, stearin, hutyrin, casein, lad-alhumin, laclo-glohulin, lactose,
phosphates of calcium, potassium and magnesium, citrates of sodium
and potassium and chloride of calcium. The calcium phosphate of
milk is the neutral calcium phosphate, CaHP04.^ ]Milk also contains
some iron but not enough for the needs of the body if milk is the only
source of the iron. It also contains at least traces of lecithin, cholesterol,
urea, creatine, creatinine, and the tri-glycerides of caproic, lauric, and
myristic acids. According to Osborne and Wakeman- milk contains
two phosphatides, one being probably stearyl-oleyl-lecithin.

Recent investigations indicate the presence in milk of some sub-
stance or substances of unknown character which are of great nutritional
importance. The presence of a grouih-promoting substance (\'itamine)
i7i butter fat has been demonstrated by McCollom and Davis and by
Osborne and Mendel.^

By passing milk through a special form of earthenware filter Van
Slyke and Bosworth^ have obtained a separation of the constituents in
milk which are in true solution from those insoluble in water or
in suspension. The soluble constituents and the water constitute
the milk serum. They suggest the following classification of milk
constituents:

CONSTITUENTS OF MILK

In true solution in milk Partly in solution and Entirely in suspension

serum. partly in suspension or or colloidal solution.

colloidal solution.

1. Lactose. i. Albumin. i. Fat.

2. Citric acid. 2. Inorganic phosphate. 2. Casein.

3. Potassium. 3. Calcium.

4. Sodium. 5. Magnesium.

5. Chlorine.

'Van Slyke and Bosworth: Jour. Biol. Chcm., 20, 135, 1915.
^Osborne and Wakeman: Jour. Biol. Client., 21, 539, 1915.

* McCollom and Davis; Jour. Biol. Chem., 15, 167, 1913; Osborne and Mendel: ibid,
15, 311, 1913; 24, 37, 1916 (previous references cited in this article).

* Van Slyke and Bosworth: Jour. Biol. Chcm., 20, 135, 1915.

3^3

314 PHYSIOLOGICAL CHEMISTRY

Fresh milk, both human and cow^s, is amphoteric in reaction to
litmus and acid to phenolphthalein. The acidity is believed to be due
in part at least to soluble acid phosphates} Upon standing for a
sufficiently long time, unsterilized milk sours, i.e., it becomes strongly
acid in reaction to litmus due to the production of the optically in-
active fermentation lactic acid,

H OH
H— C— C— COOH,

I !

H H

from the lactose contained in it. This is brought about through
bacterial activity. The white color is imparted to the milk partly
through the fine emulsion of the fat and partly through the medium of
the caseinogen in solution. The specific gravity of milk varies some-
what, the average being about 1.030. Its freezing-point is about
-o.56°C.

This lactic acid fermentation may be brought about by Bad. lactis
and other microorganisms. Certain putrefactive bacteria in the
human intestines may also cause lactic acid fermentation. The chem-
ical changes in lactic acid fermentation may be indicated thus:

C12H22O11-I-H2O — >C6Hi206-l-C6Hi206

Lactose. Galactose Glucose.

C6H12O6— ^sCsHeOs

Galactose Lactic Acid,
or Glucose.

Fresh milk does not coagulate on being boiled but a film consisting
of a combination of casein and calcium salts forms on the surface.
If the film be removed, thus allowing a fresh surface to come into
contact with the air, a new film will form indefinitely upon the applica-
tion of heat. Surface evaporation and the presence of fat facilitate
the formation of the film, but are not essential (Rettger^) . As Jamison
and Hertz^ have shown, a similar film will form on heating any protein
solution containing fat or paraffin. If the milk is of a pronounced
acid reaction, through the inception of lactic acid fermentation, or from
any other cause, no film will form when heat is applied, but instead a
true coagulation will occur. When milk is boiled certain changes occur
in its odor and taste. These changes, according to Rettger,^ are due
to a partial decomposition of the milk proteins and are accompanied
by the liberation of a volatile sulphide, probably hydrogen sulphide.

^ Rettger: American Journal of Physiology, 7, 325, 1902.
^Jamison and Hertz: Journal of Physiology, 27, 26, 1902.
•Rettger: American Journal of Physiology, 6, 450, 1902.

MILK

3^5

The milk-curdling enzymes of the gastric and the pancreatic juice
have the power of splitting the casein of the milk, through a process of
hydrolytic cleavage, into soluble paracasein and a peptone-like body.
This soluble paracasein then forms a combination with the soluble
calcium salts of the milk and an insoluble curd of paracasein results.
The clear fluid surrounding the curd is known as whey. This action
of rennin may be represented by the following scheme:

Casein (+ rennin >

Peptone-like
body

Soluble paracasein

I

-f- Ca salts

I
Paracasein

(insoluble curd)

Fig. 103. — Normal Milk and Colostrum.
a, Normal milk; b, Colostrum.

There is still considerable confusion of terms when different authori-
ties discuss milk proteins and the action of milk curdling enzymes upon
them. The English scientists^ quite uniformly call the principal pro-
tein of milk caseinogen whereas the insoluble curd formed by rennin is
termed casein. On the other hand, the Germans and many^^mericans
give the name casein to the milk protein and paracasein to the product
of the action of rennin upon this protein. The confusion of terms
may be represented thus:

English German.

Caseinogen. = Casein.

Casein. = Paracasein.

^Halliburton: Journal of Physiology, ir, 44S, iqoo.

3i6

PHYSIOLOGICAL CHEMISTRY

The most important difference between human milk and cow's
milk is in the protein content, although there are also differences in the
carbohydrate and ash and likewise striking biological differences diffi-
cult to define chemically. It has been shown that the casein of human
milk differs from the casein of cow's milk in being more difficult to
precipitate by acid or coagulate by gastric rennin. The casein curd
(paracasein) also forms in much looser and more flocculent manner
than that from cow's milk and is for this reason much more easily
digested than the latter. Both human and cow's milk contain im-
portant non-nitrogenous substances of an unknown character. Human
milk contains the greater quantity of these substances.^

The relative composition of human and cow's milk is shown in the
following table which embraces data reported by Meigs and Marsh.

COMPOSITION OF MILK (PER CENT OF WHOLE MILK) NORMAL VARIATIONS
FROM BEGINNING OF SECOND MONTH OF LACTATION

Constituent

Cow

Human

Water (Avg.).

87.0

87-5

Solids (Avg.) .

13.0

12.5

Protein

4-2-5

I -5-0- 7

Fat

2-4

2-4

Sugar

3-5-5

6-7-5

Ash

0 . 6-0 . 7

0.2-0.3

The above data indicate that human milk contains less protein,
more sugar and much less ash than cow^s milk. The percentage
composition of human milk at different periods is represented in the
following table."

PERCENTAGE COMPOSITION OF HUMAN MILK BY PERIODS

Period

Fat

Sugar

Protein

Casein

Albumin Ash

Total
solids

Colostrum (1-12 days)

. . . . 2.8^

f. en

9. 2C

0.31

13-4

Transition (12-30 days)

••■•4-37J 7-74 ; 1-56

0. 24

I^.A

Mature (1-9 raos.)

... .13.26

7-50 j i-iS

0.43

0.72

0.21

U-2

Late (10-20 mos.)

....3.16

1

7.47

1.07

0.32

0.75

0.20 12.2

^ Meigs and Marsh: Jour. Biol. Chem., 16, 147, 1913.

'Holt, Courtney and Fales: Am. Jour. Dis. Children, 10, 229, 1915.

MILK

317

The composition of the ash of milk is shown in the following table
reported by Holt, Courtney and Fales.^

PERCENTAGE COMPOSITION OF THE ASH OF MILK

CaO

1

MgO

P2O5

NaiO

1 K2O CI

Human milk

233

3-7

16.6

7.2

28.3 16.5

Cow's milk

23.5

2.8

26.5

7.2

24-9 13-6

It will be observed that the composition of the ash of the two varieties
of milk is about the same except for phosphorus. The higher phos-
phorus content in the case of cow's milk is due principally to the fact
that the milk contains a higher percentage of casein ox phospJio protein.
It should be borne in mind that cow's milk contains on the average
over three times as much ash as human milk. Therefore unless cow's
milk has been diluted with more than twice its volume, there is still
present as high a concentration of the inorganic constituents as are
present in normal human milk. Hence there is no necessity for the
addition of any of these constituents in infant feeding.

Interesting data relative to the composition of milk from various
sources may be gathered from the following table which was compiled
mainly from the results of investigations by Proscher- and by Abder-
halden^ in Bunge's laboratory. It will be noted that the composition
of the milk varies directly with the length of time needed for the young
of the particular species to double in weight.

Species

Period in which
weight of the

newborn is
doubled (days)

100 Parts of milk contain

Proteins Salts Calcium

Phosphoric
acid

Man. . .
Horse . .
Cow. . .
Goat. .
Sheep. .
Pig....
Cat....
Dog. . .
Rabbit.

180
60

47
22

15

14

9-

9

6

0. 2

0 033

0.4

0. 124

0.7

0. 160

0.8

0.197

0.8

0.245

0.8

0.24Q

1 . 0

1-3

0.455

2-5

0.891

0.047
0.I3I

0.197
0.284
0.293

o . 30S

0.508
0.997

The secretion of the mammary glands of the newborn of both sexes
is called "witches' milk." The name is centuries old and evidently

' Holt, Courtney and Fales: Am. Jour. Dis. Children, 10, 229, 1915.

- Proscher: Zcit.f. physiol. Chemie, 24, 285, 1898.

^ .\bderhalden: Ibid., 26, 487, 1899; and 27, pp. 40S and 457, 1899.

3i8

PHYSIOLOGICAL CHEMISTRY

refers to the mystery of the useless secretion. Basch^ has recently sug-
gested that this secretion of "witches milk" is brought about by the
passage of hormones (see Chapter on Pancreatic Digestion) from the
blood of the mother to the fetus.

Lactose, the principal carbohydrate constituent of milk, is an impor-
tant member of the disaccharide group. It occurs only in milk, except
as it is found in the urine of women during pregnancy, during the nurs-
ing period, and soon after weaning; it also occurs in the urine of normal
persons after the ingestion of a very large amount of lactose in the food.
It is not derived directly from the blood, but is a specific product of the
cellular activity of the mammary gland. It has strong reducing power,
is dextro-rotatory and forms an osazone with phenylhydrazine. Lac-
tose is not fermentable by pure yeast. For changes which lactose

Fig. 104. — Lactose.

undergoes in lactic acid fermentation see page 314. The crystalline
form of lactose is shown in Fig. 104.

Casein, the principal protein constituent of milk, belongs to the
group of phosphoproteins and contains 0.7 per cent of phosphorus.^
It has acidic properties and combines with bases to produce salts.^
It is probably present in milk in the form of neutral calcium caseinate
(Casein Ca4).^ It is not coagulable upon boiling and is precipitated
from its neutral solution by certain metallic salts as well as upon satu-
ration with sodium chloride or magnesium sulphate. Its acid solu-
tion is precipitated by an excess of mineral acid.

Lactalbumin and lacto-globulin, the protein constituents of milk,

^ Basch: Milnch. med. Woch., 58, 2266, 1911.

^ Bosvvorth and Van Slyke: Jour. Biol. Chem., 19, 67, 1914.

^ Van Slyke and Bosworth: Jour. Biol. Chem., 14, 207-227, 1914.

* Van Slyke and Bosworth: Jour. Biol. Chem., 20, 135, 191 5.

MILK 319

next in importance to casein, closely Resemble serum albumin and
serum globulin in their general properties.

Butter (milk fat) consists in large part of olein and palmitin.
Stearin, butyrin, caproin and traces of other fats are also present.
When butter becomes rancid through the cleavage of certain of its
constituent fats by bacteria the odors of caproic and butyric acids are
in evidence.

The pigment of the fat of cow's milk is made up of carotin and
xanthophylls. The principal pigment is carotin, an unsaturated
hydrocarbon pigment which is widely distributed in plants.^ The
pigment of the fat of hufnan milk is made up of carotin and xantho-
phylls in about equal proportions. Carotin is also probably the
pigment of human fat. The pigment of body fat, blood serum, corpus
luteum and skin secretions of the cow is principally carotin.

Colostrum is the liame given to the product of the mammary gland
secreted for a short time before parturition and during the early period
of lactation (see Fig. 103, page 315). It is yellowish in color, contains
more solid matter than ordinary milk, and has a higher specific gravity
(i. 040-1. 080). The most striking difference between colostrum and
ordinary milk is the high percentage of lactalbumin and lacto-globulin
in the former. This abnormality in the protein content is responsible
for the coagulation of colostrum upon boiling.

Such enzymes as lipase, amylase, galactase, catalase, oxidases,
peroxidases, and reductases have been identified in milk, but not all of
them in milk of the same species of animal.

Among the principal preservatives used in connection with milk are
formaldehyde, hydrogen peroxide, boric acid, borates, salicylic acid,
and salicylates. The use of milk preservatives is illegal in most states.

Experiments on Milk

1. Reaction. — Test the reaction of fresh cow's milk to htmus, phenolphthalein
and Congo red.

2. Biuret Test. — Make the biuret test according to directions given on
page 98.

3. Microscopical Examination. — Examine fresh whole milk, skimmed or
centrifugated milk, and colostnmi under the microscope. Compare the micro-
scopical appearance with Fig. 103, page 315.

4. Specific Gravity. — Determine the specific gravity of both whole and
skinmied milk (see page 324). Which possesses the higher specific gravity?
Explain why this is so.

5. Film Formation. — Place lo c.c. of milk in a small beaker and boil a few
minutes. Note the formation of a film. Remove the film and heat again. Does

'Palmer and Eckles: Jour. Biol. Client., 17, 191, 1914.

320 PHYSIOLOGICAL CHEMISTRY

the film now form? Of what substance is this fihn composed? The biuret test
was positive ; why do we not get a coagulation here when we heat to boiling?

6. Coagulation Test. — Place about 5 c.c. of milk in a test-tube, acidify sUghtly
with dilute acetic acid and heat to boiling. Do you get any coagulation? Why?

7. Action of Hot Alkali. — To a Uttle milk in a test-tube add a few drops of
potassium hydroxide and heat. A yellow color develops and gradually deepens
into a brown. To what is the formation of this color due? (See Moore's Test,
Chapter II.)

8. Test for Chlorides. — To about 5 c.c. of milk in a test-tube add a few drops
of very dilute nitric acid to form a precipitate. Filter off this precipitate and test
the filtrate for chlorides. Does milk contain any chlorides?

9. Guaiac Test. — To about 5 c.c. of water in a test-tube add 3 drops of
milk and enough alcoholic solution of guaiac (strength about i : 60)^ to cause
turbidity. Thoroughly mix the fluids by shaking and observe any change which
may gradually take place in the color of the mixture. If no blue color appears
in a short time, heat the tube gently below 6o°C. and observe whether the
color reaction is hastened. In case a blue color does not appear in the course
of a few minutes, add hydrogen peroxide or old turpentine, drop by drop, until
the color is observed.

Fresh milk will frequently give this blue color v^hen treated w^ith an
alcoholic solution of guaiac without the addition of hydrogen peroxide
or old turpentine. Those milks which respond positively, fail to do so
after boiling 15-20 seconds. What substances beside milk respond to
this test? See discussion on page 258.

10. Differentiation of Human and Cow's Milk (Modification of Bauer's Test) 2.
— Introduce 2 c.c. of fresh himian milk into a 50 c.c. test-tube and 2 c.c. of fresh
cow's milk into another similar tube. Add to the contents of each tube i drop of
a 0.25 per cent aqueous solution of nile-blue sulphate (Griibler). Shake the
tubes gently and permit them to stand undisturbed for 10-30 minutes. The
milk assimies a bluish cast in each case. At the end of the lo-minute interval
add 10 c.c. of ether to the contents of each tube and shake very thoroughly for one
minute. The ether extracts the pigment from the human milk, leaving the milk
white. In the case of cow's milk the ether does not extract the dye and the milk
remains bluish in color.

11. Tests to Differentiate between Raw Milk and Heated Milk. —

(a) Trikresol Peroxidase Reaction (Kastle). — The peroxidase reaction of
milk is founded upon the fact that small ainounts of raw milk will in-
duce the oxidation of various leuco compounds by hydrogen peroxide.
This reaction has been used in a practical way as the most convenient
means of differentiating between raw milk and heated milk. Many
substances have been employed for this purpose, e.g., guaiac, para-
phenylenedi amine, ortol, amidol, etc. Kastle has found that a dilute

' Buckmaster advises the use of an alcoholic solution of guaiaconic acid instead of an
alcoholic solution of guaiac resin. Guaiaconic acid is a constituent of guaiac resin.
^ Bauer: Monatssch. J. Kindertieil,, 11, 474, 191 2-13.

MILK 321

solution of "trikresol"^ acts as a sensitizing agent in the peroxidase
reaction and offers the following test which is based upon this fact.

Procedure. — To 2-5 c.c. of raw milk in a test-tube add 0.1-0.3 c.c. of M/io
hydrogen peroxide and i c.c. of a i per cent solution of "trikresol." A slight
though unmistakable yellow color will be observed to develop throughout the
solution. Repeat the test using milk which has been boiled or heated to
8o°C. for 10-20 minutes and cooled, and note that no yellow color is produced.

The color reaction in the case of the raw milk probably results from
the oxidation of the cresols by the hydrogen peroxide. The first
product of this oxidation^ then oxidizes the leuco compound, when such
is present, and causes the color observed.

(b) Benzidine Peroxidase Reaction {Wilkinson and Peters).^ — To 10 c.c. of the
milk to be tested add 2 c.c. of a 4 per cent alcoholic solution of benzidine, suffi-
cient acetic acid to coagulate the milk (usually 2-3 drops) and finally 2 c.c. of a
3 per cent solution of hydrogen peroxide. Raw milk yields an immediate blue
color. In adding the peroxide it is best to permit it to flow slowly down the
wall of the vessel containing the mixture instead of allowing it to mix with the
milk. Milk which has been heated to 78°C. or above remains unchanged.

12. Satxiration with Magnesium Sulphate. — Place about 5 c.c. of milk in a
test-tube and saturate with solid magnesium sulphate. What is this precipitate?

13. Influence of Gastric Rennin on Milk. — Prepare a series of five tubes as
follows :

(a) 5 c.c. of fresh milk -f 0.2 per cent HCl (add drop by drop xmtil a precipitate
forms).

(b) 5 c.c. of fresh milk + 5 drops of rennin solution.*

(c) 5 c.c. of fresh milk + 10 drops of 0.5 per cent Na^iCOj.

(d) 5 c.c. of fresh milk + 10 drops of ammonimn oxalate.

(e) 5 c.c. of fresh milk + 5 drops of 02 per cent HCl.

Now to each of the tubes (c), (d) and (e) add 5 drops of rennin solution.
Place the whole series of five tubes at 40°C. and after 10-15 minutes note what
is occurring in the different tubes. Give a reason for each particular result.

14. Preparation of Casein. — Fill a large beaker one-third full of skimmed
(or centrifugated) milk and dilute it with an equal volume of water. Add dilute
hydrochloric acid until a flocculent precipitate forms. Stir after each acidifica-
tion and do not add an excess of the acid as the precipitate would dissolve.
Allow the precipitate to settle, decant the supernatant fluid, and reserve it for
use in later (15-18) experiments. Filter off the precipitate of casein and re-
move the excess of moisture by pressing it between filter papers. Transfer the
casein to a small beaker, add enough 95 per cent alcohol to cover it and stir for
a few moments. Filter, and press the precipitate between filter papers to re-
move the alcohol. Transfer the casein again to a small dry beaker, cover the
precipitate with ether and heat on a water-bath for ten minutes, stirring con-

^ "Trikresol" is the trade name of an antiseptic which contains the three cresols in ap-
proximately equal proportions.

'^ Probably some organic pero.xide or quinoid compound.

^ Wilkinson and Peters: Z. Nahr-Genussm., 16, No. 3, p. 172.

* Any commercial rennin or rennet preparation or an extract of the gastric mucosa
of the pig may be employed.

322

PHYSIOLOGICAL CHEMISTRY

tinuously. Filter (reserve the filtrate i, and press the precipitate as dry as possible
between filter papers. Open the papers and allow the ether to evaporate spon-
taneously. Grind the precipitate to a powder in a mortar. Upon the casein
prepared in this way make the following tests :

(a) Solubility. — ^Try the solubihty in water, sodiimi chloride, dilute acid and

alkali.

(b) Millon's Reaction. — Make the test according to the directions given on

page 97.

(c) Biuret Test. — Make the test according to directions given on page 98.

(d) GlyoxyUc Acid Reaction (HopMns-Colej. — Make the test according to
the directions given on page 98.

(e) Unoxidized Sulphur. — Test for unoxidized sulphur according to the di-
rections given on page 108. The sulphur content of casein is rather low, e.g.,
about 0.7 per cent.

(f ) Fusion Test for Phosphorus.— Test for phosphorus by fusion according to
directions given on page 129. Casein contains 0.7 per cent of phosphorus.

15. Coagulable Proteins of Milk. — Place the filtrate from the original casein
precipitate in a casserole and heat, on a wire gauze, over a free flame. As the
solution concentrates, a coagultmi consisting of lactalbumin and lactoglobulin
will form. Continue to concentrate the solution until the volume is about one-
half that of the original solution. Filter off the coagulable proteins (reserve the
filtrate) and test them as follows :

(a) Millon's Reaction. — Make the test according to the directions given on

page 97.

(b) Biuret Test. — Make the test according to the directions given on page 98.

(c) GlyoxyUc Acid Reaction fHopkins-Cole). — Make the test according to
the directions given on page 98.

16. Detection of Calcivun Phosphate. — ^Evaporate the filtrate from the
coagulable proteins, on a water-bath, until crystals begin to form. It may be

necessary to concentrate to 15 c.c. before any crys-
^ ^'^^^ tallization will be observed. Cool the solution, filter
off the crystals (reserve the filtrate), and test them
as follows:

(a) Microscopical Examination. — Examine the
crystals and compare them with those in Fig. 105.

(b) Dissolve the crystals in nitric acid. Test
part of the acid solution for phosphates. Render

Fig. 105. Calcium ^he remainder of the solution slightly alkaline with
ammonia, then acidify with acetic acid and add am-
moniimi oxalate. Examine the crystals xmder the microscope and compare
them with those in Fig. 134, page 459.

17. Detection of Lactose. — Concentrate the filtrate from the calcium phos-
phate until it is of a syrup-like consistency. Allow it to stand over night and
observe the formation of crystals of lactose. Make the following experiments.

(a) Microscopical Examination. — Examine the crystals and compare them
with those in Fig. 104, page 318.

(b) Fehling's Test.— Try Fehling's test upon the mother liquor.

(c) Phenylhydrazine Test. — Apply the phenylhydrazine test to some of the
mother liquor according to the directions given on page 22.

.MILK

323

18. Milk Fat. — (a) Evaporate the ether filtrate from the casein (Experiment
13) and observe the fatty residue. The milk fat was carried down with the
precipitate of casein and was removed when the latter was treated with ether.
If centrifugated milk was used in the preparation of the caseinogen the amount
of fat in the ether filtrate may be very small. To secure a larger yield of fat
proceed according to directions given under (b) below.

(b) To 25 c.c. of whole milk in an evaporating dish add a Uttle sand or filter
paper and evaporate the fluid to dryness on a water-bath. Grind or break up
the residue after cooUng and extract with ether in a flask. Filter and remove
the ether from the filtrate by evaporation. How can you identify fats in the
ethereal residue?

19. Saponification of Butter. — Dissolve a small amount of butter in alcohol
made strongly alkaUne with potassivmi hydroxide. Place the alcohoUc-potash
solution in a casserole, add about 100 c.c. of water and boil for 10-15 minutes or
until the odor of alcohol cannot be detected. Place the casserole in a hood and
neutraUze the solution with sulphuric acid. Note the odor of volatile fatty acids,
particularly butyric acid. Under certain conditions the odor of ethyl butjrrate
may also be detected.

20. Detection of Preservatives. — (a) Formaldehyde. — In these
tests tivo controls should be run, one with pure milk and one with
milk to which a very small amount of formaldehyde has been added.

I. Leach's Hydrochloric Acid Test. — Mix 10 c.c. of milk and 10 c.c. of con-
centrated hydrochloric acid containing about 0.002 gram of ferric chloride in a
small procelain evaporating dish or casserole and gradually raise the temperature
of the mixture, on a water-bath, nearly to the boiling-point, with occasional
stirring. If formaldehyde is present a violet color is produced, while a brown
color develops in the absence of formaldehyde. In case of doubt the mixture,
after having been heated nearly to the boiling-point for about one minute,
should be diluted with 50-75 c.c. of water, and the color of the diluted fluid
carefully noted, since the violet color if present will quickly disappear. For-
maldehyde may be detected by this test when present in the proportion i : 250,000.

II. Gallic Acid Test. — Acidify 30 c.c. of milk with 2 c.c. of normal sulphuric
acid and distil. Add 0.2-0.3 c.c. of a saturated alcoholic solution of gallic acid
to the first 5 c.c. of the distillate, then incline the test-tube and slowly introduce
3-5 c.c. of concentrated sulphuric acid, allowing it to run slowly down the side-
of the tube. A green ring, which finally changes to blue, is formed at the junc-
ture of the fluids. This is claimed, by Sherman, to be twice as delicate as either
the sulphuric acid or the hydrochloric acid test for formaldehyde.

{b) Salicylic Acid and Salicylates. — Remont's Method.' — Acidify 20 c.c. of milk
with sulphuric acid, shake well to break up the curd, add 25 c.c. of ether, mix thor-
oughly, and allow the mixture to stand. By means of a pipette remove 5 c.c. of the
ethereal extract, evaporate it to dryness, boil the residue with 10 c.c. of 40 per cent
alcohol, and cool the alcoholic solution. Make the volume 10 c.c, filter through
a dry paper if necessary to remove fat. and to 5 c.c. of the filtrate, which represents
2 c.c. of milk, add 2 c.c. of a 2 per cent solution of ferric chloride. The production
of a purple or violet color indicates the presence of salicylic acid.

' For other tests see Sherman's Organic .Analysis, Second Edition, p. 3 78.

324

PHYSIOLOGICAL CHEMISTRY

This test may form the basis of a quantitative method by diluting the final
solution to so c.c. and comparing this with standard solutions of salicylic acid.
The colorimetric comparisons may be made in a Duboscq colorimeter.

(c) Hydrogen Peroxide. — Add 2-3 drops of a 2 per cent aqueous solution of
para-phenylenediamine hydrochloride to 10-15 c.c. of milk. If hydrogen peroxide
is present a blue color will be produced immediately upon shaking the mixture or
after allowing it to stand for a few minutes. It is claimed that hydrogen peroxide
may be detected by this test when present in the proportion i : 40,000.

{d) Boric Acid and Borates. — To the ash, obtained accord-
ing to the directions given in Experiment 4, page 327, add 2
drops of dilute hydrochloric acid and i c.c. of water. Place a
strip of turmeric paper in the dish and after allowing it to soak
for about one minute remove it and allow it to dry in the air.
The presence of boric acid is indicated by the production of a
deep red color which changes to green or blue upon treatment
with a dilute alkali. This test is supposed to show boric acid
when present in the proportion i : 8000.

Quantitative Analysis of Milk

1. Specific Gravity. — This may be determined con-
veniently by means of a Soxhlet, Veith, or Quevenne
lactometer. A lactometer reading of 32° denotes a
specific gravity of 1.032. The determination should
be made at about 6o°F. and the lactometer reading
corrected by adding or subtracting 0.1° for every degree
F. above or below that temperature.

2. Fat. — (a) Babcock's Centrifugal Method.^ — Prin-
ciple.— The principle of this method is the destruction
of organic matter other than fat by sulphuric acid and
the centrifugation of the acid solution in the special
tube shown in Fig. 106 and the subsequent reading of
the percentage of fat by means of the tube's gradu-
ated neck. The method is one of the most satisfac-
tory in common use and is accurate to within 0.5 per
cent.

5C,c.i

Fig. 106. — Bab-
cock Tube.

Procedure. — By means of a special narrow pipette introduce milk into the
tube up to the 5 c.c. mark. Now add sufficient sulphxiric acid (sp. gr. 1.83-
1.834) to fill the body of the tube and rotate the tube to secure a homogeneous
acid-milk solution. Fill the neck of the tube with an acid-alcohol mixture.^
Centrifuge the tube and contents for one to two minutes and read off the per-
centage of fat by means of the graduated neck of the tube. If the top of the fat

' A modification of this method for use with sweetened dairy products, e.g., ice cream,
and entailing the use of a different type of centrifuge tube has been proposed by Halverson
{Jour. Ind. and Eng. Chem., 5, 403, 1913)- , , ...

2 This mixture consists of equal volumes of amyl alcohol and concentrated hydrochloric
acid.

MILK

325

column is not at zero it may be brought there by the addition of water and a
moment's recentrifugation.

In case very rich milk ('over 5 per cent fat 1 is under examination, it may be
diluted with an equal volume of water before examination and the fat percentage
multiplied by 2. In the examination of cream it is customary to dilute the sample
with four volumes of water and multiply the resultant fat value by 5.

(b) Quantitative Determination of Fat in Milk by the Meigs' Method with
Modification and Improved Apparatus by Croll.-— The method as stated by Dr.
Meigs is: Approximately 10 c.c. of milk is care-
fully weighed and transferred to an ordinary
100 c.c. glass-stoppered graduated cyUnder.
Twenty c.c. each of distilled water and ether
(0.720) are added, the ground-glass stopper
tightly inserted in the bottle, and the whole
shaken vigorously for five minutes. Then the
bottle is carefully unstoppered, 20 c.c. 95 per
cent alcohol added, the stopper reinserted and
again shaken for five minutes. The bottle is
now placed on a table and the contents will
separate into two distinct strata, the upper of
which contains practically all the fat. This
stratimi is carefully removed by a smaU pipette
and transferred to a carefully weighed glass
evaporating dish. The thin ether layer remain-
ing is washed by the addition of 5 c.c. of ether.
This is removed by pipetting off. This wash-
ing is repeated four times. On each addition
the sides of the bottle should carefuUy be
washed down by the fresh ether. Finally, the
pipette is rinsed with a little ether. The
evaporating dish with contents is now placed
on a safety water-bath and the ether evapo-
rated. The drying is continued in a hot-air
oven at a temperature below loo^C. and finally
completed in a desiccator to constant weight.

CroU's modification consists of subsequent
repeated extraction of the end-product of
evaporation with absolute ether. The com-
bined extracts are filtered and the small filter

paper is washed repeatedly with absolute ether. The combined extracts and
washings are evaporated and dried as before and then weighed.

The piece of apparatus shown in Fig. 107, above was also devised by Croll
to do away with the use of the pipette. ^ On closing the top with a finger and
blowing into the mouthpiece, the upper stratum is forced out into the dish. The
bottle is washed by simply pouring the ether into the tube. This lessens the
possibility of accidental loss.

^ Original paper by Dr. .Arthur V. Meigs in Philadelphia Medical Times, July i, 1882.
^ Croll: Biochem. Bull., 2, 509. 1913.

'If desired a cork with two tubes may be substituted for this somewhat complicated
apparatus.

Fig. 107. — Croll's Fat
ajppar.\tus.

326

PHYSIOLOGICAL CHEMISTRY

The accuracy of the method compared with that of the Soxhlet method,
using the paper-coil modification and extracting until fresh portions of absolute
ether gave no further trace of extractive material, is shown by the average

difference on twelve samples of human milk
being only 0.017 per cent less than by the
Soxhlet and on seven samples cow's milk being
only 0.019 per cent less. The extreme differ-
ences in case of the hrnnan milk were — 0.004
per cent and — 0.044 per cent and in case of
the cow's milk — 0.006 per cent and — 0.068 per
cent.

(f) Adams' Paper-coil Method. — Introduce
about 5 c.c. of milk into a small beaker, quickly
ascertain the weight to centigrams, stand a fat-
free coU^ in the beaker and incline the vessel
and rotate the coil in order to hasten the absorp-
tion of the milk. Immediately upon the com-
plete absorption of the milk remove the coU and
again quicklj^ ascertain the weight of the beaker.
The difference in the weights of the beaker at
the two weighings represents the quantity of
milk absorbed by the coil. Dry the coil care-
fully at a temperature below loo^C. and extract
it with ether for 3-5 hours in a Soxhlet appa-
ratus (Fig. 108). Using a
safety water-bath, heat the
flask containing the fat to
constant weight at a tempera-
ture below loo'^C.

Calculation. — Divide the
weight of fat, in grams, by
the weight of milk, in grams.
The quotient is the percentage
Fig. 108. — Soxhlet Apparatus, of fat contained in the milk

examined.

(d) Nephelometric Method of Bloor.- — This method is ex-
actly similar in principle and procedure to the method given
for the determination of fat in blood. (See page 295.) One
c.c. of milk is ordinarily taken.

(e) Approximate Determination by Feser's Lactoscope.
is opaque mainly because of the suspended fat globules and
therefore by means of the estimation of this opacity we may obtain data as to
the approximate content of fat. Feser's lactoscope (Fig. 109) may be used for
this purpose. Proceed as follows: By means of the graduated pipette accompany-
ing the instrument introduce 4 c.c. of milk into the lactoscope. Add water gradually,
shaking after each addition, and note the point at which the black lines upon the
inner white glass cylinder are distinctly visible. Observe the point on the graduated

^ Very satisfactory coils are manufactured by Schleicher and Schiill.
^ Bloor: J. Am. Chem. Soc, 36, 1300, 1914.

f\

— I

0^^

^j-ii. Fig. 109 — Feser's
' Lactoscope.

MILK

327

scale of the lactoscope which is level with the surface of the diluted milk. This
reading represents the percentage of fat present in the undiluted milk. Pure milk
should contain at least 3 per cent of fat.

3. Total Solids.' — Introduce 25 grams of milk into a weighed fiat-bottomed
platinum dish- and quickly ascertain the weight to milligrams. Expel the major
portion of the water by heating the open dish on a water-bath and continue the
heating in an air-bath or water oven at 97' ioo°C. until the weight is con-
stant. (If platinum dishes are employed this residue may be used in the
determination of ash according to the method described below, i

Calculation. 3 — Divide the weight of the residue, in grams, by the weight of
milk used, in grams. The quotient is the percentage of solids contained in the
milk examined.

4. Ash. — Heat the dry solids from 2-5 grams of milk, obtained according to
the method just given, over a very low flame ^ until a white or light gray ash is
obtained. Cool the dish in a desiccator and weigh. fThis ash may be used in
testing for borates according to directions on page 324.)

5. Proteins : Nephelometric Determination of Proteins, Casein,
Globulin, and Albumin in Milk. Method of Kober." — Principle. — The
proteins are precipitated with sulphosahcyhc acid and the precipitate
estimated nephelometricaliy (see discussion of nephelometric methods,
page 290J.

Procedure. — Five c.c. of milk are carefully measured into a 250 c.c. flask
and after adding 200 c.c. of distilled water and 10 c.c. of decinormal sodium
hydroxide solution, water is added to the mark and the mixture shaken. Ten
c.c. are put with exactly 2 c.c. of ether in a centrifuge tube which is then tightly
stoppered with a cork and vigorously shaken. Allow to separate and withdraw
5 c.c. of the aqueous layer without contamination with ether. Dilute to 50 c.c.
Take 10 c.c. of this solution and add 10 c.c. of 3 per cent sulphosaUcylic acid. A
suspension of casein is obtained which can be matched acciirately with the
following standard : i voliime (5 c.c.) of a o.oi per cent casein solution* to which
is added 2 volimies (10 c.c.) of 3 per cent siilphosahcylic acid.

The protein obtained with this reagent is not all casein, and in order to obtain
the exact amount of casein the casein is precipitated according to the "official

* Shackell's method for the vacuum desiccation of frozen preparations may be used
where great accuracy is desired (see American Journal of Physiology, 24, 325, 1909).

^Lead foil dishes, costing only about one dollar per gross, make a very satisfactory
substitute for the platinum dishes.

' The percentage of total solids may be calculated from the specific gravity and percentage
of fat bj' means of the following formula which has been proposed by Richmond:

3 = 0.25 L + i. 2 F+0.14
S = total solids.
L = lactometer reading.
F = fat content.

* Great care should be used in this ignition, the dish at no time being heated above a
faint redness, as chlorides may volatilize.

* Kober: /. Am. Chem. Soc, 35, 1585, 1913.

^Standard Casein Solution. — Dissolve with stirring o.i gram of casein or its equivalent
in r c.c. of o.i N NaOH, add 95 c.c. of distilled water, add 2 c.c. of toluene, shake thoroughly
and make up to 100 c.c. This is the stock solution which keeps three or four days or longer.
The standard solution is made up fresh every day by making 10 c.c. of the stock solution
up to 100 c.c. with water. The standard is controlled bj- total nitrogen estimations using
the factor 6.38 for casein.

328 PHYSIOLOGICAL CHEMISTRY

method" or the method of Hart given below and the amount of precipitate ob-
tained in an aliquot portion of the filtrate, by adding 4 volimies of the reagent,
is determined nephelometricaUy. This fraction, for want of a better name called
the "globulin and albimiin fraction," is subtracted from the gross casein, to
give the amount of casein precipitated by the "oflBcial method."

The ether used in extracting the fat increases the volume of the solution and
hence a factor allowing for this must be used. For 10 c.c. of diluted milk and
2 c.c. of ether the factor is 0.910.

6. Proteins. — Introduce a known weight of milk (5-10 grams) into a 500 c.c.
Kjeldahl digestion flask and add 20 c.c. of concentrated sulphuric acid and about
0.2 gram of copper sulphate. Expel the major portion of the water by heating
over a low flame and finally use a full flame and allow the mixture to boil one to
two hours. Complete the determination according to the directions given under
Kjeldahl Method, page 483.

Calculation. — Multiply the total nitrogen content by the factor 6.37^ to obtain
the protein content of the milk examined.

7. Hart's Casein Method.- — Introduce 10.5 c.c. of milk into a 200 c.c. Erlen-
meyer flask and add 75 c.c. of distilled water and 1-1.5 c.c. of 10 per cent acetic
acid.^ Mix the contents by giving the flask a vigorous rotary motion. The
precipitated casein is now filtered off upon a 9-1 1 cm. filter paper.* Wash out
the adsorbed and loosely combined acetic acid by means of cold water. Con-
tinue the washing of both the casein on the filter and that adhering to the flask,
until the wash water has reached a volume of at least 250 c.c.

Now return the precipitate and paper to the original Erlenmeyer flask, add
75-80 c.c. of neutral (carbon dioxide-free) water, 10 c.c. of N/io potassimn hy-
droxide and a few drops of phenolphthalein. Stopper the flask and shake it
vigorously, by hand or machine, until the casein has been brought into solution.^
Rinse the stopper with neutral (carbon dioxide-free) water and titrate the alka-
line casein solution at once with N/io hydrochloric acid until there is a dis-
appearance of all red color. ^

Calculation. — Subtract the corrected® acid reading from the 10 c.c. of alkali
used. The difference is the percentage of casein in the milk. For example, if
it takes 6.7 c.c. of N 10 hydrochloric acid to titrate the alkaline solution to the
end point and the check test was equivalent to 20 c.c. N/io acid the casein value
would be obtained as follows :

10 — (6.7+0.2) = 3.1 per cent casein

^ The usual factor employed for the calculation of protein from the nitrogen content is
6.25 and is based on the assumption that proteins contain on the average 16 per cent of
nitrogen. This special factor of 6.37 is used to calculate the protein content from the total
nitrogen, since the principal protein constituents of milk, i.e., casein and ladalbumin,
contain about 15.7 per cent of nitrogen.

*Hart: Jour. Biol. Chem., 6, 445, 1909.

• In general 1.5 c.c. of acetic acid gives a clear solution which filters nicely but occasion-
ally, when the milk has a low casein value it is advisable to use less acetic acid.

• The process of filtration may be retarded through the packing of the casein mass
upon the filter paper. In this case conduct a fine stream of cold water against the upper
point of contact of filter paper and casein. By this means the casein precipitate is loosened
and gathers in the apex of the filter. This procedure is very essential. It is not necessary
to^remove the casein which adheres to the interior of the flask.

' Solution is indicated by the disappearance of the white casein particles which would
otherwise settle to the bottom of the flask.

• A check test should be run parallel with the entire determination. Even with special
precautions as to neutrality, it is generally found that an acid check of 0.2-0.3 wUl be
obtained. This check titration should be added to the volume of acid used in titration.

MILK 329

8. Casein. — Mix about 20 grams of mUk with 40 c.c. of a saturated solution
of magnesuim sulphate and add the salt in substance until no more will dissolve.
The precipitate consists of casein admixed with a little fat and lacto-globulin.
Filter off the precipitate, wash it thoroughly with a saturated solution of magnesium
sulphate,^ transfer the filter paper and precipitate to a Kjeldahl digestion flask, and
determine the nitrogen content according to the directions given in a previous
experiment (6).

Calculation. — Multiply the total nitrogen by the factor 6.37 to obtain the casein
content.

9. Lactalbumin. — To the filtrate and washings from the determination of
casein, in Experiment 8, add Almen's- reagent until no more precipitate forms.
Filter off the precipitate and determine the nitrogen content according to the direc-
tions given under Proteins, page 328.

Calculation. — Multiply the total nitrogen by the factor 6.37 to obtain the lactal-
bumin content.

10. Lactose. — To about 350 c.c. of water in a beaker add 20 grams of milk,
mix thoroughly, acidify the fluid with about 2 c.c. of lo per cent acetic acid and
stir the acidified mixture continuously until a flocculent precipitate forms. At
this point the reaction should be distinctly acid to litmus. Heat the solution to
boiling for one-half hour, filter, rinse the beaker thoroughly, and wash the pre-
cipitated proteins and the adherent fat with hot water. Combine the filtrate
and wash water and concentrate the mixture to about 150 c.c. Cool the solution
and dilute it to 200 c.c. in a voliunetric flask. Titrate this sugar solution accord-
ing to directions given under Fehling's Method, page 523 or Benedict's Method,
page 522.

Myers' recommends the following procedure for the determination of lactose
in milk. One part of milk is mixed with an equal volume of phosphotungstic
acid solution ''yo.o grams acid and 200 c.c. cone. HCl in i Uter of water 1 and 2-3
parts of water. Mix well, filter until clear, and titrate the clear filtrate against
Benedict's solution (2$ c.c. reducing 67 mg. of lactose.)

The milk may also be clarified for the lactose determination by means of
altimintun hydroxide '' or dialyzed iron. * The dialyzed iron procedure is as follows:
Dilute 10 gm. of milk to 25 c.c. and add about 3 c.c. of 10 per cent colloidal iron
solution adding the last portion drop by drop to determine the exact amoxmt
necessary. Filter and wash with water to make the clear filtrate 100 c.c. Titrate
using Benedict's method (see page 522).

The preparation of aluminiiun hydroxide cream and its use in protein re-
moval are described under Nitrogen Partition, p. 485, Chapter XXVI.

Calculation. — Make the calculation according to directions given imder
Fehling's Method, page 523, bearing in mind that 10 c.c. of Fehling's solution
is completely reduced by 0.0676 gram of lactose.*

^ Preserve the filtrate and washings for the determination of lactalbumin (Expt. 9).
^Alm6n's reagent may be prepared by dissolving 5 grams of tannic acid in 240 c.c. of
50 per cent alcohol and adding 10 c.c. of 25 per cent acetic acid.

* Myers: Miinch. med. Woch., 59, 1494, 1912.

* Welker and Marsh: /. Am. Chem. Soc, 35, 823, 1913.
*Hill: Jour. Biol. Chem., 20, 175, 1915.

' In case Benedict's method is used it should be remembered that 25 c.c. of the reagent
is reduced by 0.067 gram of lactose.

CHAPTER XVIII
EPITHELIAL AND CONNECTIVE TISSUES

EPITHELIAL TISSUE (KERATIN)

The albuminoid keratin constitutes the major portion of hair, horn,
hoof, feathers, nails, and the epidermal layer of the skin. There is a
group of keratins the members of which possess very similar properties.
The keratins as a group are insoluble in the usual protein solvents and
are not acted upon by the gastric or pancreatic juices. They all re-
spond to the xanthoproteic and Millon reactions and are characterized
by containing large amounts of sulphur. Keratin from any of its
sources may be prepared in a pure form by treatment, in sequence, with
artificial gastric juice, artificial pancreatic juice, boiling alcohol, and
boiling ether, from twenty-four to forty-eight hours being devoted
to each process.

The percentage composition of some typical keratins is given in the
following table:

Source

Percentage composition

S

N

C

!
H

0

Nailsi

2 . 80

17-51

51.00

6.94

21.75 [

Honi2

3-20

50.86

6.94 '

w

e
1

3

X

Indian

4.82

15.40

44.06

6-53

29.19

Japanese . .

4-96

14.64

42.99

5-91

31-50

Negro ....

4.84

14.90

43-85

6-37

30.04

Caucasian

(adults)

' C.22

15-79

44-49

6.44

28.66

Caucasian (children)

4-93

1

14-58

43-23

6.46

30.80

The composition of human hair is influenced by its color and by the
race, sex, age and purity of breeding of the individual.^ It may be dif-

^ Mulder: Versuch einer allgetn. physiol. Chem., Braunschweig, 1844-51.
^ Horbaczewski: Ladenburg's Handworterhtich d. Chem., 3.
^ Rutherford and Hawk: Jour. Biol. Chem., 3, 459, 1907.

330

EPITHELIAL AND CONNECTR'E TISSUES 33 1

ferentiated from all other animal hair or wool by its high content of
cystine. Human hair may yield nearly 12 per cent of this amino-acid.^

Experiments on Epithelial Tissue

Keratin

Horn shavings or nail parings may be used in the experiments which
follow :

1. Solubility. — Test the solubility of keratin in water, dilute and concentrated
acid and alkali.

2. Millon's Reaction.

3. Xanthoproteic Reaction.

5. GlycxyUc Acid Reaction (Hopkins-Cole).

6. Test for Unoxidized Sulphur.

CONNECTIVE TISSUE

I. WHITE FIBROUS TISSUE

The principal solid constituent of white fibrous connective tissue
is the albuminoid collagen. This body is also found in smaller per-
centage in cartilage, bone, and ligament, but the collagen from the
various sources is not identical in composition. In common with the
keratins, collagen is insoluble in the usual protein solvents. It differs
from keratin in containing less sulphur. One of the chief character-
istics of collagen is, according to Hofmeister, the property of being
hydrolyzed by boiling acid or water with the formation of gelatin.
Emmett and Gies- claim that under these conditions there is an intra-
molecular rearrangement of collagen and the resultant gelatin is conse-
quently not the product of hydrolysis. The liberation of ammonia from
the collagen during the process apparently confirms this view. Collagen
gives Millon's reaction as well as the xanthoproteic and biuret tests.

The form of white fibrous tissue most satisfactory for general ex-
periments is the tendo Achillis of the ox. According to Buerger and
Gies'"^ the fresh tissue has the following composition:

Water 62.87%

Solids 37 ■ 13

Inorganic matter 0.47

Organic matter 36.66

Fattj' substance (ether-soluble) i .04

Coagulable protein 0.22

Mucoid 1.28

Elastin 1.63

Collagen 31-59

E.xtractives, etc 0.90

' Buchtala: Zeil. physiol. Clioii., 85, 24O, 1913.

^Emmett and Gies: Jour. Biol, cheni., 3, .\xxiii (Proceedings), 1907.

' Buerger and Bies: .-Iw. Jour. Physiol., 6, 219, 1901.

332 PHYSIOLOGICAL CHEMISTRY

The mucoid just mentioned is called tendomiicoid^ and is a glyco-
protein. It possesses properties similar to those of other connective-
tissue mucoids, e.g., osseomucoid and chondromucoid.

Gelatin, the body which results from the hydrolysis of collagen
(see statement of Emmett and Gies p. 331), is sometimes classed as an
albuminoid (see Chapter V). It responds to nearly all the protein
tests. It differs from the keratins and collagen in being easily digested
and absorbed. Gelatin is not a satisfactory substitute for the protein
constituents of a normal diet, however, since a certain portion of its
nitrogen is not available for the uses of the organism. Gelatin from
cartilage differs from gelatin from other sources in containing a lower
percentage of nitrogen. Tyrosine and tryptophane are not numbered
among the decomposition products of gelatin, hence it does not respond
to ]Millon's reaction or the glyoxylic acid reaction. Cystine is also
absent.

Experiments on White Fibrous Tissue

The tendo Achillis of the ox may be taken as a satisfactory type of
the white fibrous connective tissue.

I. Preparation of Tendomucoid. — Dissect away the fascia from about the
tendon and cut the clean tendon into small pieces. Wash the pieces in running
water, subjecting them to pressure in order to remove as much as possible of
the soluble protein and inorganic salts. This washing is very important. Trans-
fer the washed pieces of tendon to a flask and add 300 c.c. of half -saturated lime
water.- Shake the flask at intervals of twenty-four hours. Filter off the pieces
of tendon and precipitate the mucoid with dilute hydrochloric acid. Allow the
mucoid precipitate to settle, decant the supernatant fluid and filter the remainder.
Test the mucoid as follows :

(a) SolubiUty. — Try the solubility in water, sodixmi choride, dilute and con-
centrated acid and alkaU.

(b) Biuret Test. — First dissolve the mucoid in potassium hydroxide solution
and then add a dilute solution of copper sulphate.

(c) Test for Unoxidized Sulphur.

(d) Hydrolysis of Tendomucoid. — Place the remainder of the mucoid in a
small beaker, add about 30 c.c. of water and 2 c.c. of dilute hydrochloric acid
and boil until the solution becomes dark brown. Cool the solution, neutralize
it with concentrated potassium hydroxide, and test by Fehling's test. With a
reduction of Fehling's solution and a positive biuret test what do you conclude
regarding the nature of tendomucoid?

• 2. Collagen.— This substance is present in the tendon to the extent of
about 32 per cent. Therefore in making the following tests upon the pieces of
tendon from which the mucoid, soluble protein, and inorganic salts were removed
in the last experiment, we may consider the tests as being made upon collagen.

' Cutter and Gies: Am. Jour. Physiol., 6, 155, 1901.

2 Made by mixing equal volumes of saturated lime water and water from the faucet.

EPITHELIAL AND CONNECTIVE TISSUES ^^T,

(a) Solubility. — Cut the collagen into very fine pieces and try its solubility
in water and dilute and concentrated acid and alkali.

(b) Millon's Reaction.

(c) Biuret Test.

(d) Xanthoproteic Reaction.

(e) GlyoxyUc Acid Reaction THopkins-Colej.

(f ) Test for Unoxidized Sulphur. — Take a large piece of collagen in a test-
tube and add about 5 c.c. of potassium hydroxide solution. Heat until the
collagen is partly decomposed, then add 1-2 drops of lead acetate and again
heat to boiling.

(g) Formation of Gelatin from Collagen. — Transfer the remainder of the
pieces of collagen to a casserole, fill the vessel about two-thirds full of water
and boil for several hours, adding water at intervals as needed. By this means
the coUagen is transformed and a body known as gelatin is produced 'see page
322).

3. Gelatin. — On the gelatin formed from the transformation of collagen
in the above experiment (gj, or on gelatin furnished by the instructor make the
following tests :

(a) Solubihty. — Try the solubihty in the ordinary solvents (see page 21)
and in hot water.

(bj Millon's Reaction.

(c) Glyoxylic Acid Reaction rHopkins-Colei. — Conduct this test according
to the modification given on page 107.

(dj Test for Unoxidized Sulphur.

Make the following tests upon a solution of gelatin in hot water :

(a) Precipitation by Mineral Acids. — Is it precipitated by strong mineral
acids such as concentrated hydrochloric acid?

(b) Salting-out Experiment. — Saturate a Uttle of the solution with soUd
ammonium sulphate. Is the gelatin precipitated? Repeat the experiment
with sodiimi chloride. What is the result?

(cj Precipitation by Metallic Salts. — Is it precipitated by metallic salts such
as copper sulphate, mercuric chloride, and lead acetate?
(dj Coagulation Test. — Does it coagulate upon boiling?

(e) Precipitation by Alkaloidal Reagents. ^Is it precipitated by such reagents
as picric acid, tannic acid, and trichloracetic acid?

(f) Biuret Test. — Does it respond to the biuret test?

(g) Bardach's Reaction. — Does it yield the typical crystals of this reaction?
(See page loi.j

(h) Precipitation by Alcohol. — Fill a test-tube one-half full of 95 per cent
alcohol and pour in a small amount of concentrated gelatin solution. Do you
get a precipitate? How would you prepare pure gelatin from the tendo Achillis
of the ox?

II. YELLOW ELASTIC TISSUE (ELASTIN)

The ligamentum nucha of the ox may be taken as a satisfactory t\pe
of the yellow elastic connective tissue. The principal solid con-
stituent of this tissue is elastin, a member of the albuminoid group.

334 PHYSIOLOGICAL CHEMISTRY

In common with the keratins and collagen, elastin is an insoluble body
and gives the protein color reactions. It differs from keratin prin-
cipally in the fact that it may be digested by enzymes and that it
contains a very small amount of sulphur.

It has been demonstrated that elastin has the property of adsorb-
ing pepsin from the gastric juice and thus protecting it so the enzyme
can function later in the intestine^ (see Chapter on Gastric Digestion).

Yellow elastic tissue also contains mucoid and collagen but these are
present in much smaller amount than in white fibrous tissue, as may be
seen from the following percentage composition of the fresh ligamentum
nuchcB of the ox as determined by Vandegrift and Gies.^

Water 57-57%

Solids 42.43

Inorganic matter 0.47

Organic matter. 41 . 96

Fatty substance (ether-soluble) 1.12

Coagulable protein 0.62

Mucoid 0.53

Elastin 31-67

Collagen 7-23

Extractives, etc o . 80

Experiments on Elastin

1. Preparation of Elastin (Richards and Gies).^ — Cut the ligament into fine
strips, run it through a meat chopper and wash the finely divided material in cold,
running water for 24-48 hours. Add an excess of half-saturated lime water,
(see note at the bottom of page 332) and allow the hashed ligament to extract
for 48-72 hours. Decant the lime water, remove all traces of alkali by washing
in water and then boil in water with repeated renewals until only traces of protein
material can be detected in the wash water. Decant the fluid and boil the liga-
ment in 10 per cent acetic acid for a few hours. Treat the pieces with 5 per cent
hydrochloric acid at room temperature for a similar period, extract again in
hot acetic acid and in cold hydrochloric acid. Wash out traces of acid by means
of water and then thoroughly dehydrate by boihng alcohol and boihng ether
in turn. Dry in an air-bath and grind to a powder in a mortar.

2. Solubility. — Try the solubility of the finely divided elastin, prepared by
yourself or furnished by the instructor, in the ordinary solvents (see page 21).
How does its solubility compare with that of collagen?

3. Millon's Reaction.

4. Xanthoproteic Reaction.

5. Biuret Test.

6. Glyoxylic Acid Reaction (Hopkins-Cole). — Conduct this test according to
the modification given on page 107.

7. Test for Unoxidized Sulphur.

^ Abderhaldcn and Meyer: Zeit. physiol. Chem., 74, 67, 191 1.
- Vandegrift and Gies: Am. Jour. Physiol., 5, 287, 1901.
^ Richards and Gies: Am. Jour. Physiol., 7, 93, 1902.

EPITHELIAL AND CONNECTIVE TISSUES 335

III. CARTILAGE

The principal solid constituents of the matrix of cartilaginous tissue
are chondromucoid, chondroitin-sulphuric acid, chondroalbumoid and
collagen. Chondromucoid differs from the mucoids isolated from
other connective tissues in the large amount of chondroitin-sulphuric
acid obtained upon decomposition. Besides being an important
constituent of all forms of cartilage, chondroitin-sulphuric acid has
been found in bone, ligament, the mucosa of the pig's stomach, the
kidney of the ox, the inner coats of large arteries and in human urine.
It may be decomposed through the action of acid and yields a nitrogenous
body known as chondroitin and later this body yields chondrosin.
Chondrosin is also a nitrogenous body and has the power of reducing
Fehling's solution more strongly than dextrose. Levene and La Forge^
claim the reducing action of chondrosin to be due to an hexosamine
isomeric with glucosamine. Sulphuric acid is a by-product in the forma-
tion of chondroitin, and acetic acid is a by-product in the formation of
chondrosin.

Chondroalbumoid is similar in some respects to elastin and keratin.
It differs from keratin in being soluble in gastric juice and in containing
considerably less sulphur than any member of the keratin group. It
gives the usual protein color reactions.

Experiments on Cartilage

1. Preparation of the Cartilage. — Boil the trachea of an ox in water until
the cartilage rings may be completely freed from the surrounding tissue. Use
the cartilage so obtained in the following experiments :

2. Solubility. — Cut one of the rings into very small pieces and try the solubiUty
of the cartilage in water and dilute and concentrated acid and alkali.

3. Millon's Reaction.

4. Xanthoproteic Reaction.

5. Glyoxyhc Acid Reaction (Hopkins-Cole). — Conduct this test according to
the modification given on page 107.

6. Test for Unoxidized Sulphur.

7. Preparation of Cartilage Gelatin.^ — Cut the remaining cartilage rings
into small pieces, place them in a casserole with water and boil for several hours.
Filter while the solution is still hot. Observe that the filtrate soon becomes
more or less soUd. What is the reason for this? Bring a portion of the material
into solution by heat and try the following tests :

(a) Biuret Test.

(b) Bardach's Reaction.

(c) Test for Unoxidized Sulphur.

(d) To about 5 c.c. of the solution in a test-tube add a few drops of barium
chloride. Do you get a precipitate, and if so to what is the precipitate due?

^Levene and La Forge: Proc. Soc. cp. Biol, and Med., ii, 124, 1914.

336

PHYSIOLOGICAL CHEMISTRY

(e) To about 5 c.c. of the solution in a test-tube add a few drops of dilute
hydrochloric acid and boil for a few moments. Now add a little bariimi chloride
to this solution. Is the precipitate any larger than that obtained in the preceding
expeiment? Why?

(f) To the remainder of the solution add a Uttle dilute hydrochloric acid
and boil for a few moments. Cool the solution, neutraUze with solid potassimn
hydroxide, and try FehUng's test. Explain the result.

IV. OSSEOUS TISSUE

Of the solids of bone about equal parts are organic and inorganic
matter. The organic portion, called ossein, may be obtained by re-
moving the inorganic salts through the medium of dilute acid. Ossein
is practically the same body which is termed collagen in the other
connective tissues, and in common with collagen yields gelatin upon
being boiled with dilute mineral acid.

In common with the other connective tissues bone contains a
mucoid and an albuminoid. Because of their origin these bodies are
called osseomucoid and osseoalhumoid. Osseomucoid, when boiled with
hydrochloric acid, yields sulphuric acid and a substance capable of
reducing Fehling's solution. The composition of osseomucoid is very
similar to that of tendomucoid and chondromucoid (see page 113).

The inorganic basis of the dry, fat-free bone is a chemical substance,
not a mixture. This fact is indicated by the uniform composition of
the bones of fasting animals as well as by the definite relationship exist-
ing between the elements present. Bones of normal and fasting animals
of the same species present no profound differences in percentage com-
position. The percentage composition of the dry, fat-free femurs of two
dogs^ after the animals had fasted for 104 and 14 days respectively was
as follows:

Dog No.

Length of fast

Ash ■

N

CaO

MgO

P2O5

I.

104 days

1

61.50

4.6

33-3

0.8

12.80

2.

14 days

61.65

4.1

33-1

0.9

12.90

The marked uniformity in composition notwithstanding the wide
variation in the fasting periods is significant. The tensile strength of
the femur of the dog has been found to be at least 25,000 pounds to the
square inch^ whereas that of oak is 10,000 and that of cast iron 20,000
pounds to the square inch.

^ Johnston and Hawk : Unpublished data. For data on a 1 1 7-day fast by dog No. i, see
Howe, Mattill and Hawk: Jour. Biol. Chem., 11, 103, 1912.

epithelial and connective tissues 337

Experiment on Osseous Tissue

The percentage composition of normal human bone and of bone from
a case of osteomalacia is given in the following table :^

Constituent

Kind of bone

Normal i Osteomalacia

Calcium (CaO)

28.85 ' 15-44
0.14 0.57

19.55 12.01
0-14 0.55

Magnesium (MgO)

Phosphorus (P2O5)

Sulphur (S)

Qualitative Analysis of Bone Ash. — Take i gram of bone ash in a small
beaker and add a little dilute nitric acid. What does the effervescence indicate?
Stir thoroughly and when the major portion of the ash is dissolved add an equal
volume of water and filter. To the acid filtrate add ammonium hydroxide to
alkaline reaction. A heavy white precipitate of phosphates results. (What
phosphates are precipitated here by the ammonia?) Filter and test the filtrate
for chlorides, sulphates, phosphates, and calciimi. Add dilute acetic acid to
the precipitate on the paper and test a Httie of this filtrate for calcium and phos-
phates. Heat the remainder of the filtrate to boiUng and add (NH4)2C03 and
NH4CI slowly to this hot solution as long as a precipitate forms. Filter off the
precipitate of CaCOs and wash with hot water until free from alkaU.- Add a
solution of Na2HP04, make strongly alkaline with NH4OH, and note the forma-
tion of a white precipitate of ammonium magnesivim phosphate (NH4MgP04)
Examine the crystals under the microscope and compare with those shown in
Fig. 129, page 408. To the precipitate on the filter paper, which was insoluble
in acetic acid add a littie dilute hydrochloric acid and test this last filtrate for
phosphates and iron.

Reference to the following scheme may facilitate the analysis,

^ McCrudden: Jour. Biol. Cheni., 7, 199, 1910.

^ Magnesium is not precipitated here because of presence of NH4CI.

338

PHYSIOLOGICAL CHEMISTRY
BONE ASH.

Add dilute nitric acid, stir thoroughly and after the major portion of the ash has been
brought into solution add a little distilled water and filter.

Residue I. Filtrate I.

(discard) Add ammonium hydroxide to

alkaline reaction and filter.

Residue n.

Treat on paper with acetic acid.

Residue HI.

Treat on paper with hydro-
chloric acid.

I
Filtrate IV.
Test for:

1. Iron.

2. Phosphates.

Filtrate HI.
Test for:

1. Phosphates.

2. Calcium.

3. Magnesium

V. ADIPOSE TISSUE

Filtrate 11.

Test for:

1. Chlorides.

2. Sulphates.

3. Phosphates.

4. Calcium.

Adipose tissue consists almost entirely of a mixture of fats.
discussion and experiments see chapter on Fats, page 176.

For

CHAPTER XIX
MUSCULAR TISSUE

The muscular tissues are divided physiologically into the voluntary
(striated) and the involuntary (non-striated or smooth). In the
chemical examination of muscular tissue the voluntary form is gener-
ally employed. Muscle contains about 25 per cent of solid matter,
of which about four-fifths is protein material and the remaining one-
fiith extractives and inorganic salts.

The proteins are the most important of the constituents of muscular
tissue. In the living muscle we find two proteins, myosinogen and
para-myosinogen. These may be shown to be present in muscle plasma
expressed from fresh muscles. In common with the plasma of the
blood this muscle plasma has the power of coagulating, and the clot
formed in this process is called myosin. According to Halliburton^
and others in the onset of rigor mortis we have an indication of the for-
mation of this myosin clot within the body. The relation between the
proteins of living and dead muscle is represented graphically by Halli-
burton as follows:

Proteins of the living muscle.

Para-myosinogen (25%). Myosinogen (75%).

Soluble myosin.

Myosin.
(The protein of the muscle clot.)

Of the total protein content of living muscle about 75 per cent is
made up by the 7nyosinogen and the remaining 25 per cent is para-
myosinogen. These proteins may be separated by subjecting the
muscle plasnia to fractional coagulation in the usual way. Under
these conditions the para-myosinogen is found to coagulate at 47°C.
and the myosinogen to coagulate at 56°C. It is also claimed by some
investigators that it is possible to separate these two proteins by the
fractional ammonium sulphate method, but the possibility of making

' Halliburton: Biochemistry of Muscle and Xervc, 1904, p. 4.

339

340 PHYSIOLOGICAL CHEMISTRY

an accurate separation by this method is somewhat doubtful. It is
well established that para-myosinogen is a globulin since it responds to
certain of the protein precipitation tests and is insoluble in water.
Myosinogen, on the contrary, is not a typical globulin since it is
soluble in water. It has been called a pseudo-globulin. Myosin pos-
sesses the globulin characteristics. It is insoluble in water but soluble
in the other protein solvents and is precipitated from its solution upon
saturation with sodium chloride.

Mellanby has reported observations which he claims indicate that
there is only one protein in muscle and that rigor mortis is due to the
coagulation of this protein under the combined influences of the salt
present in the muscle and the lactic acid developed upon the death of
the muscle. He further states that the disappearance of rigor is due
to the fact that the lactic acid which is continually formed brings this
protein into solution. There is a difference of opinion as to whether
true rigor ever occurs in connection with non-striated (smooth)^
muscle.

Our ideas concerning the cause of rigor have undergone an im-
portant revision in recent years. A very attractive theory has been
advanced by Meigs^ and experimental confirmation has been accorded
it by von Fiirth and Lenk.^ According to this theory, rigor has no
connection with the coagulation of the muscle proteins and may even
be hindered or prevented by such coagulation. The cause of rigor,
from this new viewpoint, lies in the imbibition of water by the muscle
colloids. It is well known that colloids possess the property of absorb-
ing whatever fluid may be in contact with them. Moreover, the
capacity of the colloid for water is increased if the fluid is slightly acid
in reaction. Therefore the postmortem production of lactic acid
facilitates the imbibition of muscle fluid by the muscle colloids.
Under such conditions, the fibers swell, become rigid and the condition
known as rigor mortis results. The disappearance of rigor is believed
to be due to the coagulation of the muscle protein through the agency
of the accumulated lactic acid. This change is accompanied by a re-
lease of the imbibed water by the colloids, inasmuch as the capacity
of a colloid for retaining fluid is lowered by coagulation.

Under the name extractives we class a number of muscle constituents
which occur in traces in the tissue and may be extracted by water,
alcohol, or ether. There are two classes of these extractives, the non-
nitrogenous extractives and the nitrogenous extractives. Grouped under

^ Saxl: Beilriige zur cltemischen Physiologic und Pathologie, g, i, 1907.

* Meigs: American Journal of Physiology, 26, 191, 1910.

^ von Fiirth and Lenk: Wiener klinische Wochenschrift, 24, 1079, 1911.

MUSCULAR TISSUE 34 1

the non-nitrogenous bodies we have glycogen, dextrin, sugars, lactic
acid, inosite, C6H6(OH)6, and/a^. In the class of nitrogenous extract-
ives we have creatine, creatinine, xanthine, hypoxanthine, uric acid,
urea, carnine, guanine, phosphocarnic acid, inosinic acid, carnosine,
taurine, carnitine, novaine, ignotine, neosine, oblitine, carnomuscarine,
and methylguanidine (see formulas on pp. 127 and 346). Not all of
these extractives are present in the muscles of all species of animals.
Other extractives besides those enumerated above have been described
and there are undoubtedly still others whose presence remains undeter-
mined. A detailed consideration would, however, be unprofitable in
this place.

Glycogen is an important constituent of muscle. The content
of this polysaccharide in muscle varies and is markedly decreased by
intense muscular activity. It is transformed into sugar and used as
fuel. The liver is the organ which stores the reserve supply of glycogen
and transforms it into glucose which is passed into the blood stream
and so carried to the working muscle where it is synthesized into gly-
cogen. The glycogen thus formed is then changed into glucose as the
working muscle may need it.

Glycogen is a polysaccharide and has the same percentage com-
position as starch and dextrin. It resembles starch in forming an opal-
escent solution and resembles dextrin in being very soluble, in giving
reddish color with iodine and in being dextro-rotatory. Glycogen may
be prepared from muscle by extracting with boiling water and then
precipitating the glycogen from the aqueous solution by alcohol; dilute
or concentrated potassium hydroxide may also be used to extract the
glycogen. Glycogen may be prepared in the form of a white, tasteless,
amorphous powder. It is completely precipitated from its solution
by saturation with solid ammonium sulphate, but is not precipitated by
saturation with sodium chloride. It may also be precipitated by
alcohol, tannic acid, or ammoniacal basic lead acetate. It has the
power of holding cupric hydroxide in solution in alkaline fluids but
cannot reduce it. It may be hydrolyzed with the formation of glucose
by dilute mineral acids and is readily digested by amylolytic enzymes.

Mendel and Leavenworth have drawn the conclusion, from the ex-
amination of embryo pigs, that embryonic structures do not contain
exceptionally large amounts of glycogen. The distribution of tlie
glycogen was not observed to differ from that in the adult animal ex-
cept that the liver of the embryo does not assume its glycogen-stor-
ing function early. They further draw the conclusion that the meta-
bolic transformations of glycogen in the embryo and the adult are
entirely analogous.

342

PHYSIOLOGICAL CHEMISTRY

The lactic acid occurring in the muscular tissue of vertebrates is

paralactic or sarcolaclic acid,^

H OH

I !
H— C— C— COOH.

I !

H H

The reaction of an inactive living muscle is alkaline, but upon the death
of the muscle, or after the continued activity of a living muscle, the
reaction becomes acid, due to the formation of lactic acid. There is a
difference of opinion regarding the origin of this lactic acid. Some
investigators claim it to arise from the carbohydrates of the muscle,
while others ascribe to it a protein origin. The strongest evidence
favors a carbohydrate source. -

Fig. iio. — Creatine.

Among the nitrogenous extractives of muscle, those which are of the
most interest in this connection are creatine and the purine bases,
xanthine and hypoxanthine. Creatine is found in varying amounts in
the muscles of different species, the muscles of birds having shown
the largest amount. It has also been found in the blood, the brain, in
transudates and in the thyroid gland. Creatine may be crystallized
and forms colorless rhombic prisms (Fig. no) which are soluble in
warm water and practically insoluble in alcohol and ether. Upon
boiling a solution of creatine with dilute hydrochloric acid it is dehydro-
lyzed and its anhydride creatinine is formed. The theory that the

1 This is dextro-rotatory, whereas fermentation lactic acid (<i-Mactic acid) is optically
inactive.

''Levene and Meyer: Jour. Biol. Chem., ii, 361, 1912.

MUSCULAR TISSUE 343

creatine of ingested meat is transformed into creatinine and excreted
in the urine has been proven untenable through the researches of Folin,
Klercker, and Wolf and Shaffer. It is now known that under normal
conditions the ingestion of creatine in no way influences the excretion
of creatinine. In the case of Eck fistula dogs, however, London and
Bolyarski^ found ingested creatine to increase the output of creatinine
in the urine. This finding is of importance as throwing light upon the
role of the liver in creatine and creatinine metabolism. In this con-
nection it is important to note that there is no normal excretion of
endogenous (see page 378) creatine, a statement proven by the fact that
if no creatine be ingested none will be excreted. Folin- has shown that
the main bulk of ingested creatine is retained in the body, unless the diet
contains a large amount of protein material. In fasting the urine
contains considerable creatine, i.e., 120 mg. or more per day. Under
certain pathological conditions, e.g., fevers, the urine may contain
endogenous creatine which is probably derived from the catabolism
of muscular tissue, as Benedict, ]Mellanby, and Shaffer have suggested.
Benedict and Osterberg^ believe we may have a high creatine elimina-
tion which has no relation to the catabolism of muscle.

McCrudden'* reports creatine in the urine in cases of infantilism
achondroplasia and cretinism the amount present being increased
when the carbohydrate ingestion was increased.

It has been stated that creatine does not occur in non-striated
muscle. It has, however, been found in the non-striated muscles of
the lamprey the lowest form of vertebrates.^

Amberg and Morrill,*' Sedgwick.' Rose^ and Folin^ have shown that
creatine is a normal constituent of the urine of infants and children
(10-15 mg. per day). Folin explains this phenomenon on the basis of
the relatively high protein intake, whereas Rose believes it is due to a
peculiar carbohydrate metabolism. '

Besides being a normal constituent of muscle, xanthine has been
found in the brain, spleen, pancreas, thymus, kidneys, testicles, liver,
and in the urine. It may be obtained in crystalline form (Fig. in,
p. 344), but ordinarily it is amorphous. Xanthine is easily soluble in
alkalis, less soluble in water and dilute acids, and entirely insoluble in
alcohol and ether.

1 London and Bolyarskii: Zeit. phys. chem., 62, 465, 1909.

* Folin: Hammarsten Feslschrifl, p. 15.

'Benedict and Osterberg: Jour. Biol. Chem., 18, 195, 1914.

* Mc Crudden: Jour. Expi. Med., 15, 457, 191 2.

"Mellanby: Jour, of Physiol., 36, 472, 1908. Wilson: Jour. Biol. Chem., iS, 17, 1914-
•Amberg and Morrill: Jour. Biol. Chem., 3, 311, 1907.
"Sedgwick: Jour. Am. -Med. Ass'n, 55, 117S, 1910.

8 Rose: Jour. Biol. Chem., 10, 265, 191 1.

9 Folin: Ibid., 11, 253, 1912.

344

PHYSIOLOGICAL CHEMISTRY

Hypoxanthine occurs ordinarily in those tissues and fluids which
contain xanthine. It has been found, unaccompanied by xanthine, in
bone marrow and in milk. Unlike xanthine it may be easily crystallized
in the form of small, colorless needles. It is readily soluble in alkalis,
acids, and boiling water, less soluble in cold water and practically in-
soluble in alcohol and ether.

The predominating inorganic salt of muscle is potassium phosphate.
Besides this salt we have present chlorides and salts of sodium, calcium,
magnesium, and iron. Sulphates are also present in traces.

Mendel and Saiki have made some interesting observations upon the
chemical composition of non-striated or smooth (involuntary) mammalian

Fig. I II. — Xanthine.
A ter the drawings of Horbaczewski, as represented in Neubauer and Vogel. {Ogden.)

muscle, such as the urinary bladder and the muscular coat of the stom-
ach of the pig. Hypoxanthine was found to be the predominant purine
base present. Creatine and paralactic acid were also isolated. These
investigators were unable to demonstrate, definitely, the presence of
glycogen in the non-striated muscles studied, but state that "the
tissues possess the property of transforming glycogen in the char-
acteristic enzymatic way." The most important part of their in-
vestigation consists in a rather complete analysis of the inorganic
constituents of these muscles. A notable difference in the relative
distribution of the various inorganic constituents was observed, a
difference which, according to the authors, "can be accounted for in
part only by an admixture of lymph." The comparative composition
of the inorganic portion of striated and non-striated muscle and of blood
serum for comparison is shown in the following table:

MUSCULAR TISSUE

345

Per loo parts of fresh muscle

K20lNa20Fe203

Non-striated muscle (Mendel and Saiki)io. 08110.328

Skeletal muscle (Katz) 0.3060. 210

Blood serum (Abderhalden) ,0.02710.425

CaO ! MgO CI P2O6 H2O

o.oii 0.044I0.007I0.17110.184: 80.6
0.008 o. 01 1 0.047 0.048 0-487 72.9
|o.oi2 0.004 0.363:0.020 91 -8

An interesting comparative study of the ash of the smooth muscle of
the stomach of the frog and the striated muscle from the same animal
was very recently reported by Meigs and Ryan.^ Their data indicate
"that smooth muscle contains somewhat less potassium and phos-
phorus and somewhat more sodium and chlorine than the striated
muscle of the same animal, but that the differences in these respects
between the two tissues are not by any means so marked as has some-
times been supposed." Their average figures for each type of muscle
follow :

Per 100 parts of fresh muscle

Muscle

K

Na

Fe

Ca Mg

P CI S SoUds H2O

Striated o-35o 0.054 o.oio 0.028,0.030 0.155 0.066 o. 141 20. 13 79.87

Smooth o. 325I0. 073 jO. 0007 ■0.004I0. 013 10.137 jo. 1 20|o. 161 17.70 ,82.30

The preparation from which the above data for smooth muscle
were obtained were shown by histological examination to consist in
large part of smooth muscle fibers.

Muscular tissue is said to contain a reddish pigment called myo-
hematin, which is a derivative of hemoglobin.

The so-called "fatigue substances" of muscle are carbon dioxide,
paralactic acid, and potassium dihydrogen phosphate.

The ordinary commercial "meat extract" is composed principally
of the water-soluble constituents of muscle and contains practically
nothing of nutritive value. The protein material to which meat owes
its value as an article of diet is ordinarily practically all removed in
the preparation of the extract. Occasionally some preparations are
found to contain proteose, which is formed from the meat proteins in
the process of preparation.

Lusk- has shown that Liebig's extract is without influence upon the

^ Meigs and Ryan: Journal of Biological Chemistry, 11, 401, 191 2.
-Lusk: Jotir. Biol. Chetn., 13, 155, 1912.

346

PHYSIOLOGICAL CHEMISTRY

metabolism (energy) in spite of the glandular activity it is known to
induce.

The structural formulas of some of the nitrogenous extractives of
muscle are as follows:

NH2

HN = C

I
N.(CH3).CH2.COOH.

Creatine, CiHtNsOj.

M ethyl- guanidine acetic actd.

NH2

1

c=o

I

NH2

UREA.CON2H4.

o-

co

HN
HN = C

N.(CH3).CH2

Creatinine, C4H7N3O.
Creatine anhydride.

CH2.NH2
CH2.SO2OH

Taurine, C2H7NSO3.
Amino-ethyl sulphonic acid.

-CO

(CH3)3.N

CH2— CH.OH— CH2

Carnitine, CtHuNOs.
y-trimethyloxybutyrobetaine.

OH

(CH3)3N

CH2.CH2.CH2.CH(OH)2

NOVAINE, C7H17NO2.

Tri-methyl di-hydroxyhutyl ammonium hydroxide.

Carnosine, C9H14N4O3.

Neosine, C6H17NO2.

Ignotine, C9H14N4O3.

Phosphocarnic acid, C10H17N3O5 or C10H16N3O5.

Inosinic acid, (HO)2.PO.O.CH2(CHOH)3.CH:(C5H3N40).

Purine Bodies.^ —

HN— CO HN— CO

HC C— NH

/

CH

N— C— N

Hypoxanthine, C6H4N40.
6-oxypurine.

OC C— NH

>CH
HN— C— N

Xanthine, C6H4N4O2.
2-6-dioxypurine.

1 For discussion of the purine bodies which are found as muscle extractive see Chapter
VI on Nucleic Acids.

MUSCULAR TISSUE 347

HN— CO N = C.NH,

I I I I

H2N.C C— NH HC C— NH

N— C— H N— C— N

Guanine, CaHsNtO. Adenine. dUiSi.

2-amino~6-oxy purine. 6 -amino purine.

Experiments on Muscular Tissue

I. Experiments on "Living" Muscle

1. Preparation of Muscle Plasma (Halliburton).- Wash out the blood vessels
of a freshly killed rabbit with 0.9 per cent sodium chloride. This can best be
done by opening the abdomen and inserting a carmula into the aorta. Now
remove the skin from the lower limbs, cut away the muscles and divide them
into very small pieces by means of a meat chopper. Transfer the pieces of
muscle to a mortar and grind them with clean sand and a Uttle ice cold 5 per
cent magnesivmi sulphate. Place in an ice-box over night. Filter off the salted
muscle plasma and make the following tests :

(a) Reaction. — Test the reaction to litmus, phenolphthalein, and Congo red.
What is the reaction of this fresh muscle plasma?

(b) Fractional Coagulation. — Place a little muscle plasma in a test-tube and
arrange the apparatus for fractional coagulation as explained on page 105. Raise
the temperature very carefully from 30°C. and note any changes which may occur
and the exact temperature at which such changes take place. When the first
protein (para-myosinogen) coagulates filter it ofif and then heat the clear filtrate
as before, being careful to note the exact temperature at which the next coagula-
tion (myosinogen) occurs. There will probably be a preliminary opalescence
in each case before the real coagulation occurs. Therefore do not mistake the
real coagulation-point and filter at the wrong time. What are the coagulation
temperatures of these two proteins? Which protein was present in greater
amount?

(c) Formation of the Myosin Clot. — Dilute a portion of the plasma with 3
or 4 times its volimie of water and place it on a water-bath or in an incubator
at 35°C. for several hours. A typical myosin clot should form. Note the muscle
senun surrounding the clot. . Now test the reaction. Has the reaction changed,
and if so to what is the change due? Make a test for lactic acid. What do you
conclude?

2. I*reparation of Muscle Plasma (v. Fiirth). — Remove the blood-free muscles
of a rabbit as explained above. Finely divide by means of a meat chopper and
grind in a mortar with a little clean sand and some 0.9 per cent sodium chloride.
Wrap portions of the muscle in muslin and press thoroughly by means of a tincture
press or lemon squeezer. Filter and make the tests according to the directions
given in the last experiment.

3. **Fuchsin-frog" Experiment.— Inject a saturated aqueous solution of Fuch-
sin **S" into the lymph spaces of a frog two or three times daily for one or two
days, in this way thoroughly saturating the tissues with the dye. Pith the animal
(.insert a heavy wire or blunt needle through the occipito atlantoid membrane %
remove the skin from both hind legs and expose the sciatic nerve in one of them.

348 PHYSIOLOGICAL CHEMISTRY

Insert a small wire hook through the jaws of the frog and suspend the animal
from an ordinary clamp or iron ring. Pass electrodes imder the exposed
sciatic nerve, and after tying the other leg to prevent any muscular movement,
stimtilate the exposed nerve by means of make and break shocks from an in-
duction coil. The stimulated leg responds by pronounced muscular contrac-
tions, whereas the tied leg remains inactive. Continue the stimulation until
the muscles are fatigued. The muscular activity has caused the production of
lactic acid and this in turn has reacted with the injected fuchsin to cause a pink
or red color to develop. The muscles of the inactive leg still remain imchanged
in color.

The normal color of the Fuchsin "S" when injected was red, but upon being
absorbed it became colorless through the action of the alkalinity of the blood.
Upon stimulating the muscles, however, as above explained, lactic acid was formed
and this acid reacted with the fuchsin and again produced the original color of
the dye.

n. Experiments on "Dead" Muscle

1. Preparation of Myosin. — ^Take 25 grams of finely divided lean beef
which has been carefully washed to remove blood and lymph constituents and
place it in a beaker with 10 per cent sodivmi chloride. Stir occasionally for
several hours. Strain off the meat pieces by means of cheese cloth, filter the
solution and saturate it with sodium chloride in substance. Filter off the pre-
cipitate of myosin and make the tests as given below. This filtration will pro-
ceed very slowly. Myosin collects as a film on the sides of the filter paper and
may be removed and tested before the entire volume of fluid has been filtered.
If this precipitate remains for any length of time on the paper in contact with the
air it will become transformed into the protean myosan. Test the myosin pre-
cipitate as follows :

(a) Solubility. — Try its solubility in water, sodiimi chloride, dilute acid and
alkali. Is myosin an albumin or a globulin?

(b) Xanthoproteic Reaction. — See page 98.

(c) Coagulation Test. — Suspend a Uttle of the myosin in water in a test-
tube and heat to boiling for a few moments. Now remove the suspended ma-
terial and try its solubility in 10 per cent sodiimi chloride. What property does
this experiment show myosin to possess?

Test the filtrate from the original myosin precipitate as follows :

(a) Biuret Test. — ^What does this show?

(b) Place a little of the solution in a test-tube and heat to boiling. At the
boiling-point add a drop of dilute acetic acid and filter. Test this filtrate for
proteose with picric acid. Is any proteose present? Saturate another portion
of the filtrate with ammoniimi sulphate and test for peptone in the usual way
(see page 120). Do you find any peptone?

From your experiments on ''living" and "dead" muscle what are
your ideas regarding the proteins of muscle?

2. Preparation of Glycogen. — Grind a few oysters or scallops ^ in a mortar

^ Glycogen may also be prepared from the liver of an animal which has been fed a high
carbohydrate diet for 1-2 days previously. The best yield of glycogen can, however, gen-
erally be obtained from scallops. To secure best yield of glycogen the liver, scallops or
oysters should be fresh. If permitted to stand some glycogen will be converted into
glucose.

MUSCULAR TISSUE 349

with sand. Transfer to an evaporating dish, add water, and boil for 20 minutes.
Note the opalescence of the solution. At the boiUng-point faintly acidify with
acetic acid. Why is this acid added? Filter, and divide the filtrate into two
parts. Test one part of the filtrate as follows :

(a) Iodine Test. — To 5 c.c. of the solution in a test-tube add 5-10 drops of
iodine solution and 2-3 drops of 10 per cent sodium chloride. What do you
observe? Is this similar to the iodine test upon any other body with which we
have had to deal?

If difficulty is experienced in seciuing a satisfactory iodine test proceed
as follows: Make equal volumes of glycogen solution acid in reaction with
hydrochloric acid. Boil one solution to hydrolyze the glycogen. Add equal
voliunes of iodine solution to each and note the more pronounced iodine reaction
in the unhydrolyzed solution.

(b) Reduction Test. — Does the solution reduce Fehling's solution?

(c) Hydrolysis of Glycogen. — Add 10 drops of concentrated hydrochloric acid
to 10 c.c. of the solution and boil for 10 minutes. Cool the solution, neutraUze
with soUd potassium hydroxide and test with Fehling's solution. Does it still
fail to reduce FehUng's solution? If you find a reduction how can you prove the
identity of the reducing substance?

(d) Influence of SaUva. — Place 5 c.c. of the solution in a test-tube, add 5
drops of saUva and place on the bath-water at 40°C. for 10 minutes. Does this
now reduce Fehhng's solution?

To the second part of the glycogen filtrate add 3-4 voliunes of 95 per cent
alcohol. Allow the glycogen precipitate to settle, decant the supernatant fluid,
and filter the remainder. Heat the glycogen on a water-bath to remove the
alcohol, then subject it to the following tests :

(a) SolubiUty.— Try its solubiUty in water and 10 per cent sodium chloride
solution.

(b) Iodine Test. — Place a small amount of the glycogen in a depression of a
test-tablet and add 2-3 drops of dilute iodine solution and a trace of a sodiimi
chloride solution. The same wine-red color is observed as in the iodine test
upon the glycogen solution.

3. Testing for Inorganic Constituents. — (a) Examination of Ash of Muscle.—
Incinerate a small amount of muscular tissue, dissolve the ash in dilute hydro-
chloric acid. Test for potassium, phosphates, magnesium, calcium and chlorides.

(b) Demonstration of Phosphates and Magnesium in Muscle (Hiirthle's
Experiment). — Tease a very small piece of frog's muscle on a microscopical
sUde. Expose the sUde to ammonia vapor for a few moments, then adjust a
cover -glass, and examine the muscle fibers under the microscope. Note the
large number of crystals of ammonium magnesium phosphate, distributed every-

NH4-O

\
Mg-0-P=0

\/
O

where throughout the muscle fiber, thus demonstrating the abundance of phos-
phates and magnesium in the muscle (Fig. 129, page 408).

350 PHYSIOLOGICAL CHEMISTRY

Separation of Extractives from Muscles

1. Creatine. — Dissolve about lo grams of a commercial extract of meat in
200 c.c. of warm water (Test for Protein by Biuret and Coagulation Tests, see
Chapter V.) Precipitate the inorganic constituents by neutral lead acetate,
being careful not to add an excess of the reagent. "Write the equations for the
reactions taking place here. Allow the precipitate to settle, then filter and remove
the excess of lead in the warm filtrate by hydrogen sulphide. Filter while the solu-
tion is yet warm, evaporate the clear filtrate to a syrup, and allow it to stand at
least 48 hours in a cool place. Crystals of creatine should form at this point.
Examine under the microscope (Fig. no, page 342). Treat the syrup with 200
c.c. of 88 per cent alcohol, stir well with a glass rod to bring all soluble material
into solution, and then filter. The purine bases have been dissolved and are in
the filtrate, whereas the creatine crystals were insoluble in the 88 per cent alcohol
and remain on the filter paper. Wash the crystals with 88 per cent alcohol,
then remove them and bring them into solution in a little hot water. Decolorize
the solution by animal charcoal and concentrate it to a small volume. Allow
the solution to cool and note the separation of colorless crystals of creatine. ^

Make the following tests on the crystals :

(a) Microscopical Examination. — Examine some crystals under the micro-
scope and compare the form with those reproduced in Fig. no, page 342.

(b) Transformation of Creatine into Creatinine. — Dissolve the crystals in
about 30 c.c. of hot water. To one-half of the solution in a flask add an equal
volimie of normal hydrochloric acid and heat on a boiUng water-bath for five
hours with reflux condenser. The creatine has been changed into creatinine.
Apply tests for creatinine as given in Chapter XXII to the original solution as
well as to the acidified solution.

Diacetyl Reaction. — To 5 c.c. of a dilute creatine solution add an equal vol-
ume of saturated sodiimi carbonate solution and a few drops of a solution of
diacetyl. A pink color should develop. This test has been made the basis of a
method for the quantitative determination of creatine. ^

2. Hypoxanthine. — Evaporate the alcoholic filtrate from the creatine to
remove the alcohol. Make the solution ammoniacal and add ammoniacal silver
nitrate until precipitation ceases. The precipitate consists principally of hjrpo-
xanthine silver and xanthine silver. Collect these silver salts on a filter paper
and wash them with water. Place the precipitate and paper in an evaporating
dish and boil for one minute with nitric acid having a specific gravity of i.i.
Filter while hot through a double paper, wash with the same strength of nitric
acid and allow the solution to cool. By this treatment with nitric acid hypo-
xanthine silver nitrate and xanthine silver nitrate have been formed. The
former is insoluble in the cold solution and separates on standing. After standing
several hours filter off the hypoxanthine silver nitrate and wash with water until
the wash water is only slightly acid in reaction. Examine the crystals of hypo-
xanthine silver nitrate under the microscope and compare them with those' in
Fig. 84, above. Now wash the crystals from the paper into a beaker with a Uttle
water and warm the liquid. Remove the silver by hydrogen sulphide and filter.

^ For an improved method of preparing pure creatine from creatinine see chapter on
Physiological Constituents of the Urine.
^ Walpole: Jour. Physiol., 42, 301, 1911.

MUSCULAR TISSUE

351

By this means hypoxanthine nitrate has been formed and is present in the filtrate.
(For crystalUne form of hypoxanthine nitrate see Fig. 40, p. 136.) Concentrate
on a water-bath to drive ofif hydrogen sulphide, and render the solution sUghtly
alkaUne with ammonia. Warm for a time, to remove the free ammonia, filter.

Fig. 112. — Hypoxanthine Silver Nitrate.
(Drawn from a student preparation by Dr. E. F. Hirsch.)

concentrate the filtrate to a small volume and allow it to stand in a cool place.
Hypoxanthine should crystaUize in small colorless needles. Examine the
crystals under the microscope.

3. Xanthine. — To the filtrate from the above experiment containing the

Fig. 113. — Xanthine Silver Nitrate.

xanthine silver nitrate add ammonia in excess. (The crystalhne form of xan-
thine silver nitrate is shown in Fig. 113.) A brownish -red precipitate of
xanthine silver forms. Treat this suspended precipitate with hydrogen sulphide
(do not use an excess of hydrogen sulphide), warm the mixture for a few mo-

o^2 PHYSIOLOGICAL CHEMISTRY

ments and filter whUe hot. Concentrate the filtrate to a small volume and put
away in a cool place for crystallization (Fig. in, page 344). To obtam xanthine
in crystalline form special precautions are generaUy necessary. Evaporate the
solution to dryness and test according to directions given in Chapter VI on
Nucleic Acids.

CHAPTER XX
NERVOUS TISSUE

In common with the other sohd tissues of the body, nervous tissue
contains a large amount of water. The percentage of water present
depends upon the particular form of nervous tissue but in all forms it is
invariably greater in the gray matter than in the white. Embryonic
nervous tissues also contain a larger percentage of water than the tissues
of adult life. The gray matter of the brain of the foetus, for instance,
contains about 92 per cent of water, whereas the gray matter of the
brain of the adult contains but 83-84 per cent of the fluid.

Among the solid constituents of nervous tissue are proteins, choles-
terol, cerchrosides (cerebrin, etc.), lecithin, kephalin, protagon {?), para-
nucleoprotagon, miclein, neurokeratin, collagen, extractives, and inorganic
salts. The proteins are present in the greatest amount and comprise
about 50 per cent of the total solids. Three distinct proteins, two
globulins, and a nucleoprotein, have been isolated from the nervous
tissue. The globulins coagulate at 47°C. and 7o-75°C., respectively,
while the nucleoprotein coagulates at 56-6o°C. This nucleoprotein
contains about 0.5 per cent of phosphorus (Halliburton, Levene.)
Nervous tissue is composed of a relatively large quantity of a variety
of compounds which collectively may be grouped under the term
"lipoid" — substances resembling the fats in some of their physical
properties and reactions but distinct in their composition. We will
class cholesterol, the cerebrosides and the phosphorized fats as lipoids.

The consideration of lipoids (or lipins'^) is assuming added impor-
tance. These substances constitute one of the two great groups of
tissue colloids, the proteins being the remaining group. So far as struc-
ture and chemical properties are concerned the various classes of lipoids
are entirely unlike.

The group of phosphorized fats are very important constituents of
nervous tissue. The best known members of this group are IccitJiin
prolagon (?) and kephalin. Lecithin occurs in larger amount than
the other members of the group, has been more thoroughly studied
than the others and is apparently of greater importance. Upon de-
composition lecithin yields fatty acids, glycero- phos phoric acid, and

' Rosenbloom and Gics: Biochemical Bulletin, i, 51, 191 1. The term lipoid was intro-
duced by Overton (Studien iiber die Narkose, Jena, 1901, Gustav Fischer).

23 353

354 PHYSIOLOGICAL CHEMISTRY

choline. Each lecithin molecule contains two fatty acid radicals

which may be those of the same or different fatty acids. Thus we have

different lecithins depending upon the particular fatty acids radicals

which are present in the molecule. The formula of a typical lecithin

would be the following.

CHo— OOC.C17H30

I
CH— OOC.C17H35

I
CH2O— PO— O.C2H4

\
(CH3)3 = N

/
OH HO

This lecithin would be called distearyl-lecithin or choline-distearyl-
glycero-phosphoric acid. Upon decomposition the molecule splits ac-
cording to the following reaction:

C44H90NPO9 + 3H2O -^ 2C18H36O2 + C3H9PO6 + C6H15NO2.

Lecithin. Stearic acid. Glycero-phosphoric acid. Choline.

The lecithins are not confined to the nervous tissues but are found in
nearly all animal and vegetable tissues. Lecithin is a primary con-
stituent of the cell. It is soluble in chloroform, ether, alcohol, benzene,
and carbon disulphide. The chloroform or alcohol-ether solution
may be precipitated by acetone. Lecithin may be caused to crystal-
lize in the form of small plates by cooling the alcoholic solution to a
low temperature. It has the power of combining with acids and bases,
and the hydrochloric acid combination has the power of forming a
double salt with platinic chloride.

Choline, as was indicated above, is one of the decomposition
products of lecithin. It is trimethyl-hydroxyethyl-ammonium hydroxide
and has the following formula:

CHz.CHaCOH)

/

N^(CH3)3

\
OH

Researches have shown that great importance is to be attached to the
detection of choline in the cerebro-spinal fluid and the blood in certain
cases of degenerative disease of the nervous system. In this connec-
tion tests for choline (see page 357) are of interest and value.

Protagon, another nitrogenous phosphorized substance, is a body
over which there has been much discussion. Upon decomposition it

NERVOUS TISSUE 355

is said by some investigators to yield cerebrin and the decomposition
products of lecithin. It has been shown by Posner and Gies^ as well
as by Rosenheim and Tebb- that protagon is a mixture and has no
existence as a chemical individual. Koch' reported data obtained
from purified preparations which indicate that protagon contains at
least three substances: "a phosphatide containing cholin, a cerebro-
side containing sugar, a complex combination of a cholin-free phos-
phatide with a cerebroside to which an ethereal sulphuric acid group
is attached." On the basis of his data, he believed the term pro-
tagon to have no chemical significance. He proposed the term sul-
phatide. Koch's preparation analyzed as follows (per cent) :

Choline Sugar Nitrogen Phosphorus Sulphur

i.o 12. o 2,3 1.7 1.9

He suggested the following structure:

O

11

Phosphatide^ — O — S — O — Cerebroside

grouping |, grouping

O

Kephalin is the third member of the group of phosphorLzed fats.
It is precipitated from its acetone-ether extract by alcohol. It contains
about 4 per cent of phosphorus and has been given the formula C42H79-
NPO13. Kephalin may be a stage in lecithin metabolism.

The cerebrosides are substances containing nitrogen but no phos-
phorus, and are important constituents of the white matter of nervous
tissue. Certain ones have also been found in the spleen, pus, and in egg
yolk. They may be extracted from the tissue by boiling alcohol and are
insoluble in cold alcohol, cold and hot ether, and in water and dilute
alkalis. The cerebroside termed cerebrin is a mixture containing phre-
nosin (pseudo-cerebrin or cerebron), a body yielding the carbohydrate
galactose on decomposition.

Cholesterol, one of the primary cell constituents, is present in fairly
large amount in nervous tissue. It occurs in two forms, i.e., free and
combined as an ester. It is claimed* that 99 per cent of the choles-
terol of brain tissue (boy) is in the free state. It is a mon-atomic
alcohol containing at least one double bond and possesses the formula
C27H46OH or C27H43OH. There is still some uncertainty as to the
exact structure of cholesterol. It may possess a terpene structure. It

^ Posner and Gies: Journal of Biological Chemistry, i, 59, 1905-06.
^ Rosenheim and Tebb: Journal of Physiology, 36 and 37, 1907-8.
' Koch: Journal Biological Chemisly, ii, March, 191 2, Proceedings.
*Lapworth: Jour. Path. Bad., 1911, p 256.

356 PHYSIOLOGICAL CHEMISTRY

was formerly called a " non-saponifiable fat" but since it is not changed
in any way by boiling alkalis it is not a fat. It is soluble in ether,
chloroform, benzene, and hot alcohol. It crystallizes in the form of
thin, colorless, transparent plates (Fig. 57, page 210). Cholesterol
is present in bile, occurs abundantly in one form of biliary calculus.
It is also present in blood and its quantitative determination is of
clinical importance (see Chapter XVI). It has been found in feces,
wool fat, egg yolk, and milk, frequently in the form of its esters of
higher fatty acids. It is generally believed that the cholesterol present
in the animal body has its origin in the vegetable kingdom. Some
evidence has been submitted^ indicating a synthesis of cholesterol
under certain conditions in the animal body. However, it is probable
that cholesterol is not readily synthesized in the body.-

Paranucleoprotagon is a phosphorized substance originally isolated
from brain tissue by Ulpiani and Lelli and recently reinvestigated by
Steel and Gies. It is said to possess lecithoprotein characteristics.

Nervous tissue yields about i per cent of ash which is made up in
great part of alkaline phosphates and chlorides.

Experiments on the Lipoids of Nervous Tissue^

1. Preparation of Lecithin.^ — Treat the finely divided brain of a sheep with
ether and allow it to stand in the cold for 48-72 hours. The cold ether will ex-
tract lecithin and cholesterol. Filter and add acetone to the filtrate to pre-
cipitate the lecithin. Filter off of the lecithin and test it as follows :

(a) Microscopical Examination. — Suspend a small portion in a drop of
water on a sUde and examine under the microscope.

fb) Osmic Acid Test.^ — Treat a small portion with osmic acid. What
happens?

(c) Acrolein Test. — Make the acrolein test according to directions on page
180.

(d) Test for Phosphorus. — See page 129, Chapter VI.

2. Preparation of Cholesterol. — Place a small amount of finely divided brain
tissue under ether and stir occasionally for one hour. Filter, evaporate the
filtrate to dryness on a water-bath, and test the cholesterol according to direc-
tions given below. (If it is desired, the ether extract from the so-called protagon,

1 Klein: Biochem. Zeit., 30, 465, 1910.

2 Gardner and Lander: Proc. Royal Soc, London (B), 87, 229, 1913.
^Preparation of So-called Protagon. — Divide the brain of a sheep into small pieces,

treat with 85 per cent alcohol and warm on a water-bath 45°C. for two hours. Filter hot
into a bottle or strong flask and cool to o°C. for one-half hour by means of a freezing mix-
ture. By this procedure both protagon and cholesterol are caused to precipitate. Filter
the cold solution rapidly and treat the precipitate on the paper with ice cold ether to dis-
solve out the cholesterol. The protagon may now be redissolved in warm 85 per cent
alcohol from which solution it will precipitate upon cooling.

* For the preparation of lecithin in purer form see MacLeon: Jour. Path. Bad., 18, 490,

^ Osmic acid serves to detect fats which contain unsaturated fatty acid radicals, e.g.,
oleic acid, in their molecule.

NERVOUS TISSUE

357

or the ether-acetone filtrate from the lecithin may be used for the isolation of
cholesterol. In these cases it is simply necessary to evaporate the solution to
dryness on a water-bath. ) Upon the cholesterol prepared by either of the above
methods make the following tests :

((7) Microscopical Examination. — Examine the crystals under the microscope
and compare them with those in Fig. 57, page 210.

(b) HjSOi Test (Salkowskii. — Dissolve a few crystals of cholesterol in a
little chloroform and add an equal volume of concentrated sulphuric acid.
A play of colors from bluish-red to cherry-red and purple is noted in the chloro-
from, while the acid assumes a marked green fluorescence.

(c) Acetic Anhydride- Hi^SO^ Test (Liebermann-Burchard*. — Dissolve a few
crystals of cholesterol in 2 c.c. of chloroform in a dry test-tube. Now add 10
drops of acetic anhydride and 1-3 drops of concentrated ^Iphuric acid. The
solution becomes red, then blue, and finally bluish-green in color.

(d) Iodine-sulphuric Acid Test. — Place a few crystals of cholesterol in one of
the depressions of a test-tablet and treat with a drop of concentrated sulphuric acid
and a drop of a very dilute solution of iodine. A play of colors, consisting of violet,
blue, green, and red, results.

(e) Schif's Reaction. — To a little cholesterol in an evaporating dish add a few
drops of a reagent made by adding i volume of 10 per cent ferric chloride to 3 vol-
umes of concentrated sulphuric acid. Evaporate to drj'ness over a low flame and
observe the reddish-violet residue which changes to a bluish- violet.

(/) Phosphorus. — Test for phosphorus according to directions given in Chapter
VI, page 129. Is phosphorus present?

3. Preparation of Cerebrin. —Treat 100 grams of finely divided brain tissue,
in a flask, with 200 c.c. of 95 per cent alcohol and boil on a water-bath for one-
half hour, keeping the volume constant by adding fresh alcohol as needed or by
the use of a reflux condenser. Filter the solution hot and stand the cloudy
filtrate away for 24 hours. (If the filtrate is not cloudy concentrate it upon the
water-bath until it is so.j Filter off the cerebrin (cerebrin, lecithin, kephaUn,
cholesterol 1 and test it as follows :

fa) Microscopical Examination. — Suspend a small portion in a drop of water
on a slide and examine under the microscope.

(bi SolubiUty. — Try the solubiUty of cerebrin in water, 10 per cent sodium
chloride and in dilute acid and alkaU, and in hot and cold alcohol and hot and
cold ether.

(c) Phosphorus. — Test for phosphorus according to directions in Chapter
VI, page 129. How does the result compare with that on lecithin?

(dj Place a Uttle cerebrin on platinum foil and warm. Note the odor.

(e) Hydrolysis of Cerebrin. — Place the remaining cerebrin in a small evaporat-
ing dish, add equal volumes of water and dilute hydrochloric acid, and boil for
one hour. Cool, neutralize with sohd potassium hydroxide, filter, and test
with Fehling's solution. Is there any reduction, and if so how do you explain
it?

4. Tests for ChoUne. (a) Rosenheim's Per iodide rt'^/.— Prepare an alcoholic
extract of the fluid under examination, and after evaporation apply Rosenheim's
iodo-potassium iodide solution' to a little of the residue. In a short time dark

' Prepared by dissolving 2 grams of iodine and 6 grams of potassium iodide in 100 cc.

water.

358 PHYSIOLOGICAL CHEMISTRY

brown plates and prisms of choline periodide begin to form and may be detected by
means of the microscope. Occasionally they are large enough to be visible to the
naked eye. They somewhat resemble crystals of hemin (see page 265). If the
slide be permitted to stand, thus allowing the fluid to evaporate, the crj'stals will
disappear and leave brown oUy drops. They will reappear, however, upon the
addition of fresh iodine solution, v. Stanek claims that this choline compound
has the formula CsHnNOI.Ig.

{h) Rosenheim' s Bismuth Test. — Extract the fluid under examination with
absolute alcohol, evaporate, and reextract the residue. Repeat the extraction
several times. Dissolve the final residue in 2-3 c.c. of water and add a drop of
Kraut's reagent.^ Choline is indicated by the appearance of a bright brick-red
precipitate.

^ Dissolve 272 grams of potassium iodide in water and add 80 grams of bismuth sub-
nitrate dissolved in 200 grams of nitric acid (sp. gr. 1.18). Permit the potassium nitrate to
crystallize out, then filter it off and make the filtrate up to i liter with water.

CHAPTER XXI

URINE: GENERAL CHARACTERISTICS OF NORMAL AND
PATHOLOGICAL URINE

Volume. — The volume of urine excreted by normal indiv-iduals
during any definite period fluctuates within very wide limits. The
average output for twenty-four hours is placed by German writers
between 1500 and 2000 c.c. This value is not strictly applicable to con-
ditions in America, however, since it has been found that the average
normal excretion of the adult male American falls within the lower
values of 1000-1200 c.c. The volume-excretion is influenced greatly
by the diet, particularly by the ingestion of fluids.

Certain pathological conditions cause the output of urine for any
definite period to depart very decidedly from the normal output.
Among the pathological conditions in which the volume of urine is i«-
creased above normal are the following: Diabetes mellitus, diabetes
insipidus, certain diseases of the nervous system, contracted kidney,
amyloid degeneration of the kidney, and in convalescence from acute
diseases in general. Many drugs such as calomel, digitalis, acetates,
and salicylates also increase the volume of the urine excreted. A
decrease from the normal is observed in the following pathological
conditions: Acute nephritis, diseases of the heart and lungs, fevers,
diarrhoea, and vomiting.

Color. — Normal urine ordinarily possesses a yellow tint, the depth
of the color being dependent in part upon the density of the fluid. The
color of normal urine is due principally to a pigment called nrochrome:^
traces of hemato porphyrin, urobilin, and uroerythrin have also been
detected. Under pathological conditions the urine is subject to pro-
nounced variations in color and may contain many varieties of pig-
ments. Under such circumstances the urine may vary in color from an
extremely light yellow to a verj^ dark brown or black. Vogel has con-
structed a color chart which is of some value for purposes of comparison.
The nature and origin of the chief variations in the urinary color are set
forth in tabular form by Halliburton as follows:

^ Urochrome is believed to be identical with the yellow pigment (lactochrome) of milk
whey (Palmer and Coolidge: Jour. Biol. C/tem., 17, 251, 1914).

359

360 PHYSIOLOGICAL CHEMISTRY

Color

Cause of coloration

Pathological condition

Nearly colorless

Dilution, or diminution of
normal pigments.

' Nervous conditions: hy-
druria, diabetes insipidus,
granular kidney.

Dark j^ellow to brown- red. .

Increase of normal, or oc-
currence of pathological,
pigments. Concentrated
urine.

Acute febrile diseases.

MUky

Fat globules

Chyluria.

Pus corpuscles

Purulent diseases of the
urinary tract.

Orange

Excreted drugs

Santonin, crysophanic acid.

Red or reddish

Hematoporphyrin

Unchanged hemoglobin

Hemorrhages, or hemoglo-
binuria,.

Pigments in food (logwood,
madder, bilberries, fuchsin).

Brown to brown black

Hematin

Small hemorrhages.

Methemoglobin

Methemoglobinuria.

Melanin

Melanotic sarcoma.

Hydrochinol and catechol . .

Carbolic-acid poisoning.

Greenish yellow, greenish
brown, approaching black..

Bile-pigments

Jaundice.

1
Dirty green^ or blue

A dark blue scum on surface,
with a blue deposit, due to
an excess of indigo-forming
substances.

Cholera, typhus; seen espe-
cially when the urine is
putrefying.

Brown-yellow to red-brown,
becoming blood-red upon
adding alkalis.

Substances contained in
senna, rhubarb and cheli-
donium which are intro-
duced into the system.

Transparency. — Normal urine is ordinarily perfectly clear and
transparent when voided. On standing for a variable time, however, a
cloud (nubecula) consisting principally of nucleoprotein or mucoid (see
page 396) and epithelial cells forms. A turbidity due to the precipita-
tion of phosphates is normally noted in urine passed after a hearty

1 This dirty green or blue color also occurs after the use of methylene blue in the
organism.

URINE 361

meal. The urine obtained 2-3 hours after a meal or later is ordinarily
free from turbidity. Permanently turbid urines ordinarily arise from
pathological conditions.

Odor. — The odor of normal urine is of a faint, aromatic type. The
bodies to which this odor is due are not well known, but it is claimed by
some investigators to be due, at least in part, to the presence of minute
amounts of certain volatile organic acids. Dehn and Hartman^ have
recently succeeded in isolating from urine a neutral ill-smelling substance
which they call urinod. Its empirical formula is CeHsO. Urinod occurs
in urine to the extent of only 1-2 parts in 100,000 parts of urine.
When the urine undergoes decomposition, e.g., in alkaline fermentation,
a very unpleasant ammoniacal odor is evolved. All urines are subject
to such decomposition if allowed to stand for a sufficiently long time.
Under normal conditions the urine very often possesses a peculiar odor
due to the ingestion of some certain drug or vegetable. For instance,
cubebs, copaiba, myrtol, saffron, tolu, and turpentine each imparts a
somewhat specific odor to the urine. After the ingestion of asparagus,
the urine also possesses a typical odor due to the formation of methyl
mercaptan (CH3 SH) in the intestine.

Frequency of Urination. — 'The frequency of urination varies greatly
in different individuals, but in general is dependent upon the amount of
fluid in the bladder. In pathological conditions an inflammatory affec-
tion of the urinary tract or any disturbance of the innervation of the
bladder will influence the frequency. Affections of the spinal cord
which lead to an increased irritability of the bladder or a weakening of
the sphincter, or any condition lowering the residual capacity of the
bladder, will result in increasing the frequency of urination.

Reaction. — The mixed 24-hour urinary excretion ot a normal indi-
vidual ordinarily possesses an acid reaction to litmus. This acidity in
normal cases is represented on the average by a hydrogen ion concentra-
tion of loXio"^, although it may vary from 0.40 to 150X10"'. The
reaction of the urine represents an equilibrium between a large number
of acid and basic constituents, both organic and inorganic, which it con-
tains. Organic acids and bases play a part in producing the normal
reaction, but this is probably, in the main, dependent upon the relative
amounts of the mono- and dibasic sodium and potassium phosphates.
The monobasic sodium phosphate (XaH>P04) is acid in reaction, while
the dibasic phosphate (Na2HP04) is alkaline in reaction. The ex-
cretion of acid or alkaline phosphate by the kidneys is one of the factors
in the regulation of the neutrality of the blood and of the organism
in general. The acidity of the urine as determined by titration runs

'Dehn and Hartman: Jour. .\m. Chan. Soc, 36, 2136 1914.

362

PHYSIOLOGICAL CHEMISTRY

in general parallel with the hydrogen ion concentration and seems to be
dependent upon the same factors, and in more acid urines mainly on
the phosphate content. (For further discussion of acidity see Chapter
VIII on Gastric Analysis.)

The mean acidity in cardio-renal diseases is high — about 50X10" '^
as compared with loXio"^, the normal mean. In general the acidity
tends to be increased in the greater number of pathological disorders.

The composition of the food is perhaps the most important factor
in determining the reaction of the urine (see Chapter XXVII on Met-
abolism for influence of base-forming and acid-forming foods). The
reaction ordinarily varies considerably according to the time of day
the urine is passed. For instance, for a variable length of time after
a meal the urine may be neutral or even alkaline in reaction to litmus,

/o:-.',-!^'..'! Tj''-U '-2.'

Fig. 114. — Deposit in Ammoniacal Fermentation.
a, Acid ammonium urate; b, ammonium magnesium phosphate; c, bacteria.

owing to the claim of the gastric juice upon the acidic radicals to further
the formation of hydrochloric acid for use in carrying out the digestive
secretory function. This change in reaction is known as the alkaline
tide and is common to perfectly healthy individuals. The urine may
also become temporarily alkaline in reaction to litmus, as the result of
ingesting alkaline carbonates or certain salts of tartaric and citric acids
which may be transformed into carbonates within the organism.
Normal urine upon standing for some time becomes alkaline in reaction
to litmus, owing to the inception of alkaline or ammoniacal fermentation
through the agency of micro-organisms. This fermentation has no
especial diagnostic value except in cases where the urine has undergone
this change within the organism and is voided in the decomposed state.
Ammoniacal fermentation is ordinarily due to cystitis or occurs as the
result of infection in the process of catheterization. A microscopical

URINE 363

examination of such urine (Fig. 114) shows the presence oi ammonium
magnesium phosphate crystals, amorphous phosphates, and not infre-
quently afumonium urate.

Ingestion of acid fruits (oranges, lemons, peaches, etc.) causes
the formation of alkaline urine. This is due to the fact that the ash of
such fruits is alkaline and when the fruits are combusted in the body
carbonates are formed. On the other hand, bread, cereals, etc., yield an
acid ash and an acid urine.

Occasionally a urine which possesses a normal acidity when voided,
upon standing instead of undergoing ammoniacal fermentation as above
described, will become more strongly acid in reaction. Such a phe-
nomenon is termed acid fermentation. Accompanying this increased
acidity there is ordinarily a deepening of the tint of the urinary color.

Fig. 115. — Deposit in Acid Fermentation.
a, Fungus; b, amorphous sodium urate; e, uric acid; d, calcium oxalate.

Such urines may contain acid urates, uric acid, fungi, and calcium oxalate
(Fig. 115, above). On standing for a sufficiently long time any urine
which exhibits acid fermentation will ultimately change in reaction,
due to the inception of alkaline fermentation, and will show the micro-
scopical deposits characteristic of such a urine.

Specific Gravity. — The specific gravity of the urine of normal indi-
viduals varies ordinarily between 1.015 and 1.025. This value is sub-
ject to wide fluctuations under various conditions. For instance,
following copious water- or beer-drinking the specific gravity may fall
to 1.003 or lower, whereas in cases of excessive perspiration it may rise
as high as 1.040 or even higher. Where a very accurate determina-
tion of the specific gravity is desired use is commonly made of the
Pyknometer or of the Westphal hydrostatic balance. These instruments,
however, are not suited for clinical use. The clinical method of deter-

364

PHYSIOLOGICAL CHEMISTRY

mining the specific gravity is by means of a urinometer (Fig. 116). This
affords a very rapid method and at the same time is sufficiently accurate
for clinical purposes. The urinometer is always calibrated for use at a
specific temperature and the observations made at any other tem-
perature must be subjected to a certain correction to obtain the true
specific gravity. In making this correction one unit of the last order is
added to the observed specific gravity for every three degress above
the normal temperature and subtracted for every three
degrees below the normal temperature. For instance,
if in using a urinometer calibrated for i5°C. the specific
gravity of a urine having a temperature of 2i°C. is
determined as 1.018 it is necessary to add to the
observed specific gravity two units of the third order
to obtain the real specific gravity of the urine. There-
fore the true specific gravity, at i5°C., of a urine
having a specific gravity of 1.018 at 2i°C. is 1.018 +
0.002 = 1.020.

Pathologically, the specific gravity may be sub-
jected to very wide variations. This is especially
true in diseases of the kidneys. In acute nephritis
ordinarily the urine is concentrated and of a high
specific gravity, whereas in chronic nephritis the re-
I If i verse conditions are more apt to prevail. In fact,

under most conditions, whether physiological or patho-
logical, the specific gravity of the urine is inversely
proportional to the volume excreted. This is not
true of diabetes mellitus, however, where the volume
of urine is large and the specific gravity is also high,
owing to the sugar contained in the urine.
Fig. 116.— Urin- The amount of solids eliminated in the excretion
OMETER AND Cylin- £qj. twcnty-four hours may be roughly calculated by
means of Long's coefficient, i.e., 2.6. The solid con-
tent of 1000 c.c. of urine is obtained by multiplying the last two
figures of the specific gravity observed at 2 5°C. by 2.6. To determine
the amount of solids excreted in twenty-four hours if the volume was
1 1 20 c.c. and the specific gravity was 1.018 the calculation would be as
follows :

{a) 18X2.6 = 46.8 grams of solid matter in 1000 c.c. of urine.
A6.8X1120

(&)

1000

52.4 grams of solid matter in 11 20 c.c. of urine.

The coefficient of Haser (2.33) which has been in use for years prob-
ably gives values that are inaccurate for conditions existing in America.

URINE

365

This coefficient was calculated on the basis of the specific gravity deter-
mined at a temperature of i5°C.

Freezing-point (Cryoscopy). — The freezing-point of a solution de-
pends upon the total number of molecules of solid matter dissolved in
it. The determination of the osmotic pressure
by this method has come to be of some clinical
importance, particularly as an aid in the diag-
nosis of kidney disorders. In this connection
it is best to collect the urine from each kidney
separately and determine the freezing-point in
the individual samples so collected. By this
means considerable aid in the diagnosis of renal
diseases may be secured. The fluids most fre-
quently examined cryoscopically are the blood
(see page 245) and the urine. The freezing-
point is denoted by A. The value of A for
normal urine varies ordinarily between —1.3°
and — 2.3°C., the freezing-point of pure water
being take as 0°. A is subject to very wide
fluctuations under unusual conditions. For
instance, following copious water- or beer-
drinking A may have as high a value as

— o.2°C., whereas on a diet containing much
salt and deficient in fluids the value of A may
be lowered to — 3°C. or even lower. The freez-
ing point of normal blood is generally about

— o.56°C. and is not subject to the wide
variations noted in the urine, because of the
tendency of the organism to maintain the
normal osmotic pressure of the blood under all
conditions. Variations between —0.51° and
o.62°C. may be due entirely to dietary con-
ditions, but if any marked variation is noted
it can, in most cases, be traced to a disordered
kidney function.

T-. • • i. J i. • i.' 1 1 which the mixture to be

r reezmg-pomt determmations may be made observed is placed. Two

by means of the Beckmann-Heidenhain appa- stirrers are shown, one for

, the coohng mi.xture in the

ratUS (Fig. 117) or the Zikel pektOSCOpe. The jar and one for the experi-

Beckmann-Heidenhain apparatus consists of ^^^^^ mixture,
the following parts: A strong battery jar or beaker (C) furnished
with a metal cover which is provided with a circular hole in its center.
This strong glass vessel serves to hold the freezing mixture by means

Fig. 117. — Beckmann-
Heidenhain Freezing-
point Apparatus. (Long.)

D, a delicate thermom-
eter; C, the containing
jar; B, the outside or air
mantle tube; A, the tube in

366 PHYSIOLOGICAL CHEMISTRY

of wliich the temperature of the fluid under examination is lowered.
A large glass tube (B) designed as an air-jacket, and formed after the
manner of a test-tube is introduced through the central aperture in the
metal cover and into this air-jacket is lowered a smaller tube (A) con-
taining the fluid to be tested. A very delicate thermometer (D), grad-
uated in hundredths of a degree is introduced into the inner tube and
is held in place by means of a cork so that the mercury bulb is im-
mersed in the fluid under examination but does not come into contact
with any glass surface. A small platinum wire stirrer serves to keep
the fluid under examination well mixed while a larger stirrer is used to
manipulate the freezing mixture. (Rock salt and ice in the proportion
1 : 3 form a very satisfactory freezing mixture.)

In making a determination of the freezing-point of a fluid by means
of the Beckmann-Heidenhain , apparatus proceed as follows: Place
the freezing mixture in the battery jar and add water (if necessary) to
secure a temperature not lower than 3°C. Introduce the fluid to be
tested into tube A, place the thermometer and platinum wire stirrer in
position, and insert the tube into the air-jacket which has previously
been inserted through the metal cover of the battery jar. Manipulate
the two stirrers in order to insure an equalization of temperature
and observe the course of the mercury column of the thermometer very
carefully. The niercury will gradually fall and this gradual lowering
of the temperature will be followed by a sudden rise. The point at
which the mercury rests after this sudden rise is the freezing-point.
This rise is due to the fact that previous to freezing, a fluid is always
more or less over-cooled and the thermometer temporarily registers a
temperature somewhat helow the freezing-point. As the fluid freezes,
however, there is a very sudden change in the temperature of the liquid
and this change is imparted to the thermometer and causes the rise as
indicated. It occasionally occurs that the fluid under examination is
very much over-cooled and does 7iot freeze. Under such circumstances
a small piece of ice is introduced into it by means of the side tube noted
in the figure. This so-called "inoculation" causes the fluid to freeze
instantaneously. (For details of the method of determining the
freezing-point consult standard works on physical or organic chemistry.)

Electrical Conductivity. — The electrical conductivity of the urine
is dependent upon the number of inorganic molecules or ions present,
and in this differs from the freezing-point which is dependent upon the
total number of molecules both inorganic and organic which are in
solution. The conductivity of the urine has been investigated but
slightly, but from the data secured it seems that the value generally
falls below k = o.o2,.- The conductivity of blood serum has been de-

URINE 367

termined as k = 0.012. Up to the present time the determination of
the electrical conductivity of any of the fluids of the body has been
put to very slight clinical use. Experience may show the conductivity
value to be a more important aid to diagnosis than it is now considered,
particularly if it is taken in connection with the determination of the
freezing-point. By a combination of these two methods the portion
of the osmotic pressure due respectively to electrolytes and non-
electrolytes may be determined. For a discussion of electrical con-
ductivity, the method by which it is determined, and the principles
involved consult standard works on physical or electro-chemistry.

Collection and Preservation of the Urine Sample. — If any depend-
able data are desired regarding the quantitative composition of the urine
the examination of the mixed excretion for twenty-four hours is ab-
solutely necessary. In collecting the urine the bladder may be emptied
at a given hour, say 8 A. M., the urine discarded and all the urine from
that hour up to and including that passed the next day at 8 A. M.,
saved, thoroughly mixed, and a sample taken for analysis. Until
recently it was believed that powdered thymol (isopropylmetacresol)

CH3

OH

CHs — CH — CH3,

was a very satisfactory preservative since the excess might be removed
by filtration, if desired, and it was believed that the small amount which
went into solution would have no appreciable influence upon the deter-
mination of any of the urinary constituents. It appears however that
thymol is not such a satisfactory urinary preservative as was believed.
Evidence has been presented showing it to be unsatisfactory for the
preservation of urines which contain sugar, acetone or diacetic acid
and in which it desired to estimate the quantitative content of these
constituents. Claim has also been made that thymol is not a satis-
factory preservative for urines that are to be examined quantitatively for
phosphates or magnesium. Thymol being a phenol will cause an in-
accuracy when phenols are being determined quantitatively. Urines
preserved by thymol will also give a confusing white ring when sub-
jected to the nitric acid test for albumin (see Chapter XXIII).

Toluene is a very satisfactory preservative for urine. In using this
preservative simply overlay the urine with the toluene. Rosenbloom^

* Rosenbloom: New York Medical Journal, 99, 735, 1914.

368 PHYSIOLOGICAL CHEMISTRY

claims that camphor is a very satisfactory urine preservative which
does not interfere with the tests for important urinary constituents.

In certain pathological conditions it is desirable to collect the urine
passed during the day separately from that passed during the night.
When this is done the urine voided between 8 A. M. and 8 P. M. may
be taken as the day sample and that voided between 8 P. M. and 8 A. M.
as the night sample.

The qualitative testing of urine samples collected at random, except
in a few specific instances, is of no particular value so far as giving us
any accurate knowledge as to the exact urinary characteristics of the
individual is concerned. In the great majority of cases the qualitative
as well as the quantitative tests should be made upon the mixed
excretion for a twenty-four-hour period as well as upon a night sample
as ^above described.

CHAPTER XXII

URINE: PHYSIOLOGICAL CONSTITUENTS'
I. Organic Physiological Constituents

Urea.
Uric acid.
Creatinine.
Creatine. -

Ethereal sulphuric acids.

f Indoxyl-sulphuric acid.

J Phenol- and /j-cresol-sulphuric- acids.

j Pyrocatechol-sulphuric acid.

I Skatoxyl-sulphuric acid.

Hippuric acid.
Oxalic acid.

Neutral sulphur compounds.

Allantoin.

Aromatic oxyacids.

f Cystine.

Chondroitin-sulphuric acid.
: Thiocyanates.

Taurine derivatives.

Ox}'proteic acid.

Alloxj^Droteic acid.

Uroferric acid.

' Para-oxyphenyl-acetic acid.
Para-oxyphenyl-propionic acid.
Homogentisic acid.
Uroleucic acid.
I Oxymandelic acid.
I Kynurenic acid.
Amino-acids.
Peptides.
Benzoic acid.
Nucleoprotein.
Oxaluric acid.
Glucose.

* It is impossible to make any absolute classification of the physiological and pathological
constituents of the urine. \ substance may be present in the urine in small amount physio-
logically and be sufBciently increased under certain conditions as to be termed a patholog-
ical constituent. Therefore it depends, in some instances upon the quantity of a constituent
present whether it may be correctly termed a physiological or a pathological constituent.

' Normal constituent of urine of adults but found in larger amount in urine of infants
and children (see p. 509).

24 369

370

PHYSIOLOGICAL CHEMISTRY

Pepsin.

Enzymes Gastric rennin.

Amylase.
[ Acetic acid.

Volatile fatty acids Butyric acid. •

[ Formic acid.
Paralactic acid.
Phenaceturic acid.
Urocanic acid.

Phosphorized compounds

Pigments

Ptomaines and leucomaines.

Glycerophosphoric acid.
Phosphocarnic acid.
Urochrome.
Urobilin.
Uroerythrin.

Adenine.
Guanine.
Xanthine.
Epiguanine.

Purine Bases ' Episarkine.

Hypoxanthine.
Paraxanthine.
Heteroxanthine.
i-Methylxanthine.

2. Inorganic Physiological Constituents

Ammonia.

Sulphates.

Chlorides.

Phosphates.

Sodium and potassium.

Calcium and magnesium.

Carbonates.

Iron.

Fluorides.

Nitrates.

Silicates.

Hydrogen peroxide.

Normal urine varies widely in composition, being influenced by diet
and other factors. The following table represents the composition of a
normal urine. ^

^ Vierordt: Daten und Tabellen. Jena, 1906, p. 330.

URINE

371

COMPOSITION OF A NORMAL URINE
Volume (24 hours) 1500 c.c.

Constituent

""St" ■ Approximate
l^a^ms* I percentage

Water ' 1440.00

Solids

60.0

Urea

35-0

Uric acid

0.75

Hippuric acid

0.7

Oxalic acid

0.015

Aromatic oxyacids

0.06

Creatinine

Magnesium (MgO)

0.30

96.0

4.0

2-Z2,

0.004

Thiocyanic acid (as KSCN)

0-15

o.or

Indican

o.oi

O.OOI

Ammonia

0.65

0.04 1

Sodium chloride

16.5

I.I i

Phosphoric acid

2-5

0-15

Total sulphuric acid^

2-5

1

Silicic acid

0.45

0.03

Potassium (K2O)

2-5

0.15 i

1

Sodium (NajO)

5-0

0-3

Calcium (CaO)

0.25

0-015

Iron • o . 005 o . 0004

1 For data as to "partition" of sulphur and nitrogen, see Chapter XXVII on Metabolism.

372 PHYSIOLOGICAL CHEMISTRY

NHo
UREA, C = 0.

NHo

Urea is the principal end-product of the metaboHsm of protein
substances. It was formerly believed that about 90 per cent of the
total nitrogen of the urine was present as urea. Folin, however, has
shown that the distribution of the nitrogen of the urine among
urea and the other nitrogen-containing bodies present depends entirely
upon the absolute amount of the total nitrogen excreted. He found
that a decrease in the total nitrogen excretion was always accom-
panied by a decrease in the percentage of the total nitrogen excreted
as urea, and that after so regulating the diet of a normal person as to^

Fig. 118. — Urea.

cause the excretion of total nitrogen to be reduced to 3-4 grams in 24
hours, only about 60 per cent of this nitrogen appeared in the urine as urea.
His experiments also seem to show urea to be the only one of the nitro-
genous excretions which is relatively as well as absolutely decreased as a
result of decreasing the amount of protein metabolized. This same
investigator reports a hospital case in which only 14.7 per cent of the
total nitrogen was present as urea and about 40 per cent was present as
ammonia. Morner had p'reviously reported a case in which but 4.4
per cent of the total nitrogen of the urine was present as urea, and 26.7
per cent was present as ammonia.

Urea occurs most abundantly in the urine of man and carnivora
and in somewhat smaller amount in the urine of herbivora; the urine
of fishes, amphibians, and certain birds also contains a small amount of

URINE

373

the substance. Urea is also found in nearly all the fluids and in many
of the tissues and organs of mammals. The amount excreted, under
normal conditions, by an adult man in 24 hours is about 30-35 grams.
The excretion is greatest in amount after a diet of meat, and least in
amount after a diet consisting of non-nitrogenous foods; this is due to the
fact that the urea output is regulated by the protein ingestion. It is
true also that a non-nitrogenous diet has a tendency to decrease the
metabolism of the tissue proteins and thus cause the output of urea under
these conditions to fall below the output of urea observed during starva-
tion. The output of urea is also increased after copious water- or beer-
drinking. The increase is probably due primarily to the washing out of
the tissues of the urea previously formed, but which had not been re-
moved in the normal processes, and secondarily to a stimulation of
protein catabolism.

Urea may be formed in the organism from amino-acids such as leu-
cine, glycocoll, and aspartic acid : it may also be formed from ammonium
carbonate (NH4)2C03 or ammonium carbamate, H4X.O.CO.XH2.

There are differences of opinion regarding the transformation of the
substances just named into urea, but there is rather conclusive e\ddence
that at least a part of the urea is formed in the liver; it may be formed in
other organs or tissues as well.

Urea crystallizes in long, colorless, four- or sLx-sided, anhydrous,
rhombic prisms (Fig. 118), which melt at i32°C. and are soluble in
water or alcohol and insoluble in ether or chloroform. If a crystal of
urea is heated in a test-tube, it melts and decomposes with the liberation
of ammonia. The residue contains cyanuric acid,

C.OH

N N

II I
HO.C C.OH

N

NH2

C = 0

and biuret, \

NH

/
C = 0

I
NH2

374

PHYSIOLOGICAL CHEMISTRY

The biuret may be dissolved in water and a reddish-violet color obtained
by treating the aqueous solution with copper sulphate and potassium
hydroxide (see Biuret Test, page 98). Certain hypochlorites or hypo-
bromites in alkaline solution have the power of decomposing urea into
nitrogen, carbon dioxide, and water. Sodium hypobromite brings
about this decomposition, as follows:

CO(NH2)2+3NaOBr-»3NaBr+N2+C02+2H20.

This property forms the basis for a clinical quantitative determination
of urea (see page 496).

The soy bean has been shown to contain an enzyme called urease
which has the power to decompose urea with the liberation of ammonia.^
This fact is made use of in the quantitative determination of urea
(see Chapter XXVI).

Fig. 119. — Urea Nitrate.

Urea has the power of forming crystalline compounds with certain
acids; urea nitrate and urea oxalate are the most important of these
compounds. Urea nitrate, CO(NH2)2.HN03, crytallizes in colorless,
rhombic or six-sided tiles (Fig. 119, above), which are easily soluble in
water. Urea oxalate, [CO(NH2)2]2-H2C204, crystallizes in the form
of rhombic or six-sided prisms or plates (Fig. 121, page 376): the
oxalate differs from the nitrate in being somewhat less soluble in
water. The formation of the nitrate and oxalate and the decomposition
of urea by the enzyme urease are the most satisfactory methods for the
detection of urea.

A decrease in the excretion of urea is observed in many diseases in
which the diet is much reduced and in some disorders as a result of

^Takeuchi: Jour. College of Agr., Tokyo, 1909, Part I.

URINE

375

alterations in metabolism, e.g., myxedema, and in others as a result
of changes in excretion, as in severe and advanced kidney disease. A
pathological increase is found in a large proportion of diseases which
are associated with a toxic state. In marked acidosis it may be con-
siderably decreased relative to the total nitrogen (see Ammonia).

Experiments on Urea

1. Isolation from the Urine. ^ — Place 800 c.c. of urine in a precipitating jar,
add 250 c.c. of baryta inixture,^ and stir thoroughly. Filter off the precipitate
of phosphates, sulphates, ixrates, and hippurates and
evaporate the filtrate on a water-bath to a thick syrup.
This syrup contains chlorides, creatinine, organic salts,
pigments, and urea. Extract the syrup with warm 95
per cent alcohol and filter again. The filtrate con-
tains the ixrea contaminated with pigment. Decolor-
ize the filtrate by boiUng with animal charcoal, filter
again, and stand the filtrate away in a cold place for
crystallization. Examine the crystals under the micro-
scope and compare them with those shown in Fig. 118,
page 372.

2. Solubility. — Test the solubiUty of urea, prepared
by yourself or furnished by the instructor, in water and
in alcohol and ether.

3. Melting-point. — Determine the melting-point of
some pure urea furnished by the instructor. Proceed
as follows: Into an ordinary melting-point tube, sealed
at one end, introduce powdered urea. Fasten the tube
to the bulb of a thermometer as shown in Fig. 120, and
suspend the bulb and its attached tube in a small beaker
containing sulphuric acid. Gently raise the tempera-
ture of the acid by means of a low flame, stirring the
fluid continually, and note the temperature at which
the urea begins to melt.

4. Crystalline Form. — ^Dissolve a crystal of pure
urea in a few drops of 95 per cent alcohol and place
1-2 drops of the alcohoUc solution on a microscopic
slide. Allow the alcohol to evaporate spontaneously,

examine the crystals under the microscope, and compare them with those re-
produced in Fig, n8, page 372. RecrystaUize a Uttle urea from water in the
same way and compare the crystals with those obtained from the alcohoUc
solution.

5. Formation of Biuret. — Place a small amount of urea in a dry test-tube
and heat carefully in a low flame. The lu-ea melts at I32°C. and Uberates
ammonia. Continue heating until the fused mass begins to solidify. Cool the

^ The method based upon tlie precipitation by nitric acid is also satisfactory' (see
Hoppe-Seyler's Handbuch dcr Physiol, und Pathol. Chem. Anal., Eighth edition, 1909, p. 145).

' Baryta mbcture consists of a mixture of i volume of a saturated solution of Ba(NOj)j
and 2 volumes of a saturated solution of Ba(OH)j.

Fig. 120. — ]Melting-
poiNT Tubes Fastened
TO Bulb of Thermom-
eter.

376

PHYSIOLOGICAL CHEMISTRY

tube, dissolve the residue in dilute potassium hydroxide solution, and add very
dilute copper sulphate solution (see page 98). The purpUsh -violet color is due
to the presence of biuret which has been formed from the urea through the
application of heat as indicated. This is the reaction :

NH.2

I

Urea. C = O

\

N

/<

Urea, C =0

NH,

H

H

NH2

C=0

\
NH + NH3

/
C=0

NH2

Biuret.

6. Urea Nitrate. — Prepare a concentrated solution of urea by dissolving
a little of the substance in a few drops of water. Place a drop of this solution on a
microscopic slide, add a drop of concentrated nitric acid, and examine under
the microscope. Compare the crystals with those reproduced in Fig. 119, page 374.

Fig. 121.— Urea Oxalate.

7. Urea Oxalate. — To a drop of a concentrated solution of urea, prepared as
described in the last experiment (6), add a drop of a saturated solution of oxalic
acid. Examine under the microscope and compare the crystals with those shown
in Fig. 121, above.

8. Decomposition by Sodium Hypobromite. — Into a mixture of 3 c.c. of con-
centrated sodiimi hydroxide solution and 2 c.c. of bromine water in a test-tube
introduce a crystal of urea or a small amount of concentrated solution of urea.
Through the influence of the sodium hypobromite, NaOBr, the urea is decom-
posed and carbon dioxide and nitrogen are hberated. The carbon dioxide is
absorbed by the excess of sodium hydroxide, while the nitrogen is evolved and
causes the marked effervescence observed. This property forms the basis for

URINE .577

one of the methods in common use for the quantitative determination of urea.
Write the equation showing the decomposition of urea by sodium hypobromite.

9. Furfural Test. — To a few crystals of urea in a small porcelain dish add 1-2
drops of a concentrated aqueous solution of furfural and 1-2 drops of concentrated
hydrochloric acid. Note the appearance of a yellow color which gradually changes
into a purple. Allantoin also responds to this test (see page 392).

It is claimed that all ammonium compounds and all compounds
containing the amino (— NH2) group yield nitrogen when treated with
hypobromite as in this test.

HN— CO

URIC ACID, OC C-NH

>C0.
HN— C— HN

Uric acid is one of the most important of the constituents of the
urine. It is generally stated that normally about 0.7 gram is excreted
in 24 hours, but that this amount is subject to wide variations, particu-
larly under certain dietary and pathological conditions. It has been
shown, however, that the average daily excretion of uric acid for ten
men ranging in age from 19 to 29 years and fed a normal mixed diet
was 0.597 gram, a value somewhat lower than the generally accepted
average of 0.7 gram for such a period. On a purine-free diet the uric
acid output may be o. 1-0.5 gram per day, whereas a high purine diet may
yield a daily output of 2 grams. Uric acid is a diureide and consequently
upon oxidation may yield two molecules of urea. It acts as a weak
dibasic acid and forms two classes of salts, neutral and acid. The neutral
potassium and lithium urates are the most easily soluble of the alkali
salts; the ammonium urate is difficultly soluble. The acid-alkali urates
are more insoluble and form the major portion of the sediment which
separates upon cooling the concentrated urine; the alkaline earth urates
are very insoluble. Ordinarily uric acid occurs in the urine in the form
of urates and upon acidifying the liquid the uric acid is liberated and
deposits in crystalline form. This property forms the basis of one of
the older methods for the quantitative determination of uric acid
(Heintz jMcthod, Chapter XXVI).

Uric acid is very closely related to the purine bases as may be seen
from a comparison of its structural formula with those of the purine
bases given on page 127. According to the purine nomenclature it is
designated 2-6-8-trioxypurine. Uric acid forms the principal end-
product of the nitrogenous metabolism of birds and scaly amphibians;
in the human organism it occupies the fourth position inasmuch as here

37^ PHYSIOLOGICAL CHEMISTRY

urea, ammonia, and creatinine are the chief end-products of nitroge-
nous metabolism. It is generally said that the relation existing between
uric acid and urea in human urine under normal conditions varies on
the average from i : 40 to i : 100 and is subject to wider variations under
pathological conditions; and further that because of the high content of
uric acid in the urine of newborn infants the ratio may be reduced to
1 : 10 or even lower. We now know that this ratio of uric acid to urea
is of little significance under any conditions.

In man, uric acid probably results principally from the destruction
of nuclein material. It may arise from nuclein or other purine material
ingested as food or from the disintegrating cellular matter of the organ-
ism. The uric acid resulting from the first process is said to be of ex-
ogenous origin, whereas the product of the second form of activity is
said to be of endogenous origin. As a result of experimentation, Siven,
and Burian and Schur, and Rockwood claim that the amount of endoge-
nous uric acid formed in any given period is fairly constant for each
individual under normal conditions, and that it is entirely independent
of the total amount of nitrogen eliminated. Folin has taken exception
to the statements of these investigators and claims that, following a
pronounced decrease in the amount of protein metabolized, the absolute
quantity of uric acid is decreased but that this decrease is relatively
smaller than the decrease in the total nitrogen excretion and that the
per cent of the uric acid nitrogen, in terms of the total nitrogen, is there-
fore decidedly increased. According to Mares, ^ food-stuffs act to in-
crease the endogenous uric acid output by stimulating the digestive
glands to activity. That a portion of the endogenous uric acid may
arise in this way has recently been shown by Mendel and Stehle.^

In birds the formation of uric acid is analogous to the formation
of urea in man. In these organisms it is derived principally from the
protein material of the tissues and the food and is formed through a
process of synthesis which occurs for the most part in the liver; a
comparatively small fraction of the total uric acid excretion of birds
may result from nuclein material.

When pure, uric acid may be obtained as a white, odorless, and
tasteless powder, which is composed principally of small, transparent,
crystalline, rhombic plates. Uric acid as it separates from the urine
is invariably pigmented, and crystallizes in a large variety of character-
istic forms, e.g., dumb-bells, wedges, rhombic prisms, irregular rect-
angular or hexagonal plates, whetstones, prismatic rosettes, etc. Uric
acid is insoluble in alcohol and ether, soluble with difficulty in boiling

^ Mares: Arch. f. d. ges. Physiol., 134, 59, 1910.

* Mendel and Stehle: Jour. Biol. Chem., 22, 215, 1915.

URINE 379

water (i :i8oo) and practically insoluble in cold water (i : 39,480. at
i8°C.). It is soluble in alkalis, alkali carbonates, boiling glycerol.,
concentrated sulphuric acid, and in certain organic bases such as ethyl-
amine and piperidine. It is claimed that the uric acid is held in solu-
tion in the urine by the urea and disodium hydrogen phosphate present.
Uric acid possesses the power of reducing cupric hydroxide in alkaline
solution and may thus lead to an erroneous conclusion in testing for
sugar in the urine by means of Fehling's or Trommer's test. A white
precipitate of cuprous urate is formed if only a small amount of cupric
hydroxide is present, but if enough of the copper salt is present the
characteristic red or brownish-red precipitate of cuprous oxide is ob-
tained. Uric acid does not possess the power of reducing bismuth in
alkaline solution and therefore does not interfere in testing for sugar in
the urine by means of Boettger's or Xylander's tests.

In addition to being an important urinary constituent uric acid is
normally present in the brain, heart, Uver, lungs, pancreas, and spleen;
it also occurs in the blood of birds and has been detected in traces in
human blood under normal conditions.

Pathologically, the excretion of uric acid is subject to wide varia-
tions, but the experimental findings are rather contradictory. It may be
stated with certainty, however, that in leukemia, because of the destruc-
tion of nuclein material, the uric acid output is increased absolutely as
well as relatively to the urea output; under these conditions the ratio
between the uric acid and uirea may be as low as i : 9, whereas the normal
ratio, as we have seen, is i : 50 or higher. An actual output of 12 grams
of uric acid per day has been reported in leukemia. In the study of the
influence of X-ray on metabolism Edsall and others have reached some
interesting conclusions. Edsall found that the excretion of uric acid is
usually increased and that in some conditions, particularly in leukemia,
it may be greatly increased. The excretion of total nitrogen, phos-
phates, and other sustances may also be considerably increased.

In gout the kidney is said to lose the power of properly eliminating
uric acid and it collects in the blood in abnormally high concentration.

Normal = 1-3 mg. uric acid per 100 grams of blood.
Gout = 3-6 mg. uric acid per 100 grams of blood.

In gout the uric acid content of the urine is generally low preceding
an attack and increases during the attack. Atophan has been found
to increase the uric acid output in gout, apparently due to increased
kidney activity.

The uric acid content of the urine is of importance in relation to the
formation of uric acid calculi. The administration of alkali carbonates

380 PHYSIOLOGICAL CHEMISTRY

and citrates, or the feeding of base-forming foods, by decreasing the
acidity of the urine increases its solvent power for uric acid and de-
creases the liability of formation of this type of calculus.^

Experiments on Uric Acid

1. Isolation from the Urine. — Place about 200 c.c. of filtered urine in a
beaker, render it acid with 2-10 c.c. of concentrated hydrochloric acid, stir
thoroughly, and stand the vessel in a cold place for 24 hours. Examine the pig-
mented crystals of uric acid under the microscope and compare them with those
shown in Fig. 136, page 461 , and PI. V, opposite.

2. Solubility. — Try the solubiUty of pure uric acid, furnished by the in-
structor, in water, dilute acid and alkaU and in alcohol, ether and concentrated
sulphuric acid.

3. Crystalline Form of Pure Uric Acid. — Place about 100 c.c. of water in a
small beaker, render it distinctly alkaUne with potassivun hydroxide solution and

Fig. 122. — Pure Uric Acid.

add a small amount of pure vuic acid, stirring continuously. Cool the solution,
render it distinctly acid with hydrochloric acid and allow it to stand in a cool
place for crystallization. Examine the crystals under the microscope and com-
pare them with those reproduced in Fig. 122.

4. Murexide Test. — To a small amount of pure uric acid in a small evaporating
dish add 2-3 drops of concentrated nitric acid. Evaporate to dryness carefully
on a water-bath or over a very low flame. A red or yellow residue remains which
turns purpUsh red after cooUng the dish and adding a drop of very dilute am-
monium hydroxide. The color is due to the formation of murexide. If potas-
sium hydroxide is used instead of ammonium hydroxide a purpUsh violet color
due to the production of the potassium salt is obtained. The color disappears
upon warming ; with certain related bodies (purine bases) the color persists under
these conditions.

^ Blather wick: Arch. Int. Med., 14, 409, 1914.

PLATE V.

Uric Acid Crystals. Normal Color. (From Pnrdy, after Fryer.)

URINE 381

In this reaction the uric acid is oxidized to dialuric acid and alloxan.
These two substances condense to form alloxantin. This alloxantin
reacts with ammonium hydroxide to form purpuric acid. The purple
color is due to the formation of ammonium piirpurate or miirexide.

5. Phosphotungstic Acid Reaction (Folin). — To 20 c.c. of saturated sodium
carbonate solution in a small beaker add a small amount of uric acid. Stir
the solution until the uric acid has dissolved, then add i c.c. of FoUn's uric
acid reagent (see Chapter XXVI 1. A blue color results.

6. Silver Reduction Test fSchiff 1. — Dissolve a small amount of pure uric acid
in sodium carbonate solution and transfer a drop of the resulting mixture to a
strip of filter paper saturated with silver nitrate solution. A yellowish-brown
or black coloration due to the formation of reduced silver is produced.

It is claimed that chlorides interfere with this test.

7. Ganassini's Test.^ — Dissolve a small amount of uric acid in sodium carbon-
ate. Precipitate the dissolved uric acid by means of zinc chloride, filter off the
precipitate, and permit it to stand in contact with the air. A sky-blue color will
develop, a color change which may be hastened by sunlight. A similar reaction
may be obtained by treating the original precipitate with KiSjOg.

8. Influence upon Fehling's Solution. — Dilute i c.c. of Fehling's solution
with 4 c.c. of water and heat to boiling. Now add slowly, a few drops at a
time, 12 c.c. of a concentrated solution of uric acid in potassium hydroxide,
heating after each addition. From this experiment what do you conclude re-
garding the possibiUty of arriving at an erroneous decision when testing for
sugar in the urine by means of Fehling's test?

9. Reduction of Nylander's Reagent. — To 5 c.c. of a solution of uric acid
in potassium hydroxide add about one-half a cubic centimeter of Nylander's
reagent and heat to boiUng for a few moments. Do you obtain the typical black
end-reaction signifying the reduction of the bismuth?

NH CO

' I

CREATININE, C = XH I

N.(CH3).CH2.

Creatinine is the anhydride of creatine and is a constituent of normal
human urine. The theory that creatinine is derived from the creatine
of ingested muscular tissue as well as from the creatine of the muscular
tissue of the organism has been proven to be incorrect by Folin,
Klercker. and Wolf and Shaffer. Shaffer believes that creatinine is
the result of some special process of normal metabolism which takes
place to a large extent, if not entirely, in the muscles, and further that
the amount of such creatinine elimination, expressed /;/ milligrams per
kilogram body weight, is an index of this special process.- He further

' Ganassini: Boll, svc, 1908, No. i.

-He proposes to designate as the "creatinine coefficient" the excretion of crcatininc-
nilrogcn {mg.) per kilogram of body weight.

382

PHYSIOLOGICAL CHEMISTRY

states that the muscular efficiency of the individual depends upon the
intensity of this process. Under normal conditions about i-i)-^ gram
of creatinine is excreted by an adult man in 24 hours, ^ the exact amount
depending in great part upon the nature of the food and decreasing
markedly in starvation. Very little that is important is known regard-
ing the excretion of creatinine under pathological conditions. The
creatinine content of the urine is said to be increased in typhoid fever,
typhus, tetanus, and pneumonia, and to be decreased in anaemia, chloro-
sis, paralysis, muscular atrophy, advanced degeneration of the kidneys,
and in leukemia (myelogeneous, lymphatic and pseudo). An increase

Fig. 123. — Creatinine.

of creatinine was also noted in diabetes, an increase probably due to the
creatinine content of the meat eaten. The greater part of the data,
however, relating to the variation of the creatinine excretion under
pathological conditions are not of much value since in nearly every
instance the diet was not sufficiently controlled to permit the collection
of reliable data. And further, until the advent of the Folin method
(see page 506) there was no accurate method for the quantitative
determination of creatinine. Shaffer has called attention to the fact
that a low excretion of creatinine is found in the urine of a remarkably
large number of pathological subjects, representing a variety of con-
ditions, and that it is therefore evident that the excretion of an ab-
normally small amount of this substance is by no means peculiar to any
one disease. A considerable increase in the creatinine content of the
blood has been observed in uremia.^

^ According to Shaffer the amount excreted by strictly normal individuals is between 7
and II mg. of creatinine-nitrogen per kilogram of body weight.
^ Folin and Denis: Jotir. Biol. Client., 17, 487, 1914.
Myers and Fine: Jotir. Biol. Chan., 20, 391, 1914.

URINE 383

Creatinin ecrystallizes in colorless, glistening monoclinic prisms (Fig.
123, page 382) which are soluble in about 12 parts of cold water; they
are more soluble in warm water and in warm alcohol. It forms salts only
with strong mineral acids. One of the most important and interesting
of the compounds of creatinine is creatinme-zinc chloride, (04117X30)2-
ZnCl2, which is formed from an alcoholic solution of creatinine upon
treatment with zinc chloride in acid solution. Creatinine has the power
of reducing cupric hydroxide in alkaline solution and in this way may
interfere with the determination of sugar in the urine. In the reduction
by creatinine the blue liquid is first changed to a yellow, and the forma-
tion of a brownish-red precipitate of cuprous oxide is brought about only
after continuous boiling with an excess of the copper salt. Creatinine
does not reduce alkaline bismuth solutions and therefore does not inter-
fere with Xylander's and Boettger's tests.

It has recently been shown by Folin that the absolute quantity of
creatinine eliminated in the urine on a meat-free diet is a constant
quantity different for different individuals, but wholly independent of
quantitative changes in the total amount of nitrogen eliminated.
Shaffer has very recently confirmed these findings and has shown that
the output of creatinine under these conditions is constant from hour
to hour as well as from day to day.

Experiments on Creatinine

i

I. Preparation of Pure Creatmine from Urine CFolin-Benedict^. — To 10 liters^
of undecomposed urine in a large precipitating jar add with stirring a hot solution
of 180 grams of picric acid in 450 c.c. of boiling alcohol. Allow to stand over night
and syphon off the supernatant fluid. Pour the residue upon a large Buchner
funnel, drain with suction, wash once or twice with cold saturated picric acid and
suck dry. Treat the dry or nearly dry picrate in a large mortar or evaporating
dish with enough concentrated HCl to form a moderately thin paste (about 60 c.c.
of acid for each 100 grams of picrate) and stir the mixture thoroughly with the
pestle for 3-5 minutes. Filter with suction on a hardened paper, and wash the
residue twice with enough water to cover it, sucking as nearly dry as possible
each time. Transfer the filtrate to a large flask and neutraUze with an excess of
solid magnesiimi oxide (the "heavy" variety is best). Add this oxide in small
portions with cooling of the flask under running water between the additions.
Neutralization of the acid will be indicated by a bright yellow color of the mix-
txire, or litmus paper may be used to test it. Filter with suction. Wash the
residue twice with water. Immediately add a few cubic centimeters of glacial
acetic acid to the filtrate to make it strongly acid. Pay no attention to any
precipitate that may form, but dilute the solution with about 4 volumes of 95 per

' Benedict: Jour. Biol. Clum., iS, 1S2, 1914.

Folin: Ibid., 17 463, 1914.
2 If it is simply desired to demonstrate the presence of creatinine, i liter may be em-
ployed and the various reagents reduced accordingly.

384 PHYSIOLOGICAL CHEMISTRY

cent alcohol. After 15 minutes filter off the sUght precipitate which forms.
Treat the final filtrate with 30-40 c.c. of 30 per cent zinc chloride. Stir and let
stand over night in a cool place. Pour off the supernatant Uquid and collect the
creatinine zinc chloride on a Buchner funnel, wash once with water, then thor-
oughly with 50 per cent alcohol, finally with 95 per cent alcohol and dry. A
nearly white, hght crystalline powder should be obtained. The yield should be
90-95 per cent of the original creatinine (usually about 1.5-1.8 grams of creatinine
zinc chloride per Uter of urine).

RecrystaUize the creatinine -zinc chloride by treating 10 grams with 100 c.c.'
of water and about 60 c.c. of normal sulphuric acid, heating the mixture until a
clear solution is obtained. Add about 4 grams of purified animal charcoal, con-
tinue boiUng for about a minute, filter with suction through a small Buchner
funnel, pouring the filtrate back on the filter three or four times until it runs
through perfectly colorless. Wash residue with hot water and transfer the total
filtrate to a beaker and while hot treat with a Uttle strong zinc chloride solution
(3 c.c.) and with about 7 grams of potassium acetate dissolved in a Uttle water.
After ten minutes dilute with an equal voliune of alcohol, and allow to stand in a
cold place for some hours. Filter off the crystalline product and examine under
microscope (see Fig. 124). To remove the small amount of potassitun sulphate
which it contains stir up with twice its weight of water, filter, wash with a little
water and then with alcohol. The preparation should be snow white. Yield,
85-90 per cent.

Place the finely powdered recrystallized creatinine zinc chloride in a dry
flask and treat with seven times its weight (by volume) of concentrated aqueous
ammonia. Warm sUghtly and agitate gently until a clear solution is obtained,
care being taken to drive off no more ammonia during the warming than is
necessary to obtain a clear solution. Stopper the flask, allow to cool, place in
the ice-box for an hour or more. Pure creatinine crystaUizes out. It may be
recrystallized from boiUng alcohol or concentrated ammonia, but this is usually
unnecessary. The product is perfectly pure and can be used as a standard in
the quantitative determination of creatine and creatinine. See chapters on
Quantitative Analysis of Urine and Blood.

I. Preparation of Creatine. — Creatine may be prepared from creatinine zinc
chloride by decomposition with calcium hydrate, the process being one of hydrol-
ysis (Benedict).

One hundred grams of creatinine zinc chloride are treated with about 700 c.c.
of water in a large casserole and the mixture heated to boiling; 15c grams of pure
powdered calcium hydrate are then added, with stirring, and the mixture boiled
gently for 20 minutes (with occasional stirring). The hot mixture is then filtered
with suction, the residue being washed with hot water. The filtrate is then treated
with hydrogen sulphide gas for a few minutes and poured through a folded filter
to remove the zinc. The filtrate is acidified by the addition of about 5 c.c. of glacial
acetic acid and boiled down rapidly to a volume of about 200 c.c. This solution
is allowed to stand over night, preferably in a cool place. The next day the crys-
tallized creatine is filtered off with suction, washed with a very little cold water,
and then thoroughly washed with alcohol and dried. ^ This product is then recrys-
tallized by dissolving in about seven times its weight of boiling water and allowing

' The filtrate obtained at this point should be diluted with alcohol and treated with zinc
chloride (50 c.c. of a 30 per cent solution) for recovery of the unconverted creatinine.

URINE

38:

the solution to cool slowly and stand for some hours. This product should be per-
fectly pure creatine. If necessary it can be recrystallized with verj' little loss. The
crystallized product should be filtered off, washed with alcohol and ether and dried
in air for about half an hour. Thus obtained the creatine contains water of crystal-
lization which it loses very readily upon exposure to air. To prepare creatine which
can be weighed with absolute exactness it is necessary to dehydrate this product by
heating for some hours at about 95°.

The yield in this process is about 18 grams of recrystallized creatine, and
about 55 grams of creatinine zinc chloride recovered. Longer boiling with lime
does not bring about a greater yield, as after the 20-minute point creatine is
decomposed almost exactly as fast as it is formed.

Examine the crystals of creatine under the microscope and compare with illus-
tration in Chapter XIX on Muscular Tissue. For other creatine tests see Chapter
XIX.

F'iG. 124. — Creatinixe-zixc Chloride. iSalkowski.)

3. Nitro-prusside Test (Weyl). — Take 5 c.c. of urine in a test-tube, add a few
drops of sodium nitro-prusside and render the solution alkaline with potassium
hydroxide solution. A ruby-red color results which soon turns yellow.
See Legal's test for acetone, page 437.

4. Nitro-prusside-acetic Acid Test (Salkowski). — To the yellow solution ob-
tained in Weyl's test above add an excess of acetic acid and apply heat. A green
color results and is in turn displaced by a blue color. A precipitate of Prussian
blue may form.

5. Picric Acid Reaction (Jaffe). — Place 5 c.c. of urine in a test-tube, add an
aqueous solution of picric acid and render the mixture alkaline with potassium
hydroxide solution. A red color is produced which turns yellow if the solution be
acidified. Glucose gives a similar red color but only upon the application of heat.
This color reaction observed when creatinine in alkaline solution is treated with
picric acid is the basic principle of Folin's colorimetric method for the quantitative
determination of creatinine (see page 506 j.

ETHEREAL SULPHATES

The most important of the ethereal sulphates found in the
urine are phowl-sulphurk acid, p-crcsol-sulpJiuric acid, indoxyl-sidphuric

25

386 PHYSIOLOGICAL CHEMISTRY

acid, and skatoxyl-sulphuric acid. Pyrocatechol-sulphuric acid also
occurs in traces in human urine. The total output of ethereal sulphuric
acid (as SO3) varies ordinarily from o.i gram to 0.25 gram for 24 hours
and comprise 5-15 per cent of the total sulphur. In health the ratio
of ethereal sulphuric acid to inorganic sulphuric acid is about i : 10.
These ethereal sulphuric acids originate in part from the phenol, cresol,
indole and skatole formed in the putrefaction of protein material in
the intestine. The phenol passes to the liver where part of it is conju-
gated to form phenol potassium sulphate and appears in this form in the
urine whereas the indole and skatole undergo a preliminary oxidation to
form indoxyl and skotoxyl respectively before their conjugation and
elimination.

It was formerly generally considered that each of the ethereal sul-
phuric acids was formed principally in the putrefaction of protein
material in the intestine and that therefore a determination of the total
ethereal sulphuric acid content of the urine was an index of the extent to
which these putrefactive processes were proceeding within the organism.
Folin, however, conducted a series of experiments which seemed to
show that the ethereal sulphuric acid content of the urine did not afford
an index of the extent of intestinal putrefaction, since these bodies
arise only in part from putrefactive processes. He claims that the
ethereal sulphuric acid excretion represents a form of sulphur metaboHsm
which is more in evidence upon a diet containing a very small amount of
protein or upon a diet containing absolutely no protein. The ethereal
sulphuric acid content of the urine diminishes as the total sulphur con-
tent diminishes but the percentage decrease is much less. Therefore
when considered from the standpoint of the total sulphuric acid content
the ethereal sulphuric acid content is not diminished but is increased,
although the total sulphuric acid content is diminished. Folin's experi-
ments also seem to show that the indoxyl sulphuric acid (indoxyl potas-
sium sulphate or indican) content of the urine does not originate to any
degree from the metabolism of protein material but that it arises in
great part from intestinal putrefaction and that the excretion of indoxyl
sulphuric acid may alone be taken as a rough index of the extent of putre-
factive processes within the intestine. Indoxyl sulphuric acid,

CH

HC C C(0.S03H),

! II II

HC C CH

\/\/
CH NH

URINE 387

therefore, which occurs in the urine as indoxyl potassium sulphate or

indican,

CH

^\
HC C— CCO.SOsK),

I II II
HC C CH

CH NH

is clinically the most important of the ethereal sulphuric acids. Under
normal conditions from 4 to 20 mg. of indican are excreted per day.
The variations are due mainly to diet, a high meat diet causing an
increase and a carbohydrate diet a decrease. Pathologically the great-
est increases are found in disorders involving increased putrefaction and
stagnation of intestinal contents. Bacterial decomposition of body
protein as in gangrene, putrid pus formation, etc., gives rise to an
increased indican excretion.

It was formerly believed that the phenol was excreted practically
quantitatively in the conjugated form'. Recent work of Folin and Denis^
seems to indicate that this is not true. Only pari of the phenols formed
in intestinal putrefaction are excreted in the conjugated form, the
remainder being excreted as free phenol. The phenol output tends to
vary directly but not proportionally with the protein ingestion. The
total phenol excretion of normal men on an ordinary mixed diet averages
around 0.4 gram per day.

Tests for Indican^

I. Jaffa's Test. — Nearly fill a test-tube with a mixture composed of equal
volimies of concentrated HCl and the xirine vmder examination. Add 2-3 c.c.
of chloroform and a few drops of a calcium hypochlorite solution, place the thumb
over the end of the test-tube and shake the tube and contents thoroughly.
The chloroform is colored more or less, according to the amount of indican pres-
ent. Ordinarily a blue color due to the formation of indigo-blue is produced ;
less frequently a red color due to indigo-red may be noted.

Repeat] this test on some of this same mine to which formaldehyde has
been added. Is there any variation in the reaction from what you previously
obtained?

This is the reaction (see also pages 212-213):

' Folin and Denis: Jour. Biol. Chem., 22, 309, 1915.

' The urine should always be examined fresh if this is possible. In any event formalde-
hyde should never be used as a preservative for such urines as are to be e.xamined for indican
by means of any test involving hypochlorite or potassium permanganate. The formalde-
hyde through its reducing power lowers the oxidizing efliciency of the mixture. The forma-
tion of formic acid from the aldehyde may also interfere.

388 PHYSIOLOGICAL CHEMISTRY

CH

HC C — C.OH

2 I !| II + 20-

HC C CH

CH NH

Indoxyt, CsHtXO.

CH CH

/\ /%

HC C CO O.C— C CH

I II I I II I + 2H2O

HC C c C C CH

CH NH NH CH

Indigo-blue, CiiHioX202.

2. Obennayer's Test. — Nearly fill a test-tube with a mixture composed of
equal volumes of Obennayer's reagent^ and the urine under examination.
Add 2-3 c.c. of chloroform, place the thumb over the end of the test-tube and
shake thoroughly. How does this compare with Jaffe's test?

3. Jolles' Reaction.- — To 10 c.c. of urine add i c.c. of a 5 per cent alcoholic
thymol solution and shake. Add about 10 c.c. of fuming HCl containing 5
grams of ferric chloride per hter. Shake again carefully and let stand for 15
minutes. Add about 4 c.c. of chloroform and extract the pigment by repeated
gentle shaking. The chloroform becomes intensely violet. 0.0032 mg. of indi-
can can be detected in 10 c.c. of urine. It is much the most delicate test for
indican.

CO.NH.CH2.COOH.

/\
HIPPURIC ACID,

This acid occurs normally in the urine of both the carnivora and
herbivora but is much more abundant in the urine of the latter. It is
formed by a synthesis of benzoic acid and glycocoll which takes place
in the kidneys and elsewhere^. The glycocoll comes from decomposi-
tion of protein. The benzoic acid thus utilized may come from (i) pre-
formed benzoic acid of fruits and vegetables; (2) other aromatic com-
pounds of fruits and vegetables; (3) aromatic amino-acids (tyrosine
and phenylalanine) from the alimentary tract. The average excretion
of hippuric acid by an adult man for 24 hours under normal conditions
is about 0.7 gram. Hippuric acid crystallizes in needles or rhombic
prisms (see Fig. 125, p. 389) the particular form depending upon the

^ Obermayer's reagent is prepared by adding 2-4 grams of ferric chloride to a liter of con-
centrated HCl (sp. gr. 1. 19).

"^ Zeit. physiol. Chem., 94, 79, 1915.

* Kingsbury and Bell: Jour. Biol. Chem., 21, 297, 1915.

URINE

389

rapidity of crystallization. Pure hippuric acid melts at iSy^C. The
most satisfactory method for the isolation of hippuric acid from the
urine in crystalline [form is that proposed by Roaf (see below). It
is easily soluble in alcohol or hot water, and- only slightly soluble in
ether. The output of hippuric acid is increased in diabetes owing prob-
ably to the ingestion of much protein and fruit. Plums, prunes and
cranberries in particular increase the hippuric acid output considerably
due to their relatively high content of benzoic acid. Hippuric acid
is decreased in'fevers and in certain kidney disorders where the synthetic

Fig. i2v — Hippuric Acid.

activity of the renal cells is diminished. It may be determined quan-
titatively by methods given in Chapter XXVI.

Experiments on Hippuric Acid

I. Separation from the Urine. — (a) First Method. Render 500-1000 c.c.
of urine of the horse or cow' alkahne with milk of lime, boil for a few moments and
filter while hot. Concentrate the filtrate, over a burner, to a small volume. Cool
the solution, acidify it strongly with concentrated hydrochloric acid and stand it
in a cool place for 24 hours. Filter off the crystals of hippuric acid which have
formed and wash them with a little cold water. Remove the crystals from the
paper, dissolve them in a very small amount of hot water and percolate the hot
solution through thoroughly washed animal charcoal, being careful to wash out
the last portion of the hippuric acid solution with hot water. Filter, concentrate

' If urine of the horse or cow is not available human urine may serve the purpose fuUj-
as well provided means are taken to increase its content of hippuric acid. This may be con-
veniently accomplished by ingesting 2 prams of ammonium benzoate at night. (See
chapter on Metabolism). The fraction of urine passed in the morning will be found to have
a high content of hippuric acid. The ammonium benzoate is in no way harmful. In case
ammonium benzoate is not available sodium benzoate may be substituted.

390 PHYSIOLOGICAL CHEMISTRY

the filtrate to a small volume and stand it aside for crystallization. Examine the
crystals imder the microscope and compare them with those in Fig. 125, page 389.
This method is not as satisfactory as Roaf's method (see below).

(b) Roaf's Method. — ^Place 500 c.c. of urine of the horse or cow in a cas-
serole or precipitating jar and add an equal volume of a saturated solution of
ammonium sulphate^ and 7.5 c.c. of concentrated sulphuric acid. Permit the
mixture to stand for 24 hours and remove the crystals of hippuric acid by filtration.
Purify the crystals by recrystaUization according to the directions given above
imder First Method. Examine the crystals imder the microscope and compare
them with those given in Fig. 125, page 389.

If suflficient urine is not available to permit the use of 500 c.c. a smaller volume
may be used inasmuch as it is possible, by the above technic, to isolate hippuric
acid in crystalline form from as small a volume as 25-50 c.c. of herbivorous urine.
The greater the amoimt of ammoniimi sulphate added the more rapid the crystal-
Uzation imtil at the saturation point the crystals of hippuric acid sometimes form in
about ten minutes.

2. Melting-point. — ^Determine the melting-point of the hippuric acid pre-
pared in the above experiment (see page 375).

3. SolubiUty. — ^Test the solubiUty of hippuric acid in hot and cold water and
in alcohol, and ether.

4. Formation of Nitro-Benzene (Liicke's Reaction). — To a little hippuric acid
in a small porcelain dish add 1-2 c.c. of concentrated HNO3 and evaporate to dry-
ness on a water-bath. Transfer the residue to a dry test-tube, apply heat, and
note the odor of the artificial oil of bitter almonds (nitrobenzene).

5. Spiro's Reaction. 2 — Warm the hippuric acid with acetic anhydride, anhy-
drous sodium acetate and benzaldehyde. After one-half hour permit the solution
to cool. Note the formation of crystals of the lactimide of phenylaminocinnamic
acid, melting-point 165-166°. Heat some of the crystals with concentrated sodium
hydroxide until ammonia is given off. Acidify and note the formation of phenyl-
pyroracemic acid (C6H6CH2.CO.COOH). This acid is soluble in ether.

6. Sublimation. — ^Place a few crystals of hippuric acid in a dry test-tube and
apply heat. The crystals are reduced to an oily fluid which soUdifies in a crystal-
Une mass upon cooling. When stronger heat is appUed the Uquid assumes a
red color and finally yields a sublimate of benzoic acid and the odor of hydro-
cyanic acid.

7. Formation of Ferric Salt. — ^Render a small amount of a solution of hip-
puric acid neutral with dilute potassium hydroxide. Now add 1-3 drops of
neutral ferric chloride solution and note the formation of the ferric salt of hip-
puric acid as a cream-colored precipitate.

8. Synthesis of Hippuric Acid. — To some of the glycocoU prepared in the last
experiment or furnished by the instructor, add a little water, about i c.c. of benzoyl
chloride and render alkaline with potassium hydroxide solution. Stopper the tube
and shake it until no more heat is evolved. Now render strongly alkaline with
potassium hydroxide and shake the mixture until no odor of benzoyl chloride can be
detected. Cool, acidify with hydrochloric acid, add an equal volume of petroleum
ether, and shake thoroughly to remove the benzoic acid. (Evaporate this solution
and note the crystals of benzoic acid. Compare them with those shown in Fig. 127,
page 396.) Decant the ethereal solution into a porcelain dish and extract again

1 125 grams of solid ammonium sulphate may be substituted.
^ Spiro: ZeiL physiol. Chem., 28, 174, 1899.

URINE 391

with ether. The hippuric acid remains in the aqueous solution. Filter it off and
wash it with a small amount of cold water while still on the filter. Remove it to
a small, shallow vessel, dissolve it in a small amount of hot water and set it aside
for crystallization. Examine the crystals microscopically and compare them with
those in Fig. 125, page 389.

The chemistry of the synthesis is represented thus:

CH2-NH2 COCl 0C-NH-CH2-C00H.

COOH \/ \/

Glycocoll. Benzoyl chloride. Hippuric acid.

OXALIC ACID,

COOH
COOH

Oxalic acid is a constituent of normal urine, about 15-20 mg. being
eliminated in 24 hours. It is present in the urine as calcium oxalate
which is kept in solution through the medium of the acid phosphates.
The origin of the oxalic acid content of the urine is not well under-
stood. It is eliminated, at least in part, unchanged when ingested, there-
fore since many of the common articles of diet, e.g., asparagus, apples,
cabbage, grapes, lettuce, spinach, tomatoes, etc., contain oxalic acid
(oxalates) it seems probable that the ingested food supplies a portion of
the oxalic acid found in the urine. There is also experimental evidence
that part of the oxalic acid of the urine is formed within the organism
in the course of protein and fat metabolism. It has also been suggested
that oxalic acid may arise from an incomplete combustion of carbo-
hydrates, especially under certain abnormal conditions. Patholog-
ically, oxalic acid is found to be increased in amount in diabetes mellitus,
in organic diseases of the liver, and in various other conditions which are
accompanied by a derangement of the oxidation mechanism. An
abnormal increase of oxalic acid is termed oxaluria. A considerable
increase in the content of oxalic acid may be noted unaccompanied by
any other apparent symptom. Calcium oxalate crystallizes in at least
two distinct forms, dumb-bells and octahedra (Fig. 134, page 459).

Experiments

Preparation of Calcium Oxalate. — First Method. — Place 200-250 c.c. of
urine in a beaker, add 5 c.c. of a saturated solution of calcium chloride, make the
urine slightly acid with acetic acid, and stand the beaker aside in a cool place for
24 hours. Examine the sediment under the microscope and compare the crystal-
line forms with those shown in Fig. 134, page 459.

Second Method. — Proceed as above, replacing the acetic acid by an excess of
ammonium hydroxide and filtering off the precipitate of phosphates.

392

PHYSIOLOGICAL CHEMISTRY

NEUTRAL SULPHUR COMPOUNDS

Under this head may be classed such bodies as cystine (see page 75),
chondroitin-sulphuric acid, oxyproteic acid, alloxyproteic acid, uroferric
acid, methyl mercaptan, ethyl sulphide, thiocyanates and taurine
derivatives. The sulphur content of the bodies just enumerated is
generally termed unoxidized or neutral sulphur in order that it may not
be confused with the acid or oxidized sulphur which occurs in the
inorganic sulphuric acid and ethereal sulphuric acid forms. Ordinarily
the neutral sulphur content of normal human urine is 5-25 per cent
of the total sulphur content (see "Sulphur Partition" in chapter on
Metabolism.) The actual amount excreted may be 0.2-0.4 grams

Fig. 126. — Allantoin, from Cat's Urine.

a and 6, Forms in which it crystallized from the urine; c, recrystallized allantoin. (Drawn
from micro-photographs furnished by Prof. Lafayette B. Mendel of Yale University.)

per day, calculated as SO3. Its origin is mainly endogenous. The
excretion is fairly constant for any given individual in spite of dietary
changes. In tuberculosis, cancer, cystinuria, etc., the amount may
be relatively or absolutely increased.

NH.CH.NH

ALLANTOIN, OC CO

I ! i

NH.CO NH2

Allantoin is found in the urine of practically all mammals including
man. In human urine it occurs in very small amount (5-15 mg. per
day) whereas in the case of all other mammals investigated except
anthropoid apes, it is the principal end-product of purine metabolism

URINE 393

and may constitute 90 per cent or over of the total purine output.^
Allantoin is formed by the oxidation of uric acid and the output is
increased by the feeding of thymus or pancreas to lower animals.
When pure it crystallizes in prisms (Fig. 126, page 392) and when impure
in granules and knobs. Pathologically, it has been found increased in
diabetes insipidus and in hysteria with convulsions (Pouchet). Mendel
and Dakin- have shown that allantoin is optically inactive notwith-
standing the fact that it contains an asymmetric carbon atom. This
phenomenon they believe to be due to tautomeric change. Wiechowski
has suggested an excellent method for the quantitative determination
of allantoin. (See Chapter XXVI.)

Experiments

1. Separation from the Urine. ^ — Meissner's Method. — Precipitate the urine
with baryta water. NeutraUze the filtrate carefully with dilute sulphuric acid,
filter immediately, and evaporate the filtrate to incipient crystallization. Com-
pletely precipitate this warm fluid with 95 per cent alcohol (reserve the precipi-
tate). Decant or filter and precipitate the solution by ether. Combine the
ether and alcohol precipitates and extract with cold water or hot alcohol; allan-
toin remains undissolved. Bring the allantoin into solution in hot water and
recrystallize.

2. Preparation from Uric Acid. — Dissolve 4 grams of uric acid in 100 c.c. of
water rendered alkaUne with potassium hydroxide. Cool and carefully add 3
grams of potassium permanganate. Filter, immediately acidulate the filtrate
with acetic acid and allow it to stand in a cool place over night. Filter off the
crystals and wash them with water. Save the wash water and filtrate, unite
them and after concentrating to a small volume stand away for crystaUization.
Now combine all the crystals and recrystallize them from hot water. Use these
crystals in the experiments which follow.

3. Microscopical Examination. — Examine the crystals made in the last
experiment and compare them with those shown in Fig. 126.

4. Solubility. — Test the solubility of allantoin in cold and hot water, cold and
hot alcohol and in ether.

5. Reaction. — Dissolve a crystal in water and test the reaction to htmus.

6. Furfural Test (Schiff ). — Place a few crystals of allantoin on a test-tablet or
in a porcelain dish and add 1-2 drops of a concentrated aqueous solution of fur-
fural and 1-2 drops of concentrated hydrochloric acid. Observe the formation of
a yellow color which turns to a hght purple if allowed to stand. This test is given
by urea but not by uric acid.

7. Murexide Test. — Try this test according to the directions given on page
380. Note that allantoin fails to respond.

8. Reduction of Fehling's Solution. Make this test in the usual way isee
page 416) except that the boiling must be prolonged and excessive. Ultimately

• Wiechowski: "Die Purinstoffe und das .Mlantoin" in Xeul)auiT and Huppert's "Ana-
lyse des Harris,'^ Wiesbaden, 1913.

* Mendel and Dakin: Jour. Bwl. Clicm., 7, 153, iqio.

'The urine of the dog after thymus, pancreas, or uric acid feeding may be employed.

394 PEEYSIOLOGICAL CHEMISTRY

the allantoin will reduce the solution. Compare with the result on uric acid,
page 381.

AMINO-ACIDS'

Certain of these acids are always present in normal urine. The
excretion of total amino-acid nitrogen by a normal adult averages
0.4-1.0 gram per day or about 2-6 per cent of the total nitrogen.
Free amino-acid nitrogen (see van Slyke procedure, Chapter IV) is
considerably less than this, and ordinarily constitutes 0.5-1 per cent
of the total nitrogen. The amount may be largely increased in disorders
associated with tissue waste, e.g., typhoid, acidosis, pronounced atrophy
of the liver, etc. For tests on amino-acids see Chapter IV.

AROMATIC OXYACIDS

Two of the most important of the oxyacids are parahydroxy-
phenyl-acetic acid,

CH2.COOH,

OH

and par ahydroxy- phenyl-propionic acid,

CH2.CH2.COOH.

OH

They are products of the putrefaction of protein material and tyrosine
is an intermediate stage in their formation. Both these acids for the
most part pass unchanged into the urine where they occur normally in
very small amount. The content may be increased in the same manner
as the phenol content, in particular by acute phosphorus poisoning. A
fraction of the total aromatic oxyacid content of the urine is in combina-
tion with sulphuric acid, but the greater part is present in the form
of salts of sodium and potassium.

Homogentisic Acid or di-hydroxyphenyl-acetic acid,

OH

ICH2.COOH,

OH

* For a full discussion see Underhill's "The Physiology of the Amino Acids," Yale
University Press, November, 1915.

URINE 395

is another important oxyacid sometimes present in the urine. Under
the name glycosuric acid it was first isolated from the urine by Prof.
John ^Marshall of the University of Pennsylvania; subsequently Bau-
raann isolated it and determined its chemical constitution. It occurs in
cases of alcaptonuria. A urine containing this oxyacid turns greenish-
brown from the surface downward when treated with a little sodium
hydroxide or ammonia. If the solution be stirred the color very soon
becomes dark brown or even black. Homogentisic acid reduces
alkaline copper solutions but not alkaline bismuth solutions. Uro-
leucic acid is similar in its reactions to homogentisic acid.
Hydroxymandelic Acid or parahydroxyphenyl-glycolic acid,

OH

CH(OH).COOH,

has been detected in the urine in cases of yellow atrophy of the liver.
Kynurenic Acid or 7-oxy-/3-quinoline carbonic acid,

CH COH
HC C C.COOH,

I I! I

HC C CH

\/\^
CH N

is present in the urine of the dog and has recently been detected by
Swain in the urine of the coyote. To isolate it from the urine proceed
as follows: Acidify the urine with hydrochloric acid in the proportion
1:25. From this acid fluid both the uric acid and the kynurenic acid
separate in the course of 24-48 hours. Filter off the combined crys-
talline deposit of the two acids, dissolve the kynurenic acid in dilute
ammonia (uric acid is insoluble), and reprecipitate it with hydrochloric
add. If a solution containing kynurenic acid be evaporated to dryness
with hydrochloric acid and potassium chlorate, a reddish residue is
obtained which becomes first brownish green and then emerald green on
adding ammonia (Jaffe).

Kynurenic acid may be quantitatively determined by Capaldi's
method.^

COOH.

BENZOIC ACID,

\/

Zeilschrifi fiir physiologische Chemie, 23, 92, 1897.

39^

PHYSIOLOGICAL CHEMISTRY

Benzoic acid has been detected in the urine of the rabbit and dog. It is
also said to occur in human urine accompanying renal disorders. The
benzoic acid probably originates from a fermentative decomposition of
the hippuric acid of the urine. Benzoic acid and glycocoll are synthe-
sized in the kidney and elsewhere^ to form hippuric acid (see page 585).
Certain fruits and berries contain considerable benzoic acid; e.g., cran-
berries have been shown to contain 0.06 per cent."

Experiments

1. Solubility. — Test the solubility of benzoic acid in water, alcohol, and ether.

2. Crystalline Form. — Recrystallize some benzoic acid from hot water, ex-
amine the crystals under the microscope, and compare them with those re-
produced in Fig. 127.

Fig. 127. — Benzoic Acid.

3. Sublimation. — Place a little benzoic acid in a test-tube and heat over a
flame. Note the odor which is evolved and observe that the acid sublimes in the
form of needles.

4. Dissolve a little sodium benzoate in water and add a solution of neutral
ferric chloride. Note the production of a brownish -yellow precipitate (salicylic
acid gives a reddish -violet color under the same conditions). Add ammoniimi
hydroxide to some of the precipitate. It dissolves and ferric hydroxide is formed.
Add a Uttle hydrochloric acid to another portion of the original precipitate and
stand the vessel away over night. What do you observe?

NUCLEOPROTEIN

The nubecula of normal urine has been shown by one investigator
to consist of a mucoid containing 12.7 per cent of nitrogen and 2.3
per cent of sulphur. This body evidently originates in the urinary

' Kingsbury .and Bell: Jour. Biol. Cheni., 21, 297, 1915.

- Radin [quoted by Blatherwick {Arch. Int. Med., 14, 409, 1914) from unpublished data].

URINE ,397

passages. It is probably slightly soluble in the urine. Some investiga-
tors believe that the body forming the nubecula of normal urine is
nucleoprotein and not a mucin or mucoid as stated above. A discussion
of nucleoprotein and related bodies occurring in the urine under patho-
logical conditions will be found on page 428.

NH— CO

OXALURIC ACID, CO |

NHo COOH.

Oxaluric acid is not a constant constituent of normal human urine,
and when found occurs only in traces as the ammonium salt. Upon
boiling oxaluric acid it splits into oxalic acid and urea.

GLUCOSE

This sugar occurs in traces in normal urine. It is, however, not
present in sufficient concentration to be detected by any of the ordinary
tests used in urine analysis. In certain pathological conditions (pp.
413 and 523) the sugar in the urine is notably increased. Folin has
recently modified Benedict's sugar test (see Chapter XXIII) so it may
be used to demonstrate the sugar content of normal urine. ^

ENZYMES

Various types of enzymes produced within the organism are excreted
in both the feces and the urine. In this connection it is interesting to
note that pepsin, rennin, lipase and an amylase have been positively
identified in the urine. The occurrence of trypsin in the urine, at least
under normal conditions, is questioned.

VOLATILE FATTY ACIDS

Acetic, butyric, and formic acids have been found under normal
conditions in the urine of man and of certain carnivora as well as in the
urine of herbivora. Normally they arise principally from the fermenta-
tion of carbohydrates and the putrefaction of proteins. The acids con-
taining the fewest carbon atoms (formic and acetic) are found to be
present in larger percentage than those which contain a larger number of
such atoms. The volatile fatty acids occur in normal urine in traces,
the total output for 24 hours according to older investigators varying
from 0.008 gram to 0.05 gram.

Pathologically, the excretion of volatile fatty acids is increased in

^ Folin: Jour. Biol. Client., 22, 327, 1915.

398 PHYSIOLOGICAL CHEMISTRY

diabetes, fevers, and in certain hepatic diseases in which the parenchyma
of the liver is seriously affected. Under other pathological conditions
the output may be diminished. These variations, however, in the
excretion of the volatile fatty acids possess very little diagnostic
value.

CH3

PARALACTIC ACID, CH(OH)

COOH.

Paralactic acid is supposed to pass into the urine when the supply

of oxygen in the organism is diminished through any cause, e.g., in

eclampsia, acute yellow atrophy of the liver, carbon-monoxide poisoning,

acute phosphorus poisoning, or epileptic attacks. This acid has also

been found in the urine of healthy persons following the physical exercise

incident to prolonged marching. Paralactic acid has been detected in

the urine of birds after the removal of the liver. Underhill reports the

occurrence of this acid in the urine of a case of pernicious vomiting of

pregnancy.

CH2.CO.NH.CH2.COOH.

/\
PHENACETURIC ACID, I

\/

Phenaceturic acid occurs principally in the urine of herbivorous
animals. It may be isolated from the urine of the dog after feeding
phenylacetic acid. ^ It is produced in the organism through the synthesis
of glycocoll and phenylacetic acid. It is doubtful if it occurs in normal
human urine even after the ingestion of phenylacetic acid. It may be
decomposed into its component parts by boiling with dilute mineral
acids. The crystalline form of phenaceturic acid (small rhombic plates
with rounded angles) resembles one form of uric acid crystal.

HC = C-CH = CHCOOH
UROCANIC ACID, HN N

CH

This acid has been found in the urine of dogs, but not in human
urine. It is imidazolyl-acrylic acid. Hunter^ found it among the
pancreatic digestion products of casein. It crystallizes as sickle-shaped
crystals.

1 Sherwin: Dissertation, Tubingen, 1915.
* Hunter: Jour. Biol. Chetn., 11, 537, 1913.

URINE 399

PHOSPHORIZED COMPOUNDS

Phosphorus in organic combination has been found in the urine
in such bodies as glycerophosphoric acid, which may arise from the
decomposition of lecithin, and phosphocarnic acid. It is claimed that
on the average about 2.5 per cent of the total phosphorus elimination
is in organic combination.

PIGMENTS

There are at least three pigments normally present in human urine.
These pigments are urochrome, urobilin, and uroerythrin.

A. UROCHROME

This is the principal pigment of normal urine and imparts the char-
acteristic yellow color to that fluid. It is apparently closely related to
its associated pigment urobilin since the latter may be readily converted
into urochrome through evaporation of its aqueous-ether solution. Uro-
chrome may be obtained in the form of a brown, amorphous powder
which is readily soluble in water and 95 per cent alcohol. It is less
soluble in absolute alcohol, acetone, amyl alcohol and acetic ether, and
insoluble in benzene, chloroform, and ether. Urochrome is said to be a
nitrogenous body (4.2 per cent nitrogen), free from iron. Urochrome
is believed to be identical with the yellow pigment, lactocJirome, of
milk whey.^ The chromogen of urochrome, i.e., urochromogen is present
in the urine in pulmonary tuberculosis. Its presence is said to be of
prognostic value (see page 453).

B. UROBILIN

Urobilin, which was at one time considered to be the principal pig-
ment of urine, in reality contributes little toward the pigmentation of
this fluid. It is claimed that no urobilin is present in freshly voided nor-
mal urine but that its precursor, a chromogen called urobilinogen, is
present and gives rise to urobilin upon decomposition through the in-
fluence of light. It is claimed by some investigators that there are
various forms of urobilin, e.g., normal, febrile, physiological, and patho-
logical. Urobilin is said to be very similar to, if not absolutely identical
with, hydrobilirubin (see page 222).

Urobilin may be obtained as an amorphous powder which varies
in color from brown to reddish-brown, red and reddish-yellow, depend-
ing upon the way in which it is prepared. It is easily soluble in ethyl
alcohol, amyl alcohol, and chloroform, and slightly soluble in ether,

* Palmer and Coolidge: Jour. Biol. Chetn., 17, 251, 1914.

400 PHYSIOLOGICAL CHEMISTRY

acetic ether, and in water. Its solutions show characteristic absorption
bands (see Absorption Spectra, Plate II). Under normal conditions
urobilin is derived from the bile pigments in the intestine.

Urobilin is increased in most acute infectious diseases such as ery-
sipelas, malaria, pneumonia, and scarlet fever. It is also increased in
appendicitis, carcinoma of the liver, catarrhal icterus, pernicious anemia,
and in cases of poisoning by antifebrin. antipyrin, pyridin, and potas-
sium chlorate. In general it is usually increased when blood destruction
is excessive and in disturbances of the liver. It is markedly decreased
in phosphorus poisoning.

In liver disease, of any type, urobilinogen occurs in the urine. Its
detection is the basis of a specific test ior functional liver incapacity.

Experiments

1. Ammoniacal-zinc Chloride Test. — Render some of the urine ammoniacal
by the addition of ammonixun hydroxide, and after allowing it to stand a short
time filter off the precipitate of phosphates and add a few drops of zinc chloride
solution to the filtrate. Observe the production of a greenish fluorescence.
Examine the fluid by means of the spectroscope and note the absorption band
which occupies much the same position as the absorption band of urobilin in acid
solution (see Absorption Spectra, Plate II).

2. Ether-absolute Alcohol Test. — Mix urine and pure ether in equal volumes
and shake gently in a separatory funnel. Separate the ether extract, evaporate it
to dryness, and dissolve the residue in 2-3 c.c. of absolute alcohol. Note the
greenish fluorescence. Examine the solution spectroscopically and observe the
characteristic absorption band (see Absorption Spectra, Plate II).

3. Ring Test. — Acidify 25 c.c. of urine with 2-3 drops of concentrated hydro-
chloric acid, add 5 c.c. of chloroform and shake the mixture. Separate the chloro-
form, place it in a test-tube, and add carefiilly 3-5 c.c. of an alcoholic solution of
zinc acetate. Observe the formation of a green ring at the zone of contact of the
two fluids. If the tube is shaken a fluorescence may be observed.

4. Spectroscopic Examination. — Acidify the urine with hydrochloric acid and
allow it to remain exposed to the air for a few moments. By this means if any
urobilinogen is present it will be transformed into urobilin. The urine may now be
examined by means of the spectroscope. If urobilin is present in the fluid the char-
acteristic absorption band lying between b and F will be observed (see Absorption
Spectra, Plate II). It may be found necessary to dUute the urine with water before
a distinct absorption band is observed. This test may be modified by acidifjdng
10 c.c. of urine with hydrochloric acid and shaking it gently with 5 c.c. of amyl
alcohol. The alcoholic extract when examined spectroscopically will show the
characteristic urobilin absorption band. (Note the spectroscopic examination in
experiment (i) above.)

5. Iodine Test (Gerhardt).— To 20 c.c. of urine add 3-5 c.c. of chloroform
and shake well. Separate the chloroform extract and add to it a few drops of
iodine solution (I in KI). Render the mixture alkaline with dilute solution of
potassium hydroxide and note the production of a yellow or yellowish-brown color.
The solution ordinarily exhibits a greenish fluorescence.

URIXE 401

6. Alcoholic -zinc Chloride Test (Wirsing). — To 20 c.c. of urine add 3-5 c.c.
of chloroform and shake gently. Separate the chloroform extract and add to it
a drop of an alcoholic solution of zinc chloride. Note the rose-red color and the
greenish fluorescence. If the solution is turbid it may be rendered clear by the
addition of a few cubic centimeters of absolute alcohol.

C. UROERYTHRIN

This pigment is frequently present in small amount in normal urine.
The red color of urinary sediments is due in great part to the presence
of^uroerythrin. It is easily soluble in amyl alcohol, slightly soluble in
acetic ether, absolute alcohol, or chloroform, and nearly insoluble in
water. Dilute solutions of uroerythrin are pink in color while concen-
trated solutions are orange red or bright red; none of its solutions fluor-
esce. Uroerythrin is increased in amount after strenuous physical exer-
cise, digestive disturbances, fevers, certain liver disorders, and in various
other pathological conditions.

PTOMAINES AND LEUCOMAINES

These toxic substances are said to be present in small amount in
normal urine. Very little is known definitely, however, about them.
It is claimed that five different poisons may be detected in the urine,
and it is further stated that each of these substances produces a spe-
cific and definite symptom when injected intravenously into a rabbit.
The resulting symptoms are narcosis, salivation, mydriasis, paralysis,
and convulsions. The day urine is principally narcotic and is 2-4 times
as toxic as the night urine which is chiefly productive of convulsions.

PURINE BASES

The purine bases found in human urine are adenine, carnine, epi-
guanine, episarkine, guanine, xanthine, heteroxanthine, hypoxanthine,
paraxanthine, and i-methylxanthine. The main bulk of the purine
base content of the urine is made up of paraxanthine, heteroxanthine
and i-methylxanthine, which are derived for the most part from the caf-
feine, theobromine, and theophylline of the food. The total purine
base content is made up of the products of two distinct forms of metabo-
lism, i.e., metabolism of ingested nucleins and purines and metabolism
of tissue nuclein material. Purine bases resulting from the first form of
metabolism are said to be of exogenous origin, whereas those resulting
from the second form of metabolism are said to be of endogenous origin.
The daily output of purine bases by the urine is extremely small and
varies greatly with the individual (16-60 mg.). The output is increased
after the ingestion of nuclein material as well as after the increased de-
26

402 PHYSIOLOGICAL CHEMISTRY

struction of leucocytes. A well-marked increase accompanies leukemia.
Edsall and others have shown that the output of purine bases by the
urine is increased as a result of X-ray treatment. The purine bases
form a higher percentage of the total purine excretion in the case of
the monkey, sheep and goat than in man.

Experiment

I. Formation of the Silver Salts. — ^Add an excess of magnesia mixture ^ to
25 c.c. of urine. Filter off the precipitate and add ammoniacal silver solution^
to the filtrate. A precipitate composed of the silver salts of the various purine
bases is produced. The purine bases may be determined quantitatively by means
of Kriiger and Schmidt's method (see page 513), or Welker's method (see page
515)-

2. Inorganic Physiological Constituents

Ammonia

Next to urea, ammonia is the most important of the nitrogenous
end-products of protein metabolism. Ordinarily about 2.5-4.5 per
cent of the total nitrogen of the urine is eliminated as ammonia and
on the average this would be about 0.7 gram per day. Under normal
conditions the ammonia is present in the urine in the form of the
chloride, phosphate, or sulphate. This is due to the fact that combina-
tions of this sort are not oxidized in the organism to form urea, but are
excreted as guch. This explains the increase in the output as ammonia
which follows the administration of the ammonium salts of the mineral
acids or of the acids themselves. On the other hand, when ammonium
acetate and many other ammonium salts of certain organic acids are
administered no increase in the output of ammonia occurs since the salt
is oxidized and its nitrogen ultimately appears in the urine as urea.
Acid-forming foods (see page 580) also increase the ammonia output,
whereas the administration of alkalies or of base-forming foods decreases
the excretion of ammonia

Experiments^ indicate that the nitrogen in food protein may in
part be replaced by ammonium salts.

Copious water drinking increases the ammonia output. This fact
has been interpreted as indicating a stimulation of the gastric secretion.^

^Magnesia mixture may be prepared as follows: Dissolve 175 grams of MgS04 and
350 grams of NH4CI in 1400 c.c. of distilled water. Add 700 grams of concentrated NH4-
OH, mix very thoroughly and preserve the mixture in a glass-stoppered bottle.

^ Ammoniacal silver solution may be prepared according to directions given on page 593.

^ Grafe and Schlapfer: Zeit. physio! . chem., 77, i, 191 2, experiments by Abderhalden in
same journal.

•'Wills and Hawk: Jour. Am. Chem. Soc, 36, 158, 1914.

TRINE 403

The acids formed during the process of protein destruction within
the body have an influence upon the excretion of ammonia similar to
that exerted by acids which have been administered. Therefore a
pathological increase in the output of ammonia is observed in such
diseases as are accompanied by an increased and imperfect protein
metabolism, and especially in diabetes, in w-hich disease acetoacetic
acid and /3-oxybutyric acid are found in the urine in combination with
the ammonia.

Folin claims that a pronounced decrease in the extent of protein
metabolism, as measured by the total nitrogen in the urine, is frequently
accompanied by a decreased elimination of ammonia. The ammonia
elimination is therefore probably determined by other factors than the
total protein catabolism as such. Furthermore, he believes that a
decided decrease in the total nitrogen excretion is always accompanied
by a relative increase in the ammonia-nitrogen, provided the food is of a
character yielding an alkaline ash.

The quantitative determination of ammonia must be made upon
the fresh urine, since upon standing the normal urine will undergo am-
moniacal fermentation (see page 362).

Experiments
(See Experiment 2 under Phosphates, page 408.)

Sulphates

. Sulphur in combination is excreted in two forms in the urine: first,
as unoxidized, loosely combined or neutral sulphur, and second, as oxidized
or acid sulphur. The unoxidized or neutral sulphur is excreted mainly
as a constituent of such bodies as cystine, cysteine, taurine, hydrogen
sulphide, ethyl sulphide, thiocyanates, sulphonic acids, oxyproteic acid,
alloxyproteic acid, and uroferric acid. The amount of neutral sulphur
eliminated is in great measure independent of the extent of protein
decomposition or of the total sulphur excretion. In this characteristic
it is somewhat similar to the excretion of creatinine. The oxidized
sulphur is eliminated in the form of sulphuric acid, principally as salts of
sodium, potassium, calcium, and magnesium; a relatively small amount
occurs in the form of ethereal sulphuric acid, i.e., sulphuric acid in com-
bination with such orofnatic bodies as phenol, indole, skatole. cresol,
pyrocatechol, and hydroquinol. Sulphuric "acid in combination with
Na, K, Ca or Mg is sometimes termed inorganic or preformed sulphuric
acid, whereas the ethereal sulphuric acid is sometimes called conjugate
sulphuric acid. The greater part of the sulphur is eliminated in the

404 PHYSIOLOGICAL CHEMISTRY

oxidized form, but the absolute percentage of sulphur excreted as the
performed, ethereal or loosely combined type depends upon the total
quantity of sulphur present; i.e., there is no definite ratio between
the three forms of sulphur which will apply under all conditions. The
preformed sulphuric acid may be precipitated directly from acidified
urine with BaCl2, whereas the ethereal sulphuric acid must undergo a
preliminary boiling in the presence of a mineral acid before it can be
so precipitated.

The sulphuric acid excreted in the urine arises principally from
the oxidation of protein material within the body; a relatively small
amount is due to ingested sulphates. Under normal conditions about
2.5 grams of sulphuric acid (SO3) are eliminated daily, about 75-95 per
cent of this being in the form of sulphates. About 90 per cent of this
sulphate excretion is in the form of inorganic sulphate and 10 per cent as
ethereal sulphates. Since the sulphuric acid content of the urine has,
for the most part, a protein origin and since one of the most important
constituents of the protein molecule is nitrogen, it would be reasonable
to suppose that a fairly definite ratio might exist between the excretion
of these two elements. However, when we appreciate that the per-
centage content of N and S present in different proteins is subject to
rather wide variations, the fixing of a ratio which will express the exact
relation existing between these two elements as they appear in the urine
as end-products of protein metabolism is practically impossible. It
has been suggested that the ratio 5 : i expresses this relation in a general
way.

Pathologically, the excretion of sulphuric acid by the urine is in-
creased in acute fevers and in all other diseases marked by a stimulated
metabolism, whereas a decrease in the sulphuric acid excretion is observed
in those diseases which are accompanied by a loss of appetite and a
diminished metabolic activity.

Experiments

1. Detection of Inorganic Sulphuric Acid. — Place about 10 c.c. of urine in a
test-tube, acidify with acetic acid and add some barium chloride solution. A
white precipitate of barium sulphate forms.

2. Detection of Ethereal Sulphuric Acid. — Filter off the barium sulphate
precipitate formed in the above experiment, add i c.c. of hydrochloric acid and a
little barium chloride solution to the filtrate and heat the mixture to boiling for
1-2 minutes. Note the appearance of a turbidity due to the presence of sul-
phuric acid which has been separated from the ethereal sulphates and has com-
bined with the barium of the BaClo to form BaS04.

3. Detection of Unoxidized or Neutral Sulphur. — Place about 10 c.c. of urine
in a test-tube, introduce a small piece of zinc, add sufficient hydrochloric acid

URINE

405

Fig. 1 28. — Calcium Sulphate.
(Hensel and Weil.)

to cause a gentle evolution of hydrogen, and over the mouth of the tube place a
filter paper saturated with lead acetate solution. In a short time the portion of
the paper in contact with the vapors within the test-tube becomes blackened due
to the formation of lead sulphide. The nascent hydrogen has reacted with the
loosely combined or neutral stilphur to form hydrogen sulphide, and this gas com-
ing in contact with the lead acetate paper has caused the production of the black
lead sulphide. Sulphur in the form of inorganic or ethereal sulphuric acid does
not respond to this test.

4. Calciimi Sulphate Crystals. — Place 10 c.c. of urine in a test-tube, add 10
drops of calcium chloride solution and allow the tube to stand until crystals form.
Examine the calcium sulphate crystals under

the microscope and compare them with those ^^ 'JJj^' * A "V

shown in Fig. 128. . '.'^ . .

Chlorides

Next to urea, the chlorides consti-
tute the chief solid constituent of the
urine. The principal chlorides found
in the urine are those of sodium, potas-
sium, ammonium, and magnesium, with
sodium chloride predominating. The r,\

excretion of chloride is dependent, in great part, upon the nature of the
diet, but on the average the daily output is about 10-15 grams, expressed
as sodium chloride. Copious water drinking increases the output of
chlorides considerably. Because of their solubility, chlorides are never
found in the urinary sediment.

Since the amount of chlorides excreted in the urine is due primarily
to the chloride content of the food ingested, it follows that a decrease
in the amount of ingested chloride will likewise cause a decrease in the
chloride content of the urine. In cases of actual fasting the chloride
content of the urine may be decreased to a slight trace which is derived
from the body fluids and tissues. Under these conditions, however,
an examination of the blood of the fasting subject will show the per-
centage of chlorides in this fluid to be approximately normal. This
forms a very striking example of the care nature takes to maintain the
normal composition of the blood. There is a limit to the power of the
body to maintain this equilibrium, however, and if the fasting organism
be subjected to the influence of diuretics for a time, a point is reached
where the normal composition of the blood can no longer be maintained
and a gradual decrease in its chloride content- occurs which tinally results
in death. Death is supposed to result not so much because of a lack of
chlorine as from a deficiency of sodium. This is shown from the fact that
potassium chloride, for instance, cannot replace the sodium chloride

4o6 PHYSIOLOGICAL CHEMISTRY

of the blood when the latter is decreased in the manner above stated.
When this substitution is attempted the potassium salt is excreted at
once in the urine, and death follows as above indicated.

Pathologically the excretion of chlorides may be decreased in some
fevers, chronic nephritis, croupous pneumonia, diarrhoea, certain stom-
ach disorders, and in acute articular rheumatism. Any condition ac-
companied by the formation of an exudate {e.g., pneumonia) will cause
a diminished chloride output. In convalescence and with resolution
of the exudate the chloride excretion rises again.

Experiment

Detection of Chlorides in Urine. — Place about 5 c.c. of xxrine in a test-tube,
render it acid with nitric acid and add a few drops of a solution of silver nitrate.
A white precipitate, due to the formation of silver chloride, is produced. This
precipitate is soluble in ammonium hydroxide.

Phosphates

Phosphoric acid exists in the urine in two general forms: First,
that in combination with the alkali metals, sodium and potassium,
and the radical ammonium; second, that in combination with the
alkaline earth metals, calcium and magnesium. Phosphates formed
through a union of phosphoric acid with the alkali metals are termed
alkaline phosphates, or phosphates of the alkali metals, whereas phos-
phates formed through a union of phosphoric acid with the alkaline
earth metals are termed earthy phosphates, or phosphates of the alkaline
earth metals.

Three series of salts are formed by phosphoric acid: Normal,
M3PO4/ mono-hydrogen, M2HPO4, and di-hydrogen, MH2PO4. The di-
hydrogen salts are acid in reaction, and it is claimed that about 60 per
cent of the total phosphate content of the urine is in the form of this
type of salt, and that the acidity of the urine is due in great part to the
presence of sodium di-hydrogen phosphate (see page 361). Henderson-
maintains that "determinations of hydrogen ionization in urine and its
behavior toward indicators both support the view that in urine there
exists a mixture of mono- and di-hydrogen phosphates of sodium,
ammonium and other bases."

In bones the phosphates occur principally in the form of the normal
salts of calcium and magnesium. The mono-hydrogen salts as a class
are alkaline in reaction to litmus, and it is to the presence of di-sodium

1 M may be occupied by any of the alkali metals or alkaline earth metals.
* Henderson: Am. Jour. Physiol., 15, 257, 1906.

URINE 407

hydrogen phosphate, Xa2HP04, that the greater part of the alkalinity
of the saliva is due.

The excretion of phosphoric acid is extremely variable, but on the
average the total output for 24 hours is about 2.5 grams, expressed
asP205. Ordinarily the total output is mainly in the form of phosphates
and is distributed between alkaline phosphates and earthy phosphates
approximately in the ratio 2:1. The organic phosphorus of the urine
constitutes only 1-4 per cent of the total phosphorus content. The
greater part of this phosphoric acid arises from the ingested food, either
from the preformed phosphates or more especially from the phosphorus
in organic combination such as we find it in phospho-proteins, nucleo-
proteins and lecithins; the phosphorus-containing tissues of the body
also contribute to the total output of this element. Alkaline phosphates
ingested with the food have a tendency to increase the phosphoric acid
content of the urine to a greater extent than the earthy phosphates so
ingested. This is due, in a measure, to the fact that a portion of the
earthy phosphates, under certain conditions, may be precipitated in the
intestine and excreted in the feces; this is especially to be noted in the
case of herbivorous animals. Since the extent to which the phosphates
are absorbed in the intestine depends upon the form in which they are
present in the food, under ordinary conditions, there can be no absolute
relationship between the urinary output of nitrogen and phosphorus.
If the diet is constant, however, from day to day, thus allowing of the
preparation of both a nitrogen and a phosphorus balance,^ a definite
ratio may be established. In experiments upon dogs which were fed
an exclusive meat diet, the ratio of nitrogen to phosphorus, in the urine
and feces, was found to be 8.1 : i.

It has been demonstrated by recent investigation that the ingestion of
inorganic phosphorus compounds may give rise to organic phosphorus
compounds such as lecithin, phosphatides, nucleoproteins and phospho-
proteins. This is an instance of an organic substance synthesized from
an inorganic substance. The experiments have been made principally
on ducks- and hens.''

Pathologically the excretion of phosphoric acid is increased in such
diseases of the bones as diffuse periostosis, osteomalacia, and rickets ;
according to some investigators, in the early stages of pulmonary tuber-
culosis, in acute yellow atrophy of the liver, in diseases which are ac-
companied by an extensive decomposition of nervous tissue, and after

^ In metabolism experiments, a statement showing the relation existing between the
nitrogen content of the food on the one hand and that of the urine and feces on the other,
for a definite period, is termed a nitrogen balance or a "balance of the income and outgo of
nitrogen" (see chapter on Metabolism).

*Fingerling: Biochem. Zeit., 38, 448, 191 2.

'McCollum and Halpin: Jour. Biol. Chem., 11, 47 (Proceedings), 1912.

4o8

PHYSIOLOGICAL CHEMISTRY

sleep induced by potassium bromide or chloral hydrate (Mendel). It
is also increased after copious water drinking. A decrease in the
excretion of phosphates is at times noted in febrile affections, such as
the acute infectious diseases, in pregnancy, in the period during which
the fetal bones are forming, and in diseases of the kidneys, because of
non-elimination.

The so-called "phosphaturias" many times represent decreased
acidity and not increased phosphate content of the urine. Such con-
ditions are, however, significant as indicating a possible tendency to the
formation of phosphatic calculi.

Experiments

I. Formation of "Triple Phosphate." — Place some urine in a beaker, render
it alkaline with ammonium hydroxide, add a small amount of magnesimn sul-

FiG. 129. — "Triple Phosphate." (Ogden.)

phate solution and allow the beaker to stand in a cool place over night. Crystals
of ammonium magnesiiun phosphate, "triple phosphate," form under these con-
ditions. Examine the crystalline sediment under the microscope and compare
the forms of the crystals with those shown in Fig. 129, above.

2. Ammoniacal Fermentation. — Stand some urine aside in a beaker for
several days. Ammoniacal fermentation will develop and "triple phosphate"
crystals will form.

(a) Examine the sediment under the microscope and compare the crystals with
those shown in Fig. 129.

(b) Hold a glass rod dipped in concentrated hydrochloric acid near the
surface of the urine. Note the fumes of ammoniiun chloride.

(c) Insert a strip of red litmus paper in the urine. Permit the paper to dry.
Note the gradual restoration of red color, due to volatiUzation of ammonia
(volatile alkaU). Run a control test using 0.5 per cent Na2C03 (fixed alkali).

3. Detection of Earthy Phosphates. — Place 10 c.c. of urine in a test-tube and
render it alkaline with ammonium hydroxide. Warm the mixture and note the
separation of a precipitate of earthy phosphates.

URINE 409

4. Detection of Alkaline Phosphates. — Filter off the earthy phosphates as
formed in the last experiment, and add a small amount of magnesia mixture 'see
page 602) to the filtrate. Now warm the mixture and observe the formation of a
white precipitate due to the presence of alkaline phosphates. Note the difference
in the size of the precipitates of the two forms of phosphates from this same vol-
vune of urine. Which form of phosphates was present in the larger amount,
earthy or alkaline?

5. Influence upon Fehhng's Solution. — Place 2 c.c. of Fehhng's solution in a
test-tube, dilute it with 4 volumes of water and heat to boiling. Add a solution
of sodium dihydrogen phosphate, NaHjP04, a small amount at a time, and heat
after each addition. What do you observe? What does this observation force
you to conclude regarding the interference of phosphates in the testing of dia-
betic urine by means of Fehhng's test?

Sodium and Potassium

The elements sodium and potassium are always present in the urine.
Usually they are combined with such acidic radicals as CI, CO3, SO4
and PO4. The amount of potassium, expressed as KoO, excreted in
24 hours by an adult, subsisting upon a mixed diet, is on the average
2-3 grams, whereas the amount of sodium, expressed as Na20, under
the same conditions, is ordinarily 4-6 grams. The ratio of K to Na is
generally about 3 : 5. The absolute quantity of these elements excreted
depends, of course, in large measure upon the nature of the diet. Be-
cause of the non-ingestion of XaCl and the accompanying destruction
of potassium-containing body tissues, the urine during fasting contains
more potassium salts than sodium salts.

Pathologically the output of potassium, in its relation to sodium,
may be increased during fever; following the crisis, however, the out-
put of this element may be decreased. It may also be increased in
conditions associated with acidosis.

Calcium and Magnesium

The greater part of the calcium and magnesium excreted in the
urine is in the form of phosphates. The daily output of calcium, which
depends principally upon the nature of the diet, aggregates on the
average about 0.1-0.4 gram (expressed as CaO) per day. The per-
centage of calcium salts present in the urine at any one time (10-40
per cent of total calcium output) forms no dependable index as to the
absorption of this class of salts, since they are again excreted into the
intestine after absorption. It is therefore impossible to draw any satis-
factory conclusions regarding the excretion of calcium unless we obtain
accurate analytical data from both the feces and the urine.

4IO PHYSIOLOGICAL CHEMISTRY

Very little is known positively regarding the actual course of the
excretion of the calcium under pathological conditions. An excess
is found in some diseases of the bones, e.g., osteomalacia. In others
as in rickets the urinary excretion may be very low.

The daily excretion of magnesium by way of the urine usually
amounts to between o.i and 0.3 gram, expressed as MgO. The amount
depends mainly on the diet. About 50 per cent or more of the excreted
magnesium is usually eliminated by the kidneys, the remainder passes
out in the feces. There may be a retention of magnesium in certain
bone disorders accompanying a loss of calcium; in osteomalacia for
example. Thus the excretion of calcium and magnesium do not neces-
sarily run parallel.

Carbonates

Carbonates generally occur in small amount in the urine of man
and carnivora under normal conditions, whereas much larger quanti-
ties are ordinarily present in the urine of herbivora. The alkaline
reaction of the urine of herbivora is dependable in great measure upon
the presence of carbonates. In general a urine containing carbonates
in appreciable amount is turbid when passed or becomes so shortly
after. These bodies ordinarily occur as alkali or alkaline earth com-
pounds and the turbid character of urine containing them is usually
due principally to the latter class of substances. The carbonates of
the alkaline earths are often found in amorphous urinary sediments.

Iron

Iron is present in small amount in normal urine. It probably occurs
partly in inorganic and partly in organic combination. The iron con-
tained in urinary pigments or chromogens is in organic combination.
According to different investigators the iron content of normal urine will
probably not average more than 1-5 mg. per day. After splenectomy
there is an increased loss of iron from the body particularly by way of
the feces (Asher).

Experiment

Detection of Iron in Urine. — Evaporate a convenient volume (10-15 c.c.) of
urine to dryness. Incinerate and dissolve the residue in a few drops of iron-free
hydrochloric acid and dilute the acid solution with 5 c.c. of water. Divide the
acid solution into two parts and make the following tests: (a) To the first part add
a solution of ammonium thiocyanate; a red color indicates the presence of iron.
(b) To the second part of the solution add a little potassium ferrocyanide solution;
a precipitate of Prussian blue forms upon standing.

URJNE 411

Fluorides, Nitrates, Silicates and Hydrogen Peroxide

These substances are all found in traces in human urine under nor-
mal conditions. Nitrates are undoubtedly introduced into the organ-
ism in the water and ingested food. The average excretion of nitrates
is about 0.5 gram per day, the output being the largest upon a vegeta-
ble diet and smallest upon a meat diet. Nitrites are found only in
urine which is undergoing decomposition and are formed from nitrates
in the course of ammoniacal fermentation. Hydrogen peroxide has
been detected in the urine, but its presence is believed to possess no
pathological importance.

CHAPTER XXIII
URINE: PATHOLOGICAL CONSTITUENTS^

Glucose.

Proteins

Blood

Pus.

Bile.

Serum albumin.
Serum globulin.

Proteoses.

Peptone.

Nucleoprotein.

Fibrin.
I Oxyhemoglobin.
Form elements.
Pigment.

Deutero-proteose.
Hetero-proteose.
"Bence-Jones' protein.'

J Pigments.

I Acids.
Creatine.^
Acetone.
Acetoacetic acid.
/3-Hydroxybutyric acid.
Conjugate glycuronates.
Pentoses.
Fat.

Hematoporphyrin.
Lactose.
Galactose.
Fructose.
Arsenic.
Mercury.
Inositol.
Laiose.
Melanin.
Urorosein.
Nephrorosein.
Urochromogen.
Unknown substances.

1 See note at the bottom of page 369.
" Normal constituent of urine of infants and children.

412

URINE 413

GLUCOSE

Traces of this sugar occur in normal urine, but the amount is not
sufficient to be readily detected by the ordinary simple qualitative
tests. There are two distinct types of pathological glycosuria, i.e,
transitory glycosuria and persistent glycosuria. The transitory type
may follow the ingestion of an excess of sugar, causing the assimilation
limit to be exceeded, or it may accompany any one of several disorders
which cause impairment of the power of assimilating sugar. In the
persistent type large amounts of sugar are excreted daily in the urine
for long periods of time. Under such circumstances a condition known
as diabetes mellitus exists. In this disorder the urine may contain 10
per cent of glucose and the average sugar content is 3-5 per cent.
Ordinarily, diabetic urine which contains a high percentage of sugar
possesses a faint yellow color, a high specific gravity, and a volume
which is above normal. Over 100 grams of sugar are daily eliminated
in some severe cases of diabetes mellitus.

Experiments

The various tests for glucose in the urine which are embraced in the
experiments given herewith are based upon one of the following
properties of this sugar:

(i) Its power to reduce the oxides of certain metals in alkaline solution.

(2) Its power to rotate the plane of polarized light.

(3) Its power to form crystalline osazones with phenylhydrazine.

(4) Its ability to ferment with ordinary yeast.

I. Phenylhydrazine Reaction. — Test the urine according to one of the fol-
lowing methods : (a) To a small amount of phenylhydrazine mixture (enough to
fill the rounded portion of a small test-tube), furnished by the instructor,^ add
5 c.c. of the urine, shake well, and heat on a boiling water-bath for one-half to
three-quarters of an hour. Allow the tube to cool slowly (not imder the tap) and
examine the crystals microscopically (Plate III, opposite page 22). If the solu-
tion has become too concentrated in the boiling process it will be Ught red in color
and no crystals will separate until it is diluted with water.

Yellow crystalline bodies called osazones are formed from certain
sugars under these conditions, in general each individual sugar giving
rise to an osazone of a definite crystalline form which is typical for that
sugar.

It is important to remember in this connection that, of the simple
sugars of interest in physiological chemistry, glucose and fructose yield
the same osazone, with phenylhydrazine. Eachozazone has a definite

1 This mixture is prepared by combining one part of phenylhydrazinc-hydrochloride and
two parts of sodium acetate, by uriglit. These are thoroughly mi.xed in a mortar.

414

PHYSIOLOGICAL CHEMISTRY

melting-point, and as a further and more accurate means of identifica-
tion it may be recrystallized and identified by the determination of its
melting-point and nitrogen content. The reaction taking place in the
formation of phenylglucosazone is as follows:

CH2OH CH2OH

(CH0H)3
CHOH

+C6HbNH-NH2-

Glue
CH2OH

Glucose

Phenylhydrazine

(CH0H)3

+C6H5NH-NH2-
CHOH
yN-NHCeHe+HaO

Phenylhydrazone

CH2OH

(CH0H)3

! +C6H5NH-NH2-^

C = 0

|^N-NHC6H5+C6H5NH2+NH3

C

Aniline

(CH0H)3

C = N-NHC6H5+H20
I^N-NHCeHs

C

Glucosazone

(b) Place 5 c.c. of the urine in a test-tube, add i c.c. of phenylhydrazine-
acetate solution fiunished by the instructor/ and heat on a boiling water-bath
for one-half to three-quarters of an hour. Allow the Uquid to cool slowly and
examine the crystals microscopically (Plate III, opposite page 22).

The phenylhydrazine test has been so modified by Cipollina as to
be of use as a rapid clinical test. The directions for this test are given
in the next experiment.

2. CipoUina's Test. — Thoroughly mix 4 c.c. of urine, 5 drops of phenylhydrazine
(the base) and yi. c.c. of glacial acetic acid in a test-tube. Heat the mixture for
about one minute over a low flame, shaking the tube continually to prevent loss of
fluid by bumping. Add 4-5 drops of potassium hydroxide or sodium hydroxide
(sp. gr. 1. 1 6), being certain that the fluid in the test-tube remains acid; heat the
mixture again for a moment and then cool the contents of the tube. Ordinarily
the crystals form at once, especially if the urine possesses a low specific gravity.
If they do not appear immediately allow the tube to stand at least 20 minutes before
deciding upon the absence of sugar.

Examine the crystals under the microscope and compare them with those shown
in Plate III, opposite page 22.

3. Riegler's Reaction.'* — Introduce o.i gram of phenylhydrazine-hydrochloride
and 0.25 gram of sodium acetate into a test-tube, add 20 drops of the urine under

^ This solution is prepared by mixing one part by volume, in each case of glacial acetic
acid, one part of water and two parts of phenylhydrazine (the base).
^Riegler: Compt. rend. soc. biol., 66, p. 795.

URINE 415

examination, and heat the mixture to boiling. Now introduce 10 c.c. of a 3 per
cent solution of potassium hydroxide and gently shake the tube and contents. If
the urine under examination contains glucose the liquid in the tube will assume a
red color. One per cent glucose yields an immediate color whereas 0.05 per cent
yields the color only after the lapse of a period of one-half hour from the time the
alkali is added. If the color appears after the 30-minute interval the color change
is without significance inasmuch as sugar-free urines will respond thus. The reac-
tion is given by all aldehydes and therefore the test cannot be safely employed in
testing urines preserved by formaldehyde. Albumin does not interfere with the
test.

4. Bottu's Test.^ — To 8 c.c. of Bottu's reagent- in a test-tube add i c.c. of the
urine under examination and mix the liquids by gentle shaking. Now heat the
upper portion of the mixture to boiling, add an additional i c.c. of urine and heat
the mixture again immediately. The appearance of a blue color accompanied by
the precipitation of small particles of indigo blue indicates the presence of glucose
in the urine under examination. The test will serve to detect the presence of o.i
per cent of glucose and is uninfluenced by creatinine or by ammonium salts.

5. Reduction Tests. — To their aldehyde or ketone structure many
sugars owe the property of readily reducing the alkaline solutions of the
oxides of metals like copper, bismuth, and mercury; they also possess
the property of reducing ammoniacal silver solutions vi^ith the separa-
tion of metallic silver. Upon this property of reduction the most widely
used tests for sugars are based. When whitish-blue cupric hydroxide in
suspension in an alkaline liquid is heated it is converted into insoluble
black cupric oxide, but if a reducing agent like certain sugars be present
the cupric hydroxide is reduced to insoluble yellow cuprous hydroxide,
which in turn on further heating may be converted into brownish-red or
red cuprous oxide. These changes are indicated as follows:

OH

/
Cu -^Cu = 0+H20.

\ Cupric oxide

\ (black).

OH

Cupric hydroxide
(whitish-blue).

OH

/
Cu

\
OH

-^ 2Cu-0H-f HoO+0.

/^XJ Cuprous hydroxide
^•"- (yellow).

Cu

\
OH

^ Bottu: Cpmpl. rend. soc. bioL, 66, p. 972.

*This reagent contains 3.5 grams of c-nitrophenylpropiolic acid and 5 c.c. of a freshly
prepared 10 per cent solution of sodium hydro.xide per liter.

41 6 PHYSIOLOGICAL CHEMISTRY

Cu

Cu— OH
Cu— OH

0+H20.

Cu ■

Cuprous hydroxide Cuprous oxide
(yellow). (brownish-red).

The chemical equations here discussed are exempHfied in Trommer's
and Fehling's tests.

(a) Trommer^s Test. — To 5 c.c. of urine in a test-tube add one-half its volume
of KOH or NaOH. Mix thoroughly and add, drop by drop, agitating after the
addition of each drop, a very dilute solution of copper sidphate. Continue the addi-
tion until there is a slight permanent precipitate of cupric hydroxide and in conse-
quence the solution is slightly turbid. Heat, and the cupric hydroxide is reduced
to yellow cuprous hydroxide or to brownish-red cuprous oxide.

If the solution of copper sulphate used is too strong, a small brownish-red pre-
cipitate produced in the presence of a low percentage of glucose may be entirely
masked. On the other hand, if too little copper sulphate is used a light-colored
precipitate formed by uric acid and purine bases may obscure the brownish-red
precipitate of cuprous oxide. The action of KOH or NaOH in the presence of an
excess of sugar and insufficient copper will produce a brownish color. Phosphates
of the alkaline earths may also be precipitated in the alkaline solution and be mis-
taken for cuprous hydroxide. Trommer's test is not very satisfactory.

Salkowski^ has proposed a modification of the Trommer procedure which he
claims is a very accurate sugar test.

(b) Fehling's Test. — To about i c.c. of Fehling's solution- in a test-tube add'
about 4 CO.. of water, and boil.^ [The cupric hydroxide is held in solution by the
sodium potassium tartrate (Rochelle salt).] This is done to determine whether
the solution will of itself cause the formation of a precipitate of brownish-red
cuprous oxide. If such a precipitate forms, the Fehhng's solution must not be
used. Add urine to the hot Fehhng's solution, a few drops at a time, and heat the
mixture to boihng after each addition (never add more urine than the original
volume of Fehling's solution). The production of yellow cuprous hydroxide or
brownish-red cuprous oxide indicates that reduction has taken place. The
yellow precipitate is more hkely to occur if the urine is added rapidly and in large
amount, whereas with a less rapid addition of smaller amounts of urine the
brownish-red precipitate is generally formed.

This is a much more satisfactory test than Trommer's, but even
this test is not entirely reliable when used to detect sugar in the urine.

' Salkowski: Zeit. physiol. Chem., 79, 164, 191 2.

- Fehling's solution is composed of two definite solutions — a copper sulphate solution
and an alkaline tartrate solution, which may be prepared as follows:

Copper sulphate solution = 2,A-^S grams of copper sulphate dissolved in water and made
up to 500 c.c.

Alkaline tartrate solution = 1 25 grams of potassium hydroxide and 1 73 grams of Rochelle
salt dissoh-ed in water and made up to 500 c.c.

These solutions should be preserved separately in rubber-stoppered bottles and mixed
in equal volumes when needed for use. This is done to prevent deterioration.

^ More dilute Fehling solution should be used in testing urines containing small amounts
of sugar. In case of urines containing a high concentration of sugar it may sometimes be
desirable to use a larger volume of Fehling's solution.

URINE 417

Such bodies as conjugate glycuronates , uric acid, nucleo protein, and homo-
gentisic acid, when present in sufficient amount, may produce a result
similar to that produced by sugar. PJwsphates of the alkaline earths
may be precipitated by the alkali of the Fehling's solution and in appear-
ance may be mistaken for the cuprous hydroxide. Cupric hydroxide
may also be reduced to cuprous oxide and this in turn be dissolved by
creatinine, a normal urinary constituent. This will give the urine under
examination a greenish tinge and may obscure the sugar reaction even
when a considerable amount of sugar is present. According to Laird^
even small amounts of creatinine will retard the reaction velocity of re-
ducing sugars with P'ehling's solution.

Conjugate glycuronates are formed after the ingestion of such sub-
stances as chloral hydrate, camphor, menthol, thymol, antipyrin,
phenol, etc. The chloral hydrate is excreted in the urine as trichlor-
ethylglycuronic acid, C2CI3H2.C6H9O7. This compound reduces Fehl-
ing's solution and is levoiotdXory , whereas glucose also reduces but is
dextroioi2iiovy . Therefore by means of a polariscopic test we may dif-
ferentiate between a "chloral urine" and a "sugar urine."

In testing urine preserved by chloroform a positive test may be ob-
tained in the absence of sugar. This is due to the fact that the hot
alkali -produces formic acid (a reducing fatty acid) from the chloroform.

x^mmonium salts also interfere with Fehling's test. If present in
excess the urine should be made alkaHne and boiled in order to decom-
pose the ammonium salts.

(c) Benedict's Modifications of Fehling's Test. — First Modification. — To 2
c.c. of Benedict's solution- in a test-tube add 6 c.c. of distilled water and 7-^
drops (not more) of the urine under examination. Boil the mixture vigorously
for about 15-30 seconds and permit it to cool to room temperature spontaneously.
(If desired this process may be repeated, although it is ordinarily unnecessary.)
If sugar is present in the solution a precipitate will form which is often bluish-
green or green at first, especially if the percentage of sugar is low, and which
usually becomes yellowish upon standing. If the sugar present exceeds 0.06
per cent this precipitate generally forms at or below the boiling-point, whereas if
less than 0.06 per cent of sugar is present the precipitate forms more slowly and
generally only after the solution has cooled. The greenish precipitate obtained
with urines containing small amounts of sugar may be a compound of copper with
the sugar or a compound of some constituent of the urine with reduced copper

1 Laird: Journ. Path, and Bad., 16, 398 191 2.

* Benedict's modified Fehling solution consists of two definite solutions — a copper
sulphate solution and an alkaline tartrate solution, which may be prepared as follows:

Copper sulphate solution = 34.65 grams of copper sulphate dissolved in water and made
up to 500 c.c.

Alkaline tartrate solulion = ioo grams of anhydrous sodium carbonate and 173 grams of
Rochelle salt dissolved in water and made up to 500 c.c.

These solutions should be preserved separately in rubber-stoppered bottles and mi.xed
in equal volumes when needed for use. This is done to prevent deterioration.
27

41 8 PHYSIOLOGICAL CHEMISTRY

oxide instead of being a precipitate of cuprous hydroxide or oxide as is the case
when the original Fehhng solution is reduced.

Benedict claims that, whereas the original Fehling's test will not
serve to detect sugar when present in a concentration of less than o.i
per cent, that the above modification will serve to detect sugar when
present in as small quantity as 0.015-0.02 per cent. This claim has
been corroborated by Harrison.^ The modified solution used in the
above test differs from the original in that 100 grams of sodium car-
bonate is substituted for the 125 grams of potassium hydroxide ordi-
narily used, thus forming a Fehhng solution which is considerably
less alkaline than the original. This alteration in the composition of
the Fehling solution is of advantage in the detection of sugar in the
urine inasmuch as the strong alkalinity of the ordinary Fehling solu-
tion has a tendency, when the reagent is boiled with a urine containing
a small amount of glucose, to decompose sufficient of the sugar to
render the detection of the remaining portion exceedingly difficult
by the usual technic. Benedict claims that for this reason the use of
his modified solution permits the detection of smaller amounts of sugar
than does the use of the ordinary Fehling solution.

Second Modification. ^ — ^Benedict has fitrther modified his solution and has
succeeded in obtaining one which does not deteriorate upon long standing.*
The following is the procedure for the detection of glucose in the urine : To 5 c.c.
of the reagent in a test-tube add 8 (not more) drops of the urine to be examined.
The fluid is then boiled vigorously for from one to two minutes and then allowed
to cool spontaneously. In the presence of glucose the entire body of the solution
will be filled with a precipitate, which may be red, yellow, or green in color, de-
pending upon the amount of sugar present. If no glucose is present, the solution
will either remain perfectly clear, or will show a very faint turbidity, due to
precipitated urates.

Even very small quantities ot glucose in urine (o.i per cent)
yield precipitates of surprising bulk with this reagent, and the positive
reaction for glucose is the filhng of the entire body of the solution
with a precipitate, so that the solution becomes opaque. Since amount

1 Harrison: Pharm. Jour., 87, 746, 191 1.

2 Benedict: Jour. Am. Med. Ass'n, 57, 1193, 191X.
^Benedict's new solution has the following composition:

Copper sulphate 17 • 3 g™-

Sodium citrate 1 73 . o gm.

Sodium carbonate (anhydrous) 100. o gm.

Distilled water to 1000. o c.c.

With th'e aid of heat dissolve the sodium citrate and carbonate in about 600 c.c. of water.
Pour (through a folded filter if necessary) into a glass graduate and make up to 850 c.c.
Dissolve the copper sulphate in about 100 c.c. of water and make up to 150 c.c. Pour the
carbonate-citrate solution into a large beaker or casserole and add the copper sulphate
solution slowly, with constant stirring. The mixed solution is ready for use, and does not
deteriorate upon long standing.

URINE 419

rather than color of the precipitate is made the basis of this test, it
may be applied, even for the detection of small quantities of glucose,
as readily in artificial light as in daylight. Chloroform does not in-
terfere with this test nor do uric acid or creatinine interfere to such
an extent as in the case of Fehling's test.

(d) Haines' Test. — This is a copper reduction test similar in many
respects to the Fehling and Benedict reactions. In Haines' solution^
the cupric hydroxide is held in solution by glycerol instead of Rochelle
salt as in Fehling's solution.

Perform the test as follows : Introduce about 5 c.c. of Haines' solution^ into a
test-tube and heat to boUing. If no reduction occurs add 6-8 drops of the urine
and again bring to a boil. If glucose is present an abundant yeUow ("cuprous
hydroxide) or brownish-red ("cuprous oxidej precipitate is thrown down. This
test is about as delicate as Fehling's test.

(e) Allen's Modification of Fehling's Test. — The following procedure is recom-
mended: "From 7 to 8 c.c. of the sample of urine to be tested is heated to boiling
in a test-tube, and, without separating any precipitate of albumin which may be pro-
duced, 5 c.c. of the solution of copper sulphate used for preparing Fehling's solution is
added. This produces a precipitate containing uric acid, xanthine, hj-poxanthine,
phosphates, etc. To render the precipitation complete, however, it is desirable
to add to the liquid, when partially cooled, from i to 2 c.c. of a saturated solution of
sodium acetate having a feebly acid reaction to litmus. ^ The liquid is filtered and
to the filtrate, which will have a bluish-green color, 5 c.c. of the alkaline tartrate
mixture used for preparing Fehling's solution is added, and the liquid boiled for
15-20 seconds. In the presence of more than 0.25 per cent of sugar, separation of
cuprous oxide occurs before the boUing-point is reached; but with smaller quantities
precipitation takes place during the cooling of the solution, which becomes greenish,
opaque, and suddenly deposits cuprous oxide as a fine brownish-red precipitate."

Mercuric Oxide Reduction Test (Cramer).^ — This test depends on
the reduction of mercuric oxide in a weakly alkaline solution with the
formation of metallic mercury. The degree of alkalinity is an impor-
tant factor, as the test becomes more sensitive but less specific tke
greater the alkalinity of the reagent.

Apply the test as follows :

Introduce 3 c.c. of Cramer's "2.5 standard reagent"* into a test-tube and heat
to boiling. The reagent remains clear but becomes shghtly yellow. Add 3 c.c.
of urine and heat the mixture to boihng. Remove the tube from the flame, and

1 Haines solution may be prepared by dissolving 8.314 grams of copper sulphate in
400 c.c. of water adding 40 c.c. of glycerol and 500 c.c. of 5 per cent potassium hydroxide
solution.

* Sufficient acetic acid should be added to the sodium acetate solution to render it feebly
acid to litmus. A saturated solution of sodium acetate keeps well, but weaker solutions are
apt to become mouldy, and then possess the power of reducing Fehling's solution. Hence
it is essential in all cases of importance to make a blank test by mixing equal measures of
copper sulphate solution, alkahne tartrate solution and water, adding a little sodium acetate
solution, and heating the mixture to boiling.

'Cramer: Bioch. Jour., 9, 156, 1915.

* See Chapter II, page 28.

420 PHYSIOLOGICAL CHEMISTRY

after 30 seconds acidify with a few drops of acetic acid. Hold the tube over
ordinary print. If the tirine is normal, a slight but distinct turbidity remains
but the print is clearly readable. If sugar is present in the urine above the nor-
mal concentration, the contents of the tube darken and on standing a finely di-
vided precipitate of mercury settles to the bottom of the tube. The amount of
the precipitate depends upon the concentration of reducing sugar in the urine.

It is claimed that this test is free from fallacies inherent in Fehling's
test as the result of the reducing action of uric acid and creatinine.
The test is said to be more sensitive than Fehling's test or the bismuth
reduction tests, and is particularly suitable for the examination of
urines in which the amount of sugar present exceeds the normal amount
only slightly.

If the reagent be made more alkaline than indicated, it ceases to be
specific for reducing sugars.

(f) Bismuth Reduction Test (Boettger). — To 5 c.c. of urine in a test-tube add
I c.c. of KOH or NaOH and a very small amount of bismuth subnitrate, and boil.
The solution will gradually darken and finally assume a black color due to reduced
bismuth. If the test is made with urine containing albumin this must be removed,
by boiling and filtering, before applying the test, since with albumin a similar change
of color is produced (bismuth sulphide).

(g) Bismuth Reduction Test (Nylander). — To 5 c.c. of urine in a test-tube
add one-tenth its volume of Nylander's reagent^ and heat for five minutes
in a boiling water-bath. ^ The mixture will darken if reducing sugar is present
and upon standing for a few moments a black color will appear.

This color is due to the precipitation of bismuth. If the test is
made on urine containing albumin this must be removed, by boiling
and filtering, before applying the test, since with albumin a similar
change of color is produced. Glucose when present to the extent of
0.08 per cent may be easily detected by this reaction (Rabe^ claims that
o.oi per cent may be so detected). Uric acid and creatinine which
interfere with the Fehling test do not interfere with the Nylander's
reaction. It is claimed by Bechold that the bismuth reduction tests
give a negative reaction with solutions containing sugar when mercuric
chloride or chloroform is present. Other observers^ have failed to
verify the inhibitory action of the mercuric chloride and have shown
that the inhibitory influence of chloroform may be overcome by raising

1 Nylander's reagent is prepared by digesting 2 grams of bismuth subnitrate and 4 grams
of Rochelle salt in 100 c.c. of a 10 per cent potassium hydro.xide solution. The reagent is
then cooled and filtered.

^Hammarsten suggests that the solution be boiled for 2-5 minutes (according to the
sugar content) over a free flame and the tube then permitted to stand five minutes before
drawing conclusions.

*Rabe: Apolh. Ztg., 29, 554, 1914.

* Rehfuss and Hawk: Jour. Biol. Chem., 7, 267, 1910; also Zeidlitz: Upsala Lakdre-
foren Fork, N. F., 11, 1906.

URINE 421

the temperature of the urine to the boiling-point for a period of five
minutes previous to making the test.

Urines rich in indican, uroerythrin, urochrome or Jiema to porphyrin,
as well as urines excreted after the ingestion of large amounts of certain
medicinal substances, may give a darkening of the Xylander's reagent
similar to that of a true sugar reaction. It is a disputed point whether
the urine after the administration of urotropin will reduce the Xylan-
der reagent.^

Strausz- has recently shown that the urine of diabetics to whom
"lothion" (diiodohydroxypropane) has been administered will give a
negative Nylander's reaction and respond positively to the Fehling and
polarization tests. "lothion" also interferes with the Nylander test
in vitro whereas KI and I do not.

According to Rustin and Otto the addition of PtCU increases the
delicacy of Nylander's reaction. They claim that this procedure causes
the sugar to be converted quantitatively. No quantitative method has
yet been devised, however, based upon this principle.

A positive bismuth reduction test is probably due to the following
reactions:

(a) Bi(OH)2(NO)3+KOH->Bi(OH)3+KN03.

(b) 2Bi(OH)3— 30-^Bi2+3H20.

Bohmansson,^ before testing the urine under examination treats it
(10 c.c.) with 1 5 volume of 25 per cent hydrochloric acid and }i volume
of boneblack. This mixture is shaken one minute, then filtered,
and the neutralized filtrate tested by Nylander's reaction. Bohmansson
claims that this procedure removes certain interfering substances,
notably urochrome.

6. Fermentation Test. — Rub up in a mortar about 15 c.c. of the urine with a
small piece of compressed yeast. Transfer the mixture to a saccharometer
(Fig- 3> page 31 ) and stand it aside in a warm place for about 12 hours. If glu-
cose is present, alcohoUc fermentation will occur and carbon dioxide will collect
as a gas in the upper portion of the tube. On the completion of fermentation,
introduce, by means of a bent pipette, a little KOH solution into the graduated
portion, place the thumb tightly over the opening in the apparatus and invert the
saccharometer. Remembering that KOH has the power to absorb COj how
do you explain the result?'

7. Polariscopic Examination. — For directions as to the use of the polariscope
see Chapter II.

' Abt: Archives of Pediatrics, 24, 275, 1907; also VVeitbrecht: Schweiz. Woch., 47, 577,
1909.

"Strausz: Miiiich. mcd. Woch., 59, 85, 1912.

^Bohmansson: Biochcm. ZciL, 19, p. 281.

* The findings of Neuberg and associates indicate that the liberation of carbon dioxide
by yeast is not necessarily a criterion of the presence of sugar. The presence of an enzyme
called carboxylase has been demonstrated in yeast which has the power of splitting off COi
from the carboxyl group of amino- and other aliphatic acids.

42 2 PHYSIOLOGICAL CHEMISTRY

PROTEINS

Normal urine contains a trace of protein material, but the amount
present is so slight as to escape detection by any of the simple tests in
general use for the detection of protein urinary constituents. The
following are the more important forms of protein material which have
been detected in the urine under pathological conditions:

(i) Serum albumin.

(2) Serum globulin.

I Deutero-proteose.

(3) Proteoses \ Hetero-proteose.

[ "Bence- Jones' protein."

(4) Peptone.

(5) Nucleoprotein.

(6) Fibrin.

(7) Oxyhemoglobin.

ALBUMIN

Normal urine contains a trace of albumin which is too slight to be
detected by the usual procedures.

Albuminuria is a condition in which serum albumin or serum globulin
appears in the urine. There are two distinct forms of albuminuria, i.e.,
renal albuminuria and accidental albuminuria. Sometimes the terms
"true" albuminuria and "false" albuminuria are substituted for those
just given. In the renal type the albumin is excreted by the kidneys.
This is the more serious form of the malady and at the same time is more
frequently encountered than the accidental type. Among the causes of
renal albuminuria are altered blood pressure in the kidneys, altered
kidney structure, or changes in the composition of the blood entering
the kidneys, thus allowing the albumin to diffuse more readily. In the
accidental form of albuminuria the albumin is not excreted by the
kidneys as is the case in the renal form of the disorder, but arises from
the blood, lymph, or some albumin-containing exudate coming into
contact with the urine at some point below the kidneys. It has been
suggested^ that albuminurias may be classed as pre-renal, renal and
post-renal. The pre-renal type is illustrated by the albuminuria of
heart disease, whereas the post-renal form corresponds to what we have
called "accidental" albuminuria.

The determination of albumin may be of assistance in following the
course of kidney disturbances, but the results can only be interpreted
in the light of other clinical findings.

^ Bruce: Lancet, May 6, 191 1, p. 1205.

URINE 423

Experiments
(The urine should be filtered before performing these tests.)

Nitric Acid Ring Test (Heller.) — Place 5 c.c. of concentrated HNO3 in a test-
tube, incline the tube, and by means of a pipette allow the urine to flow slowly
down the side. The liquids should stratify with the formation of a white zone
of precipitated albumin at the point of juncture.

If the albumin is present in very small amount the white zone may
not form until the tube has been allowed to stand for several minutes.
If the urine is quite concentrated a white zone, due to uric acid or urates,
will form upon treatment with nitric acid as indicated. This ring may
be easily ditlerentiated from the albumin ring by repeating the test
after diluting the urine with 3 or 4 volumes of water, whereupon the
ring, if due to uric acid or urates, will not appear. It is ordinarily
possible to differentiate between the albumin ring and the uric acid ring
without diluting the urine, since the ring, when due to uric acid, has
ordinarily a less sharply defined upper border, is generally broader than
the albumin ring and frequently is situated in the urine above the point
of contact with the nitric acid. Concentrated urines also occasionally
exhibit the formation, at the point of contact, of a crystalline ring with
very sharply defined borders. This is urea nitrate and is easily dis-
tinguished from the "fluffy" ring of albumin. If there is any diflBi-
culty in differentiation a simple dilution of the urine with water, as
above described, will remove the difficulty. Various colored zones, due
either to the presence of indican, bile pigments, or to the oxidation of
other organic urinary constituents, may form in this test under certain
conditions. These colored rings should never be confounded with the
white ring which alone denotes the presence of albumin.

After the administration of certain drugs a white precipitate of
resin acids may form at the point, of contact of the two fluids and may
cause the observer to draw wrong conclusions. This ring, if composed
of resin acids, will dissolve in alcohol, whereas the albumin ring will not
dissolve in this solvent.

Weinberger has shown that a ring closely resembling the albumin
ring is often obtained in urines preserved for a considerable time by
thymol when subjected to the nitric acid test. The ring is due to the
formation of nitrosothymol and possibly nitrothymol. If the thymol
is removed from the urine by extraction with petroleum ether' previous
to adding nitric acid, the ring does not form.

An instrument called the albumoscope ijiorismascope) has been de-

1 Accomplished readily by gently agitating equal volumes of petroleum ether and the
urine under examination for two minutes in a test-tube before applying the test.

424

PHYSIOLOGICAL CHEMISTRY

vised for use in this test and has met with considerable favor. The
method of using the albumoscope is described below.

Use of the Albumoscope. — This instrument is intended to facilitate
the making of "ring" tests such as Heller's and Roberts'. In making
a test about 5 c.c. of the solution under examination is first intro-
duced into the apparatus through the larger arm (see Fig. 130),
and the reagent used in the particular test is then introduced through
the capillary arm and allowed to flow down underneath the solution
under examination. If a reasonable amount of care is taken there is
no possibility of mixing the two solutions and a defi-
nitely defined white "ring" is easily obtained at the
zone of contact.

2. Nitric Acid and Magnesium Sulphate Ring Test
(Roberts). — ^Place 5 c.c. of Roberts' reagent^ in a test-
tube, incline the tube, and by means of a pipette allow the
urine to flow slowly down the side. The liquids shovild
stratify with the formation of a white zone of precipitated
albumin at the point of juncture.

This test is a modification of Heller's ring test
and is rather more satisfactory than that test, since
the colored rings never form and the consequent
confusion is avoided. The albumoscope (see above)
may also be used in making this test.

Fig.

130. — Albumo-
scope.

3. Spiegler's Ring Test. — Place 5 c.c. of Spiegler's reagent^ in a test-tube, in-
cline the tube and, by means of a pipette, allow 5 c.c. of urine, acidified with acetic
acid, to flow slowly down the side. A white zone wUl form at the point of contact.
This is an exceedingly delicate test, in fact too delicate for ordinary clinical purposes,
since it serves to detect albumin when present in the merest trace (i : 250,000) and
hence most normal urines wUl give a positive reaction for albumin when this test is
applied. Proteose and peptone are also said to respond to this test.

4. Coagulation or Boiling Test. — (a) Heat 5 c.c. of urine to boiling in a test-
tube. (K the urine is not clear it should be filtered.) A precipitate forming at
this point is due either to albumin or to phosphates. Acidify the urine slightly
by the addition of 3-5 drops of very dilute acetic acid, adding the acid drop by
drop to the hot solution. If the precipitate is due to phosphates it will disappear
under these conditions, whereas if it is due to albumin it will not only fail to
disappear but will become more fiocculent in character, since the reaction of a

1 Robert's reagent is composed of i volume of concentrated HNO3 and 5 volumes of a
saturated solution of MgSO*.

* Spiegler's reagent has the following composition:

Tartaric acid 20 grams.

Mercuric chloride 40 grams.

Sodium chloride 5° grams.

Glycerol 100 grams.

Distilled water 1000 grams.

URINE 425

fluid must be acid to secure the complete precipitation of the albumin by this
coagulation process.

Too much acid should be avoided since it will cause the albumin to
go into solution. Certain resin acids may be precipitated by the
acid, but the precipitate due to this cause may be easily differentiated
from the albumin precipitate by reason of its solubility in alcohol.

(b) A modification of this test in quite general use is as follows : Fill a test-
tube two-thirds full of urine and gently heat the upper half of the fluid to boiling,
being careful that this fluid does not mix with the lower half. A turbidity indi-
cates albumin or phosphates. Acidify the urine sUghtly by the addition of 3-5
drops of dilute acetic acid, when the turbidity, if due to phosphates, will disappear.

Nitric acid is often used in place of acetic acid in these tests. In
case nitric acid is used ordinarily 1-2 drops is sufficient.

5. Acetic Acid and Potassium Ferrocyanide Test. — To 5 c.c. of urine in a
test-tube add 5-10 drops of acetic acid. Mix well and add potassium ferro-
cyanide drop by drop, until a precipitate forms.

This is a very delicate test. Schmiedl claims that a precipitate of
Fe(Cn)6K2Zn or Fe(Cn)6Zn2 is formed when urines containing zinc
are subjected to this test and that this precipitate resembles the
precipitate secured with protein solutions. In the case of human
urine a reaction was obtained when 0.000022 gram of zinc per cubic
centimeter was present. Schmiedl further found that the urine col-
lected from rabbits housed in zinc-lined cages possessed a zinc content
which was sufficient to yield a ready response to the test.

Proteoses may also be detected by this test. To differentiate
albumin from proteose perform the coagulation test (see page 424).

6. Tanret's Test. — To 5 c.c. of urine in a test-tube add Tanret's reagent* drop
by drop until a turbidity or precipitate forms. This is an exceedingly delicate test.
Sometimes the urine is stratified upon the reagent as in Heller's or Roberts' ring
test. According to Repiton, urates interfere with the delicacy of this test. Tanret,
however, claims that urates do not interfere inasmuch as any precipitate due to
urates may be brought into solution by heat, whereas an albumin precipitate under
the same conditions will persist. Tanret further states that mucin interferes with
the delicacy of the test and that it should therefore be removed from the urine
under examination by acidification with acetic acid and filtration before testing for
albumin. This test also serves to detect proteoses.

7. Sodium Chloride and Acetic Acid Test, — Mix two volumes of urine and one
volume of a saturated solution of sodium chloride in a test-tube, acidify with acetic
acid, and heat to boiling. The production of a cloudiness or the formation of a
precipitate indicates the presence of albumin. The resin acids may interfere here

^Tanret's reagent is prepared as follows: Dissolve 1.35 grams of mercuric chloride in
25 c.c. of water, add to this solution 3.32 grams of potassium iodide dissolved in 25 c.c. of
water, then make the total solution up to 60 c.c. with water and add 20 c.c. of glacial acetic
add to the mixture.

426 PHYSIOLOGICAL CHEMISTRY

as in the ordinary coagulation test (page 424), but they may be easily differentiated
from albumin by means of their solubility in alcohol.

GLOBULIN

Serum globulin is not a constituent of normal urine but frequently
occurs in the urine under pathological conditions and is ordinarily
associated with serum albumin. In albuminuria globulin in varying
amounts often accompanies the albumin, and the clinical significance
of the two is very similar. Under certain conditions globulin may occur
in the urine unaccompanied by albumin.

Experiments

Globulin will respond to all the tests just outlined under Albumin.
If it is desirable to differentiate between albumin and globulin in any
urine the following processes may be employed:

1. Saturation with Magnesium Sulphate. — Place 25 c.c. of neutral urine in
a small beaker and add pulverized magnesium sulphate in substance to the point
of saturation. If the protein present is globulin it will precipitate at this point.
If no precipitate is produced acidify the saturated solution with acetic acid and
warm gently. Albumin will be precipitated if present.

The above procedure may be used to separate globulin and albumin
if present in the same urine. To do this filter off the globulin after it
has been precipitated by the magnesium sulphate, then acidify the clear
solution and warm gently as directed. Note the formation of the
albumin precipitate.

2. Half-saturation with Ammonimn Sulphate. — Place 25 c.c. of neutral urine
in a small beaker and add an equal volume of a saturated solution of ammonium
sulphate. Globulin, if present, will be precipitated. If no precipitate forms add
ammonium sulphate in substance to the point of saturation. If albumin is present
it will be precipitated upon saturation of the solution as just indicated. This
method may also be used to separate globulin and albumin when they occur in the
same urine.

Frequently in urine which contains a large amount of urates a precipitate of
ammonium urate may occur when the ammonium sulphate solution is added to the
urine. This urate precipitate should not be confounded with the precipitate due
to globulin. The two precipitates may be differentiated by means of the fact that
the urate precipitate ordinarily appears only after the lapse of several minutes
whereas the globulin generally precipitates at once.

PROTEOSE AND PEPTONE

Proteoses, particularly deutero-proteose and hetero-proteose, have
frequently been found in the urine under various pathological con-
ditions such as diphtheria, pneumonia, intestinal ulcer, carcinoma,

URINE 427

dermatitis, osteomalacia, atrophy of the kidneys, and in sarcomata
of the bones of the trunk. The presence of proteose in the urine may
frequently be demonstrated in any pathological condition in which there
is absorption of partially digested pus. "Bence-Jones' protein," a
proteose-like substance, is of interest in this connection and its appear-
ance in the urine is believed to be of great diagnostic importance in
cases of multiple myeloma or myelogenic osteosarcoma. By some in-
vestigators this protein is held to be a variety of hetero-proteose, whereas
others claim that it possesses albumin characteristics. The origin of
"Bence- Jones' protein" is unknown. Its origin has at various times
been ascribed to the blood proteins, the bones or to abnormal metabo-
lism of protein material in the body. It occurs in the urine in about
80 per cent of the cases of multiple myeloma. If its presence is unac-
companied by multiple myeloma it is nearly always associated with
some disease of the blood-forming organs or of the bones. When
"Bence-Jones' protein" is hydrolyzed it is found to contain all the amino-
acids which are characteristic of typical proteins.

Peptone certainly occurs much less frequently as a constituent of
the urine than does proteose, in fact most investigators seriously ques-
tion its presence under any conditions. . There are many instances
of peptonuria cited in the early literature, but because of the uncertainty
in the conception of what really constituted a peptone it is probable that
in many cases of so-called peptonuria the protein present was really
proteose.

Experiments

I. Phosphotungstic Precipitation Test (v. Aldor). — ^Acidify 10 c.c. of urine
with hydrochloric acid, add phosphotungstic acid until no more precipitate forms
and centrifugate' the solution. Decant the supernatant fluid, add some abso-
lute alcohol to the precipitate, and centrifugate again. This washing with alcohol
is intended to remove the urobilin and hence should be continued so long as the
alcohol exhibits any coloration whatever. Now suspend the precipitate in water
and add potassium hydroxide to bring it into solution. At this point the solution
may be blue in color, in which case decolorization may be secured by gently
heating. Apply the biuret test to the cool solution. A positive biuret test indi-
cates the presence of proteoses.

2. Boiling Test. — Make the ordinary coagulation test according to the di-
rection given under Albumin, page 424. If no coagulable protein is found allow
the boiled urine to stand and note the gradual appearance, in the cooled fluid, of
a flaky precipitate of proteose. Spiegler's reaction may also be applied at this
point. A precipitalc indicates proteose.

3. Schulte's Method. — Acidify 50 c.c. of urine with dilute acetic acid and filter
off any precipitate of nucleoprotein which may form. Now test a few cubic centi-

^ If not convenient to use a centrifuge the precipitate may be filtered off and washed on
the filter paper with alcohol.

428 PHYSIOLOGICAL CHEMISTRY

meters of the urine for coagulable protein, by tests 2 and 4 under Albumin, pages
424-5. If coagulable protein is present remove it by coagulation and filtration
before proceeding. Introduce 25 c.c. of the urine, freed from coagulable protein,
into 150 c.c. of absolute alcohol and allow it to stand for 12-24 hours. Decant the
supernatant fluid and dissolve the precipitate in a small amount of hot water. Now
filter this solution, and after testing again for nucleoprotein with very dilute acetic
acid, try the biuret test. If this test is positive the presence of proteose is indicated.^

Urobilin does not ordinarily interfere with this test since it is almost entirely
dissolved by the absolute alcohol when the proteose is precipitated.

4. Detection of "Bence-Jones' Protein." — Heat the suspected urine very
gently, carefully noting the temperature. At as low a temperature as 4o°C. a
turbidity may be observed, and as the temperature is raised to about 6o°C. a
floccvdent precipitate forms and clings to the sides of the test-tube. If the urine
is now acidified very slightly with acetic acid and the temperature further raised
to ioo°C. the precipitate at least partly disappears; it wiU return upon cooling
the tube.

This property of precipitating at so low a temperature and of dissolving at a
higher temperature is typical of "Bence-Jones' protein" and may be used to differ-
entiate it from all other forms of protein material occurring in the urine.

NUCLEOPROTEIN

There has been considerable controversy as to the proper classifica-
tion for the protein body which forms the "nubecula" of normal urine.
By different investigators it has been called mucin, mucoid, phospho-
protein, nucleoalhumin, and nucleoprotein. Of course, according to
the modern acceptation of the meanings of these terms they cannot be
synonymous. Mucin and mucoid are glycoproteins and hence contain
no phosphorus (see page 112), whereas phosphoproteins and nucleo-
proteins are phosphorized bodies. It may possibly be that both these
forms of protein, i.e., the glycoprotein and the phosphorized type,
occur in the urine under certain conditions (see page 396). In this
connection we will use the term nucleoprotein. The pathological con-
ditions under which the content of nucleoprotein is increased includes
all affections of the urinary passages and in particular pyelitis, nephritis,
and inflammation of the bladder.

Experiments

I. Detection of Nucleoprotein. — Place 10 c.c. of urine in a small beaker,
dilute it with three volumes of water to prevent precipitation of urates, and make
the reaction very strongly acid with acetic acid. If the urine becomes turbid
it is an indication that nucleoprotein is present.

^ If it is considered desirable to test for peptone the proteose may be removed by satu-
ration with (NH4)2SO< according to the directions given on p. 120 and the filtrate tested
for peptone by the biuret test.

URINE 429

If the urine under examination contains albumin the greater portion of this
substance should be removed by boiling the urine before testing it for the pres-
ence of nucleoprotein.

2. Tannic Acid Precipitation Test (Ott). — Mix 25 c.c. of the urine with
an equal volimie of a saturated solution of sodixmi chloride and slowly add
Almen's reagent.' In the presence of nucleoprotein a voluminous precipitate
forms.

BLOOD

The pathological conditions in which blood occurs in the urine may
be classified under the two divisions hematuria and honoglohimiria.
In hematuria we are able to detect not only the hemoglobin but the
unruptured corpuscles as well, whereas in hemoglobinuria the pig-
ment alone is present. Hematuria is brought about through blood
passing into the urine because of some lesion of the kidney or of the
urinary tract below the kidney. Hemoglobinuria is brought about
through hemolysis, i.e., the rupturing of the stroma of the erythrocyte
and the liberation of the hemoglobin. This may occur in scurvy,
t3rphus, pyemia, purpura, and in other diseases. It may also occur as
the result of a burn covering a considerable area of the body, or may
be brought about through the action of certain poisons or by the in-
jection of various substances having the power of dissolving the
erythrocytes. Transfusion of blood may also cause hemoglobinuria.

Even in true hematuria the erythryocytes may escape detection if
the urine is ammoniacal inasmuch as the cells disintegrate under these
conditions.

Experiments

1. Potassixim Hydroxide Test (Heller) .—Render loc.c. of urine strongly alka-
line with potassium hydroxide solution and heat to boiling. Upon allowing the
heated urine to stand a precipitate of phosphates, colored red by the contained
hematin, is formed. It is ordinarily well to make a *' control " experiment using
normal urine, before coming to a final decision.

Certain substances, such as cascara sagrada, rhubarb, santonin, and senna,
cause the urine to give a similar reaction. Reactions due to such substances
may be differentiated from the true blood reaction by the fact that both the pre-
cipitate and the pigment of the former reaction disappear when treated with
acetic acid, whereas if the color is due to hematin the acid will only dissolve the
precipitate of phosphates and leave the pigment undissolved.

2. Teichmann's Hemin Test. — Place a small drop of the suspected urine or a
small amount of the moist sediment on a microscopic sUde, add a minute grain
of sodimn chloride and carefully evaporate to dryness over a low flame. Put a
cover-glass in place, run underneath it a drop of glacial acetic acid, and warm
gently until the formation of gas bubbles is observed. Cool the preparation,
examine under the microscope, and compare the form of the crystals with those

1 Dissolve 5 grams of tannic acid in 240 c.c. of 50 per cent alcohol and add 10 c.c. of 25
per cent acetic acid.

43© PHYSIOLOGICAL CHEMISTRY

reproduced in Figs. 78 and 79, page 265. (See Atkinson and Kendall's and
Nippe's modifications, page 264.)

3. Heller-Teichmann Reaction. — Produce the pigmented precipitate according
to directions given in Heller's test above. If there is a copious precipitate of phos-
phates and but little pigment the phosphates may be dissolved by treatment with
acetic acid and the residue used in the formation of the hemin crystals according
to directions in Experiment 2, above.

4. V. Zeynek and Nencki's Hemin Test. — To 10 c.c. of the urine under examina-
tion add acetone until no more precipitate forms. Filter ofif the precipitate and
extract it with 10 c.c. of acetone rendered acid with 2-3 drops of hydrochloric acid.
Place a drop of the resulting colored extract on a slide, immediately place a cover-
glass in position, and examine under the microscope. Compare the form of the
crystals with those shown in Figs. 78 and 79, page 265. Hemin crystals produced
by this manipulation are sometimes very minute, thus rendering it difficult to de-
termine the exact form of the crystal.

6. Guaiac Test. — Place 5 c.c. of urine in a test-tube and by means of a
pipette introduce a freshly prepared alcoholic solution of guaiac (strength about
I : 60) into the fluid until a turbidity results, then add old turpentine or hydro-
gen peroxide, drop by drop, until a blue color is obtained.

This is a very delicate test when properly performed. Buckmaster
has suggested the use of guaiaconic acid instead of the solution of
guaiac. The test is positive both before and after boiling the blood
for 15-20 seconds. Pus does not respond after boiling. Old, partly
putrefied pus gives the test even without the addition of hydrogen
peroxide or old turpentine whereas /res/? pus responds upon the addition
of hydrogen peroxide. See discussion on page 258 and test on page 262.

7. Schxunm's Modification of the Guaiac Test. — To about 5 c.c. of lurine^ in a
test-tube add about 10 drops of a freshly prepared alcoholic solution of guaiac.
Agitate the tube gently, add about 20 drops of old turpentine, subject the tube to
a thorough shaking, and permit it to stand for about 2-3 minutes. A blue color
indicates the presence of blood in the solution under examination. In case there
is not sufficient blood to yield a blue color under these conditions, a few cubic centi-
meters of alcohol should be added and the tube gently shaken, whereupon a blue
coloration will appear in the upper alcohol-turpentine layer.

A control test should always be made using water in place of urine. In the
detection of very minute traces of blood only 3-5 drops of the guaiac solution should
be employed. '\

8. Ortho-Tolidin Test (Ruttan and Hardisty).^ — To i c.c. of a 4 per cent
glacial acetic acid solution of o-tolidin' in a test-tube add i c.c. of the solution

^ Alkaline urine should be made sHghtly acid with acetic acid as the blue end-reaction
is very sensitive to alkaU.

2 Ruttan and Hardisty: Canadian Medical Assn. Journal, Nov., 191 2, also Biochemical
Bull., 2, 22s, 1913.

"NHz NH2

\ /

CsH^ — C6H4

/ \

CHj CH3

URINE 431

under examination and i c.c. of 3 per cent hydrogen peroxide. In the presence
of blood a bluish color develops (sometimes rather slowly) and persists for some-
time (several hours in some instances).

This test is said to be as sensitive for the detection of occult blood
in feces and stomach contents as is the benzidine reaction. It is also
claimed to be more satisfactory for urine than any other blood test.
The acetic acid solution may be kept for one month with no reduction
in delicacy.

9. Benzidine Reaction. — This is one of the most delicate of the reac-
tions for the detection of blood. Different benzidine preparations vary
greatly in their sensitiveness, however. Inasmuch as benzidine solu-
tions change readily upon contact with light, it is essential that they
be kept in a dark place.

The test is peformed as follows: To a saturated solution of benzidine in
alcohol or glacial acetic acid add an equal volume of 3 per cent hydrogen peroxide
and I c.c. of the urine under examination. If the mixture is not already acid,
render it so with acetic acid, and note the appearance of a blue color. A
control test should be made substituting water for the urine.

Often when urines containing a small amount of blood are tested by
this reaction, the mixture is rendered so turbid as to make it difl&cult to
decide as to the presence of a faint green color. Such urines should
be washed with water before the test is applied to it. The sensitiveness
of the benzidine reaction is greater when applied to aqueous solutions
than when applied to the urine.

For a modification of this test and further discussion see Chapter
XV on Blood and Lymph.

9. Spectroscopic Examination. — Submit the urine to a spectroscopic exami-
nation according to the directions given on page 296, looking especially for the
absorption bands of oxyhemoglobin and methemoglobin (see Absorption Spectra,
Plate I).

PUS

Pus may be present in the urine in inflammatory affections of
various types. Such a condition is termed pyuria. Albumin always
accompanies the pus. In catarrh of the bladder and in inflammation
of the urethra or of the pelvis of the kidney pus is particularly apt to
be present in the urine. If a urine of high pus concentration is voided
it may indicate the rupturing of an abscess in some part of the genito-
urinary tract. Pus may be detected by one of the procedures given
below.

Experiments

I . Microscopical Detection of Pus. — The characteristic form elements of pus are
leucocytes. They may occur in very small number in normal urine. Examine the

432 PHYSIOLOGICAL CHEMISTRY

urine (centrifugated if necessary) under the microscope. Any considerable number
of pus corpuscles indicates a pathological urine. In acid urine the pus corpuscles
appear as round, colorless cells, composed of refractive, granular protoplasm.
Sometimes they may exhibit amoeboid movements, particularly if the slide contain-
ing them be warmed slightly. They are nucleated (one or more nuclei), the nuclei
being clearly visible only upon treating the cells with water, acetic acid or some
other suitable reagent. In alkaline urine the pus corpuscles are often degenerated.
They may occur as swollen, transparent cells, which exhibit no granular structure.
If the degeneration has proceeded far enough the nuclei fade and the cell disinte-
grates and only debris remains.

Sometimes it is almost impossible to differentiate between pus corpuscles and
certain types of epithelial cells. In such a case apply one of the following chemical
tests.

2. Guaiac Test. — This test is not specific for pus, but is given by certain
other substances and particularly by blood (see Chapter XV). Perform the test
as follows : Acidify the urine (if alkaline) with acetic acid, filter, ^ and add tinc-
ture of guaiac to the sediment on the paper. If the pus is old, and partly putrefied
it will give a blue color. If no blue color is secured, add old turpentine, or hy-
drogen peroxide, drop by drop. A blue color formed only under these conditions
indicates fresh pus.

As a control test boil some of the urine (or sediment) for 15-20 seconds and
repeat the test. Pus does not respond after boiling. In the case of blood the
test is positive both before and after boiUng.

3. Potassium Hydroxide Test (Donne). — Separate the sediment from the
urine (by decantation, filtration or centrifugation) ; place a small piece of solid
potassium hydroxide on the sediment and stir. If pus is present (and particu-
larly if it be fresh pus and not disintegrated) the sediment will become slimy and
tough. If the sediment is mucus it will more or less pass into solution in the
concentrated alkali.

BILE

Both the pigments and the acids of the bile may be detected in the
urine under certain pathological conditions. Of the pigments, bilirubin
is the only one which has been positively identified in fresh urine; the
other pigments, when present, are probably derived from the bilirubin.
A urine containing bile may be yellowish-green to brown in color and
when shaken foams readily. The staining of the various tissues of the
body through the absorption of bile due to occlusion of the bile duct
cause a condition known as icterus or jaundice. Bile is always present
in the urine under such conditions unless the amount of bile reaching
the tissues is extremely small.

Experiments

Tests for Bile Pigments

Practically all of these tests for bile pigments are based on the
oxidation of the pigment by a variety of reagents with the formation
1 If desired, the urine may be centrifuged and the sediment used in the test.

URINE 433

of a series of colored derivatives, e.g., biliverdin (green), bilicyanin
(blue), choletelin (yellow).

1. Gmelin's Test— To about 5 c.c. of concentrated nitric acid in a test-tube
add an equal volume of urine carefully so that the two fluids do not mix. At the
point of contact note the various colored rings, green, blue, violet, red, and red-
dish-yellow.

2. Rosenbach's Modification of Gmelin's Test. — Filter 5 c.c. of urine through
a small filter paper. Introduce a drop of concentrated nitric acid into the cone
of the paper and observe the succession of colors as given in Gmelin's test.

3. Nakayama's Reaction. — To 5 c.c. of urine in a test-tube add an equal volume
of a 10 per cent solution of barium chloride. Centrifugate the mixture, pour off
the supernatant fluid, and heat the precipitate with 2 c.c. of Nakayama's reagent.^
In the presence of bUe pigments the solution assumes a blue or green color.

3. Huppert's Reaction. — Thoroughly shake equal volumes of urine and milk of
lime in a test-tube. The pigments imite with the calcium and are precipitated.
Filter off the precipitate, wash it with water, and transfer to a small beaker. Add
alcohol acidified slightly with hydrochloric acid and warm upon a water-bath untU
the solution becomes colored an emerald green.

According to Steensma, this procedure may give negative results even in the
presence of the pigments, owing to the fact that the acid-alcohol is not a suflBciently
strong oxidizing agent. He therefore suggests the addition of a drop of a 0.5 per
cent solution of sodium nitrite to the acid-alcohol mixture before warming on the
water-bath. Try this modification also.

4. Salkowski's Test — Render 5 c.c. of urine alkaline with a few drops of a 10
per cent sodium carbonate solution and add a 10 per cent solution of calcium
chloride, drop by drop, until the supernatant fluid exhibits the normal urinary color
when the contents of the test-tube are thoroughly mixed. Filter oft the precipitate,
and after washing it place it in a second tube with 95 per cent alcohol. Acidify the
alcohol with hydrochloric acid and, if necessary, shake the tube to bring the pre-
cipitate into solution. Heat the solution to boiling and observe the appearance of
a green color which changes through blue and violet to red; if no bile is present
the solution does not undergo any color change. This test will frequently exhibit
greater delicacy than Gmelin's test. Steensma's suggestions mentioned under
Huppert's Reaction, above, apply in connection with this test also.

5. Hammarsten's Reaction. — To about 5 c.c. of Hammarsten's reagent- in a
small evaporating dish add a few drops of urine. A green color is produced. If
more of the reagent is now added the play of colors as noted in Gmelin's test may
be obtained.

6. Smith's Test. — To 2-3 c.c. of urine in a test-tube add carefully about 5 c.c.
of dilute tincture of iodine (i : 10) so that the fluids do not mix. A green ring is
observed at the point of contact.

7. Salkowski-Schippers Reaction. — XeutraUze the acidity of 10 c.c. of the
urine under examination with a few drops of a dilute solution of sodium carbonate,
and add 5 drops of a 20 per cent solution of sodium carbonate and 10 drops of a 20

' Prepared by combining 99 c.c. of alcohol and i c.c. of fuming hydrochloric acid con-
taining 4 grams of ferric chloride per liter.

^ Hammarsten'.s reagent is made by mixing i volume of 25 per cent nitric acid and 19
volumes of 25 per cent hydrochloric acid and then adding i volume of this acid mixture
to 4 volumes of 95 per cent alcohol.
28

434 PHYSIOLOGICAL CHEMISTRY

per cent solution of calcium chloride. Filter off the resultant precipitate upon a
hardened filter paper and wash it with water. Remove the precipitate to a small
porcelain dish, add 3 c.c. of an acid-alcohol mixture^ and a few drops of a dilute
solution of sodium nitrite and heat. The production of a green color indicates the
presence of bile pigments.

8. Bonanno's Reaction. ^ — Place 5-10 c.c. of the urine under examination in a
smaU porcelain evaporating dish and add a few drops of Bonanno's reagent.' If
bile is present an emerald-green color will develop. Bonanno says the reaction is
not interfered with by any known normal or pathological urinary constituent.

Tests for Bile Acids

1, Sucrose — HjS04 Test (Pettenkofer). — To 5 c.c. of urine in a test-tube add
5 drops of a 5 per cent solution of sucrose. Now incline the tube, run about
2-3 c.c. of concentrated sulphmric acid carefully down the side and note the
red ring at the point of contact. Upon slightly agitating the contents of the
tube the whole soultion gradually assumes a reddish color. As the tube be-
comes warm, it should be cooled in running water in order that the tempera-
ture may not rise above 7o°C.

It is claimed that this test is not satisfactory in the presence of
protein and chromogenic substances which yield interfering colors
with sulphuric acid.

2. Furfural — H2SO4 Test (Mylius). — To approximately 5 c.c. of urine in a
test-tube add 3 drops of a very dilute (i : 1000) aqueous solution of furfural,

HC CH

HC C.CHO.

O

Now incline the tube, run about 2-3 c.c. of concentrated sulphuric acid carefully
down the side and note the red ring as above. In this case also, upon shaking
the tube, the whole solution is colored red. Keep the temperature below 7o°C.
as before.

3. Foam Test (v. Udransky). — To 5 c.c. of urine in a test-tube add 3-4 drops
of a very dilute (i : 1000) aqueous solution of furfural. Place the thiunb over the
top of the tube and shake until a thick foam is formed. By means of a small
pipette add 2-3 drops of concentrated sulphuric acid to the foam and observe the
dark pink coloration produced.

4. Surface Tension Test (Hay). — This test is based upon the principle that
bile acids have the property of reducing the surface tension of fluids in which
they are contained. The test is performed as follows: Cool about 10 c.c. of
urine in a test-tube to i7°C. or lower, and sprinkle a little finely pulverized sul-
ph\ir upon the surface of the fluid. The presence of bile acids is indicated if the

^ ^lade by adding 5 c.c. of concentrated hydrochloric acid to 95 c.c. of 96 per cent,
alcohol.

^11 Tommasi, 2, Xo. 21.

'This reagent may be prepared by dissolving 2 grams of sodium nitrite in 100 c.c. of
concentrated hydrochloric acid.

URINE 435

sulphur sinks to the bottom of the liquid, the rapidity with which the sulphur sinks
depending upon the amount of bile acids present in the urine. The test is said to
react with bile acids when the latter are present in the proportion i : 120,000.
Allen^ has recently suggested the quantitative determination of bile acids by a
surface tension method.

5. Neukomm's Modification of Pettenkofer's Test. — To a few drops of urine
in an evaporating dish add a trace of a dilute sucrose solution and one or more drops
of dilute sulphuric acid. Evaporate on a water-bath and observe the development
of a violet color at the edge of the evaporating mixture. Discontinue the evapora-
tion as soon as the color is observed.

6. Peptone Test (Oliver). — To 5 c.c. of urine add 2-3 drops of acetic acid,
filtering if necessary. Add an equal volume of a i per cent, solution of Witte's
peptone to the acid solut'on. A precipitate is formed which is insoluble in an excess
of acetic acid. This precipitate is a compound of protein and bile acids.

CH3

!

ACETONE, C=0.

CH3

It was formerly very generally believed that acetone appeared in the
urine under pathological conditions because of increased protein de-
composition. It is now generally thought that, in man, the output
of acetone arises principally from the breaking down of fatty tissues
or fatty foods within the organism. The quantity of acetone elimi-
nated has been shown to increase when the subject is fed an abundance
of fat-containing food as well as during fasting, whereas a replace-
ment of the fat w^th carbohydrates is followed by a marked decrease
in the acetone excretion. If no carbohydrate food is fed the output of
acetone bodies increases at once, producing a physiological acidosis
(see Chapter XXVII on Metabolism).

Acetone and the closely related bodies, i3-hydrox\'butyric acid and
acetoacetic acid, are generally classified as the acetone bodies. They
are all associated with a deranged metabolic function and may appear
in the urine together or separately, depending upon the conditions.
Acetone and diacetic acid may occur alone in the urine but ^-hy-
droxybutyric acid is never found except in conjunction with one or the
other of these bodies. Acetone and acetoacetic acid arise chiefly
from the oxidation of (3-hydroxybutyric acid. The relation existing
between these three bodies is shown in the following equations.

(a) CH3.CH(OH).CH2.COOH+O^CH3CO.CH2.COOH+H20.

fl-hydroxybutyric acid. Acetoacetic acid.

(b) CH3CO.CH2.COOH-^(CH3)2CO+COo.

Acetoacetic acid. Acetone.

^ Allen: Jour. Biol. Cliem., 22, 505, 1915.

436 PHYSIOLOGICAL CHEMISTRY

Acetone, chemically considered, is a ketone, di-methyl ketone. When
pure it is a liquid which possesses a characteristic aromatic fruit-like
odor, boils at 56-5 7°C. and is miscible with water, alcohol, or ether
in all proportions. Acetone is a physiological as well as a pathological
constituent of the urine and under normal conditions the daily output
(preformed acetone + acetoacetic acid) is about 3-15 mg.

Pathologically, the elimination of acetone is often greatly increased
and at such times a condition of acetonuria is said to exist. Values
from 0.02-6 grams or higher have been obtained for preformed acetone
plus acetone derived from acetoacetic acid. This pathological ace-
tonuria may accompany diabetes mellitus, scarlet fever, typhoid
fever, pneumonia, nephritis, phosphorus poisoning, grave anemias,
fasting, and a deranged digestive function; it also frequently accom-
panies auto-intoxication and chloroform and ether anethesia. The
types of acetonuria most frequently met with are those noted in febrile
conditions and in advanced cases of diabetes mellitus. The blood in
diabetic comas has been found to contain as high as 45 mg. of total
acetone (acetone + acetoacetic acid) for 100 c.c. of blood serum.

Experiments

1, Isolation from the Urine. — In order to facilitate the detection of acetone in
the urine, the specimen under examination should be distilled and the tests as given
below applied to the resulting distillate. If it is not convenient to distil the urine,
the tests may be conducted upon the undistilled fluid. To obtain an acetone dis-
tillate proceed as follows: Place 100-250 c.c. of urine in a distillation flask or retort
and render it acid with acetic acid. Collect about one-third of the original volume
of fluid as a distillate, add 5 drops of 10 per cent hydrochloric acid and redistil about
one-half of this volume. With this final distillate conduct the tests as given below.

2. Gunning's Iodoform Test. — To about 5 c.c. of the urine or distillate in
a test-tube add a few drops of Lugol's solution^ or ordinary iodine solution (I in
KI) and a few drops of dilute NH4OH to form a black precipitate (nitrogen iodide).
Allow the tube to stand (the length of time depending upon the content of
acetone in the fluid under examination) and note the formation of a yellowish sedi-
ment consisting of iodoform. Examine the sediment under the microscope and
compare the form of the crystals with those shown in Fig. 8, page 42.

If the crystals are not well formed recrystallize them from ether
and examine again. The crystals of iodoform should not be confounded
with those of calcium phosphate (Fig. 105, page 322) which may be formed
in this test, particularly if made upon the undistilled urine. This test
is preferable to Lieben's test (4) since no substance other than acetone
will produce iodoform when treated according to the directions for

^ Lugol's solution may be prepared by dissolving 4 grams of iodine and 6 grams of potas-
sium iodide in 100 c.c. of distilled water.

URIXE 437

this test; both alcohol and aldehyde yield iodoform when tested by
Lieben's test.

Gunning's test is rather satisfactory for the detection of acet<mc,
and has been used with good results even upon the undistilled urine.
Protein material apparently interferes with the reaction, and when
present the urine should be distilled and the distillate used.^ In
some instances where the amount of acetone present is very small it
is necessary to allow the tube to stand 24 hours before making the ex-
amination for iodoform crystals. This test serves to detect acetone
when present in the ratio i : 100.000.

3. Sodium Nitroprusside Test ('Legal;. — Introduce about 5 c.c. of the urine or
distillate into a test-tube, add a few drops of freshly prepared aqueous solution
of sodium nitroprusside and render the mixture alkaline with potassium hydrox-
ide. (Be sure to add the nitroprusside before the solution is rendered alkaline.)
A ruby-red color, due to creatinine, a normal urinary constituent, is produced (see
Weyl's test, page 385J. Add an excess of acetic acid and if acetone is present
the red color will be intensified, whereas in the absence of acetone a yellow color
will result. Make a control test upon normal urine to show that this is so.

A similar red color may be produced by paracresol in urines con-
taining no acetone.

Two hypotheses have been proposed to explain the color reaction
between acetone and nitroprusside: (i) The formation of a complex ion
of ferropentacyanide with the isonitroso compound of the ketone,
or (2) the formation of such an ion with the isordtroamine derivative
of the ketone. 2

4. Iodoform Test (Lieben). — Introduce 5 c.c. of the urine or distillate into a
test-tube, render it alkaUne with potassiimi hydroxide and add 1-2 c.c. of iodine
solution drop by drop. If acetone is present a yellowish precipitate of iodoform
will be produced. Identify the iodoform by means of its characteristic odor and
its typical crystalline form (see Fig. 8, page 42).

While fully as delicate as Gunning's test (2) this test is not as
accurate since, by means of the procedure involved, either alcohol or
aldehyde will yield a precipitate of iodoform. This test is especially
liable to lead to erroneous deductions when urines from the advanced
stages of diabetes are under examination, because of the presence of
alcohol formed from the sugar through fermentative processes.' If
protein is present in the urine to be tested it may prevent the acetone
from responding to the above reaction. It is therefore advisable to use

' Rosenbloom: Jour. Am. Med. Ass'n, 59, 445, 191 2.

*Cambi: Atli. accad, Lincei, 22, 376, 1913.

' Welker reports the production of a pink or red color during the application of this test
to the distillates from pathological urines which had been preserved with powdered thymol.
He found the color to be due to an iodothymol compound which had been previously pre-
pared synthetically by Messinger and Vortmann.

438 PHYSIOLOGICAL CHEMISTRY

the distillate to secure most accurate results.^ SobeP has suggested a
quantitative method for acetone based on Lieben's test.

5. Reynolds -Gunning Test. — This test depends upon the solubility of mercuric
oxide in acetone and is performed as follows : To 5 c.c. of the urine or distillate add
a few drops of mercuric chloride, render the solution alkaline with potassium hy-
droxide and add an equal volume of 95 per cent alcohol. Shake thoroughly in
order to bring the major portion of the mercuric oxide into solution and filter.
Render the clear filtrate faintly acid with hydrochloric acid and stratify some am-
monium sulphide (NH4)2S upon this acid solution. At the zone of contact a
blackish-gray ring of precipitated mercuric sulphide, HgS, will form. Aldehyde
also responds to this test. Aldehyde, however, has never been detected in the urine
and could be present in this instance only if the acidified urine was distilled too far.

6. Rothera's Reaction.^ — To 5-10 c.c. of urine or distillate in a test-tube add a
little solid ammonium sulphate, 2-3 drops of a freshly prepared 5 per cent solution
of sodium nitroprusside and 1-2 c.c. of concentrated ammonium hydroxide. The
development of a permanganate color indicates the presence of acetone.

Hunter* claims that this reaction serves to detect acetoacetic acid rather than
acetone. Others claim it detects both acetone and acetoacetic acid.

8. Salicylaldehyde Reaction (Frommer). — Render 10 c.c. of urine strongly
alkaline with potassium hydroxide, add 10-12 drops of a 10 per cent solution of
salicylaldehyde in absolute alcohol and warm the mixture to about 70°. K
acetone be present the fluid becomes yellow, then red, reddish-piurple and dark
red in turn. The color of the urine is practically unchanged if no acetone is
present.

This color is due to the formation of dihydroxydibenzoylacetone
through the interaction of saUcylaldehyde and acetone.

CH3

I
ACETOACETIC ACID, C = 0

I
CH2COOH.

Acetoacetic or diacetic acid occurs in traces in normal urine.
The sum of the acetone and the acetoacetic acid excreted in normal
urine per day ranges from 3 to 15 mg. and ordinarily three-quarters
of this is acetoacetic acid. Under certain pathological conditions
it occurs in larger quantities and is rarely found except associated
with acetone. It is formed from jS-hydroxybutyric acid, another of
the acetone bodies, and upon decomposition yields acetone and car-
bon dioxide. Acetoaceturia occurs ordinarily under the same condi-
tions as the pathological acetonuria, i.e., in fevers, diabetes, etc. (pp.
435 and 534). If very little acetoacetic acid is formed it may be
transformed into acetone, whereas if a larger quantity is produced both

^Rosenbloom: Jour. Am. Med. Ass'n, 59, 445, 1912.
^Sobel: Schweiz. Apoth. Zlg., 52, 62, 1914.
•Rothera: Jour. Physiol., 37, 491, 1908.
* Hunter: Quart. Jour. Exp. Physiol., 8, 13, 1914.

URINE 439

acetone and acetoacetic acid may be present in the urine. Aceto-
aceturia is most frequently observed in children, especially accompany-
ing fevers and digestive disorders; it is perhaps less frequently observed
in adults, but when present, particularly in fevers and diabetes it is
frequently followed by fatal coma.

Acetoacetic acid is a colorless liquid which is miscible with water,
alcohol and ether, in all proportions. It differs from acetone in giving
a violet-red or Bordeaux-red color with a dilute solution of ferric
chloride.

Experiments^

1. Le Nobel Reaction.- — Make lo c.c. of urine add with acetic acid, add a
few drops of a dilute aqueous solution of sodium nitroprusside and stratify con-
centrated ammonium hydroxide upon the mixture. In the presence of aceto-
acetic acid a violet ring forms at once.

Acetone also responds to this test, but the test is more delicate for aceto-
acetic acid and the response is more prompt.

2. Ferric Chloride Test (Gerhardt). — To 5 c.c. of urine in a test-tube add
ferric chloride solution, drop by drop, until no more precipitate forms. In the
presence of acetoacetic acid a Bordeatix-red color is produced; this color may be
somewhat masked by the precipitate of ferric phosphate, in which case the fluid
should be filtered.

A positive result from the above manipulation simply indicates the possible
presence of acetoacetic acid. Before making a final decision regarding the pres-
ence of this body make the two following control experiments :

(aj Place 5 c.c. of urine in a test-tube, small beaker, or Erlenmeyer flask
and boil it vigorously for 3-5 minutes. Cool the vessel and, with the boiled
urine, make the test as given above. As has been already stated, acetoacetic
acid yields acetone upon decomposition and acetone does not give a Bordeaux-
red color with ferric chloride. By boiling as indicated above, therefore, any
acetoacetic acid present would be decomposed into acetone and carbon dioxide
and the test upon the resulting fluid would be negative. If positive, the color
is due to the presence of bodies other than acetoacetic acid.

(b) Place 5 c.c. of urine in a test-tube, acidify with HjS04, to free aceto-
acetic acid from its salts, and carefully extract the mixture with ether by shaking.
If acetoacetic acid is present it will be extracted by the ether. Now remove
the ethereal solution, evaporate it to dryness, dissolve the residue in 1-2 c.c.
of water and add 3-5 drops of 3 per cent ferric chloride. Acetoacetic acid is
indicated by the production of the characteristic Bordeaux-red color.

This color disappears spontaneously in 24-48 hours. Such sub-
stances as antipyrin, kairin, phenacetin, saHcyhc acid, saHcylates,
sodium acetate, thiocyanates, and thallin yield a similar red color

^ To prepare a diacetic acid solution which may be added to urine, if urines containing
this acid are not available, proceed as follows: Treat 13 grams of ethyl acetoacetate with
500 c.c. of N/5 sodium hydroxide. Allow to stand for 48 hours to hydrolyze'the ester.
In preparing urine for tests add i part of this solution to 10 parts of urine.

^Harding and Ruttan: Biochem. Jour., 6, 445, 1912; also Biochem. Bull., 2, 223, 1913.

440 PHYSIOLOGICAL CHEMISTRY

under these conditions, but when due to the presence of any of these
substances the color does not disappear spontaneously but may re-
main permanent for days. Many of these disturbing substances are
soluble in benzene or chloroform and may be removed from the urine
by this means before extracting with ether as above. Acetoacetic
acid is insoluble in benzene or chloroform.

3. Sodium Nitrite — ^Ferrous Sulphate Reaction (Hurtley). — Place 10 c.c.
of urine in a large test-tube, add 21/2 c.c. of concentrated hydrochloric acid
and I c.c. of fresh i per cent sodium nitrite. Shake the tube and permit it to
stand for two minutes. Add 15 c.c. of concentrated ammonium hydroxide and
5 c.c. of 10 per cent ferrous sulphate. Shake the tube and permit it to stand.
Note the slow development of a violet or purple color in the presence of aceto-
acetic acid.

This test serves to detect acetoacetic acid when present in a dilu-
tion of I to 50,000. The concentration of the acetoacetic acid regulates
the speed at which the color develops. If the concentration be very
low an interval of five hours may elapse before the color appears.
The test is believed to be specific for acetoacetic acid.

4. Arnold -Lipliawsky Reaction. — This reaction is somewhat more delicate than
Gerhardt's test (2) and serves to detect acetoacetic acid when present in the pro-
portion of I 125,000. It is also negative toward acetone, /?-hydroxybutyric acid
and the interfering drugs mentioned as causing erroneous deductions in the applica-
tion of Gerhardt's test. If the urine under examination is highly pigmented it
should be partly decolorized by means of animal charcoal before applying the test
as indicated below.

Place 5 c.c. of the urine under examination and an equal volume of the Arnold-
Lipliawsky reagent^ in a test-tube, add a few drops of concentrated ammonia and
shake the tube vigorously. Note the production of a brick-red color. ' Take 1-2
c.c. of this colored solution, add 10-20 c.c. of hydrochloric acid (sp. gr. 1.19), 3 c.c.
of chloroform, and 2-4 drops of ferric chloride solution and carefully mix the fluids.
Acetoacetic acid is indicated by the chloroform assuming a violet or blue color; if
acetoacetic acid is absent the color may be yellow or light red.

H OHH
^-HYDROXYBUTYRIC ACID, H — C — C — C — COOH.

H H H

This acid occurs in normal urine in traces, e.g., 20-30 mg. jper day.^

It is found under certain pathological conditions in larger quantities

^ This reagent consists of two definite solutions which are ordinarily preserved separately
and mixed just before using. The two solutions are prepared as follows:

(a) One per cent aqueous solution of potassium nitrite.

(b) One gram of ^-amino-acetophenon dissolved in 100 c.c. of distilled water and
enough hydrochloric acid (about ? c.c.) added, drop by drop, to cause the solution, which
is at first yellow, to become entirely colorless. An excess of acid must be avoided.

Before using, a and b are mixed in the ratio 1:2.

2 Shaffer and Marriott: Jour. Biol. C/iem., 16, 265, 1913.

URINE 44 1

and then always in conjunction with either acetone or acetoacetic acid.
Either of these bodies may be formed from /3-hydroxybutyric acid under
proper conditions. It is present in especially large amount in severe
cases of diabetes and has also been detected in digestive disturbances,
continued fevers, scurvy, measles, and in fasting. It is probable
that, in man, /S-hydroxybut^Tic acid, in common with acetone and
acetoacetic acid, arises principally from the breaking down of fatty
tissues mthin the organism. Any condition in which large amounts
of acetone and acetoacetic acid, and in severe cases /3-hydroxybutyric
acid also, are excreted in the urine is known as an "acidosis." In
diabetes the deranged metabolic conditions cause the production of
great quantities of these suDstances which lead to an acid intoxication
and ultimately to diabetic coma. In severe diabetes 50-100 grams or
over per day may be excreted. In such conditions the jS-hydroxy-
butyric acid may constitute 60-80 per cent of the total acetone bodies.
In rare cases we may have an excretion of large amounts of j8-hydroxy-
butyric acid with a low acetone output. An acidosis may also occur
under certain physiological conditions (see Chapter XXVII on Metab-
olism).

Ordinarily jS-hydroxybutyric acid is an odorless, transparent syrup
which is levorotatory and easily soluble in water, alcohol, and ether;
it may be obtained in crystalline form.

Experiments

I. Black's Reaction.' — Inasmuch as the urinary pigments as well as any
contained sugar or acetoacetic acid will interfere with the delicacy of this test
when applied to the urine directly, the following preliminary procedure is neces-
sary: Concentrate 10 c.c. of the urine under examination to one-third or one-
fourth of its original volume in an evaporating dish at a gentle heat. Acidify
the residue with a few drops of concentrated hydrochloric acid, add sufficient
plaster of Paris to make a thick paste and allow the mixture to stand until it
begins to "set." It should now be stirred and broken up in the dish by means
of a stirring rod with a blunt end. Extract the porous meal thus produced twice
with ether by stirring and decantation. Any ,3-hydroxybutyric acid present
will be extracted by the ether. Evaporate the ether extract spontaneously or
on a water-bath, dissolve the residue in water, and neutralize it with barium
carbonate. To 5 to 10 c.c. of this neutral fluid in a test-tube add 2 to 3
drops of ordinary commercial acid hydrogen peroxide. Mix by shaking and
add a few drops of Black's reagent.- Permit the tube to stand and note the
gradual development of a rose color which increases to its maximum intensity
and then gradually fades. ^

^ Black: Jour. Biol. C/tem., 5, 207, 1908.

* Made by dissolving 5 grams of ferric chloride and 0.4 gram of ferrous chloride in 100
c.c. of water.

^ This disappearance of color is due to the further o.xidation of the acetcacedc acid.

44 2 PHYSIOLOGICAL CHEMISTRY

In carrying out the test care should be taken to see that the solution
is cold and approximately neutral and that a large excess of hydrogen
peroxide and Black's reagent are not added. In case but little
/3-hydroxybutyric acid is present the color will fail to appear or will
be but transitory if the oxidizing agents are added in too great excess.
It is preferable to add a few drops of the reagent and at intervals of
a few minutes repeat the process until the color undergoes no further
increase in intensity. One part of /3-hydroxybutyric acid in 10,000
parts of the solution may be detected by this test.

2. Polariscopic Examination. — Subject some of the urine (free from protein)
to the ordinary fermentation test (see page 421). This will remove glucose
and fructose, which would interfere with the polariscopic test. Now examine the
fermented fluid in the polariscope and if it is levorotatory the presence of /3-hy-
droxybutyric acid is indicated. This test is not absolutely reliable, however, since
conjugate glycuronates are also levorotatorj^ after fermentation.

CONJUGATE GLYCURONATES

Glycuronic acid does not occur free in the urine, but is found, for
the most part, in combination with phenol. Much smaller quantities
are excreted in combination with indoxyl and skatoxyl. The total
content of conjugate glycuronates seldom exceeds 0.004 per cent Under
normal conditions. The output may be very greatly increased as
the result of the administration of antipyrin, borneol, camphor,
chloral hydrate, menthol, morphine, naphthol, turpentine, etc. The
glycuronates as a group are levorotatory whereas glycuronic acid is
dextrorotatory. Most of the glycuronates reduce alkaUne metallic
oxides and so introduce an error in the examination of urine for sugar.
Conjugate glycuronates often occur associated with glucose in glyco-
suria, diabetes mellitus, and in some other disorders. As a class the
glycuronates are non-fermentable.

Experiments

1. Naphthoresorcinol Reaction (ToUens). — Introduce 5 c.c. of urine in a
test-tube and add 0.5-1 c.c. of a i per cent solution of naphthoresorcinol in
95 per cent alcohol, and 5 c.c. of concentrated hydrochloric acid. Raise the
temperature gradually to the boiling-point and boil for one minute, shaking the
tube continuously. Stand the tube aside four minutes, then cool vmder the
tap. Extract with an equal volume of ether. Glycuronates are indicated by
the ether extract assuming a violet-red color. The spectroscope shows this
extract to possess two absorption bands, one on the D line and one to the right
of this line.

2. Polariscopic-Fermentation Test. — If glucose is present in the urine tested

URINE 443

for glycuronates the urine may first be subjected to a polariscopic examination,
then fermented and a second polariscopic examination made. The sugar being
dextrorotatory and fermentable and the glycuronates being levorotatory and
non-fermentable the second polariscopic test will show a levorotation indicative
of conjugate glycuronates.

3. Reduction-Polariscopic Test. — Test the urine by FehUng's test. If
positive try the Resorcinol-HCl reaction for fructose. If negative test the optical
activity. Levorotation indicates glycuronates.

PENTOSES

We have two distinct types of pentosuria, i.e., alimentary pentosuria,
resulting from the ingestion of large quantities of pentose-rich vegetables
such as prunes, cherries, grapes, or plums, and fruit juices, in which
condition the pentoses appear only temporarily in the urine; and the
chronic form of pentosuria, in which the output of pentoses bears no
relation whatever to the quantity and nature of the pentose content
of the food eaten. In occurring in these two forms, pentosuria re-
sembles glycosuria (see page 413), but it is definitely known that pen-
tosuria bears no relation to diabetes melhtus and there is no generally
accepted theory to account for the occurrence of the chronic form of
pentosuria. The pentose detected most frequently in the urine is
arabinose, the inactive form generally occurring in chronic pentosuria
although keto-pentose^ may occur in some cases. The levorotatory
variety occurs in the aHmentary t^-pe of the disorder.

Experiments

1. Orcinol-Hydrochloric Acid Reaction (Bial).- — To 5 c.c. of Bial's reagent'
in a test-tube add 2-3 c.c. of urine and heat the mixture gently until the first
bubbles rise to the surface.^ Immediately or upon cooling the solution becomes
green and a fiocculent precipitate of the same color may form.

This test is believed to be more accurate than the original orcinol
test. It is claimed that urines containing menthoL kreosotal, etc.,
respond to the old orcinol reaction, but not to Bial's. If so desired
the osazone of the pentose may be formed, then distilled with hydro-
chloric acid and the distillate tested by Bial's test (Jolles).

2. Phloroglucinol-Hydrochloric Acid Reaction (Tollensi. — To equal volxmies
of urine and hydrochloric acid (sp. gr. 1.09) add a Uttle phloroglucinol and heat
the mixture on a boiling water-bath. Pentose, galactose, or glycuronic acid

'Levene and La Forge: Jour. Biol. Cliem., 18, 319, 1Q14.

'Bial: Deut. tned. Woch., 28, 252, 1902

'Orcinol ... 15 grams.

Fuming HCl 500 grams.

Ferric chloride (10 per cent) 20-30 drops.

* The test may also be performed by adding the urine to the hot reagent. No further
heating should be necessary if pentose is present.

444 PHYSIOLOGICAL CHEMISTRY

will be indicated by the appearance of a red color. To differentiate between
these bodies examine by the spectroscope and look for the absorption band
between D and E given by pentoses and glycuronic acid, and then differentiate
between the two latter bodies by the melting-points of their osazones.

3. Orcinol Test. — Place equal volumes of urine and hydrochloric acid (sp. gr.
1.09) in a test-tube, add a smaU amount of orcinol, and heat the mixture to boiling.
Color changes from red through reddish-blue to green will be noted. When the
solution becomes green it should be shaken in a separatory funnel with a little
amyl alcohol, and the alcoholic extract examined spectroscopically. An absorption
band between C and D will be observed.

FAT

When fat finds its way into the urine through a lesion which brings
some portion of the urinary passages into communication with the
lymphatic system a condition known as chyluria is established. The
turbid or milky appearance of such urine is due to its content of chyle.
This disease is encountered most frequently in tropical countries, but
is not entirely unknown in more temperate climates. Albumin is a
constant constituent of the urine in chyluria. Upon shaking a chylous
urine with ether the fat is dissolved by the ether and the urine becomes
clearer or entirely clear.

HEMATOPORPHYRIN

Urine containing this body is occasionally met with in various
diseases, but more frequently after the use of quinine, tetronal, trional,
and especially sulphonal. Such urines ordinarily possess a reddish
tint, the depth of color varying greatly under different conditions.

Experiments

1. Spectroscopic Examination. — ^To 100 c.c. of urine add about 20 c.c. of
a 10 per cent solution of potassium hydroxide or ammonium hydroxide. The
precipitate which forms consists principally of earthy phosphates to which the
hematoporphyrin adheres and is carried down. Filter off the precipitate, wash
it and transfer to a flask and warm with alcohol acidified with hydrochloric acid.
By this process the hematoporphyrin is dissolved and on filtering will be found
in the filtrate and may be identified by means of the spectroscope (see page
296, and Absorption Spectra, Plate 11),

2. Acetic Acid Test. — To 100 c.c. of urine add 5 c.c. of glacial acetic acid and
allow the mixture to stand 48 hours. Hematoporphyrin deposits in the form of a
precipitate.

LACTOSE

Lactose is rarely found in the urine except as it is excreted by women
during pregnancy, during the nursing period, or soon after weaning.

URINE 445

It is rather difficult to show the presence of lactose in the urine in a
satisfactory manner, since the formation of the characteristic lactos-
azone is not attended with any great measure of success under these
conditions. It is, however, comparatively easy to show that it is not
glucose, for, while it responds to reduction tests, it does not ferment
with pure yeast and does not give a glucosazone. An absolutely
conclusive test, of course, is the isolation of the lactose in crystalline
form (Fig. 104, page 318) from the urine.

On oxidation with nitric acid lactose and galactose yield mucic acid.
This test is frequently used in urine examination to differentiate lactose
and galactose from other reducing sugars. To differentiate lactose
from pentose, since neither ferments, we may apply the Orcinol— HCl
test of Bial, see page 443.

Experiments

1. Mucic Acid Test. — Treat 100 c.c. of the urine under examination with
20 c.c.^ of concentrated nitric acid and evaporate the mixture in a broad, shallow
glass vessel, upon a boiling water-bath until the volimie of the solution is only
about 20 c.c. At this point the fluid should be clear and a fine white precipitate
of mucic acid should separate.

If the percentage of lactose in the urine is low it may be necessary
to cool the solution and permit it to stand for some time before the
precipitate \\-ill form. It is impossible to differentiate between galactose
and lactose by means of this test, but the reaction does serve to dif-
ferentiate these two sugars from all other reducing sugars. A sat-
isfactory differentiation between lactose and galactose in pure solution
may be made by means of Barfoed's test, page 30. This test is,
however, not suited for urine examination. To differentiate galactose
and lactose in urine use the Phloroglucinol-Hydrochloric Acid Reaction
of Tollens, see pages 36 and 443.

2. Rubner's Test. — To 10 c.c. of urine in a small beaker add some lead acetate,
in substance, heat to boiling, and add NH4OH until no more precipitate is dissolved.
In the presence of lactose a brick-red or rose-red color develops, whereas glucose
gives a coffee-brown color, maltose a light yellow color, and fructose no color at all
under the same conditions.

3. Compotmd Test. — Try the Nylander reaction. If positive tr>- the phenyl-
hydrazine test. If negative (the lactosazone is not readily formed in urine) apply
the fermentation test. If this test is also negative, differentiate between lactose
and pentose by Orcinol-HCl reaction (Bial) and mucic acid tests.

^ If the specific gravity of the urine is 1020 or over it is necessary to use 25-35 c.c. of
nitric acid. Under these conditions the mixture should be evaporated until the remaining
volume is appro.ximately equivalent to that of the nitric acid added.

44^ PHYSIOLOGICAL CHEMISTRY

GALACTOSE

Galactose has occasionally been detected in the urine, and in par-
ticular in that of nursing infants afiflicted with a deranged digestive
function. Lactose and galactose may be differentiated from other
reducing sugars which may be present in the urine by means of the
mucic acid test. This test simply consists in the production of mucic
acid through oxidation of the sugar with nitric acid.

V Experiments

1. Mucic Acid Test. — Treat loo c.c. of the urine under examination with
20 c.c.^ of concentrated nitric acid and evaporate the mixture in a broad, shallow
glass vessel, upon a boiling water-bath, until the volume of the solution is only
20 c.c. At this point the fluid should be clear and a fine, white precipitate of
mucic acid should separate.

If the percentage of galactose present in the urine is low it may be
necessary to cool the solution and permit it to stand for some time
before the precipitate will form. It is impossible to differentiate
between galactose and lactose by means of this test, but the reaction
does serve to differentiate these two sugars from all- other reducing
sugars. A satisfactory differentiation between galactose and lactose
may be made by the Phloroglucinol-Hydrochloric Acid Test of Tollens,
below.

2. Phloroglucinol-Hydrochloric Acid Reaction (Tollens). — To equal volumes of
the urine and hydrochloric acid (sp. gr. 1.09) add a little phloroglucinol and heat
the mixture on a boiling water-bath. Galactose, pentose, and glycuronic acid will
be indicated by the appearance of a red color. Galactose may be differentiated
from the two latter substances in that its solutions exhibit no absorption bands
upon spectroscopical examination.

FRUCTOSE

Diabetic urine frequently possesses the power of rotating the plane of
polarized light to the left, thus indicating the presence of a levorotatory
substance. The levorotation is sometimes due to the presence of
fructose, although not necessarily confined to this carbohydrate, since
conjugate glycuronates and j8-hydroxybutyric acid, two other levo-
rotatory bodies, are frequently found in the urine of diabetics. Fructose
is invariably accompanied by glucose in diabetic urine, but Jruc-
tosuria has been observed as a separate anomaly. The presence of

^ If the specific gravity of the urine is 1020 or over it is necessary to use 25-35 c.c. of
nitric acid. Under these conditions the mixture should be evaporated until the remaining
volume is approximately equivalent to that of the nitric acid added.

URINE 447

fructose may be inferred when the percentage of sugar, as determined
by the titration method, is greater than the percentage indicated by
the polariscopic examination.

Experiments

1. Borchardt's Reaction. — To about 5 c.c. of urine in a test-tube add an equal
volume of 25 per cent hydrochloric acid and a few crystals of resorcinol. Heat to
boiling and after the production of a red color, cool the tube under running water
and transfer to an evaporating dish or beaker. Make the mixture sUghtly alka-
line with solid potassium hydroxide, return it to a test-tube, add 2-3 c.c. of
acetic ether, and shake the tube vigorously. In the presence of fructose the
acetic ether is colored yellow.

The only urinary constituents which interfere with the test are
nitrites and indican and these interfere only when they are simul-
taneously present. Under these conditions, the urine should be acidified
with acetic acid and heated to boiling for one minute to remove the
nitrites. In case the indican content is very large, it will impart a blue
color to the acetic ether, thus masking the yellow color due to fructose.
When such urines are to be examined, the indican should first be re-
moved by Obermayer's test (see page 388). The chloroform should
then be discarded, the acid-urine mixture diluted with one-third its
volume of water, and the test applied as described above. The urine
of patients who have ingested santonin or rhubarb responds to the test.
The test will serve to detect fructose when present in a dilution of
I : 2000, i.e., 0.05 per cent.

2. Resorcinol-Hydrochloric Acid Reaction (Seliwanofif). — To 5 c.c. of SeUwa-
nofif's reagent^ in a test-tube add a few drops of the urine under examination
and heat the mixture to boiling. The presence of fructose is indicated by the
production of a red color and the separation of a red precipitate. The latter
may be dissolved in alcohol to which it will impart a striking red color.

If the boiling be prolonged a similar reaction may be obtained with
urines containing glucose. This has been explained- in the case of
glucose as due to the transformation of the glucose into fructose by
the catalytic action of the hydrochloric acid. The precautions neces-
sary for a positive test for fructose are as follows: The concentration of
the hydrochloric acid must not be more than 12 per cent. The reac-
tion (red color) and the precipitate must be observed after not more than
20-30 seconds of boiling. Glucose must not be present in amounts
exceeding 2 per cent. The precipitate must be soluble in alcohol with
a bright red color.

' Seliwanofif's reagent may be prepared by dissolving 0.05 gram of resorcinol in 100 c.c.
of dilute (i: 2) hydrochloric acid.

^Koenigsfeld: Bioch. Zeit. 38, 311, 1912.

448 PHYSIOLOGICAL CHEMISTRY

3. Phenylhydrazine Test. — Make the test according to directions under Glu-
cose, 3, page 22.

4. Polariscopic Examination. — A simple polariscopic examination, when taken
in connection with other ordinary tests, will furnish the requisite data regarding
the presence of fructose, provided fructose is not accompanied by other levorotatory
substances, such as conjugate glycuronates and )3-hydroxybutyric acid.

ARSENIC

When any soluble form of arsenic is introduced into the body in
any way, it is quickly absorbed and distributed by the blood and
lymph. The absorption is influenced by the quantity and quality of
the food in the stomach, and the activity of the circulation of the part
in contact with the poison. Some of the absorbed arsenic may be
returned to the alimentary canal by way of the bile and gastro-intes-
tinal mucous membrane. After absorption it may be deposited in the
Uver, kidneys, brain, bone, muscles, and walls of the stomach and
intestines. It is eHminated in all of the excretions, but chiefly by the
kidneys and through the feces. It does not appear very promptly in
the urine but continues to be excreted in the urine over a long period
of time, in some cases for several months. The urine may be examined
for arsenic by the following methods.

I. Marsh and Marsh-Berzelius Method. — This method has the advantage of
serving as a qualitative and quantitative determination, and is a very delicate test ;
it is, however, long and tedious. The various steps in the analysis are: (i) the
destruction of the organic matter in the urine; (2) treatment with sulphuric acid to
drive off excess nitric acid and break up nitro-compounds; and (3) application of
independent test to the resultant solution. Proceed as follows: The urine, to
which is added one-third its volume of nitric acid, is placed in a casserole or evapo-
rating dish and evaporated at 150° to 160° to a syrupy consistency. The mass is
then allowed to cool and 5 c.c. concentrated sulphuric acid added, and gentle heat
applied. The heating must be done cautiously, or deflagration takes place and
some of the arsenic is sure to be lost. The mass will liquefy and finally darken,
indicating organic matter. Cool and add concentrated nitric acid, i c.c, and apply
very gentle heat; copious reddish-brown fumes are evolved. Gradually raise the
temperature until darkening of the solution occurs, then cool, add i c.c. concentrated
nitric acid and again apply gentle heat, and repeat the process until the solution
faUs to darken. Now raise the temperature until white fumes begin to come off.
At this temperature excess nitric acid will have been removed and all nitro-com-
pounds broken up. The solution at this point is clear and at most a pale straw color.
Cool and add a mixture of 10 c.c. concentrated sulphuric acid and 40 c.c. water,
and test for arsenic using a Marsh apparatus. The apparatus (see Fig. 131, p. 449)
consists of a wide-mouth flask — 250 c.c. capacity — fitted with a two-hole stopper.
Through one hole is passed the stem of a separatory funnel of 50 to 60 c.c. capacity.
Through the other hole a piece of glass tube bent at right angles, which is fitted to
a calcium chloride tube, and this in turn to a narrow quartz tube, the distal end of

URINE

449

which is drawn to a fine bore and bent up almost at a right angle. All joints must
be air-tight.

Introduce 30 to 40 grams of arsenic-free granulated zinc into the flask, insert
the stopper and through the funnel introduce 50 c.c. dilute sulphuric acid (i part
to 4 parts water). After a few minutes collect a test-tube of gas by inverting a
test-tube over the end of the quartz tube, and test it by igniting. When the gas in
the test-tube ignites quietly, light the gas issuing from the quartz tube.

Hold a clean porcelain crucible lid in the flame and note whether any deposit
occurs. This precaution must be taken to insure that the chemicals and apparatus
are not contaminated with arsenic.

Now introduce the prepared urine solution into the funnel and adjust the flow
so that 6 to 8 drops are introduced into the flask per minute. Immediately hold a
clean porcelain crucible lid in the flame and at the first evidence of a dark deposit
apply heat, using a wing-top burner, to the quartz tube. The arsenic if present
will deposit in the quartz tube beyond the flame. Now test the spot on the lid
to see if it is arsenic; it should dissolve readily in sodium hypochlorite solution.

.jZ.

Fig. 131. — Marsh Apparatus.

Continue the operation for two hours, remove the Bunsen burner and again hold
the lid in the flame. If no more deposits on the lid, the arsenic has all come over
and is deposited in the quartz tube; if deposition occurs, apply the Bunsen again
and repeat.

When complete, remove the quartz tube, weigh it after cooling, then dissolve
out the arsenic with nitric acid, wash, dry, and weigh again. The difference in
weight is the weight of metallic arsenic in the volume of urine taken.

2. Reinsch's Test. — This test is very much simpler, but not so delicate. It
has the advantage of application in the presence of organic matter. The test is
performed as follows: The urine, acidified with one-fifth its volume of pure hydro-
chloric acid, is placed in a beaker. A piece of bright copper foil free from arsenic
is then introduced, and the urine heated almost to the boiling-point. It is then
set aside for six to eight hours. The arsenic is deposited on the copper foil, bluish-
gray color. The foil is then removed, washed successively in pure water, alcohol,
ether, and dried without heat. The foil is then rolled into a scroll and inserted
into a 3 mm. bore glass tube 4 inches long, about i inch from the end. The tube is
29

450 PHYSIOLOGICAL CHEMISTRY

then held in the bunsen flame at an angle of 20 to 25 degrees applying heat where
the copper foil is situated. The arsenic volatilizes and is oxidized, and deposits as
octahedral crystals of arsenic trioxide on the cooler part of the tube. The crystals
can readily be recognized by the microscope and sometimes with a simple magnify-
ing lens.

Mercury

The rapidity of absorption of mercury depends upon a number of
conditions such as, mode of administration, the nature of the com-
pound and its physical state, the state and condition of the stomach
and intestines, the quantity and quaHty of the food in the stomach
and the state of the circulation of the portal of entrance. There is
no definite knowledge as to the form in which it is absorbed. Elimina-
tion depends upon the state of the excretory organs. It is eliminated
as an albuminate in all the excretions of the body, urine, feces, saliva,
sweat, tears, and milk. Elimination begins about two hours after
introduction. Depending upon the amount introduced and absorbed,
the time required for its complete elimination varies from 24 hours to
many weeks. Mercury may be detected in the urine by the following
methods.

1. Reinsch's Test. — The procedure is carried out in the same manner as for
arsenic (see above). A piece of arsenic-free copper foil is introduced into the urine
acidified with one-fifth its volume of pure hydrochloric acid. The urine is, how-
ever, not heated to boUing, but warmed to 50° or 60° and set aside for 12 hours
or preferably 24 hours. Metallic mercury is deposited on the foil as a bright lus-
trous mirror. The foil is then washed with pure water, alcohol, ether, and dried
without heat, rolled into a scroll, inserted into a glass tube and heated in the same
manner as under arsenic. The mercury is deposited in the metallic state in the
form of globules readily distinguished with the microscope.

2. Amalgamation Test. — A more rapid method than the above is by amalga-
mation with zinc. Add 5 grams of zinc dust to the urine and heat for 15 minutes,
stirring continuously. Allow the amalgamated zinc to settle and decant the urine.
Then wash by decantation several times with pure water, then with alcohol, and
finally with ether and dry in air. Now introduce the dry zinc into a narrow dry
glass tube sealed at one end. With the Bunsen soften the tube about 2 inches
above the zinc and constrict the tube by pulling the ends apart. Introduce a small
bit of glass wool or asbestos sufficient to support a small piece of iodine. Intro-
duce the iodine supported by the asbestos at the constriction. Apply heat to the
zinc amalgam, and then gently to the region holding the iodine to gently volatilize
it, and immediately reapply heat to the zinc. The mercury volatilizes and meeting
the iodine vapor unites with it, and is deposited as the red iodide of mercury.

CHOH

HOHC CHOH

INOSITOL, I I

HOHC CHOH

CHOH

URINE 451

Inositol occasionally occurs in the urine in albuminuria, diabetes
mellitus, and diabetes insipidus. It is claimed also that copious water-
drinking causes this substance to appear in the urine. Inositol was at
one time considered to be a sugar but is now known to be hexahy-
droxybenzene, as the above formula indicates. It is an example of a
non-carbohydrate in whose molecule the H and O are present in the
proportion to form water. In other words it has the formula of the
hexoses, i.e., C6H12O6. Inositol occurs widely distributed in the
vegetable kingdom, and because of this fact the theory has been voiced
that it represents one of the first stages in the conversion of a car-
bohydrate into the benzene ring. It is found in the liver, spleen,
lungs, brain, kidneys, suprarenal capsules, muscles, leucocytes, testes,
and urine under normal conditions.

Experiment

I. Detection of Inositol (Scherer). — Acidify the urine with concentrated nitric
acid and evaporate nearly to dryness. Add a few drops of ammonium hydroxide
and a little calcium chloride solution to the moist residue and evaporate the mixture
to dryness. In the presence of inositol (o.ooi gram) a bright red color is obtained.

For a more satisfactory test, which is also more time-consuming, see Salkowski's^
modification of Scherer's test.

LAIOSE

This substance is occasionally found in the urine in severe cases of
diabetes mellitus. By some investigators laiose is classed with the
sugars. It resembles fructose in that it has the property of reducing
certain metallic oxides and is levorotatory, but differs from fructose
in being amorphous, non-fermentable, and in not possessing a sweet
taste.

MELANINS

These pigments never occur normally in the urine, but are present
under certain pathological conditions, their presence being especially
associated with melanotic tumors. Ordinarily the freshly passed urine
is clear, but upon exposure to the air the color deepens and may at
last be very dark brown or black in color. The pigment is probably
present in the form of a chromogen or melanogcn and upon coming
into contact with the air oxidation occurs, causing the transforma-
tion of the melanogen into melanin and consequently the darkening
of the urine.

It is claimed that melanuria is proof of the formation of a visceral
' Salkowski: Zeit. physiol. chctit., 69, 478, 1910.

452 PHYSIOLOGICAL CHEMISTRY

melanotic growth. In many instances, wdthout doubt, urines rich in
indican have been wrongly taken as diagnostic proof of melanuria.
The pigment melanin is sometimes mistaken for indigo and melanogen
for indican. It is comparatively easy to differentiate between indigo
and melanin through the solubiUty of the former in chloroform.

In rare cases melanin is found in urinary sediment in the form of fine
amorphous granules.

Experiments

1. Ferric Chloride Reaction (von Jaksch-Pollak). — ^Add a few drops of
ferric chloride solution to lo c.c. of urine in a test-tube and note the formation of
a gray color. Upon the further addition of the chloride a dark precipitate forms,
consisting of phosphates and adhering melanin. An excess of ferric chloride
causes the precipitate to dissolve.

This is the most satisfactory test for the indentification of melanin in the
urine.

2. Bromine Test (Zeller). — To 50 c.c. of urine in a small beaker add an equal
volume of bromine water. In the presence of melanin a yellow precipitate will
form and will gradually darken in color, ultimately becoming black.

UROROSEIN

This is a pigment which is not present in normal urine but may
be detected in the urine in various diseases, such as pulmonary tuber-
culosis, typhoid fever, nephritis, and stomach disorders. Urorosein,
in common with various other pigments, does not occur preformed in
the urine, but is present in the form of a chromogen, which is trans-
formed into the pigment upon treatment with a mineral acid. Herter^
showed this chromogen to be indole acetic acid,

H
I
iCCCOOH

H

Normal urine responds to the urorosein reaction (see below) if nitrites
are present.

Experiments

I. Nitrite -Hydrochloric Acid Test (Urorosein Reaction). — To 10 c.c. of urine
in a test-tube add 2 c.c. of concentrated hydrochloric acid and a few drops of a
I per cent solution of potassiimi nitrite. A rose-red color indicates urorosein.

The chromogen (indole acetic acid) has been changed into urorosein
by oxidation.

1 Herter: Jour. Biol. Chem., 4, 253, 1908.

URINE 453

2. Robin's Reaction. — Acidify lo c.c. of urine with about 15 drops of con-
centrated hydrochloric acid. Upon allowing the acidified urine to stand, a rose-red
color will appear if urorosein is present.

3. Nencki and Sieber's Reaction. — To 100 c.c. of urine in a beaker add 10 c.c.
of 25 per cent sulphuric acid. Allow the acidified urine to stand and note the ap-
pearance of a rose-red color. The pigment may be separated by extraction with
amyl alcohol.

NEPHROROSEIN

This pigment is closely related to urorosein^ and like urorosein it is
produced from a chromogen when the urine is treated with nitric acid
or with concentrated hydrochloric acid and a Uttle sodium nitrite
solution. It is sometimes called /3-urorosein to differentiate it from the
true urorosein which is termed a-urorosein. Xephrorosein occurs only
in pathological urines.

UROCHROMOGEN

This is the chromogen of urochrome, the normal urinary pigment
(see Chapter XXI). It is claimed that the iirochromogen reaction of the
urine is an aid to prognosis and diagnosis of pulmonary tuberculosis.
Urochromogen is not present in normal urine. Its presence in patho-
logical urine is due probably to faulty oxidation, i.e., failure to oxi-
dize the chromogen to urochrome. Urochromogen ma}- be detected by
oxidizing it to urochrome by means of potassium permaganate. In
this process a certain antecedent of urochromogen is also oxidized
to urochrome. Whereas the diazo reaction (see page 454) is also
given by urines containing urochromogen, it is claimed that the diazo
reaction does not show the presence of the precursor of urochromogen.
Hence the urochromogen reaction is said to be more constant and uni-
form in its appearance.

Experiment

Urochromogen Reaction (Weisz).- — Fill a test-tube a little less than one-
third full of urine, dilute it with 2 volumes of distilled water and mix thoroughly.
Pour one-half the diluted urine into another tube and to one of the tubes add 3
drops of a I per cent solution of potassium permanganate. Shake the tube
thoroughly. In the presence of urochromogen a yellow tint will appear in the
tube to which permanganate was added.

The reaction is due to the oxidation of urochromogen to urochrome,
and is believed to be of value as an aid in prognosis and diagnosis of

' Arnold: Zeil. physiol. Chetn., 71.

-Weisz: Munch, med. Woch., 58, 1348, igii.

Vitri: Seviana Mcdica, 20, No. 28, 1913.

Hcflebower: Am. Jour. Med. Sci., 143, 221, 1912.

Metzger and Watson: Jour. Am. Med. Ass'n., 62, i8S6, 1914.

Pignacca: Gazeila d. Osp. e delle Clin., 25, 353, 191 4.

Ferrannini: Riforma med., 31, 479, 1915.

454 PHYSIOLOGICAL CHEMISTRY

pulmonary tuberculosis. The presence of sugar, albumin or urobilin
in low concentration does not interfere with the test. The test often
runs parallel with the diazo reaction (see below.) The test is supposed
to be positive when the focus of the lung is so active or extensive as to
flood the blood with toxins or to break down the defensive forces of the
body. It is claimed, therefore, that this test will differentiate the
cases in which the tuberculosis is beyond help from the tuberculin
from those in which the body is liable to respond favorably to its
action.^ Some investigators claim the test is not specific and that a
positive reaction will be obtained in many disorders other than
tuberculosis.^

UNKNOWN SUBSTANCES

I. Ehrlich's Diazo Reaction. — Place equal volumes of urine and Ehrlich's
diazobenzenesulphonic acid reagent^ in a test-tube, mix thoroughly by shaking,
and quickly add anmionium hydroxide in excess. The test is positive if both the
fluid and the foam assume a red color. If the tube is allowed to stand a precipi-
tate forms, the upper portion of which exhibits a blue, green, greenish-black, or
violet color. Normal urine gives a brownish-yellow reaction with the above
manipulation.

The exact nature of the substance or substances upon whose presence
in the urine this reaction depends is not well understood. Some in-
vestigators claim that a positive reaction indicates an abnormal de-
composition of protein material, whereas others assume it to be due
to an increased excretion of alloxyproteic acid, oxyproteic acid, or uro-
ferric acid. Weisz^ claims that urochromogen is the principal urinary
substance which causes a positive diazo reaction.

The reaction may be taken as a metabolic symptom of certain dis-
orders, which is of value diagnostically only when taken in connection
with the other symptoms. The reaction appears principally in the urine
in febrile disorders and in particular in the urine in typhoid fever,
tuberculosis, and measles. The reaction has also been obtained in the
urine in various other disorders such as carcinoma, chronic rheumatism,

1 M. and A. Weisz: Wien. klin. Woch., 25, 1183, 1912.
Dozzi: Gazetla d. Osp. e delle Clin., 34, 815, 1914.
Burgess: Jour. Am. Med. Ass'n., 66, 82, 1916.

'^Tuliato: Gazetta d. Osp. e delle Clin., 35, 1914.
Martelli and Pizzetti: Policlinico, 21, April i, 1914.

' Two separate solutions should be prepared and mixed in definite proportions when
needed for use:

(a) Five grams of sodium nitrite dissolved in i liter of distilled water.

ib) Five grams of sulphanilic acid and 50 c.c. of hydrochloric acid in i liter of distilled
water.

Solutions a and b should be preserved in well-stoppered vessels and mixed in the propor-
tion I : 50 when required, Green asserts that greater delicacy is secured by mixing the
solutions in the proportion i :ioo. The sodium nitrite deteriorates upon standing and
become? unfit for ufc in the course of a few weeks.

* Weisz: Miinch. mcd. Woch., 58, 1348, 1911.

URINE 455

diphtheria, erysipelas, pleurisy, pneumonia, scarlet [fever, syphilis,
typhus, etc. The administration of alcohol, chrysarobin, creosote,
cresol, dionin, guaiacol, heroin, morphine, naphthalene, opium, phenol,
tannic acid, etc., will also cause the urine to give a positive reaction.
The following chemical reactions take place in this test:

(a) NaNOo+HCl^HXOo + XaCl.

NH2 N

/ / %

(b) C6H4 +HNO>^C6H4 X+2H2O.

\ \ /

HSO3 SO3

Sulphanilic acid Diazo-benzenesulphonic acid.

2. MethyleneBlue Reaction (Russo).^ — To 5 c.c. of urine add 4 drops of a o.i per
cent solution of methylene blue. In cases of typhoid fever, measles, smallpox and
certain other disorders there will be a change in color from blue to green. In
normal urine the blue color persists. The test is sometimes used as a substitute
for the diazo reaction (see p. 454).

PHENOLSULPHONEPHTHALEIN TEST FOR KIDNEY

EFFICIENCY

This test for renal function was devised by Rowntree and Geraghty.^
It depends upon the injection into the tissues of a dyestuff which
is^eliminated rapidly by the normal kidneys, and can be easily estimated
quantitatively in the urine.

This dyestuff, phenolsulphonephthalein, is non-irritative to the
body either when taken by mouth or when injected into the tissues,^
so that it does no harm to an already weakened kidney.

The patient upon whom the test is to be performed is given 300-400
c.c. of water 20-30 minutes previously, in order to assure a free flow
of urine.

The procedure is as follows : One c.c. of a solution containing 6 mg. of phenol-
sulphonephthalein^ is injected intramuscularly in the lumbar region, the time of
injection being noted. The patient is then catheterized and the urine as it forms
thereafter allowed to drop into a beaker containing 2 drops of 25 per cent NaOH.
The appearance of a red color in the alkaUnized urine indicates beginning excre-
tion of the drug, the normal time being within 5 to 10 minutes after its injection.

1 Russo: Kiforma vied., Xo. ig, 1905.
Peskow: Semainc med., 103, 1912.
da Pozzo: Gaz. Osp. Clin., 35, 865, 1914.

^ Rowntree and Geraghty: Jour. Pliarm. and E.vper. Therap., i, 579, 1910: also Arch.
Int. Med., March, 191 2, p. 284.

'Abel and Rowntree: Jour. Pharm. and E.xpcr. Therap., i, 231, 1910.

* This solution is prepared by adding 0.6 gram phenolsulphonephthalein and 0.84 c.c.
of 2/N NaOH to enough 0.75 per cent NaCl solution to make 100 c.c. This gives the mono-
sodium or acid salt which is slightly irritant locally when injected. It is necessary to add
2-3 drops more 2/N XaOH which changes the color to a bordeau.x red. This_ prepara-
tion is non-irritant.

456 PHYSIOLOGICAL CHEMISTRY

Urine is now collected in one-hour samples. In patients with obstruction to the
flow of urine from the bladder the retention catheter is stoppered and the urine
drawn off at the end of each hour. Other patients may simply be allowed to urinate
at the hourly periods.

To each hour sample of urine is added 25 per cent NaOH, drop by drop, imtil
the mayimnm intensity of color appears. This color will remain constant for an
indefinite period of time. Each sample is then placed in a 1000 c.c. volvunetric
flask and diluted to the mark with distilled water.

Comparison is made in a Duboscq (Hellige or Sargent) colorimeter (see p. 486)
with a standard consisting of 3 mg. of phenolsulphonephthalein in 1000 c.c. of solu-
tion. The cylinder containing the standard may conveniently be placed at the 10
mm. mark. Since the volmne of each urine sample is the same as that of the
standard, the percentage elimination of phenolsulphonephthalein in each may be
easily calculated as follows :

Reading of Urine : Reading of Standard : : 100 : X.

The amount of the drug eliminated normally is 40-60 per cent during
the first hour and 20-25 per cent during the second hour, or a total of
60-85 P^r cent for two hours. The amount of the drug excreted has
been found to be independent of the quantity of urine obtained.
In case of delayed excretion the collection of hourly samples may be
continued until practically all of the drug has been recovered in the
urine.

If it is desired to test the function of each kidney separately,
ureteral catheterization must be resorted to, the experiment other-
wise being performed as above described.

The phenolsulphonephthalein test may be used to indicate the
amount of derangement in quantitative functional disturbance of the
kidneys, as in chronic interstitial and chronic parenchymatous neph-
ritis or uremia.

McLean^ has very recently suggested a method for studying kidney
function which is based upon the relationship between the urea con-
tent of the blood and the rate at which the urea is excreted by the
kidney. It gives similar values to the phenol-sulphonephthalein test.
It has an advantage in that it enables one to measure kidney function
by a study of an actual normal function of the organ, i.e., urea excre-
tion. The method, however, is more or less complex.

^McLean: Jour. Am. Med. Assn., 66., 415, 1916.

CHAPTER XXIV

URINE : ORGANIZED AND UNORGANIZED
SEDIMENTS

The data obtained from carefully conducted microscopical exami-
nations of the sediment of certain pathological urines are of very great
importance diagnostically. Too little emphasis is sometimes placed
upon the value of such findings.

The sedimentary constituents may be divided into two classes,
i.e., organized and unorganized. The sediment is ordinarily collected

Fig. 132. — The Purdy Electric Centripvge.

Fig. 133. — Sediment Tube FOR THE
PcTRDY Electric Centrifvge.

for examination by means of the centrifuge (Fig. 132). An older
method, and one still in vogue in some quarters, is the so-called gravity
method. This simply consists in placing the urine in a conical glass
and allowing the sediment to settle. The collection of the sediment by
means of the centrifuge, however, is much preferable, since the process
of sedimentation may be accomplished by the use of this instrument in a
few minutes, and far more perfectly, whereas when the other method is
used it is frequently necessary to allow the urine to remain in the con-

457

45^ PHYSIOLOGICAL CHEMISTRY

ical glass 12-24 hours before sufficient sediment can be secured for the
microscopical examination.

(a) Unorganized Sediments

Ammonium magnesium phosphate ("triple phosphate")-

Calcium oxalate.

Calcium carbonate.

Calcium phosphate.

Calcium sulphate.

Uric acid.

Urates.

Cystine.

Cholesterol.

Hippuric acid.

Leucine (?) and tyrosine.

Hematoidin and bilirubin.

Magnesium phosphate.

Indigo.

Xanthine.

Melanin.

Ammonium Magnesium Phosphate ("Triple Phosphate"). —
Crystals of "triple phosphate" are a characteristic constituent of the
sediment when alkaline fermentation of the urine has taken place
either before or after being voided. They may even be detected in
amphoteric or slightly acid urine provided the ammonium salts are
present in large enough quantity. This substance may occur in the
sediment in two forms, i.e., prisms and the feathery type. The pris-
matic form of crystals (Fig. 129, page 408) is the one most commonly
observed in the sediment; the feathery form (Fig. 129, page 408) pre-
dominates when the urine is made ammoniacal with ammonia.

The sediment of the urine in such disorders as are accompanied by
a retention of urine in the lower urinary tract contains "triple phos-
phate" crystals as a characteristic constituent. The crystals are fre-
quently abundant in the sediment during paraplegia, chronic cystitis,
enlarged prostate, and chronic pyelitis.

Calcium Oxalate. — Calcium oxalate is found in the urine in the
form of at least two distinct types of crystals, i.e., the dumb-bell type
and the octahedral type (Fig. 134, page 459). Either form may occur
in the sediment of neutral, alkaline, or acid urine, but both forms are
found most frequently in urine having an acid reaction. Occasionally,
in alkaline urine, the octahedral form is confounded with "triple phos-

URINE

459

phate" crystals. They may be differentiated from the phosphate
crystals by the fact that they are insoluble in acetic acid.

The presence of calcium oxalate in the urine is not of itself a sign of
any abnormality, since it is a constituent of normal urine. It is increased
above the normal, however, in such pathological conditions as diabetes

©

^

#

^

^

^

W^^ ^"

Fig. 134. — Calcium Oxalate. (Ogden.)

mellitus, in organic diseases of the liver, and in various other conditions
which are accompanied by a derangement of digestion or of the oxida-
tion mechanism, such as occurs in certain diseases of the heart and
lungs.

Calcium Carbonate. — Calcium carbonate crystals form a typical
constituent of the urine of herbivorous animals. They occur less fre-

FiG. 135. — Calcium Carbonate.

quently in human urine. The reaction of urine containing these
crystals is nearly always alkaline, although they may occur in ampho-
teric or in slightly acid urine. It generally crystallizes in the form
of granules, spherules, or dumb-bells (Fig. 135). The crystals of
calcium carbonate may be differentiated from calcium oxalate bv the

460 PHYSIOLOGICAL CHEMISTRY

fact that they dissolve in acetic acid with the evolution of carbon dioxide
gas.

Calcium Phosphate (Stellar Phosphate). — Calcium phosphate may-
occur in the urine in three forms, i.e., amorphous, granular, or crystal-
line. The crystals of calcium phosphate are ordinarily pointed, wedge-
shaped formations which may occur as individual crystals or grouped
together in more or less regularly formed rosettes (Fig. 105, page 322).
Acid sodium urate crystals (Fig. 137, page 462) are often mistaken for
crystals of calcium phosphate. We may differentiate between these
two crystalline forms by the fact that acetic acid will readily dissolve
the phosphate, whereas the urate is much less soluble and when finally
brought into solution and recrystallized one is frequently enabled to
identify uric acid crystals which have been formed from the acid urate
solution. The clinical significance of the occurrence of calcium phos-
phate crystals in the urinary sediment is similar to that of "triple
phosphate" (see page 458).

Calcium Sulphate. — Crystals of calcium sulphate are of quite rare
occurrence in the sediment of urine. Their presence seems to be
limited in general to urines which are of a decided acid reaction.
Ordinarily it crystallizes in the form of long, thin, colorless needles or
prisms (Fig. 128, page 405) which may be mistaken for calcium phos-
phate crystals. There need be no confusion in this respect, however,
since the sulphate crystals are insoluble in acetic acid, which reagent
readily dissolves the phosphate. As far as is known their occurrence
as a constituent of urinary sediment is of very little clinical significance.

Uric Acid. — Uric acid forms a very common constituent of the sedi-
ment of urines which are acid in reaction. It occurs in more varied
forms than any of the other crystalline sediments (Plate V, opposite
page 380, and Fig. 136), some of the more common varieties of crystals
being rhombic prisms, wedges, dumb-bells, whetstones, prismatic
rosettes, irregular or hexagonal plates, etc. Crystals of pure uric acid
are always colorless (Fig. 122, page 380), but the form occurring in
urinary sediments is impure and under the microscope appears pig-
mented, the depth of color varying from yellow to a dark reddish-
brown according to the size and form of the crystal.

The presence of a considerable uric acid sediment does not, of neces-
sity, indicate a pathological condition or a urine of increased uric acid
content, since this substance very often occurs as a sediment in urines
whose uric acid content is diminished from the normal merely as a re-
sult of changes in reaction, etc. Pathologically, uric acid sediments oc-
cur in gout, acute febrile conditions, chronic interstitial nephritis, etc.
If the microscopical examination is not conclusive, uric acid may be

"URINE

461

dififerentiated from other crystalline urinary sediments from the fact
that it is soluble in alkalis, alkali carbonates, boiling glycerol, concen-
trated sulphuric acid, and in certain organic bases such as ethylamine
and piperidin. It also responds to the murexide test (see page 380),
Schiflf's reaction (see page 381) and to Folin's phosphotungstic acid
reaction (see page 381).

Urates. — The urate sediment may consist of a mixture of the urates
of ammonium, calcium, magnesium, potassium, and sodium. The
ammonium urate may occur in neutral, alkaline, or acid urine, whereas
the other forms of urates are confined to the sediments of acid urines.
Sodium urate occurs in sediments more abundantly than the other

Fig. 136. — Various Forms of Uric Acid.

I, Rhombic plates; 2, whetstone forms; 3, 3, quadrate forms; 4, 5, prolonged into
points; 6, 8, rosettes; 7, pointed bundles; 9, barrel forms precipitated by adding hydro-
chloric acid to urine.

urates. There are two sodium urates, the mono and the di, which may

Na"'"\ _ Na'^X _

be expressed thus jj+ >C5H2N403 and j^^+ yCsHaNiOs . Both

salts dissociate with the production of an alkaline reaction, the alka-
linity being stronger in the case of the di-sodium urate. The so-called
quadriurate or hemiurate have no existence as chemical units. ^ The
urates of calcium, magnesium, and potassium are amorphous in
character, whereas the urate of ammonium is crystalline. Sodium
urate may be either amorphous or crystalline. When crystalline it
forms groups of fan-shaped clusters or colorless, prismatic needles (Fig.

* Taylor: Jour. Biol. Cliem., i, 177, 1905.

462

PHYSIOLOGICAL CHEMISTRY

137. Ammonium urate is ordinarily present in the sediment in the
burr-like form of the "thorn-apple" crystal, i.e., yellow or reddish-
brown spheres, covered with sharp spicules or prisms (Plate VI,
opposite). The urates are all soluble in hydrochloric acid or acetic
acid and their acid solutions yield crystals of uric acid upon standing.
They also respond to the murexide test. The clinical significance of

Fig. 137. — Acid Sodium Urate.

urate sediments is very similar to that of uric acid. A considerable
sediment of amorphous urates does not necessarily indicate a high uric
acid content, but ordinarily signifies a concentrated urine having a very
strong acidity.

Cystine. — Cystine is one of the rarer of the crystalline urinary sedi-
ments. It has been claimed that it occurs more often in the urine of

0

#

/

Fig. 138. — Cystine. (Ogden.)

men than of women. Cystine crystallizes in the form of thin, color-
less, hexagonal plates (Fig. 26, page 76, and Fig. 138) which are
insoluble in water, alcohol, and acetic acid, and soluble in minerals,
acids, alkalis, and especially in ammonia. Cystine may be identified
by burning it upon platinum foil, under which condition it does not

PLATE VI.

Ammonium Urates, showing Spherules and Thorx-apple-shaped Crystals.
(From Ogden, after Pcycr.)

URINE 463

melt but yields a bluish-green flame. For preparation of Cystine see
Chapter IV.

Cholesterol. — Cholesterol crystals have been but rarely detected in
urinary sediments. When present they probably arise from a patho-
logical condition of some portion of the urinary tract. Crystals of
cholesterol have been found in the sediment in cystitis, pyelitis,
chyluria, and nephritis. Ordinarily it crystallizes in large regular and
irregular colorless, transparent plates, some of which possess notched
corners (Fig. 57, page 210). Frequently, instead of occurring in the
sediment, it is found in the form of a film on the surface of the urine.

Hippuric Acid. — This is one of the rare sediments of human urine.
It deposits under conditions similar to those which govern the formation
of uric acid sediments. The crystals,
which are colorless needles or prisms
(Fig. 125, page 389) when pure, are in-
variably pigmented in a manner similar
to the uric acid crystals when observed
in urinary sediment and because of this

fact are frequently confounded with the \ff^ .^jfa^

rarer forms of uric acid. Hippuric acid ^© ^Qf

may be differentiated from uric acid ^

from the fact that it does not respond to Fig. 139.— Crystals of Impure

Leucixe. (Ogden.)
the murexide test and is much more

soluble in water and in ether. The detection of crystals of hippuric
acid in the urine has very little chnical significance, since its pres-
ence in the sediment depends in most instances very greatly upon
the nature of the diet. It is particularly prone to occur in the sedi-
ment after the ingestion of certain fruits as well as after the ingestion of
benzoic acid (see pages 388 and 585).

Leucine and Tyrosine. — ^Leucine and tyrosine have frequently
been detected in the urine, either in solution or as a sediment. Neither
of them occurs in the urine ordinarily except in association with the
other, i.e., whenever leucine is detected it is more than probable that
tyrosine accompanies it. They have been found pathologically in
the urine in acute yellow atrophy of the liver, in acute phosphorus
poisoning, in cirrhosis of the liver, in severe cases of typhoid fever
and small-pox, and in leukemia. In urinary sediments leucine ordi-
narily crystallizes in characteristic spherical masses which show both
radial and concentric striations and are highly refractive (Fig. 139).
Some investigators claim that these crystals which are ordinarily called
leucine are, in reality, generally urates. This view point has become
more general in recent years. For the crystalline form of pure leucine

464 PHYSIOLOGICAL CHEMISTRY

obtained as a decomposition product of protein see Fig. 28, page 80.
Tyrosine crystallizes in urdinary sediments in the well-known sheaf
or tuft formation (Fig. 25, page 76). For other tests on leucine and
tyrosine see pages 86 and 87.

Hematoidin and Bilirubin. — There are divergent opinions regard-
ing the occurrence of these bodies in urinary sediment. Each of them
crystallizes in the form of tufts of small needles or in the form of small
plates which are ordinarily yellowish-red in color (Fig. 56, page 205).
Because the of fact that the crystalline form of the two substances is
identical many investigators claim them to be one and the same body.
Other investigators claim, that while the crystalline form is the same
in each case, there are certain chemical differences which may be brought
out very strikingly by properly testing. For instance, it has been
claimed that hematoidin may be differentiated from bilirubin through
the fact that it gives a momentary color reaction (blue) when nitric acid
is brought into contact with it, and, further, that it is not dissolved on
treatment with ether or potassium hydroxide. Pathologically, typical
crystals of hematoidin or bilirubin have been found in the urinary
sediment in jaundice, acute yellow atrophy of the liver, carcinoma of
the liver, cirrhosis of the liver, and in phosphorus poisoning, typhoid
tever, and scarlatina.

Magnesium Phosphate. — Magnesium phosphate crystals occur
rather infrequently in the sediment of urine which is neutral, alkaline,
or feebly acid in reaction. It ordinarily crystallizes in elongated,
highly refractive, rhombic plates which are soluble in acetic acid.

Indigo. — Indigo crystals are frequently found in urine which has
undergone alkaline fermentation. They result from the breaking
down of indoxyl-sulphates or indoxyl-glycuronates. Ordinarily indigo
deposits as dark blue stellate needles or occurs as amorphous particles
or broken fragments. These crystalline or amorphous forms may occur
in the sediment or may form a blue film on the surface of the urine.
Indigo crystals generally occur in urine which is alkaline in reaction,
but they have been detected in acid urine.

Xanthine. — Xanthine is a constituent of normal urine but is found
in the sediment in crystalline form very infrequently, and then only in
pathological urine. When present in the sediment xanthine generally
occurs in the form of whetstone-shaped crystals somewhat similar in
form to the whetstone variety of uric acid crystal. They may be dif-
ferentiated from uric acid by the great ease with which they may be
brought into solution in dilute ammonia and on applying heat. Xan-
thine may also form urinary calculi. The clinical significance of
xanthine in urinarv sediment is not well understood.

URIISTE 465

Melanin. — Melanin is an extremely rare constituent of urinary
sediments. Ordinarily in melanuria the melanin remains in solution;
if it separates it is generally held in suspension as fine amorphous
granules.

(b) Organized Sediments

Epithelial cells.

Pus cells.

Hyaline.

Granular.

Epithelial.

Casts. ^ Blood.
Fatty.
Waxy.
. Pus.

Cyhndroids. '. ' '

Erythrocytes.

Spermatozoa.

Urethral filaments.

Tissue debris.

Animal parasites.

Micro-organisms.

Fibrin.

Foreign substances due to contamination.

Epithelial Cells. — The detection of a certain number of these cells
in urinary sediment is not, of itself, a pathological sign, since they
occur in normal urine. However, in certain pathological conditions
they are greatly increased in number, and since different areas of the
urinary tract are lined with different forms of epithelial cells, it becomes
necessary, when examining urinary sediments, to note not only the
relative number of such cells, but at the same time to carefully observe
the shape of the various individuals in order to determine, as far as
possible, from what portion of the tract they have been derived. Since
the different layers of the epithelial lining are composed of cells dif-
ferent in form from those of the associated layers, it is evident that a
careful microscopical examination of these cells may tell us the par-
ticular layer which is being desquamated. It is frequently a most diffi-
cult undertaking, however, to make a clear differentiation between the
various forms of epithelial cells present in the sediment. If skilfully
done, such a microscopical differentiation may prove to be of very
great diagnostic aid.

The principal forms of epithelial cells met with in urinary sediments
are shown in Fig. 140, page 466.

466

PHYSIOLOGICAL CHEMISTRY

Pus Cells.- — Pus corpuscles or leucocytes are present in extremely
small numbers in normal urine. Any considerable increase in the
number, however, ordinarily denotes a pathological condition, gener-
ally an acute or chronic inflammatory condition of some portion of the
urinary tract. The sudden appearance of a large amount of pus in a
sediment denotes the opening of an abscess into the urinary tract. Other
form elements, such as epithelial cells, casts, etc., ordinarily accompany
pus corpuscles in urinary sediment and a careful examination of these
associated elements is necessary in order to form a correct diagnosis as
to the origin of the pus. Protein is always present in urine which
contains pus.

Fig. 140. — Epithelium from Different Areas of the Urinary Tract.

a, Leucocyte (for comparison); b, renal cells; c, superficial pelvic cells; d, deep pelvic
cells; e, cells from calices; /, cells from ureter; g, g, g, g, g, squamous epithelium from the
bladder; h, h, neck-of-bladder cells; i, epithelium from prostatic urethra; k, urethral cells;
/, /, scaly epithelium; m, m', cells from seminal passages; n, compound granule cells; 0,
fatty renal cell. (Ogden.)

The appearance which pus corpuscles exhibit under the microscope
depends greatly upon the reaction of the urine containing them. In
acid urine they generally present the appearance of round, colorless cells
composed of refractive, granular protoplasm, and may frequently exhibit
ameboid movements, especially if the slide containing them be warmed
slightly. They are nucleated (one or more nuclei), the nuclei being
clearly visible only upon treating the cells with water, acetic acid, or
some other suitable reagent. In urine which has a decided alkaline
reaction, on the other hand, the pus corpuscles are often greatly de-
generated. They may be seen as swollen, transparent cells, which
exhibit no granular structure and as the process of degeneration con-

URIXE.

467

tinues the cell outline ceases to be visible, the nuclei fade, and finally
only a mass of debris containing isolated nuclei and an occasional
cell remains.

It is frequently rather difficult to make a differentiation between pus
corpuscles and certain types of epithelial cells which are similar in form.
Such confusion may be avoided by the addition of iodine solution (I in
KI), a reagent which stains the pus corpuscles a deep mahogany-brown
and transmits to the epithelial cells a light yellow tint. The test pro-
posed by Vitali often gives very satisfactory results. This simply
consists in acidifying the urine fif alkaline) with acetic acid, then filter-
ing, and treating the sediment on the filter paper with freshly prepared
tincture of guaiac. The presence of pus in the sediment is indicated

Fig. 141. — Pus Corpuscles. (After Ullzmann.)

I, Normal; 2, showing amoeboid movements; 3, nuclei rendered distinct by acetic acid; 4,
as observed in chronic pyelitis; 5, swollen by ammonium carbonate.

if a blue color is observed. Large numbers of pus corpuscles are present
in the urinary sediment in gonorrhoea, leucorrhcra, chronic pyelitis,
and in abscess of the kidney. In addition to the usual constituents
found in leucocytes Mandel and Levene^ claim that pus cells contain
glucolhionic acid. See Pus tests, page 431.

Casts. — These are cylindrical formations, which originate in the
uriniferous tubules and are forced out by the pressure of the urine.
They vary greatly in size, but in nearly every instance they possess
parallel sides and rounded ends. The finding of casts in the urine is
very important because of the fact that they generally indicate some
kidney disorder; if albumin accompanies the casts the indication is

' Mandel and Levene: Biochemischc Zeitschrift, 4, jH, 1007.

468

PHYSIOLOGICAL CHEMISTRY

much accentuated. Casts have been classified according to their
microscopical characteristics as follows: (a) hyaline, {b) granular, (c)
epithelial, (d) blood, {e) fatty, (/) waxy, (g) pus.

(fl) Hyaline Casts. — These are composed of a basic material which
is transparent, homogeneous, and very light in color (Fig. 142).
In fact, chiefly because of these physical properties, they are the
most difl&cult form of renal casts to detect under the microscope.
Frequently such casts are impregnated with deposits of various forms,
such as erythrocytes, epithelial cells, fat globules, etc., thus rendering
the form of the cast more plainly visible. Staining is often resorted to

Fig. 142. — Hyaline Casts.
One cast is impregnated with four renal cells.

in order to render the shape and character of the cast more easily
determined. Ordinary iodine solution (I in KI) may be used in this
connection; many of the aniline dyes are also in common use for this
purpose, e.g., gentian- violet, Bismarck-brown, methylene-blue, fuchsin,
and eosin. Generally, but not always, albumin is present in urine
containing hyaline casts. Hyaline casts are common to all kidney
disorders, but occur particularly in the earliest and recovering stages
of parenchymatous nephritis and interstitial nephritis.

{b) Granular Casts. — The common hyaline material is ordinarily the
basic substance of this form of cast. The granular material generally
consists of albumin, epitheial cells, fat, or disintegrated erythrocytes or

URIXE

469

leucocytes, the character of the cast varjdng according to the nature
and size of the granules (Fig. 143, and Fig. 144, page 470J. Thus
we have casts of this general type classified as finely granular and
coarsely granular casts. Granular casts, and in particular the finely
granular types, occur in the sediment in practically every kidney dis-
order but are probably especially characteristic of the sediment in in-
flammatory disorders.

{c) Epithelial Casts. — These are casts bearing upon their surface
epithelial cells from the lining of the uriniferous tubules (Fig. 145,
page 470). The basic material of this form of cast may be hyaline or

Fig. 143. — Granular Casts. (After Peyer.)

granular in nature. Epithelial casts are particularly abundant in the
urinary sediment in acute nephritis.

(d) Blood Casts. — Casts of this type may consist of erythrocytes
borne upon a hyaline or a fibrinous basis (Fig. 146, page 470). The
occurrence of such casts in the urinary sediment denotes renal hemor-
rhage and they are considered to be especially characteristic of acute
diffuse nephritis and acute congestion of the kidney.

(e) Fatty Casts. — Fatty casts may be formed by the deposition of
fat globules or crystals of fatty acid upon the surface of a hyaline or
granular cast (Fig. 147, page 471). In order to constitute a true fatty
cast the deposited material must cover the greater part of the surface
area of the cast. The presence of fatty casts in urinary sediment in-

470

PHYSIOLOGICAL CHEMISTRY

dicatesjatty degeneration of the kidney; such casts are particularly
characteristic of subacute and chronic inflammation of the kidney.

Fig. 144. — Granular Casts.
a Finely granular; b, coarsely granular.

Fig. 145. — Epithell^l Casts.

(/) Waxy Casts. — These casts possess a basic substance similar to
that-which enters into the foundation of the hvaline form of cast. In

Fig. 146. — Blood, Pus, Hyaline and Epithellil Casts.
a, Blood casts; b, pus cast; c, hyaline cast impregnated with renal cells; d, epithelial casts.

common with the hyaline type they are colorless, refractive bodies,
but diflfer from this form of cast in being, in general, of greater length
and diameter and possessing sharper outlines and a light yellow color

URINE

471

Fig. 147. — Fatty Casts. {Aitei Peyer.)

Fig. 148. — Fatty and Waxy Casts.
a, Fatty casts; b, waxy casts.

472

PHYSIOLOGICAL CHEMISTRY

(Fig. 148, page 471). Such casts occur in several forms of nephritis,
but do not appear to characterize any particular type of the disorder
except amyloid disease, in which they are rather common.

(g) Pus Casts. — Casts whose surface is covered with pus cells or
leucocytes are termed pus casts (Fig. 146, p. 470). They are frequently
mistaken for epithehal casts. The differentiation between these two
types is made very simple, however, by treating the cast with acetic
acid which causes the nuclei of the leucocytes to become plainly visible.
The true pus cast is quite rare and indicates renal suppuration.

Cylindroids. — These formations may occur in normal or pathological
urine and have no particular clinical significance. They are frequently

Fig. 149. — CvLiNDRorDS. {Mter Peyer.)

mistaken for true casts, especially the hyaline type, but they are
ordinarily flat in structure with a rather smaller diameter than casts,
may possess forked or branching ends, and are not composed of homo-
geneous material as are the hyaline casts. Such ''false casts" may
become coated with urates, in which event they appear granular in
structure. The basic substance of cylindroids is often the nucleo-
protein of the urine (Fig. 149, above).

Erythrocytes. — These form elements are present in the urinary
sediment in various diseases. They appear as the normal biconcave,
yellow erythrocyte (Plate IV, opposite page 249) or may exhibit certain
modifications in form, such as the crenated type (Fig. 150)
which is often seen in concentrated urine. Under different condi-

URINE

473

tions they may become swollen sufl&ciently to entirely erase the bi-
concave appearance and may even occur in the form of colorless spheres
having a smaller diameter than the original disc-shaped corpuscles.
Erythrocytes are found in urinary sediment in hemorrhage of the
kidney or of the urinary tract, in traumatic hemorrhage, hemorrhage
from congestion, and in hemorrhagic diathesis.

Spermatozoa. — Spermatozoa may be detected in the urinary sedi-
ment in diseases of the genital organs, as well as after coitus, nocturnal
emissions, epileptic, and other convulsive attacks, and sometimes in
severe febrile disorders, especially in typhoid fever. In form they con-
sist of an oval body, to which is attached a long, delicate tail (Fig.

Fig. 150. — Crenated Erythrocytes.

151, page 474). Upon examination they may show motility or may be
motionless.

Urethral Filaments. — These are peculiar thread-like bodies which
are sometimes found in urinary sediment. They may occasionally be
detected in normal urine and pathologically are found in the sediment in
acute and chronic gonnorrhcea and in urethrorrhcea. The ground-sub-
stance of these urethral filaments is, in part at least, similar to that of the
cylindroids (see page 47 2) . The urine first voided in the morning is best
adapted for the examination for filaments. These filaments may ordi-
narily be removed by a pipette since they are generally macroscopic.

Tissue Debris. — Masses of cells or fragments of tissue are frequently
found in the urinary sediment. They may be found in the sediment in
tubercular affections of the kidney and urinary tract or in tumors of
these organs. Ordinarily it is necessary to make a histological ex-

474

PHYSIOLOGICAL CHEMISTRY

amination of such tissue fragments before coining to a final decision as
to their origin.

Animal Parasites. — The cysts, hooklets, and membrane shreds
of echinococci are sometimes found in the urinary sediments. Other
animal organisms which are more rarely met with in the urine are em-
bryos of the Filaria sanguinis and eggs of the Distoma hematohinm and
Ascarides. Animal parasites in general occur most frequently in the
urine in tropical countries.

Micro-organisms. — Bacteria as well as yeasts and moulds are fre-
quently detected in the urine. Both the pathogenic and non-patho-
genic forms of bacteria may occur. The non-pathogenic forms most
frequently observed are micrococcus urecB, bacillus urecB, and staphylo-
coccus urece liquefaciens. Of the pathogenic forms many have been

Fig. 151. — Human Spermatozoa.

observed, e.g., Bacterium Coli, typhoid bacillus, tubercle bacillus, gono-
coccus, bacillus pyocyaneus, and proteus vulgaris. Yeast and moulds
are most frequently met with in diabetic urine.

Fibrin. — Following hematuria, fibrin clots are occasionally ob-
served in the urinary sediment. They are generally of a semi-gelatin-
ous consistency and of a very light color, and when examined under
the microscope they are seen to be composed of bundles of highly re-
fractive fibers which run parallel.

Foreign Substances Due to Contamination.^ — Such foreign sub-
stances as fibers of silk, linen, or wool; starch granules, hair, fat, and
sputum, as well as muscle fibers, vegetable cells, and food particles, are
often found in the urine. Care should be taken that these foreign
substances are not mistaken for any of the true sedimentary con-
stituents already mentioned.

CHAPTER XXV
URINE: CALCULI

Urinary calculi, also called concretions, or concrements are solid
masses of urinary sediment formed in some part of the urinary tract.
They vary in shape and size according to their location, the smaller
calculi, termed sand or gravel, in general arising from the kidney or the
pelvic portion of the kidney, whereas the large calculi are ordinarily
formed in the bladder. There are two general classes of calculi as
regards composition, i.e., simple and compound. The simple form is
made up of but a single constituent, whereas the compound type con-
tains two or more individual constituents. The structural plan of
most calculi consists of an arrangement of concentric rings about a
central nucleus, the number of rings frequently being dependent upon
the number of individual constituents which enter into the structure
of the calculus. However, layers quite different in macroscopical
appearance may be almost identical in composition. In case two or
more calculi unite to form a single calculus the resultant body %vill
obviously contain as many nuclei as there were individual calculi
concerned in its construction. Under certain conditions the growth of
a calculus will be principally in only one direction, thus preventing
the nucleus from maintaining a central location. The qualitative
composition of urinary calculi is dependent, in great part, upon the
reaction of the urine, e.g., if the reaction of the urine is acid the calculi
present will be composed, in great part at least, of substances that are
capable of depositing in acid urine, e.g., uric acid, urates and calcium
oxalates.

According to Ultzmann, out of 545 cases of urinary calculus, uric
acid and urates formed the nucleus in about 81 per cent of the cases;
earthy phosphates in about 9 per cent; calcium oxalate in about 6 per
cent; cystine in something over i per cent, while in about 3 per cent
of the cases some foreign body comprised the nucleus.

More recent analyses^ of twenty-four calculi showed the nucleus in
75 per cent of them to be calcium oxalate (60 per cent) and in 25 per
cent to be phosphate (56 per cent). All of the calculi contained some
uric acid and urates, but only three gave more than 10 per cent.

^ Kahn and Roscnbloom: J our. Am. Med. Ass'n, 59, 2252, 1913.

475

476 PHYSIOLOGICAL CHEMISTRY

In the chemical examination of urinary calculi the most valuable
data are obtained by subjecting each of the concentric layers of the
calculus to a separate analysis. Material for examination may be
conveniently obtained by sawing the calculus carefully through the
nucleus, then separating the various layers, or by scraping off from
each layer (without separating the layers) enough powder to conduct
the examination as outlined in the scheme (see page 477).

Varieties of Calculus

Uric Acid and Urate Calculi. — Uric acid and urates constitute the
nuclei of a large proportion of urinary concretions. Such stones are
always colored, the tint varying from a pale yellow to a brownish-red.
The surface of such calculi is generally smooth but it may be rough
and uneven.

Phosphatic Calculi.— Ordinarily these concretions consist prin-
cipally of "triple phosphate" and other phosphates of the alkaline
earths, with very frequent admixtures of urates and oxalates. The
surface of such calculi is generally rough but may occasionally be rather
smooth. The calculi are somewhat variable in color, exhibiting gray,
white, or yellow tints under different conditions. When composed of
earthy phosphates the calculi are characterized by their friability.

Calcium Oxalate Calculi.— This is the hardest form of calculus
to deal with, and is rather difficult to crush. They ordinarily occur
in two general forms, i.e., the small, smooth concretion which is char-
acterized as the hemp-seed calculus, and the medium-sized or large stone
possessing an extremely uneven surface, which is generally classed as
a mulberry calculus. This roughened surface of the latter form of
calculus is due, in many instances, to protruding calcium oxalate
crystals of the octahedral type.

Calcium Carbonate Calculi.^ — Calcium carbonate concretions are
quite common in herbivorous animals, but of exceedingly rare occur-
rence in man. They are generally small, white, or grayish calculi,
spherical in form and possess a hard, smooth surface.

Cystine Calculi. — The cystine calculus is a rare variety of calculus.
Ordinarily they occur as small, smooth, oval, or cylindrical concretions
which are white or yellow in color and of a rather soft consistency.

Xanthine Calculi. — This form of calculus is somewhat more rare
than the cystine type. The color may vary from white to brownish-
yellow. Very often uric acid and urates are associated with xanthine
in this type of calculus. Upon rubbing a xanthine calculus it has the
property of assuming a wax-like appearance.

URINE

477

On Heating the Powder on Platinum Foil, It

Does not burn

The powder when treated with HCI

Does not effervesce

The powder gently heated,
then treated with HCI

The powder when moist-
ened with a little KOH

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478 PHYSIOLOGICAL CHEMISTRY

Urostealith Calculi. — This form of calculus is extremely rare.
Such concretions are composed principally of fat and fatty acid. When
moist they are soft and elastic, but when dried they become brittle.
Urostealiths are generally light in color.

Fibrin Calculi. — Fibrin calculi are produced in the process of blood
coagulation within the urinary tract. They frequently occur as nuclei
of other forms of calculus. They are rarely found.

Cholesterol Calculi. — An extremely rare form of calculus somewhat
resembling the cystine type.

Indigo Calculi. — Indigo calculi are extremely rare, only two cases
having been reported. One of these indigo calculi is on exhibition in
the museum of Jefferson Medical College of Philadelphia.

The scheme, proposed by Heller and given on page 477, will be
found of much assistance in the chemical examination of urinary calculi.

CHAPTER XXVI

URINE : QUANTITATIVE ANALYSIS

In analyzing a normal or pathological urine quantitatively for
any of its constituents it is particularly necessary that the complete
and exact 24-hour sample be obtained. For directions with regard to
the collection and preservation of urine for analysis see Chapter
XXI on General Characteristics of Normal and Pathological Urine.
Methods for the determination of the specific gravity of the urine are
also there described. Before any urine is taken for analysis its total
volume should be measured, using a large graduated cylinder, and this
volume is thereafter taken as a basis for the calculations of the daily
output of the individual constituents determined. If the urine be
pathological it is of course necessary to precede its quantitative
analysis by qualitative tests for the pathological constituents.

Acidity by Titration

Folin's Method. — Principle: — The urine is titrated with standard
sodium hydroxide solution, using phenolphthalein as an indicator.
Potassium oxalate is added to precipitate the calcium which would
otherwise interfere with the end-point due to the precipitation of calcium
phosphate on neutralization of the urine. The acidity of the urine as
determined in this way is not a correct measure of the true acidity, which
is dependent upon the concentration of hydrogen ions. The results
obtained do, however, ordinarily show a certain parallelism with the
hydrogen ion concentration and are of value for comparative purposes.

Procedure. — Place 25 c.c. of urine in a 200 c.c. Erlenmeyer flask and add
15-20 grams of finely pulverized potassium oxalate and 1-2 drops of a i per cent
phenolphthalein solution to the fluid. Shake the mixture vigorously for 1-2
minutes and titrate it immediately with N 10 sodiimi hydroxide until a faint but
unmistakable pink remains permanent on further shaking. Take the burette
reading and calculate the acidity of the urine under examination.

Calculation. - If y represents the number of cubic centimeters of N 10 sodium
hydroxide used and y' represents the volume of urine excreted in 24 hours, the
total acidity of the 24-hour urine specimen may be calculated by means of the
following proportion :

479

480 PHYSIOLOGICAL CHEMISTRY

25 : y : : y' : X (acidity of 24-hour urine expressed in cubic centimeters of N/io

sodium hydroxide).

Each cubic centimeter of N/io sodium hydroxide contains 0.004 gram of
sodium hydroxide, and this is equivalent to 0.0063 gram of oxaUc acid. There-
fore, in order to express the total acidity of the 24-hour urine specimen in equiva-
lent grams of sodium hydroxide, multiply the value of x, as just determined,
by 0.004, or multiply the value of x by 0.0063 if it is desired to express the total
acidity in grams of oxaUc acid.

Interpretation. — (Under the heading ''Interpretation^^ there will
be found, in connection with the various quantitative methods which
follow, brief notes as to the possible significance of the results ob-
tained. For some further points (and reference to literature) see the
chapters on the Normal and Pathological Constituents of Urine and
on Metabolism. Consult text-books on physiological chemistry and
clinical diagnosis for complete discussion). The acidity of the urine
expressed in cubic centimeters N/io alkali required to neutralize the
24-hour output varies ordinarily from 200 to 500 under normal con-
ditions with an average of perhaps 350. It is dependent almost
entirely upon the diet, being low on a vegetable (base-forming diet)
and high on a diet containing much meat, rice, whole wheat products,
fruits containing benzoic acid, as prunes and cranberries, etc. (acid-
forming foods). On the administration of 15 grams of sodium bicar-
bonate it may go down to 100; the ingestion of much acid-forming
food may increase it to 600. In fasting it may rise in a few days to
800. It must be borne in hiind that acidities of less than 250 usually
indicate a true alkalinity of the urine inasmuch as phenolphthalein
changes in an alkaline solution. Samples of urine collected shortly
after a meal may be alkaline due to the so-called ''alkaline tide."

Bacterial decomposition of the urea of the urine occurring in the
urinary tract will increase the amount of ammonia and decrease the
acidity of the urine. The same change usually occurs in urine left in
contact with the air. The acidity of the urine is increased in acidosis,
cardio-renal and certain other disorders. The acidity of the urine
may be somewhat increased by administration of mineral acids, acid
phosphates, or benzoates, but it is much more difficult to increase than
to decrease this acidity.

Hydrogen Ion Concentration or True Acidity

Indicator Method (Henderson and Palmer's Adaptation of Soren-
sen's Method). ^^ — Principle. — The reaction of the urine is estimated

' Henderson and Palmer: Tour. Biol. Chent., 13, 393, 1913.

URINE 481

by matching the colors produced when a few drops of indicator are added
respectively to the diluted urine and to standard solutions of known
reaction similarly diluted. Similar hydrogen ion concentrations
are indicated by similar colors. The indicator must be properly
chosen.

Standard Solutions. — A series of standard solutions of known hy-
drogen ion concentration must be prepared. The solutions as indi-
cated in Table I (page 482) are satisfactory for urine analysis. The
table also indicates the H ion concentration of each solution, the figure
given being the logarithm of this concentration (Ph+). It is more
convenient and rational to express the concentration by this logarithmic
notation. True H ion concentrations corresponding to the logarithmic
figures are given in Table II (page 482).

The 13 solutions indicated are made up by mixing equal volumes
of their ingredient solutions of the composition indicated. Solutions
4 to 12 are all that are ordinarily required as the normal urinary H
ion concentrations lie between 4.80 and 7.50 and pathological variations
are usually within these limits. The mean normal value is almost
exactly 6.00.

Procedure. — Select eleven 250 c.c. flasks of good glass and indistinguishable
in color and form. Into each of ten of these introduce 10 c.c. of the various stand-
ard solutions. Make up to 250 c.c. with distilled water and add to each exactly the
same amount of an aqueous solution of sodiimi alizarine sulphonate (10-15 drops).
Mix well by inverting. Introduce 10 c.c. of the urine to be tested into a similar
250 c.c, flask, dilute and add indicator in exactly the same way as before. Match
the color of the diluted urine solution with one of the standard solutions. By
consulting Table 11 (page 482) determine to what H ion concentration this corre-
sponds. This table points out the indicators to be used for different ranges of
acidity. From 5.3-6.7 /j-nitrophenol is satisfactory and is used in the same way
as aUzarin except that it must be present in concentration of 0.08 per cent.
Neutral red is used in the same way for acidities from 6.7-7.5 about 1.5 c.c. of
the I per cent solution being required. For acidities greater than 5.5 methyl red
is used in the following way : 10 c.c. portions of the standard solutions are intro-
duced into carefully selected colorless test-tubes and 10 c.c. of urine is introduced
into another tube. The standard solutions are then colored to match the urine
by the addition of small amounts of />-nitrophenol, methyl orange, aUzarine or
bismark brown. Then to standard solutions and urine add 0.15 c.c. of a satu-
rated solution in 50 per cent alcohol, of methyl red and match the colors. For
concentrations of 7.5-9.27 or less undiluted urine is matched in test-tubes against
undiluted standard solutions, using phenolphthalein as an indicator (without
previous coloration of standard solution >. In all cases estimations are made in
duplicate.

31

482

PHYSIOLOGICAL CHEMISTRY

TABLE I

S'o.

XaH^PO,

Xa2HP04

^H +

Indicate

r

I

o.iooo X

9.27 "

2

o.oooi X

0 . 0480 N

8.7

Phenolphthalein

3

o.oooi X

0.0120 X

8.0

]

4

5

0.0166 X
o.ooio X

0.0833 ^
0 . 0060 N

7.48
7.38

• Xeutral red \

6

o.ooio X
CH3COOH

0.0023 N
CH3COOX

6.90

a

'

7

0.0009 N

0.0920 X

6.70

Sodium alizarine

8

0.0023 X

0.0920 X

6.30

sujphonate.

9

0 . 0046 X

0.0920 X

6.00

10

0.0092 X

0.0920 X

S-70

^Xitrophenol

II

0.0230 X

0.0920 X

530

] , , ,

12

0 . 0460 X

0.0920 X

4.90

\ Methyl red

13

0.0920 X

0.0920 X

4-70.

TABLE II

Log

+

H

Log

+
H

4.6

25oXio~'

6.4

4.0 XlO-7

4.8

i6oXio~^

6.6

2.S XlO-7

5-0

looXio"^

6.8

1.6 Xio-^

5-2

63X10-7

7.0

i.o Xio-^

5-4

40X10 7

7.2

0.63x10-7

5-6

25X10-7

7-4

0.40x10-7

5-8

16 X 10-7

7.6

0.25x10-7

6.0

10X10-'

7.8

O.I6XIO-7

6.2

6.3X10-7

8.0

O.IoXlO-7

Inter pr elation. — The H ion concentration of the urine is influenced
by the same factors as the titratable acidity (^see page 480). The
normal values lie between 4.80 and 7.50 with a mean value of almost
exactly 6.00. For vegetarians the mean value is about 6.64. In
cardio-renal disorders the mean is 5.3. In most pathological conditions
the hvdrogen ion concentration is increased.

Total Solids

1. Drying Method. — Place 5 c.c. of urine in a weighed shallow dish, acidify
very slightly with acetic acid (1-3 drops), and dry it in vacuo in the presence of sul-
phuric acid to constant weight. Calculate the percentage of solids in the urine
sample and the total solids for the 24-hour period.

Interpretation. — The average excretion of total solids by a normal adult man is
about 70 grams. It is largely dependent upon the protein and salts of the diet.
It may be decreased in severe nephritis due to impaired excretion, and greatly in-
creased in diabetes with high sugar elimination.

Practically all the methods the technic of which includes evaporation at an
increased temperature, either under atmospheric conditions or in vacuo, are attended
with error.

Shackell's method* which entails the vacuum desiccation of the frozen sample
is extremely satisfactory and should be used in all biological work where the great-
est accuracy is desired.

1 Shackell: American Journal of Physiology, 24, 325, 1909

URINE 483

2. Calcxilation by Long's Coefficient. — The quantity of solid material contained
in the urine excreted for any 24-hour period may be approximately computed by
multiplying the second and third decimal figures of the specific gravity by 2.6.
This gives us the number of grams of solid matter in i liter of urine. From this value
the total solids for the 24-hour period may easily be determined.

Calculation. — If the volume of urine for the 24 hours was 11 20 c.c. and the spe-
cific gravity 1.018, the calculation would be as follows:

(c) 18X2.6 = 46.8 grams of solid matter in i liter of urine.

... 46.8X1I2O r i-j ^^ • t •

(0) - =52.4 grams of solid matter m 1120 c.c. of unne.

Long's coefiicient was determined for urine whose specific gravity was taken
at 25°C. and is probably more accurate, for conditions obtaining in America, than
the older coefficient of Haeser, 2.33.

Interpretation. — See above.

Total Nitrogen

I. Kjeldahl Method J — Principle. — The principle of this method is
the conversion of the various nitrogenous bodies of the urine into am-
monium sulphate by boiling with concentrated sul-
phuric acid, the subsequent decomposition of the
ammonium sulphate by means of a fixed alkah
(NaOH) and the collection of the liberated ammonia
in an acid of known strength. Finally, this partly
neutralized acid solution is titrated with an alkali
of known strength and the nitrogen content of the
urine under examination computed.

Procedure. — Place 5 c.c. of urine in a 500 c.c. long-
necked Jena glass Kjeldahl flask, add 20 c.c. of concen- Fume^ Absorber^
trated sulphuric acid and about 0.2 gram of copper sulphate
and boil the mixture for some time after it is colorless (about; one hour). If
a suitable hood or fimie chamber is not available the sulphuric acid vapors may
be carried away by suction. Coimect the outlet tube of a 2-3 liter wash bottle
filled with caustic soda solution with a suction pump. The inlet tube is connected
with a Folin fume absorption tube such as illustrated in Fig. 152. If such a tube
is not at hand a small funnel may be attached. The absorption tube is placed
loosely over the mouth of the digestion flask and a constant current of air drawn
through the apparatus.

Allow the flask to cool and dilute the contents with about 200 c.c. of am-
monia-free water. Add a little more of a concentrated solution of NaOH than is
necessary to neutralize the sulphuric acid- and introduce into the flask a little
coarse pumice stone or a few pieces of granulated zinc,^ to prevent bumping, and a

' There are numerous modifications of the original Kjeldahl method; the one described
here, however, has given excellent satisfaction and is recommended for the determination of
the nitrogen content of urine.

*This concentrated sodium hydroxide solution should be prepared in quantity and
"check" tests made to determine the volume of the solution necessary to neutralize the
volume (20 c.c.) of concentrated sulphuric acid used.

* Powdered zinc may be substituted.

484 PHYSIOLOGICAL CHEMISTRY

small piece of paraffin to lessen the tendency to froth. By means of a safety-
tube connect the flask with a condenser so arranged that the delivery-tube passes
into a vessel containing a known volume (the volume used depending upon the
nitrogen content of the urine) of N/io sulphuric acid, using care that the end of
the delivery-tube reaches beneath the surface of the fluid. ^ Mix the contents
of the distillation flask very thoroughly by shaking and distil the mixture imtil
its volvune has diminished about one-half. Titrate the partly neutralized N/io
sulphuric acid solution by means of N/io sodivmi hydroxide, using congo red as
indicator, and calculate the content of nitrogen of the urine examined.

Calculation. — Subtract the number of cubic centimeters of N/io sodium
hydroxide used in the titration from the number of cubic centimeters of N/io
sulphuric acid taken. The remainder is equivalent to the number of cubic centi-
meters of N/io sulphuric acid, neutralized by the ammonia of the urine. One
c.c. of N/io sulphuric acid is equivalent to 0.0014 gram of nitrogen. Therefore,
if y represents the volimie of urine used in the determination, and y' the number
of cubic centimeters of N/io sulphuric acid neutralized by the ammonia of the
urine, we have the following proportion:

y: 100:: y'Xo. 0014: X (percentage of nitrogen in the urine examined).

Calculate the quantity of nitrogen in the 24-hour urine specimen.

Interpretation. — An adult of medium size on a mixed diet will usually
excrete 12-18 grams of nitrogen per day. It varies, hov^^ever, almost
directly with the protein ingestion and hence usually runs parallel to
the excretion of urea (see page 493). In a normal adult the total
nitrogen of the feces and of the urine will often be almost exactly
equal to the total nitrogen of the food. Such a condition is called
''nitrogen equilibrium." The feces usually contain very little nitrogen.
(See also Ammonia, Creatinine, etc.)

Calculation of Percentage Nitrogen Distribution.— In modern metabo-
lism studies where the various forms of nitrogen are determined, in
addition to the total nitrogen as yielded by the Kjeldahl method, it is
customary to indicate what portion of the total nitrogen was present in
the form of each of the individual nitrogenous constituents. These
percentage values are secured by dividing the weight (grams) of
nitrogen excreted for the day in the form of each individual nitrogenous
constituent by the weight of the total nitrogen output for the same
period. For example, if the total nitrogen excretion is 9.814 grams
and the excretion of urea-nitrogen is 8.520 grams and the excretions
of nitrogen in the forms of ammonia and creatinine are 0.271 gram and
0.639 gram respectively, the percentage distribution for these forms of
nitrogen would be calculated as follows:

8.520 grams urea-nitrogen -i- 9.814 grams total nitrogen = 84.3 per cent

o. 271 gram ammonia-nitrogen -r- 9.814 grams total nitrogen = 2.7 per cent
0.639 gram creatinine-nitrogen "^ 9.814 grams total nitrogen = 6.5 per cent

^This delivery-tube should be of large caliber in order to avoid the "sucking back"
of the fluid.

URINE 485

Nitrogen Partition in Urines Containing Albumin. — If the urine to
be tested contains albumin this must be removed before an attempt at
a nitrogen partition is made. This may be done by heating to boil-
ing, acidifying with acetic acid to coagulate the protein, filtering and
making up the filtrate to the original volume of the urine. If very small
amounts of albumin are present this is attended with difficulty. In
these cases Tracy and Welker^ have suggested the use of aluminium
hydroxide cream. It apprently removes none of the nitrogenous con-
stituents of normal urine.

Procedure. — One liter of urine (containing not over i per cent of albvunin)
is mixed with one liter of aluminium cream- and filtered.

2. Folin-Farmer Microchemical Method.'' — Principle. — This
method belongs with the so-called microchemical methods inasmuch as
it is adapted to the determination of amounts of nitrogen in the neigh-
borhood of I mg. while in the ordinary Kjeldahl procedure 30-100 mg.
of nitrogen are generally manipulated. One c.c. of diluted urine is
decomposed with sulphuric acid as in the Kjeldahl method, the am-
monia formed is set free by the addition of alkali and carried over into
an acid solution by means of a current of air. The ammonia solution
is then treated with the Nessler- Winkler reagent and the color produced
compared with that of a standard solution of an ammonium salt
treated in the same way.

Colorimeter. — For this method as well as for a number of other
methods commonly used in urinary and blood analysis an instrument
known as a colorimeter is required. Through its aid we are able ac-
curately to measure the respective depths of color in two solutions and
hence to calculate the comparative amounts of substances which form
colored compounds in a quantitative manner. The most satisfactory
instrument for this purpose is the Duboscq colorimeter (see Fig. 153,
page 486). This enables the two colored solutions to be compared in
the same optical field and with a degree of accuracy of about i per
cent. The later type of the Duboscq colorimeter with cylinders instead
of prisms movable is to be preferred, particularly as this type may be
readily adapted to the comparison of cloudy solutions or suspensions,
the instrument thus modified being called a nephelometer (see Fig. 83,
page 291). In this later form of colorimeter the depths of the colored

1 Tracy and Welker: Jour. Biol. Clicni. 22, 55, 1915; For other applications of alu-
minium hydroxide precipitation of colloids, see Welker and Marshall, /. Avi. Client. Soc,
25, 820, 1Q13.

'^Aluminium Hydroxide Cream. — To a i per cent solution of ammonium alum at room
temperature add a slight excess of a i per cent solution of ammonium hydroxide. Wash by
decantation until the wash water shows only the faintest trace of residue on evaporation.
Stronger solutions should not be used.

^ Folin and Farmer: Jour. Biol. Clirm., 11, 493, 1912.

486

PHYSIOLOGICAL CHEMISTRY

solutions through which the light passes are regulated by raising or
lowering the cups and are accurately indicated in millimeters on a
vernier scale at the back of the instrument. The standard solution is
placed at any convenient depth and the color of the solution to be ex-
amined is matched with it by raising or lowering cups. When the color
is of the same intensity as the standard the depth of the solution is
read. The amounts of the colored substance in solution are inversely
proportional to the depths of the columns of fluid. Thus if the standard
is set at lo mm. and the solution under examination has the same color

Fig. 153. — DuBOSCQ Colorimeter.

density at 20 mm. the latter has just one-half the concentration of the
standard.

A large number of other colorimeters have been devised and
may be used in place of the Duboscq. Most of these though less ex-
pensive than this instrument are also less accurate. The HelHge
colorimeter has been recommended, particularly for cHnical de-
terminations by Myers and Fine.^ Kober has devised a combined
colorimeter and nephelometer which may be obtained in this country
(see page 293). For merely approximate determinations the color

1 Myers and Fine: Post-graduate, 1914-1915.

URINE

487

comparisons may be made directly with a series of colored standards of
varying strengths made up in exactly similar test-tubes or small flasks.

Procedure. — Introduce 5 c.c. of urine into a 50 c.c. volumetric fiask if the
specific gravity of the urine is over 10 18, or into a 25 c.c. fiask if the specific
gravity is less than 1018.^ Fill the fiask to the mark with distilled water and
invert it several times in order to guarantee thorough mixing. Transfer i c.c.^
of the diluted urine to a large (20-25 °^™- X 200 mm.) Jena-glass test-tube.
Add to this i c.c. of concentrated sulphuric acid, i gram of potassium sulphate,
I drop of 5 per cent copper sulphate solution and a small, clean, quartz pebble or

Q e

Fig. 154. Fig. 155.

Figs. 154 and 155. — Forms of App.\ratus used in Methods of Folin and Associ-
ates FOR Determination of Total Nitrogen, Urea and Ammonia. (From Jour. Biol.
1912.)

Chem. vol.

glass bead. (The pebble or bead is added to prevent bumping.) Boil the mix-
ture over a micro-burner' for about six minutes, i.e., about two minutes after the
mixture has become colorless. Allow to cool until the digestion mixtiu-e begins
to become viscous. This ordinarily takes about three minutes, but in any event
the mixture must not be permitted to soUdify. Add about 6 c.c. of water (a
few drops at a time, at first, then more rapidly) to prevent sohdification. To this
acid solution add an excess of sodiiun hydroxide (3 c.c. of a saturated solution is
sufficient) and aspirate the Uberated ammonia by means of a rapid air current*

* The purpose is to so dilute the urine that i c.c. of the diluted fluid shall contain 0.75-
1.5 mg. of nitrogen.

^This measurement should be made by means of a modified Ostwald pipette (see Ost-
wald-Lulher: Physiko-Chemische Messungen, 2d. ed., p. 135). Such pipettes may be
obtained from Eimer and Amend, New York.

' A type of burner which has proven satisfactory is Eimer and Amcnd's No. 2587.

* Either a vacuum pump or compressed air or a force pump may be used. The com-

{)ressed air method is rather the more convenient inasmuch as the ammonia may be col-
ected directly in a volumetric flask. Inasmuch as the necks of such flasks (100 c.c.) are

488 PHYSIOLOGICAL CHEMISTRY

into a volumetric flask (loo c.c.) containing about 20 c.c. of ammonia-free water
and 2 c.c. of N/io hydrochloric acid (see Figs. 154 and 155, page 487). The
air current should be only moderately rapid for the first two minutes but at the
end of this two-minute period the current should be run at its maximum speed
for an interval of eight minutes.

Disconnect the flask, dilute the contents to about 60 c.c. with ammonia-
free water and dilute similarly i mg. of nitrogen in the form of ammonitrai sul-
phate^ in a second volimietric flask. Nesslerize both solutions as nearly as
possible at the same time with 5 c.c. of Nessler-Winkler solution- diluted, imme-
diately before using, with about 25 c.c. of ammonia-free water to avoid turbidity.
Immediately fill the two flasks to the mark with ammonia-free water, mix well
and determine the relative intensity of the two colors by means of a Duboscq
colorimeter. 3

The color of the unknown should be adjusted to that of the standard both from
above and below the level of the latter. The matching of the colors is ordinarily
very easy. It is desirable to make the readings by diffused dayUght if possible.
If e'ectric light must be used, a sheet of smooth white paper should be interposed
between the colorimeter and the source of Ught.

Calculation. — The reading of the standard divided by the reading of the un-
known gives the nitrogen in milligrams in the volume of the urine taken. Calcu-
late the total nitrogen output for the 24-hour period.

Interpretation. — See page 484.

3. Bock and Benedict's Modification of the FoUn-Farmer Procedure. —
Bock and Benedict* have found distillation of the ammonia more acciu-ate than

not large enough to permit of the use of a two-hole rubber stopper when suction is used,
the ammonia should be collected in one of the Jena test-tubes previously described which
contains 2 c.c. of N/io hydrochloric acid and about 5 c.c. of ammonia-free water. The am-
monium salt is then transferred to the volumetric flask with 40-50 c.c. of water and Nes-
slerized as described.

^ Care should be taken to secure the pure salt. All ammonium salts contain pyridine
bases which titrate like ammonia but do not react with Nessler's reagent. Pure ammonium
sulphate may be prepared by decomposing a high-grade ammonium salt with sodium hy-
droxide and passing the liberated ammonia into pure sulphuric acid. The salt is then pre-
cipitated by means of alcohol, then brought into solution in water and re-precipitated by
alcohol. The final product should be dried in a desiccator over sulphuric acid. Dr. H. L.
Emerson of Boston prepares a salt which is very satisfactory for use in this method.
According to Bock and Benedict, Kahlbaum's "Zur Analyse" ammonium chloride is
satisfactory.

^ Chetn. Zeil., 1899, p. 541. The Nessler-Winkler solution has the following formula:

Mercuric iodide 10 grams.

Potassium iodide 5 grams.

Sodium hydro.xide 20 grams.

Water 100 c.c.

The mercuric iodide is rubbed up in a small porcelain mortar with water, then washed
into a flask and the potassium iodide added. The sodium hydroxide is dissolved in the
remaining water and the cooled solution added to the above mixture. The solution cleared
by standing is preserved in a dark bottle.

The 25 c.c. portion of the diluted reagent should be added about one-third at a time to
the contents of the flask. It is verj' essential that the dilution of the reagent takes place
immediately preceding its use, inasmuch as the diluted reagent deteriorates in a few minutes as
is indicated by the formation of a brick-red precipitate. Fortunately the reagent does not
decompose in this manner in the presence of the ammonium salt.

^ The standard may be set at any desired depth but a very satisfactory depth is 20 mm.
The depth should be uniform throughout any series of comparative tests.

*Bock and Benedict: Jour. Biol. Cliem., 20, 47, 1915.

URINE

489

aspiration. They connect the large Jena test-tube in which the digestion was
carried out with a small Liebig condenser (made from a piece of glass tubing
30 by 150 mm. with two-hole rubber stoppers at each end through which pass
the inlet and outlet tubes and the condenser tube itself j. See Fig. 156. The lower
end of the condenser is connected with a glass tube (or better an old pipette, to
prevent back suction) which reaches nearly to the bottom of the voliunetric flask
used as a receiver. The distillation tube also has a two-hole rubber stopper. It
is connected with the condenser and also carries a long straight tube which reaches
nearly to the bottom of the test-tube, and is closed above with a piece of rubber
tubing and a pinch-cock. The digestion is carried out just as in the Folin-Farmer
method (see page 485) and when partially cool 7 c.c. of water are added. Into the
long tube passing through the stopper suck 3 c.c. of saturated sodium hydroxide
solution and close the pinch-cock. Insert the stopper, connect with the condenser

Fig. 156. — Bock and Benedict Apparatus.

and allow the alkah to run into the test-tube. The fluids are mixed by blowing a
few bubbles of air through the apparatus. The test-tube is then heated to vigor-
ous boiling (over a large free flame), the distillation being continued until a sepa-
ration of salts occurs in the test-tube and the mixture begins to bump. This
distillation requires about two minutes. The test-tube is then disconnected from
the condenser and the latter washed down with a few cubic centimeters of water.
The liquid in the receiving flask is diluted and Nesslerized as in the Folin-Farmer
method (see page 485).

Bock and Benedict, while holding the distillation procedure to be
more accurate than aspiration, do not consider that the colorimetric
method is equivalent to the standard Kjeldahl procedure in accuracy
or reliability, although usually it agrees with the latter method within
about 2-3 per cent, and is indispensable where very small amounts of
nitrogen are to be determined. According to Folin^ and others the
method is capable of greater accuracy than this, and the aspiration

* Folin: Jour. Biol. Cfictn., 21, 195, 1915.

490 PHYSIOLOGICAL CHEMISTRY

procedure gives satisfactory results. The method should be checked
up carefully by each new learner of the method, using pure solutions.
Outside air is better than laboratory air for aspiration purposes.
Care is needed in using the pipettes, which should be of the Ostwald
type and accurate. In using them allow the pipette to drain against
the side of the vessel for lo seconds and then blow out clean so that
nothing is left behind in the tip. The reagents used must be as free
as possible from ammonia and must be checked up, particularly the
sulphuric acid and potassium sulphate. Those who have trouble in
using a colorimeter may substitute titration with N/50 hydrochloric
acid using alizarin, or better methyl red, as an indicator.

4. Gulick's Modification of the Folin -Fanner Colorimetric Method.' — Prin-
ciple.— By using small amounts of sulphuric acid and potassium sulphate it is possi-
ble to Nesslerize the products of the digestion directly
without the necessity of previous aspiration of the
ammonia.

Procedure. — Dilute the sample of urine to an exact
multiple of its original volume (about 4-10 times) with
acid mixture,^ so that 0.5 c.c. of the dilution will contain
between 0.4 and 0.7 mg. of nitrogen. With an Ostwald
pipette introduce 0.5 c.c. of this mixture into the bulb
of a micro-oxidation flask. The type illustrated in Fig.
157, with a bulb capacity of about 15 c.c, is the most
convenient. Add also a small spherical glass bead or
scrap of platinum or, better, a piece of platinum wire 4-5
mrn. long bent into a tight spiral. Agitate continually
while boiling off the water over a micro-burner (about
one minute). Set up to heat over a very small flame well
guarded against the wind. A luminous flame 6-7 mm.
CRO-oxiDATioN Flask^' ^^^^ comiug from a burner tube of about 3 mm. outside
diameter may be used. The digestion bulb is set at a
slant so that the mouth is directed upward and the heat applied at the tip.
Heat for at least one minute after the acid becomes clear white. The boiling and
oxidation require about 6-10 minutes. As soon as the glass is cool enough to bear
water add sufficient ammonia-free water to dissolve the contents, and rinse quanti-
tatively into a 50 c.c. volumetric flask.

Introduce into a second 50 c.c. flask 0.5 mg. of nitrogen in the form of pure
ammonium sulphate. Fill both flasks to about 40 c.c. with ammonia-free water.
Into each of the flasks then inject 5 c.c. of the modified Winkler solution^ in a vigor-
ous stream from a pipette. Fill to the mark and mix thoroughly. Compare

^ Gulick: Jour. Biol. Client., 18, 541, 1914.

^ Acid Oxidizing Mixture. — To 125 c.c. of ammonia-free water add 40 c.c. of sulphuric
acid, 5 c.c. of a saturated solution of mercuric chloride and 20 gm. of potassium sulphate.
Then make up to 200 c.c. with ammonia-free water.

^ Modified Winkler Solution.— Dissolve 40 grams of sodium hydroxide in about 200 c.c.
of ammonia-free water. Mix 15 grams of mercuric iodide and 10 grams of potassium iodide
and dissolve in about 15 c.c. of water. Transfer with the aid of the alkali to a 500 c.c.
volumetric flask and make up to 500 c.c. with ammonia-free water. Transfer to an Erlen-
meyer flask and let stand 24 hours to settle.

URINE 491

at once or at least within an hour in a colorimeter, using a depth of standard of
20-30 mm.

Urea

I. Urease Methods. — Principle. — These methods depend upon the
principle that the enzyme urease is able, at ordinary temperatures, to
transform urea, quickly and completely, into ammonium carbonate.
Takeuchi^ in 1909 discovered the presence of this enzyme in the soja
or soy bean. The application of this enzyme to the determination
of urea in urine, blood, etc., was first proposed by Marshall,- whose
methods have been modified by Van Slyke and CuUen.^ These latter
investigators prepared a permanent preparation of the enzyme, in a
water-soluble form, the use of which makes more convenient the rapid
and accurate determination of urea in urine, blood and other biological
fluids.

The urease method is probably the most satisfactory of all methods
for the determination of urea. Other nitrogenous constituents such
as allantoin are not decomposed by urease. The method involves no
carefully regulated heating procedures, and is apphcable to diabetic
urines.

The procedure for the determination in urine consists in treating
the urine sample with urease, aerating the ammonia formed into fiftieth-
normal acid, and titrating the excess of acid with fiftieth-normal
alkali. (For colorimetric procedure see page 492.)

Preparation of Solid Urease.* — Digest one part of soy bean meal with five parts
of water at room temperature, with occasional stirring, for an hour, and clear the solu-
tion by filtration through paper pulp or centrifugation. Pour this extract slowly,
with stirring, into at least 10 volumes of acetone. The acetone dehydrates the
enzyme preparation. Filter, dry in vacuum, and powder. The activity of the
preparation is retained indefinitely. Thus prepared it is not perfectly soluble in
water, but this fact interferes in no way with its use.

Standardization of the Enzyme Preparation. — Make up accurately a 3 per cent
solution of pure urea. Treat this solution exactly as the urine is treated in the
following method, using 1.2 c.c. of the solution. The ammonia formed should
neutralize 25 c.c. of N/50 acid. If it does so the preparation is of sufiicient strength
to use as indicated. If not, more of the preparation must be used for a
determination.

The ground soy bean may also be used directly in this determination. It
should pass through a 20-mesh sieve. Rose and Coleman for their micro-procedure

1 Takeuchi: 7o»r«. Coll. Agr. Tokyo, 1909, Part i.

* Marshall, E. K., Jr. :/. Biol. CItcm., 14, 283, 1913; 15, 495, 1913; 15, 487, 1913; 17,

351, iQU-

^Van Slyke, D. D., and Cullen, G. E.: /. .Iw;. Med. Ass'n, 62, 1558, 1914. See, also,
J. Biol. CItcm., 19, 141, 1914.

* Van Slyke and Cullen: Jour. Biol. Chem., 19, 211, 1914. Satisfactory preparations
of Urease may be obtained from the Arlington Chemical Company, Yonkers, N. Y., and
from Hynson, Westcott and Co., Baltimore.

492

PHYSIOLOGICAL CHEMISTRY

(see below) use 0.2-0.4 gram of bean flour acting in a water-bath at 50-60° for five
minutes. In their macro-method, using 5 c.c. of urine they dilute with 30 c.c. of
water warmed to 50-60° and then add 5 grams of the soy bean flour and let stand
for 30 minutes. They then add 5 c.c. of saturated sodium carbonate solution and
aerate as usual.

(a) Procedure of Van Slyke and Cullen. — Dilute 5 c.c .of urine to 50 c.c. with
ammonia-free water. Measure 5 c.c. of the diluted urine into Tube "A" (see
Fig. 158), add i drop of caprylic alcohol (to prevent frothing), and i c.c.
of enzyme solution. ^ Close "A" with stopper shown in figure, and let the tube
stand 15 minutes for the enzyme to act. Measure into Tube "B" 25 c.c. of N/50
HCl or H2SO4. Add i drop of capryUc alcohol and i drop of a i per cent alizarin
solution,^ as indicator. Connect "A" and "B" as shown in the figure. At the

end of 15 minutes aspirate for about one-half
minute to remove any ammonia present in the
free condition in "A." After this aspiration,
open "A" and introduce 5 c.c. of saturated
potassium carbonate. Close "A" at once and
aspirate until all the ammonia has been re-
moved from "A" and carried over into the acid
in "B." The time needed for the aspiration
varies for different pumps from 5 to 30 minutes,
and should be determined by trial for the par-
ticular apparatus used. At the end of the time
needed for the aeration,' the pvmip is discon-
nected (care being taken to avoid back suc-
tion) and the excess acid in "B" is titrated by
means of fiftieth-normal alkali.

Calculations. — The number of cubic centi-
meters of fiftieth-normal acid neutralized is
multiplied by the factor 0.056 to give the
niunber of grams of urea-plus ammonia-nitro-
gen in 100 c.c. of the urine. The ammonia
alone may be determined at the same time as the ammonia plus urea, using
the same technic except that 5 c.c. of the undiluted urine, no urease, and the
factor 0.0056 are used for the determination of ammonia alone. The am-
monia tubes are run in the same series as those for the urea determination,
using the same air current for all.

(b) Color imetric Modification. — Rose and Coleman^ suggest the colorimetric
determination of the ammonia which is carried over by the aspiration, rather than
titration of the excess of acid. They Nesslerize the solution in "B," and compare
the color produced with the color of a Nesslerized solution of known ammonia con-
tent, as in the Folin-Farmer method for total nitrogen. If this procedure is fol-
lowed, the amount of urea and ammonia nitrogen in the solution acted upon by the

1 The enzyme solution is prepared by dissolving 2 grams of the enzyme preparation, 0.6
gram of dipotassium-hydrogen phosphate, and 0.4 gram of monopotassium-dihydrogen
phosphate in 10 c.c. of water. Solution is aided by stirring with a glass rod. The slightly
opalescent solution should be covered with toluol and may be kept for two weeks without
losing activity.

* Folin states that methyl red is preferable to alizarin for ammonia titrations.

^See Fiske {Jour. Biol. Chew. 23, 455, 1915) and Van Slyke and Cullen (Jour. Biol.
Chem., 24, 117, 1916) for discussion of details of method.

*Rose and Coleman; Biochem. Bull., 3, 411, 1914.

Fig. 158. — Van Slyke and

CtJLLEN APPAR.A.TUS.

URINE 493

urease must not exceed 2 mg. This procedure has been found useful where small
quantities of urea are to be estimated.

Interpretation. — The mean average daily excretion of urea by normal
adults is usually placed at about 30-35 grams but is very closely de-
pendent upon the protein ingestion and hence may vary widely. It
is of significance only when the amount of nitrogen ingested is known
with some degree of accuracy. In disorders associated with increased
tissue catabolism as in fevers, the excretion of urea is increased. It
may be decreased in pronounced kidney and liver disorders due to
decreased formation and decreased power of elimination, but these
findings are not constant.

The per cent of the total nitrogen of the urine occurring as urea
varies on the average from 80-90. On a high protein diet it is nearer
90 per cent; on a very low nitrogen but high calorie diet it may not
be over 60 per cent. In marked acidosis it may be considerably
decreased relative to the total nitrogen (see ammonia).

(c) Marshall's Urease Method.' — Principle. — This is a simple clin-
ical method for the determination of urea in urine. It differs from the
preceding method in that instead of aspirating off the ammonia formed
from the urea by the action of the urease, it is titrated directly in the
urine mixture, thus simplifying the procedure. The method is nearly
as accurate as the preceding, for normal urine the error being only
about 2 per cent which is very satisfactory for a rapid clinical procedure.
For diabetic urines the aeration procedure should be used as such urines
contain substances which render the titration inaccurate.

Procedure. — Two 5 c.c. portions of the urine are measured into flasks of
200-300 c.c. capacity and diluted with distilled water to about 100-125 c.c.
One c.c. of a 10 per cent solution of urease prepared as described on page 491 is
added to one flask, a few drops of toluene to each and the solution allowed to
remain, well stoppered, at room temperature over night (or five hours). The
fluid in each fiask is titrated to a distinct pink color with N 10 hydrochloric acid
using methyl orange as an indicator. A few cubic centimeters of the enzyme
solution used should also be titrated to determine the amount of N/io hydro-
chloric acid required to neutraUze i c.c.

Calculation. — The amount of hydrochloric acid required for the contents of
the flask containing the urine and enzyme solution, less the amount used for
5 c.c. of urine alone and that previously determined for i c.c. of enyzme solution,
corresponds to the urea originally present in the sample of urine. Since i c.c.
of N/io HCl is equivalent to 3 mg. of urea, the number of cubic centimeters
required, multiplied by 0.6 gives the value of urea expressed in grams per Uter
of urine.

Interpretation. — See above.

' Marshall: Jour. Biol. Cliem., 14, 283, 1913.

494 PHYSIOLOGICAL CHEMISTRY

2. Benedict's Method.^ — Principle. — The urea is decomposed by
heating with a mixture of potassium bisulphate and zinc sulphate. The
fact that the hydrolyzing agent is a salt and that the digestion takes
place in the practical absence of water seem to insure less decomposition
of substances other than urea. The ammonia formed is distilled off
and determined in the usual manner.

Procedure. — Five c.c. of urine are introduced into a rather wide Jena glass
test-tube, about 3 grams of potassium bisulphate and 1-2 grams of zinc sulphate*
added, a small quantity of powdered pumice and a bit of parafl&n are introduced
and the mixture boiled almost to drjrness either over a free flame or by immersion
in a sulphuric acid bath at about 130°. The tubes are then weighted (a screw
clamp is convenient) and immersed for three-fourths of their length in a bath of
sulphuric acid at a temperature of 162-165° (not lower) for one hour.

The contents of the tube are then washed into an 800 c.c. Kjeldahl distillation
flask, diluted to about 400 c.c. with water, made alkaline by the addition of 15-20
c.c. of 10 per cent KOH (or 25 c.c. 15 per cent Na2C03) and distilled as usual in the
Kjeldahl method (page 483). The value obtained must be corrected for ammonia
by a separate determination of the latter.

Welker^ has suggested an electrical bath for use in the first part of this method.

3. Microchemical Method of Folin and VeMihone^^Principle. —

The urine is heated with potassium acetate and acetic acid to hydro-
lyze the urea. The desired temperature is maintained with the aid
of a temperature indicator. The ammonia formed is aspirated ofT
and determined colorimetrically with Xessler-Winkler reagent.

Procedure. — Dilute the urine so that 1 c.c. contains 0.75-1.5 mg. of urea
nitrogen. Generally dilutions of i : 20 or i : 10, depending on the concentration,
are satisfactory. By means of an Ostwald pipette (see page 487) introduce i c.c.
of the diluted urine into a large dry Jena test-tube (20-25 mm. by 200 mm.) which
already contains 7 grams of dry ammonia-free potassium acetate^ (free from
lumps), I c.c. of 50 per cent acetic acid, a small sand pebble or a little powdered zinc
(not zinc dust) to prevent bumping during boiling and a temperature indicator."

^ Benedict: Jour. Biol. Chem., 8, 405, 191 1.

^ An excess of zinc salt is to be avoided as too large quantity tends to cause slight frothing
during the final distillation.

' Welker: Biochem. Bull., i, 439, 191 2.

* Folin and Pettibone: Jour. Biol. Chem., 11, 513, 1912.

^ A satisfactory preparation containing less than i per cent of moisture and free from
ammonia maj' be obtained from J. T. Baker Chemical Co., Phillipsburg, N, J.

• "This temperature indicator consists of powdered chloride-iodide of mercury (HglCl)
inclosed in a sealed glass bulb not over i mm. in diameter. This salt is bright red at ordi-
nary temperatures. At ii8°C. it turns yellow and melts to a clear dark red liquid at i55°C.
It solidifies again at about i48°C. and resumes its red color gradually ordy in the course of
about 24 hours. The melting-point temperature, i53°C., is fortunately a temperature
very readily obtained and maintained by means of potassium acetate and as the acetate
begins to cake and solidify at i6o°-i6i°C., there is no danger in this combination of having
either too high or too low a temperature without its being unmistakably apparent.

The HglCl may be prepared by heating, in a dry state, intimately mixed mercuric
chloride and mercuric iodide in molecular proportions at i5o°-i6o°C. for 6-8 hours. At the
end of the heating the product should be powdered and used as it is for it cannot be purified
by the use of solvents. It should be kept dry until sealed up as indicated." These tern*
perature indicators may be obtained ready prepared in tubes from Eimer and Amend
New York.

URINE 495

Close the test-tube by means of a rubber stopper carrying an empty narrow
"calcium chloride tube" (1.5 cm. by 25 cm., without bulb) as a condenser. Sus-
pend the test-tube and condenser above a micro-burner (see page 487 • by means
of a burette clamp or some similar device in such a way that they may be easily
raised or lowered. Heat gently, using a bottomless beaker or some similar
device as a wind shield if needed. The acetate will soon dissolve (two minutes)
and the mixture begin to boil. At this point the indicator begins to melt showing
that the desired temperature (i53-i6o°C.) has been reached. Continue the
boiling in a gentle, even manner for ten minutes at the end of which time the
decomposition of the urea is complete. Remove the apparatus from the flame
and dilute the contents with 5 c.c. of water. ^ Add an excess of alkali 12 c.c. of a
saturated solution of sodium hydroxide or potassium carbonate] and remove
the Uberated ammonia by means of a strong air current (see page 487). The
ammonia may be caught in a 100 c.c. volumetric flask which contains about 35
c.c. of ammonia-free water and 2 c.c. of N/io acid. With a stiong air current
this process requires only about ten minutes. Determine the ammonia colori-
metrically against i mg. of nitrogen in the form of ammonium sulphate. For
the colorimetric procedure see the total nitrogen determination page 485.

4. Method of Folin and Denis. ^^ — Principle. — Sugar interferes with the de-
composition of urea. This was formerly believed to be due to the formation of
nitrogenous "melanins,"* but is more probably due to the formation of definite,
stable ureids.* This difficulty may be overcome by proper dilution of the urine
thus preventing the formation of the ureids. Because of this great dilution titration
procedures are inapplicable, and the colorimetric procedure is applied.

Procedure. — Dilute i c.c. of the urine with 20 to 100 volumes of ammonia-free
water and decompose i c.c. of this dilute urine with potassium acetate and acetic
acid as described under the method of Folin and Pettibone on page 494.

By means of an air current remove the ammonia to a second test-tube which
contains about 2 c.c. of water and 0.5 c.c. of N/io hydrochloric acid. Add to the
contents of this tube about 2 c.c. of water and 3 c.c. of the diluted (1:5) Nessler-
Winkler solution (page 490). Wash this colored solution into a 10 c.c. volumetric
flask and dilute it to the mark with ammonia-free water. Transfer the entire vol-
ume to a dry cylinder of a Duboscq colorimeter and determine the depth of color
against a standard containing i mg. of nitrogen per 100 c.c. of solution. For the
detailed colorimetric procedure see the method for total nitrogen, page 494.

5. Method of Folin. ^ — Principle. — The urea is decomposed by heating with
magnesium chloride and hydrochloric acid. The ammonia is distilled off and de-
termined by titration. This method was one of the first accurate methods for the
determination of urea. .\lIantoin is also included in the results from this method
but occurs only in minute quantities in human urine. The method is not applicable
to urines containing sugar as ureides are formed. For such urines the method of
Folin and Denis (above) or the urease method using aspiration (page 491) may
be employed. The earlier Morner-Sjoqvist method* has been combined with that

^ This water should be added by means of a pipette through the calcium chloride tube so
as to rinse the sides of the tube and the bottom of the rubber stopper from any possible traces
of ammonium acetate. Not more than 5 c.c. of water should be used for this purpose.

-Folin and Denis: Jour. Biol. Chem., 11, 520, 1912.

'Morner: Skatid. Arch. Physiol., 14, 319.

* Folin: Am. Jour. Physiol., 13, 46, 1905.

'Folin: Am. Jour. Physiol., 13,46, 1905.

•M6rner: Skand. Arch. Physiol, 14, 297, 1903. See also Fourth Edition of this book.

496

PHYSIOLOGICAL CHEMISTRY

Q^^mJ*

of the Folin procedure in such a way as to render the latter applicable to urines
containing sugar, to remove certain interfering substances such as allantoin and
make the separate determination of ammonia unnecessary. The method is, how-
ever, time-consuming and the other methods mentioned are on this account to be
preferred for the analysis of diabetic urines.

Procedure. — Place 5 c.c. of urine in a 200 c.c. Erlenmeyer flask and add to it
5 c.c. of concentrated hydrochloric acid, 20 grams of crystallized magnesium chlo-
ride, a piece of paraffin the size of a hazel nut, and 2-3 drops of a i per cent aqueous

solution of "alizarin red." Insert a Folin safety
tube (Fig. 159) into the neck of the flask and
boil the mixture until each drop of reflow from
the safety tube produces a very perceptible bump;
the heat is then reduced somewhat and con-
tinued one and one-half hours. The contents
of the flask must not remain alkaline, and to
obviate this, at the first appearance of a red-
dish tinge in the contents of the flask a few drops
of the acid distillate are shaken back into the
flask. At the end of one and one-half hours the
contents of the vessel are transferred to a i -liter
flask with about 700 c.c. of distilled water, about
20 c.c. of ID per cent potassium hydroxide or so-
dium hydroxide solution is added and the mix-
ture distilled into a known volume of N/io sul-
phuric acid until the contents of the flask are
nearly dry or until the distillate fails to give an
alkaline reaction to litmus, showing the absence
of ammonia. The time devoted to this process
is ordinarily about an hour. Boil the distillate a
few moments to free it from CO2, then cool and
titrate the mixture with N/io sodium hydroxide,
using "alizarin red" as indicator.

A " check " experiment should always be made

to determine the original ammonia content of

the urine and of the magnesium chloride, if it

is not absolutely pure, which of course should be

subtracted from the total amount of ammonia

as determined by the above process.

6. Hypobromite Methods. — Principle. — The hypobromite methods are based

upon the fact that urea is decomposed by a solution of sodium hypobromite with

the formation of carbon dioxide and gaseous nitrogen according to the following

equation :

CO(NH) 2-f 3NaOBr = Na-f- CO2+ 2H20-h 3NaBr

Fig. i5g. — Folin's Urea
App.'Vratus.

The carbon dioxide is retained by the alkaline solution and the nitrogen gas is col-
lected and measured. On account of its simplicity this has been the most widely
used of clinical methods for the determination of urea. It possesses, however, sev-
eral essential inaccuracies among which may be mentioned the fact that all of the
urea nitrogen is not liberated, while on the other hand substances always present

URINE

497

in urine such as ammonia, creatinine, and uric acid yield nitrogen more or less
rapidly when the urine is treated with hypobromite. The measurement of the gas
as ordinarily carried out involves considerable errors. The results are usually high,
and may be excessively so. Robinson and Muller^ have suggested that the
ureometcr be shaken for five minutes to hasten the reaction and that the results
as obtained be multiplied by the factor 0.917 to insure more accurate results.
They use the Doremus-Hinds apparatus.

(a) Hypobromite Method {using the Doremus-Hinds Ureometer). — The Doremus-
Hinds ureometer (Fig. 160) is one of the simplest and cheapest forms of appa-

r^

ratus in general use for the determination of
urea by the hypobromite process. It is, how-
ever, much less accurate than those types of
apparatus which involve the measurement of
the nitrogen in a gas burette over water w'ith
equalization of pressure. In using this appa-
ratus proceed as follows: Fill the side tube B
and the lumen of the stop-cock C with the
urine under examination. Carefully wash out
tube A with water and introduce into it sodium
hypobromite solution,^ being careful to fill the
bulb sufficiently full to prevent the entrance
of air into the graduated portion. Now allow
I c.c. of urine- to flow from tube B into tube A,
and after the evolution of gas bubbles has ceased
(10-20 minutes) take the reading of the gradu-
ated scale on tube A.

Calculation. — Observe the reading on the
graduated scale of tube A. This tube is so
graduated as to represent the weight of urea, in
grams, per cubic centimeter of urine. If w-e
wish to compute the percentage of urea present
this may be done very readily by simply moving
the decimal point two places to the right; e.g., if
the reading is 0.02 gram the urine contains 2
per cent of urea.

Interpretation. — See page 493.

{b) Hypobromite Method (using Marshall's Urea Apparatus). — Place the thumb
over the side opening of the bulbed-tube of the apparatus (Fig. 162) and carefully
fill the tube with sodium hypobromite solution.' Close the opening in the end of
the tube with a rubber stopper, incline the tube to allow air-bubbles to escape, and

* Robinson and Muller: Jonr. Am. Med. Ass'n, 62, 514, 1914.

^ If the content of urea in the urine under examination is large, tlie urine may be diluted
with water before determining the urea. If this is done it must of course be taken into con-
sideration in computing the content of urea.

' The ingredients of the sodium hypobromite solution should be prepared in the form of
two separate solutions. When needed for use mi.\ one volume of solution a, one volume of
solution b, and 3 volumes of water.

(a) Dissolve 125 grams of sodium bromide in water, add 125 grams of bromine and make
the total volume of the solution i liter.

(b) A solution of sodium hydroxide having a specific gravity of i .250. This is approxi-
mately a 22.5 per cent solution.

Preserve both solutions in rubber-stoppered bottles.

32

Fig

I 60. DORF-MlS-HlNDS

Ureometer.

498

PHYSIOLOGICAL CHEMISTRY

finally invert the tube and fix the stoppered end in the saucer-shaped vessel. By
means of the graduated pipette rapidly introduce i c.c. of urine^ into the hypo-
bromite solution through the side opening of the bulbed-tube. Withdraw the
pipette immediately after the urine has been introduced. When the decomposition
of the urea is completed (10-20 minutes), gently tap the bulbed-tube with the finger
in order to dislodge any gas bubbles which may have collected on the inner surface
of the glass. The atmospheric pressure should
now be equalized by attaching the funnel-tube
to the bulbed-tube at the side opening and
introducing hypobromite solution into it un-
til the columns of liquid in the two tubes are
uniform in height. The graduated scale of
the bulbed-tube should now be read in order
to determine the number of cubic centimeters
of nitrogen gas evolved. By means of the ap-
pended formula the weight of the urea present
in the urine under examination may be com-
puted.

jTTTTTTnTIIIHIIIIIIIHIMI i|i'|ni|||lllli;|i|li|l.'ihJilnl!-^^

Fro. 161. — Marshall Urea Apparatus.
(Tyson.)
a, Bulbed measuring tube; b, saucer-
shaped vessel; c, graduated pipette; d,
funnel-tube.

Fig. 162. — HiJFNER Urea Apparatus.

Calculation.^ — By properly substituting in the following formula, the weight of
urea, in grams, contained in the volume of urine decomposed (i c.c. or more) may
readily be determined:

1 Ordinarily i c.c. of urine is sufficient; more may be used, however, if its content of urea
is very low.

2 0.00366s = coefficient of expansion of gases for i°C. 354.5 = number of c.c. of nitrogen
gas evolved from i gram of urea.

URINE

499

vjp - T)

354.5X760(1+0.0036650

IV = weight of urea, in grams.

V = observed volume of nitrogen expressed in cubic centimeters.
p = barometric pressure expressed in millimeters of mercury.

T = tension of aqueous vapor^ for temperature /.
t = temperature (Centigrade).

If we wish to calculate the percentage of urea we may do so by means of the
following proportion in which y represents the volume of urine used and w denotes
the weight of the urea contained in the volume y:

y :w :: X : {percentage of urea).

Sodium hypobromite solution may also be employed for the determination of
urea in the apparatus devised by Hiifner, which is pictured in Fig. 162.
Interpretation. — See page 493.

Ammonia

I. Folin's Method. — Principle. — The ammonia of the urine is set
free bv the addition of an alkali and this ammonia is then carried over

Fig. 163. — FoLiN Ammonia App.-\ratus.

by an air current into a flask containing a measured amount of standard
acid. The excess acid is then titrated. The necessity for distillation
is avoided.

^The values of T for the temperatures ordinarily met with are given in the following
table:

Temp. Tension in mm.

IS°C 12.677

i6°C 13519

i7°C 14.009

i8°C 15.351

19 (^' 16-345

20°C 17-396

Temp. Tension in mm.

2i°C 18.505

22°C 19-675

23°C 20.909

24°C 22.311

25'C 23.582

500

PHYSIOLOGICAL CHEMISTRY

Procedure. — Place 25 c.c. of urine in an aerometer cylinder, 30-40 cm. in
height (Fig. 163, p. 499), add about i gram of dry sodium carbonate and introduce
some crude petroleum to prevent foaming. Insert into the neck of the cylinder a
rubber stopper provided with two perforations, into each of which passes a glass
tube, one of which reaches below the surface of the Uquid. The shorter tube
(10 cm. in length) is connected with a calcium chloride tube filled with cotton, and
this tube is in turn joined to a glass tube extending to the bottom of a 500 c.c.
wide-mouthed flask which is intended to absorb the ammonia and for this pur-
pose should contain 20 c.c. of N/io sulphuric acid, 200 c.c. of ammonia-free
distilled water and a few drops of an indicator (alizarin red
or Congo red). To insure the complete absorption of the
ammonia the absorption flask is provided with a Folin im-
proved absorption tube (Fig. 164), which is very effec-
tive in causing the air passing from the cylinder to come
into intimate contact with the acid in the absorption flask.
In order to exclude any error due to the presence of am-
monia in the air a similar absorption apparatus to the one
just described is attached to the other side of the aerom-
eter cylinder, thus insuring the passage of ammonia-free
air into the cylinder. With an ordinary filter pump and
good water pressure the last trace of ammonia should be
removed from the cylinder in about one and one-half hours. ^
The number of cubic centimeters of the N/io sulphuric acid
neutraUzed by the ammonia of the urine may be determined
by direct titration with N/io sodium hydroxide.

Steele^ has suggested a modification for use on
urines containing triple phosphate sediments. In
this modification 0.5-1.0 gram of NaOH and
about 15 grams of NaCl are substituted for the
Na2C03 of the Folin method. The use of sodium
hydroxide and chloride instead of carbonate has also been recom-
mended by other workers^ as a general procedure, inasmuch as triple
phosphate crystals are almost always formed on adding sodium car-
bonate and these are decomposed with some difficulty by sodium
carbonate but readily by the hydroxide. It has not been shown
that the use of sodium hydroxide in this manner brings about the
decomposition of any other urinary nitrogen compounds.

Fig. 164. — Folin
Improved Absorp-
tion Tube.

Calculation. — Subtract the number of cubic centimeters of N/io sodium
hydroxide used in the titration from the number of cubic centimeters of N/io sul-
phuric acid taken. The remainder is the number of cubic centimeters of N/io
sulphuric acid neutralized by the NH3 of the urine. One c.c. of N/io sulphuric

^ With any given filter pump a " check " test should be made with urine or, better, with a
solution of an ammonium salt of known strength to determine how long the air current must
be maintained to remove all the ammonia from 25 c.c. of the solution.

^Steele: Jour. Biol. Chetn., 8, 365, 1910.

^Benedict and Ostcrberg: Biochem. Bull., 3, 41, 1913.
Shulansky and Gies: Biochem. Bull., 3, 45, 1913.

URINE 501

acid is equivalent to 0.0017 gram of NH3. Therefore if y represents the volume
of urine used in the determination and y' the number of cubic centimeters of
N/io sulphuric acid neutralized by the NH3 of the urine, we have the following
proportion :

y' : ioo::y'Xo.ooi7:x (percentage of NH3 in the urine examined).

Calculate the quantity of NH3 in the 24-hour urine specimen.

Interpretation. — The average daily output of ammonia in the urine
is about 0.7 gram, amounting to 2.5-4.5 per cent of the total nitrogen
excretion. It is increased by the ingestion of acids or acid-forming
foods and decreased by the ingestion of alkalis or base-forming foods.
In acidosis it may be very greatly increased, being excreted in com-
bination with hydro-oxybutyric and other acids. Values of 5 grams
have been noted. It is at the same time increased relative to total
nitrogen and urea. In pronounced liver disorders the same thing is
noted, as ammonia is not so completely transformed into urea before
excretion.

2. Micro -chemical Method of Folin and MacCallum. ^ — Principle. —
This method is a combination of the aeration procedure for ammonia
with its colorimetric determination by means of Nessler-Winkler solu-
tion. It gives satisfactory results, but is probably not as accurate as
the regular Fohn procedure where the amount of substance for analysis
is not limited.

Procedure. — ^By means of Ostwald pipettes introduce 1-5 c.c. of urine-
into a Jena test-tube (20-25 mm. by 200 mm.) and add to the urine a few drops
of a solution containing 10 per cent of potassium carbonate and 15 per cent of
potassixnn oxalate. To prevent foaming add a few drops of kerosene or heavy,
crude machine oil. Pass a strong air current (see page 487) through the mixture
imtil the ammonia has been entirely removed.' Collect the ammonia in a 100
c.c. volumetric flask containing about 20 c.c. of ammonia-free water and 2 c.c.
of N/io acid.

Nesslerize as described in the method for total nitrogen, page 488, and com-
pare with I mg. of nitrogen obtained from a standard ammoniimi sulphate solu-
tion and similarly Nesslerized.

It has been noted that a trace of something capable of giving a color with
the Nessler-Winkler solution continues to come long after all the ammonia
has been removed from the urine. The nature of this substance has not yet
been determined. In actual determinations by this method, the influence of
this unknown substance, because of the small volume of urine used, is entirely
negUgible.

1 Folin and MacCallum: Jour. Biol. Chcin., ii, 523, 1912.

^The volume of urine taken should contain 0.75-1.5 mg. of ammonia nitrogen. With
normal urines 2 c.c. will generally yield the desired amount. With very dilute urines 5 c.c.
may be required, while with diabetic urines rich in ammonium salts i c.c. may be excessive^
thus requiring dilution.

^ Ordinarily a period of ten minutes is suflSciently long.

502 PHYSIOLOGICAL CHEMISTRY

3. Formol Titration Method (Malfatti).^ — Principle. — This method

is based on the reaction taking place when formalin solution is
added to a solution containing ammonium salts (see Amino-acid
Nitrogen, below). An acid reaction is produced in the mixture,
which is then titrated with standard alkaH using phenolphthalein as
an indicator. Amino-acids give the same reaction so that the result
of the titration represents ammonia + amino-acid nitrogen. This
method may be used for the rapid cHnical estimation of these forms of
nitrogen as a substitute for an ammonia determination, but the results
do not represent ammonia as is sometimes stated.

Procedure. — To 25 c.c. of urine in a 200 c.c. Erlenmeyer flask add 15-20
grams of finely pulverized potassiiim oxalate, a few drops of phenolphthalein,
and titrate to a faint but permanent pink color with N/'io NaOH. (The urine
mixture just after neutralization in the urinary acidity determination (see page
479) may be used.) Then add 10 c.c. of neutral formalin solution (see amino-
acid nitrogen), mix well and titrate with N/io sodium hydroxide to a permanent
pink color.

Calculation. — One c.c. of N/'io sodivmi hydroxide is equivalent to 1.7
mg. of ammonia. Multiply the nvunber of cubic centimeters of N/io alkali
used by 1.7 and by 4 to get the number of milligrams of ammonia + amino-
acid nitrogen (expressed as ammonia) in 100 c.c. of the urine examined.

Amino-Acid Nitrogen

I. Henriques-Sorensen Formol Titration Method.- — Principle. —
A solution containing amino-acids is nearly neutral in reaction. If
formaldehyde be added, however, the following reaction takes place
with the formation of methylene derivatives which an more strongly acid
in reaction due to the destruction of the basic properties of the amino
groups. The carboxyl groups may then be titrated using phen-
olphthalein as an indicator.

R.CH.NH2

I + CH2O = R— CH— N: CH2 + H2O.

COOH I

COOH

The acidity as shown by the titration is a measure of the amount of
amino-acid nitrogen present. Ammonia likewise reacts with formalde-
hyde in a siinilar manner as is shown in the following equation:

4NH4Cl-h6CH20 = N4(CH2)6+6H20-f4HCl.

Hence the formol titration in the presence of ammonia gives results
which include both amino-acid and ammonia nitrogen. Ammonia

' Malfatti: Z. anal. Chem., 47, 273, 1908.

^Henriques and Sorensen: Zeit. physiol. chem., 64, 120, igog.

URIXE 503

may be determined and a correction applied, or the ammonia may be
removed by means of phosphotungstic acid. Phosphates also inter-
fere by obscuring the end-point and are removed by the addition of
barium salts.

It must be borne in mind that polypeptides and still more complex
protein derivatives likewise react with formol to a certain degree so
that the results do not strictly represent "amino-acid nitrogen."

The method is, with some modifications involving the preparation
of the solution to be titrated, applicable in the determination of amino-
acids in any medium, e.g., urine, protein digests, etc. When poorly
dissociated acids, e.g. some fatty acids, are present, these will in part
be included in the result and lead to values which are too high. Certain
of the amino-acids when present in large amounts will give erroneous
results, but in the ordinary urine or digest these errors are either
negligible or compensate each other. In the titration of colored solu-
tions the control solution which is necessary in this method must be
colored to correspond with the color of the unknown solution.

Procedure. — The determination of the amino-acids is carried out as follows :
The solution to be analyzed, if carbonates, phosphates and ammonia are absent,
is made neutral to litmus (paper) and the solution titrated with formalde-
hyde as below. 1 In case carbonates, phosphates or ammonia are present a
preliminary treatment is necessary which will vary according to the quantity
of ammonia present.

(a) For Small Amounts of Ammonia. — Applicable to most urines. Fifty
c.c. of the material under examination is pipetted into a 100 c.c. measuring
flask and i c.c. phenolphthalein solution- and 2 grams of solid barium chloride
are added; the whole is shaken, to saturate the solution with barium chloride;
saturated barium hydroxide solution is added until the red color of the phenol-
phthalein develops and then an excess of 5 c.c. is added. The flask is filled
to the graduation mark with water, shaken and permitted to stand for 15 minutes,
after which it is filtered through a dry filter. Eighty c.c. of the clear red filtrate
iwhich corresponds to 40 c.c. of the liquid under examination! are placed in
a 100 c.c. measuring flask, neutraUzed to Utmus and diluted to 100 c.c. with
freshly boiled water. Equal portions of this solution, 40 c.c. (equivalent to
16 c.c. of the original solution), may be taken for analysis, one for the formol
titration and the other for the determination of ammonia nitrogen.''

(b) For Large Amounts of Ammonia. — After the treatment with phenol-
phthalein, bariimi chloride, and barium hydroxide, and the solution has been
diluted to 100 c.c. as in (a) above, the ammonia is distilled off, in vacuo.*

' As a standard of comparison the litmus paper used for neutralization ii contrasted with
a similar piece dipped in a phosphate solution having a neutral reaction (M, 15 KHjPO^and
M/is NajHPO^).

^ A solution of 0.5 gram of phenolphthalein in 50 c.c. of alcohol and 50 c.c. of water.

'The determination of ammonia may be dispensed with in case a separate determina-
tion is made.

* For particulars with regard to the distillation, etc., see Henriques and Sorensen: Zeit.
physiol. Client., 64, 137, igog.

504 PHYSIOLOGICAL CHEMISTRY

In case the solution is deeply colored, as in protein digests, it may be neces-
sary to decolorize^ before the titration is attempted.

Final Titration. — For the final titration a volume of from 20-40 c.c. which con-
tains approximately 0.025 gram of nitrogen is the most desirable. A control
solution is run composed of an equal volume of boiled distilled water and 20 c.c.
of the formaldehyde mixture. ^ This control solution is colored^ so that its
tint matches that of the solution to be titrated.

To this control is added about half the volume of N '5 alkali which will be
used in the titration of the solution under investigation and it is then titrated
with N/5 acid to a faint red (first stage). ^

An additional drop of N/5 alkali is added, which imparts a distinct red to
the solution (second stage).

The solution to be analyzed is now titrated to the color produced in the
second stage of the control. The formaldehyde mixture is now added; 10 c.c.
for each 20 c.c. of the solution, and the mixture again titrated to the second
stage with N/5 alkaU.^

Two drops of the N/5 alkali are now added to the control solution which
assumes a deep red color (third stage). Fifth normal alkali is now added to
the solution under examination until it assumes a color corresponding to the
third stage of the control. This completes the titration.

Calculation. — The calculations are similar to those which pertain to any
acidimetry procedure. Each cubic centimeter of an N/5 alkali or acid solution
is equivalent to 0.0028 gram of nitrogen. An example will illustrate the pro-
cedure: 40 c.c. of solution (16 c.c. of urine) required 5.10 c.c. N/5 NaOH;
control, o.io c.c. N/5 NaOH; total required for amino-acids 5.00 c.c. equivalent
to 0.014 gram of nitrogen. Ammonia nitrogen in i6 c.c. of urine 0.007 gram N.
Then 0.014 — 0.007 = 0.007 gram amino-acid nitrogen in i6 c.c. of urine.

Interpretation. — The excretion of total amino-acid nitrogen by a
normal adult averages between 0.4 to i.o gram per day or from 2 to 6
per cent of the total nitrogen. Free amino-acid nitrogen (see Van
Slyke procedure) is considerably less than this, ordinarily 0.5 to i.o
per cent of the total nitrogen. The amount may be largely increased
in disorders associated with tissue waste as typhoid, in pronounced
atrophy of the liver, acidosis, etc.

2. Benedict-Murlin Modification.^ — Principle. — In this method the ammonia
is removed by means of phosphotungstic acid, and excess acid as well as carbonates
and phosphates carried down with barium.

^ For methods see Jessen-Hansen, Abderhalden's Arbeits Methoden, vol. 6, p. 202, 1912.

2 The formaldehyde solution is freshly prepared for each set of determinations as follows:
to 50 c.c. of commercial formaldehyde (formol) (30-40 per cent) add i c.c. of the phenol-
phthalein solution. N/5 alkali is then added until the mixture acquires a faint red color.
The volume of the formaldehyde used will vary with the volume of the solution to be ana-
lyzed; approximately 10 c.c. of the formalin solution are added for each 20 c.c. of the un-
known solution.

^ Solution of Bismark brown is very satisfactory for urines. Tropaeolin O, Tropaeolin
00, />-nitro-phenol, methyl orange or alizarin sulphonate, may be used.

* This procedure is recommended in order that the final volume of the control and the
unknown solutions shall be approximately the same when the process is complete.

' This is best accomplished by adding alkali until the color is deeper than that of the
control, then acid again until lighter and finally alkali to the desired color.

* Benedict and Murlin: Jour. Biol. Cheni., 16, 385, 1913.

URINE 505

Procedure. — Measure into a 500 c.c. Erlenmeyer flask 200 c.c. of a 24-hour
urine which has been diluted to 2000 c.c. (or its equivalent). Add an equal volume
of 10 per cent phosphotungstic acid (Merck) ^ in 2 per cent HCl. Let stand at least
three hours, better over night. Pour off 250 c.c. of the clear fluid, add i c.c. of a
0.5 per cent solution of phenolphthalein and then barium hydroxide in substance
until the whole fluid turns decidedly pink. The barium hydroxide should be added
a very little at a time. Let stand one hour. Filter off two 100 c.c. samples (=50
c.c. urine). Neutralize these samples to litmus (using good quality litmus paper)
with N/5 HCl. Add at once 10-20 c.c. of neutral formalin- and titrate cautiously
to a deep red color, i.e., until the drop produces no additional color with N/io
NaOH. Deduct from the result thus obtained the amount of N/io NaOH neces-
sary to produce the same depth of color in an equal quantity of water, freed from
carbon dioxide by boiling and cooling, and to which an equal volume of neutral
formalin has been added.

Calculation. — One c.c. of N/io NaOH is equivalent to 1.4 mg. of amino-acid
nitrogen. Multiply the number of cubic centimeters of N/io NaOH used (after
deducting for control as indicated above) by 1.4 and by 2 (as the equivalent of 50
c.c. of urine was used) to obtain the number of milligrams of amino-acid nitrogen
in 100 c.c. of the urine.

Interpretation. — See page 504.

3. Method of Frey-Gigon,^ — Principle. — The ammonia is removed from the
urine by aspiration after treatment with barium hydroxide and the formol titration
performed in the usual manner.

Procedure. — Treat 50 c.c. of urine in an aerometer cylinder such as used in the
Folin ammonia method, with 20 c.c. of saturated barium hydroxide solution and
15 c.c. of alcohol. Aspirate for two or three hours, using a slow current of air.
The ammonia is carried off. (It may be collected in standard acid solution and
determined as in the Folin method (see page 499) if desired.) Transfer the urine
mixture quantitatively to a 250 c.c. flask and make to mark with distilled water.
Shake well, allow to settle, filter. Take 100 c.c. of the filtrate and just neutralize
with N/5 hydrochloric acid, using rosolic acid as an indicator. Then to another
100 c.c. portion of the filtrate add an amount of the standard acid equal to that
added to the first portion. Next add 10 c.c. of neutral formalin solution, a few
drops of phenolphthalein and titrate in the usual manner to a red-violet color.
Calculate as in the preceding method.

The amino-acid nitrogen may also be appro.ximately determined by carr>'ing
out the titration for ammonia + and amino-acid nitrogen as given under Ammonia,
page 502, making a separate determination of ammonia, and subtracting the latter
result from the former.

4. Van Slyke's Method for Total Amino-Acid Nitrogen.*— Take 25 c.c. of
urine^ and mix with i c.c. of concentrated sulphuric acid and heat in an auto-
clave at 180° (oil bath temperature) for one and one-half hours. Transfer to a
50 c.c, flask and add 2 grams powdered calcium hydroxide. Shake thoroughly,
make up to 50 c.c. and filter through a dry folded filter. Transfer 20 c.c. of the

' Kahlbaum's preparation is a very different substance.

- To 50 c.c. commercial formalin solution (30-40 per cent) add i c.c. of phenolphthalein
solution and then N/s NaOH to a very faint pink color. The solution should be freshly
prepared.

•' Prey and Gigon: Biochem. Zeil., 22, 309, 1909.

* Van Slyke: Jour. Biol. Chcm., 16, 125, 1913.

'See (Van Slyke: Proc. Soc. Exp. Biol, and Med., 13, 63, 1915) for treatment of urines
containing glucose or albumin.

5o6 PHYSIOLOGICAL CHEMISTRY

filtrate to a Jena glass evaporating dish and concentrate to dryness on the water-
bath. This requires about half an hour. The residue is moistened with i c.c.
of 50 per cent acetic acid to bring the calcium hydroxide and carbonate into
solution, and is then washed into a 10 c.c. flask and filled up to the mark. One
can use the entire solution for determination of the amino -nitrogen in the large
amino -apparatus, or use 2 c.c. portions for the micro -apparatus. (See Van
Slyke Apparatus, Figs. 34 and 35, p. 88 in Chapter IV on Proteins.)

The length of time which the nitrous acid solution should be shaken in order
to drive off all the amino-nitrogen depends somewhat on the temperature.
When the latter is 15-20° the time should be five to four minutes; for §0-25° it
is three minutes, for 25-30°, two and a half to two minutes. It is preferable
that the solution should be shaken vigorously with a motor and the time kept
down to these limits, for the sake not only of rapidity but of accuracy.

Van Slyke's Method for Free Amino-Acid Nitrogen. — To 25 c.c. of urine^
in a 50 c.c. flask add urease solution and allow to stand for one and one-half
times the interval which has been found necessary to effect the maximimi de-
composition of urea, as observed by titration of the ammonia. The last traces
of urea are decomposed. At the end of the digestion period 10 c.c. of a 10 per
cent suspension of calcium hydroxide are added, the mixture shaken and made
up to 50 c.c. Then filter, evaporate, and complete the determination according
to the method outhned under total amino-acid nitrogen, above.

Creatinine

Folin's Colorimetric Method. — Principle.- — This method is based
upon the characteristic property possessed by creatinine, of yielding a
certain definite color-reaction in the presence of picric acid in alkaline
solution.

Procedure. — Place 10 c.c of urine in a 500 c.c. volxometric flask, add 15 cc. of a
saturated solution of picric acid and 5 c.c. of a 10 per cent solution of sodium hy-
droxide, shake thoroughly and allow the mixture to stand for five minutes. During
this interval pour a little N/2 potassiimi bichromate solution^ into each of the two
cylinders of the colorimeter (Duboscq's, see Fig. 153, p. 486) and carefully adjust
the depth of the solution in one of the cylinders to the 8 mm. mark. A few prelimi-
nary colorimetric readings may now be made with the solution in the other cylinder,
in order to insure greater accuracy in the subsequent examination of the solution of
unknown strength. Obviously the two solutions of potassium bichromate are
identical in color and in their examination no two readings should differ more than
0.I-0.2 mm. from the true value (8 mm.). Four or more readings should be made
in each case and an average taken of all of them exclusive of the first reading, which
is apt to be less accurate than the succeeding readings. In time as one becomes
proficient in the technic it is perfectly safe to take the average of the first two
readings.

At the end of the five-minute interval already mentioned, the contents of the
500 c.c. flask are diluted to the 500 c.c. mark, the bichromate solution is thoroughly
rinsed out of one of the cyclinders and replaced with the solution thus prepared and
a number of colorimetric readings are immediately made.

1 See note 5, page 505.

''This solution contains 24.55 grams of potassium bichromate to the liter A pure
creatinine standard is to be preferred, see p. 507.

URINE 507

Ordinarily 10 c.c. of urine is used in the determination by this method, but if
the content of creatinine is above 15 mg. or below 5 mg. the determination should
be repeated with a volume of urine selected according to the content of creatinine.
This variation in the volume of urine according to the content of creatinine is quite
essential, since the method loses in accuracy when more than 15 mg. or less than
5 mg. of creatinine is present in the solution of unknown strength.

Calculation. By experiment it has been determined that 10 mg. of pure crea-
tinine, when brought into solution and diluted to 500 c.c. as explained in the above
method, yields a mixture 8.1 mm. of which possesses the same colorimetric value
as 8 mm. of a N/ 2 solution of potassium bichromate. Bearing this in mind the
computation is readily made by means of the following proportion in which y repre-
sents the number of millimeters of the solution of unknown strength equivalent to
the 8 mm. of the potassiimi bichromate solution :

y :8.i : : 10 : X (mg. of creatinine in the quantity of urine used).

This proportion may be used for the calcvdation no matter what volvune of
urine (5, 10, or 15 c.c.) is used in the determination. The 10 represents 10 mg. of
creatinine which gives a color equal to 8.1 mm., whether dissolved in 5, 10, or 15 c.c.
of fluid.

Calculate the quantity of creatinine in the 24-hour urine specimen.

Interpretation. — The daily excretion of creatinine by an adult of
medium weight averages about 1^:4 grams. The value is nearly con-
stant from day to day for a given individual being influenced by the diet
hardly at all unless this contains much preformed creatinine (as in case
of a heavy meat diet) . The excretion of creatinine is to a certain extent
a measure of muscular efficiency and of the amount of active muscle
tissue in the body. Relative to body weight less creatinine is excreted
by obese persons.

Creatinine excretion is decreased in disorders associated with mus-
cular atrophy and muscular weakness. It increases with increased
tissue cetabolism as in fever.

By the "creatinine coefl&cient" is meant the number of milligrams
of creatinine — ////rogc« excreted daily per kilo of body weight. This
varies under normal conditions from 7-1 1.

Use of Pure Creatinine Standards. — Instead of using as a standard a potassium
dichromate solution as above indicated, a solution of pure creatinine is to be recom-
mended. By using this certain arbitrary factors are eliminated and the method
becomes of more general applicability. The standard need not be set at a definite
mark as is necessary in the case of dichromate and temperature and time have less
inlluence on the accuracy of the results. A stock solution of pure creatinine (made
according to Benedict's directions; see Chapter XXII on Physiological Constituents
of Urine) is made by dissolving i gram of the substance in sutVicient N/ 10 HCl to
make a liter. This solution contains i mg. of creatinine per cubic centimeter. In
carrying out the determination treat 10 c.c. of the stock solution in the same \vay and
at the same time as the 10 c.c. sample of urine. Compare in the colorimeter. The
calculation s simple. The reading of the standard divided by the reading of the

5o8 PHYSIOLOGICAL CHEMISTRY

urine gives directly the number of milligrams of creatinine per cubic centimeter of
urine.

Folin's Microchemical Modification.' — Principle. — The principle is the same
as that of the original colorimetric method (see page 506). This procedure is to be
recommended particularly where only small amounts of material are available.

Procedure. — One c.c. of the standard creatinine (see above) solution (i mg. per
c.c.) is measured into a 100 c.c. volumetric flask and i c.c. of urine into another;
20 c.c. of saturated picric acid solution (measured with a cylinder) are added to
each and then 1.5 c.c. of a 10 per cent solution of sodium hydroxide. At the end
of ten minutes the flasks are fiUed up to the mark with tap water and the color
of the unknown is determined. The reading of the standard divided by the
reading of the unknown gives directly the number of milligrams of creatinine in
the amount of urine taken for analysis.

3. Shaffer's Modification for the Determination of Creatinine in Very Dilute
Solutions. 2 — The regular Folin procedure is not accurate when applied to urines
containing less than 20 mg. of creatinine per 100 c.c. By a slight modification it
becomes applicable to creatinine solutions containing as little as i mg. or less per
100 c.c.

Procedure. — To the solution under examination add an equal volume of satu-
rated picric acid solution and one-tenth this volume of 10 per cent sodium hydroxide
solution. After standing 6-10 minutes the liquid is diluted to a definite volume
depending upon the intensity of the color developed. With very dilute solutions
one may add solid picric acid equivalent to half saturation (0.6 per cent) and when
dissolved, one-twentieth the volume of sodium hydroxide. Provided the creatinine
solution itself has not sufficient color to interfere, the results by this method appear
to be as accurate as the original procedure. The colorimetric readings and calcu-
lations are made in the same way as in the preceding methods.

Creatine

Folin-Benedict Method.^ — Principle. — Creatinine on boiling with
acid is transformed into creatinine. By determining the content of
creatinine before and after the acid treatment we are able to calculate
the amount of creatinine originally present in the urine. The Folin
colorimetric method (page 506) is used for determining the creatinine
in both cases. The method is not applicable to diabetic urines.

Procedure. — Introduce into a small flask or beaker 10 c.c. of the urine to
be examined. (If 10 c.c. contains more than 12 or less than 7 mg. of total
creatinine use a correspondingly smaller or larger volmne of urine.) Add from
10-20 c.c. of normal HCl, and a pinch or two of powdered or granulated lead.
Boil the mixure over a free flame as slowly or as rapidly as may be desired, until
very nearly down to dryness, when the heating should be continued to dryness
either on the water-bath or very easily by simply holding the vessel in the hand
and heating carefully for a moment or two. Let the residue stand on the water-
bath for a few minutes until most of the excess of hydrochloric acid gas has been

' Folin: Jour. Biol. Client., 17, 469, 1914.
-Shaffer: Jour. Biol. Chem., 18, 525, 1914.
^Benedict: Jour. Biol. Chem., 18, 191, 1914.

URINE 509

expelled, after which dissolve it in about 10 c.c. of hot water and rinse the solu-
tion quantitatively through a plug of cotton or glass wool (to remove aU metallic
lead) into a 500 c.c. volumetric flask. Add 20-25 c.c. of a saturated picric acid
solution and about 7-8 c.c. of a 10 per cent NaOH solution, which contains 5
per cent of Rochelle salt.' At the end of five minutes fill to the mark with water
and read in the colorimeter just as in the case of creatinine (see page 5061.

Calculation. — Calculate the creatinine content of the solution in the same
manner as given under Creatinine fpage 507 ) . From the value thus obtained sub-
tract the value for the creatinine content of the urine before dehydration. The
difference will be the creatine content of the original urine in terms of creatinine.

Interpretation. — Creatine occurs only in very small amounts in the
urine of normal adults, but is found in larger amounts in that of children
(10 to 56 mg. per day). Creatine ingestion in adults has little effect
on the urinary excretion. In fasting, the amount is markedly increased
(it may amount to 100 mg. or more per day). Creatine also appears
in the urine after high water ingestion. It is found in many pathological
conditions associated with malnutrition and disintegration of muscular
tissue, in fever, etc. Very large amounts have been found in cases of
carcinoma of the liver.

2. Folin -Benedict and Myers Method. ^ — To 20 c.c. of urine in a 50 c.c. volu-
metric flask, add 20 c.c. of normal hydrochloric acid and place the flask in an auto-
clave at a temperature of 117-120° C. for one-half hour. Add distilled water until
the volume of the acid-urine mixture is exactly 50 c.c, close the flask by means of
a stopper, and shake it thoroughly. Approximately neutralize 25 c.c. of this mix-
ture, introduce it into a 500 c.c. volumetric flask and determine its creatinine con-
tent according to Folin's Colorimetric Method (see page 506).

For calculation and interpretation see the foregoing method.

3. Method of Folin. ^ — Water-hath Procedure. — Heat 10 c.c. of urine with 5 c.c.
of normal hydrochloric acid on the boiling water-bath or at 90°C. for three hours.
The creatine is transformed into creatinine. Some darkening takes place but this
does not interfere because of the subsequent dilution. The mixture is made up to
50 c.c, 25 c.c. of this is taken, neutralized, and creatinine plus creatine determined
just as in the case of creatinine alone. The creatine is obtained by difi^erence.
This procedure may be used for diabetic urines which is not the case with the auto-
clave procedure nor with the Benedict modification. It is perhaps not quite so
accurate as the autoclave procedure.

4. Microchemical Modification of Folin.* — By greatly diluting the urine the
time required for the conversion of creatine to creatinine is decreased, and picric
acid can be substituted for mineral acid.

Procedure. — Enough urine to give 0.7-1.5 mg. of creatinine is measured into
a weighed Erlenmeyer Jena flask (capacity 200 c.c); 20 c.c. of saturated picric acid
solution, about 130 c.c. of water, and a few very small pebbles to promote even
boiling are added and the mixture is gently boiled, preferably over a micro-burner

' The Rochelle salt should be present to prevent any formation of turbidity, which
otherwise may occur, due to the presence of traces of dissolved lead.
- Benedict and ^Iyers: -Iw. .T . Phys., 18, 397, 1907.
^ Folin: Zeilscttr, f. physiol. Ckem., 41, 222, 1904.
* Folin: Jour. Biol. Clum., 17, 469, 1914.

lO PHYSIOLOGICAL CHEMISTRY

for about one hour. At the end of this time the heat is increased and the solution
is boUed down to rather less than 20 c.c. The flask is transferred to the scales
and enough water is added to make the total solution equal to 20-25 grams. The
solution is cooled in running water, 1.5 c.c. of 10 per cent sodium hydroxide are
added, and the total creatinine is determined as in the preformed creatinine deter-
mination using I mg. of creatinine as a standard. The method has been found to
give good results in the presence of glucose and other sugars.

Morris^ has suggested that in the case of diabetic urines the total creatinine
be determined after precipitation of the creatine and creatinine with picric acid.
The method is not recommended as a regular procedure.

Uric Acid

I. Microchemical Colorimetric Method. — Benedict and Hitchcock
Modification of the Folin-Macallmn-Denis Procedure. — The principle
of the method depends upon the fact, first noted by FoHn and Macallum^
and further investigated by Folin and Denis, ^ that uric acid gives, with
phosphotungstic acid and alkali, a deep blue color the depth of which is
proportional to the amount of uric acid present. Since certain other
substances present in urine produce a similar blue color with the phos-
photungstic acid, it is necessary to separate the uric acid from them.
This is accomplished by precipitation as the silver salt. The silver
urate is subsequently dissolved and treated with the uric acid reagent.

Benedict and Hitchcock'* have examined the method of Folin and
Denis and have suggested a number of important modifications.

Procedure. — Measure such an amount of urine as will contain from 0.7
to 1.3 mg. of uric acid (2 to 4 c.c. is usually the correct amount) into a centrifuge
tube, dilute with water to about 5 c.c, and add 15 to 20 drops of an ammoniacal
silver magnesiiun solution.^ Mix the contents of the tube with a small stirring
rod and centrifuge the tube for one or two minutes. Pour off the supernatant
liquid, as completely as possible, by inverting the tube, allowing it to drain a
moment, and then touching the inside of the lip of the tube with a towel or piece
of filter paper. Add to the residue in the tube two drops of a 5 per cent solution
of potassium cyanide to dissolve the silver urate, stir the mixture thoroughly
with a thin rod, for half a minute, add a few drops (0.5 to i.o c.c.) of water, and
stir again. ^ Two c.c. of the uric acid reagent^ are added and the mixture stirred

^ Morris: Jour. Biol. Chetn., 21, 201, 1915.

2 Folin and Macallum: /. Biol. Chem., 13, 363, 1912.

^ Folin and Denis: J. Biol. Client., 14, 95, 1913; ibid., 13, 469, 1913.

"• Benedict and Hitchcock: /. Biol. Chem., 20, 619, 1915; Benedict: ibid., 20, 629, 1915.

*This solution has the following composition:

3 per cent silver lactate solution 70 c.c.

M agnesia mixture 30 c.c.

Concentrated ammonium hydroxide solution 100 c.c.

' At this point perfectly clear solutions are obtained with pure uric acid solutions in phos-
phate mixture or in pyridin. With urines some magnesium ammonium phosphateisprecipi-
tated with the uric acid, which does not dissolve in the cyanide. After adding the two
subsequent reagents, however, a perfectly clear solution is obtained.

' Preparation of the Uric Acid Reagent. — Place 100 grams of sodium tungstate, 80 c.c.
of 85 per cent phosphoric acid, and 750 c.c. of distilled water in a liter flask. Boil the mix-
ture with a reflux condenser for two hours, cool and dilute to i liter, filtering if necessary.

URINE 5 1 1

again, after which add lo c.c. of 20 per cent sodium carbonate solution/ transfer
quantitatively to a 50 c.c. flask, and at the end of about one-half minute, dilute
to mark. Compare this solution in the Duboscq colorimeter ipage. 4861 with a
simultaneously prepared solution obtained by treating 5 c.c. of the standard uric
acid solution,- contained in a 50 c.c. flask, with 2 drops of the potassium cyanide
solution, 2 c.c. of the uric acid reagent, 10 c.c. of 20 per cent sodium carbonate solu-
tion, and diluting to the mark at the end of about one-half minute. The stand-
ard solution is best set at a height of 15 mm. in the colorimeter.

Calculation. — The reading of the standard divided by the reading of the urine
gives the number of miUigrams of uric acid in the amount of sample taken.

Interpretation. — For adults on a mixed diet the average excretion of
uric acid is about 0.7 gram. It arises from the purines of ingested food
(exogenous uric acid) and from purines derived from the body tissues
by disintegration of nuclein material (endogenous uric acidj. Exog-
enous uric acid depending entirely upon the diet is greatly increased
by the ingestion of purine-rich foods (meat, liver, sweetbreads, etc.) and
reduced to a very low level on purine-free foods, e.g., milk, eggs, etc.
(see Chapter XXVII). Endogenous uric acid is influenced by exercise
and by the diet (protein foods particularly giving rise to increases).
It appears to be partly the result of gastro-intestinal secretory activity.
On a purine-free diet the average excretion is 0.1-0.5 gram. On a high
purine diet the uric acid output may be 2 grams per day.

In gout the uric acid content of the urine is low preceding an attack
and increases during the attack, this fall and rise being more or less
characteristic. The excretion rises after atophan administration ap-
parently due to increased kidney activity. In leukemia the excretion
is extremely high due to nuclear destruction. The uric acid content
of the urine is of importance in relation to the formation of uric acid
calculi. The administration of alkali carbonates and citrates by de-
creasing the acidity of the urine increases its solvent power for uric
acid, and decreases the liability of the formation of this type of calculus.

3. Folin-Shailer Method.^ — Principle. — The uric acid is precipitated
as ammonium urate by the addition of ammonia, the precipitate filtered
off, washed and titrated with potassium permanganate. A preliminary

1 Sodium Carbonate Solution. — Dissolve 200 grams of anhydrous sodium carbonate in
warm water and make up to i liter.

-Standard Uric Acid Solution. — The solution of uric acid in phosphate solution is very
readily prepared, does not need to be standardized, and appears to keep indefinitely. It is
prepared in the following manner. Dissolve 9 grams of pure crystallized disodium hydro-
gen phosphate, together with i gram of crystallized sodium dihydrogen phosphate, in 200
to 300 c.c. of hot water, and tilter if the solution is not perfectly clear. Make this
filtrate up to about 500 c.c. with hot wafer, and pour this hot or warm (and perfectly clear)
solution upon exactly 200 mg. of pure uric acid suspended in a few cubic centimeters of
water in a liter volumetric flask. Agitate the mixture for a few minutes until the uric acid
completely dissolves. Cool, add exaclly 1.4 c.c. of glacial acetic acid, dilute lo the mark,
and mix. Add about 5 c.c. of chloroform to prevent the growth of bacteria or moulds in the
solution. Five c.c. of this solution contains exactly i mg. of uric acid.

' Folin and Shaffer: Zcil. physiol. Chcm., 32, 552, 1901.

512 PHYSIOLOGICAL CHEMISTRY

treatment with an ammonium sulphate-uranium acetate solution is for
the purpose of removing interfering organic substances. The method
gives accurate results.

Procedure. — Introduce loo c.c.^ of urine into an Erlenmeyer flask, add
25 c.c. of the Folin-Shafifer reagent- and after shaking the flask to thoroughly
mix the fluids allow the mixtiire to stand," with or without further stirring, until
the precipitate has settled (^5-10 minutes). Filter, transfer 100 c.c. of the filtrate
to a 200 c.c. Erlenmeyer flask, add 5 c.c. of concentrated ammonimn hydroxide
and allow the mixture to stand for 24 hours. Transfer the precipitated ammo-
niiun urate quantitatively to a filter paper, ^ using 10 per cent ammoniimi sulphate
to remove the final traces of the urate from the flask. Wash the precipitate
approximately free from chlorides by means of 10 per cent ammonium sulphate
solution,^ remove the paper from the fvmnel, open it, and by means of hot water
rinse the precipitate back through the fvuinel into the flask in which the urate
was originally precipitated. The volmne of fluid at this point should be about
100 c.c. Cool the solution to room temperature, add 15 c.c. of concentrated
sulphuric acid and titrate at once with N/20 potassium permanganate, K2Mn208,
solution. The first tinge of pink color which extends throughout the fluid after
the addition of two drops of the permanganate solution, while stirring with a
glass rod, should be taken as the end-reaction. Take the burette reading and
compute the percentage of uric acid present in the urine under examination.

Calculation. — Each cubic centimeter of N/20 potassium permanganate solu-
tion is equivalent to 3.75 mg. (0.00375 gram) of uric acid. The 100 c.c. from
which the ammonivmi urate was precipitated is equivalent to only four -fifths
of the 100 c.c. of urine originally taken; therefore we must take five-fourths of
the burette reading in order to ascertain the nvmiber of cubic centimeters of the
permanganate solution required to titrate 100 c.c. of the original urine to the correct
end point. If y represents the nvmiber of cubic centimeters of the permanganate
solution required, we may make the following calculation :

yXo. 00375 = weight of uric acid in 100 c.c. of urine.

Because of the solubility of the ammonitun urate a correction of 3 mg. should
be added to the final result.

Calculate the quantity of uric acid in the 24-hour urine specimen.

4. Heintz Method. — This is a very simple method and was the first one in
general use for the quantitative determination of uric acid. It is less accurate than
the metBods just described. The procedure is as follows: Place 100 c.c. of filtered
urine in a beaker, add 5 c.c. of concentrated hydrochloric acid, stir the fluid thor-
oughly, and stand it away in a cool place for 24 hours. Filter off the uric acid
crystals upon a washed, dried and weighed filter paper and wash them with cold
distilled water, a few cubic centimeters at a time, until the chlorides are removed.

^ It is preferable to use more than 100 c.c. of urine if the fluid has a specific gravity less
than 1 .020.

^ The Folin-Shaflfer reagent consists of 500 grams cf ammonium sulphate, 5 grams of
uranium acetate and 60 c.c. of 10 per cent acetic acid in 650 c.c. of distilled water.

' The mixture should not be allowed to stand for too long a time at this point, since uric
acid may be lost through precipitation.

* The Schleicher and Schiill hardened papers or the Baker and Adamson washed, ashless
variety are very satisfactory for this purpose.

* This washing may be conveniently done by decantation if desired, thus retaining the
major portion of the precipitate in the flask.

URINE

513

Purine Bases

Now wash, in turn, with alcohol and with ether and finally dry the paper and
tals to constant weight at iio°C. In the process of washing the uric acid free
chlorides an error is introduced, since every cubic centimeter of
water so used dissolves 0.00004 gram of uric acid.^ For this rea-
son a correction is necessary. It has been suggested that the pig-
ment of the crystals is equivalent in weight to the amount of uric
acid dissolved by the first 30 c.c. of water, and this factor should be
taken into account in the computation of the percentage of uric
acid.

Calculation. — Since 100 c.c. of urine was used the corrected ,
weight of the uric acid crystals, in grams, will express the percentage \
of uric acid present. 1

5. Kriiger-Schmidt Method. — Kriiger and Schmidt have de- j
vised a method for the combined determination of uric acid and {
the other purine bodies of urine. This procedure is described under !
Purine Bases, below. A modification of this method by Hunter
is also given.

6. Ruhemann's Uricometer Method. — Principle. — When iodine
solution is added to urine an amount of iodine is absorbed roughly
proportional to the amount of the uric acid present. A special grad-
uated tube is required and carbon disulphide is used to indicate the
presence of excess iodine.

Procedure. — Fill the tube (see Fig. 165) to the lowest mark S
with carbon disulphide (the bottom of the meniscvis should rest
on the line). Then add iodine solution (1.5 grams iodine, 1.5
grams potassium iodide, 15 grams absolute alcohol, and 185 grams
distilled water) to the mark J. Add urine to mark 2.45 (2.6 c.c).
Insert the glass stopper and shake. The carbon disulphide will
show the dark brown color of iodine. Add more urine gradually
with continued shaking untU only a violet-pink color remains in the
disulphide after shaking. Then add drop by drop with vigorous
shaking until the disulphide becomes colorless. Read on the scale
the amount of uric acid in parts per thousand of urine.

When the uric acid content of the urine is low this method
gives reasonably accurate results from the cUnical standpoint. -
At a level of 0.3 gram per day the probable error will not exceed
10-15 per cent. Above i gram no limit can safely be placed on
the degree of error in pathological cases especially where albumin,
diacetic acid, purine bases and certain drugs are likely to be present.
The results by this method are ordinarily high.

crys-
from

ox in*

o.in

0.178
0.181
O.IM
O.tST
0.190
0.198
0.196
0.199
0.202
0.20»
0.208
0.211
0315
0.219
0.221
0.225
0.228
fl.23l
fl.235
0.238
0.M2
0.245
0.249

o.nt

026
0.28

Fig. 165. —
Ruhemann's
Uricometer.

I. Kriiger and Schmidt's Method. — Principle. — This
method serves for the determination of both uric acid
and the purine bases. The principle involved is the precipitation of
both the uric acid and the purine bases in combination with copper

1 His and Paul: Zeit. physiol. Chcrn., 31, i, 1900.

* Bradley and Bunta: Jour. Am. Med. Assn., Jan. 4, 1913.

33

514 PHYSIOLOGICAL CHEMISTRY

oxide and the subsequent decomposition of this precipitate by means
of sodium sulphide. The uric acid is then precipitated by means of
hydrochloric acid and the purine bases are separated from the filtrate
in the form of their copper or silver compounds. The nitrogen content
of the precipitates of uric acid and purine bases is then determined
by means of the Kjeldahl method (see page 483) and the correspond-
ing values for uric acid and purine bases calculated.

Procedure. — To 400 c.c. of albumin-free urine^ in a liter flask-, add 24
grams of sodixun acetate, 40 c.c. of a solution of sodium bisulphite^ and heat
the mixtiire to boiling. Add 40-80 c.c.^ of a 10 per cent solution of copper sul-
phate and maintain the temperature of the mixture at the boiling-point for at
least three minutes. Filter off the flocculent precipitate, wash it with hot
water until the wash water is colorless, and return the washed precipitate to
the flask by pimcturing the tip of the filter paper and washing the precipitate
through by means of hot water. Add water imtil the volume in the flask is
approximately 200 c.c, heat the mixture to boiUng and decompose the precipi-
tate of copper oxide by the addition of 30 c.c. of sodium sulphide solution.*
After decomposition is complete, the mixture should be acidified with acetic
acid and heated to boiling imtil the separating sulphur collects in a mass.
Filter the hot flmd by means of a filter-pump, wash with hot water, add 10
c.c. of 10 per cent hydrochloric acid and evaporate the filtrate in a porcelain
dish imtil the total volume has been reduced to about 10 c.c. Permit this
residue to stand about two hours to allow for the separation of the uric acid,
leaving the purine bases in solution. Filter off the precipitate of uric acid,
using a small filter paper, and wash the uric acid, with water made acid with
sulphuric acid, until the total volume of the original filtrate and the wash water
aggregates 75 c.c. Determine the nitrogen content of the precipitate by means
of the Kjeldahl method (see page 483), and calculate the uric acid equivalent.^

Render the filtrate from the uric acid crystals alkaline with sodium hydroxide,
add acetic acid until faintly acid and heat to 7o°C. Now add i c.c. of a 10 per
cent solution of acetic acid and 10 c.c. of a suspension of manganese dioxide^
to oxidize the traces of uric acid which remain in the solution. Agitate the mix-
ture for one minute, add 10 c.c. of the sodium bisulphite solution^ and 5 c.c.
of a 10 per cent solution of copper sulphate and heat the mixture to boiling for

' If albumin is present, the urine should be heated to boiling, acidified with acetic acid,
and filtered.

2 The total volume of urine for the 24 hours should be suflaciently diluted with water to
make the total volume of the solution 1600-2000 c.c.

* A solution containing 50 grams of Kahlbaum's commercial sodium bisulphite in 100
c.c. of water.

* The exact amount depending upon the content of the purine bases.

'This is made by saturating a i per cent solution of sodium hydroxide with hydrogen
sulphide gas and adding an equal volume of i per cent sodium hydroxide.

Ordinarily the addition of 30 c.c. of this solution is sufficient, but the presence of an
excess of sulphide should be proven by adding a drop of lead acetate to a drop of the solution.
Under these conditions a dark brown color will snow the presence of an excess of sodium
sulphide.

'This may be done by multiplying the nitrogen value by three and adding 3 J^ mg.
to the product as a correction for the uric acid remaining in solution in the 75 c.c.

^ Made by heating a 0.5 per cent solution of potassium permanganate with a little alco-
hol until it is decolorized.

* To dissolve the excess of manganese dioxide.

URINE

:)i:>

three minutes. Filter off the precipitate, wash it with hot water, and determine
its nitrogen content by means of the Kjeldahl method (see page 483). Inas-
much as the composition and proportion of the purine bases present in urine is
variable, no factor can be appUed. The result as regards these bases must
therefore be expressed in terms of nitrogen.

Benedict and Saiki' report cases in which the total purine nitrogen by this
method was less than the uric-acid nitrogen as determined by the Fohn-Shaffer
method. The inaccuracy was found to he in the Kxiiger and Schmidt method.
To obviate this they advise the addition of 20 c.c. of glacial acetic acid for each
300 c.c. of urine employed, the acid being added before the first precipitation.

Interpretation. — The amount of purine bases excreted by a normal
man is small and variable. Values from 16-60 mg. have been found.
The purine base nitrogen is of course only a fraction of this. The
amount excreted is influenced by the diet somewhat in the same way
as is the excretion of uric acid being also increased in disorders asso-
ciated with increased uric acid excretion such as leukemia. The purine
bases form a higher percentage of the total purine excretion in the case
of the monkey, sheep, and goat than in the case of man.

2. Hunter and Givens' Modification of Kriiger-Schmidt Method. ^ —
Principle. — The Kriiger-Schmidt process is combined ^\dth the micro-
chemical colorimetric method for uric acid (see page 510).

Procedure. — The first copper-purine precipitate as obtained in the Kriiger-
Schmidt procedvu'e is suspended in about 200 c.c. of water, to which there is
added about i c.c. of concentrated hydrochloric acid. The mixture is vigorously
boiled, whereupon the whole or greater part of the precipitate goes into solution.
Removal of the copper is effected by treatment with hydrogen sulphide in the heat,
and excess of the sulphide is completely expelled by renewed boihng. Filtration
under suction, and thorough washing of flask and filter result in a filtrate which
is perfectly clear and nearly colorless. This is concentrated if necessary, and
made up to a convenient volume which must of course be sufficiently large to
retain, when cool, the uric acid in solution. Of this an aUquot part is utihzed
directly for the colorimetric determination of uric acid. In the remainder the
residual luic acid is destroyed and bases determined according to the regular
Kriiger-Schmidt procedure. This modification is recommended particularly
where the amount of uric acid present is minute.

3. Welker's Modification of the Methods of Amstein and of Salkowski.^ —
Principle. — The phosphates are removed by treatment with magnesia mixture.
The purine bases and uric acid are then thrown down as their silver salts and the
nitrogen content of this precipitate determined.

Procedure. — Four hundred c.c. of urine, free from protein, are treated with
100 c.c. of magnesia mixture and 600 c.c. of water. This is then filtered and of the
clear filtrate a measured quantity (600-800 c.c. )is treated with an excess (10 c.c.)
of a 3 per cent silver nitrate solution. Concentrated ammonium hydroxide is
added in small quantities, with stirring, until all the chlorides have dissolved.

1 Benedict and Saiki: Jour. Biol. Chem., 7, 27, 1909.
^Hunter and Givens: Jour. Biol. Chem., 17,37, 1914.
^ Dittman and Welker: Xew York Med. Jour., May-June, 1909.

5l6 PHYSIOLOGICAL CHEMISTRY

Allow the flocculent precipitate of the silver purine compounds to settle to the
bottom, then pass the supernatant liquid through the filter before disturbing the
precipitate. Finally transfer the precipitate quantitativelj' to the paper which
must be of known nitrogen content. The precipitate is washed with dilute (i per
cent) ammonium hydroxide. The paper with the precipitate is then transferred
to a Kjeldahl flask and about loo c.c. of water and a small quantity (about o.i
gram) of magnesium oxide are added. The water is then boiled until all the am-
monia has been driven off. Test the steam with litmus paper.

The material in the flask is then digested by means of the usual Kjeldahl method
(see page 483). The digestion must be watched carefully at the time the sulphuric
acid reaches sufficient concentration to affect the filter paper, inasmuch as the SO2
produced causes considerable frothing. The total nitrogen (purine base, uric acid
and filter-paper nitrogen) is now determined in the usual way (see Kjeldahl Method,
page 483). This result minus the uric acid and filter-paper nitrogen will give the
figure for the purine-base nitrogen.

4. Salkowski's Method. — Principle. — The purin bases and uric acid are pre-
cipitated as silver-magnesium salts, these compounds decomposed with hydrogen
sulphide, and the uric acid precipitated by means of sulphuric acid. The purin
bases in the filtrate are again precipitated as their silver salts and the silver content
■of the precipitate determined after ignition by titration with thiocyanate.

Procedure. — Place 400-600 c.c. of protein-free urine in a beaker. Introduce
into another beaker 30-50 c.c. of an ammoniacal silver nitrate solution^ wih 30-50
•c.c. of magnesia mixture,^ add some ammonium hydroxide and if necessary some
ammonium chloride to clear the solution. Now add this solution to the urine,
stirring continually with a glass rod, and allow the mixture to stand for one-half
hour. Collect the precipitate on a filter paper, wash it with dilute ammonium
hydroxide, and finally wash it back into the original beaker. Suspend the precipi-
tate in 600-800 c.c. of water, add a few drops of hydrochloric acid and decompose
it by means of hydrogen sulphide. Now heat the solution to boiling, filter while
hot and evaporate the filtrate to dryness on a water-bath. Extract the residue
with 20-30 c.c. of hot 3 per cent sulphuric acid and allow the extract to stand 24
hours. Filter off the uric acid, wash it, make the filtrate ammoniacal and precipitate
the purine bases again with silver nitrate. Collect this precipitate on a small-sized
chlorine-free filter paper, wash, dry, and incinerate it in the usual manner. Now
dissolve the ash in nitric acid and titrate with ammonium thiocyanate according to
the Volhard-Arnold method (see page 556). Calculate the content of purine bases
in the urine examined, bearing in mind that in an equal mixture of the silver salts
of the purine bases, such as we have here, one part of silver corresponds to 0.277
gram of nitrogen or to 0.7381 gram of the bases.

For interpretation see page 515.

Purine Nitrogen

Hall's Purinometer.' — By means of the instrument shown in Fig. 166, urine
may be examined for total purine nitrogen, i.e., nitrogen in the form of purine bases,

^ Prepared by dissolving 26 grams of silver nitrate in about 500 c.c. of water, adding
enough ammonium hydroxide to redissolve the precipitate which forms upon the first addi-
tion of the ammonia and making the balance of the mixture up to i liter with water.

^ Directions for preparation may be found on p. 602.

2 Hall: The Purine Bodies, Philadelphia, 1904.

URINE

517

urates and uric acid. The method does not give an absolutely accurate measure
of the purine values. It is, however, of considerable service clinically. The
principle of the method is the preliminary precipitation of
the phosphates present followed by the precipitation of the
purine bodies in the form of their silver compounds by means
of an ammoniacal silver nitrate solution. The volume of this
silver precipitate is then determined and its nitrogen value
interpolated by means of a table of equivalent values.

Procedure. — Collect the 24-hour urine and mix it
thoroughly. Take 100 c.c. of the urine and if albumin is
present make slightly acid with acetic acid and boil and filter.
Close the stopcock of the instrument and introduce 90 c.c.
of urine and 20 c.c. of a modified magnesia mixture.* Turn
the stopcock and permit the precipitated phosphates to pass
into the lower chamber of the instrument. After an interval
of ten minutes has elapsed the stopcock should be closed
and sufficient ammoniacal silver nitrate solution^ added to
make the total volume in the upper chamber 100 c.c. The
precipitate of the silver compounds of the purine bodies
should be pale yellow, Anj^ silver chloride present may be
brought into solution in the strong ammoniacal solution by
the repeated inversion of the purinometer. In case the
chloride does not dissolve it should be brought into solution
by the addition of further ammonium hydroxide. Place the
purinometer in a dark room for 24 hours and at the end of
this time read the volume of the purine precipitate. Inter-
polate the value in terms of purine nitrogen by means of the following table:

Fig. 166. — H.a.ll's
Purinometer.

Precipitate, Purine nitrogen,

c.c. per cent

(grams in 100 c.c.)

4 0.007S

5 0.0097

6 0.0117

7 0.0136

8 0.0156

9 0.0175

10 0.0185

II 0.0195

12 O. 0205

13 0.0218

14 0.0225

15 0.0234

16 0.0249

17 0.0 2t)0

18 0.0265

19 0.0270

^This is prepared as follows: Dissolve 10 grams of magnesium chloride in about 75 c.c.
of water and add to grams of ammonium chloride. Introduce 100 c.c. of concentrated
ammonium hydro.\ide into this mixture. If a precipitate forms add ammonium hydroxide
until a clear solution is obtained. ]Make the volume 200 c.c. by means of water and add 10
grams of purified talcum.

-This solution has the following formula:

Silver nitrate i gram.

Ammonium hydroxide (sp. gr. 0.90) 100 c.c.

Talcum 5 grams.

Distilled water. . . too c.c.

5l8 PHYSIOLOGICAL CHEMISTRY

Precipitate, Purine nitrogen,

c.c. per cent

(grams in loo c.c.)

20 0.0275

21 0.0283

22 0.0286

23 o . 0299

24 0,0312

25 0.0325

Calculation. — Multiply the purine nitrogen percentage by the total volume of
urine and divide by 100 to obtain the total purine nitrogen value. For example,
if the precipitate was found to be 12 c.c. and the total volume of the 24-hour urine
was 1300 c.c. the calculation would be as follows:

12 c.c. = 0.0205 per cent purine nitrogen.
0.0205 X 13.0 = 0.2665 gram purine nitrogen.

Interpretation. — The endogenous purine nitrogen excretion (on purine-free
diet) averages about 0.15 gram per day, though variations are considerable. As
uric acid makes up about nine-tenths of this the amount varies much as uric acid
varies. The exogenous purine nitrogen excretion may be largely influenced by the
methyl purines of tea, coffee, and cocoa which are excreted unchanged, as well
as by the purine bases which are normally oxidized to uric acid (see Uric Acid,
page 511).

Allantoin

I. Method of Wiechowski-Handovsky.^ — Principle. — The urine is precipitated
with phosphotungstic acid and lead acetate and in the presence of chlorides with
silver acetate. The heavy metals are removed with hydrogen sulphide. The allan-
toin is then precipitated as a mercuric compound and the amount of mercury and
hence of allantoin in the precipitate determined by titration with ammonium
thiocyanate. This method, though rather tedious, is probably the most accurate
method for the determination of allantoin.

Procedure.— The. urine is diluted to about i per cent urea. As rabbit urine
contains in the day's output about 2-4 grams of urea, and that of other herbivora
usually forms about a 4 per cent urea solution, it is usually desirable to dilute 3-4
times. A greater dilution is not desirable. The urine is treated with i per cent of
sulphuric acid and about 3 c.c. of acetic acid for each day's volume. Test a small
quantity of the urine to determine the amount of 50 per cent phosphotungstic acid
required to completely precipitate it. The bulk of the urine is then treated on this
basis with sufficient solid phosphotungstic acid to precipitate it completely. Stir
to dissolve the acid and allow to stand for several hours. Filter with suction, first
lining the filter with infusorial earth by rubbing up a little of the substance with some
of the urine mixture and filtering with suction. To some ordinary lead oxide in a
mortar add a small amount of the filtrate and stir until it becomes warm, then add
the rest of the filtrate and stir, adding more oxide if necessary untU the solution
reacts alkaline due to the formation of basic lead acetate.

Filter again. The filtrate should give no precipitate with basic lead acetate.

A measured volume of the filtrate is then treated with measured volumes of acetic

acid and silver nitrate solution to completely precipitate any chlorides present.

Filter again preferably through infusorial earth. Pass hydrogen sulphide through

^ Handovsky: Zeit. physinl. Chem., 90, 211, 1914.

VViechowski: Neubauer-Huppert: Analyse des Hams, Wiesbaden, 1913, p. 1076.

URINE 519

the filtrate until the heavy metals are completely precipitated. Filter again. Pass
a current of air through the filtrate to remove all hydrogen sulphide (test with lead
acetate paper). Neutralize this final filtrate with calcium carbonate and remove
the carbon dioxide with a current of air.

The neutral filtrate is then treated with an amount of allantoin reageni in excess
of that required to precipitate the allantoin as indicated by a preliminary test.
(The allantoin reagent is a solution containing 5 per cent mercuric acetate and 20
per cent of sodium acetate. The reagent when used must be clear.)

Allow to stand for half an hour (not too long) and then filter. A measured
amount of the filtrate is taken and treated with about 10 c.c. of iron-ammonium alum
and the red solution decolorized with dilute sulphuric acid. (The solution is not
completely decolorized but retains a faint greenish tint.) Any calcium sulphate
precipitate formed at this point may be disregarded. Titrate with N/io ammonium
thiocyanate solution to a yellow color, which increases in intensity on the addition
of 1-2 drops more of solution. The titration should not be carried out in artifi-
cial light and some practice is required to get the exact end point. The thiocya-
nate solution should be standardized occasionally against standard silver nitrate
solution.

Calculation. — One c.c. of X/io NH4SCN solution corresponds to 0.00436 gram
of allantoin. The limit of error of the method is about 5 mg. for the daily output
of allantoin. In the calculation of course all losses through filtration, etc., must
be considered.

For the considerable modifications required in carrying out the determination
on human urine with its very low content of allantoin see the section by Wiechowski
in Neubauer-Huppert.^

Interpretation. — Allantoin may be found in very small amounts in human urine
(5-15 mg. per day), appearing to be mainly, though not entirely, exogenous in origin.
It forms, however, the principal end-product of the purine metabolism of practically
all mammals other than man and the anthropoid apes. Thus over 90 per cent of
the purine-allantoin nitrogen excretion of the dog, the cow, and the pig occurs in
this form. In these animals its origin is from exogenous and endogenous purines,
and its excretion is influenced by much the same factors as is that of uric acid in
man.

2. Determination by Difference.— ^Method of Plimmer and Skelton.- — Allan-
toin is transformed into urea and determined as such in the acid-magnesium chloride
method of Folin for urea in urine (page 495). Urease, however, has no effect upon
allantoin. Therefore, determine the urea -|- allantoin of the urine according to Fo-
lin's procedure (see Urea), and also determine the true urea according to the
urease method (see Urea). The difference between the results thus obtained rep-
resents allantoin. If sugar is present it must be removed before applying Folin's
procedure.

Hippuric Acid

I. Method of Folin and Flanders.^— Pr/;/677>/f. — The hippuric acid
is hydrolyzod to benzoic acid in alkaline sohition and then the solution
is boiled with strong nitric acid to remove pigments and emulsifying

^ Wiechowski: Neubauer-Huppert; Analyse dcs Hams, Wiesbaden, 191,^, p. 1076.
'^Plimmer and Skelton: Bioclt. J., 8, 70 and 641, 1914.
^ Folin and Flanders: Jottr. Biol. Chein , 11, 257, 191 2.

520 PHYSIOLOGICAL CHEMISTRY

substances. The benzoic acid is extracted with chloroform and ti-
trated with sodium ethylate.

Procedtire. — Measure loo c.c. of urine into a porcelain evaporating dish by
means of a pipette. Add lo c.c. of 5 per cent NaOH and evaporate to dryness
on the steam-bath. Transfer the residue to a 500 c.c. Kjeldahl flask by means of
25 c.c. of water and 25 c.c. of concentrated HNO3. Add 0.2 gram of copper
nitrate, a couple of pebbles or glass pearls and boil very gently for four and one-
half hours over a micro-burner. Fit the necks of the flasks with condensers of
the Hopkins type made from large test-tubes fitted with two-hole rubber stoppers,
the inlet tubes extending near the bottom of the test-tubes while the outlet tube
is shorter. These condensers should fit rather loosely. A good current of water
flowing through the condensers prevents loss of benzoic acid or change in con-
centration of the nitric acid.

After cooling, rinse the condensers down with 25 c.c. of water and transfer the
contents of the flask to a 500 c.c. separatory funnel, with the aid of 25 c.c. more
of water. The total voliune of the solution is now 100 c.c. Add to the solution
sufl5cient ammoniimi sulphate to just saturate it (about 55 grams). Make four
extractions with freely washed chloroform, using 50, 35, 25, and 25 c.c. portions.
The first two portions may be used to further rinse out the Kjeldahl flask.

Collect the successive portions of chloroform in another separatory funnel.
Add to the combined extracts 100 c.c. of a saturated solution of pure sodiimi chlo-
ride, to each Uter of which has been added 0.5 c.c. of concentrated HCl. Shake
well, draw the chloroform into a dry 500 c.c. Erlenmeyer flask and titrate with N/io
sodium alcoholate,' using 4 or 5 drops of phenolphthalein as an indicator. The
first distinct end point should be taken, although it may fade on standing a short
time.

Calculation. — Multiply the mmiber of cubic centimeters of alcoholate used by
the factor for hippuric acid as determined by standardization to obtain the
amount of hippuric acid in the 100 c.c. of urine used. One c.c. of exactly N/io
sodiimi alcoholate is equivalent to 0.0179 gram of hippuric acid. Calculate the
daily output of hippuric acid from the 24-hour volimie.

Interpretation. — The average excretion of hippuric acid by a normal
adult man is about 0.7 gram per day. The amount is increased by
the ingestion of benzoic acid or fruits containing it (plums, prunes,
cranberries). It arises in part apparently from putrefaction products
formed in the intestine. In herbivora it is often the most abundant
nitrogenous constituent of the urine.

2. DaMn's Methods.- — Preliminary Procedure. — Place 150 c.c. (or more) of the
urine under examination in a porcelain evaporating dish and evaporate almost to
dryness upon a water-bath. Add about i gram of sodium dihydrogen phosphate,

' The sodium alcoholate is made by dissolving 2.3 grams of cleaned metallic sodium in i
liter of absolute alcohol. It is advisable that it be slightly weaker rather than stronger
than tenth-normal. It may be standardized against pure benzoic acid in washed chloro-
form. It may also be standardized against N/io HCl provided the alcoholate solution
contains not more than traces of carbonate.

^ Private communication to the author from Dr. H. D. Dakin.

URINE 5 2 I

about 25 grams of gypsum (CaS04, 2H2O) a^d rub up with a pestle and stir with a
spatula until a uniform mixture results. Dry the powder thus produced in a water-
oven for about two hours, at the end of which period it should be rubbed up a
second time, to remove lumps, and transferred to a Schleicher and Schiill "extrac-
tion shell" and extracted in a Soxhlet apparatus in the usual way (see page 326J.
The extraction medium is ethyl acetate and the flask containing the acetate should
be strongly heated over a sand-bath^ for about two hours. The ethyl acetate
extract is now transferred to a separatory funnel, and the original flask rinsed with
sufficient fresh ethyl acetate to make the total volume in the separatory funnel-
about 100 c.c. Wash the ethyl acetate solution /?f times with a saturated solution
of sodium chloride, using 8 c.c. of the sodium chloride solution at each extraction,
shaking vigorously and removing the sodium chloride extract in each case before
adding fresh sodium chloride solution. The sodium chloride removes the urea com-
pletely and the hippuric acid is then determined in the urea-free solution by the
following volumetric or gravimetric procedure:

1. Volumetric Determination. — Transfer the urea-free ethyl acetate solution,
prepared as described above, to a Kjeldahl flask, add about 25 c.c. of water, a small
piece of pumice stone to prevent bumping, attach a condenser and distil off the
acetate' over a free flame. After practically all of the ethyl acetate has been dis-
tilled off, the nitrogen in the remaining solution should be determined by means of
the Kjeldahl method (sec page 483).

The main source of error in this method is the fact that any nitrogen present
in the form of phenaceturic acid or indole acetic acid is determined as hippuric acid
nitrogen. The error from this source is, however, usually trifling.

Calculation. — Calculate as usual for nitrogen determinations, remembering
that I c.c. o/N/io sulphuric acid is equivalent to 0.0179 gro.ni hippuric acid.
Interpretation. — See page 520.

2. Gravi^netric Determination. — The urea-free ethyl acetate solution contained
in the separatory funnel, after washing with sodium chloride solution, as described
under Preliminary Procedure, page 520, is washed with 5 c.c. of distilled water to
remove the major portion of the sodium chloride. Transfer the solution from the
separatory funnel to a round-bottomed flask and subject it to a steam distillation
in the usual way. A slow current of steam should be used while the ethyl acetate
is being distilled off and later a more rapid current may be employed. The dis-
tillation should be continued for 20 minutes. Now add about o. i gram of charcoal
to the aqueous solution which is heated to boiling and filtered hot. Evaporate the
solution in a weighed Jena glass dish on a water-bath until the volume of the solu-
tion is reduced to about 3 c.c. Stand the dish in a warm place until evaporation
is complete and a crystalline residue remains. Wash the residue, in turn, with 2 c.c.
of dry ether and i c.c. of water, dry it in an air-bath at ioo°C. and weigh. If it is
so desired the residue may be recrystallized from a little hot walcr and the melt-
ing-point determined. Pure hippuric acid melts at i87°C. Contamination with
phenaceturic acid may be detected both by the melting-point and the microscopical
characteristics.

* A water-bath cannot be substituted inasmuch as the resultant extraction would be
too slow.

-This ethyl acetate solution contains hippuric acid, urea, and other substances.

^ The ethyl acetate after scjiaration from the watery layer of the distillate may be dried
over calcium chloride and used again. >

522 PHYSIOLOGICAL CHEMISTRY

Glucose

I. Benedict's Method.^- — Principle.- — Benedict's reagent for the esti-
mation of reducing sugars contains potassium thiocyanate as well as
copper sulphate, and in the presence of the former a white precipitate
of cuprous thiocyanate is formed on reduction instead of the usual red
precipitate of cuprous oxide. The small amount of potassium ferro-
cyanide also aids in keeping cuprous oxide in solution. As the pre-
cipitate formed is white the loss of all blue tint in the solution, indicating
complete reduction of the copper, is readily observed. The alkali
used is sodium carbonate, which has the advantage over the hydroxides
in that there is less danger of destruction of small amounts of sugar.
The solution also has the great advantage of being stable for an in-
definite length of time. The method is recommended for simplicity
and accuracy.

Procedure. — The urine, lo c.c. of which should be diluted with water to loo
c.c. (unless the sugar content is believed to be low, when it may be used undiluted),
is povu-ed into a 50 c.c. burette up to the zero mark. Twenty-five c.c. of the
reagent- are measured with a pipette into a porcelain evaporation dish (25-30 cm.
in diameter), 10 to 20 grams of crystallized sodimn carbonate (or one-half the
weight of the anhydrous salt) are added, together with a small quantity of pow-
dered pumice stone or talcum, and the mixture heated to boiling over a free
flame until the carbonate has entirely dissolved. The diluted urine is now run in
from the burette, rather rapidly, until a chalk-white precipitate forms and the
blue color of the mixture begins to lessen perceptibly, after which the solution
from the burette must be nm in a few drops at a time, until the disappearance of
the last trace of blue color, which marks the end point. The solution must be
kept vigorously boiling throughout the entire titration. If the mixture becomes
too concentrated during the process, water may be added from time to time to
replace the volume lost by evaporation.

Calculation. — The calculation of the percentage of sugar in the original sample
of urine is very simple. The 25 c.c. of copper solution are reduced by exactly 50
mg. of glucose. Therefore the volume run out of the burette to effect the reduc-
tion contained 50 mg. of the sugar. When the luine is diluted i : 10, as in the

^Benedict: Jour. Am. Med. Ass'n, 57, 1193, igii.

^ Copper sulphate (crystallized) 18.0 grams.

Sodium carbonate (crystallized, one-half the weight of the

the anhydrous salt may be used) 200. o grams.

Sodium or potassium citrate 200.0 grams.

Potassium thiocyanate 125.0 grams.

Potassium ferrocyanide (5 per cent solution) 5.0 c.c.

Distilled water to make a total volume of 1000. o c.c.

With the aid of heat dissolve the carbonate, citrate and thiocyanate in enough water to
make about 800 c.c. of the mixture and filter if necessary. Dissolve the copper sulphate
separately in about 100 c.c. of water and pour the solution slowly into the other liquid, with
constant stirring. Add the ferrocyanide solution, cool and dilute to exactly i liter. Of the
various constituents, the copper salt only need be weighed with exactness. Twenty-five
c.c. of the reagent are reduced by 50 mg. of glucose.

URINE

0-0

usual titration of diabetic urines, the formula for calculating the per cent of the

sugar is the following:

0.050

X 1000 = per cent in original sample, wherein X

is the number of cubic centimeters of the diluted urine required to reduce 25 c.c.
of the copper solution.

In the use of this method chloroform must not be present during the titration.
If used as a preservative in the urine it may be removed by boiUng a sample for
a few minutes, and then diluting to its original volume.

Interpretation. — Sugar in the urine in amounts sufficient to be de-
tected by the commonly employed qualitative tests indicates a patho-
logical condition, unless very large amounts of sugar have been ingested
just previously, in which case the condition is spoken of as an alimentary
glycosuria. Persistent glycosuria thus indicates diabetes mellitus, a
disorder in which the amount of sugar may rise as high as 10 per cent
and averages 3-5 per cent. The volume of urine excreted per day is
usually also large and the absolute sugar excretion may thus be very
great (100 grams of glucose per day are not uncommon) . The quantita-
tive methods for the estimation of sugar in urine enable us to deter-
mine the severity of the disorder as well as to follow its course under
treatment, etc.

2. Fehling's Method.— Principle. — Diluted urine is run into a
measured amount of Fehling's solution at the boiling-point until all
of the copper it contains is reduced as indicated by the loss of blue color.
This method has several disadvantages over Benedict's method. The
end point is difficult to determine and the mixed solution is unstable.
It gives less accurate results.

Procedure. — Place 10 c.c. of the urine under examination in a 100 c.c. volu-
metric flask and make the volume up to 100 c.c. with distilled water. (If the
urine contains less than 0.5 per cent of sugar it may be used without dilution. A
concentration of about 0.5 per cent is the most satisfactory for this titration.")
Thoroughly mix this diluted urine by pouring it into a beaker and stirring with
a glass rod, then transfer a portion of it to a burette which is properly supported
in a clamp.

Now place 10 c.c. of Fehling's solution^ in a small beaker, dilute it with approxi-
mately 40 c.c. of distilled water, heat to boiUng, and observe whether decomposi-
tion of the FehUng's solution itself has occurred as indicated by the production of
a turbidity. If such turbidity is produced the Fehling's solution is unfit for use.
Clamp the burette containing the dilute urine immediately over the beaker and
carefully allow from 0.5-1 c.c. of the diluted urine to flow into the boihng Fehl-
ing's solution. Bring the solution to the boiling-point after each addition of
urine and continue running the urine from the burette, 0.5-1 c.c. at a time, as in-
dicated, until the Fehling's solution is completely reduced, i.e., until all the cupric

^ Directions for the preparation of Fehling's solution are given in a note at the bottom
of p. 26.

524 PHYSIOLOGICAL CHEMISTRY

oxide in solution has been precipitated as cuprous oxide. This point will be
indicated by the absolute disappearance of all blue color. When this end point
is reached note the number of cubic centimeters of diluted urine used in the proc-
ess and calculate the percentage of dextrose present, in the sample of urine
analyzed, according to the method given below.

This is a satisfactory method, the main objection to its use being the
uncertainty attending the determination of the end-reaction, i.e., the difficulty
with which the exact point where the blue color finally disappears is noted. Sev-
eral means of accurately fixing this point have been suggested, but they are
practically all open to objection. As good a "check" as any, perhaps, is to filter
a few drops of the solution through a double paper, after the blue color has
apparently disappeared, acidify the filtrate with acetic acid and add potassium
ferrocyanide. If the copper of the Fehling's solution has been completely
reduced, there will be no color reaction, whereas the production of a brown color
indicates the presence of unreduced copper. Harrison has recently suggested
the following procedure to determine the exact end point : To about i c.c. of a
starch iodide solution^ in a test-tube add 2-3 drops of acetic acid and introduce
into the acidified mixture 1-2 drops of the solution to be tested. Unreduced
copper will be indicated by the production of a purpUsh-red or blue color due to
the liberation of iodine.

It is ordinarily customary to make at least three determinations by Fehling's
method before coming to a final conclusion regarding the sugar content of the
urine under examination.

Calculation. — Ten c.c. of Fehhng's solution is completely reduced by 0.05
gram of dextrose.- If y represents the nmnber of cubic centimeters of undiluted
urine (obtained by dividing the burette reading by 10) necessary to reduce the
10 c.c. of Fehling's solution, we have the following proportion.

y : 0.05 : : 100 : x (percentage of dextrose).

Interpretation. — See page 523.

3. Bang's Method.^ — Principle.- — The solution to be tested is boiled
with alkaline cupric chloride solution containing thiocyanate and potas-
sium chloride. The cupric salt under these conditions is reduced to
the cuprous form without any precipitation taking place. The re-
duced copper is titrated with standard iodine solution using starch as
an indicator. The titration reaction is as follows:

CuCl + I + K0CO3 = CUCO3 + KCl + KI.

Procedure. — A 100 c.c, Jena flask with a straight neck the flange of which has
been cut off is used for the boiUng procedure. Over the neck of the flask place

^ The starch-iodide solution may be prepared as follows: Mix o.i gram of starch with
cold water in a mortar and pour the suspended starch granules into 75-100 c.c. of boiling
water, stirring continuously. Cool the starch paste, add 20-25 grams of potassium iodide
and dilute the mixture to 250 c.c. This solution deteriorates upon standing, and therefore
must be freshly prepared as needed.

^ The values for certain other sugars are as follows:

Lactose 0.0676 gram.

Maltose o. 074 gram.

Invert sugar o o475 gram.

^ Bang: Biochem. Zeit., 49, i, 1913.

URINE

3^3

a piece of tight fitting rubber tubing sufficiently long (about 2 inches), so that it
may be provided with a pinch cock or clamp to shut ofif the contents of the flask
from the outside air (see Fig. 81, page 281 j.

Introduce into the flask o.i to 2.0 c.c. (or more) of the sugar solution contain-
ing not more than 10 mg. of glucose. Then add 55 c.c. of the diluted copper
solution.' Heat over an asbestos gauze with a flame standardized to bring the
solution to the boiUng-point in from 3 12-3 3 4 minutes. Boil for exactly 3
minutes, being prepared to close the flask with the pinch-cock at the end of the
3 minutes. Remove from the flame and at once cool under the tap to room tem-
perature. Remove the rubber tubing, add to the contents of the flask 121
c.c. of the starch solution (i gram of soluble starch in 100 c.c. of saturated KCl
solution, which keeps indefinitely). Titrate with the standard iodine solution'
run in from an accurate burette with a glass stopcock. When the iodine starch
color appears throughout the solution rotate gently and let stand a few seconds.
The end point is reached when the blue color endures for 10-20 seconds. It is
preferable to carry out the titration in an atmosphere of carbon dioxide, main-
tained by means of a deUvery tube hung over the side of the flask. Otherwise
the titration must be carried out rapidly to prevent reoxidation by the oxygen of
the air.

Calculation. — Divide the number of cubic centimeters of N 100 iodine solu-
tion used in the titration by 2.7 to obtain the niunber of milligrams of glucose in
the amount of solution used.

This method is suitable for urine analysis. The urine must however be free
from albumin and as urine contains substances reacting slowly with iodine the
end point must be taken when the blue color persists for about 10 seconds and any
slow decolorization disregarded.

Interpretation. — See page 523.

4. Peters' Method.- — Principle. — The sugar solution is boiled with an alkaline
copper solution under rigidly standardized conditions and after filtration the un-
reduced copper is determined by adding potassium iodide and titrating the liber-
ated iodine with standard thiosulphate solution.

Procedure. — .1 . The Healing Power. — It is necessary to standardize the heating
power of the flame used in the reduction process. A 200 c.c. Erlenmeycr flask of
Jena glass and of about 6 cm. basal diameter is used. This bears a two-hole rubber
stopper, one hole of which carries a thermometer. The lower end of the thermome-

^ Copper solution. — Stock Solution. — Dissolve first 160 grams potassium bicarbonate,
100 grams potassium carbonate and 66 grams of potassium chloride with about 700 c.c.
of distilled water in a liter flask. Pure salts must be used in each case. As the bicarbonate
is diflicultj' soluble it should be finely powdered and brought into solution first, preferably
with warming to 30°C. The KCl is then dissolved and finally, with cooling, the carbonate.
Then add 100 c.c. of a 4.4 per cent solution of pure crystalline CUSO4.5H2O. Fill to the
mark with distilled water. ]ML\ without strong shaking and let stand for 24 hours before
using.

Dilute Copper Solution. — Dilute 300 c.c. of the stock solution to 1000 c.c. ^lix with
only gentle shaking. Allow to stand for several hours before using.

Standard Iodine Solution. — The N/ioo iodine solution is made by dilution of N/io
iodine solution (see appendix) with boiled out distilled water. The solution is stable for
three months if kept in a dark bottle. It may also be prepared daily from KI and KIOj.
Introduce into a 100 c.c. flask about i c.c. of 2 per cent KIO3. and2-2.5 grams of KI and
then e.xactly 10 c.c. of N/io HCl. The HCl liberates an equivalent amount of iodine (.sul-
phuric acid is less desirable). Make to 100 c.c. with distilled water and mix.

* Peters: /. Am. Chent. Soc, 34, 928, 1912; 34, 422, 1912.

526 PHYSIOLOGICAL CHEMISTRY

ter shovdd extend to about 2 mm. from the bottom of the flask and the 35° mark
on the thermometer stem should be visible above the stopper. The flask is placed
on an asbestos gauze supported by an adjustable ring stand. A Bunsen or Meker
burner is used and is placed at from 3-5 cm. beneath the lower surface of the asbestos
gauze. Use a large flame and allow the ring and gauze to become thoroughly-
heated. Then place the flask, into which 60 c.c. of distilled water has been intro-
duced, in the center of the gauze and observe the time required for the temperature
in the flask to rise from 35 to 95°C. By several trials the flame and position of the
gauze are so adjusted that it requires (within a few seconds either way) just 120
seconds for the temperature to rise from 35-95°C. This standard flame is then
used in the determinations which follow.

B. The Reduction Process. — Into a 200 c.c. Jena Erlenmeyer flask fitted as
above, introduce 20 c.c. of alkaline tartrate solution,^ 20 c.c. of the copper sulphate
solution^ and the sugar solution to be analyzed which should first be made up to
20 c.c. so that the total volume of the fluid in the reduction flask is always 60 c.c.
Place the flask over the standard flame and note when the temperature of the mix-
ture reaches 95°C. Allow to boil for exactly 20 seconds after the temperature
reaches 95°. Then the flask is promptly removed with the stopper still in place
and held under the tap for a moment to stop the reduction but not to cool the mix-
ture more than a few degrees below the boiling-point. Filter hot through a pre-
viously prepared Gooch crucible with a heavy asbestos mat through which suflScient
of a suspension of talcum has been filtered so that with suction, not a stream but a
rapid succession of drops comes through the filter. (A calcium chloride tube
packed with glass wool and asbestos may also be used.) The suction flask should
have a capacity of about 200 c.c. so that the titration may be carried out in it di-
rectly. Wash the filter with a fine stream of water using not more than 15-20 c.c.
of water in all. To the filtrate add 4 c.c. of concentrated sulphuric acid and cool
to 2o°C. Add 6-7 c.c. of a saturated solution of potassium iodide. Titrate the
liberated iodine with standard thiosulphate solution,^ adding a few drops of a solu-
tion of soluble starch as an indicator near the close of the titration. The "spot
test " may be used in determining the end point. As long as a drop of thiosulphate
produces a perceptible white area in falling upon the quiet solution the end point
has not been reached. The chocolate-brown color of the mixture changes to a
light cream white as the last necessary drop of thiosulphate is added.

A blank should be run in exactly the same way but with the omission of the
sugar solution.

Calculation. — Subtract the number of cubic centimeters of thiosulphate re-
quired for the titration of unreduced copper from the number of cubic centimeters
required for the blank. This gives the amount of thiosulphate equivalent to copper

^ Copper Solution. — Dissolve 34,639 grams of highest purity crystallized copper sulphate
(Kahlbaum's "zur Analyse mit Garantieschein) in water to make 500 c.c.

Alkaline Tartrate Solution. — Dissolve 173 grams of sodiumpotassium tartrate and 125
grams of potassium hydroxide in water to make 500 c.c.

^ N/5 Sodium Thiosulphate. — Dissolve about 50 grams of ordinary c.p. sodium thio-
sulphate or exactly 49.66 grams of the pure, dry, recrystalHzed salt, in enough boiled-out
distilled water to make a liter. Allow to stand for several days. The solution should be
standardized against the copper solution prepared as above. For this purpose introduce
20 c.c. of the copper solution into a 200 c.c. Erlenmeyer flask, add 20 c.c. of 30 per cent
acetic acid and 40 c.c. of water. Add about 7 grams of a saturated solution of KI and
titrate with the thiosulphate using starch as an indicator. Calculate the equivalent of i
c.c. of thiosulphate in Cu. One c.c. of the copper sulphate solution contains 17.647 mg.
of Cu. The thiosulphate remains constant for some months. It should be kept in a dark
bottle.

URINE 527

reduced. Multiply this result by the value of i c.c. of thiosulphate expressed as
Cu, and obtain the number of milligrams of copper reduced. Then by consulting
the table of values (below) determine the weight of glucose equivalent to this
amount of copper.

Cole^ has determined the copper values for lactose using this method exactly
as outlined. He has also suggested the following empirical formula which agrees
well with the values derived from his table:

Mg. anhydrous lactose = 1.25 + 0.77S X mg. Cu.

Inter pr elation. — See page 523.

TABLE FOR THE DETERMINATION OF GLUCOSE
According to Peters

Glucose

Copper,
mg.

Glucose

ratio
Cu

Glucose

Coi)pcr,
mg.

Glucosc

ratio
Cu

I

1 .2

0-833

60

II5-5

0.522

2

2.8

0.714

70

134-4

0.522

5

8.2

0.610

80

152-9

0.522

8

13-8

0.580

90

171. 0

0.522

10

17-4

0-575

100

191. 6

0.522

15

27.7

0.542

no

208.9

0.527

20

371

0-539

120

228.1

0.526

25

48.1

0.522

135

255-0

0.529

30

57-3

0.522

150

280.8

0.534

35

67.6

0.522

165

306.8

0.538

40

76.2

0.522

180

330-5

0.545

45

86.0

0.522

200

349-6

0-572

50

96.0

0. 522

5. Bertrand's Method.'' Principle. — The sugar is boiled with alkaline copper
sulphate solution and the precipitated cuprous oxide filtered off, dissolved in an
acid solution of ferric sulphate and the resultant ferrous salt titrated with potassium
permanganate. This method of titrating cuprous oxide may be conveniently used
where other reduction procedures such as that of Peters or of Munson and Walker,*
have been employed. In this case the tables corresponding to the particular
method and not the Bertrand tables must be consulted in calculating the sugar
equivalent.

The following reactions are involved in the Bertrand titration:

CuoO + Fe2(S04)3 + H2SO4 = 2CUSO4 + 2FeS04 + HjO
loFeSO* + 2KMn04 + 8H2SO4 = 5Fe2(S04)s + K2SO4 + 2MnS04 -f 8H,0.

Procedure. — Introduce into an Erlenmeyer flask of 150 c.c. capacity, 20 c.c. of
the sugar solution (of a concentration of 0.5 per cent or less), 20 c.c. of the copper

^Cole: Biochem. J., 8, 134, 1914-

* Bertrand: BM. Soc. Chivi. de France, 35, 1285, 1906.

'Munson and Walker: Bull. 107, U. S. Dept. of Agriculture.

52S

PHYSIOLOGICAL CHEMISTRY

TABLE FOR THE DETERMINATION OF REDUCING SUGARS
According to Bertrand

Sugar in mg.

Glucose
Cu

Invert sugar
Cu

Galactose

rcu

Maltose
Cu

Lactose
Cu

lO

20.4

20.6

19 3

II . 2

14.4

II

22.4

22

6

21.2

12

3

15

8

12

24-3

24

6

23.0

13

4

17

2

13

26.3

26

5

24.9

14

5

18

6

14

28.3

28

5

26.7

15

6

20

0

15

30.2

30

5

28.6

16

7

21

4

16

32.2

32

5

30-5

17

8

22

8

17

34-2

34

5

32.3

18

9

24

2

18

36.2

36

4

34-2

2D

0

25

6

19

38.1

38

4

36.0

21

I

27

0

20

40. r

40

4

37-9

22

2

28

4

21

42.0

42

3

39-7

23

3

29

8

22

43-9

44

2

41.6

24

4

31

I

: ^3

45-8

46

I

43-4

25

5

32

5

24

47-7

48

0

45-2

26

6

33

9

25

49.6

49

8

47.0

27

7

35

2

26

51-5

51

7

48.9

28

9

36

6

27

53-4

53

6

50.7

30

0

38

0

28

55-3

55

5

52. 5

31

I

39

4

29

57-2

57

4

54-4

32

2

40

7

30

59 I

59

3

56.2

33

3

42

I

31

60.9

61

I

58.0

34'

4

43

4

32

62.8

63

0

59-7

35

5

44

8

33

64.6

64

8

61. s

36

5

46

I

34

66.5

66

7

633

37

6

47

4

35

68.3

68

5

65.0

38

7

48

7,

36

70.1

70

3

66.8

39

8

50

I

37

72.0

72

2

68.6

40

9

51

4

38

73-8

74

0

70.4

41

9

52

7

39

75-5

75

9

72.1

43

0

54

I

40

77-5

77

7

73-9

44

I

55

4

• 41

79-3

79

5

75-6

45

2

56

7

42

81. 1

81

2

77-4

46

3

58

0

43

82.9

83

0

79.1

47

4

59

3

44

84.7

84

8

80.8

48

5

60

6

45

86.4

86

5

82.5

49

5

61

9

46

88.2

88

3

84-3

50

6

63

3

47

90.0

90

I

86.0

51

7

64

6

48

91.8

91

9

87.8

52

8

65

9

49

93-6

93

6

895

53

9

67

2

50

95-4

95

4

91 .2

55

0

68

5

51

97.1

97

1

92.9

56

I

69

8

52

98.9

98

8

94.6

57

I

71

I

53

100.6

100

6

96.3

58

2

72

4

54

102.3

102

3

98.0

59

3

73

7

55

104. 1

104

0

99-7

60

3

74

9

i 56

1

105.8

los

7

101.5

61

4 ,

76

2

URINE

529

TABLE FOR THE DETERMINATION OF REDUCING SVG ARS.— (Continued)

According to Bertrand

Glucose

Invert sugar

Galactose

Maltose

Lactose

Sugar in mg.

Cu

Cu

Cu

Cu

Cu

S7

107.6

107.4

103.2

62.5

77-5

58

109.3

109. 2

104.9

63-5

78.8

59

III. I

no. 9

106.6

64.6

80.1

60

112. 8

112. 6

108.3

65-7

81.4

61

II4-5

114-3

no.o

66.8

82.7

62

116. 2

115.9

111.6

67-9

839

63

117. 9

117. 6

II3-3

68.9

85.2

64

119. 6

119. 2

115.0

70.0

86.5

65

121. 3

120.9

116.6

71.1

87.7

66

123.0

122.6

118.3

72.2

89 0

67

124.7

124.2

120.0

73-3

90.3

68

126.4

125.9

121.7

74-3

91.6

69

128. 1

127-S

123.3

75-4

92.8

70

129.8

129.2

125.0

76.5

94.1

71

131-4

130.8

126.6

77-6

95.4

72

133- 1

132.4

128.3

78.6

96.6

73

134-7

134.0

130.0

79-7

97-9

74

136.3

135-6

131.5

80.8

99-1

75

137-9

137.2

133-1

81.8

100.4

76

139.6

138.9

134-8

82.9

lOI .7

77

141. 2

140.5

136.4

84.0

102.9

78

142.8

142. 1

138.0

85.1

104.2

79

144-5

143-7

139.7

86.1

105.4

80

146. 1

145-3

141.3

87.2

106.7

81

147-7

146.9

142.9

83.3

107.9

82

149-3

148. 5

144.6

89-4

109.2

83

150.9

150.0

146.2

90.4

110.4

84

152. 5

151. 6

147.8

91-5

III. 7

85

154-0

153-2

149.4

92.6

112.9

86

155-6

154-8

151. 1

93-7

114. 1

87

157-2

156.4

152.7

94-8

II5-4

88

158.8

157-9

154.3

95-3

116. 6

89

160.4

159-5

156.0

96.9

117.9

90

162.0

161.1

157.6

98.0

119. 1

91

163.6

162.6

159-2

99.0

120.3

92

165.2

164.2

160.8

100. 1

121. 6

93

166.7

165.7

162.4

10:. 1

122.8

94

168.3

167.3

164.0

102.2

124.0

95

169.9

168.8

165.6

103.2

125.2

96

171-S

170.3

167.2

104. 2

126.5

97

173-1

171.9

168.8

105.3

127.7

98

174-6

173-4

170.4

106.3

128.9

99

176. 2

175-0

172.0

107.4

130.2

100

177-8

^ -('' '

173 -6

108.4

131 4

34

530 PHYSIOLOGICAL CHEMISTRY

solution^ and 20 c.c. of the alkaline tartrate solution.^ Heat to boiling over an
asbestos gauze and boil gently for exactly three minutes. Let stand a moment that
the copper oxide may settle and then filter with suction through a Gooch crucible
with a heavy asbestos mat (or a calcium chloride tube with successive layers of
glass wool, coarse asbestos and fine asbestos -wool) into a flask of about 150 c.c.
capacity. Wash the residue in the flask twice by decantation with a little hot
water pouring the supernatant liquid through the filter. Throw away the clear
filtrate, rinse the flask and replace it. To the flask containing the cuprous oxide
add 5-20 c.c. of the acid ferric sulphate solution.^ A green solution containing
ferrous sulphate is formed. Pour through the filter together with a little more of
the acid solution if necessary to completely dissolve the copper oxide. Wash flask
and filter with a little water. Titrate the filtrate with standard potassium per-
manganate solution^ to a rose color. The procedure should be carried out as rapidly
as possible.

Calculation. — Multiply the number of cubic centimeters of permanganate used
by its copper equivalent as determined by standardization, and from the table
(page 528-529) obtain the corresponding value for the sugar under examination.

Interpretation — See page 523.

6. Fermentation Method. — Principle. — This method consists in
the measurement of the volume of carbon dioxide evolved when the
dextrose of the urine undergoes fermentation with yeast. None of
the various methods whose manipulation is based upon this principle
is absolutely accurate. The method in which Einhorn's saccharometer
(Fig. 3, page 31) is the apparatus employed is perhaps as satisfactory
as any for clinical purposes.

Procedure. — Place about 15 c.c. of urine in a mortar, add about i gram of
yeast (1/16 of the ordinary cake of compressed yeast) and carefully crush the
latter by means of a pestle. Transfer the mixture to the saccharometer, being
careful to note that the graduated tube is completely filled and that no air bubbles
gather at the top. Allow the apparatus to stand in a warm place (30°C.) for 12
hours and observe the percentage of dextrose as indicated by the graduated scale
of the instrument. Both the percentage of dextrose and the number of cubic
centimeters of carbon dioxide are indicated by the graduations on the side of the
saccharometer tube.

The fermentation method becomes a much more accurate procedure
if the saccharometer of Lohnstein is used.^

^ (a) Copper Sulphate Solution. — Forty grams of pure crystallized copper sulphate are
dissolved in water to make a liter.

Q)) Alkaline Tartrate Sol uti 071. — Dissolve 200 grams of Rochelle salts and 150 grams of
NaOH in water to make 1000 c.c.

(c) Acid Ferric Sulphate Solution. — Dissolve 50 grams of ferric sulphate in about 200 c.c.
of water and pour into this a mixture of 200 c.c. of concentrated sulphuric acid diluted
with about 400 c.c. of water. Mix and make up to 1000 c.c.

{d) Potassium Permanganate Solution. — Dissolve 5 grams of potassium permanganate in
water to make 1000 c.c. Standardization. — Dissolve 0.250 gram of ammonium oxalate in
50-100 c.c. of water, add 1-2 c.c. of concentrated sulphuric acid and titrate with the per-
manganate to a rose color. About 22 c.c. will be required. Multiplj^ the number of grams
of oxalate used by 0.895 to get the equivalent in Cu of the number of cubic centimeters of
permanganate used. Calculate the Cu value of i c.c.

^Lohnstein: MUnch. med. Woch., 1S99, 1671.

URINE

531

The availability of the fermentation procedure as a quantitative
aid has been appreciably lowered through the important findings of
Neuberg and Associates.^ They show that yeast has the property of
splitting off carbon dioxide from the carhoxyl group of amino- and other
aliphatic acids. The active agent in this "sugar-free fermentation" is
an enzyme called carboxylase. Inasmuch as amino-acids are always
present in the urine, the error from this source is apparent.

7. Polariscopic Examination. — Before subjecting urine to a polariscopic
examination the slightly acid fluid should be decolorized as thoroughly as possible
by the addition of a little lead acetate. The urine should be well stirred and then
filtered through a filter paper which has not been previously moistened. In this
way a perfectly clear and almost colorless Uquid is obtained.

In determining dextrose by means of the polariscope it should be borne in
mind that this carbohydrate is often accompanied by other optically active sub-
stances, such as proteins, fructose, /3-hydroxybutyric acid, and conjugate gly-
curonates which may introduce an error into the polariscopic reading ; the method
is, however, sufiiciently accurate for practical piuposes.

For directions as to the manipulation of the polariscope see page 31.

Below are given the specific rotations of some physiologically important sugars
as well as of certain other optically active substances the possible presence of
which must be borne in mind in determining glucose polarimetrically in urine.

Specific Rotation

Specific Rotation

Glucose

+ 52.49

Fructose

-92.25

Maltose

+ 136.5

.:(-Hydroxybutyric

— 24.12

Isomaltose

+68.0

acid.

Lactose

+ 52.53

Conjugated Gly-

Levorotatory in

Pentose (i-ara-

0.0

curonic Acids.

varying degrees.

binose).

Protein

I. Scherer's Coagulation Method. The content of coagulable protein
may be accurately determined as follows : Place 50 c.c. of urine in a small beaker
and raise the temperature of the fluid to about 40°C. upon a water-bath. Add
dilute acetic acid, drop by drop, to the warm urine, to precipitate the protein which
will separate in a flocculent form. Care should be taken not to add too much
acid ; ordinarily less than 20 drops is sufiicient. The temperature of the water in
the water-bath should now be raised to the boiUng-point and maintained there
for a few minutes in order to insure the complete coagulation of the protein pres-
ent. Now filter the urine- through a previously washed, dried, and weighed

1 Xeuberf,' and Associates: Biochcm. Zeilschr., vol. 31 and 36, iqii.

- If it is desired the precipitate may be filtered off on an unweighed paper, and its nitrogen
content determined by the Kjeldahl method (see p. 483). In order to arrive at correct
figures for the protein content it is then simply necessary to multiply the total nitrogen
content by 6.25 (see p. 328). Correction should be made for the nitrogen content of the
filter paper used unless this factor is negligible.

532

PHYSIOLOGICAL CHEMISTRY

filter paper, wash the precipitated protein, in turn, with hot water, 95 per cent
alcohol, and with ether, and dry the paper and precipitate, to constant weight, in
an air-bath at i io°C. Subtract the weight of the filter paper from the combined
weight of the paper and precipitate and calculate the percentage of protein in the
urine specimen.

Calculation. — To determine the percentage of protein present in the urine
under examination, multiply the weight of the precipitate, ex-
pressed in grams, by 2.

Interpretation. — The amount of albumin occurring
in the urine is not necessarily an index of the severity
or type of the disorder giving rise to it. Hence no sig-
nificant figures can be given. Normal human urine
probably contains a trace of albumin which is too slight
to be detected or determined by the usual procedures.
The determination of albumin may be of assistance in
following the course of kidney disturbances, but the re-
sults can be interpreted only in the light of other clinical
findings.

2. Esbach's Method. — This method depends upon the pre-
cipitation of protein by Esbach's reagent^ and the apparatus
used in the estimation is Esbach's albuminometer (Fig. 167).
In making a determination fill the albmninometer to the
point U with urine, then introduce the reagent imtil the
point R is reached. Now stopper the tube, invert it slowly
several times in order to insure the thorough mixing of the
fluids, and stand the tube aside for 24 hours. Creatinine, resin,
acids, etc., are precipitated in this method, and for this and
other reasons it is not as accurate as the coagulation method.
It is, however, extensively used clinically. According to Sahli^
the method is "accurate approximately to one part per 1000,"
whereas Pfeiffer^ claims it is not accurate for less than one-
half or for more than five parts per 1000.

Calculation. — ^The graduations on the albuminometer indi-
cate grams of protein per liter of urine. Thus, if the protein
precipitate is level with the figure 3 of the graduated scale, this
denotes that the urine examined contains 3 grams of protein to
the liter. To express the amotmt of protein in per cent simply move the deci-
mal point one place to the left. In the case under consideration the urine
contains 0.3 per cent protein.

Interpretation. — See above.

3. Kwilecki's Modification of Esbach's Method.^ — Add 10 drops of a 10 per
cent solution of FeCU to the acid urine before introducing the Esbach's reagent.

^ Esbach's reagent is prepared by dissolving 10 grams of picric acid and 20 grams of
citric acid in i liter of water.

^Sahli: Lehrbuch d. klin. U titer suchungs-Methoden, 5th Aufl., 1909.
3 Pfeiffer: Berl. klin. Woch., 49, 114, 191 2.
* Kwilecki: Miinch med. Woch., 56, p. 1330.

Fig. 167.—
Esbach's Albu-
minometer.

URINE

533

Wann the tube and contents in a water-bath at 72°C. for 5-6 minutes and make
the reading.

4. Turbidity Method of Folin and Denis.' — Principle. — The albumin of the
urine is precipitated with sulphosalicylic acid and the turbidity produced com-
pared with that of a standard protein solution.

Procedure. — To about 75 c.c. of water in each of two 100 c.c. volumetric flasks
is added 5 c.c. of a 25 per cent solution of sulphosalicylic acid. To one flask is then
added 5 c.c. of the standard protein solution containing 10 mg. of albumin and to
the other is added the albuminous urine i c.c. at a time (by means of an Ostwald
pipette) until the turbidity obtained seems to be reasonably near that of the
standard. The two flasks are then filled up to the mark with water, cautiously
inverted a few times to secure mixing, and are then ready for the quantitative
comparison just as in colorimetric work. The standard must invariably be read
against itself. The standard- containing 10 mg. of protein is set at 20 mm. The
unknown must not read less than 10 nor more than 30.

Calculation. — Dividing 200 by the product of the reading of the unknown and
the number of cubic centimeters of urine taken gives the albumin in milligrams per
cubic centimeter of urine. The albuminous suspensions must not be shaken but
mixed very carefully. The method is fairly accurate and requires but a few minutes
if a standard solution is at hand. The method is not applicable to urines deeply
colored with blood or bile but may be used for albuminous fluids other than urine
if such fluids are not highly pigmented. It must be borne in mind that different
proteins, as serum albumin and serum globulin, may give markedly different degrees
of turbidity under the same conditions.^

Interpretation. — See page 532.

Acetone and Acetoacetic Acid

I. Folin-Hart Method. — Principle. — This method as well as the
two following serve the purpose of determining the acetone, and aceto-
acetic acid together in terms of acetone. Acetoacetic acid on heating
is decomposed with the formation of acetone. In this method the
acetone preformed and that derived from the acetoacetic acid are
carried over by means of an air current into a solution of iodine in potas-
sium hydroxide (alkaline hypoiodite solution). The acetone is here
absorbed and retained as iodoform. The excess iodine over that
necessary to combine with the acetone is'determined by titration with
sodium thiosulphate. The method is simple and accurate if directions
are carefully followed.

^ Folin and Denis: Jour. Biol. Client., iS, 273, 1914.

- Standard Albumin solution. Fresh blood serum free from hemoglobin is used.
25-35 c.c. of the serum are diluted with a 15 per cent solution of chemically pure sodium
chloride to about 1500 c.c. The solution is mixed and filtered. By means of nitrogen
determinations the protein content of the filtrate is determined (protein = XX6. 25) and
on the basis of the figure obtained the solution is diluted with 15 per cent sodium chloride
solution so that it contains 2 mg. of protein per cubic centimeter. It is best to saturate
the albumin solution with chloroform. The solution keeps for months.

'Marshall and Banks: Proceedings of the American Philosophical Society, 54, 176,
1915.

534 PHYSIOLOGICAL CHEMISTRY

Procedure, — ^Introduce into a wide-mouth bottle 200 c.c. of water, an accu-
rately measured excess of N/io iodine solution^and an excess of 40 per cent potas-
sium hydroxide. Prepare an aerometer cylinder containing alkaline hypoiodite
solution to absorb any acetone which may be present in the air of the laboratory,
and between the cylinder and bottle suspend a test-tube about 2 inches in diam-
ter. This large test-tube should contain 20 c.c. of the urine under examination,
ID drops or a 10 per cent solution of phosphoric acid, 10 grams of sodium chloride
and a Uttle petroleum, and should be raised sufficiently high to facilitate the easy
application of heat to its bottom portion. The connections on the side of the tube
should be provided with bulb-tubes containing cotton. When the apparatus is
arranged as described, it should be connected with a Chapman pmnp and an air
current passed through for twenty-five minutes. During this period the contents
of the test-tube are heated just to the boiling-point and after an interval of five
minutes again heated in the same manner. By this means the diacetic acid is
converted into acetone and at the end of the twenty-five-minute period this
acetone, as well as the preformed acetone, will have been removed from the urine
to the absorption bottle and there retained as iodoform.

The contents of the absorption bottle should now be acidified with concen-
trated hydrochloric acid,- and titrated with N/io sodiimi thiosulphate and starch
as in the Messinger-Huppert method (see below).

Interpretation. — iNormal adults on a mixed diet excrete on the
average 3-15 mg. of combined acetone and acetoacetic acid per day and
anything over 20 mg. is usually pathological. The amount is con-
siderably increased in fasting and on a carbohydrate-free diet due to the
development of acidosis. In severe diabetic acidosis values up to 6
grams per day or even higher may be noted. It is sometimes found in
large amounts in intoxications associated with pregnancy. It may be
found in increased amounts in the urine in a great variety of patho-
logical conditions. Quantitative estimation enables us to follow the
course of the acidosis. Ammonia excretion is also largely increased in

1 Proceed as follows in order to obtain a rough idea regarding the amount of N/io
iodine solution to be used: Introduce into a test-tube 10 c.c. of the urine under examina-
tion and I c.c. of a solution of ferric chloride made by dissolving 100 grams of ferric chloride
in 100 c.c. of distilled water. After permitting the mixture to stand for two minutes,
compare the color with that of an equal volume of the ferric chloride solution in a test-
tube of similar diameter. If the two solutions be of approximately the same color intensity,
20 c.c. of the urine under examination will yield sufl&cient acetone to require nearly 10 c.c.
of N/io iodine solution. In case the»nuxture is darker in color than is the ferric chloride
solution, the former should be diluted with distilled water untU it is of approximately the
same intensity as the ferric chloride solution. From this data the amount of N/io iodine
solution required may be roughly estimated by means of the following table:

Urine c.c.

Ferric chloride

Water

N/io Iodine required c.c.

xo

I
I

I
I

10

10
10
10

10
20
30

20

35
40

^ An excess of iodine is indicated by the development of a brown color.

URINE 535

these conditions, being used in the neutralization of the excess acids
formed in the body. Usually about three-quarters of the combined
acetone and acetoacetic acid excretion is in the form of acetoacetic acid,
but the proportion is not constant.

Acidosis is due mainly to a disturbance in the metabolism of fats.
The fatty acids are ordinarily oxidized through hydroxybutyric acid to
acetoacetic acid which is in turn oxidized through formic and acetic
acids to carbon dioxide and water. When fat catabolism is increased
to such an extent that the body cannot bring about complete oxidation
of the products formed, a considerable portion of the acetoacetic acid
instead of being oxidized in this way is transformed into acetone
(a process taking place but to a slight extent normally). This acetone
as well as acetoacetic acid and in more severe cases /3-hydroxy butyric
acid will then be eliminated to varying degrees in the urine.

The relation of the acetone bodies is indicated in the following
scheme :

CH3— CHOH— CH2— COOH (/3-hydroxybutyric acid)

oxidation I T reduction

CH3— CO— CH2— COOH (acetoacetic acid)

I loss of CO2

CH3 — CO — CHa (acetone)

In fasting the decomposition of fat is increased due to the lack of
carbohydrate material and acidosis develops. The same holds true
for a carbohydrate-free diet. Apparently also fat is much less readily
oxidized in the presence of a carbohydrate deficiency.

2. Messinger-Huppert Method. — Principle. — This method differs from the
preceding in that distillation of the acetone is substituted for aspiration. It is an
accurate method of determining acetone and diacetic acid together.

Procedure. — Place 100 c.c. of urine in a distillation flask and add 2 c.c. of 50
per cent acetic acid. Connect the flask with a condenser, properly arrange a re-
ceiver, attach a terminal series of bulbs containing water, and distil over about
nine-tenths of the urine mixture. Remove the receiver, attach another, and sub-
ject the residual portion of the mi.xture to a second distillation. Test this fluid for
acetone and if the presence of acetone is indicated add about 100 c.c. of water to
the residue and again distil. Treat the united acetone distillates with i c.c. of
dilute (12 per cent) sulphuric acid and redistil, collecting this second distillate in a
glass-stoppered flask. During distillation, however, the glass stopper is replaced
by a cork with a double perforation, the glass tube from one perforation passing
to the condenser, while the bulbs containing water, before mentioned, are attached
by means of the tube in the other perforation, .\llow the distillation process to pro-
ceed until practically all of the fluid has passed over, then remove the receiving
flask and insert the glass stopper. Xow treat the distillate carefully with 10 c.c.

536

PHYSIOLOGICAL CHEMISTRY

of a N/io solution of iodine and add an excess of sodium hydroxide solution (15-25
c.c. of 20 per cent). Stopper the flask and shake it for about one minute. Add
1-2 drops of concentrated hydrochloric acid, and note the production of a brown
color at the point of contact if an excess of iodine is present. In case there is no
such excess, the solution should be treated with N/io iodine solution until an excess
is obtained. Retitrate this excess of iodine with N/io sodium thiosulphate solu-
tion until a light yellow color is observed. At this point a few cubic centimeters
of starch paste should be added and the mixture again titrated until no blue color
is visible. This is the end-reaction.

Calculation. — Subtract the number of cubic centimeters of X/io thiosulphate
solution used from the volume of N/io iodine solution employed. Since i c.c. of
the iodine solution is equivalent to 0.967 mg. of acetone, and since i c.c. of the thio-
sulphate solution is equivalent to i c.c. of the iodine solution, if we multiply the
remainder from the above subtraction by 0.967 we will obtain the number of milli-
grams of acetone in the 100 c.c. of urine examined.

Calculate the quantity of acetone in the twenty-four-hour urine specimen.

Interpretation. — See page 534.

3. Method of Scott-Wilson.^ — Principle. — The urine is distilled
with acid and the acetone (preformed and from acetoacetic acid by

Fig. •168. — ScoTT-WiLsoN Apparatus.

hydrolysis) collected in an alkaline solution of basic mercuric cyanide.
A precipitate of keto-mercuric cyanide is formed according to the
following equation:

C3H6O + 2Hg(CN)2 + 3HgO = C30Hg5C4N4 + 3H2O

The precipitate is filtered off and its mercury content determined by
titration with potassium thiocyanate solution. The method is adapted
to the determination of acetone in small amounts, and has the ad-
vantage over the iodoform method that it is not affected by alcohol.

Procedure. — The apparatus for the distillation of acetone is set up as in the
illustration (Fig. 168). Introduce 100 c.c. of the normal urine (or a lesser quan-

' Scott- Wilson: Jour. Physiol., 42, 444, 191 1.

URINE 537

tity of an abnormal urine high in acetone) into flask A, together with 25 grams
anhydrous sodium sulphate and i c.c. of concentrated sulphuric acid. Ten c.c.
of 40 per cent sodiimi hydroxide solution are placed in flask C and 10 c.c. or more
of the mercuric cyanide solution' in the Erlenmeyer flask E, the tube D being
arranged so as to dip beneath the surface of the reagent.

If more than 0.4 mg. of acetone is present in the amount of urine taken, the
quantity of reagent should be proportionately increased. It is desirable to make
a test to determine the approximate amount of acetone bodies as outUned under
the Folin-Hart method 'page 534). Connect up the apparatus closing B with a
glass-rod plug, and hght the burners under A and C. The sodium hydroxide
solution in C must boil before the urine in A as otherwise condensation would
take place in C. Keep the hydroxide solution just at the boiUng point and aUow
A to boil briskly. Note the first appearance of turbidity in flask E and distil for
five minutes from that time. Remove the plug at B and extinguish the burners.
Remove tube D and rinse with distilled water into flask E. Allow to stand for
ten minutes.

Filter off the precipitate on an asbestos mat in a Gooch crucible. The pores
of the filter should have been partially closed by filtering a suspension of talc
through it. If the first portions of the filtrate are not clear, pass them through
the filter again. Transfer any precipitate adherent to the sides of the flask to the
filter with the aid of water and wash the filter thoroughly with water. Transfer
the asbestos and precipitate to an Erlenmeyer flask by means of a glass rod.
Any precipitate adherent to the crucible or glass rod is washed into the flask with
a jet of "acid mixtiire" (nitric acid 40 parts, sulphuric acid 5 parts and water 55
parts). About 10 c.c. of this acid mixture should be used altogether. Then add
I c.c. of N '5 potassium permanganate solution.- Boil until the brown color given
by the permanganate has completely disappeared. This should occur in one to
two minutes but if the decolorization occurs more rapidly (a few seconds),
insufficient permanganate has been added and another cubic centimeter or so
should be run in so that the color is not dispelled on two minutes boiling. Clear
with a few drops of yellow nitric acid.

Cool the completely decolorized solution under the tap and add 2 c.c. of a
saturated solution of ferric alum. Titrate with standard potassium thiocyanate
solution' until a brownish tinge appears throughout the solution. Care should be
taken with the end point as the addition of several drops after the end point has
been reached will not perceptibly darken the color.

Calculation. — One c.c. of the thiocyanate solution if made up exactly is
equivalent to i mg. of Hg or 0.058 mg. of acetone. Multiply the number
of cubic centimeters of thiocyanate used by its equivalent of mercury in milli-
grams and by 0.058 to get the amount of acetone and acetoacetic acid (expressed
as acetone) in the amount of urine analyzed. Calculate the daily output from the
24-hour volume.

^ Scott-Wilson Reagent. — Dissolve 0.5 gram mercuric cyanide and 9 grams sodium hy-
droxide in 60 c.c. of water and then run in with constant stirring 20 c.c. of 0.726S per cent
silver nitrate solution. (The silver nitrate solution is made by taking i part of standard
silver nitrate solution (i c.c. = 10 mg. XaCl) and 3 parts of water.)

2 Made by dissolving 6.324 grams of potassium permanganate in water and making up
to a liter.

' Make up an appro.ximately o.i per cent solution of potassium thiocyanate and stand-
ardize it against mercuric nitrate or silver nitrate. It is convenient to have the solution
of such a strength that i c.c. = i mg. of Hg.

538 PHYSIOLOGICAL CHEMISTRY

Interpretation. — See page 534.

Acetone

Folin's Method. — Principle. — The preformed acetone is aspirated
from the urine mixture at room temperature to prevent decomposition
of acetoacetic acid. The acetone is collected in alkaline hypoiodite
solution as in the Folin-Hart method (page 533) . Iodoform is formed
quantitatively and the excess of iodine is titrated with sodium thio-
sulphate.

Procedure. — ^The same type of apparatus is used in this method as that
described in Folin's method for the determination of ammonia (see page 499).
Introduce 20-25 c.c. of the urine under examination into the aerometer cylinder
and add 10 drops of 10 per cent phosphoric acid/ 8-10 grams of soditun chloride,^
and a little petroleum. Introduce into an absorption flask,' such as is used in the
ammonia determination (see page 499), 150 c.c. of water, 10 c.c. of a 40 per cent
solution of potassixim hydroxide, and an excess of a N/io iodine solution. Con-
nect the flask with the aerometer cyUnder, attach a Chapman pump, and permit
an air current, slightly less rapid than that used for the determination of ammonia,
to be drawn through the solution for 20-25 minutes. All of the acetone will, at
this point, have been converted into iodoform in the absorption flask. Add
10 c.c. of concentrated hydrochloric acid (a volimie equivalent to that of the strong
alkali originally added), to the contents of the latter and titrate the excess of
iodine by means of N/io sodimn thiosulphate solution and starch, as in the Mes-
singer-Huppert method (see page 535).

Folin has further made suggestions regarding the simultaneous determination
of acetone and ammonia by the use of the same air current.* This is an important
consideration for the clinician inasmuch as urines which contain acetone and aceto-
acetic acid are generally those from which the ammonia data are also desired. The
procedure for the combination method is as follows: Arrange the ammonia appar-
atus as usual (see page 499), and to the aerometer of the ammonia apparatus attach
the acetone apparatus set up as described above. Regulate the air current with
special reference to the determination of acetone and at the end of 20-25 minutes
disconnect the acetone apparatus and complete the determination of the acetone
as just described. The air current is not interrupted, and after having run one
and one-half hours the ammonia apparatus is detached and the ammonia determina-
tion completed as described on page 500.

If data regarding acetoacetic acid are desired, the result obtained by Folin's
method may be subtracted from the result obtained by the Messinger-Huppert
method (see page 535), inasmuch as the latter method determines both acetone and
acetoacetic acid. Under all conditions the determination of acetone should be as
expeditious as possible. This is essential, not only because of the fact that any

1 Oxalic acid (0.2—0.3 gram) may be substituted if desired.

2 Acetone is insoluble in a saturated solution of sodium chloride.

' Folin's improved absorption tube (see Fig. 128, p. 500) should be used in this connec-
tion inasmuch as the original type embracing the use of a rubber stopper is unsatisfactory
because of the solvent action of alkaline hypoiodite on rubber.

* These determinations may even be made on the same sample of urine if the sample is
too small for the double determination.

URINE 539

acetoacetic acid present in the urine will become transformed into acetone, but also
because of the rapid spontaneous decomposition of the alkaline hypoiodite solution
used in the determination of the acetone. It has been claimed that alkaline hypo-
iodite solutions are almost completely converted into iodale solutions in one-half
hour. Folin states, however, that the transformation is not so rapid as this, but
he nevertheless emphasizes the necessity of rapidity of manipulation. At the same
time it should be remembered that the air current must not be as rapid as for am-
monia, inasmuch as the alkaline hypoiodite solution will not absorb all the acetone
under those conditions.

Interpretation.— \Js,u.a.\\y about one-fourth of the total acetone and
acetoacetic acid excretion is in the- form of acetone, but the proportion
varies considerably- See Acetone and Acetoacetic Acid.

Acetoacetic Acid

1. Folin-Hart Method. — Arrange the apparatus as described under the
Folin-Hart method for the determination of acetone and acetoacetic acid (see
page 533). Start the air current in the usual way and permit it to nin 25 minutes
without the application of heat to the urine under examination. Under these
conditions the preformed acetone present in the solution is all removed 'see
page 538). Immediately attach a freshly prepared absorption bottle or intro-
duce fresh alkaline hypoiodite solution into the original bottle. Apply heat to
the large test-tube as akeady described (see page 533), in order to convert the
acetoacetic acid into acetone, permit the air current to continue for the usual
25-minute period, and determine the acetoacetic acid value in terms of acetone
by the usual titration procedure (see page 5361.

Interpretation. — Ordinarily about three-fourths of the total acetone
and acetoacetic acid excretion occurs in the form of acetoacetic acid,
which, however, is readily transformed into acetone with loss of carbon
dioxide. See Acetone and Acetoacetic Acid.

2. Folin-Messinger-Huppert and Folin-Scott-Wilson Method. — Determine
the combined acetone and acetoacetic acid, in terms of acetone, by the Messinger-
Huppert method or the Scott -Wilson method (see pages 535 and 536 ^ and sub-
sequently determine the acetone by FoUn's method (see page 5381. Subtract
the value determined by the second method from that obtained in either of the
first two methods to secure data regarding the acetoacetic acid content of the
urine, in terms of acetone.

Acetone, Acetoacetic Acid, and ^-Hydroxybutyric Acid

I. Method of Shaffer and Mairiott.^—P rincifylc. By this procedure
the combined acetone and acetoacetic acid is determined in the same
sample of urine used in the determination of /3-hydroxybutyric acid.
The preformed acetone and the acetoacetic acid are distilled off to-

' Shaffer and Marriott: Jour. Biol. Chein., 16, 265, 1915.

54© PHYSIOLOGICAL CHEMISTRY

gether as acetone and determined by the iodine titration method.
The )8-hydroxybutyric acid remains in the residue from distillation
and is oxidized by means of potassium bichromate. The product
of the oxidation is acetone which is distilled off and determined as
such.

Procedure. — Determination of Acetone and Acetoacetic Acid. — Measure
from 25-100 c.c.^ or more of urine (usually 50 c.c.) with a pipette into a 500 c.c.
volumetric flask containing 200-300 c.c. of water. Add basic lead acetate
solution (U. S. P.) in volume equal to that of the urine used- and mix well. Add
concentrated ammonium hydroxide in amount equal to about one-half that of
the lead acetate solution. Dilute the contents of the flask to the mark with
water, shake, and after standing a few minutes filter the liquid, preferably
through a folded filter. Measure 200 c.c. of the filtrate into a round bottom
flask (800 c.c. or liter Kjeldahl flasks are convenient) dilute with water to about
600 c.c. and add 15 c.c. of concentrated sulphuric acid and a little talc or a boiling
stone. Distil until about 200 c.c. of distillate have been collected. The tube
of the condenser should dip beneath the surface of the water in the receiving
flask so that no loss of acetone will occur. The distiUing flask must also be
fitted with a dropping tube or dropping funnel so water may be run in from time
to time and the volinne of liquid in the flask kept from becoming less than
400-500 c.c. A good condenser should be used, but it is not necessary to cool
the distillate in ice.

The distillate thus obtained is transferred to a second Kjeldahl flask and
10 c.c. of 10 per cent NaOH added. It is then redistilled for about 20 minutes.^
This second distillate is then titrated with standard iodine and thiosulphate
solution as in the method for acetone and acetoacetic acid previously given
(see Messinger-Huppert method, page 535), and the calculation made in the
same way. The result gives the combined acetone and acetoacetic acid content
of the urine expressed as acetone.

Determination of the /3-Hydroxybutyric Acid. — The flask containing the
residue from the first distillation above is used in the determination of the
^-hydroxybutyric acid. A new receiver is arranged as before with the tip from the
condenser dipping beneath the surface of the water. The distillation is then
continued and water added whenever necessary to keep the volume between
400 and 600 c.c. A dilute solution (i per cent) of potassiimi bichromate is added
during the distillation. At first 20 c.c. of this i per cent solution is added slowly
through the dropping tube and then 10 c.c. portions every 15-20 minutes until

1 The amount used depends upon the expected yield of /3-oxybutyric acid. In the case
of urines which give a strong ferric chloride reaction for diacetic acid, or when 5-10 grams
or more of /3-oxybutyric acid is expected, it is unnecessary to use more than 25-50 c.c. of
urine. However, in case only a trace of /3-oxybutyric acid is expected, the volume should be
much larger as indicated. Under all conditions, the amount specified is sufficient for dupli-
cate determinations. It is desirable to use such a volume of urine as contains the proper
amount of /3-oxybutyric acid to yield 25-50 mg. of acetone.

2 If the urine contains but little or no sugar only half the amount or less of lead acetate
should be used.

2 In many instances when a high degree of accuracy is not required this redistillation
may be omitted and the first distillate titrated directly. The results so obtained are
slightly higher than those after redistillation from alkali. The object of the redistillation
is to get rid of fatty acids of which formic acid is one of the most troublesome.

URINE 541

the whole has been added. ^ Should the liquid become markedly green the
bichromate must be added at correspondingly shorter intervals and in amount
suflBcient to maintain a sUght red-yellow color of the chromic acid which may be
detected even in the presence of the green. Continue the distillation with moder-
ate boihng for from two to three hours. The distillate which should be collected
in a liter flask to avoid transference is again distilled for about 20 minutes
after adding 10 c.c. of 10 per cent sodium hydroxide and 25 c.c. of 3 per cent
hydrogen peroxide. The flask must be heated cautiously until the peroxide has
been decomposed. This final distillate is titrated with standard iodine and
thiosulphate in the usual manner (see page 536; and the result expressed as
hydroxybutyric acid. One c.c. of N/ 10 iodine solution is equivalent to 1.736
mg. of hydroxybutyric acid. One c.c. of the 1.035 N/io iodine which is recom-
mended for acetone titrations is equivalent to 1.793 n^g- of hydroxybutyric acid.
About 10 per cent should be added to the results for /3-hydroxybutyric acid as
obtained by this method as the yield of acetone is only about 90 per cent of
the theoretical. This error appears to be practically constant, so that satisfactory
results may be obtained by correction.

Interpretation. — i3-Hydroxybutyric acid may occur in normal human
urine to the extent of 20-30 mg. per day. In fasting or on a carbo-
hydrate-free diet very large amounts may be excreted (up to 20 grams
per day). In severe diabetes mellitus the largest amounts are found.
Excretions of 50 or even 100 grams or over per day have been noted.
It is always 'present in the urine when large amounts of acetone are
present. In severe diabetes it is usually the most abundant of the
acetone bodies making up from 60-80 per cent of the total. The
ratio is, however, by no means constant and it should be borne in mind
that in rare cases large amounts of /3-hydroxybutyric acid may be
eliminated although the acetone excretion is very low. (See Acetone
and Acetoacetic Acid.)

2. Nephelometric Methods for Acetone, Acetoacetic Acid, and
/3-Hydroxybutyric Acid. — Folin and Denis'- have suggested nephelo-
metric methods for the determination of the acetone bodies in urine.
The methods are similar to those used by Marriott for blood analysis
(see Chapter XVI) but the air current is used instead of distillation.

/3 -Hydroxybutyric Acid

I. Black's Method — Principle. — The urine is mixed with plaster
of Paris to form a coarse meal and extracted with ether to obtain
the hydr()xybut\ric acid which is then determined by means of the
polariscope.

^ From 0.5 gram to i gram of bichromate will usually be sufficient, and not more than
I gram should be added unless the liquid turns Rreen indicatinn a preat reduction to
chromium sulphate. Very rarely 2 or 3 grams of bichromate may be necessary, especially
if the sugar has not been completely removed.

^ Folin and Denis: Jour. Biol. Cliem., 18, 263, 1914.

542 PHYSIOLOGICAL CHEMISTRY

Procedure. — Render 50 c.c. of the urine under examination faintly alkaline
with sodium carbonate and evaporate to one-third the original volume. Con-
centrate to about 10 c.c. on a water-bath, cool the residue, acidify it with a few
drops of concentrated hydrochloric acid^ and add plaster of Paris to form a
thick paste. Permit the mixture to stand until it begins to "set," then break
it up with a stout glass rod having a blunt end and reduce the material to the
consistency of a fairly dry coarse meal.- Transfer the meal to a Soxhlet appa-
ratus and extract with ether for six to ten hours. At the end of this period
evaporate the ether-extract either spontaneously or in an air current. Dissolve
the residue in water, add a httle boneblack, if necessary, filter until a clear
solution is obtained and make up the filtrate to a known volvmie (25 c.c. or less)
with water. The /3-hydroxybutyric acid should then be determined by means of
the polariscope. Its specific rotation is —24.12.

This method is satisfactory where the amount of hydroxybutyric
acid present is not too small. Errors due to incomplete extraction of
the acid are partly counterbalanced by the extraction of other levo-
rotatory substances.

Interpretation. — See page 541.

2. Method of Schaffer and Marriott. — See page 539.

Indican

Ellinger's Method. — Principle. — This method for the quantitative
determination of indican is based upon the principle underlying Jaffe's
qualitative test for indican. The urine after removal of interfering
substances with basic lead acetate is treated with Obermayer's reagent
to oxidize the indican to indigo. The indigo is extracted with chloro-
form, the chloroform evaporated off and the residue titrated with
potassium permanganate. The method is not very accurate but is as
satisfactory as any.

Procedure. — To 50 c.c. of urine^ in a small beaker or casserole add 5 c.c.
of basic lead acetate solution,* mix thoroughly, and filter. Transfer 40 c.c. of
the filtrate to a separatory funnel, add an equal volmne of Obermayer's reagent
(see page 388) and 20 c.c. of chloroform, and extract in the usual manner. This
extraction with chloroform should be repeated untU the chloroform solution
remains colorless. Shake up the combined chloroform extracts two or three
times with distilled water in a separating funnel and complete the purification
by extracting with very dilute sodium hydroxide (i: 1000). Remove all traces
of alkaU by washing with water. Now filter the combined chloroform extracts
through a dry filter paper into a dry Erlenmeyer flask. Distil off the chloro-
form, heat the residue on a boihng water-bath for five minutes in the open

^ The residue should give a distinct red color with litmus paper.

^ Before this is accomplished it may, in some cases, be necessary to add a little more
plaster of Paris.

' If the urine under examination is neutral or alkaline in reaction it may be made
faintly acid with acetic acid before adding the basic lead acetate.

* For preparation of basic lead acetate solution see Appendix.

URINE 543

flask, and wash the dried residue with hot water.' Add lo c.c. of concentrated
sulphuric acid to the washed residue, heat on the water-bath for five to ten
minutes, dilute with loo c.c. of water, and titrate the blue solution with a very
dilute solution of potassium permanganate.- The end point is indicated by the
dissipation of all the blue color from the solution and the formation of a pale
yellow color.

Beautiful plates of indigo blue sometimes appear in the chloroform extract
of urines containing abundant indican. In urines preserved by thymol the
determination of indican is interfered with unless great care is taken in washing
the chloroform extract with dilute alkah. Care should be taken, therefore, to
make the indican determination upon fresh urine, before the addition of the
preservative.

Plasencia^ has suggested a method which is shorter than Ellinger's and ac-
cording to its sponsor, just as accurate.

Calculation. — One cubic centimeter of the diluted permanganate solution
is equivalent to about 0.15 mg. of indigo. Ellinger claims that one-sixth of the
amount determined must be added to the value obtained by titration in order to
secure accurate data. This correction should always be made.

Interpretation. — From 4-20 mg. of indican are excreted per day by
normal men. In normal individuals the variations are dependent
mainly upon the diet. A meat diet increases the indican excretion,
while a milk or carbohydrate-rich diet decreases it. Pathologically
the greatest increases are found in disorders involving increased
putrefaction and stagnation of intestinal contents. Bacterial de-
composition of body protein as in gangrene, putrid pus formation, etc.,
gives rise to increases.

Phenols

Colorimetric Method of Folin and Denis. ^ — Principle.- — This method
is based upon the fact that phenols yield with a solution of phospho-
tungstic-phosphomolybdic acid and alkali a deep blue color the depth
of which is proportional to the amount of such substances present.
Traces of protein, which may be present in the urine, and uric add
give a blue color with the reagent and are removed by precipitation
with an ammoniacal silver solution and colloidal iron as a preUminary
to the determination of the phenols.

Procedure. — Removal of Interfering Substances.- Place 10 c.c. of ordinary
urine, or 20 c.c. of a dilute urine in a 50 c.c. volumetric flask. To this add an

* The washing should be continued until the wash water is no longer colored. Ordi-
narily two or three washings are sullicient. If a separation of indigo particles takes place
during the washing process, the wash water should be filtered, the indigo extracted with
chloroform, and the usual method applied from this point.

^ A "stock solution" of potassium permanganate containing 3 grams per liter should be
prepared, and when needed for titration purposes a suitable volume of this solution should
be diluted with 40 volumes of water. The potassium permanganate soliition may be
standardized with pure indigo.

' Plasencia: Revista de Medicina y Cirugia., 17, r, 1912.

* Folin and Denis: J. Biol. Ghent., 22, 305, 191 5.

544 PHYSIOLOGICAL CHEMISTRY

acid silver lactate solution (from 2 to 20 c.c. of a 3 per cent solution of silver
lactate in 3 per cent lactic acid) until no further precipitate is obtained. Add
a few drops of colloidal iron, shake the flask, dilute to mark with distilled water,
shake again, and filter the contents through a dry filter. Phenols are not pre-
cipitated by this procedure but are recovered quantitatively in the filtrate. Trans-
fer 25 c.c. of the filtrate to a 50 c.c. volumetric flask, and add a sufficient quantity
of saturated sodium chloride solution, containing 10 c.c. of strong hydrochloric
acid per liter, to precipitate all the silver. Fill the flask to the mark with dis-
tilled water, mix thoroughly, and filter through a dry filter. This filtrate, which
contains half the phenol from the urine taken for analysis, is used for the deter-
mination of free and total phenols.

Free Phenols. — Place 20 c.c. of the filtrate mentioned above in a 50 c.c.
volumetric flask, add 5 c.c. of the phosphotungstic-phosphomolybdic acid re-
agent^ and 15 c.c. of a saturated solution of sodium carbonate. Dilute to volume
with luke warm water (30-35°C.), mix thoroughly and after allowing to stand
for 20 minutes compare the deep blue color in the Duboscq colorimeter (see
Fig' i53> page 486) against a standard solution of phenol (see below) similarly
treated.

Total Phenols (Free and Conjugated). — Place 20 c.c. of the same filtrate
used for the determination of free phenols in a large test-tube, add 10 drops
of concentrated hydrochloric acid, cover the tube with a small funnel, heat
rapidly to boiUng over a free flame, and then place in a boiling water-bath
for ten minutes. This process serves to decompose the conjugated phenols.
At the end of the ten minutes, remove the tube, cool, and transfer the contents
to a 100 c.c. volumetric flask. Add lo c.c. of the phosphotungstic-phospho-
molybdic reagent, 25 c.c. of saturated sodium carbonate solution, dilute to mark
with luke warm water (30-35°C.), mix thoroughly, allow to stand for 20 minutes,
and read in the Duboscq colorimeter (see page 486) against a standard solution
of phenol (see below).

Standard Solution of Phenol. — The standard used is a solution of pure phenol
in N/ioo hydrochloric acid containing i mg. of phenol in 10 c.c, standardized by
means of the iodometric titration. The preparation is carried out as follows: Make
a phenol solution in N/io hydrochloric acid, which contains approximately i mg. of
crystallized phenol per cubic centimeter. Transfer 25 c.c. of this solution to a
250 c.c. flask, add 50 c.c. of N/io sodium hydroxide, heat to 65°C., add 25 c.c. of
N/io iodine solution, stopper the flask, and let stand at room temperature 30 or
40 minutes. Add 5 c.c. of concentrated hydrochloric acid and titrate the excess
of iodine with N/io thiosulphate solution. Each cubic centimeter of N/io iodine
solution corresponds to 1.567 mg. of phenol. On the basis of the result dilute the
phenol solution so that 10 c.c. contain i mg. of phenol. Five c.c. of this solution
(equivalent to 0.5 mg. of phenol), when 10 c.c. of the phosphotungstic phospho-
molybdic reagent and 25 c.c. of saturated sodium carbonate solution are added, and
the whole made up with water at about 3o°C. to 100 c.c, give when set in the
colorimeter at 20 mm. a convenient standard.

Calculation. — The filtrate used for the determination of free and total phenols

^ This reagent is prepared as follows: Boil together for two hours (using a reflux con-
denser) 100 grams of sodium tungstate, 20 grams of phosphomolybdic acid (or an equiva-
lent of molybdic acid), 50 c.c. of phosphoric acid (85 per cent.), and 75 c.c. of distilled
water. After the period of heating, cool, dilute to i liter with distilled water, and filter
If necessary.

URINE 545

contains the phenols from one-half the amount of urine analyzed. The actual
determination of phenols, both free and total, is made upon a two-fifths portion
of this filtrate and this amount of filtrate contains the phenols from one-fifth
of the amount of urine analyzed. In the determination of free phenols the colored
solution is diluted to only half that of the standard while in the determination
of total phenols the dilution is the same as that of the standard.
Hence,

Ri

and

= miUigrams of free phenol
R2 X 4

= miUigrams of total phenol
R2 X 2

in 2 c.c. or 4 c.c. of urine according to whether 10 c.c. or 20 c.c. of urine was
taken for analysis, when Ri is taken as the reading obtained with the standard
solution, and R2 is taken as the reading obtained with the unknown.

Interpretation. — By this method total phenol excretions of from
0.2-0.5 gram per day have been noted in normal individuals. These
results are much higher than figures previously obtained by other
methods. The free phenols varied from 0.1-0.3 gram per day. The
total phenol excretion appears to vary directly but not proportionately
with the protein intake. The amount of conjugated phenol indicates
the extent to which the phenols have been detoxicated. The excretion
of phenols is increased in gastro-intestinal disorders associated with
increased putrefaction. It is increased by the ingestion of phenols or
of benzene.

Oxalic Acid

Salkowski-Autenrieth and Barth Method. — Principle. — The o.xalic acid is pre-
cipitated by means of CaC^. From the solution of this precipitate in hydrochloric
acid the oxalic acid is extracted with ether and reprecipitated as calcium oxalate.

Procedure. — Place the 24-hour urine specimen in a precipitating jar, add an
excess of calcium chloride, render the urine strongly ammoniacal, stir it well, and
allow it to stand 18-20 hours. Filter oflf the precipitate, wash it with a small
amount of water and dissolve it in about 30 c.c. of a hot 15 per cent solution of
hydrochloric acid. By means of a separatory funnel extract the solution with 150
c.c. of ether which contains 3 per cent of alcohol, repeating the extraction four or
five times with fresh portions of ether. Unite the ethereal extracts, allow them to
stand for an hour in a flask, and then filter through a dry filter paper. Add 5 c.c.
of water to the filtrate, to prevent the formation of diethyl oxalate when the solu-
tion is heated, and distil ofif the ether. If necessary, decolorize the Hquid with
animal charcoal and filter. Concentrate the filtrate to 3-5 c.c, add a Httle calcium
chloride solution, make it ammoniacal, and after a few minutes render it slightly
acid with acetic acid. Allow the acidified solution to stand several hours, collect
35

546 PHYSIOLOGICAL CHEMISTRY

the precipitate of calcium oxalate on a washed filter paper, ^ wash, incinerate strongly
(to CaO), and weigh in the usual manner.

Calculation. — Since 56 parts of CaO 'are equivalent to 90 parts of oxalic acid,
the quantity of oxalic acid in the volume of urine taken may be determined by
multiplying the weight of CaO by the factor 1.6071.

Interpretation. — From 15-20 mg. of oxalic acid are excreted by a normal adult
on an ordinary mixed diet. It arises from oxalates of the food ingested and from
fat and protein metabolism. It is increased by the ingestion of apples, grapes,
cabbage, etc., although most of the ingested oxalate is destroyed. It is increased
in disturbances of metabolism associated with decreased oxidation, according to
certain observers. The term "oxaluria" has been largely a misnomer.

Sulphur
(a) Gravimetric Procedures

I. Total Sulphates.^ — Folin's Method. — Principle. — The sulphuric
acid of the conjugated sulphates is set free by boiling with acid. The
total sulphates are then precipitated with barium chloride.

Procedure. — Place 25 c.c. of urine in a 200-250 c.c. Erlemneyer flask, add
20 c.c. of dilute hydrochloric acid^ (i volume of concentrated HCl to 4 voltunes of
water) and gently boil the mixture for 20-30 minutes. To minimize the loss of
water by evaporation the mouth of the flask should be covered with a small watch
glass during the boiling process. Cool the flask for 2-3 minutes in running water,
and dilute the contents to about 150 c.c. by means of cold water. Add 10 c.c.
of a 5 per cent solution of baritmi chloride slowly, drop by drop, to the cold solu-
tion.^ The contents of the flask should not be stirred or shaken during the addi-
tion of the barium chloride. AUow the mixture to stand at least one hour, then
shake up the solution and filter it through a weighed Gooch crucible.*

Wash the precipitate of BaS04 with about 250 c.c. of cold water, dry it in an
air-bath or over a very low flame, then ignite,* cool and weigh.

Calculation. — Subtract the weight of the Gooch crucible from the weight of
the crucible and the BaSO^ percipitate to obtain the weight of the precipitate.

' Schleicher and Schiill, No. 5S9, is satisfactory.

- If it is desired, 50 c.c. of urine and 4 c.c. of concentrated acid may be used instead.

' A dropper or capillary funnel made from an ordinary calcium chloride tube and so
constructed as to deliver 10 c.c. in 2-3 minutes is recommended for use in adding the barium
chloride.

* If a Gooch crucible is not available, the precipitate of BaS04 may be filtered off upon
a washed filter paper (Schleicher & SchuU's, No. 589, blue ribbon), and after washing the
precipitate with about 250 c.c. of cold water the paper and precipitate may be dried in an
air-bath or over a low flame. The ignition may then be carried out in the usual way in the
ordinary platinum or porcelain crucible. In this case correction must be made for the
weight of the ash of the filter paper used.

5 Care must be taken in the ignition of precipitates in Gooch crucibles. The flame
should never be applied directly to the perforated bottom or to the sides of the crucible, since
such manipulation is invariably attended by mechanical losses. The crucibles should
always be provided with lids and tight bottoms during the ignition. In case porcelain Gooch
crucibles, whose bottoms are not provided with a non-perforated cap, are used, the crucible
may be placed upon the lid of an ordinary platinum crucible during ignition. The lid
should be supported on a triangle, the crucible placed upon the lid and the flame applied
to the improvised bottom. Ignition should be complete in 10 minutes if no organic matter
is present.

URINE 547

The weight of SO^^ in the volume of urine taken may be determined by means of
the following proportion.

Mol. Wt. Wt. of Mol. wt.

BaS04 : BaSO^ : : SO3 : x(wt. of SO3 in grams).

Representing the weight of the BaS04 precipitate by y and substituting the proper
molecular weights, we have the following proportion :

233-43 : y : : 80.06 : x (wt. of SO3 in grams in the quantity of urine used).

Calculate the quantity of SO 3 in the twenty-four-hour specimen of urine.
To express the result in percentage of SO3 simply divide the value of x, as just
determined, by the quantity of urine used.

Interpretation. — The total sulphate excretion (ethereal and inorganic
sulphates) by a normal adult on a mixed diet is usually between 1.5 and
3.0 gram of SO3 with an average of about 2.0 gram. The sulphuric
acid is derived but to a slight extent ordinarily from ingested sul-
phates, being mainly dependent on the sulphur of the protein ingested
and will consequently vary widely with the protein content of the diet.
From 75 to 95 per cent of the total sulphur of the urine is ordinarily
found as sulphate, the proportion being greatest on a high protein diet.
The sulphate excretion is increased in all conditions associated with
increased decomposition of body protein as in acute fevers and de-
creased whenever there is a decrease in metabolic activity.

2. Inorganic Sulphates. — Folin's Method. — Place 25 c.c. of urine and 100
c.c. of water in a 200-250 c.c. Erlenmeyer flask and acidify the diluted urine
with 10 c.c. of dilute hydrochloric acid (i volimie of concentrated HCl to 4 vol-
umes of water). In case the urine is dilute 50 c.c. may be used instead of 25 c.c.
and the volume of water reduced proportionately. Add 10 c.c. of 5 per cent bar-
ium chloride slowly, drop by drop, to the cold solution and from this point proceed
as indicated in the method for the determination of Total Sulphates, page 546.

Calculate the quantity of inorganic sulphates, expressed as SO3, in the twenty-
four-hour urine specimen.

Calculation. — Calculate according to the directions given imder Total Sul-
phates, above.

Interpretation. — On an average about 90 per cent of the total sul-
phates of the urine exists as inorganic sulphates but the proportion
of the sulphates existing in this form varies widely, being greater on
a high protein diet than on a very low protein diet. The amount
varies with the total sulphates (which see).

3. Ethereal Sulphates. — Folin's Method. — Principle. — The inorganic sul-
phates are removed with barium chloride and the conjugated sulphates then
determined after hydrolysis.

Procedure. — Place 125 c.c. of urine in an Erlenmeyer flask of suitable size,

^ It is considered preferable by many investigators to express all sulphur valucs'in terms-
of S rather than SO3.

548 PHYSIOLOGICAL CHEMISTRY

dilute it with 75 c.c. of water and acidify the mixture with 30 c.c. of dilute hydro-
chloric acid (i volume of concentrated HCl to 4 volumes of water). To the cold
solution add 20 c.c. of a 5 per cent solution of barium chloride, drop by drop.^
Allow the mixture to stand about one hour, then filter it through a dry filter paper.'
Collect 125 c.c. of the filtrate and boil it gently for at least one-half hour. Cool
the solution, filter off the precipitate of BaS04, wash, dry and ignite it according to
the directions given on page 546.

Calculation. — The weight of the BaS04 precipitate should be multiplied by
2 since only one-half (125 c.c.) of the total volume (250 c.c.) of fluid was precipi-
tated by the barivmi chloride. The remaining calculation should be made accord-
ing to directions given under Total Sulphates, page 546.

Calculate the quantity of ethereal sulphates, expressed as SO 3, in the twenty-
four-hour urine specimen.

Interpretation. — The excretion of ethereal sulphates (expressed as
SO3) varies ordinarily from o.i to 0.25 gram per day comprising from
5 to 15 per cent of the total sulphur excretion. The absolute amount
of ethereal sulphate increases with increase in the protein of the diet and
particularly with increase of putrefactive processes in the intestine or
elsewhere. The amount excreted cannot however be taken as an
index of the extent of intestinal putrefaction.

4. Total Svilphur.^ — ^Benedict's Method.^ — Principle. — The urine
is evaporated and ignited with a solution of copper nitrate and
potassium chlorate. Organic matter is thus destroyed and all un-
oxidized sulphur is oxidized to the sulphate form and can be readily
precipitated with barium chloride in the usual manner. The method
is very convenient and accurate.

Ten c.c. of urine are measiired into a small (7-8 cm.) porcelain evaporating dish
and 5 cc" of Benedict's sulphur reagent^ added. The contents of the dish are
evaporated over a free flame which is regulated to keep the solution just below the
boiling-point, so that there can be no loss through spattering. When dryness is
reached the flame is raised sUghtly vmtil the entire residue has blackened. The

^ See note (3) at the bottom of p. 546.

2 This precipitate consists of the inorganic sulphates. If it is desired, this BaSO*
precipitate may be collected in a Gooch crucible or on an ordinary quantitative filter
paper and a determination of inorganic sulphates made, using the same technic as that
suggested 'above. In this way we are enabled to determine the inorganic and ethereal
sulphates in the same sample of urine.

^ Benedict: Journal of Biological Chemistry, 6, 363, 1909.

* If the urine is concentrated the quantity should be slightly increased.

^ Crystallized copper nitrate, sulphur-free or of known sulphur content 200 grams.

Sodium or potassium chlorate 50 grams

Distilled water to 1000 c.c.

Denis has suggested the use of the following solution:

Copper nitrate 25 grams.

Sodium chloride 25 grams.

Ammonium nitrate 10 grams.

Water to make 100 c.c.

The procedure is the same as the above except that 25 c.c. of urine and 5 c.c. of reagent
are taken. It gives accurate results.

URINE 549

flame is then turned up in two stages to the full heat of the bxinsen burner and the
contents of the dish thus heated to redness for ten minutes after the black residue
(which first fuses) has become dry. This heating is to decompose the last traces of
nitrate (and chlorate). The flame is then removed and the dish allowed to cool
more or less completely. Ten to 20 c.c. of dilute (i 14) hydrochloric acid is then
added to the residue in the dish, which is then warmed gently until the contents
have completely dissolved and a perfectly clear, sparkling solution is obtained.
This dissolving of the residue requires scarcely two minutes. With the aid of a
stirring rod the solution is washed into' a small Erlenmeyer flask, diluted with
cold, distilled water to 100-150 c.c, 10 c.c. of 10 per cent barium chloride solution
added drop by drop, and the solution allowed to stand for about an hour. It is
then shaken up and filtered as usual through a weighed Gooch crucible. Controls
should be run on the oxidizing mixture.

Calculation. — Make the calculation according to directions given under Total
Sulphates, page 546. Calculate the quantity of sulphur expressed as SO3 or S,
present in the twenty-four-hour urine specimen.

Interpretation. — The total sulphur (SO3) excretion averages about 2.5
grams per day. It runs more or less parallel with the decomposition
of endogenous and exogenous protein and a definite ratio between the
excretion of total N and total S might be expected. It has been
suggested that the ratio 5 : i expresses this relation in a general way but
no constant value can be given. Sec Total Sulj'jhates.

5. Total Sulphur. — Osbome-Folin Method. — Principle. — This
method depends on the destruction of organic matter by means of
sodium peroxide. It is employed particularly for the determination
of sulphur in foods and feces. Benedict's procedure (see above) is
simpler and fully as satisfactory for urine.

Place 25 c.c. of urine- in a 200-250 c.c. nickel crucible and add about 3 grams of
sodium peroxide. Evaporate the mixtiure to a syrup upon a steam water-bath and
heat it carefully over an alcohol flame xmtil it soUdifies (15 minutes). Now remove
the crucible from the flame and allow it to cool. Moisten the residue with 1-2 c.c. of
water, ^ sprinkle about 7 8 grams of sodium peroxide over the contents of the crucible
and fuse the mass over an alcohol flame for about 10 minutes. Allow the crucible
to cool for a few minutes, add about 100 c.c. of water to the contents and heat at
least one-half hour over an alcohol flame to dissolve the alkali and decompose the
sodiimi peroxide. Next rinse the mixture into a 400 450 c.c. Erlenmeyer flask,
by means of hot water, and dilute it to about 250 c.c. Heat the solution nearly to
the boihng-point and add concentrated hydrochloric acid slowly until the nickelic
oxide, derived from the crucible, is just brought into solution.' A few minutes'
boiling should now yield a clear solution. In case too Uttle peroxide or too much
water was added for the final fusion a clear solution will not be obtained. In this
event cool the solution and remove the insoluble matter by filtration.

' Sometimes the porcelain glaze cracks during heating, in whi. 1- . i-i- th." -..luiinn should
be filtered into the flask.

* If the urine is verj- dilute 50 c.c. may be used.

^ This moistening of the residue with a small amount of waur is very essential and
should not be neglected.

* About iS c.c. of acid are required for S grams of sodium peroxide.

550 PHYSIOLOGICAL CHEMISTRY

To the clear solution add 5 c.c. of very dilute alcohol (about 18-20 per cent) and
continue the boiling for a few minutes. The alcohol is added to remove the
chlorine which was formed when the solution was acidified. Add 10 c.c. of a
10 per cent solution of barium chloride, slowly, drop by drop,^ to the liquid.
Allow the precipitated solution to stand in the cold two days and then filter and
continue the manipulation according to the directions given under Total Sul-
phates, page 546.

Calculation. — Make the calculation according to directions given under Total
Sulphates, page 546. Calculate the quantity of sulphur, expressed as SO3 or S,
present in the twenty-four-hovir urine specimen.

Interpretation. — See page 549.

(b) Volumetric Procedures

6. Volumetric Determination of Ethereal and Inorganic Sulphates.
— ^Method of Rosenheim and Drummond.-— Pmzc?^/^.- — The sulphates
of the urine are precipitated by means of benzidine solution, the pre-
cipitate of benzidine sulphate being filtered off and the sulphuric
acid of the compound titrated with N/io KOH using phenolphthalein
as an indicator. This is possible because the benzidine is a very weak
base and its sulphate readily dissociates. It is necessary that excess
of HCl be avoided in the precipitation process.

Procedure.^ — (a) Inorganic Sulphates. — Preparation of the benzidine solu-
tion. Rub 4 grams of benzidine (Kahlbaum) into a fine paste with about 10
c.c. of water and transfer to a 2-hter flask with the aid of about 500 c.c. of water.
Add 5 c.c. of concentrated HCl (sp. gr. 1.19) and make up to 2 liters with distilled
water. One hundred and fifty c.c. of this solution, which keeps indefinitely,
are sufficient to precipitate o.i gram H2SO4.

Measure 25 c.c. of urine into a 250 c.c. Erlenmeyer flask and acidify with
dUute hydrochloric acid (1:4) until the reaction is distinctly acid to Congo red
paper. Usually 1-2 c.c. of dilute acid are reqxiired. One himdred c.c. of the
benzidine solution, as prepared above, are then run in and the precipitate,
which forms in a few seconds, allowed to settle for ten minutes. Filter with
suction and wash the precipitate with 10-20 c.c. of water saturated with benzidine
sulphate. 2 Transfer the precipitate and filter paper to the original precipitation
flask with about 50 c.c. of water and titrate hot with N/io KOH, after first
adding a few drops of saturated alcohohc solution of phenolphthalein.

' Calculation. — One c.c. of N/io KOH corresponds to 4.9 mg. H0SO4 or 4.0 mg.
of SO3. Multiply the number of cubic centimeters of N/io KOH required by
4.9 and by 4 to get the amount of H2SO4 in 100 c.c. of the urine analyzed.

^ See note (3) at the bottom of p. 546.

* Rosenheim and Drummond: Biochcm. J., 8, 143, 1914.

' In order to obtain accurate results it is most important that the precipitate should be
finely suspended in water before titration and this again entails certain precautions during
filtration so as to prevent the caking together of the precipitate. The authors use a funnel
of 6 cm. diameter and a perforated porcelain plate (5-7 mm.) covered either with paper pulp
or with a well-fitting filter paper. Do not allow the precipitate to be sucked drj' on the fil-
ter. The final filtrate should show no acid reaction to Congo red.

URINE

33-

(b) Total Sulphates (Inorganic and Ethereal). — Measure 25 c.c. of urine
into an Erlenmeyer flask, add 2-2.5 c.c of dilute HCl ("1:41 and 20 c.c. of water
and boil for 15-20 minutes. The ethereal sulphates are hydrolized.' Allow the
solution to cool and then precipitate the sulphate with benzidine as in the deter-
mination of inorganic sulphates. The titration and calculation are also carried
out in the same way.

(c) Ethereal Sulphates. — Determine the total sulphates and inorganic sul-
phates as indicated above. Subtract the amount of inorganic sulphate from
that of the total sulphate and obtain the amount of ethereal sulphate present.

(d) Total Sulphur. — According to Rosenheim and Drummond- the benzidine
method may be employed for the estimation of total sulphur in the solution ob-
tained on the oxidation of urine by the Wolf-Osterberg^ modification of Bene-
dict's method. This modification involves the use of larger quantities of urine
than the Benedict method or a reduction in accuracy and hence probably has
no advantages over Benedict's original procedure. See below for modification
of Raiziss and Dubin.

(e) Neutral Sulphur. — Neutral sulphur is most readily determined by dif-
ference. Subtract from the total sulphur as determined by one of the methods
given above the amount of total sulphates. The difference corresponds to the
neutral sulphur of the urine sample examined.

Interpretation. — The neutral sulphur of the urine is made up of
cystine and related bodies, thiocyanate, oxyproteic acids, etc. It
makes up ordinarily from 5-25 per cent of the total sulphur of the urine,
or on the average 0.2 to 0.4 gram per day calculated as SO3. The
absolute amount is fairly constant for a given individual through wide
variations of protein intake, indicating that its origin is mainly en-
dogenous, that is, that it arises principally from the decomposition of
tissue protein. On this account the percentage of the total sulphur
excretion existing in the neutral form may rise to 25 per cent on a very
low protein diet and decrease to 5 per cent on a high protein diet, the
absolute amount remaining nearly constant. In fasting percentages
as high as 70 have been noted. In many disorders as tuberculosis,
cancer, cystinuria, etc., the amount may be relatively and in some
cases absolutely increased but no fixed relations have been determined
for the various conditions.

7. Total Sulphur. — Method of Raiziss and Dubin. ^ — Principle. — The urine is
oxidized by Benedict's mclhod (page 548) the sulphur precipitated as benzidine
sulphate and the benzidine titrated with N/io permanganate solution. \'ery
small amounts of sulphur may be determined in this way.

Procedure. — To 2 c.c. of urine in an 8 cm. porcelain dish, add 0.5 c.c. of Bene-
dict's reagent (page 548) and evaporate to dryness on the water-bath. Heat the dish

1 A larger amount of HCl may be used (20 c.c. of the dilute acid) if desired. In this
case it is necessary to neutralize the solution carefully after boiling and again add dilute
HCl until the reaction is acid to Congo red.

^Rosenheim and Drummond: Bioch. Jour., 8, 143, 1014.

' Wolf and Osterlierg: Bioch. Zcit., 29, 429, 1910.

* Raiziss and Duliin: Jour. Biol. Clicm., 18, 297, 1914.

552 PHYSIOLOGICAL CHEMISTRY

carefully over a small flame till the contents are black, and then heat to redness for
only two rm'nutes. Cool, add 2 c.c. of hydrochloric acid (1:4) and warm. Neutralize
the clear solution with NaOH (10 per cent) and again acidify with i drop of HCl
(i :4). Add 25 c.c. of a solution of benzidine hydrochloride* with stirring. Let
stand 15 minutes and then filter off on an asbestos filter. Transfer the precipitate
to the filter by means of the filtrate and wash with 5 c.c. of cold water, drop by drop.
Put the filter into a 500 c.c. Erlenmeyer flask, add i c.c. of NaOH (10 per cent) and
200 c.c. of water. Boil the suspension for five minutes and then cool to room tem-
perature. Add 20 c.c. concentrated sulphuric acid and titrate the warm solution at
once with N/io potassium permanganate solution till a distinct pink coloration is
obtained, which should last 20 seconds. In titrating at first add only about 0.5 c.c.
at a time and toward the end only 2 drops at a time, waiting tiU the color disappears
before further addition of permanganate solution. As the titration progresses it
win be noticed that the yeUow color gradually disappears, the solution turning prac-
tically colorless. It is at this stage of the titration that care should be taken in add-
ing only 2 drops of permanganate at a time.

Calculation. — One c.c. of N/io potassium permanganate is equivalent to 0.099
mg. of sulphur. Multiply the number of cubic centimeters of permanganate used
by 0.099 S'lid divide by 2 in order to obtain the weight of sulphur in i c.c. of urine.
Calculate the day's sulphur output.

Interpretation. — See page 549.

Phosphorus

I. Total Phosphates. — Uranium Acetate Method. — Principle. —
Standard uranium acetate is run into a measured quantity of urine
until all of the phosphate has been precipitated as insoluble uranium
phosphate. An excess of uranium is indicated by a reddish coloration
with potassium ferrocyanide. This method is accurate and gives
practically the total phosphorus of urine inasmuch as the latter exists
generally almost entirely as phosphates.

Procedvire. — To 50 c.c. of urine in a small beaker or Erlenmeyer flask add
5 c.c. of a special sodium acetate solution^ and heat the mixture to the boiling-
point. From a burette, run into the hot mixture, drop by drop, a standard solu-
tion of uranium acetate^ until a precipitate ceases to form and a drop of the mix-
ture when removed by means of a glass rod and brought into contact with a

* Six and seven-tenths grams of benzidine (Merck reagent) are put in a i-liter flask, 29
c.c. of hydrochloric acid (sp. gr. i. 12) added and the solution diluted up to the mark.

' The sodium acetate solution is prepared by dissolving 100 grams of sodium acetate in
800 c.c. of distilled water, adding 100 c.c. of 30 per cent acetic acid to the solution, and
making the volume of the mixture up to i liter with water.

' Uranium Acetate Solution. — Dissolve about 35.0 grams of uranium acetate in i liter
of water with the aid of heat and 3-4 c.c. of glacial acetic acid. Let stand a few days
and filter. Standardize against a phosphate solution containing 0.005 gram of P2O6 per
cubic centimeter. For this purpose dissolve 14.721 grams of pure air-dry sodium am-
monium phosphate (NaNH4HP04-l-4H20) in water to make a liter. To 20 c.c. of this
phosphate solution in a 200 c.c. beaker add 30 c.c. of water and 5 c.c. of sodium acetate
solution (see above) and titrate with the uranium solution to the correct end reaction as
indicated in the method above. If exactly 20 c.c. of uranium solution are required i c.c.
of the solution is equivalent to 0.005 gram P2O8. If stronger than this dilute accordingly
and check again by titration.

URINE 553

drop of a solution of potassium ferrocyanide on a porcelain test-tablet produces
instantaneously a brownish-red coloration.^ Take the burette reading and
calculate the P2O5 content of the urine under examination.

Calculation. — Multiply the number of cubic centimeters of uranium acetate
solution used by 0.005 to determine the number of grams of P;:05 in the 50 c.c.
of urine used. To express the result in percentage of P^Oj multiply the value
just obtained by 2, e.g., if 50 c.c. of urine contained 0.074 gram of P-Os it would
be equivalent to 0.148 per cent.

Calculate, in terms of P2O5, the total phosphate content of the 24-
hour urine specimen.

Interpretation. — The excretion of phosphoric acid is extremely
variable but on the average the total output for the 24 hours is about
2.5 grams expressed as PoOs- Ordinarily the total output is mainly in
the form of phosphates and is distributed between alkaline and earthy
phosphates in the ratio of 2 : i but this is likewise inconstant. The
greater part of the phosphate excretion arises from the ingested food,
either from the preformed phosphates or more especially from the
organic combinations as phospho- and nucleoproteins. The ex-
cretion is consequently very largely dependent upon the phosphorus
content of the diet. Some of the phosphoric acid results from the
breakdown of the tissues of the body, and this endogenous phosphoric
acid excretion is increased in conditions of increased metabolism as in
fevers. The findings in pathological conditions have been somewhat
contradictory due to lack of control of diet. The so-called "phos-
phaturias" nearly always represent decreased acidity and not in-
creased phosphate content of the urine. Such conditions are, however,
signiticant as indicating a possible tendency to the formation of phos-
phatic calculi.

2. Earthy Phosphates. — Principle. — The earthy phosphates are
precipitated by making the urine alkaline. The precipitate is filtered
off, dissolved in acid and titrated with uranium acetate.

Procedure. — To 100 c.c. of urine in a beaker add an excess of ammonium
hydroxide and allow the mixture to stand 12 24 hours. Under these conditions
the phosphoric acid in combination with the alkaUne earths, calcium and mag-
nesium, is precipitated as phosphates of these metals. Collect the precipitate
on a filter paper and wash it with very dilute ammonium hydroxide. Pierce
the paper, and remove the precipitate by means of hot water. Bring the phos-
phates into solution by adding a small amount of dilute acetic acid to the warm
solution. Make the volume up to 50 c.c. with water, add 5 c.c. of sodium acetate
solution, and determine the PjOj content of the mixture according to the direc-
tions given under the previous method.

Calculation. — Multiply the number of cubic centimeters of uranium acetate
solution used by 0.005 to determine the number of grams of PjOs in the 100 c.c.

^ A 10 per cent solution of potassium ferrocyanide is s;itisfactory.

554 PHYSIOLOGICAL CHEMISTRY

of iirine used. Since loo c.c. of urine was taken this value also expresses the
percentage of P2O5 present.

Calculate the quantity of earthy phosphates, in terms of P2O5, present in the
24-hour urine specimen.

The quantity of phosphoric acid present in combination with the alkali
metals may be determined by subtracting the content of earthy phosphates
from the total phosphates.

Interpretation: — Ordinarily the earthy phosphates make up from
30-40 per cent of the total phosphate excretion. The amount varies
with the excretion of calcium and magnesium (which see).

3. Total Phosphorus. — {a) Volumetric Procedure. — Principle. — The
organic matter is destroyed by digestion with a mixture of sulphuric
and nitric acids or some other oxidizing agent. The phosphorus is then
precipitated as the phosphomolybdate and determined gravimetrically
or volumetricall3\

Preparation of the Solution. — Pipette 10 c.c. of urine (or an amount of sub-
stance containing about 20 mg. of P2O5) into a Kjeldahl flask. Add 10 c.c. of a
mixture of equal parts of concentrated H2SO4 and concentrated HNO3. Digest
over a low flame until red fumes cease to come off. If the mixture darkens due
to the charring action of the sulphuric acid, add nitric acid from a separatory
funnel a few drops at a time and continue the digestion. When the mixture
remains clear on evaporation to the point where white sulphuric fumes come off
the digestion is completed by heating for 10-15 minutes longer. Cool and transfer
the solution to a 400 c.c. Erlenmeyer flask with the aid of enough water to
make a total volxune of about 75 c.c.^

Instead of oxidizing the material as described above it may be
ignited with magnesia to destroy organic matter. About 2 grams of
the solid substance or 25 c.c. of urine (previously evaporated nearly
to dryness) are mixed with a httle more than an equal bulk of mag-
nesium oxide in a porcelain dish of about 30 c.c. capacity. Five c.c.
of magnesium nitrate solution (see Reagents and Solutions, page 602)
are added and the mixture heated very gently at first, then gradually
to bright redness. The mixture is cooled and transferred with water
to a 250 c.c. flask. An excess (20-30 c.c.) of HCl are added and the
mixture boiled a few minutes. Remove from the flame and add at
once enough barium chloride solution to precipitate any sulphate
present. Cool, make to mark, filter and take an aliquot for analysis.

Precipitation of the Phosphomolybdate.^NeutraUze the solution with
ammonia, make slightly acid with nitric acid, and add 15 grams of ammonium
nitrate in substance (or 25 c.c. of a 60 per cent solution). Heat on a water-bath
to 6o-65°C. (not higher) and add 30-40 c.c. of molybdate solution,^ stir and let

' In the case of urine it is possible to neutralize this acid solution with ammonia, make
it acid with acetic acid and titrate with uranium acetate as in the preceding method.

2 Made by adding 5 c.c. of concentrated HNO3 to 100 c.c. of the ordinary molybdate
solution (see Reagents and Solutions, page 602).

URINE 555

stand for about 15 minutes at 60-65°. Filter at once through a small paper,'
washing the precipitate twice by decantation with 2 per cent ammonium nitrate
solution using about 25 c.c. each time, stirring up the precipitate well in each
case, and allowing to settle. Transfer the precipitate to the filter and wash with
2 per cent ammonium nitrate solution until two fillings of the filter (collected
separately) do not greatly diminish the color produced with phenolphthalein
by I drop of the standard alkaU.

Titration of the Phosphomolybdate. — Transfer the precipitate and filter
back to the original beaker and dissolve in a small excess of N 5 NaOH Tabout
2-3 c.c. more than required to completely dissolve the yellow precipitate . Add
about 100 c.c. of boiled and cooled water and a few drops of phenolphthalein
as an indicator (a red color should be observed indicating excess of NaOH)
and titrate the excess of NaOH with N/io acid.

Calculation. — Divide the number of cubic centimeters of N/io acid required
by 2 and subtract from the number of cubic centimeters of N 5 NaOH used.
This gives the number of cubic centimeters of N/5 NaOH required. Multiply
by 1.268 (the equivalent of i c.c. of N '5 NaOH in P2O5) and obtain the number
of milligrams of PX)i in 10 c.c. of the urine analyzed. Calculate the daily output
of P2O5 in this case from the 24-hour volume.

Interpretation. — Nearly all of the phosphorus of the urine exists as
alkali and earthy phosphates. Consequently the total phosphorus
varies in the same way as the total phosphates (which see). A small
portion of the phosphorus of the urine may exist in organic com-
bination though never in a reduced form. This organically bound
phosphate may amount to from 1-4 per cent of the total phosphorus
excretion. Little is known with regard to the compounds in which it
occurs. Possibly some glycerophosphoric acid may occur either free
or as lecithin.

Gravimetric Modification. — The phosphorus may be determined somewhat
more accurately by substituting a gravimetric procedure for the above titration.
In this case the washed phosphomolybdate precipitate is dissolved on the filter
paper with ammonium hydroxide and hot water to make a volmne of not more than
100 c.c. Nearly neutrahze with HCl, cool, and add about 10 c.c. of magnesia
mixture (see Appendix) from a burette. Add slowly (about i drop per second)
stirring vigorously. After 15 minutes add 12 c.c. of ammoniimi hydroxide
solution (sp. gr. 0.90). Let stand for some time (two hours is usually enough)
then filter and wash the precipitate with 2.5 per cent ammonia until practically
free from chlorides. Ignite to whiteness or to a grayish-white ash and weigh.
Multiply the weight of magnesium pyrophosphate thus obtained by 0.637 to get
the weight of PjOs.

Calculation. -Calculate as explained above.

' It is better to use a special filter tube of about i }-^ inches diameter (similar to a Gooch
filtering tube) in which is placed a perforated porcelain plate i ' s inches in diameter, covered
with a layer of asbestos 1/8 inch tliick. Filtration is carried out with suction and is very
rapid. Ordinary Gooch crucibles lined with asbestos may also be used but arc not so s;itis-
factory. The asbestos used should be specially prepared (see Appendix). For a good dis-
cussion of the details of procedure and sources of error of this volumetric method sec
Hibbard: /. Ind. Eng. Chein., 5, 098, 1913.

556 PHYSIOLOGICAL CHEMISTRY

Chlorides

I. Volhard -Arnold Method. — Principle.— The urine is acidified
with nitric acid and the chlorides precipitated with a measured excess
of standard silver nitrate solution. The silver chloride formed is
filtered off and in the filtrate the excess silver nitrate is titrated
back with standard ammonium thiocyanate solution. Ferric am-
monium sulphate is used as an indicator. A red color due to the forma-
tion of ferric thiocyanate indicates that an excess of thiocyanate is
present and that the end point has been reached.

Procedure. — Place 10 c.c. of urine in a 100 c.c. voliimetric flask, add 20-30
drops of nitric acid (sp. gr. 1.2) and 2 c.c. of a cold saturated solution of ferric
altim. If necessary, at this point a few drops of 8 per cent solution of potassium
permanganate may be added to dissipate the red color. Now slowly run in a
known volimie of the standard silver nitrate^ solution (20 c.c. is ordinarily used)
in order to precipitate the chlorine and insure the presence of an excess of silver
nitrate. The mixture should be continually shaken during the addition of the
standard solution. Allow the flask to stand 10 minutes, then fill it to the 100
c.c. graduation with distilled water and thoroughly mix the contents. Now
filter the mixture through a dry filter paper, collect 50 c.c. of the filtrate and
titrate it with standardized ammoniimi thiocyanate solution. ^ The first per-
manent tinge of red-brown indicates the end point. Take the burette reading
and compute the weight of sodium chloride in the 10 c.c. of urine used.

Calculation. — The number of cubic centimeters of ammonium thiocyanate
solution used indicates the excess of standard silver nitrate solution in the
50 c.c. of filtrate titrated. Multiply this reading by 2, inasmuch as only one-half
of the filtrate was employed, and subtract this product from the number of cubic
centimeters of silver nitrate (20 c.c.) originally used, in order to obtain the actual
number of cubic centimeters of silver nitrate utilized in the precipitation of the
chlorides in the 10 c.c. of urine employed.

To obtain the weight in grams of the sodium chloride in the 10 c.c. of urine
used, multiply the number of cubic centimeters of the standard silver nitrate
solution, actually utiUzed in the precipitation, by o.oio. If it is desired to express
the result in percentage of sodium chloride move the decimal point one place
to the right.

In a similar manner the weight, or percentage of chlorine may be computed
using the factor 0.006 instead of 0.0 10.

^ Standard silver nitrate solution may be prepared by dissolving 29.042 grams of silver
nitrate in i liter of distilled water. Each cubic centimeter of this solution is equivalent to
O.OIO gram of sodium chloride or to 0.006 gram of chlorine.

'^This solution is made of such a strength that i c.c. of it is equal to i c.c. of the stand-
ard silver nitrate solution used. To prepare the solution dissolve 13 grams of ammonium
thiocyanate, XHS4CN, in a little less than a liter of water. In a small flask place 20 c.c.
of the standard silver nitrate solution, 5 c.c. of the ferric alum solution and 4 c.c. of nitric
acid (sp. gr. 1.2), add water to make the total volume 100 c.c. and thoroughly mix the con-
tents of the flask. Now run in the ammonium thiocyanate solution from a burette until a
permanent red-brown tinge is produced. This is the end-reaction and indicates that the
last trace of silver nitrate has been precipitated. Take the burette reading and calculate
the amount of water necessary to use in diluting the ammonium thiocyanate in order that
10 c.c. of this solution may be e.xactly equal to 10 c.c. of the silver nitrate solution. Make
this dilution and titrate again to be certain that the solution is of the proper strength.

URINE 557

Calculate the quantity of sodium chloride and chlorine in the 24-hour urine
specimen.

Interpretation. — From 10-15 grams of chlorine, expressed as sodium
chloride, are excreted per day, on the average, by normal adults. The
amount is, however, closely dependent upon the chloride content of
the food ingested. In fasting, the chloride excretion falls rapidly to
a very minimal quantity. On high water ingestion it is increased.
In pneumonia and certain other acute infectious diseases the excretion
of chlorides may be markedly diminished particularly during the
periods in which exudates are forming. In convalescence and with
resolution of the exudates the chlorine excretion rises again. A de-
crease has also been noted in nephritis associated with edema.

2. VoLhard -Harvey Method.^ — Principle. — This procedure diflfers
from the Volhard-Arnold method in that the excess of silver nitrate
is titrated directly without filtering and hence in the presence of the
silver chloride. The procedure is thus more rapid but the exact end
point is more difiicult to determine.

Procedure. — Introduce 5 c.c. of urine into a small porcelain evaporating
dish or casserole and dilute with about 20 c.c. of distilled water. Precipitate
the chlorides by the addition of 10 c.c. of standard silver nitrate solution- and
add 2 c.c. of acidified indicator.^ Now run in a standard ammonixun thiocyanate
solution^ from a burette until a faint red-brown tint is visible throughout the
mixture. This point may be determined readily by permitting the precipitate
to settle somewhat. Calculate the sodiimi chloride value as indicated below.

(If a red tint is produced when the first drop of thiocyanate is added an addi-
tional 10 c.c. of the standard silver nitrate solution must be introduced. The
titration should then proceed as above described and proper allowance made in
the calculation for the extra volimie of silver nitrate employed.)

Calculation. — Since 2 c.c. of the ammoniiun thiocyanate solution is equivalent
to I c.c. of the silver nitrate solution, divide the burette reading by 2 and sub-
tract the quotient from 10 c.c, the quantity of silver nitrate solution taken.
This value is the niunber of cubic centimeters of silver nitrate solution actually

1 Harvey: Archives of Internal Medicine, 6, 12, 19 10.

2 See p. 556.

'This is prepared as follows: To 30 c.c. of distilled water add 70 c.c. of 33 per cent
nitric acid (sp. gr. 1.2) and dissolve 100 grams of crystalline ferric ammonium sulphate in
this dilute acid solution. Filter and use the filtrate which is a saturated solution of the iron
salt. This single reagent takes the place of the nitric acid and ferric alum as used in Vol-
hard-Arnold method, and insures the use of the proper quantity of acid.

* This is a solution of ammonium thiocyanate of such a strength that 2 c.c. is equivalent
to I c.c. of the silver nitrate solution. First make a concentrated solution by dissolving 13
grams in i liter of water. To determine the requisite dilution to make such a solution that
2 c.c. shall be equivalent to i c.c. of the silver nitrate solution proceed as follows: Introduce
10 c.c. of the silver nitrate solution into a small porcelain evaporating dish or casserole, add
30-50 c.c. of distilled water, 2 c.c. of the acid indicator and titrate as described above with
the ammonium thiocyanate solution. The total volume of the concentrated thiocyanate
solution excluding that used in this titration is divided by 10, and the result multiplied by
the difiference between this burette reading and 20 c.c. This will give the volume of dis-
tilled water which must be added to the concentrated thiocyanate solution to render 2 c.c.
equivalent to i c.c. of the silver nitrate solution.

558 PHYSIOLOGICAL CHEMISTRY

used in the precipitation of the chlorides. As i c.c. of the silver nitrate solution
is equivalent to o.oi gram of sodixim chloride, the nxunber of cubic centimeters
of silver nitrate solution used multiplied by o.oi gram will give the weight of
sodium chloride in the 5 c.c. portion of urine used. The weight of chlorine may
be computed by using the factor 0.006 instead of o.oi.

Calculate the weight of sodium chloride and chlorine in the 24-hour urine
specimen.

A "short cut" method of calculating the 24-hour output of sodium chloride
consists in subtracting the burette reading from 20 c.c, multiplying this value
by the total mine volume and pointing off three places.

Interpretation. — See above.

3. Dehn-Clark Method^ — Principle. — In this method any organic matter
which may interfere with the titrimetric determination of the chlorides is destroyed
by oxidation with sodium peroxide. The chlorides are then determined by the Vol-
hard-Arnold titration procedure.

Procedure. — To 10 c.c. of urine in a 75-100 c.c. casserole, add i. 0-1.2 grams of
sodium peroxide and evaporate the mixture to dryness on a boiling water-bath. In
case the residue is not pure white, thus indicating that insufficient sodium peroxide
has been added, the residue should be moistened with distilled water, additional
sodium peroxide added, and the mixture again evaporated to dryness. When the
oxidation is complete, treat the mass with 10-20 c.c. of distilled water and stir
untU it has practically all been brought into solution. Then introduce a bit of lit-
mus paper and add dilute nitric acid (i: i) until the litmus paper turns red and all
efervescence ceases. Now place the casserole on a hot plate or on a gauze and heat
the contents almost to the boiling-point.^ To the hot solution add a standard solu-
tion of silver nitrate (see page 556) in slight excess.' Filter off the silver chloride
whUe the solution is still hot and wash the precipitate thoroughly with distilled
water. To the filtrate, add i c.c. of a saturated solution of ferric ammonium sul-
phate and then titrate with a standard solution of ammonium thiocyanate (see page
556) untU the clear, slightly yellow fluid (or the opalescent, milky fluid, in case there
is much excess of silver nitrate) changes to a slight reddish-brown color. The color
of the end point varies with the individual. The exact end point reached is not so
important as is the securing of the same end point in a series of determinations as
that obtained in the standardization of the standard solutions used.

Calculation. — The standard solution of silver nitrate should be made up so that.
I c.c. equals o.oio gram of sodium chloride and i c.c. of the ammonium thiocyanate
should be equivalent to i c.c. of the silver nitrate solution. The calculation is then
exactly the same as in the Volhard-Arnold method (page 556) except that the
burette reading is not multiplied by 2.

Interpretation. — See page 557.

4. Mohr's Method. — Principle. — The organic matter of the urine is destroyed
by ignition with potassium nitrate. To the solution of the ash potassium chromate
is added and then standard silver nitrate solution run in from a burette. The first

' Private communication to the author from Mr. S. C. Clark.

- If there is a slight precipitate, due to silicic acid from the casserole, this is filtered ofif
and the filtrate collected in a 200 c.c. beaker.

3 This point is most easily recognized by keeping the solution hot and in constant agita-
tion while adding the silver nitrate so that the silver chloride formed coagulates and sinks,
leaving a clear, supernatant fluid.

URINE 559

excess of silver nitrate over that necessary to precipitate the chlorides reacts with the
chromate to form red silver chromatc (Ag2Cr04). This indicates the end point.
The method is accurate when applied to the ash of urine in this manner.

Procedure. — To lo c.c. of urine in a small platinum or porcelain crucible or dish
add about 2 grams of chlorine-free potassium nitrate and evaporate to dryness at
ioo°C. (The evaporation may be conducted over a low flame provided care is taken
to prevent loss by spurting.) By means of crucible tongs hold the crucible or dish
over a free flame until all carbonaceous matter has disappeared and the fused mass is
slightly yellow in color. Cool the residue somewhat and bring it into solution in a
small amount (15-25 c.c.) of distilled water acidified with about 10 drops of nitric
acid. Transfer the solution to a small beaker, being sure to rinse out the crucible or
dish very carefully. Test the reaction of the fluid, and if not already acid in reac-
tion to litmus, render it slightly acid with nitric acid. Now neutralize the solution
by the addition of calcium carbonate' in substance, add 2-5 drops of neutral potas-
sium chromate solution to the mixture, and titrate with a standard silver nitrate
solution.

This standard solution should be run in from a burette, stirring the liquid in
the beaker after each addition. The end-reaction is reached when the yellow color
of the solution changes to a slight orange-red. At this point take the burette read-
ing and compute the percentage of chlorine and sodium chloride in the urine
examined.

Calculation. — The calculation is made exactly as in the Volhard-Arnold
method, page 556, except that the reading is not multiplied by two.

Calculate the quantity of sodium chloride and chlorine in the twenty-four-
hour urine specimen.

Interpretation. — See page 557.

Calcium and Magnesium

McCrudden's Methods. ^^ — Principle. — Urine contains magnesium,
phosphates and a small amount of iron, each of which will interfere
with the accurate determination of its calcium content if proper con-
ditions of acidity are not maintained during the precipitation. In the
following method the proper acidity is attained through the use of
sodium acetate and hydrochloric acid, and this with slow addition of
the ammonium oxalate reduces the danger of occlusion of magnesium
oxalate, calcium phosphate, or ferric phosphate in the calcium oxalate
precipitate.

The calcium oxalate precipitate is either ignited and weighed as
CaO or determined volumetrically by titration with potassium per-
manganate. Magnesium is determined in the filtrate from the calcium
determination after destruction of the organic matter. It is determined
in the usual way by ignition of the magnesium ammonium phosphate
precipitate and weighing as the pyrophosphate.

'The cessation of effervescence and the presence of some undecomposed calcium
carbonate at the bottom of the vessel are the indications of neutralization.
^McCrudden: Jour. Biol. CItem., 7, 83, 1910; 10, 187, 191 1.

560 PHYSIOLOGICAL CHEMISTRY

Lyman has suggested a nephelometric method ioj: the determination
•of calcium in urine and feces. ^

Procedure for Calcitun. — ^If the urine is alkaline make it neutral or slightly
acid and filter. Take 200 c.c. of the filtered urine for analysis. If it is only
faintly acid to Utmus paper add 10 drops of concentrated hydrochloric acid (sp.
gr. 1.20). If the urine is strongly acid it may be made just alkaUne with ammonia
and then just acid with hydrochloric acid after which the 10 drops of concentrated
hydrochloric acid are added. Then add 10 c.c. of 2.5 per cent oxalic acid. Run
in slowly with stirring 8 c.c. of 20 per cent sodiimi acetate. Allow to stand over
night at room temperature or shake vigorously for ten minutes. Filter off the
precipitate of calcixun oxalate on a small paper and wash free from chlorides
with 0.5 per cent ammonium oxalate solution. The precipitate may then be
dried, ignited to constant weight and weighed as calcium oxide or it may be
manipulated voliunetrically as described below.

Volumetric Procedure. — ^If free from uric acid the calcium oxalate precipitate
may be washed three times with distilled water, filling the filter about two-
thirds full and allowing it to drain completely before adding more. A hole is
made in the paper and the calcitmi oxalate washed into the flask. The volmne
of the fluid is brought up to about 50 c.c. and 10 c.c. of concentrated sixlphuric
acid added. Titrate with standard potassimn permanganate solution to a pink
color which endures for at least a minute.

Calculation. — One c.c. of N/io permanganate solution is equivalent to 2.8
mg. of CaO. Calculate the daily output of calciimi expressed as CaO.

Interpretation. — The average urinary excretion of calcium by normal
adults lies between o.i to 0.4 gram (expressed as CaO) per day. It is
dependent very largely upon the amount of calcium in the diet. From
10 to 40 per cent of the ingested calcium ordinarily is excreted by this
channel, the greater part being eliminated by the feces. The pro-
portion is dependent particularly on the amount of calcium in the food.
If the calcium ingestion is very high the per cent of the total excretion
taking place by way of the kidneys will be low, and vice versa. As ex-
cretion takes place by way of the intestine as well as by the kidneys no
conclusions can be drawn from urinary analyses alone. The excretion
of calcium may be greatly increased in certain bone disorders as osteo-
malacia. In others as in rickets the urinary excretion may be very
low.

Procedure for Magnesium. — Transfer the filtrate from the determination
of calciimi as above to a porcelain dish, add about 20 c.c. of concentrated nitric
acid and evaporate to dryness. Heat the residue over a free flame until the
ammonium salts are destroyed and the residue fuses. After cooUng take the
residue up with water and a Uttle hydrochloric acid and filter if necessary.
Dilute to about 80 c.c, nearly neutraUze with ammonia and cool. Add a slight
excess of sodium acid phosphate and then ammonia drop by drop with constant
stirring until the solution is alkaline and then add enough more slowly with

'Lyman: Jour. Biol. Ckem., 21, 551, 1915.

URINE 561

constant stirring to make the solution contain one-fourth its bulk of dilute
ammonia fsp. gr, 0.96). Allow to stand over night. Filter and wash free from
chlorides with alcoholic ammonia solution f i part alcohol, i part dilute ammonia,
3 parts water). The precipitate with filter paper is incinerated slowly and care-
fully with good supply of air to prevent reduction, in the usual manner, and ignited
and weighed as the pyrophosphate.

Calculation. — To obtain the weight of MgO multiply the weight of magnesium
pyrophosphate by 0,3624.

Interpretation. — The daily excretion of magnesium by way of the
urine usually amounts to between o.i and 0,3 gram (expressed as MgO).
The amount depends mainly upon the diet. Usually 50 per cent or
more of the excreted magnesium is eliminated by the kidneys, the re-
mainder passing out in the feces. The proportion varies, however, and
it is impossible to draw any conclusions from the urinary output alone.
There may be a retention of magnesium in certain bone disorders ac-
companying a loss of calcium; in osteomalacia for example. Thus the
excretions of calcium and magnesium do not necessarily run parallel.

Determination of Calciiun in Ash of Foods or Feces. — Ignite the material in a
crucible to a white ash and dissolve the ash with the aid of a little hydrochloric acid.
Bring the volume of the ash solution to 75-150 c.c. INIake just alkaline with strong
ammonia added drop by drop (using litmus paper or alizarin as an indicator). Add
concentrated HCl drop by drop until just acid to litmus. Then add 10 drops of
concentrated HCl (sp. gr. 1.20), and 10 c.c. of 2.5 per cent oxalic acid. Either
of two procedures may then be followed, (a) The solution is boiled until the pre-
cipitated calcium oxalate is coarsely crystalline, and then an excess of 3 per cent
ammonium oxalate is slowly added to the boiling solution and the boiling continued
until the precipitate is coarsely crystalline. (If but little calcium is present nothing
will precipitate at this point and it is not necessary to add oxalate.) Or {b) the
flask closed with a rubber stopper is shaken vigorously for ten minutes, An excess
of 3 per cent ammonium oxalate is then added. Cool to room temperature. Add
8 c.c. of 20 per cent sodium acetate solution. (In case of ash of feces add 15 c.c.)
The solution may either be (c) allowed to stand over night or {b) stoppered and
vigorously shaken for ten minutes. The calcium oxalate is filtered off on a small
ash-free paper and washed free from chlorides with 0.5 per cent ammonium oxalate
solution. Either of two procedures may next be followed, (a) The precipitate
and filter are dried, burned in a platinum or porcelain crucible to constant weight as
CaO, {b) The precipitate is washed three times with cold distilled water, as given
under the method for urine and the oxalate titrated with potassium permanganate.

Magnesium is determined in the filtrate from calcium just as given above.

Sodium and Potassium

Determination of Combined Sodiimi and Potassium, irum ^c tu 100 c.c. of

urine, depending upon the s()ocilk gravity, arc oxidized in a Kjeldahl flask with

nitric and sulphuric acids as in the Neumann procedure tor total phosphorus (see

page 554). To remove the sulphuric acid as comnl'f'K >- i>ossiblc transfer with

36

62 PHYSIOLOGICAL CHEMISTRY

the aid of a little water to a platinum dish and evaporate to drj^ness over a free
flame. (The alkalies are in the form of sulphate and do not volatilize.) Dissolve
the residue in hot water with the aid of a little dilute hydrochloric acid. Heat to
boiling and add barium chloride solution until no more precipitate forms. While
still hot add an excess of ammonia and ammonium carbonate. The barium chlor-
ide precipitates the sulphates and part of the phosphates: the ammonia in the
presence of excess barium precipitates the rest of the phosphates, and the carbonate
precipitates the calcium and most of the magnesium, as well as the excess barium.
Filter and wash the precipitate well with hot water containing a few drops of am-
monia. Evaporate filtrate and washings to dryness and heat the residue to dull
redness for a moment. Redissolve in water and treat again with ammonia and
ammonium carbonate to remove any remaining alkaline earth metals. FUter and
wash as before. Transfer filtrate and washings to a weighed platinum dish, add a
few drops of hydrochloric acid and evaporate to dryness. Heat the residue gently
to remove ammonium salts and then to dull redness for a moment. Desiccate
and weigh. Reheat to constant weight which represents the combined chlorides
of sodium and potassium. The reagents used in the determination must be tested
and found free from alkali metals or a correction made for the alkali metals present
in the reagents used. The sodium is determined by difference after potassium has
been estimated by the method given below.

Potassium, — Dissolve the alkaH chlorides from the preceding determination in a
little water and add a slight excess of lo per cent platinic chloride over that neces-
sary to precipitate all of the alkali present calculated as sodium chloride (about 1 7
c.c. being required for each gram of sodium chloride). Evaporate to a syrupy con-
sistencj- on the water-bath and add about 50 c.c. of 80 per cent alcohol. Stir
occasionally for a few minutes. This operation must be carried out in the absence of
ammonia vapors. Filter through a weighed Gooch crucible, washing the precipi-
tate with 80 per cent alcohol first thoroughly by decantation and then on the filter,
for some time after the filtrate is colorless. Dry at iio-ii5°C. and weigh.

Calculation. — ^Multiply the weight of potassium platinic chloride by 0.1941 to
obtain the amount of K2O present. Express as KCl by using instead of this factor
the factor 0.30712. Subtract from the \\ eight of total alkali chlorides as determined
in the preceding method, the weight of potassium chloride as calculated and obtain
the amount of sodium chloride present.

Interpretation. — The average alkali excretion of an adult on a mixed diet is about
2-3 grams of potassium expressed as KoO and 4-6 grams of sodium expressed as
Xa20. The ratio of Na to K is thus about 5:3. Both the ratio and the absolute
amounts of these elements excreted are, however, largel}' dependent upon the salt
content of the diet. Because of the non-ingestion of sodium chloride and the
accompanying destruction of potassium-containing body tissues, the urine during
fasting contains more potassium than sodium salts. The excretion of the bases,
particularly K, maj' be increased in fevers and in acidosis.

Iron

Method ofWolter.' — Principle. — The urine is ashed, the ash dissolved, and the
iron present oxidized to the ferric form by means of hydrogen peroxide. The iron is
then determined iodometrically.

' Wolter: Bioch. Zeil., 24, 108. iqio.

URINE 563

Procedure. — The 24-hour specimen of urine is treated with 30 c.c. of concen-
trated iron-free nitric acid and then evaporated to low volume in a large evaporating
dish on the water-bath. Transfer to a small evaporating dish. Heat to dryness on
the sand bath and then char, using a small flame. Transfer the charred mass by
means of a glass spatula to a crucible. The remaining material in the evaporating
dish is transferred with the aid of a little hot water and a rubber "policeman" to a
second crucible. Evaporate to dryness on the water-bath and then ash the material
in both crucibles. Dissolve the ash in about 30 c.c. of iron-free hydrochloric acid,
transfer to an Erlenmeyer flask, add 2 c.c. of hydrogen peroxide and boil for three-
quarters of an hour. After cooling, 2 grams of potassium iodide and a few drops of
fresh starch paste are added. The liberated iodine is titrated with X/ioo thiosul-
phate solution. Controls should be run on reagents. A correction of 0.32 mg. is
usually necessary for the undecomposed hydrogen peroxide. The thiosulphate solu-
tion is made up as needed from an N/io stock solution by dilution. It is standard-
ized against an iron solution containing 2 mg. of iron in 10 c.c. The number of
cubic centimeters of thiosulphate used in titration of the iodine set free from the
ash solution is multiplied by the iron equivalent of i c.c. of the thiosulphate (about
0.2 mg.) to obtain the total amount of iron in the 24-hour specimen of urine. From
1-5 mg. of iron are usually excreted per day.

CHAPTER XXVII
METABOLISM

Metabolism is a part of that complex series of processes grouped
together under the head of Nutrition. It embraces a consideration
of those changes taking place in the body other than those customarily
classified as secretion, digestion, excretion, etc. Metabolism may be de-
fined as all chemical and physical changes which occur in living matter
and which constitute the basis of the material phenomena of life. This
conception of metabolism holds for the simple individual cell of the
amoeba as well as for the complex mechanism of the human body. There
are two types of metabolism, one constructive, the other destructive.
The constructive metabolism is termed anabolism; the destructive
metabolism is termed catabolism.
Thus:

,, ^ , ,. ( Anabolism (constructive metabolism).

Metahohsm „ , ,. ,, . ■, t n

[ Lataboksm (destructive metabolism).

In general we may say that the main bulk of the food-stuffs of the diet,
i.e., protein, fat and carbohydrate, is transformed in the gastro-in-
testinal tract and that the end-products of this transformation are
carried to the cells of the body and there built up by anabolic (synthetic)
processes into cell structure or stored as a reserve to be used as required.
All living cells undergo wear and tear in the course of their life cycle.
By catabolic (cleavage) processes therefore a portion of the living cell
substance or of the stored material is reduced to simpler fragments and
these are eliminated from the body after having yielded the bulk of
their energy in the form of heat or mechanical work. It is apparent,
therefore, that the chemical side of metabolism is closely associated
with the physical side. Each of the three types of food-stuffs (protein,
fat and carbohydrate) is concerned with the upkeep of the tissues and
with the liberation of energy. It is true, however, that the main
burden of the upkeep falls upon the proteins whereas the combustion of
fats and carbohydrates yields the major portion of the required energy.
The above facts are embraced in the following scheme:

564

METABOLISM 565

THE CELL

PROTEIN. FAT, 1 , ^^,^ t,.,^^,.^ „

CARBOHYDRATE / ^ ^ END-PRODUCTS

COMBUSTION

Without doubt both anabolic and catabolic processes are going on in-
cessantly within every individual living cell. At one time the anabolic
phase will be more prominent; at another the catabolic activity will be
in the ascendency. It should also be borne in mind that metahoUsm
implies a transfonnation of energy as well as an exchange of materials.

For further brief discussions of certain phases of metabolism see
the following experiments. A detailed discussion being out of place
in this volume, the reader is referred to the following books :

(i) Taylor's "Digestion and ]\Ietabolism, " Lea and Febiger, 191 2.

(2) Sherman's " Chemistry of Food and Nutrition," Macmillan.

(3) Osier & McCrae's "Modern Medicine," Vol. II, Second Edi-
tion, 1914, Lea and Febiger. The author's section on "General Con-
sideration of ^Metabolism, " pages 549-673.

METABOLISM EXPERIMENTS

I . Metabolism Procedures Involving the Manipulation of the Urine

1. Collection and Preservation of the Urine. — In metabolism tests,
such as those given in this chapter the accurate collection of the urine
for the exact 24-hour period is of the utmost importance. Proceed as
follows: Empty the bladder at a given hour, e.g., 8 a.m. and discard tJie
urine. Prepare a thoroughly clean bottle of proper size, introduce into
it sufficient toluene to cover the bottom of the bottle and use this bottle
for the collection of all urine voided from 8 a.m. until 8 a.m. the next
day. During the day, when not actually in use for the introduction
of a urine fraction, the bottle should be kept in a refrigerator or cold
room in order that the sample may not deteriorate before it is examined.
Measure the volurne of the sample and determine its specific gravity
(see Chapter XXI) and reaction before proceeding to the quantitative
estimation of any specific urinary constituents.

2. Complete Analysis of Urine. — Ingest an ordinary mixed diet (or any special
diet) and collect the urine accurately for a 24-hour period (see above). Measure
the volume of the sample, determine the specific gravity and preserve the urine
(see above) until the following constituents have been determined (for Methods

566

PHYSIOLOGICAL CHEMISTRY

of Analysis, see Chapter XXVI). Total solids, titratable acidity, hydrogen ion
concentration, total nitrogen, amino-acid nitrogen, ammonia, urea, uric acid,
creatinine, total sulphur, ethereal sulphates, inorganic sulphates, neutral sulphur
(by difference) total phosphates and sodiiun chloride.

Calculate the nitrogen and sulphur "partitions," i.e., the percentage of the
total nitrogen and sulphur which occur in the different forms and tabulate the data
from the complete analysis. Compare your results with those listed in the table
on pages 371 and 578.

3. Hyperglycemia Produced by Carbohydrate Ingestion.^The

average glucose content of normal blood is somewhat less than o.i per
cent. This is increased (hyperglycemia) on the ingestion of carbo-
hydrate food. The increase is noted more quickly after the ingestion of

0.18

T'

\

"^

A

\

a

II

\

\

4

1
1
1

\

\
\

_B__

\

^

1/

V'^x

_C--

il

n

y'

\
\

\

^--^

-^^^

om

^V,s.

^ \

iKr--^

"^^

^\

Vz

Fig. 169.

J'/z

Z ZVz 3
Hours

3Vz

^Vz 5

-Blood Sugar as Influenced by Diet.
A = glucose; B — starch;
C = starch and fat; D = fat.

monosaccharides than after the ingestion of the more complex carbo-
hydrates. After the ingestion of 100 grams of glucose or starch an
increase in the sugar of the blood sometimes occurs in five minutes.^
(See Fig. 169.)

(a) Influence of Glu(iose. — In the morning before breakfast, or three to five
hours after breakfast, determine the normal sugar content of your blood by means
of some accurate micromethod. (See Chapter XVI.) Ingest 100 grams of
glucose dissolved in 250 c.c. of water, and again determine the blood sugar
level at intervals of 5, 15 and 30 minutes and one, two and three hoiirs. (Plot
a curve similar to the one shown in Fig. 169. The urine may also be examined
for sugar at intervals of one hour after the sugar ingestion.

Repeat the experiment on another day using 250 grams of glucose and com-
pare the results with those obtained after the ingestion of 100 grams. Explain
your findings. If desired this experiment may be combined with the ones on
"Alimentary Glycosuria," and " Carbohydrate in Feces," see pages 568 and 591.

1 Jacobson: Bioch. Zeit., 56, 471, 1913.

METABOLISM 567

(b) Influence of Starch. — Repeat the experiment as given above for glucose
except that 170 grams of white bread or 100 grams of starch made into a paste-
are substituted for the 100 grams of glucose.

The experiment may be repeated as described above using an increased
amount of starch.

The various experiments may be conducted on patients suffering from dia-
betes meUitus if such are available and instructive data collected. The ahmen-
tary hyperglycemia will generally be more prolonged than in the case of normal
subjects.

4. Influence of Physical Exercise upon Blood Sugar. — After strenuous physical
exertion by a normally nourished individual there is an increase in the sugar concen-
tration of the blood. ^ Similar increases are not shown by resting individuals simi-
larly nourished nor by fasting individuals after strenuous physical exercise. This
point is illustrated in the following protocol:

INFLUENCE OF PHYSICAL EXERCISE OX BLOOD SUGAR (Normal Man)

' Blood Blood

Day Experimental conditions examined, sugar,

hour per cent

Normal.

7 A. M.

0.043

Marched 8 miles in 2 hours ; ate 200 grams sucrose.

12 A.M.

0 080

Normal. 1

7 A. M. '

0.045

Complete rest; ate 200 grams sucrose.

12 A.M.

0 055

1 Fasting and complete rest.

7 A. M.

0.047

1
Fasting and complete rest.

12 A.M.

0.045

Fasting.

7 A. M.

0.047

Fasting and 2 -hour march (8 miles). ' 12 A. M. , 0.053

The increase in blood sugar under the influence of exercise occurs rather sooner in
the diabetic organism. Typical data follow:

Experiment. — Ingest a simple uniform diet (see Experiment 34, page 592) for
five days taking the first meal after 12 o'clock (noon) and the last one before 10
P. M. On the morning of the second day (7 .\. M.) determine the sugar in your
blood (see methods, Chapter X\T). About three hours later take a brisk walk
for 8 miles covering the distance in about two hours and consume 200 grams
sucrose during the walk. Make a second analysis of the blood sugar. On the third
day analyze your blood for sugar at 7 A. M. and again at noon, remaining quiet in
the meantime. The fourth day should be passed without physical exertion whereas
on the second day between 10 A. M. and 12 M. a brisk S-mile walk is taken but no

' In making starch paste, rub up the dry starch in a mortar wiiJi cold water and pour the
suspended starch granules into boiling water and stir.
* Moraczewski: Bioch. Zeit., 71, 268, 1915.

568 PHYSIOLOGICAL CHEMISTRY

sucrose ingested. Sugar analyses should be made at 7 A. M. and 12 M. each day.
INFLUENCE OF EXERCISE ON BLOOD SUGAR (Diabetes Patient)

Blood

Blood

.^^^^•^ su^'ar .

Day examined, ° ' Experimental conditions

hour

per
cent

I I

8 A. M. 0.062 j Rest. Diet consisting of 2500 grams milk, 300 grams
I bread, 50 grams fat.

8 A. M. 0. 120 Eight-mile march (2 hours). Diet as above.

3 P. M. 0.08s

8 A. M. 0.055 t Rest. Diet as on first day.

3 P. M.

0.050

Rest. Diet as on first day.

8 A. M.

0.050

Rest. Diet as on first day.

4

3 P. M.

O.OS5

Rest. Diet as on first day.

5

8 A. M.

1

0.084

Eight-mile march (2 hours).

Diet as on first day.

Calculate your results, tabulate them and compare them with those given above.

5. Alimentary Glycosuria. — Normal urine contains a trace of glucose but not
enough to permit detection by the ordinary tests used in urinary analysis. If
more glucose is ingested than can be absorbed and assimilated by the body the
excess will be eliminated in the iirine. The "assimilation limit" for the glucose
has been exceeded, and a transient alimentary glycosuria results. To demon-
strate this, glycosuria proceed as follows : Before breakfast or luncheon empty
the bladder and test the urine for sugar by any reliable test (see Chapter XXXII).
If the test is negative, ingest along with the other articles of diet, 250 grams of
glucose, sucrose, or lactose dissolved in water. Empty the bladder at the end
of every hour for a period of three hours and test the urine for reducing sugar
and the sugar ingested.

Was there any glycosuria and if so how soon after the sugar ingestion did it
appear? If no glycosuria resulted repeat the test on a subsequent day using
a larger quantity of sugar. If desired, the sugar in the urine may be
determined quantitatively by one of the methods given in Chapter XXVI.

This experiment may be made more complete by making determinations of
blood sugar at short intervals as described in Experiment 3, page 566. If
desired, data on glycosuria, hyperglycemia and carbohydrate in feces (page 591)
may be collected from one experiment.

6. Absorption of Carbohydrate as Influenced by Fat Ingestion. — When fat is
eaten along with carbohydrate food the absorption of the latter is somewhat
delayed. This has been shown experimentally.^ To demonstrate the point pro-
ceed as follows: Determine the content of sugar in the blood at various intervals

^ Jacobson: Bioch. Zeit., 56, 471, 1913.

METABOLISM 569

after the ingestion of 170 grams of white bread as described in Experiment 3(b),
page 567. Plot a curve for these values similar to the one shown in Fig. 169, page
566. On a later day repeat the experiment and ingest 1 70 grams of white bread and
85 grams of butter. Plot the curve for these blood sugar concentrations along with
blood sugar values obtained after the ingestion of white bread as described above.
Has the fat exerted any influence upon the absorption of the carbohydrate? Re-
peat the above experiment on a case of diabetes mellitus if such is available and
note that fat exerts the same influence upon carbohydrate absorption as it exerts in
the normal human bod)'.

7. Time Relations of Protein Metabolism. — It is a well-known

physiological fact that an interval elapses between the ingestion of protein
food and the appearance in the urine of certain products representing the
complete catabolism of this food. For example, if one ingests an excess
of protein material an interval elapses before the urine gives evidence
of the complete excretion of certain products representative of the
catabolism of the protein. Urea is the chief of these. The term "nitro-
gen lag" has been used to designate the period elapsing between the
ingestion of protein and the excretion in the urine of a quantity of
nitrogen equivalent to that contained in the protein.

Experiment. — Ingest a simple uniform diet whose exact composition has been
determined by analysis or whose approximate composition has been estimated.
(See table below.) Continue this diet from one to four days. Collect the
urine in two-hour periods from 7 A. M. to 1 1 P. M. and in an eight-hour period be-
tween II P. M. and 7 A. M. Analyze each specimen for total nitrogen or urea.
At the end of this preliminary period add to the uniform diet, at one meal, a
weighed quantity (150-250 grams) of lean meat specially prepared and analyzed.
Collect the urine in periods as before and determine total nitrogen or urea.
Calculate the total nitrogen or urea excretion; tabulate the data and plot curves
showing the course of the nitrogen excretion on the various days of the experi-
ment. How long was the "nitrogen lag?"

COMPOSITION' OF COMMON FOODS'

Food

1 Water

Protein
(NX6.2S)

Fat

' Carbo-
hydrates

Ash

Calories per
pound

Beef

Loin
Ribs
Round

Percent
61.3
57. 0
67.8

Per cent
19.0
17.8
30.9

Per cent
19.1
34.6
10.6

Per cent

Per cent
i.o
0.9
1. 1

II3S

1338

8l3

Mutton

Loin

Leg

Shoulder

SO. 2
67.4
67.2

16.0
19-8
19-5

33.1

13.4
13.9

0.8
1. 1
1.0

1643
86s
905

Sweetbreads

1 70.9

16.8

13. I

1.6

800

Liver

1 6S.6

30.3

3.1

3.S

1.3

539

Heart

62.6

16.0

30.4

1.0

1135

Tongue

70.8

18.9

9.3

1.0

719

Brain

80.6

8.8

9.3

1. 1

540

Ham

49.3

33.5

31.0

5.8

1366

1 Sherman's "Food Products," Macmillan, 1914.

570

PHYSIOLOGICAL CHEMISTRY

Food Water ^Sx'&) ^^* h?dra°^ Ash

Calories per
pound

i

; Per cent

r-i,;„i,»„ Broilers i 74.8
Chicken p^^i 1 63.7

Per cent Per cent
21.5 2.5
19.3 1 16.3

Per cent

Per cent
I.I
i.o

492
1016

„.. Halibut 75.4 18.6 5.2
^'^•^ Salmon 64.6 22.0 12.8

i.o

1-4

550
922

Oatmeal (boiled) 84.5 2.8 0.5

Cereals Rice (boiled) 72.5 2.8 o.i

Shredded Wheat 8.1 lo.s 1.4

II. 5
24.4
77.9'

0.7
0.2
2.1

280
498
1660

Graham s . 4

Crackers Oatmeal 6.3

Soda S-9

10. 0 9.4

II. 8 II. I

9.8 9.1

73.81
69. oi

73.1'

1-4
1.8
2. 1

1904
1920
187s

ri„-^ White 35.3
^^^^^ Graham 35. 7

9.2 1.3
8.9 1.8

53. 1'
52. i>

I.I
I.S

1182
1189

Boiled ! 75.5

T> t t„„^ Mashed 75.1
Potatoes (,j^.p3 1 22

Sweet S r . 9

2.5 i 0.1

2.6 3.0
6.8 39.8
3.0 1 2.1

20.9'
17.8
46.7
42.1

1.0
1.5
4.5
0.9

429

493

2598

903

White
Eggs (hen) g°^jj.g g^ijjig pQ^.
tion.

86.2
49.5

73.7

12.3 0.2
15.7 33.3

13.4 10.5

0.6
I.I

1.0

231
1643

672

Milk

87.0

3.3 4.0

so

0.7 314

Butter

12.7

1.3

84.0

1.92

3450

1 Peanut butter

2. 1

29-3

46. 5

17. 1

S.o

2741

Consomm6

0^ ^„ Tomato

Soups pga

j Celery (cream)

96.0
90.0
86.9
88.6

■

2.5
1.8
3.6
2.1

I.I
0.7
2.8

7.6
5.0

I.I
1.5
1 .2
1.5

S3
179
232
243

Tapioca pudding

64. 5 j 3.3

3.2

28.2

0.8

702

Doughnuts 18.3 ] 6.7

21.0

53.1^

0.9

1942

Ginger snaps 6.3 6.5

8.6 76. oi

2.6

1848

Peas (cooked)

73.8 6.7

3.4 i 14.6

I.S

525

Lettuce

94-7 ' 1.2

0.3 I 2.91

0.9

87

Apples 84.6 0.4 1 0.5 14.2"

0.3

28S

Oranges

86 . 9 0.8

0.2 II. 6

o.S

233

Bananas

75. 3 1.3

0.6 1 22.0*

0.8

447

Figs

79. 1 i.S 18.8

0.6

368

Sandwiches Chfcken

41.4 9.6 1 12.7 1 34. 5

48. 5 12.3 ' 5-4 32.1

1.8
1.7

1319
1026

Cheese (American)

30.0 28.8 j 35.9 0.3

5.08

1990

A less accurate experiment than the above but one which yields
interesting data may be carried out as follows:

Ingest a simple diet whose nitrogen content can be estimated with some
degree of accuracy (see table above). Collect the urine in two-hour periods
from 7 A. M. to ii P. M. and in an eight -hour period from ii P. M. to

^Percentage of fiber, included under carbohydrate: shredded wheat (1.7), Graham
crackers (1.5), oatmeal crackers (1.9), soda crackers (0.3), white bread (0.5), Graham
bread (i.i), boiled potatoes (0.6), doughnuts (0.7), ginger snaps (0.7), lettuce (0.7),
apples (1.2), bananas (1.0).

2 Including salt.

^ Including salt and sugar.

METABOLISM 571

7 A. M. and analyze for total nitrogen or urea. The next day ingest the same diet
plus 150-250 grams of lean meat whose nitrogen content has been determined by
analysis or estimated. Collect the urine as upon the previous day and determine
its total nitrogen or urea content. Plot curves showing the course of the nitrogen
or urea excretion on each of the days. How soon after the ingestion of the large
quantity of meat did you note an increase in the nitrogen or urea excretion?
How many hours after the meal was the maximum quantity of nitrogen or urea
excreted?

8. Influence of Purine-free and High Purine Diets. — The uric acid
of the body has a two-fold origin, i.e., it may arise from the metabolism
of the purine (nuclein) material of body tissue (glandular organs in
particular) or it may arise from the ingestion of purine (nuclein)
material. That uric acid which arises from the first source is called
endogenous while that which arises from the second source is termed
exogenous. Secretory activity may also act to increase the endogenous
uric acid output. The urine will therefore contain uric acid even though
no precursor of the acid be ingested. We may also increase the uric acid
output markedly by ingesting a high purine diet. However, no matter
how much purine material is eaten only a small part of this purine
material reappears in the urine as uric acid. In gout it is claimed
there is an accumulation of uric acid in the blood due to the fact that
the kidney has lost the ability to maintain the normal blood uric acid
level. In this disease the excretion of uric acid may be low before an
attack and increase considerably during an attack. The excretion of
exogenous uric acid in gout is also much slower than normal.

Experiment. — Ingest a purine-free diet containing about 16 grams of nitrogen
and consisting of egg, cheese, milk, starch, fruit, sugar and water for a period
of two days (for purine content of foods, see table, page 572). Determine or
estimate the nitrogen content (see table, page 569) and during the next two
days substitute sweetbreads, thymus or Uver for all the nitrogen of the diet
maintaining the calorific value of the diet the same as before. Return to the
original purine-free diet for a third interval of two days. During the final period
of two days feed a diet of sweetbreads or liver containing 50 per cent more
nitrogen than that of the first sweetbread period. Collect the urine for each
of the eight days of the experiment and determine uric acid, and total nitrogen
or urea. Note the rise in the uric acid output during the sweetbread periods.
The uric acid output on the purine-free diet is endogenous in origin. Tabulate
your results. The following data were secured by Taylor and Rose ' in a similar
but much more carefully controlled test than that just outlined.

' Taylor and Rose: Jour. Biol. C/ictn., 14, 419, 1913.

572

PHYSIOLOGICAL CHEMISTRY

INFLUENCE OF PURINE-FREE AND HIGH PURINE DIETS

(Daily Output)

Urinary constituents determined
(grams)

Purine-free
diet

Purine diet
(medium)

Purine diet
(increased)

Purine-free
diet

Uric acid

0.09

0. 14

0. 24

0.07

Total nitrogen

8.9

8.7

9.1

8.8

UreaN (+NH3)

7-3

7-1

7-1

7-oS

Creatinine

1-57

1.49

1-51

PURINE CONTENT OF FOODSi
(Percentage purine base nitrogen)

Food

Analyzed by

Food

Analyzed by

Vogel*

HalP

Bessau

and
Schmid^

Vogel* Hall'

Bessau

and
Schmid*

Beef

O.O^O O.OC2

0.037

Lettuce

0.003

Liver

0.000

0.110

0.093

Cucumbers

None.

Mutton

0.026

Rye bread

0.014 !

Trace.

Tongue

1

0-0S5

White bread....

0.008

None.

None.

Chicken

0.029

Milk

0.0002

0.C002

None.

Thymus

0.398 0.403

0.330

Eggs

None.

None.

None.

Cod fish

0.040 ' 0.023

0.038

Cheese

0.0004

None.

Potatoes

1

0 . 001 0 . 0007

0.009

Rice

0.0004

None.

None.

'Celery

1

0.005

Tapioca

None.

Peas

o.oi6 i 0.016

1

0.018

Oatmeal

None.

Spinach

0.022

0.024

Onions

None.

Hominy

0.004 1

Tomatoes

None.

None.

1 Other purine-free foods not listed here are fruits, butter, cream and starch.

^Vogel: Miinch. med. Woch., 58, 2433, 1911.

3 Hall: "The Purine Bodies," Philadelphia, 1904.

* Bessau and Schmid: Therap. Monatsch., March, 1910.

METABOLISM

573

9. A Study of Endogenous Uric Acid Output. — The uric acid in the
urine is said to have two sources, i.e., from the purine material of the
tissues and from the purine material ingested. The former is endogenous
uric acid, the latter exogenous uric acid.^ The output of uric acid
on the purine-free diet in Experiments 571 and 574 is endogenous.

30

""

20

H

10

H

^

A

^ 8 9 10 li le

2 3 4 ^ G 7 8 9

Fig. 170 — IxFLCExcE of Protein Ingestiox on Exdogenoxjs Uric Acid Output.
Gluten (130 Grams) ingested at i P.M. {Mendel 6* Stehle: Jour. Biol. Chem., 22, 215,
1915-)

Mares" claims that food-stuffs act to increase the endogenous uric
acid output by stimulating the digestive glands to actiWty. A
similar finding is reported by Mendel and Stehle.^ The food-stuff
having the most pronounced influence was protein. Pilocarpine
which stimulates the digestive glands was found to increase the endog-
enous uric acid output whereas atropine which inhibits secretory
activity was found to decrease the output of endogenous uric acid.

1 10

^ °7 8 9 lOII it 12 3 4 f 6 7 8 9 (H0UR5)

. Fig. 171 — The Endogenous Uric .Acid Output during Fasting. {Mendel is" Stehle:
Jour. Biol. Chetn., 22, 215, 1915.)

The influence of protein upon the endogenous uric acid e.xcretion is
shown by the chart in Fig. 170. The fasting output by the same
individual is shown, for comparison, in Fig. 171.

Experiment. — Ingest a purine-free diet consisting of millt, egg, fruit, cheese,
butter, sugar and bread for one day. Continue the diet for breakfast and lunch-
eon the next day but eat nothing after 12 o'clock noon, until 12 o'clock noon the

* Burian and Schur: Zeit. physiol. Client., 43, 532, 1904-5.

* Mares: Arch. f. d. ges. Physiol., 134, 59, 1910.
*Mendl andd Stehle: Jour. Biol. Chem., 22, 215, 1915.

574 PHYSIOLOGICAL CHEMISTRY

following day, i.e., the third day of the experiment. At that time ingest 125-150
grams of gluten or some other purine -free protein preparation. On the fourth
day of the experiment eat nothing imtil 9 P. M.

Collect the urine each day in hour periods from 7 A. M. to 9 P. M. and analyze
for uric acid (see methods in Chapter XXVI). Chart your data similarly to
those shown in Figs. 170 and 171, page 573, and compare them with the findings
there recorded.

10. The Rate of FHirine Excretion.— The purine material ingested
by the average normal person and which is not transformed in the body
will be eliminated in about 24 hours. In the case of persons afflicted
with gout the purine elimination is delayed. The establishment of this
delayed purine elimination is often of diagnostic assistance.

Demonstrate the rate of purine excretion as follows: Ingest a purine-free
diet consisting of egg, milk, cheese, starch, sugar, fruit and water for two days and
follow this by a day in which sweetbreads, thymus or Uver is substituted for one
of the meals of the day (see table page 572 for purine content of foods). Finish
the experiment by ingesting the original purine-free diet for two days. Collect'
each day's urine and analyze for uric acid. How soon after the sweetbread
ingestion was the original plane of endogenous uric acid elimination reestab-
lished? If one desires to locate this time more definitely the urine may be
collected in short periods (one to two hours) and the uric acid content of each
specimen determined. Particularly instructive data may be collected by per-
forming the above experiment on a gout patient and upon a normal person for
comparison. •

11. A Study of Creatinine Elimination.— It has been estabHshed
that a normal person ingesting a creatinine-free diet will excrete a uni-
form quantity of creatinine from day to day. The daily excretion of an
adult man of average weight ranges from 1-1.5 grams. For data as to
creatinine excretion of a 60 kg. man see Taylor and Rose's figures in
table on page 572. The creatinine excretion depends primarily on the
active mass of protoplasmic tissue, and therefore, it is generally true
that a fat man will show a lower creatinine output than a lean man of
like body weight. For further discussion of creatinine see Chapter XXTL

Experiment. — Ingest an ordinary mixed diet (non-meat) for a period of three
days varying the character of the diet daily. Collect the urine and analyze for
creatinine. (See Chapter XXVI for methods of analysis.)

Did the creatinine elimination change with the change in diet?

12. Influence of Water. — It has been demonstrated that increased
water ingestion influences many of the functions and activities of the
human body.^ The increase in protein catabolism which accomp-
anies high-water intake is shown in the following data collected from

^ Hawk: The relationship of water to certain life processes and more especially to nu-
trition. Read before American Philosophical Society, Philadelphia, Feb., 1914. (See
Bioch. Bull., 3, 420, 1914).

METABOLISM

:>/;>

an experiment upon a normal man.^ In this experiment the water in-
gestion at meals was increased 3 liters per day during the Water Period.

INFLUENCE OF HIGH- WATER INTAKE UPON URINE VOLUME AND
NITROGEN PARTITION

Day of
experi-
ment

Urine
volume

Nitrogen

Urea- Ammonia- Creatinine- Creatine-
nitrogen nitrogen nitrogen nitrogen

Preliminary Period

4
S
6

c.c.
830
920
S80

grams
12.987

12.084
13-183

grams
"•338
11.476
11.568

grams grams grams ;
0. 288 0.629

0.305 0.619

0. ■?6o cdiji

Water Period

7
8

9
10
II

3440
3S40
3670
3610
4020

14.161

13-491
12.981
12.976
13-138

12.596

11-583
II .212

11-455
11.879

0.486 0.610 0.063 i
0.499 0.616 0.024 1
0.553 0.589 0.102 1
0.485 0.608 0.055
0.456 0.589 0.128

The above data indicate an increased catabolism of protein material
as is shown by an increased output of total nitrogen upon the first and
second days (days 7 and 8) of the Water Period. Part of this increase
may, however, have been due to a "flushing" of the tissues rather than
to increased catabolism of protein structures.

Experiments — (a) Relation of Water Intake to Volume and Specific Gravity of
the Urine. — Ingest an ordinary mixed diet for two days. Collect the urine in 24-
hour periods. During the first day ingest very little fluid of any kind either at
meals or between meals. On the second day ingest as much water as you can
without physical inconvenience. A person of average size should have no difii-
culty in drinking 5-6 quarts per day.

Measure the volimie of each day's urine and take the specific gravity. Note
the pronounced increase in volvune and the low specific gravity of the urine
under the influence of high-water ingestion.

(b) Influence on Protein Catabohsm. That water stimulates protein catabolism
may easily be demonstrated as follows: Ingest a imiform diet imilk, crackers,
butter, peanut butter and water) for a period of four days. During the fii st two days
ingest your customary volume of water per day. During the last two days increase
the water ingestion to 5-6 liters per day. Collect urine in 24-hour periods and
analyze for total nitrogen by Kjeldahl method (see Chapter XXVI and Note on
page 589). Note the increased excretion of nitrogen under the influece of high-
water intake. If time permits other nitrogenous urinary constituents may be
determined (see table above).

1 Fowler and Hawk: Jour. Expt. Med., 12, 388, 1910.

576' PHYSIOLOGICAL CHEMISTRY

13 "Salt -free" Diet. — In order to be properly nourished we must
ingest a certain amount of inorganic matter daily. If we fail to do
this our metabolic processes become abnormal and the urine is one
index of this abnormah'ty.^

Experiment. — Ingest an ordinary mixed diet containing an ample salt content
for a period of two days. Follow this period by the ingestion of a diet which has
had its salt content reduced to a very low value.- Sugar and ohve oil or non-
salted butter may supply the bulk of the calorific part of the diet and dialyzed egg
white or casein or commercial protein preparations, e.g., plasmon, gluten or gUdine
may supply the protein. Ingest such a diet for three days. (This is an "acid-
forming" diet, see page 580.) Collect the urine and analyze for sodium chloride,
acidity, ammonia and total nitrogen. Compare the data from the normal days
with those obtained when the "salt-free" diet was ingested. Test the urine
(Chapter XXVIj and blood (Chapter XVI) for acetone. An acidosis follows
the ingestion of a salt-free diet for a sufficient length of time.

Did you feel perfectly normal during the interval you were ingesting the
"salt-free" diet?

14. Salt -rich Diet.- — On an ordinary mixed diet a normal adult
will daily excrete 10-15 grams of chloride, expressed as sodium chloride,
in the urine. On a salt-free diet this excretion decreases, whereas if
the diet contains an excessive quantity of sodium chloride this excess
will be promptly excreted in the urine. Normal feces contain very
little sodium chloride even after excessive sodium chloride ingestion
(see Experiment 33).

Experiment. — Ingest an ordinary mixed diet for two days. On each of the
following two days take a similar diet plus a weighed amoimt (e.g., 10 grams) of
sodium chloride. Collect the urine for the four days in 24-hour samples, pre-
serve and analyze for sodium chloride (for methods see Chapter XXVI). What
proportion of the added chloride was recovered?

If it is desired to make the experiment quantitative in character ingest a uni-
form diet (see Experiment, page 592) each day instead of the ordinary mixed diet,
and examine urine and feces (see Experiment 33) for chloride.

15. Acidosis. — Acidosis may be induced in a normal person by the
ingestion of a "salt-free" diet such as described in Experiment 13,
above, or by the ingestion of a carbohydrate-free diet. The acidosis
appears somewhat earlier under the latter conditions. The non-
carbohydrate diet is rather better suited for the demonstration of
acidosis because of its greater palatability. When carbohydrates are
ingested there is an oxidation of fatty acids to carbon dioxide and
water. When no carbohydrates are ingested a portion of the fatty
acids are converted into acetone bodies. These are difficult to oxidize
and are excreted as such. The ketomiria (excretion of acetone and

^ Taylor: University of California Publications, Pathology, i.

'^ It is practically impossible to secure an absolutely "salt-free" diet.

MET.\BOLISiI 577

diacetic acid) is particularly pronounced. The following table shows
the data obtained in an actual case of the withdrawal of carbohydrate
food from the diet of a normal man (von Noorden).

ACIDOSIS ACCOMPANYING CARBOHYDRATE WITHDRAWAL

Day

Diet

Excretion of acetone bodies cal-
culated as ^-hydroxj-butyric
acid (grams)

I

Protein, fat and carbohydrate.

None.

2

Protein and fat.

0.8

1

3

Protein and fat.

1. 9

4

Protein and fat.

8.7

5

Protein and fat.

20.0 I

6

Protein, fat and carbohydrate.

2.2

Experiment. — Ingest an ordinary mixed diet for one day. Follow this by a
period of two to four days in which no digestible carbohydrate is eaten. CA diet
of meat, eggs, butter, agar-agar and water has a very low digestible carbohydrate
value.) Collect the urine for each day of the experiment, examine it quaUtatively
for acetone bodies (see tests in Chapter XXlll). If present, determine the total
acetone bodies quantitatively (for methods see Chapter XXVI). The blood may
also be examined (see Chapter XVI). Did the withdrawal of carbohydrate food
cause an acidosis or ketonuria? How did it compare with the acidosis in the
above table?

i6. "Alkaline Tide." — For a time after a meal the normal acid
reaction of the urine may be changed to neutral or alkaline. This
has been explained as due to the withdrawal of hydrogen ions to manu-
facture the hydrochloric acid of the gastric juice.

Experiment. — Ingest an ordinary mixed diet. Urinate just before dinner and
note the reaction of the urine to htmus. If acid, determine the hydrogen ion
concentration by the method given in Chapter XXVI. {li alkaline, discard the
urine and make the test on another day.) After eating a heavy dinner (meats)
collect the urine at intervals of a half -hour and take the reaction to Utmus and
determine the hydrogen ion concentration as before. Did your urine change in
reaction after the meal and if so how long a period elapsed between the meal and
the occurrence of the maximimi change in reaction?

17. The "Partition" of Urinary Nitrogen and Sulphur as Influenced

by Diet. — It was first shown by Folin^ that the percentage of the total

nitrogen and total sulphur of the urine which appeared in the form of

any particular nitrogenous constituent or in any particular form of

' Folin: Amer. Jour. Physiol., 13, 118, 1905.

37

578

PHYSIOLOGICAL CHEMISTRY

sulphur was regulated directly by the extent of the total nitrogen and
sulphur elimination. This point is well illustrated in the following
table which contains data regarding the so-called "partition" or
"distribution" of the urinary nitrogen and sulphur.

THE NITROGEN AND SULPHUR " PARTITIONS" AS INFLUENCED BY DIET^

Constituent of the urine

Normal protein diet

Starct

i-cream

diet

Weight, grams

Nitrogen,
grams

Per cent of
total N or S

Weight, grams

Nitrogen,
grams

CO

M

«-. °

S3 *^
61.7

Urea

31.6

14-7 87.5

4.72

2. 2

1
Ammonia

0.6

0.49: 3.0

1

1 0.51

1

0.42

II-3

Creatinine

1-55

0.58 3.6

1. 61

0.60

17.2

Uric acid

0.54

0. 18 I.I

0.27

0.09

2.5

Undetermined

0.8s 4.9

0.27

7-5 '

Total N

16.8

100. 0

3.6

100. 0

Inorganic SO3

3 27

90.0

0.46

60.5

Ethereal'sOa

0.19

5-2

4-8

0. ID

13-2

1

Neutral SO3

0.18

0. 20

26.3

1

Total SO3

3-^4

100. 0

0. 76

100. 0 •

It will be observed from an examination of this table that a normal
protein diet which gave 16.8 grams of urinary nitrogen yielded 87.5
per cent of this nitrogen as urea, 3 per cent as ammonia, 3.6 per cent as
creatinine and i.i per cent as uric acid; whereas a "non-protein diet"
(starch and cream containing about i gram of nitrogen) which gave
only 3.6 grams of urinary nitrogen yielded only 61.7 per cent of this
nitrogen as urea but gave a greatly increased percentage output in the
case of each of the other nitrogenous constituents mentioned, e.g., 11. 3
per cent as ammonia, 17.2 per cent as creatinine and 2.5 per cent as
uric acid. The percentage output of neutral sulphur was also greatly
increased.

It will furthermore be observed that the actual daily output of
' Folin: Am. Journ. Physiol., 13, 118, 1905.

METABOLISM 579

certain of the constituents is uninfluenced by the amount of protein
ingested. Among these are creatinine and neutral sulphur. On the
other hand the output of inorganic sulphur and urea is more or less
directly proportional to the protein ingestion. The observation
of such facts as these led Folin to formulate his theory of protein
metabolism.^

Experiment. — During a period of two or three days ingest an ordinary mixed
diet containing 100-125 grams of protein (16-20 grams of nitrogen) per day.
Collect the urine accurately in 24-hour periods (page 565) preserve it and analyze
the xirine of the second and third days for total nitrogen, urea, creatinine, total
sulphur, inorganic sulphates, ethereal sulphates and neutral sulphur (by differ-
ence). For methods of analysis see Chapter XXVI. Follow this period by
one of three days in which a diet of starch and cream having a similar calorific
value is ingested. Analyze the urine for the second and third days as indicated
above. Calculate your results and tabulate as shown in the table on page 578.
How did the change in the diet alter the metabolism of nitrogen and sulphur?

In calculating the calorific value of a diet make use of the following values :

I gram protein 4.1 large calories

I gram fat 9.3 large calories

I gram carbohydrate 4.1 large calories.

18. Protein-Sparing Action of Carbohydrate and Fat. — The non-nitrogenous
nutrients, carbohydrate and fat, have the power to diminish the extent of the catabo-
lism of protein in the normal human body. In other words they are said to ' ' spare
protein. This point is illustrated in data reported by von Noorden and Dieters,
which are tabulated below.

PROTEIN-SPARING ACTION OF CARBOHYDRATE AND FAT

Nitrogen ingested

Nitrogen in urine

12.6 grams.

10.4 grams.

12.6 grams +200 grams sucrose.

9.0 grams. 13 per cent reduction in protein
catabolism.

It will be observed that the addition of 200 grams of sucrose to the diet was
accompanied by a decrease of 13 per cent in the amount of protein catabolized.
It has been established that carbohydrates are more efficient "protein sparers"
than are the fats. For example Voit found carbohydrate to produce a 9 per cent
decrease in protein catabolism whereas fats produced only a 7 per cent decrease.

Experiment. — Ingest a uniform diet of known or estimated nitrogen content
for a period of four days. Collect and preserve the urine accurately (see page 565)
in 24-hour samples and analyze the excretion of the third and fourth days for total
nitrogen. On the fifth day add 200 grams of sucrose to the diet. Analyze this urine

^The author's article on "General Considerations of Metabolism" in "Modern Medi-
cine" (Osier and McCrae) 2nd Edition, 1914, p. 594. See also Folin: American Journal
Physiol., 13, 118, 1905.

58o

PHYSIOLOGICAL CHEMISTRY

also for total nitrogen. Calculate your results and tabulate the data as shown in
table on page 579.

Did the sucrose influence the catabolism of protein in your body?

19. Hydrogen Ion Concentration of the Urine as Influenced by
the Ingestion of Acid-Forming and Base-Forming Foods. — It has been
demonstrated by Sherman and Gettler^ that vegetables and fruits,
on burning, leave an ash in which the basic elements (sodium, potassium,
calcium and magnesium) predominate, whereas cereals, meats and fish
foods leave an ash in which the acid-forming elements (chlorine, sulphur
and phosphorus) predominate. A list of acid-forming and base-
forming foods is given in the following table.

EXCESS OF ACID-FORMING OR BASE-FORMING ELEMENTS IN FOODS

(Sherman and Gettler)

Article of Food

Excess acid or base in terms of
normal solutions. Per 100 grams

Acid (c.c.)

Base (c.c.)

Apples

Asparagus

Bananas

Beans (dried)

Beans (lima, dried)

Beets

Cabbage

Cantaloup

Carrots.

Cauliflower

Celery

Crackers

Eggs

Egg-white

Egg-yolk

Fish (haddock).
Lemons

Lettuce

Meat (lean beef) .
Milk (cow's) ....

Oatmeal

Oranges

Potatoes

Prunes

Raisins

Rice

Wheat (entire).

7.81

II. ID

S-24
26.69
16.07

13-91

12.93

8.10
9.66

3-76

0.81

5-56

23.87

41.65

10.86

4.34

7-47
10.82

5-33

7.78

5-45
7 37

2-37

S-6i

7.19

24-40*

23.68

1 Sherman and Gettler: Jour. Biol. Cliem., 11, 323, 191 2.

" Prunes, plums and cranberries yield an alkaline ash but serve to htcrease the hydrogen
ion concentration of the urine because of their benzoic acid content, this acid being syn-
thesized with glycocoU in the kidney and elsewhere to form hippuric acid.

METABOLISM 58 1

The above data indicate that potatoes, oranges, raisins, apples,
bananas and cantaloups are important base-forming foods. Among
the most important acid-forming foods are found rice, whole wheat
bread, oatmeal, meats and eggs. Certain fruits, e.g., cranberries,^ prunes
and plums yield a basic ash but are acid-forming foods.

This is due to the fact that they contain benzoic acid which is
synthesized with glycocoll in the body to produce hippuric acid (see
page 585). It is worthy of note that some plant foods are base-formers
and others are acid-formers. It is also an important fact that acid
fruits yield a basic ash (see page 580) .

The normal diet should contain sufhcient base-forming elements to
neutralize the acids formed. If these acids are not neutralized by
the basic elements in the diet they will be neutralized by the fixed
bases of the tissues of the body and a seriously deranged metabolism
may result. (See experiment on "salt-free diet," page 576.) Organic
salts of the alkalis (c.^., sodium bicarbonate or sodium acetate) are often
given therapeutically. They reduce the H ion concentration of the
urine: the same result so far as urine reaction is concerned may be
secured by feeding properly selected base-forming foods. The ingestion
of sodium dihydrogen phosphate (NaH2P04) will increase the acidity
of the urine: a like result may be produced by feeding properly selected
acid-forming foods. Anything which produces an increase in the H ion
concentration of the urine will produce an increase in the ammonia
output.

On a mixed diet the H ion concentration of the urine- has been
found to be 6 ± 0.1. ^ In nephritis the H ion concentration of the
urine may be increased to 5.33 or higher. Alkalis have been used with
apparent success in the treatment of nephritis.^ It is evident that base-
forming foods properly selected should be suitable dietary articles for
nephritics.^ For a detailed discussion of acid-forming and base-forming
foods see article by Blatherwick.^

Experiment, — Ingest a uniform diet consisting of milk, crackers, butter, pea-
nut butter, and water in desired quantities for a period of three days. Follow this
by a period of six days during the first three of which considerable quantities of
acid-forming foods (see table page 580) are added to the diet. During the second

^ Radin reports this berry to contain 0.06 per cent benzoic acid (Blatherwick: Arch.
Int. Med., 14, 409, 1914).

^Henderson and Palmer: Jour. Biol. Clicm., 14, 81, 1913.

' H ion concentration may be expressed as gram of ionized H per liter of water. A neu-
tral solution has a H ion concentration of iXio"', or 0.000,000,1 gram per liter. It is
often customary to express the H ion concentration according to Sorensen's logarithmic
notation. For example instead of expressing the H ion concentration of a neutral solution
as I X io~^ he expresses it as 7.00. An increasing H ion concentration decreases this value
and an increasing OH ion concentration increases the value.

■• Fisher: Nephritis, New York, 191 2.

* Blatherwick: Arch. Inl. Med., 14, 409, 1914.

582

PHYSIOLOGICAL CHEMISTRY

half of the period (days four to six) add an abundance of base -forming foods to the
diet. Distilled water should be used for drinking purposes and a uniform volimie
should be ingested daily. Collect the urine in 24-hour periods, preserve and
analyze for H ion concentration, titratable acidity and ammonia (for methods
see Chapter XXVI). Compare your results with those tabulated in the table
below.

REACTION OF URINE AS INFLUENCED BY DIET^

Basal
diets-

4

Determi-
nation.

Baked pota-

No. I No. 2 i,°^il?f>.
grams per

day)+basal

I diet No. I

, S S (6 days)

days ! days

Rice (210 Cranberry | Bread'
grams per sauce (300- (whole
day) +basal 600 grams wheat) 450
diet No. I per day) + grams for i
(4 days) basal diet, day + basal
No. I diet. No. i
; (6 days) |

Prunes Cantaloup*
(330-550 (260 grams
grams per per day) +
day) +basal basal diet,
diet. No. 2 No. 2

(3 days) (5 days)

H ion con- 7 19
centration.

5.57

7.74

7. 4^-6. 90

7.14

' 6.30-5.70
6.19

! 1 i

6.80 1 s. 30-4. 80 ' 5.30-7.38

(Previous ■ ■ ■ '

day 6.90) 5.07 6.70

Titratable

aciditv 275
(c.c. N/io

474

196-216
203

166-297
233

391-488
407

350 570-540-578 466-250

(Previous ■ ■ ■ •

day 297) 563 328

Ammonia 0
N (grams) 0.310 0.464 —

221-0. 248
. . -
0.238

0.166-0. 251
0.198

0.219-0. 391
0.30s

0.280 0.602-0.729 o.s 13-0. 220

;day 0.251) 0.654 0.310

20. Hydrogen Ion Concentration of the Urine as Influenced by
Alkali and Acid Ingestion. — The ingestion of certain organic salts of the
alkaHs, e.g., sodium citrate and sodium bicarbonate will cause a decrease
in the hydrogen ion concentration of the urine. The ingestion of acids

INFLUENXE OF INGESTED SODIUM BICARBONATE ON H ION
CONCENTRATION OF URINE

Experiment
Number

Sodium
Bicarbonate,

Hydrogen Ion Concen-
tration before Bicarbon-

Time of Collection of Specimen,
of Urine and H Ion Concen-
tration

Grams ate Ingestion

11.00
A.M.

12.00
noon

1. 00
P.M.

2 . 00 3 . 00
P. M.P. M.

1

I
2
3
4
S
6

4
8
12
8
8

7.40

5 -40

5-30
7.40

5-85
6.70

8.30

8.50
8.70
8.50

7.48
8.30
8.70
8.70

7.48
6.50
8.70
8.50
8.70
8.50

7.40
6.50
8.70
8.50
8.70
8.70

5.85

7-40

8.70 '

8.50

8.30

8.50

8

7.48

8.70

1 Tabulated from data reported by Blatherwick (Arch. Int. Med., 14, 409, i9i4)'
Experiments all made on the same subject (B).

^ Basal diet No. i contained 100 grams Graham crackers, 25 grams butter, 400 c.c. whole
milk ingested at each of the three dailj- meals. One apple and one soft boiled egg added at
supper. In diet No. 2 whole wheat crackers were substituted for the Graham crackers.

* This day was preceded by NaHCOa ingestion for three days and by rice ingestion for
four days.

* This diet followed immediately after the diet of prunes (see 5).

MET.ABOLISM

583

(either organic or inorganic) or acid salts, e.g., sodium dihydrogen phos-
phate will increase the hydrogen ion concentration of the urine. The
alkahs are much more effective in producing changes in reaction than
are the acids. The influence of ingested alkali (sodium bicarbonate) is
shown in the foregoing table containing data submitted by Henderson
and Palmer.^

Blatherwick- reports a decrease in ammonia nitrogen output from
0.256 gram to 0.072 gram, and an accompanying decreased acidity
under the influence of bicarbonate ingestion (25 grams in two days).

The influence of ingested acid (benzoic) is shown in the following
data reported by Blatherwick.-

INFLUENCE OF BENZOIC ACID INGESTION"

Day

Titratable acidity
(c.c. N/io)

H ion concentration

Ammonia N (grams)

1 1
I 392 6.15

0.292 !

2 410

6.15

0.374

3 443

6.00

0.422 '

4 J 434 6.00

0.408

5 468 5.70

0.418

(For further discussion of dietary alterations of urine reaction see
preceding experiment.)

Experiments. — (a) Influence of Alkali. — Ingest a uniform diet consisting of
milk, crackers, butter, peanut butter and distilled water for a period of two
days. During the next two days take the same diet and ingest 24 grams of
sodiimi bicarbonate between meals (12 in A. M. and 12 in P. M.). Collect the
urine in 24-hour periods and analyze it for titratable acidity, H ion concentra-
tion and ammonia. Compare yovu: results with those shown in table on
page 582.

If desired the bicarbonate may be given in one dose of 8-12 grams and the
urine collected in hourly specimens for the next five hours and each specimen
analyzed. Data from such experiments are shown in table on page 582 .

(b) Influence of Acid. — Proceed as above except that i gram of benzoic acid
(in capsule) is ingested before each meal of the experimental period.

The experiment may also be varied by ingesting 10 grams of sodium dihydro-
gen phosphate early in the day and collecting the urine in hoiurly fractions or in
one 24-hour sample.

^ Henderson and Palmer: Jour. Biol. Cliem., 14, 81, 1913.
^See p. 581.

" One gram of benzoic acid in a capsule before each meal. Basal diet Xo. i described on
page 582 was used.

584 PHYSIOLOGICAL CHEMISTRY

From yotir experiments what do you conclude as to the relative eflBciency of
acid and alkali in altering the reaction of the urine?

21. Influence of a High Calorie Non -Nitrogenous Diet. — If an

individual fasts there is a combustion of a certain amount of protein
tissue each day of the fast. The destruction of such tissue is rather
low on the first day due to the fact that the glycogen stores of the body
are being utilized to furnish the necessary energy. If an individual
instead of fasting, ingests a diet of high calorific value and very low in
nitrogen the output of nitrogen in the urine of the third or fourth day
will be less than on the third or fourth day in fasting. This is due to
the fact that the body derives sufficient energy from the high calorie
diet and there is less destruction of protein body tissues than occurs in
fasting. For a discussion of energy value of foods see "Determination
of Fuel Value of Foods," below, and the table on page 569.

Experiment. — ^Ingest a high calorie diet which is very low in nitrogen or
actually non-nitrogenous. A satisfactory diet may include sugar, butter, starch,
cream, agar-agar and water. (For energy values see below and table, page
568.) Ingest such a diet for three days. Collect the urine in 24-hour periods,
preserve and analyze it for total nitrogen, acidity and ammonia. Note the low
nitrogen excretion on the third day as compared with the nitrogen output of the
third day of fasting. If so desired, you may (at some later date) fast for three
days and repeat the above analyses for comparison.

Determination of Fuel Value of Food. — When organic substances are oxidized
or burned in the human body they liberate a certain amount of heat. This calorific
energy or heat value varies according to the type of organic matter undergoing
oxidation. Thus the proteins, fats and carbohydrates of the diet when they are
burned in the body yield different quantities of heat per unit of substance than do
organic acids, alcohol, etc. The energy values of pure protein fat and carbohydrate
are the following:

Protein =41 large calories per gram.

Fat =9-3 large calories per gram.

Carbohydrate = 4.1 large calories per gram.

In arriving at the energy value of any given diet it is customary to burn weighed
samples of the various foods in an oxygen atmosphere in an apparatus called a
bomb calorimeter (see Fig. 172, page 586). By this means we may determine how
much heat is liberated when the ingested food is oxidized in the body. A correction
must be made for the incompletely oxidized substances of the urine and feces. A
large mass of data concerning the heat value of foods has been collected and tabu-
lated, and it is therefore possible to arrive at an approximate idea of the energy
value of a diet by calculation (see table, page 569). The bomb colorimeter shown
in Fig. 172, page 586, is one of the most satisfactory for actual determination of the
heat of combustion of organic substances.

22. Metabolism in Fasting.— The metabolism of a fasting man is
entirely different from the metabolism of a well-nourished person.

METABOLISM

O^O

The collection and analysis of the urine during a short fast (three
to seven days) will demonstrate many important facts. The following
table, which contains data from fasting tests made in the author's
laboratory/ illustrates some of the points in which fasting metabolism
differs from normal metabolism:

METABOLISM IN FASTING

Day

Body

Total

Ammonia

Creatine

Acidity.

P2O6

Chloride

of

weight,

X

N

X

c.c. N/io

grams,

period

H.

grams

grams

grams

XaOH

XaCl

Preliminary Feeding Period

1-4

Av. 74.16

10.430

0.112

None

238.6

2.768

9.007

Fasting Period

I

73-32

10.072

0.288

0.269

328.9

2.616

5-035

2

71.98

15-072

0.642

0.073

677.1

2.509

3-231

3

70.92

14-463

0.862

0.089

770.4

2.851

2-539

4

70.24

13.080

1. 201

0.068

664.2

2.490

I -253

5

69.61

I I. 801

1.266

0.033

5250

2.376

1-474

6

69.12

II. 214

1-373

0.022

462 . 4

1. 186

1-132

7

68.70

10-734

1-371

0.003

438.9

0955

I-I37

Abstinence from food for a few days can in no way operate to the
disadvantage of a normal person. In fact indi\dduals affected with
certain types of gastro-intestinal disorders are benefited by fasting.
The fasting treatment^ is also being used with success in cases of diabetes
mellitus.

In order to determine experimentally how the fasting metabolism differs from
normal metaboUsm proceeds as follows : Ingest an ordinary mixed diet and col-
lect your urine (see page 565) for a day. Measure the volimie and analyze the
sample for total nitrogen, ammonia, creatine, sodium chloride, total phosphates
and acidity' (for methods see Chapter XXVI). For the next few days (three to
seven as desired) ingest nothing but water and collect the urine accurately and
analyze for the constituents enumerated above. Tabulate your results and
compare them with those given in the table above.

23. Synthesis of Hippuric Acid in Human Body. — Hippuric Acid is
present in human urine in small amount, about 0.7 gram being excreted

' The chloride, phosphate and acidity determinations were collected during one seven-
day fast and the other data collected during a different fast on the same man. (See
Howe, Mattill and Hawk: Jour. Amer. Chem. Soc, 3$, 568, 191 1; and Wilson and Hawk:
Jour. Amcr. Chem. Soc, 36, 137, 1914.)

-Allen: Amer. Jour. Med. Set., 150, 480, 1915.

' A more accurate e.\periment may be carried out by ingesting a uniform diet of known
composition (see page 569) for a few days before the fast.

586

PHYSIOLOGICAL CHEMISTRY

per day. The urine of herbivorous animals contains much larger quan-
tities. This acid is formed in the animal body, by synthesis from ben-
zoic acid and glycocoll which takes place in the kidneys and elsewhere.^

Experiment. — Ingest 2 grams of sodium benzoate or ammoniimi benzoate
before retiring at night. Collect the first fraction of urine voided the next morn-
ing. The benzoate has been synthesized with glycocoU to form hippuric acid.

Fig. 172. — -BERTHELOT-AxWATKli BoMB CALORIMETER.

The urine will therefore be found to contain much more of this acid than is nor-
mally present. Isolate the hippuric acid by one of the following methods :

(a) First Method. — Render the urine alkaline with milk of lime, boil for a few
moments and filter while hot. Concentrate the filtrate, over a burner, to a small
volume. Cool the solution, acidify it strongly with concentrated hydrochloric acid
and stand it in a cool place for 24 hours. Filter off the crystals of hippuric acid
which have formed and wash them with a little cold water. Remove the crystals
^Kingsbury and Bell: Jour. Biol. Chem., 21, 297, 1915.

METABOLISM 587

from the paper, dissolve them in a very small amount of hot water and percolate
the hot solution through thoroughly washed animal charcoal, being careful to wash
out the last portion of the hippuric acid solution with hot water. Filter, concen-
trate the filtrate to a small volume and stand it aside for crystallization. Examine
the crystals under the microscope and compare them with those in Fig. 125, page 389.
This method is not as satisfactory as Roaf's method (see below).

{b) Roaf's Method. — Place the urine in a casserole or precipitating jar and add
an equal volume of a saturated solution of ammonium sulphate and 1.5 c.c. of
concentrated sulphuric acid per 100 c.c. of urine. Permit the mixture to stand for
twenty-four hours and remove the crystals of hippuric acid by filtration. Purify
the crystals by recrystallization according to the directions given above under First
Method. Examine the crystals under the microscope and compare them with those
given in Fig. 125, page 389.

It is possible, by the above technic, to isolate hippuric acid in crystalline form
from as small a volume as 25-50 c.c. of herbivorous urine. The greater the amount
of ammonium sulphate added the more rapid the crystallization until at the satura-
tion point the crystals of hippuric acid sometimes form in about ten minutes.

n. METABOLISM PROCEDURES INVOLVING THE
MANIPULATION OF THE FECES^

24. "Separation" of Feces. — In order to differentiate the feces
which correspond to the food ingested during any given interval it is
customary to cause the person under observation to ingest some sub-
stance, at the beginning and end of the period in question, which shall
sufficiently differ in color and consistency from the surrounding feces as
to render such differentiation comparatively easy. Two "markers"
very widely used in such tests are wood charcoal and carmine. In
making an actual separation of feces in a metabolism experiment
proceed as follows: Just preceding or in the early part of the first meal
(usually breakfast) of the metabolism test, ingest a gelatine capsule
(No. 00) containing 0.2-0.3 gram of carmine or charcoal. From this
time collect all stools in flat-bottom porcelain dishes and examine for the
presence of the "marker." All fecal matter containing portions of the
marker may be considered as representing the diet in question. This
fecal matter should be retained and preserved (see page 588). Just
before or in the early part of the first meal (usually breakfast) following
the end of the metabolism test a second "marker" in a gelatine capsule
should be ingested. The feces should be carefully inspected until the
marker makes its appearance. Retain all fecal matter uncolored by
the marker, reject the remainder. Frequent difficulties are encountered
in the practical separation of feces, but the character of such difficulties
will be most satisfactorily impressed by the performance of actual
separations.

' For other practical work on feces see Chapter XIV.

588 PHYSIOLOGICAL CHEMISTRY

25. Collection and Preservation of Feces and the Mixing and
"Weighing for Analysis. — The older methods in vogue in metabolism
work embraced the analysis of dried feces. Various investigators later
demonstrated that the drying of feces was accompanied by losses and
changes of some of the organic constituents' of the feces. ^ Therefore
the chemical examination of all stools wherever possible should be
made on the fresh feces. If a study is being made which extends over
several days and it is desired to economize time and effort in the
chemical examination the daily fecal output or an aliquot portion of each
stool may be collected in a friction-top can or pail of suitable size and
preserved by thymol and refrigeration.^ This method has been found
satisfactory when the feces are to be examined for inorganic constituents
or total nitrogen. For the determination of fat, carbohydrate, etc.,
the fresh stool should be employed.

In the preservation of feces for the determination of total nitrogen
the following simple procedure may be used: Introduce each stool into
a weighed friction-top can or pail and place the vessel in a cold room or
refrigerator.^ At the end of the period mix the feces thoroughly and
analyze weighed portions. In case individual stools are analyzed, the
stool should be collected in a weighed flat-bottom porcelain dish."* After
mixing the feces very thoroughly the weight of dish, spatula and feces is
determined and the weight of the feces secured by difference.^ A por-
tion of the well-mixed feces is then introduced into a large weighing
bottle containing a glass hoe. Desired amounts of feces are then
removed for analysis and the exact weight of such amounts obtained by
difference.

26. Bacterial Nitrogen in Feces.^ — About 50 per cent, of the total nitrogen of
the feces is made up of bacterial cells (see Chapter XIV on Feces). To demon-
strate this point proceed as follows:

(a) Ingest an ordinary mixed diet. Collect a representative stool from this
diet and after mixing it thoroughly separate the bacterial cells from a weighed por-
tion as described in Chapter XIV. After examining some of the suspension under
the microscope and noting the bacterial cells determine the bacterial nitrogen in

^ Zaitschek: Pflugers Arch., 98, 595, 1903.
Schimidzu: Bioch. ZeiL, 28, 237, 1911.
Konig: Landw. Vers. Slat., 38, 230.

Frear and Holter: Report, Penn. Stale College, p. 123, 1891.
Emmett and Grindley: Jour. Am. Cheni. Soc, 31, 570, 1909.
- Howe, Rutherford and Hawk: Jour. Amer. Chem. Soc, 32, 1683, 1910. This proce-
dure is not satisfactory if fat is to be determined (Smith, Miller and Hawk: Jour. Biol.
Chem., 21, 395, 1915). Such feces shows an hydrolysis of fat to fatty acid and a decrease
in total fat.

'; The author uses a brine tank at — i2°C. in which the feces are quickly frozen.
* The spatula for mixing the feces should be weighed with the dish.
^In case it is desired an aliquot part of each stool may be placed in a friction-top can
or pail and preserved as a "composite sample" for the period.

METABOLISM 589

the entire volume of suspension by the Kjeldahl method^ (see Chapter XXV'I).
Also determine the total nitrogen in weighed portions of the original feces by the
Kjeldahl method. What percentage of the total nitrogen of the feces is bacterial
nitrogen?

(b) If it is desired to determine the actual amount of nitrogen which is excreted
daily in the feces in the form of bacterial cells, proceed as follows: Ingest an ordi-
nary mixed diet for a period of three days. Separate the feces for this period accord-
ing to directions given on page 587, using charcoal for the first separation and
carmine for the second or vice versa. Preserve the feces for the period according
to directions given on page 588. Mix the weighed feces thoroughly and analyze
for bacterial nitrogen and total nitrogen according to directions given elsewhere-
(see Chapters XIV and XXVI). Calculate the actual output of bacterial nitrogen
per day and the percentage of the total nitrogen of the feces which was excreted
per day in the form of bacterial nitrogen.

27. "Metabolic Product" Nitrogen in Feces. — A certain quota of the fecal
nitrogen is due to the presence of residues of digestive secretions, epithelial cells,
bacteria, etc. The nitrogen in these forms has been called "metabolic nitrogen."
To determine this form of nitrogen proceed as foUows: Ingest a non- nitrogenous
diet for a period of two days. The diet may include desired quantities of starch,
cream, sugar, butter, water and sodium chloride. About 15 grams of agar-agar
should be added to the diet to prevent constipation and to insure the evacuation
of approximately the normal quantity of feces. (For inJfluence of agar-agar see
Experiment 28.) To separate the feces properly ingest a capsule of carmine at
the beginning of the test and one of charcoal at the end (see page 587). Preserve
the feces as described on page 588. After mixing the feces thoroughly determine
the nitrogen in weighed quantities by the Kjeldahl method^ according to direc-
tions given in Chapter XXVI. Calculate the quantity of nitrogen eliminated per
day. Inasmuch as no nitrogen was ingested the nitrogen present in the feces is
of metabolic origin, i.e., it is made up principally of nitrogen in the form of cells,
digestive secretions and bacteria.

28. Influence of Indigestible Non-Nitrogenous Material upon
Fecal Output. — This may be demonstrated by agar-agar ingestion.
This indigestible hemicellulose has the property of absorbing water
readily and therefore when ingested it increases the bulk of the feces
considerably. This fact is made use of in some forms of constipation
and in the determination of metabolic product nitrogen (see Experi-
ment 27).

Experiment. — Ingest a uniform diet for four days. Divide the interval into
periods of two days each,^ and "separate" the feces by charcoal or carmine (see
Experiment 24). On the third and fourth days ingest 10 g^ams of agar-agar at
each meal. Collect the feces for each two-day period (see Experiment 24,
page 587), and note the increase in the daily excretion under the influence of
the agar ingestion. What was the increase per gram of agar?

' In the oxidation process use 10 grams of potassium sulphate instead of the copper
sulphate. The remainder of the procedure is the same as for urine.

* More accurate results will be secured if the bacterial nitrogen is determined on each
individual stool in the fresh condition.

'Longer periods are desirable where great accuracy is desired.

59° PHYSIOLOGICAL CHEMISTRY

29. Protein Utilization. — By "protein utilization" is meant the
percentage of the ingested protein which is actually absorbed and
assimilated.

This may be determined by the following procedure : Ingest any diet of
known nitrogen content for a period of three days^ (see table, page 569). Collect
all feces from the diet making the "separations" as directed on page 587, using
carmine as the initial "marker" and charcoal as the final "marker" or vice
versa. Preserve the feces as directed on page 588. Mix the total feces thor-
oughly and determine the nitrogen by the Kjeldahl method (see Chapter XXVI and
note on page 589). The approximate nitrogen utihzation may be calculated as
follows :

(Food nitrogen — Feces nitrogen) X 100

Food^^trogen = Approximate percentage nitrogen util-
ization. If it is desired to ascertain the actual percentage of the ingested ni-
trogen which has been utilized by the body we must make a correction for meta-
boUc nitrogen. In doing this proceed as follows : Ingest a non-nitrogenous diet
as described on page 589 for a period of two days, using sufficient agar-agar to
insure a daily fecal output which shall approximate in weight that obtained when
the regular protein diet was ingested.^ Separate and preserve the feces as
directed on page 588. Mix thoroughly and analyze for nitrogen according to
the Kjeldahl method (see Chapter XXVI and note on page 589). Calculate the
actual percentage utihzation of the diet as follows :
[Food Nitrogen — (Fecal nitrogen— metabolic nitrogen)] X 100

^ Food~niSoi^n =^^^^^ P^'^^^*"

age nitrogen utihzation. If urinary nitrogen is determined the above data
enable us to prepare a nitrogen balance (see Experiment 34, page 592).

30. Influence of Defective Mastication on Food Residues in Feces. — Rapid
eating accompanied by defective mastication leads to the appearance of relatively
large macroscopic food residues in the feces. Under some conditions, however, pro-
tein utilization (see above) may be as satisfactory during food "bolting" as when
the food is very thoroughly masticated.^ This problem may be studied by the
following method:

(o) Ingest a diet containing meat and be certain to masticate the diet very
thoroughly. Collect a stool, examine macroscopically; mix carefully and examine
microscopically (see page 229).

{h) Ingest a diet similar to that employed in above experiment (a). "Bolt"
the food, i.e., ingest it practically without mastication. Examine the feces as
above. Note the difference in the macroscopical and microscopical findings under
(a) and {b).

If the nitrogen of food and feces is determined we may calculate the protein
utilization (see Experiment 29). By the additional determination of urinary
nitrogen, we may prepare a nitrogen balance (see Experiment 34, page 592).

1 See note 3, p. 589.

* It is frequently difficult to so regulate the agar-agar intake as to secure the proper fecal
output. In such an event the proper value for metabolic nitrogen must be obtained by cal-
culation. For example if 89.1 grams of feces were excreted per day on the protein diet, and
166.5 grams per day (with a nitrogen value of 0.5 gram) when agar was employed, the
actual value for metabolic product nitrogen may be obtained by the following proportion,
assuming that the content of metabolic nitrogen is proportional to the weight of feces ex-
creted: 89.1 : 166.5 : -.x :o.5. x = 0.268 gram metabolic nitrogen per day.

^Foster and Hawk: Jour. Amer. Chetn. Soc, 37, 1347, 1915.

METABOLISM 591

31. Fat in Feces. — A normal adult will digest and absorb at least
90 per cent of the fat in the diet when the amount ingested does not
exceed ibo grams. If the diet contains an excessive amount of fat,
e.g.i 300 grams per day, considerable appears in the feces. In pancreatic
diseases and such conditions as are accompanied by a decrease in bile
flow the digestion and assimilation of fat is lessened.

Experiments. — (a) Ingest an ordinary mixed diet containing an average amount
of fat per day, e.g., 75-100 grams. Collect a stool and examine it microscopically as
directed in Chapter XTV. (b) Now ingest a diet containing an excessive quantity
of fat, e.g., 300 grams per day. Separate the feces and subject a representative
sample of the feces from the high fat diet to microscopical examination, (c)
If it is desired the fat may be extracted from some of the stool by applying the
principle involved in the quantitative determination of fat in the Saxon method
(see Chapter XTV) . Evaporate the ether extract and identify the fat in the residue
by tests given in Chapter IX.

32. Carbohydrate in Feces. — Under normal conditions the great
bulk of the soluble carbohydrate in the food is absorbed from the intes-
tine even when the ingestion is high. Hence the content of soluble
carbohydrate in feces is low. To demonstrate this proceed as follows:

(a) Ingest for three days an ordinary mixed diet to which 100 grams of glucose
or sucrose is daily added. Separate and preserve the feces (see page 588) and
when the final "marker" appears extract an aUquot portion of the total mixed feces^
with water, decolorize with boneblack, filter, and after making the filtrate up to
a known volimie determine the sugar by Benedict's method (see page 522).
Calculate the soluble carbohydrate content of the feces for the three-day interval.
(b) Proceed as above with the exception that at least 250 grams of sugar should
be added to the' diet instead of 100 as in (a).

How did the daily excretion of soluble carbohydrate in (a) compare with that
in (b)? Why is this so? If a diet of known carbohydrate content is fed this
experiment will give us accurate data as to soluble carbohydrate utiUzation (see
Protein Utilization, page 590). If it is desired this experiment may be combined
with the hyperglycemia and glycosuria experiments on pages 566 and 568. See
also Experiment 36, page 593.

33. Inorganic Elements in the Feces. — The salts of sodium and
potassium being very soluble are almost completely absorbed, from the
intestine. The same is true of the chlorides including that of sodium
which is of greatest importance. Hence the alkali metals and chlorides
are excreted mainly in the urine and are found only in very small
amounts in the feces even when large amounts are ingested. With
calcium, magnesium, iron and phosphate conditions are different. Not
only are salts of calcium, magnesium and iron less readily absorbed but
they are excreted to a large extent by way of the intestinal mucosa rather
than by the kidneys. Ordinarily about 90 per cent of ingested calcium is

^ If time permits it is more satisfactory to analyze each individual stoolin /r«/i condition.

592

PHYSIOLOGICAL CHEMISTRY

eliminated by way of the feces and a little less than half of the magnes-
ium. From 20-30 per cent of the phosphorus ingested is usually found
in the feces.

Experiments. — (a) Ingest for a period of three days an ordinary mixed diet
without added salt and containing no milk. Separate the feces for the period (see
page 587) and retain a portion of the well -mixed feces for analysis.

(b) Proceed as above with the exception that there is added to the mixed diet
10 grams of conmion salt and a quart of milk (containing about 1.6 grams of CaO,
0.2 gram MgO, 1.4 grams of chloride expressed as sodiimi chloride, and 2.2
grams P2O6). Mix feces well and reserve part for analysis.

Ash 10 gram samples of the feces from the above diets. Dissolve with the aid
of a Uttle dilute nitric acid, filter and make up to 100 c.c. Determine in aliquot
portions of this solution: (i) Chlorides by Volhard method. (2) Calciimi and
magnesivun by McCrudden's method. (3) Phosphorus by uranixmi titration.
(For details of analytical methods see Chapter XXVI.) Calculate the percentages
of the added Ca, Mg, P, and CI which are recovered from the feces.

For a more detailed study of chloride excretion combine this experiment and
Experiment 14 (see Experiment 13).

m. METABOLISM PROCEDURES INVOLVING THE
MANIPULATION OF BOTH URINE AND FECES

34 Preparation of a Metabolic Balance. — This test entails the
analysis of the food ingested and of the urine and feces excreted, i.e.,
a study of the income and outgo. Proceed as follows:

Select a diet which is simple, i.e., consists of few constituents, and which
lends itself readily to accurate chemical analysis. A good type of diet for ordi-
nary metaboUsm experiments of this sort consists of crackers (graham or soda),

BALANCE OF CALCIUM, MAGNESIUM, PHOSPHORUS, SULPHUR, AND NITRO-
GEN IN ACROMEGALY

Calcium
oxide

Magnesium Phosphoric
oxide ; anhydride i

Sulphur Nitrogen

Grams

Ingestion (daily)

.... I . 404

0.486

3.192

1. 190

18.84

Excretion (urine)

.... O.IS9 j

0.160

1.701

1.006

17.60

Excretion (feces)

....' 1.093

0.226

1 .002

0.13s

1. 10

Excretion (total) ,

1.252 0.386

2.703 I. 141 18.70

Retention (daily).

0.242 0.100

0.489 0.049 0.14

Retention (per cent).

16.2 20.6

iS-3

41

0.7

METABOLISM 593

milk, butter, water and agar-agar (to prevent constipation). Meat specially
prepared in quantity sufficient for an entire experiment may also be utilized.
Ingest uniform quantities of these dietary constituents each day for a period of
three days.^ Make an accurate collection of the urine passed during this interval
(see page 565). Separate the feces representing the three-day period (see page
587), and analyze foods, urine and feces. The balances ordinarily prepared are
those for nitrogen, sulphur, phosphorus and calcium. Analytical methods for the
determination of these elements may be found in Chapter XXVI.

The foregoing table includes balances obtained in a metaboUsm test on
acromegaly.-

35. Excretion of Urinary and Fecal Chloride after a High Chloride Ingestion. —
Combine the procedures outlined under Experiments 14 and 33, pages 576 and

591-

36. A Study of the Elimination of Carbohydrate in Urine and Feces after

Excessive Carbohydrate Ingestion. — Combine the procedures outlined in Experi-
ments 5 and 32, pages 568 and 591.

1 See note 3, p. 589.

^Bergeim, Stewart and Hawk: Jour. Expl., Med., 20, 218, 1914.

38

REAGENTS AND SOLUTIONS

Alizarin. ^ — A i per cent solution of alizarin mono-sodium sulphonate
in water.

Almen's Reagent.- — Dissolve 5 grams of tannic acid in 240 c.c. of
50 per cent alcohol and add 10 c.c. of 25 per cent acetic acid.

Aluminium Hydroxide Cream. ^ — To a i per cent solution of ammon-
ium alum at room temperature add a slight excess of a i per cent solu-
tion of ammonium hydroxide. Wash by decantation until the wash
water shows only the faintest trace of residue on evaporation.

Ammoniacal Silver Solution.* — Dissolve 26 grams of silver nitrate
in about 500 c.c. of water, add enough ammonium hydroxide to redis-
solve the precipitate which forms upon the first addition of the ammon-
ium hydroxide and make the volume of the mixture up to i liter with
water.

Ammoniimi Thiocyanate Solution.^ — This solution is made of such
a strength that i c.c. of it is equal to i c.c. of the standard silver nitrate
solution mentioned below. To prepare the solution dissolve 12.9 grams
of ammonium thiocyanate, NH4SCN, in a little less than a liter of
water. In a small flask place 20 c.c. of the standard sUver nitrate
solution, 5 c.c. of a cold saturated solution of ferric alum and 4 c.c. of
nitric acid (sp. gr. 1.2), add water to make the total volume 100 c.c, and
thoroughly mix the contents of the flask. Now run in the ammonium
thiocyanate solution from a burette until a permanent red-brown tinge is
produced. This is the end-reaction and indicates that the last trace
of silver nitrate has been precipitated. Take the burette reading and
calculate the amount of water necessary to use in diluting the ammon-
ium thiocyanate in order that 10 c.c. of this solution may be exactly
equal to 10 c.c. of the silver nitrate solution. Make the dilution and
titrate again to be certain that the solution is of the proper strength.

Amold-Lipliawsky Reagent." — This reagent consists of two definite
solutions which are ordinarily preserved separately and mixed just before
using. The two solutions are prepared as follows:

{a) One per cent aqueous solution of potassium nitrate.

^ Indicator in various procedures, pp. 174 and 481.

-Ott's precipitation test, p. 429. Determinatiofi of lactalbumin, p. 329.

^ Removal of protein in various methods, pp. 329, 485.

* Salkowski's method, p. 516.

* Volhard-Arnold method, p. 556, and Dehn-'Clark method, p. 557.
' Arnold-Lipliawsky reaction, p. 440.

594

REAGENTS AND SOLUTIONS 595

(b) One gram of ^-amino-acetophenon dissolved in loo c.c. of
distilled water and enough hydrochloric acid (about 2 c.c.) added drop
by drop, to cause the sdution, which is at first yellow, to become entirely
colorless. An excess of acid must be avoided.

Asbestos for Suction Filters.^ The asbestos is shredded, placed in a
wide mouth flask and covered with 10 per cent HCl. Heat on water-
bath for five hours. Filter on Buchner funnel, wash free from acid,
return to the flask, cover with 5 per cent NaOH and heat on water-bath
for three hours. Filter, wash free from alkali, then with dilute acid
and finally with water until free from acid. Suspend in a large volume
of water, allow to settle for five minutes. Pour ofi" the upper two- thirds
and discard. Repeat the washing of the desired coarse portion several
times until the supernatant liquid remains nearly clear.

Bang's Sugar Reagents.- — (a) Acid KCl Solution. — Consisting
of 1360 c.c. of saturated KCl to which is added 640 c.c. of water and
1.5 c.c. 25 per cent. HCl.

{h) Stock Copper Solution. — Introduce into a 1000 c.c. flask 700 c.c.
of boiled and cooled water. Warm to about 3o°C. and add 160 grams
of pure potassium bicarbonate in powder form. When dissolved and
66 grams of pure KCl. Cool and then add 100 grams potassium carbon-
ate. Finally add 100 c.c. of 4.4. per cent, solution of pure crystalline
copper sulphate. Let stand a short time, then make to mark with
boiled water. Allow to stand a day or so before using.

(c) N/200 I Solution. — Made fresh each day. Dilute N/io I
solution 20 times. Or make as follows: Introduce into a 100 c.c.
flask 2 grams KI, 1-2 c.c. of 2 per cent KIO3 solution and 5 c.c. of N/io
HCl. Make to mark with boiled and cooled distilled water.

{d) Starch Solution. — A i per cent, solution of Kahlbaum's soluble
starch in a saturated KCl solution.

(e) Dilute Copper Solution. — Dilute 300 c.c. of the stock solution
to 1000 c.c. Mix with only gentle shaking. Let stand several hours
before using.

Barfoed's Solution.'' — Dissolve 4.5 grams of neutral, crystalUzed
copper acetate in 100 c.c. of water and add 1.2 c.c. of 50 per cent acetic
acid.

Baryta Mixture.'' — A mixture consisting of i volume of a saturated
solution of bariuyi nitrate and 2 volumes of a saturated solution of
barium hydroxide.

' See methods entailing use of Gooch crucibles.
- Determination of sugar, pages 280 and 524.
^ Barfoed's test, p. 30.
* Isolation of urea from urine, p. 375.

596 PHYSIOLOGICAL CHEMISTRY

Basic Lead Acetate Solution. ^^ — This solution possesses the following

formula:

Lead acetate ♦ 180 grams.

Lead oxide (Litharge) no grams.

Distilled water to make 1000 grams.

Dissolve the lead acetate in about 700 c.c. of distilled water, with boiling.
Add this hot solution to the finely powdered lead oxide and boil for one-
half hour with occasional stirring. Cool, filter and add sufficient dis-
tilled water to the filtrate to make the weight i kg.

Benedict's Solutions. ^ — First Modification. — Benedict's modified
Fehling solution consists of two definite solutions — a copper sulphate
solution and an alkaline tartrate solution, which may be prepared as
follows :

Copper sulphate solution = 34.65 grams of copper sulphate dissolved
in water and made up to 500 c.c.

Alkaline tartrate solution = 100 grams of anhydrous sodium carbon-
ate and 173 grams of Rochelle salt dissolved in water and made up to
100 c.c.

These solutions should be preserved separately in rubber-stoppered
bottles and mixed in equal volumes when needed for use. This is done
to prevent deterioration.

Second Modification. — Benedict has further modified his solution
and has succeeded in obtaining one which does not deteriorate upon
long standing. It has the following composition:

Copper sulphate 17.3 grams.

Sodium citrate i73-o grams.

Sodium carbonate 100. o grams.

Distilled water to make i liter.

With the aid of heat dissolve the sodium citrate and carbonate in
about 600 c.c. of water. Pour (through a folded filter paper if neces-
sary) into a glass graduate and make up to 850 c.c. Dissolve the
copper sulphate in about 100 c.c. of water and make up to 150 c.c.
Pour the carbonate-citrate solution into a large beaker or casserole and
add the copper sulphate solution slowly, with constant stirring. The
mixed solution is ready for use and does not deteriorate upon long
standing.

Benedict's Sugar Reagent.^

Copper sulphate (crystallized) 18.0 grams.

Sodium carbonate (crystallized, one-half the weight of the

anhydrous salt may be used) 200.0 grams.

Sodium or potassium citrate 200.0 grams.

Potassium thiocyanate 125.0 grams.

Potassium ferrocyanide (5 per cent solution). 5.0 c.c.

Distilled water to make a total volume of 1000. o c.c.

^ Indican determination, p. 542.

^Benedict's modifications of Fehling's test, pp. 27 and 417.

^ Quantitative determination of sugar, p. 522.

REAGENTS AND SOLUTIONS 597

With the aid of heat dissolve the carbonate, citrate and thiocyanate
in enough water to make about 800 c.c. of the mixture and filter if
necessary.

Dissolve the copper sulphate separately in about 100 c.c. of water
and pour the solution slowly into the other liquid, with constant stirring.
Add the ferrocyanide solution, cool and dilute to exactly i liter. Of the
various constituents, the copper salt only need be weighed with exact-
ness. Twenty-five c.c. of the reagent are reduced by 50 mg. of glucose.

Benedict's Sulphur Reagent.

Crystallized copper nitrate, sulphur-free or of known sulphur

content 200 grams.

Sodium or potassium chlorate 50 grams.

Distilled water to 1000 c.c.

Benzidine Solutions for Volumetric Sulphur Determinations.

— (a) Rosenheim and Drummond. — Rub 4 grams of benzidine (Kahl-
baum) into a fine paste with about 10 c.c. of water and transfer to a
2-liter flask with the aid of about 500 c.c. of water. Add 500 c.c. of con-
centrated HCl (sp. gr. 1. 1 9) and make up to 2 liters with distilled
water. 150 c.c. of this solution, which keeps indefinitely, are sufficient
to precipitate o.i gram H2SO4.

{h) Raiziss and Duhin. — Put 6.7 grams of benzidine (Merck Reagent)
in a i-liter flask, add 29 c.c. of hydrochloric acid (sp. gr. 1.12) and dilute
up to the mark.

Bertrand Sugar Reagents.^ — {a) Copper Sulphate Solution. — Forty
grams of pure crystallized copper sulphate are dissolved in water to
make a liter.

(&) Dissolve 200 grams of Rochelle salts and 150 grams of NaOH in
water to make 1000 c.c.

(c) Acid Ferric Sulphate Solution. — Dissolve 50 grams of ferric sul-
phate in about 200 c.c. of water and pour into this a mixture of 200 c.c.
of concentrated sulphuric acid diluted with about 400 c.c. of water.
Mix and make to 1000 c.c.

{d) Potassium Permanganate Solution. — Dissolve 5 grams of potas-
sium permanganate in water to make 1000 c.c. Standardization. —
Dissolve 0.250 gram of ammonium oxalate in 50-100 c.c. of water add
1-2 c.c. of concentrated sulphuric acid and titrate with the permangan-
ate to a rose color. Multiply the number of grams of oxalate used by
0.895 ^^ g^t the equivalent in Cu of the number of cubic centimeters of
permanganate used. Calculate the Cu value of i c.c.

* Determination of sugar, p. 527.

598 PHYSIOLOGICAL CHEMISTRY

Bial's Reagent.^

Orcinol 1.5 grams.

Fuming HCl 500 . 00 grams.

Ferric chloride (10 per cent) 20-30 drops.

Biuret Reagent, Gies.-— This reagent consists of lo per cent KOH
solution to which 25 c.c. of 3 per cent CUSO4 solution per liter has been
added. This imparts a slight though distinct blue color to the clear
liquid.

Biuret Paper (Kantor and Gies).- — Immerse filter paper in Gies'
Biuret Reagent (above) then dry and cut into strips.

Black's Reagent.^ — Made by dissolving 5 grams of ferric chloride
and 0.4 gram of ferrous chloride in 100 c.c. of water.

Blood Serum. — This may easily be obtained in quantity by the
procedure described under Hemagglutination in the chapter on Blood.

Boas' Reagent."* — Dissolve 5 grams of resorcinol and 3 grams of
sucrose in 100 c.c. of 50 per cent alcohol.

Bonnano's Reagent. — Dissolve 2 grams of sodium nitrite in 100 c.c.
of concentrated hydrochloric acid.

Bottu's Reagent. — To 3.5 grams of o-nitrophenylpropiolic acid
add 5 c.c. of a freshly prepared 10 per cent solution of sodium hydroxide
and make the volume of the solution i liter with distilled water.

Carmine -Fibrin.^ — Prepared by running fibrin through a meat
chopper, washing carefully and placing in 3^^ per cent ammoniacal
carmine solution (very little excess ammonia should be present) until
the maximum coloration of the fibrin (dark red) is obtained. The fibrin
is then washed in water and in water acidified with acetic acid. It is
preserved under glycerol.

Chloride Reagents for Blood Analysis.^— (a) An acid M/29.25
solution of silver nitrate, i c.c. of which is equivalent to 2 mg. of NaCl.

AgNOs 5.812 grams.

HN03(sp. gr. 1.42) 250 c.c.

Water to 1000 c.c.

{b) A solution of M/58.5 potassium iodide, i c.c. of which is equiva-
lent to I mg. of NaCl.

KI 3.0 grams.

Water to 1000 c.c.

This solution is standardized against the silver solution by adding 5 c.c.
of the latter to 5 c.c. of solution (c) and titrating with the iodide solution

I Test for pentose, p. 37.

* Protein tests, p. 100.

'Black's reaction, p. 441.

♦Test for free acid, p. 154-

"Tests on proteases, p. 12.

« Method of McLean and Van Slyke, p. 286.

REAGENTS AND SOLUTIONS 599

to the blue end point. The iodide solution is then diluted to such a
degree that lo c.c. are exactly equivalent to 5 c.c. of the silver solution.
(c) A solution used as an indicator, to regulate acidity, and provide
an oxidizing agent.

Sodium citrate (NaaCoHsOz+sM H2O) 446.0 grams.

Sodium nitrite 20.0 grams.

Soluble starch 2.5 grams.

Water to looo.o c.c.

The starch is first dissolved with the aid of heat in about 500 c.c. of the
water. The citrate and nitrite are then added, and the mixture is heated
until all is dissolved. The solution while still hot is filtered through
cotton, the filter washed with hot water, the filtrate allowed to cool,
and made up to 1000 c.c. The solution keeps indefinitely.

Combined Hydrochloric Acid (Protein Salt). — To prepare so-called
combined hydrochloric acid simply add a soluble protein such as Witte's
peptone to free hydrochloric acid of the desired strength until it no
longer responds to free acid tests (see chapter on Gastric Digestion).
For example, if 0.2 per cent combined acid is required the protein would
be added to 0.2 per cent free hydrochloric acid.

Strictly speaking there is no such thing as "combined" acid in this
sense. When the protein is added a protein salt of the acid is formed
which ionizes differently from the free acid.

Congo Red.^ — Dissolve 0.5 gram of Congo red in 90 c.c. of water
and add 10 c.c. of 95 per cent alcohol.

Congo Red-Fibrin. — This may be prepared by placing fibrin in
faintly alkaline Congo red solution and heating to 8o°C. The fibrin is
then washed and preserved under glycerol.

Creatinine, Standard Solution for Colorimetric Method. ^ — Dissolve
I gram of pure creatinine in 1000 c.c. of N/io HCl. The solution con-
tains I mg. of creatinine per cubic centimeter.

Cross and Sevan's Reagent. — Combine t-d'o parts of concentrated
hydrochloric acid and one part of zinc chloride hy weight.

Ehrlich's Diazo Reagent. '' — Two separate solutions should be pre-
pared and mixed in definite proportions when needed for use.

(a) Five grams of sodium nitrite dissolved in i liter of distilled water.

{h) Five grams of sulphanilic acid and 50 c.c. of hydrochloric acid in
I'liter of distilled water.

Solutions (a) and {b) should be preserved in well-stoppered vessels
and mixed in the proportion i : 50 when required. Green asserts that

^ Test for free acid, p. 153.

^ Determination of creatinine, p. 506.

' Ehrlich's diazo reaction, p. 454.

6oo PHYSIOLOGICAL CHEMISTRY

greater delicacy is secured by mixing the solutions in the proportion
I :ioo. The sodium nitrite deteriorates upon standing and becomes
unfit for use in the course of a few weeks.

Esbach's Reagent.^ — Dissolve lo grams of picric acid and 20 grams
of citric acid in i liter of water,

Fehling's Solution.^ — Fehling's solution is composed of two definite
solutions — a copper sulphate solution and an alkaline tartrate solution,
which may be prepared as follows:

Copper sulphate solution = 34.65 grams of copper sulphate dissolved
in water and made up to 500 c.c.

Alkaline tartrate solution =125 grams of potassium hydroxide and
173 grams of Rochelle salt dissolved in water and made up to 500 c.c.

These solutions should be preserved separately in rubber-stoppered
bottles and mixed in equal volumes when needed for use. This is done
to prevent deterioration.

Ferric Alum Solution. ^ — A cold saturated solution.

Folin-Shaffer Reagent.'*- — This reagent consists of 500 grams of am-
monium sulphate, 5 grams of uranium acetate, and 60 c.c. of 10 per
cent acetic acid in 650 c.c. of distilled water.

Formalin Solution (Neutral).^ — To 50 c.c. of commercial formalde-
hyde solution (30-40 per cent) add i c.c. of phenolphthalein solution
and then standard alkali solution until the mixture assumes a faint
red color. The solution should be freshly prepared for each set of
determinations. *

Fiurfural Solution.^ — Add i c.c. of furfural to 1000 c.c. of distilled
water.

Gallic Acid Solution.^ — A saturated alcoholic solution.

Guaiac Solution.^ — Dissolve 0.5 gram of guaiac resin in 30 c.c. of
95 per cent alcohol.

Gulick's Acid Oxidizing Mixture.^ — To 125 c.c. of ammonia free
water add 40 c.c. of sulphuric acid, 5 c.c. of a saturated solution of
mercuric chloride, and 20 grams of potassium sulphate. Then make up
to 200 c.c. with ammonia-free water.

Gulick's ModifiedWinkler Solution." — Dissolve 40 grams of sodium

' Esbach's method, p. 532.

2 Fehling's method, p. 523. Fehling's test, pp. 26 and 416.

^ Volhard-Arnold method, p. 556.

* Folin-Shaffer method, p. 511.

' Formol titration procedure, p. 502.

« Mylius's modification of Pettenkofer's test, pp. 208 and 434. v. Udrdnsky's test, pp.
208 and 434.

^ Gallic acid test, p. 32 3.

* Guaiac test, pp. 15, 235, 262, and 432.

* Determination of total nitrogen, p. 490.
'0 Determination of total nitrogen, p. 490.

REAGENTS ANT) SOLUTIONS 6oi

hydroxide in about 200 c.c. of ammonia-free water. Mix 15 grams of
mercuric iodide and 10 grams of potassium iodide and dissolve in about
15 c.c. of water. Transfer with the aid of the alkali to a 500 c.c. volu-
metric flask and make up to 500 c.c. with ammonia-free water. Trans-
fer to an Erlenmeyer flask and let stand 24 hours to settle.

Giinzberg's Reagent.^ — Dissolve 2 grams of phloroglucinol and i
gram of vanillin in 100 c.c. of 95 per cent alcohol.

Haines' Solution.- — This solution may be prepared by dissolving
8.314 grams of copper sulphate in 400 c.c. of water adding 40 c.c. of
glycerol and 500 c.c. of 5 per cent potassium hydroxide solution.

Hammarsten's Reagent.^ — Mix i volume of 25 per cent nitric
acid and 19 volumes of 25 per cent hydrochloric acid and add i volume
of this acid mixture to 4 volumes of 95 per cent alcohol. It is prefer-
able that the acid mixture be prepared in advance and allowed to stand
until yellow in color before adding it to the alcohol.

Hayem's Solution. — This solution has the following formula:

Mercuric chloride 0.25 grams.

Sodium chloride 0.5 grams.

Sodium sulphate 2.5 grams.

Distilled water 100. o grams.

Hopkins-Cole Reagent.'' — To i liter of a saturated solution of
oxalic acid add 60 grams of sodium amalgam and allow the mixture
to stand until the evolution of gas ceases. Filter and dilute with 2-3
volumes of water.

Hopkins-Cole Reagent (Benedict's Modification). — Ten grams
of powdered magnesium are placed in a large Erlenmeyer flask and
shaken up with enough distilled water to liberally cover the magnesium.
Two hundred and fifty c.c. of a cold, saturated solution of oxalic acid is
now added slowly. The reaction proceeds very rapidly and with the
liberation of much heat, so that the flask should be cooled under running
water during the addition of the acid. The contents of the flask are
shaken after the addition of the last portion of the acid and then poured
upon a filter, to remove the insoluble magnesium oxalate. A little
wash water is poured through the filter, the filtrate acidified with
acetic acid to prevent the partial precipitation of the magnesium on long
standing, and made up to a liter with distilled water. This solution
contains only the magnesium salt of glyoxylic acid.

Hypobromite Solution.^ — The ingredients of this solution should

' Test for free acid, p. 154.

-Haines' test, p. 419.

^ Hammarsten's reaction, pp. 207 and 433.

* Hopkins-Cole reaction, p. 98.

* Methods for determination of urea, p. 496.

602 PHYSIOLOGICAL CHEMISTRY

be prepared in the form of two separate solutions which may be united
as needed.

(a) Dissolve 125 grams of sodium bromide in water, add 125 grams
of bromine and make the total volume of the solution i liter.

{h) A solution of sodium hydroxide having a specific gravity of
1.25, This is approximately a 22.5 per cent solution.

Preserve both solutions in rubber-stoppered bottles and when needed
for use mix i volume of solution (a), i volume of solution (6), and 3
volumes of water.

Iodine Solution (N/io).^ — Weigh out 12.685 grams of pure resub-
limed iodine into a small weighing bottle using a porcelain spatula.
Dissolve 18 grams of pure KI in about 150 c.c. of water. Transfer the
iodine to a liter flask washing out the last traces with some of the KI
solution, which is then poured into the flask. Stopper and shake
occasionally until dissolved. If necessary a few more crystals of KI
may be added to aid solution. Dilute to the mark and mix well.
Keep in glass-stoppered bottle in cool dark place. Standardize at once
against N/io sodium thoisulphate solution. Measure out accurately
25 c.c. of the iodine solution into an Erlenmeyer flask, run in sodium
thiosulphate until the color is pale yellow, then add a few cubic centi-
meters of a I per cent solution of starch (preferably soluble starch)
and titrate to disappearance of blue color. Care should be taken near
the end point.

Iodine Solution. ^ — Prepare a 2 per cent solution of potassium iodide
and add suflicient iodine to color it a deep yellow.

Iodine-Zinc Chloride Reagent.^ — Dissolve 20 grams of zinc chloride
in 8.5 c.c. of water. Cool, and introduce iodine solution (3 grams KI+
1.5 gram I in 60 c.c. of water) drop by drop until iodine begins to pre-
cipitate.

Kraut's Reagent.^ — Dissolve 272 grams of potassium iodide in
water and add 80 grams of bismuth subnitrate dissolved in 200 grams
of nitric acid (sp. gr. 1.18). Permit the potassium nitrate to crystallize
out. then filter it off and make the filtrate up to i liter with water.

Lead Acetate, Basic. (See Basic Lead Acetate.)

Lugol's Solution.^ — Dissolve 4 grams of iodine and 6 grams of potas-
sium iodide in 100 c.c. of distilled water.

Magnesia Mixture.^ — Dissolve 175 grams of magnesium sulphate
and 350 grams of ammonium chloride in 1400 c.c. of distilled water.

' Determination of acetone and acetoacetic acid, p. 5 33.

* Iodine test, p. 45.

^ Amyloid formation, p. 49.

* Rosenheim's bismuth test for choline, p. 357.

' Gunning's iodoform test, page 436, and Bardach's reaction, p. loi.
6 Method for determination of total phosphorus, p. 554.

REAGENTS AND SOLUTIONS 603

Add 700 grams of concentrated ammonium hydroxide, mix thoroughly,
and preserve the mixture in a glass-stoppered bottle.

Magnesium Nitrate Solution for Ignition.^ — Dissolve 320 grams of
calcined magnesia in nitric acid, avoiding an excess of the latter; then
add a little calcined magnesia in excess; boil; filter from the excess of
magnesia, ferric oxide etc., and dilute with water to 2 liters.

Methyl Red.- — Saturated solution in 50 per cent alcohol.

Millon's Reagent."* — Digest i part (by weight) of mercury with
2 parts (by weight) of nitric acid (sp. gr. 1.42) and dilute the resulting
solution with 2 volumes of water.

Molisch's Reagent.^ — A 15 per cent alcoholic solution of a-naphthol.

Molybdate Solution.^ — Dissolve 100 grams of molybdic acid in 144
c.c. of ammonium hydroxide (sp. gr. 0.90) and 271 c.c. of water; slowly
and with constant stirring pour the solution thus obtained into 489 c.c.
of nitric acid (sp. gr. 1.42) and 1148 c.c. of water. Keep the mLxture in
a warm place for several days, or until a portion heated to 4o°C. deposits
no yellow precipitate of ammonium phosphomolybdate. Decant the
solution from any sediment and preserve in glass-stoppered bottles.

Momer's Reagent.'^ — Thoroughly mix i volume of formalin, 45
volumes of distilled water, and 55 volumes of concentrated sulphuric
acid.

Nakayama's Reagent.'' — Prepared by combining 99 c.c. of alcohol
and I c.c. of fuming hydrochloric acid containing 4 grams of ferric
chloride per liter.

a-Naphthol Solution.^ — Dissolve i gram of a-naphthol in 100 c.c of
95 per cent, alcohol.

Nessler-Winkler Solution.

Mercuric iodide lo grams.

Potassium iodide 5 grams.

Sodium hydroxide 20 grams.

Water 100 c.c.

The mercuric iodide is rubbed up in a small porcelain mortar with
water, then washed into a flask and the potassium iodide added. The
sodium hydroxide is dissolved in the remaining water and the cooled
solution added to the above mixture. The solution cleared by standing
is preserved in a dark bottle.

' Determination of phosphorus, p. 554.

^ Determination of H ion concentration, pp. 158 and 480.

' Millon's reaction, p. 97.

* Molisch's reaction, p. 21.

* Detection and determination of phosphorus, pp. 129 and 554.
' Momer's test, p. 86.

^ Nakayama's reaction, pp. 207 and 433.

* Oxidases p. 14. For other a-naphthol solution see Molisch reaction.

6o4 PHYSIOLOGICAL CHEMISTRY

Neutral Olive Oil.^ — Shake ordinary olive oil with a lo per cent
solution of sodium carbonate, extract the mixture with ether, and
remove the ether by evaporation. The residue is neutral olive oil.

Neutral Red.^^ — ^A i per cent solution in 50 per rent alcohol.

p-Nitrophenol.^ — A i per cent solution in 50 per cent alcohol.

Nylander's Reagent.^ — Digest 2 grams of bismuth sub nitrate
and 4 grams of Rochelle salt in 100 c.c. of a 10 per cent solution
of potassium hydroxide. The reagent should then be cooled and
filtered.

Obennayer's Reagent.^ — Add 2-4 grams of ferric chlorid to a
liter of hydrochloric acid (sp. gr. 1.19).

Oxalated Plasma.^ — Allow arterial blood to run into an equal volume
of 0.2 per cent ammonium oxalate solution.

Para-dimethylaminobenzaldehyde Solution.^ — This solution is made
by dissolving 5 grams of para-dimethylaminobenzaldehyde in 100 c.c.
of 10 per cent sulphuric acid.

Para-phenylenediamine Hydrochloride Solution.'^ — Two grams dis-
solved in 100 c.c. of water.

Peters' Sugar Reagents.^ — {a) Copper Solution. — Dissolve 34.639
grams of highest purity crystallized copper sulphate (such as Kahl-
baum's "zur analyse mit garantieschein") in water to make 500 c.c.

{h) Alkaline Tartrate Solution. — Dissolve 173 grams of sodium
potassium tartrate and 125 grams of potassium hydroxide in water to
make 500 c.c.

(c) iV/5 Sodium Thiosulphate. — Dissolve about 50 grams of ordinary
c.p. sodium thiosulphate or exactly 49.66 grams of the pure, dry,
recrystallized salt, in enough boiled out distilled water to make a
liter. Allow to stand for several days. The solution should be stan-
dardized against the copper solution prepared as above. For this
purpose introduce 20 c.c. of the copper solution into a 200 c.c. Erlen-
meyer flask, add 20 c.c. of strong acetic acid (30 per cent) and 40 c.c. of
water. Add about 7 grams of a saturated solution of KI and titrate
with the thiosulphate using starch as an indicator. Calculate the
equivalent of i c.c. of thiosulphate in Cu. One c.c. of the copper
sulphate solution contains 17.647 mg. of Cu. The thiosulphate remains
constant for some months. It should be kept in a dark bottle.

* Emulsification of fats, p. 180.

'^ Determination of H ion concentration, pp, 158 and 480.
'Nylander's test, pp. 29 and 420.

* Obermayer's test, p. 388.

^ Experiments on blood plasma, p. 268.

* Herter's para-dimethylaminobenzaldehyde reaction, p. 219.
' Detection of hydrogen peroxide, p. 323.

* Determination of sugar, p. 525.

REAGENTS AND SOLUTIONS 605

Phenolphthalein.^ — Dissolve i gram of phenolphthalein in loo c.c.
of 95 per cent alcohol.

Permanganate Solution (Alkaline) for Van Slyke Method. ^ — The

alkaline permanganate solution contains 50 grams of potassium per-
manganate and 25 grams of potassium hydroxide per liter.

Potassium Permanganate Standard (N/io) Solution. — Dissolve
3.162 grams of pure potassium permanganate in a liter of distilled
water, allow to stand a few days, and filter through glass wool. Stand-
ardize against N/io oxalic acid solution or against pure dry sodium or
potassium oxalate. One c.c. of N/io permanganate is equivalent to
7.0 mg. of sodium oxalate.

Phenylhydrazine Mixture.^ — This mixture is prepared by com-
bining I part of phenylhydrazine-hydrochloride and 2 parts of sodium
acetate by weight. These are thoroughly mixed in a mortar.

Phenylhydrazine -Acetate Solution.^ — This solution is prepared by
mixing i volume of glacial acetic acid, i volume of water, and 2 volumes
of phenylhydrazine (the base).

Picramic Acid. — Permanent Standard for Lewis-Benedict Blood Sugar

Method} — A solution of picramic acid makes a very satisfactory

permanent standard. The color is identical in quality with that formed

in the method and its solution keeps perfectly. The formula of the

permanent standard is:

Picramic acid o . 064 gram.

Sodium carbonate (anhydrous) *. o. loo gram.

Water to make 1000. o c.c.

Dissolve the picramic acid with the aid of heat in 25-50 c.c. of distilled
water which has been made alkaline with sodium carbonate. Cool and
dilute to I liter. This solution has the same intensity of color as that
obtained by the proposed method with 0.64 mg. of sugar when the
final volume of the reaction fluid is made 10 c.c. The solution should
be standardized against pure glucose. A satisfactory preparation of
picramic acid may be obtained from the J. T. Baker Chemical Co.,
Phillipsburg, N. J.

Roberts' Reagent.*' — Mix i volume of concentrated nitric acid and
5 volumes of a saturated solution of magnesium sulphate.

Rosenheim's lodo-Potassiimi Iodide Solution." — Dissolve 2 grams
of iodine and 6 grams of potassium iodide in 100 c.c. of water.

' Tdpfer's method, p. 174.

* Determination of amino-acid nitrogen p. 88.
'Phenylhydrazine reaction, pp. 22 and 413.

* Phenylhydrazine reaction, pp. 22 and 413.
' Determination of sugar in blood, p. 279.

* Roberts' ring test, pp. 104 and 424.
^ Rosenheim's periodide test, p. 273.

6o6 PHYSIOLOGICAL CHEMISTRY

Sahli's Reagent.^ — This reagent consists of a mixture of equal parts
of a 48 per cent solution of potassium iodide and an 8 per cent solution of
potassium iodate.

Salted Plasma. 2 — Allow arterial blood to run into an equal volume
of a saturated solution of sodium sulphate or a 10 per cent solution of
sodium chloride. Keep the mixture in the cold room for about 24
hours.

Schweitzer's Reagent.^ — Add potassium hydroxide to a solution of
copper sulphate which contains some ammonium chloride. Filter off
the precipitate of cupric hydroxide, wash it, and bring 3 grams of the
moist cupric hydroxide into solution in a liter of 20 per cent ammonium
hydroxide.

Scott-Wilson Acetone Reagents.^ — (a) Mercury Reagent. — This
reagent is made up as follows: Mercuric cyanide 10 grams, sodium
hydroxide 180 grams, water 1200 c.c. The solution is agitated in a flask
and 400 c.c. of a 0.7268 per cent solution of silver nitrate slowly run in.
Let stand three days and decant supernatant liquid. The silver nitrate
solution is made by taking i part of standard silver nitrate solution
(i c.c. = 10 mg. NaCl) and 3 parts of water.

{h) Standard Potassium Thiocyanate Solution. — Make up an approxi-
mately 0.1 per cent solution of potassium thiocyanate and standardize
it against mercuric nitrate or silver nitrate. It is convenient to have the
solution of such strength that i c.c. = i mg. of Hg.

(c) Acid Mixture. — Nitric acid 40 parts, sulphuric acid 5 parts, and
water 55 parts.

{d) Permanganate N/s Solution. — Dissolve 6.324 grams of potassium
permanganate in water and make up to a liter.

Seliwanoff's Reagent.^ — Dissolve 0.05 gram of resorcinol in 100 c.c.
of dilute (i : 2) hydrochloric acid.

Sherrington's Solution.*' — This solution possesses the following
formula :

Methylene-blue o . i gram.

Sodium chloride 1.2 grams.

Neutral potassium oxalate .' 1.2 grams.

Distilled water 300 . o grams.

Silver Nitrate Solution.^ — Dissolve 29.042 grams of silver nitrate in
I liter of distilled water. Each cubic centimeter of this solution is

' Determination of free acid, p. 164.
^ Experiments on blood plasma, p. 268.
' Schweitzer's solubility test, p. 49.

* Determination of acetone and acetoacetic acid, pp. 284 and 536.

* Seliwanoff's reaction, pp. 35 and 447.

* "Blood counting," p. 305.

' Volhard-Arnold method, p. 556, Mohr's method, p. 558, and Dehn-Clark method,
p. 558.

REAGENTS AND SOLUTIONS 607

equivalent to o.oi gram of sodium chloride or to 0.006 gram of
chlorine.

Sodium Acetate Solution.^ — Dissolve loo grams of sodium acetate
in 800 c.c. of distilled water, add 100 c.c. of 30 per cent acetic acid
to the solution, and make the volume of the mixture up to i liter with
distilled w^atcr.

Sodium Alcoholate (N/io) Solution.- — The sodium alcoholate is
made by dissolving 2.3 grams of cleaned metallic sodium in i liter of
absolute alcohol. It is advisable that it be slightly weaker than stronger
than tenth-normal. It may be standardized against pure benzoic acid
in washed chloroform. It may also be standardized against N/io HCl
provided the alcoholate solution contains not more than traces of
carbonate.

Sodium Alizarin Sulphonate.^ — Dissolve i gram of sodium alizarin
sulphonate in iDo c.c. of water.

Sodium Sulphide Solution.^ — Saturate a i per cent solution of
sodium hydroxide with hydrogen sulphide gas and add an equal volume
of I per cent sodium hydroxide.

Sodium Thiosulphate Standard (N/io) Solution.^ — Weigh out 25
grams of ordinary c.p. sodium thiosulphate or 24.83 grams of the pure
dry recrystallized salt. Dissolve in water and dilute to a liter. Boiled
distilled water must be used. Keep in a bottle wdth a siphon arrange-
ment and carrying a soda lime tube to exclude CO2.

It is best standardized against acid potassium iodate KH(I03)2-
Weight out accurately 0.3249 gram of acid potassium iodate. Dissolve
in 50 c.c. of water, heating gently if necessary. Transfer the solution to
a 100 c.c. flask, rinsing the beaker carefully and make to mark with
water. This solution is exactly decinormal. Pipette out 25 c.c. into an
Erlenmeyer flask, add i gram of potassium iodide dissolved in a
little water, and a few cubic centimeters of dilute hydrochloric add.
Titrate immediately with the thiosulphate solution. When the solution
becomes pale yellow add a few cubic centimeter of i per cent solution of
soluble starch and titrate to loss of blue color.

Solera's Test Paper. ^' — Saturate a good quality of filter paper with
0.5 per cent starch paste to which has been added sufficient iodic acid
to make a i per cent solution of iodic acid and allow the paper to dry
in the air. Cut it in strips of suitable size and preserve for use.

^ Uranium acetate method, p. 552.

- Determination of hippuric acid, p. 519.

^Topfer's metliod, p. 174.

* Kruger and Schmidt's method, p. 513.

' Determination of acetone and acetoacetic acid, p. 533.

* Solera's reaction, p. 59.

6o8 PHYSIOLOGICAL CHEMISTRY

Spiegler's Reagent.^ — This reagent has the following composition:

Tartaric acid 20 grams.

ISIercuric chloride 40 grams.

Sodium chloride 50 grams.

Glycerol 100 grams.

Distilled water 1000 grams.

Starch Iodide Solution.^ — Mix o.i gram of starch powder with
cold water in a mortar and pour the suspended starch granules into 75-
100 c.c. of boiling water, stirring continuously. Cool the starch paste,
add 20-25 grams of potassium iodide and dilute the mixture to 50 c.c.
This solution deteriorates upon standing, and therefore must be freshly
prepared as needed.

Starch Paste. — Grind 2 grams of starch powder in a mortar with a
small amount of water. Bring 200 c.c. of water to the boiling-point and
add the starch mixture from the mortar with continuous stirring. Bring
again to the boiling-point and allow it to cool. This makes an approxi-
mate I per cent starch paste which is a very satisfactory strength for
general use.

Stokes' Reagent.^ — A solution containing 2 per cent ferrous sulphate
and 3 per cent tartaric acid. When needed for use a small amount
should be placed in a test-tube and ammonium hydroxide added until
the precipitate which forms on the first addition of the hydroxide has
entirely dissolved. This produces ammonium ferrotartrate, which is a
reducing agent.

Suspension of Manganese Dioxide.^ — Made by heating a 0.5 per
cent solution of potassium permanganate with a little alcohol until it is
decolorized.

Tanret's Reagent.^ — Dissolve 1.35 grams of mercuric chloride in
25 c.c. of water, add to this solution 3.32 grams of potassium iodide
dissolved in 25 c.c. of water, then make the total solution up to 60 c.c.
with distilled water and add 20 c.c. of glacial acetic acid to the mixture.

Tincture of Iodine."— Dissolve 70 grams of iodine and 50 grams of
postassium iodide in i liter of 95 per cent alcohol.

Toison's Solution.^ — This solution has the following formula:

Methyl violet o . 025 gram.

Sodium chloride i . o gram.

Sodium sulphate 8.0 grams.

Glycerol 30.0 grams.

Distilled water 160.0 grams.

' Spiegler's ring test, pp. 104 and 424.

* Fehling's method, p. 523.

' Hemoglobin, p. 296. Hemochromogen, p. 299.

* Kriiger and Schmidt's method, p. 513.
' Tanret's test, pp. 104 and 425.

* Smith's test, pp. 268 and 433.
' "Blood counting," p. 305.

REAGENTS AND SOLUTIONS 609

Topfer's Reagent J — Dissolve 0.5 gram of di-methylaminoazobenzene
in 100 c.c. of 95 per cent alcohol.

Tropaeolin OO.- — Dissolve 0.05 gram of tropaeolin 00 in 100 c.c.
of 50 per cent alcohol.

Uffelmann's Reagent. ' — Add a 5 per cent solution of ferric chloride
to a I per cent solution of carbolic acid until an amethyst-blue color is
obtained.

Uranium Acetate Solution.^ — Dissolve about 35.0 grams of uranium
acetate in i liter of water with the aid of heat and 3-4 c.c. of glacial
acetic acid. Let stand a few days and filter. Standardize against a
phosphate solution containing 0.005 gram of P2O5 per cubic centimeter.
For this purpose dissolve 14.721 grams of pure air-dry sodium am-
monium phosphate (NaNH4HP04+4H20) in water to make a liter.
To 20 c.c. of this phosphate solution in a 200 c.c. beaker add 30 c.c.
of water and 5 c.c. of sodium acetate solution (see above) and
titrate with the uranium solution to the correct end reaction as indi-
cated in the method proper, page 552. If exactly 20 c.c. of uranium
solution are required i c.c. of the solution is equivalent to 0.005 gram
P2O5. If stronger than this dilute accordingly and check again by
titration.

Urease.^ — (a) Soy Bean Meal. — Grind the soy bean to a powder
which will pass through a 20-mesh sieve.

(b) Solid Urease Preparation. — Digest i part of soy bean meal with
5 parts of water at room temperature, with occasional stirring for an
hour, and clear the solution by filtration through paper pulp or centri-
fugation. Pour this extract slowly, with stirring, into at least 10 volumes
of acetone. The acetone dehydrates the enzyme preparation. Filter,
dry in vacuum and powder. For standardization procedure see the
determination of urea in urine.

(c) Enzyme Solution. — Dissolve 2 grams of urease, prepared as above,
together with 0.6 gram of di-potassium-hydrogen phosphate and 0.4
gram of mono-potassium-dihydrogen phosphate in 10 c.c. of water.
The solution may be kept under toluol for two weeks, without losing
activity.

Uric Acid Reagents.*"' — (a) Silver Magnesium Solution. —

3 per cent silver lactate solution 70 c.c.

Magnesia mixture 30 c.c.

Concentrated ammonium hydroxide solution 100 c.c.

^ Topfer's method, p. 174.
^Test for free acid, p. 154.

* Uffelmann's reaction, p. 170.

* Phosphate determination, p. 552.
^ Determination of urea, p. 491.

* Determination of uric acid, p. 274 and p. 510.

39

6lO PHYSIOLOGICAL CHEMISTRY

(b) Uric Acid Reagent for Colorimetric Method. — Place loo grams of
sodium tungstate, 80 c.c. of 85 per cent phosphoric acid, and 750 c.c. of
distilled water in a liter flask. Boil the mixture with a reflux condenser
for two hours, cool and dilute to i liter, filtering if necessary.

(c) Sodium Carbonate Solution. — Dissolve 200 grams anhydrous
sodium carbonate in warm water and make up to i liter.

{d) Uric Acid Formaldehyde Standard. — Place i gram of uric acid in
a liter volumetric flask and dissolve with 200 c.c. of a 0.4 per cent lithium
carbonate solution. Add to the solution 40 c.c. of 40 per cent formalde-
hyde solution, shake the mixture and allow to stand for a few minutes.
Acidify the clear solution with 20 c.c. of normal acetic acid and dilute
to mark with distilled water The solution should remain perfectly
clear and the next day (not before) may be standardized against a
freshly prepared solution of uric acid in lithium carbonate. The color
produced by 5 c.c. of this solution corresponds very closely to that
produced from i mg. of pure uric acid. The colorimeter reading ob-
tained from the solution when thus compared with pure uric acid (i mg.)
is, of course, thereafter used as the standard value corresponding to i mg.
of uric acid.

{e) Uric Acid Standard in Phosphate Solution. — Dissolve 9 grams of
pure crystallized disodium hydrogen phosphate, together with i gram
of crystallized sodium dihydrogen phosphate, in 200 to 300 c.c. of hot
water, and filter if the solution is not perfectly clear. Make this
filtrate up to about 500 c.c. with hot water, and pour this hot or warm
(and perfectly clear) solution upon exactly 200 mg. of pure uric acid
suspended in a few cubic centimeters of water in a liter volumetric
flask. Agitate the mixture for a few minutes until the uric acid com-
pletely dissolves. Cool, add exactly 1.4 c.c. of glacial acetic acid,
dilute to the mark, and mix. Add about 5 c.c. of chloroform to pre-
vent the growth of bacteria or moulds in the solution. Five c.c. of
this solution contain exactly i mg. of uric acid.

The solution of uric acid in the phosphate solution is very readily
prepared, does not need to be standardized, and appears to keep
indefinitely.

REAGENTS AND SOLUTIONS

6ll

INTERNATIONAL ATOMIC WEIGHTS, 191 6

0= 16.

Aluminium Al 27.1

Antimony Sb 120.2

Arsenic As 74 96

Barium Ba 137-37

Bismuth Hi 208.0

Boron B 11 .0

Bromine Br 79.92

Cadmium Cd 1 1 2 . 40

Calcium Ca 40.07

Carbon C 12. 005

Chlorine CI 35 46

Chromium Cr 52.0

Cobalt Co '58.97

Copper Cu 63.57

Fluorine F 19.0

Glucinum Gl 9.1

Gold Au 197. 2

Hydrogen H i . 008

Iodine I 126.92

Iridium Ir 193 . i

Iron Fe 55 84

Lanthanum La 1390

Lead Pb 207 . 20

Lithium Li 6.94

Magnesium ^Ig 24.32

0= 16.

Manganese Mn 54. 93

Mercury Hg 200.6

Molybdenum Mo 96.0

Nickel Ni 58.68

Nitrogen N 14.01

Osmium Os 190.9

Oxygen O 16.00

Palladium Pd 106 . 7

Phosphorus P 31 04

Platinum Pt 195 . 2

Potassium K 39- 10

Radium Ra 226.0

Selenium Se 79 • 2

Silicon Si 28.3

Silver Ag 107.88

Sodium Na 23 . 00

Strontium Sr 87 . 63

Sulphur S 32.06

Tantalum Ta 181 . 5

Tellurium Te 127.5

Tin Sn 118. 7

Titanium Ti 48. i

Tungsten W 184.0

Ui'anium U 238. 2

Zinc Zn 65.37

INDEX

Main references are in heavy-faced type.

Abderhalden test for pregnancy, principle of, 3
Absorption of carbohydrate as influenced by fat

ingestion, 568
Acacia solution, formation of emulsion by, 178
Acetoacetic acid, 270, 284, 412, 438, 539
Amold-Lipliawsky test for, 440
formula for, 438
Gerhardt's test for, 439
Hurtley's reaction for, 440
Le Nobel reaction for, 439
quantitative determination of, 284, 294, S39
Acetone, 270, 284, 294, 412, 43S, 538
bodies, 270, 284, 435i 533

determination of in blood, 284
of in urine, 533
formula for, 435
Frommer's test for, 438
Gunning's iodoform test for, 436
Legal's iodoform test for, 437
Lieben's test for, 437

quantitative determination of, 284, 294, 538
Reynolds-Gunning test for, 438
Rothera's reaction for, 438
Acholic stool, 223
Achroo-dextrins, 43, 56
a-achroo-dextrin, 56
0-achroo-dextrin, 56
-)-achroo-dextrin, 56
Acid, acetic, 335, 370, 397

acetoacetic, 270, 284, 412, 438, 539

alloxyproteic, 369, 392

amino-acetic, 69, 71

amino-butyric, 214

amino-ethyl-sulphonic, 204, 346

a-amino-/3-hydroxy-propionic, 69, 73

a-amino-^-imidazol-propionic, 68, 77

a-amino-iso-butyl-acetic, 69, 79

a-amino-/S-methyl-^-ethyl-propionic, 68, 80

a-amino-normal glutaric, 69, 82

ot-amino-propionic, 68, 72

amino-succinic, 69, 82

amino- valerianic, 214

a-amino-iso- valerianic (see Valine), 69, 78

a-diamino-^-dithiolactyl, 69, 75

aspartic, 69, 82

benzoic, 72, 369. 390, 395, 583. S86

butyric, 8, 319, 323, 370, 397

caproic, 313, 319

carbamic, 247

cholic, 204

chondroitin-sulphuric, 335, 369, 392

citric, 313

combined hydrochloric (protein salt), 56, I40j

I7S
cyanuric, 373
a-«-diamino-caproic, 68, 80

Acid, diaminotrihydroxydodecanoic, 68, 85
diazo-benzene-sulphonic, 454
ethereal sulphuric, 212, 369, 385
fatty, 176, 178. 182, 212. 370, 397
formic, 26, 370, 397

free hydrochloric, 56, 140, 155, 164, 175
glucothionic, 467
glutamic, 69, 82

glycerophosphoric, 353. 354. 370, 399
glycocholic, 204
glycosuric, 395
glycuronic, 36, 38, 442
glyoxylic, 98

guanidine-or-amino-valerianic, 68, 79
hippuric, 72, 369. 388, 390, 396, 585
homogentisic, 26, 369, 394, 417
hydroxymandelic, 369. 395
iminazolpropionic, 214
indolacetic, 214. 452
indole-ot-amino-propionic, 68, 77
indoxyl-sulphuric, 212, 369, 385
inosinic, 341, 346
kynurenic, 369, 394
lactic. 40, 140, 159. 170, 3i4i 340, 342
lauric, 313

mucic, 36, 40, 445. 446
myristic, 313

nucleic 94. 123. I24. I30-I33
osmic, 356
oxalic, 369. 391. 545
oxaluric, 369, 397

oxy-a-pyrrolidine-carboxylic, 68, 8s
oxyproteic, 369, 392

palmitic, 176. i77, 181, 182

para-cresolesulphuric, 369, 385

para-oxyphenyl-acetic, 212, 214, 369, 394

para-oxy-^-phenyl-o-amino-propionic, 69, 74
86

para-oxyphenyl-propionic. 212, 214,369.394

paralactic, 247, 314. 342. 370, 398

phenaccturic, 370. 398

phenol-sulphuric, 369, 38s

phenylacetic, 214

phcnyl-a-amino propionic, 69. 73

phenylpropionic, 214

phosphocarnic, 341, 346, 370. 399

phosphoric. 406

pyrocatechin-sulphuric, 369, 385

a-pyrrolidine-carboxylic, 68. 85

sarcolactic, 342

skatole acetic, 77

skatole carbonic, 217, 220
, skatoxyl-sulphuric, 369, 385

stearic. 177, 354

succinic, 214

sulphanilic, 455
613

6i4

INDEX

Acid, tannic, 45, 48, 103
taurocholic, 204
trichlorethylglucuronic, 417
uric. 26, 127, 247, 274. 341. 369. 371, 377. 438,

460, 475. 510
urocanic, 370, 398
uroferric, 369, 392
uroleucic, 369

volatile fatty, 212, 215, 370, 397
Acid albuminate. See Acid metaprotein.
Acid-forming foods, influence of on hydrogen ion

concentration of urine, 580
Acid infraprotein. See Acid metaprotein.
Acid metaprotein, 95, 115, 116
coagulation of, 116
experiments <- i. 116
precipitati' . ■;, ii6
preparation of, 116
solubility of, 116
sulphur content of, 116
Acidity of gastric juice, quantitative determina-
tion of, 148, IS9, 162
urine, cause of, 361, 406

quantitative determination of, by hy-
drogen ion concentration, 840
by titration, 479
Acidosis, 441, 576

metabolism in, 576
Acid-hematin, 254, 269, 299
Acree-Rosenheim formaldehyde reaction, 100
Acrolein, formation of, from olive oil, 180

from glycerol, 183
Activation, 6, 187
Activation by calcium salts, 187
Adam's paper coil method for determination of

fat in milk, 326
Adaptation, 57
Adenase, 4

Adenine, 4, 125, 126, 127, 132, 347, 370, 401
Adipocere, 179

Adrenaline, determination of in adrenals, 290
Agar-agaj-, 20, 50, 22J, 589
Agglutination, 250, 262
Alanine, 68, 72, 214
Albumin, egg, 93, 107

crystallized, preparation of, 106
powdered, preparation of, 107

tests on, 107
serum, 93, 245, 268, 412, 422
solution, preparation of, 97
Albumin in urine, 412, 422

acetic acid and potassium ferrocyanide
test for, 425
coagulation or boiling test for, 424
determination of, 531
Heller's ring test for, /<23
Roberts' ring test for, 424
sodium chloride and acetic acid test for, 425
Spiegler's ring test for, 42J
Tanret's test for, 425
tests for, 423
Albumins, 93, 95, 96
Albuminates. See Metaproteins.
Albuminates, formation of, by metallic salts, 102
Albuminoids, 93, 112, 330
Albumoscope, 103, 423
Albumoses (see Proteoses, p. 118)
Alcohol-soluble proteins (see Prolamins, p. 1 1 1)

Alcoholic-zinc chloride test for urobilin, 401

Aldehyde, 25, 42

Aldehyde group, 39

Aldehyde test for alcohol, 42

v. Aider's method of detecting proteose in urine,

427
Aldose, 19

Aliphatic nucleus, 65, 68

Alizarin yellow R, use of, as indicator, 157, 158
Alkali albuminate. See Alkali metaprotein.
Alkali-hematin, 254, 298
Alkali metaprotein, 95, 115, 116
experiments on, 116
precipitation of, 116
preparation of, 116
sulphur content of, 116
Alkaline tide, 362, 577

demonstration of, 577
AUantoin, 369, 392

crystalline form of, 392
experiments on, 393
formula for, 392

preparation of, from uric acid, 393
quantitative determination of, by Wiechow-
ski-Handovsky method, 518
by difference, 510
separation of, from urine, 393
Allen's modification of Fehling's test, 419
Alm^n's reagent, preparation of, 429
Alloxyproteic acid, 369, 392
Aloin-turpentine test for "occult blood," 73s
Aluminium hydroxide, use of, in removal of

protein, 276, 329
Amalgamation test for mercury, 450
Amandin, 93
Amide nitrogen, 64

Amino acids, 65, 67. 68, 186, 195, 248, 270, 369,
394
group, 65, 88, 99

preparation of, in crystalline form, &S, 87
a-amino-^-hydroxy-propionic acid, 69, 73
a-amino-/3-imidazol-propionic acid, 68, 77
a-amino-iso-butyl-acetic acid, 69, 78
«-amino-normal-glutaric acid, 69, 82
Amino-butyric acid, 214
Amino-nitrogen, quantitative determination of,

88, 91, 277, 502
Amino-succinic acid, 69, 82
Amino-valerianic acid, 214
cr-amino-iso-valerianic acid, 69, 78
Ammonia, 64, 67, 71, 107
in blood, 247, 270

quantitative determination of, 278
in urine, 370, 402, soi, S7S

quantitative determination of, 499
Ammoniacal cupric hydroxide, solubility test, 49
Ammoniacal silver solution, preparation of, 594
Ammoniacal-zinc chloride test for urobilin, 400
Ammonium benzoate, synthesis of, to form

hippuric acid, 585
Ammonium magnesium phosphate ("Triple
phosphate"), 363, 408
in urinary sediments, 458
Ammonium purpurate, 381
Ammonium urate, 363, 377, 461, sn

crystalline form of, Plate VI, opposite
p. 462
Amphopeptone, 95, ii9 ,

INDEX

6l

Amygdalin, 4

Amylase, pancreatic, 4, 11, 187, 192

digestion of dry starch by, 188, 192

inulin by, 192
experiments on, 11, 191
influence of bile upon action of, 192
most favorable temperature for action
of, 192
salivary, 4, 10. 55, 140

activity of, in stomach, 57, 140
experiments on, 10, 59
inhibition of activity of, 57, 61
nature of action of, 56
products of action of, 56
vegetable, 4, 10
Amylases, 4, 10, SS. 187

experiments on, 10, 59, 191, 239
Amyloid, 49, 113
Amylolytic enzymes. See Amylases.

quantitative determination of activity
of, 192, 239
Anabolism, 564
Animal parasites in feces, 227

in urinary sediments, 465, 474
Anti-enzymes, 9

experiments on, 17
Antimony pentachloride as cellulose solvent. 50
Antimony trichloride as cellulose solvent, 49
Antipepsin, 9, 17
Antipeptone, 95, 119
Antirennin, 9
Antithrombin, 257
Antitrypsin. 9, i8
Aporrhegmas, 214
Arabinose. 19, 37, 443

Bial's reaction for, 37, 443
orcinol test on, 38. 444
phenylhydrazine test on, 38
Tollens' reaction on, 38, 443
Arginase, 4

Arginine, 4. 67, 68, 79, i86

Arnold-Lipliawsky reaction for acetoacetic acid,
440
reagent, preparation of, 440
Aromatic oxyacids, 369, 394
Arsenic in urine, detection of, 448

determination of, 448
Ascaris, 17, 18

Ash of milk, quantitative determination of, 327
Asparagine, 82

formula for, 82
Aspartic acid, 65, 67, 69, 82

crystalline form of, 81
formula for, 82
Assimilation limit, 2t

Assimilation limit of dextrose, 21, 413. 568
Atkinson and Kendall's hemin test, 266
Autolytic enzymes, 3
Azolitmin, use of, as indicator, 158

Babcock fat method, 324

tube, 324
Bacteria iiT feces. 221. 224, 225, 588

quantitative determination of. 241
Bacterial nitrogen in feces, 226, 588
determination of, 241
Balance, metabolic preparation of, 592
calcium, 592

Balance, magnesium, 592
nitrogen, 592
phosphorus, 592
sulphur, 592
Bang reduction flask, 281
Bang's method for estimation of sugar in blood.

280
Bang's method for estimation of sugar in urine, 524
Bardach's reaction, loi

Barfoed's reagent, preparation of, 30. 200, 595
Barfoed's test for monosaccharides, 30
Baryta mixture, preparation of, 37s, S9S
Base-forming foods, influence of on hydrogen ion

concentration of urine, 362, 580
Basic lead acetate solution, 542, 596
Bayberry tallow, saponification of, 181

source of, 181
Bayberry wax. See Bayberry tallow, i8i
Bead test (Einhorn), 238
Beckmann-Heidenhain apparatus, 365
" Bence-Jones' protein," detection of, 428
Benedict creatine preparation, 384
Benedict and Bock's method for quantitative

determination of total nitrogen, 488
Benedict and Lewis method for sugar in blood, 279
Benedict-Folin creatinine preparation, 383
Benedict-Folin method for creatine in urine, 508
Benedict-Hitchcock method for uric acid in urine,

Sio
Benedict- Murlin method for amino-acid nitrogen

in urine, 504
Benedict-Pearce method for sugar in blood, 280
Benedict's method for quantitative deter-
mination of sugar, 522
Benedict's method for quantitative deter-
mination of sulphur, 548
Benedict's method for quantitative deter-
mination of urea, 494
Benedict's method for uric acid in blood, 275
Benedict's modifications of Fehling's test. 27, 417
solution, for use in quantitative deter-
mination of sugar, preparation of, 522. 596
solutions, preparation of, 27, 417, 596
sulphur reagent, preparation of. 597
Benzidine peroxidase reaction (Wilkinson and

Peters). 321
Benzidine reaction for blood, 171, 233, 263, 431
Benzoic acid. 72, 369, 390, 39s, 583. 585
crystalline form of. 396
experiments upon, 396
formula for, 395
solubility of, 396
sublimation of, 396
Bergeim's modification of the Herter-Foster

method for indole in feces. 242
Bergeim's phosphonuclease theory for the origin

of hydrochloric acid of gastric juice, 141
Berthelot-Atwater bomb calorimeter. 586
Bertrand's method for sugar determination, 527
Bial's reaction for pentoses, 37. 443
Bial's reagent, preparation of, 37. 443
Bile, 171. 203, 412. 432
analysis of. 203.
constituents of, 203
daily secretion of. 203
freezing-point of, 203
influence on digestion, gastric. 147
pancreatic, 178, 190

6i6

INDEX

Bile, inorganic constituents of, 203, 209
nucleoprotein of, 203, 207
reaction of, 202 207
secretion of, 202
specific gravity of, 203,
Bile acids, 204

Hay's test for, 209
Mylius's test for, 208
Neukomm's test for, 209
Oliver's test for, 209
Pettenkofer's test for, 208
tests for, 208

V. Udr4nsky's test for, 208
Bile acids in feces, detection of, 236
Bile acids in urine, 412, 434

Hay's test for, 434
Myliys's test for, 434
Neukomm's test for, 43s
Oliver's test for, 43s
Pettenkofer's test for, 434
tests for, 434

V. Udrdnsky's test for, 434
Bile pigments, 203, 204, 207

Gmelin's test for, 207
Hammarsten's reaction for, 207
Huppert's reaction for, 207
Xakayama's reaction for, 207
Rosenbach's test for, 207
Smith's test for, 208
tests for, 207
Bile pigments in urine, 412, 432

Gmelin's test for, 433
Hammarsten's reaction for, .133
Huppert's reaction for, 433
Nakayama's reaction for, 433
Rosenbach's test for, 433
Salkowski-Schipper's reaction for,

433
Salkowski's test for, 433
Smith's test for, 433
tests for, 432
Bile salts, 204, 434

crystallization of, 204, 209
Biliary calculi, 206, 209
analysis of, 209
Bilicyanin, 204
Bilifuscin, 204
Bilihumin, 204
Biliprasin, 204
Bilirubin, 204

crystalline form of, 205
in urinary sediments, 458, 464
BJliverdin, 204, 206
"Biological" blood test, 258
Bismuth, influence on color of feces, 222, 238
Bismuth reduction tests, 29, 420
Bismuth test for choline, 358
Biuret, 99. 373, 375

formation of, from urea, 99, 373
Biuret paper of Kantor and Gies, 100
Biuret potassium cupric hydroxide. See Cupri-
potassium biuret, 99
test, 98

Posner's modification of, 100
Biuret reagent (Gies), preparation of, 100
Black's method for determination of 0-hydroxy-
butyric acid, 541
reaction for ^-hydroxybutyric acid, 441

Black's reagent, preparation of, 441
Blood, 171, 225, 233, 245, 270, 412, 429
acetoacetic acid in, 270 284
acetone in, 247, 270, 284
agglutination of, 250, 262
amino-acid nitrogen in, 270
amino-acids in, 247, 248
ammonia in, 270, 278
Bordet test for, 258
Blood, cholesterol in, 247, 270, 285
coagulation of, 257

Howell's theory of, 257
composition of normal and pathological, 270
constituents of, 247, 248
creatine in, 248, 270, 276
creatinine in, 248, 270, 276
crystallization of oxyhemoglobin of, 250, 266
defibrinated, 257, 260
detection of, 171, 233, 263, 429
determination of acetone in, 284, 294
acetoacetic acid in, 284, 294
amino acid nitrogen in, 277
ammonia in, 278
chlorides in, 286
cholesterol in, 285
creatine in, 276
creatinine in, 276
fat in, 295

/3-hydroxybutyric acid in, 284, 294
hydrogen ion concentration in, 288
non-protein nitrogen in, 271
sugar in, 279
total nitrogen in, 279
total solids in, 288
urea in, 274
uric acid in, 274
erythrocytes of, 249, 261, 472
experiments on, 260, 270
fat in, 247, 295
form elements of, 249
guaiac test for, 23s, 258, 262, 430
hemin test for, 264, 429
fl-hydroxybutyric acid in, 270, 284
in arthritis, 270, 271
in cholelithiasis, 247, 270, 271
in diabetes, 270, 271
in gout, 270, 271
in lipemia, 270, 271
in nephritis, 270, 271
in uremia, 270, 271
in urine, 412. 429
leucocytes of, 255
medico-legal tests for, 257, 203
menstrual, 257
microscopical examination of. 249, 260, 261

269
non-protein nitrogen of, 270

determination of, 271
nucleoprotein of, 246, 247
"occult," in feces, 22s, 233
ortho-tolidin test for, 171, 233, 263, 430
oxyhemoglobin of, 250. 296
pigment of, 250
plaques, 256
plasma, 245, 268
platelets, 256
plates, 256
preparation of hematin from, 266

INDEX

617

Blood preparation of "laky," 24s, 261
reaction of, 24s, 260
serum, 247, 267
specific gravity of, 24s, 260
spectroscopic examination of, 296
sugar in, 247, 270, 271
test for iron in, 261
total amount of, 24s

V. Zeynek and Nencki's hemin test for, 266
Blood analysis, 270
Blood casts in urine, 465, 469
Blood corpuscles, 249, 255, 261, 472

"counting," 304, 308
Blood dust, 245, 256
Blood in urine, 412, 429

benzidine reaction for, 431

guaiac test for, 430

Teichmann's hemin test for, 429

Heller's test for, 429

Heller- Teichmann reaction for, 430

ortho-tolidin test for, 430

Schumm's modification of guaiac test

for, 430
spectroscopic examination of, 431
tests for, 429

V. Zeynek and Nencki's hemin test for,
430
Blood plasma, 245, 268

constituents of, 24s
effect of calcium on oxalated, 268
experiments on, 268
preparation of fibrinogen from, 268
oxalated, 268
salted, 268
Blood serum, 247, 267

coagulation temperature of, 267
constituents of, 247, 267
experiments on, 267
precipitation of proteins of, 267
separation of albumin and globulin of, 268
sodium chloride in, 268
sugar in, 268
Blood stains, examination of, 269
Bloor's nephelometer, cut of, 291
Boas' reagent, as indicator, 155

preparation of, 155 *

Bock and Benedict's apparatus, cut of, 489
Bock and Benedict's microchemical method for

total nitrogen in urine, 488
Boettger's test for sugar, 29, 420
"Bolting" of food, influence of, on food residues

in feces, 590
Bomb calorimeter, Berthelot-Atwatcr, 586
Bonanno's reaction, 208, 434
Bonanno's reagent, preparation of, 208, 434
Bone, constituents of, 336-338
ossein of, preparation of, 336
quantitative composition of, 236, 237
Bone ash, scheme for analysis of, 338
Borchardt's reaction for fructose, 35, 447
Bordet test, detection of human blood by, 258
Boric acid and borates in milk, detection of, 324
Bottu's reagent, preparation of, 23, 415
Bottu's test, 23, 41 s
Bromelin, s

Bromine test for melanin, 452
for tryptophane, 189
Buccal glands, 54

Buffy coat, formation of, 247
Bunge's mass action theory, 140
Burker's hemocytometer, 308
Butter, composition of, 319
Butyric acid, 8, 319. 321, 370, 397
Butyrin, 177. 3i3
Bynin, 93, 11 1

Cadaverin, 81, 212
Calcium in urine, 370, 409

quantitative determination of, 559

balance, preparation of, 592

carbonate in urinary sediments, 458, 459

caseinate, 318

in bone, detection of, 337-8

in feces, estimation of, 592

oxalate, 391, 458

in urinary sediments, 458
paracasein, 143, 315

phosphate in urinary sediments, 458, 460
in bone, detection of, 337-8
in milk, 313, 322
sulphate in urinary sediments, 458, 460
Calculi, biliary, 206, 209
urinary, 475

calcium carbonate in, 476
oxalate in, 476
cholesterol in, 478
cystine in, 476
fibrin in, 478
indigo in, 478
phosphates in, 476
uric acid and urates in, 476
urostealiths in, 479
xanthine in, 476
Calliphora, larvae of, formation of fat .from

protein by, 179
Cambogia, influence of, on color of feces, 238
Calomel, influence on color of stool, 222, 238
Camphor as urine preservative, 368
Cane sugar (see Sucrose, p. 41)
Canton silk. 69
Caproic acid, 313, 319
Carbamic acid, 247
Carbocyclic nucleus, 65. 68-9
Carbohydrosis, 4
Carbohydrates, 19

absorption of, as influenced by fat ingestion,

S68
classification of, 19
composition of, 19
control of putrefaction by, 213
in feces, estimation of, 591
protein-sparing, action of, S79
review of, 51

scheme for detection of. SJ
variation in solubility of, 20
Carbonates in urine, 370, 410
Carbon moiety of protein molecule, 179
Carbon monoxide, hemoglobin, 254, 255, 297
potassium iodide, test for, 298
tannin test for, 298
Carboxylase, 4, 10, 31, 421
Carmine, use in feces separation, 239, 587
Carmine-fibrin, preparation of, 12
Carnine, 341
Carnitine, 341

formula for, 346

6i8

INDEX

Carnomuscarine, 341
Carnosine, 341, 346
Carotin, 319
Cartilage, 335

constituents of, 33s

experiments on, 335
Hopkins-Cole reaction on, 33s
Millon's reaction on, 335

preparation of gelatin from, 335

solubility of, 335

unoxidized sulphur in, 335

xanthoproteic test on, 335 1

Casein, 67, i43, 3i3. 3iS. 318

decomposition of, 67

quantitative determination of, 327-329

soluble, 128, 236

action of rennin upon, 143, 313

biuret test on, 322

Millon's test on, 322

precipitation of, 321

preparation of, 321

quantitative determination of. Hart's method
for, 327

solubility of, 322

test for phosphorus in, 322

test for unoxidized sulphur in, 322
Caseinate, calcium, 318
Caseinogen. See Casein.
Casts, 46s, 467

blood, 46s, 469

epithelial, 465, 469

fatty, 46s. 469

granular, 465, 468

hyaline, .-165, 468

pus. 46s, 472

waxy, 465, 470
Casts in urinary sediments, 465, 467
Catabolism, 564
Cat gut, 146
Catalase, 5, 15

animal, 16

experiments on, 16

quantitative determination of, 16

vegetable. 16
Catalysis, 2
Cell. S65
Cellulose, 20, 48

action of Schweitzer's reagent on, 49

hydrolysis of, 49

iodine test on, 49

solubility of, 49

solvents, 49

utilization by animals, 48
Cellulose group, 20
Cerebrin (cerebroside,) 353. 355. 357

experiments on, 357

hydrolysis of, 357

microscopical examination of, 357

preparation of, 337

solubility of, 357
Cerebro-spinal fluid, choline in, 354
Cerebrosides, 353. 3SS
Charcot-Leyden crystals, 225

form of, 225
Chlorides in blood, 270, 286

in urine, 370, 405, 556
detection of, 406
quantitative determination of, 536

Cholecyanin, 206
Choleprasin, 204

Cholera-red reaction for indole, 218
Cholesterol, 203, 210, 247, 270, 271, 285, 313, 353,
355
crystalline form of, 210
formula for, 355
in blood, 247, 270, 271, 285

determination of, 285
iodine-sulphuric acid test for, 210, 357
isolation of, from biliary calculi, 209
Liebermann-Burchard test for, 210, 357
occurrence of, in urinary sediments, 458, 463
origin of, 356

preparation of, from nervous tissue, 356
Salkowski's test for, 210, 357
Schiff's reaction for, 210, 357
tests for, 210, 357
Choletelin, 204
Choline, 212, 354, 357

as putrefaction product, 212
formula for, 354
tests for, 357
Chondrigen, 113
Chondroalbumoid, 335
Chondromucoid, 113, 335
Chondroitin, 335

Chondroitin-sulphuric acid, 335, 369, 392
Chondrosin, 33s

reducing action of, 335
Chromoproteins (see Hemoglobins), 113
Chyle, 260

Cipollina's test, 23, J14
Clark's modification of Dehn's method for

determination of chlorides, 558
Cleavage products of protein (see Decompo-
sition products), 64, 68-69
Clupeine, 67, 94
Coagulases, 4

Coagulated proteins, 95, 116
biuret test on, 118
digestion of, 118
formation of, 1 16
Hopkins-Cole reaction on, 118
Millon's reaction on, 118
solubility of, 118
xanthoproteic reaction on, 118
Coagulation of blood, 256

Howell's theory of, 257
Coagulation of proteins, 116

changes in composition during, 117
fractional, 105, 117
Coagulation temperature of proteins, 105, 117 «
apparatus used in determining, 106
method employed in determining, 105
Co-enzyme, 7
Cochineal, use of, 158
Collagen, 93. 112, 331. 332
experiments on, 332
percentage of, in ligament. 334

in tendon, 331
production of gelatin from, 333
solubility of, 333
transformation of, 332, 333
Collection and preservation of feces in meta-
bolism experiments, 588
of urine in metabolism experiments, 565
Collodion dialyzer, 24

INDEX

619

Colloidal solution, 313
Colloids, 313, 340

tissue, 340
Colostrum, 315. 316, 319

microscopical appearance of, 315
Combined hydrochloric acid (protein salt), 56
140, 175
preparation of. 599
tests for, 175
Combustion of foodstuffs, 584
Composition of common foods (Table), 569
Compound test for lactose in urine, 44s
Congealing-point of fat, 184
Congo red, as indicator, 153, 154

preparation of, 599
Congo-red fibrin, preparation of, 12
Conjugated proteins, 9J, 112
classes of, 94, 112
nomenclature of, 94, 112
occurrence of, 9J, 112
Conjugate glycuronates, 26, J 17, 442

naphthoresorcinol reaction for, 442
polariscopic-fermentation test for, 442
reduction-polariscopic test for, 443
Connective tissue, 330
Constipation, aid in, 51, 223
Cowie's guaiac test, 235
Cramer's mercuric oxide test for reducing sugar,

28, 419
Creatine, 247, 248. 270, 276, 341. 342, 350, 369.
384, 412
crystalline form of, 342
diacetyl reaction for, 350
formula for, 346

quantitative determination of, 276, 508
separation of, from meat extract, 350
transformation into creatinine, 350
Creatinine, 26, 248. 270, 369, 381
coefficient, definition of, 294
crystalline form of, 382
daily excretion of, 382
elimination, a study of, 574
experiments on, 383
formula for, 381
from creatine, 350
JafTe's reaction for, 385
quantitative determination of. 276, 506
Salkowski's test for. 385
separation of. from urine. 383
Weyl's test for. 385
Creatinine-zinc chloride, formation of, 383, 385
Cresol, para, 212
tests for, 219
Cross and Sevan's reagent, 49
preparation of, 49
solubility test, 49
Cryoscopy, 365
Cul-de-sac, 139
Cupri-potassium biuret, formation of. 99

formula for, 99
Cyanuric acid, 373

formula for, 373
Cylindroids in urinary sediments, 46s. 472
flt-Cyprinine. 67

Cystine, 65. 67-69. 75, 87, 458. 462
crystalline form of, 76
detection of, 462
formula for, 76

Cystine in hair, 87

in urinary sediments, 458. 462
preparation of. in crystalline form. 87

Cytosine, 12s, 126, 128, 133

Wheeler-Johnson reaction for, 133

Dakin's methods for quantitative determination

of hippuric acid, 520
Dare's hemoglobinometer, 302
description of. 302

determination of hemoglobin by. 302
Deaminases. 4

Decomposition products of proteins. 63, 67, 68,
69. 71
crystalline forms of. 72-84
experiments on. 85-87
isolation of, 85-87
Defensive enzymes, 3

Degradation products of protein (see Decomposi-
tion products). 63, 67-69, 71
Dehn-Clark method for chlorides, 558
Delusive feeding experiments, 138
Derived proteins, 94. 114
Detection of preservatives in milk, 323
boric acid and borates, 324
formaldehyde, 323
hydrogen peroxide, 324
salicylic acid and salicvlates, 323
Determination of acetoacetic acid in blood, 284, 294
in urine. 533
acetone in blood. 284, 294

in urine. 538
acetone and diacetic in blood, 284, 294

in urine, 533
acidity of urine, by titration. 479

by hydrogen ion concentration. 470
albumin in urine. 531
allantoin in urine, 518
amino acid nitrogen. 88. 91. 277. 502
in blood. 277

in protein hydrolysis. 64. 88. 91
in urine. 502
of ammonia in urine. 499
amylolytic activity. 192
ash of milk, 327
calcium in urine, 559
casein of milk, 327-329
catalase, 16
chlorides in blood. 286

in urine. 556
cholesterol in blood. 285
creatine in blood. 276

in urine. 508
creatinine in blood. 276

in urine. 506
diacetic acid in blood. 284. 294

in urine, 533
fat in blood. 295
in feces, 243
in milk, 324
fecal amylase. 2i<)
fecal bacteria. 241
glucose in urine. 522
hippuric acid in urine, 519
hydrogen ion concentration vii i.-'.. --^a

of urine, 480
^-hydroxybutyric acid in blood. 284. 294
in urine. SiO- 54*

020

INDEX

Determination, indican in urine, 542

indole in feces, 242

iron in urine, 591

lactalbumin in milk, 329

lactose in milk, 329

magnesium in urine, 559

nitrogen in urine, 483-491

partition in urine, 484, 577

oxalic acid in urine, 545

0-oxybutyric acid in blood, 284, 294
in urine, 539, 541

peptic activity, 165

phenols in urine, 543

phosphorus in urine, 552

potassium in urine, 561

protein in milk, 327, 328

protein in urine, 531

purine bases in urine, 513

purine nitrogen in urine, 516

sodium in urine, 561

sulphur in urine, 546

total solids in milk, 327

total solids in urine, 483

tryptic activity, 169

urea in blood, 274

in urine, 491-499

uric acid in blood, 274

in urine, 510-513
Deuteroprotcose, 95, 119
Dextnn, 20, 43, 47, 56

achroo-, 43, 56

a-achroo-, 56

/3-achroo-, 56

7-achroo-, 56

erythro-, 43. 56

action of tannic acid on 48

diffusibility of, 48

Fehling's test on, 48

hydrolysis of, 48

iodine test on, 47

solubility of, 47
Dextrosazone, crystalline form of, Plate III,

opposite p. 22
Dextrose (see Glucose) .
Diacetic acid (see Acetoacetic acid), 270, 284.

412, 438, 539
Diamine acid nitrogen, 64

Diaminotrihydroxydodecanoic acid, 65, 67-69, 8s
a-<-di-amino-caproic acid, 68, 80
Dialysis, 24

Dialyzers, preparation of, 24
Diastase (see Vegetable amylase), 4, 10
Diazo-benzene-sulphonic acid, 454

reagent, preparation of, 454
Diazo reaction (Ehrlich's), 454
Differentiation between pepsin and pepsinogen,

141. 145
Digestion, gastric, 138
intestinal, 195

pancreatic, 185
salivary, 51
Di-iodo-hydroxypropane (lothion), 30, 421
Di-methyl-amino-azobenzene (see Topfer's re-
agent), 175
2, s-dinitrohydroquinol, use of, 158
Dipeptides, 66, 95
Disaccharides, 19, 38
classification of, 19

Dissociation products of protein (see Decom-
position products, 63).

Donne's pus test, 432

Doremus-Hinds ureometer, 497

Drying method for determination of total solids
in urine, 482

Duodenum, epithelial cells of, 185

Earthy phosphates in urine, 406, 408

quantitative determination of, 553
Edestan, 94, 114

experiments on, 115
Edestin, 67, 93, 109

coagulation of, 109

crystalline forms of, 109

decomposition of, 67

microscopical examination of, 109

Millon's test on, 109

preparation of, 109

solubility of, 109

tests on crystallized, 109
filtrate of, no
Ehrlich's diazo-benzene-sulphonic acid reagent,

preparation of, 454
Ehrlich's diazo reaction, 454
Ehrlich's mechanical eye-piece, use of, 307
Einhorn's bead test, 238
Einhorn's saccharometer, 31
Elastin, 93, 331, 333. 334

adsorption of pepsin by, 334

experiments on, 334

preparation of, 334

solubility of, 334
Electrical conductivity of urine, 366
Electrolytes, influence on enzyme activity, 7, 188
Embryos, glycogen in, 341
Emulsin, 4

Energy metabolism, 564, 584
Enterokinase, 187, 196

demonstration of, 197
Enzymes, i

activation of, 6

adsorption of, 6

classification of, 4

defensive, 3

definition of, 2

experiments on, 10

influence of electrolytes, 7, 188

list of, 4

preparation of, 5, 11, 13, 14

properties of, 6

reference books, 10
Epiguanine, 370, 401
Epinepherine, determination of in adrenal glands,

290
Episarkine, 370, 401
Epithelial cells in urinary sediments, 465

casts in urinary sediments, 465, 469
Epithelial tissue, 330

experiments on, 331
Epstein's sugar method, 282

apparatus for, 283
Erepsin, 5, 195, 198

experiments on, 198
Erythrocytes, 2^9, 261, 472

counting the, 304, 308

diameter of, 249

form of, 249

INDEX

621

Erythrocytes, influence of osmotic pressure on,
261

in urinary sediments, 46s, 472

number of, per cubic millimeter, 249, 250

of different species, 249

stroma of, 249

variation in number of, 250
Erythro-dextrin, 43, 56
Esbach's albuminometer, 532

method for determination of albumin, 532

reagent, preparation of, 532
Ester, definition of, 176 ^

hydrochloric acid, of hematin, 266

sulphuric acid, of hematin, 266
Ethereal sulphates, 369, 385

quantitative determination of, 547, ssr
Ethereal sulphuric acid, 212, 369, 385
Ethyl butyrate test for pancreatic lipase, 193

sulphide, 392
Euglobulin, 246
Excelsin, 109

crystalline form of, no
Extractives of muscular tissue, 340
nitrogenous, 341
non-nitrogenous, 341

Fasting, feces in, 227

metabolism in, 584
Fatigue substances of muscle, 34s
Fats, 176

absorption of, 178, 188

apparatus for determination of melting-
point of, 183

chemical composition of, 176, 177

congealing-point of, 184

crystallization of, 178, l8i

digestion of, 178, 188

emulsification of, 178, 180

experiments on, 180

formation of, from protein, 179-180

formation of acrolein from, 180

hydrogenation of, 177

hydrolysis of, 177

influence of, on carbohydrate absorption, 568

in milk, 313, 319, 323

in urine, 412, 444, 465, 469

melting-point of, 183

nomenclature of, 176, 177

occurrence of, 176

permanent emulsions of, 178, 180

protein-sparing, action of, 579

quantitative determination of, in milk, 324

rancid. 178

reaction of, 178

saponification of, 177, 181, 182

solubility of, 178, i8o-

transitory emulsions of, 178, 180
Fat-splitting enzymes (see Lipases, s, 13, 178,

i88, 193)
Fatty acid, 176, 178, 182, 212, 370, 397
Fatty casts in urinary sediments, 46s, 469
Fatty degeneration, 179

Fecal amylase, quantitative determination of, 239
Fecal bacteria, 221, 224, 225, 241, 588

quantitative determination of, 241
Feces, 221, 587, 592

agar-agar, influence of, 223-224, 589

albumin and globulin in, 237

Feces, bacteria in, 221, 224, 238, 241, 588

bacterial nitrogen in, demonstration of, s88

bile acids in, 236

bilirubin in, 222, 236

blood in, 225, 233

carbohydrate in, estimation of, 591

casein in, 236

cholesterol in, 224, 232

collection and preservation in metabolism
experiments, 588

color of, influence of drugs and foods upon,
238

daily excretion of, 221, 589

enzymes of, 226, 239

experiments on, 229, 587, 592

"fasting," 227

fat in, determination of, 243

food residues in, 227, 590

form and consistency of, 223

hydrobilirubin in, 222, 235, 237

hydrogen ion concentration of, 223

indole in, 223, 237
determination of, 242

influence of defective mastication on, 590

inorganic constituents of, 225, 237, 591
elements of, demonstration of, 591

macroscopic constituents of, 224

metabolic product, nitrogen in, 227 589

microscopic constituents of, 224

microscopical examination of, 229

nitrogen of, 227

nucleoprotein in, 236

odor of, 223

parasites and ova in, 227

pigment of, 222

proteose and peptone in, 237

reaction of, 223

Scybala form of, 223

separation of, importance of, 224, 587

separation of, experiment on, 239, 587
Fehling's method for determination of glucose,
in blood, 279
in urine. 523
Benedict's modifications of, 522

solution, preparation of, 600

test, 26, 416

Allen's modification of. 419
Benedict's modifications of, 27, 417
Ferments, classification of, 4
Fermentation, lactic acid, 170, 314

"sugar-free," 4, 10. 31. 421
Fermentation method for determination of glu-
cose, 530
Fermentation test. 31, 421
Ferric chloride test for thiocyanate in saliva, 59

for melanin in urine. 452
Fibrin, 257, 268, 465, 47-4

carmine, preparation of. 12

congo-red. preparation of. 12

in urinary sediments. 465. 474

separation of, from blood, 247, 257

solubility of, 268
Fibrin ferment, 247, 257
Fibrin-heteroproteose, 68
Fibrinogen, 247, 256. 257, 268
Fibroin, Tussah silk, 68
Fischer apparatus, 75

photograph of, 75

622

INDEX

Fleischl's hemometer, 300
description of, 299

determination of hemoglobin by, 299
Fleischl-Miescher hemometer, 301
Fluorides in urine, 370, 411
Fly-maggots, experiments on, 179
Foam test for bile acids, 208, 434
Folin-Hart method for determination of com-
bined acetone and acetoacetic acid, 533
for determination of acetoacetic acid-
539
Folin-Messinger-Huppert method for determina-
tion of acetoacetic acid, 539
Folin's method for determination of acetone
in urine, 538
acidity of urine, by titration, 479
ammonia, 499
creatinine, in blood, 276

in urine, 506, 508
ethereal sulphates, 547
inorganic sulphates, 547
total sulphates, 546
urea, in urine, 495
of preparing cystine, 87
test for uric acid, 381
Folin and Denis' method for determination of

uric acid in blood, 274
Folin and Denis' method for determination of

uric acid in urine, modification of, 510
Folin and Denis' method for phenols in urine, 543
Folin and Denis' method for urea, 49s
Folin and Denis' nephelometric method for

albumin in urine, 533
Folin and Denis' nephelometric method for ace-
tone bodies in urine, 541
Folin and Flanders' method for hippuric acid in

urine, 519
Folin and Macallum's microchemical method for

ammonia, 501
Folin and Pettibone's microchemical method for

urea in urine, 494
Folin, Benedict and Myers' method for deter-
mination of creatine, 509
Folin-Benedict method for determination of

creatine, 508
Folin-Farmer microchemical method for total

nitrogen in urine, 485
Folin-Farmer microchemical method. Bock and

Benedict's modification of, 488
Folin-Farmer microchemical method, Gulick's

modification of, 490
Folin-Shaffer method for determination of uric

acid, SI I
Foods, composition of, 569
purine content of, 572
Foreign substances in urinary sediment, 465. 4 74
Formaldehyde, as milk preservative, 323

reaction (Konto), 218
Formaldehyde-H2S04 test (Morner), 86
Formation of methyl-phenylfructosazone, 35
Form elements of blood, 245
Formic acid, 26, 370, 397

Formol titration method of Benedict-Murlin, 504
of Malfatti, 502
of Sorensen, 502
Fractional coagulation of proteins, 105, 117

method of gastric analysis, 148, 159
Free hydrochloric acid, 56, 140, 155

Free hydrochloric acid, tests for, 155
Freezing-point of bile, 203
blood, 24s
milk, 314

pancreatic juice, 186
urine, 36s
Frey-Gigon method for amino-acid nitrogen in

urine, 505
Fructose, Borchardt's reaction for, 35
in urine, 446

methyl-phenylhydrazine test for, 35
Seliwanoff's reaction for, 35
Fuchsin-frog experiment, 347
Fuld and Levison's method for peptic activity,

167
Fundus glands, 139
Furfural, formation of, 22

solution, preparation of, 600
Fusion mixture, preparation of, 129

Galactans, 20, so

Galactase, 319

Galactose, 19, 36, 314, 446

experiments on, 36
Gallic acid test for formaldehyde, 323
Ganassini's test, 381

Gastric acidity and the use of indicators, 152
Gastric analysis, 148, 174

detection of bile in, 171
of blood in, 171
of food rests in, 173
of lactic acid in, 170
of mucus in, 173
determination of free acidity in, 164
of peptic activity in, 165
of total acidity in, 162
of tryptic activity in, 169
examination of samples in, 162
. fractional method of, 148, 159
introduction of the tube in, 159
Rehfuss tube, use of in, 148, 159
retention meal in, 161
test meals in, 161
use of indicators in, 152
Gastric digestion, 138

conditions essential for, 14s

general experiments on, 145

influence of bile on, 147

influence of dififerent temperatures on,

influence of water on, 138
most favorable acidity for, 14s
power of different acids in, 146
products of, 141, 144

Gastric fistula, 138

Gastric juice, 139

acidity of, 140, 151

influence of water on, 138

of regurgitation on, 140, 151
analysis of, 148, 174
artificial, preparation of, 144
composition of, 125, 151
enzymes of, 139
lactic acid in, test for, 170
origin of hydrochloric acid of, 140
quantitative analysis of, 148, 174
quantity of, 138
reaction of, 139

INDEX

623

Gastric juice, secretion of, 138, 139

influence of water on, 138
specific gravity of, 139
Gastric lipase, 139, '43
Gastric protease, 12
Gastric rennin, 139, 143. I47. 31S. 32i

action of, upon casein, 143, IJ7, 315, 321
experiments on, 147, 32 i
influence of, upon milk, 147, 321
in gastric juice, absence of, 143
nature of action of, 143, 315
occurrence of, 143
Gastric residuum, 160

composition of. 151
Gelatin, 67. 68, 332, 33i
coagulation of, 333
decomposition of. 67, 68
experiments on, 333
formation of, 333
Hopkins-Cole reaction on, 333
Gelatin, Millon's reaction on, 333
precipitation of, by alcohol, 333
alkaloidal reagents, 333
metallic salts, 333
by mineral acids, 333
preparation of, from cartilage, 335

from collagen, 333
salting-out of, 333
solubility of, 333
Gerhardt's test for acetoacetic acid, 439
Gerhardt's test for urobilin. 400
Gies' biuret reagent, preparation of, 100
Gliadin, 93, 1 11, 112

decomposition of, 67
preparation of, 112
tests on, 1 12
Globin, 67, 93, 113, 250

decomposition of. 67
Globulins, 93. 108

experiments on, 109
preparation of, 109
serum, 93, 246, 412, 422
in urine, 412, 422
tests for, 423
vegetable. 109
Glucoproteins (see Glycoproteins, pp. 94, 112)
Glucose, Allen's modification of Fehling's test for,
419
Barfoed's test on, 30
Benedict's modification of Fehling's test, 27,

417
Boettger's test on, 29, 420
Bottu's test on, 23, 415
Cipollina's test on, 23, 414
Cramer's mercuric oxide test on, 28, 419
diflFusibility of, 24
experiments on, 21, 413
Fehling's test on, 26, 416
fermentation of, 31, 421
formula for, 21
glycosuria produced by, 568
Haines test on, 419
hyperglycemia produced by, 566
iodine test on, 24
Molisch's reaction on, 21
Moore's test on, 24
Nylander's test on, 29, 420
phenylhydrazine test on, 22, 413

Glucose, quantitative determination of, 522

reduction tests on, 25. 415

Riegler's reaction, 23, 414

solubility of, 21

Trommer's test on, 25, 416
Glucosidases, 4
o-Glucosides, 4
/3-Glucosides, 4

Glucosazone, crystalline form of, Plate III, oppo-
site p. 22
Glucothionic acid, 467
Glutamic acid, 69, 82, 186

formula for, 82
Glutelins, 93, no

tests on. III
Gluten, preparation of, in

tests on. III
Glutenin, 93, no, iii

preparation of, in

tests on, in
Glycerol, 176, 177, 178, 182

borax fusion test on, 183

experiments on, 182

formula for, 177

hypochlorite-orcinol reaction for, 183
Glycerol extract of pig's stomach, preparation of,

144
Glycerophosphoric acid, 353, 354, 370, 399
Glycocholic acid, 204
Glycocholic acid group, 204
GlycocoU, 6s, 69, 71, 204

crystalline form of, 211

formula for, 71, 204

preparation of. 211
GlycocoU ester hydrochloride, crystalline form

of, 72
Glycogen, 20, 47. 341. 348

experiments on, 349

hydrolysis of, 349

in embryos, 341

influence of saliva on, 349

iodine test on. 349

preparation of. 3J8
Glycogenase, 4
Glycolytic enzymes. 3. 4
Glycoproteins, 94, 112-113, 332

experiments on, 332

hydrolysis of, 332
Glycosuria, alimentary, 21, 568

by glucose ingestion, 21, 568
Glycosuric acid, 395
Glycuronates, conjugate, 26, 417. 442

tests for, 442
Glycuronic acid, 36, 38, 442
Glycyl-glycine. formation of. 70
Glycyl-tryptophanc test, 195, 199
Glyoxylic acid, 98

formula for, 98
reaction (Hopkins-Cole), 98
Gmelin's test for bile pigments. 207, 433

Roscnbach's modification of, 207, 433
Gout, blood in, 248, 270, 271, 379
Granular casts in urinary sediment, 465, 467
Granulose, 43

Green stools, cause of, 222, 238
Gross' method for quantitative determination of

tryptic activity, 191
Guaiac solution, preparation of, 600

624

INDEX

Guaiac test on blood, 23s, 258, 262, 430

on feces, 235

on milk, 320

on pus, 432

on urine, 430
Guaiac test, Schumm's modification of, 262
Guanase, A

Guanidine-a-amino-valerianic acid, 68, 79
Guanidine-residue, 64
Guanine, 4, 125-127, I33. 34i
Guanine chloride, crystalline form of, 135
Gulick's colorimetric method for total nitrogen in

urine, 490
Gulick's micro-oxidation flask, 490
Gum arable, 20, 50, 51

Gums and vegetable mucilage group of carbo-
hydrates, 20
Gunning's iodoform test for acetone, 436
Gunzberg's reagent, as indicator, 155

preparation of, ISS

Haine's test on sugar, 419

Hair, human, 330

Hammerschlag's method for determination of

specific gravity of blood, 260
Hammarsten's reaction, 207, 433

reagent, preparation of, 207, 433
Harding and MacLean's method for determina-
tion of amino-acid nitrogen, 91
Hart's casein method, 328
Haser's coefficient, 364, 483
Hayem's solution, 601
Hay's test for bile acids, 209, 434
Heintz method for determination of uric acid, 512
Helicoprotein, 94

Heller's test for blood in urine, 429
Heller's ring test for pi-otein, 103
Heller- Teichmann reaction for blood in urine, 430
Hemagglutination, 250, 262
Hemagglutinin, 250, 262
Hematein test for blood in feces, 234
Hematin, 113, 250, 254, 266

acid-, 254, 299

alkali-, 254, 298

preparation of, 266

reduced alkali-, 299
Hematoidin, 205, 222, 224

crystalline form of, 205, 222

in urinary sediments, 458, 464
Hematoporphyrin, 205, 254, 359, 412, 444

in urine, 359, 412, 444
Hematuria, 429
Hemicellulose, 20, 50

experiments on, 51

utilization of, by animals, 50
Hemin crystals, form of, 265

tests, 264, 266, 429
Hemiurate, 461

Hemochromogen, 113, 250, 254, 269, 299
Hemocyanin, 94, 113
Hemocytometer, Btirker's, 308

Thoma-Zeiss, 304
Hemoconein (see Blood dust, 24s, 256)
Hemoglobin, 94, 113, 249, 250, 254, 25S,'262,|266,
296

carbon monoxide, 254, 297

decomposition of, 250

derivatives of, relationship of, 254

Hemoglobin, diffusion of, 262

met, 254, 298

oxy, 250, 254, 266, 296

quantitative determination of, 299-304

reduced, 254, 296
Hemoglobins, 94, 113
Hemoglobinuria, 429
Hemolysis, 245, 261

Henderson and Palmer's method for determina-
tion of hydrogen ion concentration, 480
Herter's naphthaquinone reaction for indole,

218
Herter's para-dimethylaminobenzaldehyde reac-
tion, 219
Heterocyclic nucleus, 65, 68, 69
Heteroprotebse, 96 119
Heteroxanthine, 370, 401
Hexone bases, 80
Hexosans, 20
Hexoses, 19, 20
Hippuric acid, 72, 369, 388, 390, 396, 585

cystalline form of, 389

Dakin's method for quantitative determi-
nation of, 520

experiments on, 389, 585

formula for, 388

in urinary sediments, 463

Liicke's reaction for, 390

melting-point of, 389

Roaf 's method for crystallization of, 390

separation of, from urine, 389

solubility of 390

sublimation of, 390

synthesis of, 390, 585

demonstration of, 585
Histidine, 65, 77

hydrochloride, crystalline form of, 78

Knoop's color reaction for, 78
Histones, 93

Hoffmann's reaction for tyrosine, 86
Homogentisic acid, 26, 369, 394, 417

formula for, 394
Hopkin's thiophene reaction for lactic acid, 171
Hopkins-Cole reaction, 98

on solutions, 98
on solids, 107
Hopkins-Cole reagent, preparation of, 98
Hopkins-Cole reagent (Benedict modification),

preparation of, 98
Hordein, 93, in

Horismascope (see Albumoscope, 103, 423)
Hormones definition and discussion of, 185, 318

in blood, 185
Hiifner's urea apparatus, 498
Human fat, composition of, 178

hair, composition of, 330

milk, differentiation from cow's, 316, 320
Hunter and Givens' modification of Kruger and

Schmidt's method, 515
Huppert's reaction for bile pigments, 207, 433
Hurthle's experiment, 349
Hurtley's test for acetoacetic acid, 440
Hyaline casts in urinary sediments, 465, 468
Hydrobilirubin, detection of, in feces, 222, 23s

extraction of, 235
Hydrochloric acid of the gastric juice, 140, ISI
origin of, theories as to, 140
seat of formation of, 139

INDEX

62:

Hydrochloric acid test for formaldehyde (Leach),
323
acid-zinc chloride solubility test, 49
Hydrogen ion concentration and titratable
acidity, iS5, 479-480
mode of expressing, 152
of blood, determination of, 288
of urine, determination of, 480
as influenced by diet, 580
by acids, 582, 583
by alkali, 582, 583
comparison of, with titratable

acidity, ISS. is8
determination of, by means of
indicators, 158, 480

of McClendon's electrode,
149
Hydrogen peroxide in urine, 369, 411

detection of, in milk, 324
Hydrogenated fat, 177
Hydrogenation, definition of, 177
Hydrolysis of cellulose, 48, 49
cerebrin, 357
dextrin, 47, 48
glycogen, 349
inulin, 46
proteins, 64
starch, 43, 45
sucrose, 41, 42
/9-Hydroxybutyric acid, 270, 271, 284, 295, 412,
440, S41
Black's method for determination of,

S4I
Black's reaction for, 441
formula for, 440
in blood, 270, 284, 295
origin of, 441

polariscopic examination for, 442
quantitative determination of, in blood,
284, 295
in urine, 539. 54 1
Shaffer and Marriott's method for
determination of, 539
Hyperacidity, 140, 164

curve, 164
Hypercholesterolemia, 247, 270, 271
Hyperglycemia, 270, 566

produced by carbohydrate ingestion, 566
Hypoacidity, 140
Hypobromite methods for determination of urea

in urine, 496
Hypobromite solution, preparation of, 601
Hypochlorite-orcinol reaction for glycerol, 183
Hypoxanthine, 127, 341, 346, 350, 370, 401
chloride, crystalline form of, 136
formula for, 127, 346
oxidase, 127
Hypoxanthine silver nitrate, crystalline form of,
351

Ichthulin, 94
Ignotine, 341, 346

formula for, 346
Imide bonds, 70
Iminazolethylamine, 214
Iminazolpropionic acid, 214
Indican, 212, 386, 542

formula for, 212, 387
40

Indican, Jaffe's test for, 387

Jolles' reaction for, 388

Obermayer's test for, 388

origin of, 212, 386
Indicator method for determination of hydrogen
ion concentration, 158, 480

solutions, preparation of, 158
use of, 158
Indicators, experiments on, 152

table of, 153, 158

tabulation of results of tests on, 154

use of, 152

in gastric analysis, 152
Indigo-blue, 213, 388

formula for, 213, 388
Indigo in urinary sediments, 458, 464
Indolacetic acid, 214, 4i2
Indole, 212, 218, 223, 237

formula for, 212

origin of, 212

in feces, quantitative determination of, by
Bergeim's method, 242

test for, 218, 237
/S-Indole-a-amino-propionic acid, 68, 77
Indolpropionic acid, 214
Indoxyl, 212

formula for, 212, 388

origin of, 212

potassium sulphate (see Indican, p. 212,
387. 542
Indoxyl-sulphuric acid, 212, 369, 385

formula for, 212, 386
Influence of purine-free and high purine diets, 571
Infraproteins (see Metaproteins, 94, 115, 116)
Inorganic elements in feces, absorption of, 591

physiological constituents of urine, 370, 402
Inosinic acid, 341, 346

formula for, 346
Inositol, 19, 412, 450

formula for, 450

in urine, 412, 450
Intestinal digestion, 19s

jviice, 195

enzymes of, 195, 196, 198-201
preparation of, 199-201
Inulase, 4, 46
Inulin, 20, 46

action of amylolytic enzymes on, 46

Fehling's test on, 46

hydrolysis of, 46

iodine test on, 46

reducing power of, 46

solubility of, 46

sources of, 46
Inversion, 41, 43

Invertase (see Sucrase, 4. 41. ipSt 199)
Invertases. experiments on, 199
Invertin (see Sucrase, 4, 41, 19s, 199)
Inverting enzymes, 3
Invert sugar, 41
Iodide of dextrin, 45

of starch, 47
Iodine absorption test, 183

test for starch and dextrin, 45. 46, 47. 49.
SJ. 56

for urobilin, 400
Iodine-sulphuric acid test for cholesterol, a 10, 357
lodine-zinc-chloride reaction, 49

626

INDEX

Iodoform test for alcohol, 42

for acetone (Lieben), 437
lodothymol compound, 437
"lothion," 30, 421

Iron, reduced, influence on color of feces, 238
in blood, 261

detection of, 261
in bone ash, 338

detection of, 338
in protein, 63
in urine, 410, 562, 591
detection of, 410
determination of, 591
Isoleucine, 6s, 80
Isomaltose, 19, 40
Isopropylmetacresol (see Thymol)
Isovalerianic acid, 214

Jacoby-Solms method, 167

Jaffe's reaction for creatinine, 382

Jafle's test for indican, 387

V. Jaksch-Pollak reaction for melanin, 452

Jejunum, epithelial cells of, 185

Jolles' reaction for indican, 388

Juice, gastric, 138, 150

pancreatic, 185

intestinal, 19s

Kantor and Gies's biuret paper, 100
Kastle's peroxidase reaction, 320
Kephalin. 353, 355
Kephyr, 40
Keratin, 93, 112, 330
experiments on, 331
solubility of, 330
sources of, 330
sulphur content of, 330
Ketone, 25
Ketose, 19

Kidney efficiency test, 455
Kjeldahl method for determination of nitrogen,

483
Kjeldahl-Folin-Farmer nitrogen method, 485
Knoop's color reaction for histidine, 78
Konto's reaction for indole, 218
Koumyss, 40

Kraut's reagent, preparation of, 602
Kreosotal, 443

Kruger and Schmidt's method for the quantita-
tive determination of pu-
rine bases, 513
of uric acid, 513
Kwilecki's modification of Esbach's method, S32
Kynurenic acid, 369, 395
formula for, 39s
isolation of, from urine, 395
quantitative determination of, 395

Laccase, 5

Lactalbumin, 93, 313, 318

quantitative determination of, 329
Lactase, 4, 196, 200

experiments on, 200
Lactic acid, 40, 170, 342

ether-ferric chloride test (Strauss) for, 170

fermentation, 40, 314

ferric chloride test (Kelling) for, 170

Hopkins' thiophene reaction for, 171

Lactic acid in muscular tissue, 342
in stomach contents, 170
tests for, 170.
Uffelmann's test for, 170
Lactochrome, 319, 399
Lacto-globulin, 313, 318
Lactometer, determination of specific gravity of

milk by, 324
Lactosazone, crystalline form of, Plate III, oppo-
site p. 22
Lactoscope, Feser's, 326
Lactose, 19, 40, 318

experiments on, 40
fermentation of, 40, 318
in urine, 412, 444
quantitative determination of, 329
Laiose in urine, 451
"Laked" blood, 24s, 261
Laky blood, 261
Lanolin, 178, 188
Laurie acid, 313
Leach's hydrochloric acid test for formaldehyde,

323
Lecithin, 94, 247, 353

acrolein test on, 356
decomposition of, 354

experiments on, 356 ^

formula for, 35/)

microscopical examination of, 356
osmic acid test on, 356
preparation of, 356
test for phosphorus in, 356
Lecithoproteins, 94, 114
Legal's reaction for indole, 218

test for acetone, 437
Le Nobel reaction for diacetic acid. 439
Lenzmann-Kober nephelometer, cut of, 293
Leucine, 67, 69, 79, 85, 87

crystalline form of impure, 463

pure, 80
experiments on, 87
formula for, 79
in urinary sediments, 463
microscopical examination of, 87
separation of, from tyrosine, 86
solubility of, 87
sublimation of, 87
Leucocytes, 245, 255
counting the, 306

number of, per cubic millimeter, 255
size of, 25s

variation in number of, 255 *

Leucocytosis, 255
Leucosin, 103

Leucyl-alanyl-glycine, formation of, 70
Leucyl-glycyl-alanine, 57
Leucyl-leucine, formation of, 70
Levo-a-proline, 83

Levulosazone, crystalline form of, Plate III, op-
posite p. 22
Levulose, (see Fructose), 19, 34
Lichenin, 20, 47
Lieben 's test for acetone, 437
Lieberkuhn's jelly (see Alkali metaprotein, p. 116)
Liebermann-Burchard test for cholesterol, 2 10, 357
Liebermann's reaction, 100
Linoleic acid, 177
Lipase, gastric, 139, 143

INDEX

627

Lipase, pancreatic, 5, 13, 178, 188, 193
experiments on, 13, 193
ethyl-butyrate test for, 193
litmus-milk test for, 193
Lipases, s, I3. 178, 188, 193

autolytic, s

experiments on, 13, 193

pancreatic, 13

vegetable, 13
Lipemia, blood in, 270, 271
Lipeses, 9
Lipins, 353

Lipoids of nervous tissue, 353. 356
Lipolytic enzymes (see Lipases, p. 5, 13, 178. 188,

193)
"Litmus-milk" test for pancreatic lipase, 193
Long's coefficient, 364, 483
Lucke's reaction for hippuric acid, 390
Lugol's solution preparation of, 602
Lymph, 245, 259
Lysine. 68, 80, 142, 186
Lysine picrate, crystalline form of, 81

McClendon's electrode, determination of H ion

cone, by, 149
Magnesia mixture, preparation of, 602
Magnesium balance, preparation of,592

in bone, detection of, 337, 338
in urine, 370, 409

quantitative determination of,
559
phosphate in urinary sediments, 458,
464
Malfatti's formol titration method for ammonia in

urine, 502
Maltase, 4, 57, 196, 201
experiments on, 201
Maltosazone, crystalline form of, Plate III, op-
posite p. 22
Maltose, 19, 39

experiments on, 39
structure of, 39
Marsh apparatus, 449
cut of, 449
method for arsenic, 448
Marshall's hypobromite urea apparatus, 498
Marshall's clinical urease method for estimation

of urea in urine, 493
Mastication, defective, influence of, on food

residues in feces, 227, 590
Mauvein, use of, as indicator, 158
McCrudden's method for determination of cal-
cium, 559
of magnesium, 559
McLean and Van Slyke's method for determina-
tion of chlorides in blood, 286
Melanin in urine, 412. 451
tests for, 452

urinary sediments. 458, 465
Melting-point apparatus, 183

of fats, determination of, 183
Mercuric oxide test for reducing sugar, 28, 419
Mercury in urine, 450

detection of, 450
Metabolism, 564

experiments, 565

balance of income and outgo in, prepa-
ration of, 592

Metabolism experiments, collection and preserva-
tion of feces in, 588
urine in, 565
separation of feces in, 587
in acidosis, 576
in fasting, 584
in gout, 571, 574
influence of acids on, 582
of alkalies on, 582
of defective mastication on, 590
of digestion on, 577
of fats and carbohydrates as protein

sparers in, 579
of high calorie, non-nitrogenous diet on,

584
indigestible, non-nitrogenous material

on, 589
of water on, 574
of acid-forming and base-forming foods, 580
of ammonium benzoate, 585
of carbohydrates, 566-568, 591, 593
of energy, 579. 584
of fat, 591

of inorganic elements, 591, 593
of nitrogen and sulphur as influenced by

diet, 577
of proteins, 569, 590

time relations of, 569
of purines, 571-574
on "salt-free" diet, 576
on salt-rich diet, 576
relation of bacterial nitrogen of feces to, 588

of metabolic nitrogen of feces to, 589
study of creatinine elimination in, 574
Menstrual blood, 257
Messinger-Huppert method for determination of

combined acetone and diacetic acid, 535
Metaproteins, 94. 115 ■•

acid, 94, 115, 116
alkali, 94. ii5. 116
experiments on, 116
precipitation of, 116
sulphur content of, 116
Methemoglobin, 254, 298
Methylene blue, 146

reaction (Russo), 455
Methyl-mercaptan, 212
Methyl orange, use of, as indicator, 158
red, use of, as indicator, 158
violet, use of, as indicator, 158
Methyl-pentose (see Rhamnose, p. 19)
Methylphenylhydrazine, 35
Methylphenylfructosazone, formation of, 35
i-methylxanthin, 370, 401
Mett's method for determination of peptic

activity, 165
Mett's tubes, preparation of, 166
Micro-organisms in urinary sediments, 465, 474
in feces, 221, 225
in intestine, 212, 225
xMilk, 313

ash of human and cow's, 316, 317
casein of, 313. 3IS. 3i8
citrates in, 313

composition of human and cow's, 316, 317
detection of calcium phosphate in, 322
lactose in, 322
preservatives in, 323

628

INDEX

Milk, difference between human and cow's, 316,
317. 320
experiments on, 319
formation of film on, 314, 319
freezing-point of, 314
guaiac test on, 320

human and cows, differentiation, 316, 320
influence of rennin on, 147, 321
isolation of fat from, 323, 324
Kastle's peroxidase reaction on, 320
lactose in, 313, 318, 322

crystalline form of, 318
fermentation of, 314
microscopical appearance of, 315, 319
preparation of casein from, 321
properties of casein of, 318, 322
quantitative analysis of, 324
reaction of, 314, 319
separation of coagulable proteins of, 323
serum, 313

specific gravity of, 314, 319
unknown constituents of, 313
Millon's reaction, 97

reagent, preparation of, 97
Mohr's method for determination of chlorides, 558
Molisch's reaction, 21
Molybdate solution, preparation of, 603
Monamino acid nitrogen, 64
Monosaccharides, 19, 20
Barfoed's test for, 30
classification of, 19
Morner-Sjoqvist-Folin method for determination

of urea, 495
Morner's reagent, preparation of, 86

test for tyrosine, 86
Motor and functional activities of the stomach,

146 .
Mucic acid, 36, 40, 44s, 4J6

test, 36, 40, 445, 446
Mucin, 55, s8, 94, 113
biuret test on, 59
hydrolysis of, 59
isolation of, from saliva, 59
Mfllon's reaction on, 59
Mucins, 55, s8, 94, 113
Mucoid, 94, 113, 331, 332
experiments on, 332
hydrolysis of, 332
in urine, 397, 428
preparation of, from tendon, 332
Mucoids, 94. 113. 331. 332
Murexide test, 380
Muscle plasma, 339, 347

formation of myosin clot in, 339, 347
fractional coagulation of, 339, 347
preparation of, 347
reaction of, 342, 347
Muscular tissue, 339

ash of, smooth and striated, 345
commercial extracts of, 345
experiments on "dead," 348

"living," 347
extractives of, 341, 34s
fatigue substances of, 34s
formulas of nitrogenous extractives of,

346
glycogen in, 341, 348
involuntary, 339

Muscular tissue, lactic acid in, 340, 342, 348
magnesium in, demonstration, 349
nonstriated, 339

phosphate in, demonstration of, 349
pigment of, 345

preparation of glycogen from, 348
muscle plasma from, 347
Muscular tissue, proteins of, 339, 348
reaction of living, 342, 348
rigor mortis of, 339. 340
separation of extractives from, 350
striated, 339
voluntary, 339
Myohematin, 345
Myosan, 94, 348

formation of, 348
Myosin, 339, 348

biuret test on, 348
coagulation of, 348
preparation of, 348
solubility of, 348
Myosinogen, 339, 347
Myristic acid, 313
Myristin, 177
Myrtle wax (see Bay berry tallow, 182)

Nakayama's reaction for bile pigments, 207, 433

reagent, preparation of, 207, 433
a-Naphthol reaction, 21
Naphthoresorcinol reaction for glycuronates

(Tollens), 442
Nencki and Sieber's reaction for urorosein, 453
Neosine, 341

formula for, 346
Nephelometer, Bloors, cut of, 291
description of, 290
Lenzmann-Kober, cut of, 293
Nephelometric methods, 290, 326, 327, 533, 541
Nephelometric, determination of, acetone bodies
in blood, 294
acetone and diacetic acid in urine, 541
fat in blood, 295
in milk, 326
0-hydroxybutyric acid in urine, 541
proteins in milk, 327
in urine, 533
Nephritis, blood in, 248, 270, 271
Nephrorosein in urine, 453
Nervous tissue, 353

constituents of, 353 ,

experiments on lipoids of, 356
lipoids of, 353. 356
percentage of water in, 353
phosphorized fats of, 353
proteins of, 353
Nessler- Winkler solution, 603
Neurine, 212

Neumann's method for total phosphorus, 554
Neurokeratin, 353
Neutral fats, 177, 178, 180
Neutral olive oil, preparation of, 180
Neutral red, use of, 158
Neutral sulphur compounds, 369, 392
Nippe's hemin test, 264
Nitrates in urine, 370, 411
Nitric acid test (Heller), 103
for phenol, 220
Nitric acid-MgS04 test (Roberts), 104

INDEX

629

Nitrilase, 8

Nitrilese, 8

Nitrites in saliva, test for, 59

Nitrogen, 63, 64

forms of in protein molecule, 64
importance of, in sustaining life, 64
in urine, quantitative determination of, 483
Nitrogen distribution, calculation of, 484
Nitrogen iodide, formation of, 436
Nitrogen "lag," 569

"partition," 48s. 577
Nitrogenous extractives of muscular tissue, 341,
3S0
formulas for, 346
^-Nitrophenol, use of, as indicator, 158
Nitroprusside reaction for indole (Legal), 218
Nitroprusside test for creatinine (Weyl), 385
Nitroprusside-acetic acid test for creatinine

(Salkowski), 385
Kitroso-indole nitrate test, 219
Nitrosothymol, formation of in Heller's test, 423
Non-nitrogenous extractives of muscular tissue,

341
Non-protein nitrogen of blood, 248, 270, 271
Normal urine, 359, 369, 37 1

characteristics of, 359
constituents of, 369, 371
experiments on, 373-410
Novaine, 341

formula for, 346
Nubecula, 396, 428
Nucleases, 5

experiments on, 134
Nucleic acid, 124-128, 131-137
decomposition of, 124-126
experiments on, 131— 137
from yeast, formula for, 125
Nucleicacidase, s» 126
Nucleins, 123, 124, 144, 571
Nucleoproteins, 94, 112, 123, 128-131, 396, 428
decomposition of, 123-124
experiments on, 128-131
from yeast, 128

preparation of, 128

protein, carbohydrate and phosphoric

radicals in, 130
tests on, 129

thymus, preparation of, 130
experiments on, 130
in bile, 203, 207
in feces, 236
in nervous tissue, 353
in urine. 369, 396, 412, 428

test for, 428
occurrence of, 123
Ott's precipitation test for, 428
Nucleosidase, s, 126 '
Nucleoside, 125
Nucleotidase, s, 126
Nucleotide, 125
Nylander reaction, 29. 420
Nylander reagent, preparation of, 29, 420

Obermayer's test for indican, 388
reagent, preparation of, 388
Oblitine, 341

"Occult" blood in feces, 225, 233
tests for, 233

Olein, 177. 313
Olive oil, 180

emulsification of, 180
neutral, preparation of. 180
Oliver's peptone test for bile acids, 209, 433
Optical methods, 31-34
Orcinol-HCl reaction (Bial). 37, 443
Orcinol test, 38, 444

Organic physiological constituents of urine, 369
Organized ferments, i
Organized urinary sediments, 457, 465
Ornithine, 63, 214

Ortho-tolidin test for blood, 171, 233, 263, 430
Osbome-Folin method for determination of total

sulphur in urine, 349
Ossein, 336

preparation for, 336
Osseoalbumoid, 336
Osseomucoid, 94, 113, 336

chemical composition of. 113
Osseous tissue. 336

experiment on, 337
Ott's precipitation test for detection of nucleo-

protein in urine. 428
Ovalbumin, 93
Ovoglobulin, 93

Oxalated plasma, preparation of, 268
Oxalic acid, 369. 39i. 343

formula for, 391

in urine, 369. 391

quantitative determination of, 543
Oxaluria, 391
Oxaluric acid. 369, 397
Oxamide. 99
Oxidases, 3, 14, 319

experiments on, 14
Oxy acids. 212. 217. 220. 369, 394

tests for. 220
^-Oxybutyric acid (see /3-hydroxybutyric acid,

270. 271. 284, 293, 412, 440, 341)
Oxyhemoglobin, 64, 250, 234. 233

Reichert's method for crystallization of, 266

crystalline forms of, 231-234
Oxymandelic acid. 369. 395
Oxyproline, 63, 67. 83
Oxyproteic acid, 369. 392. 434

Palmitic acid, 176, 177. 181. 182
crystalline form of. 182
experiments on. 182
formula for. 177
preparation of. 182
Palmitin. 176, 319
Pancreatic amylase, 4. 11, 187, 192

digestion of dry starch by. 18S. 192

inulin by. 192
experiments on. ii. 191
influence of bile upon action of, 192
most favorable temperature for action
of. 193
Pancreatic digestion, 183

general experiments on. 190
products of. 186. 189
Pancreatic insufficiency, Schmidt's nuclei test for.

237
Pancreatic juice. 123, 185, 186, 187

artificial, preparation of. 189
daily excretion of, 186

630

INDEX ,

Pancreatic juice, enzymes of, 186
freezing-point of, 186
mechanism of, secretion of, 185
reaction of, 186
solid content of, 186
specific gravity of, 186
Pancreatic lipase, 5, 13, 178, 188
experiments on, 13, 193
ethyl-butyrate test for, 193
litmus-milk test for, 193
Pancreatic protease (see Trypsin, pp. 5, 12, 186)
Pancreatic rennin, 5, 189, 194
experiments on, 194
Papaih, 5, 13
Papayotin (see Papain)
Paracasein, 315

Para-cresol-sulphuric acid, 369, 385
Paradimethylamino benzaldehyde solution, prep-
aration of, 604
Paralactic acid, 247, 314, 342, 370, 398
Paramyosinogen, 339
Paranucleoprotagon, 353, 356
Paraoxyphenylacetic acid, 212, 214, 369, 394
Paraoxy-/3-phenyl-a-amino-propionic acid, 69, 74,

86
Paraoxyphenylpropionic acid, 212, 214, 369, 394
Paraphenylenediamine hydrochloride, 324
Parasites, 227, 465, 474
Paraxanthine, 370, 401
Parietal cells, 139
Parotid glands, characteristics of saliva secreted

by, 54
Pathological constituents of urine, 412
Pathological urine, 359, 412
constituents of, 412
experiments on, 413
"Partition" of nitrogen and sulphur in urine, 577
Pektoscope, 365
Pentamethylenediamine, 214
Pentapeptides, 66, 95
Pentoses, 19, 37

experiments on, 37
in urine, 412, 443
tests for, 443
Pentosans, 20, 36, 50

Pepsin (see Gastric Protease), S, 12, 141, 165
action of, influence of bile upon, 147

influence of diflferent acids upon, 146
influence of metallic salts upon, 146
temperature upon, 145
conditions essential for action of, 14s
differentiation of, from pepsinogen, 141, 145
digestive properties of, 141
formation of, 141

most favorable acidity for action of, i43
presence of, in intestine, 142
proteolytic action of, 141
Pepsin-hydrochloric acid, 145
Pepsin-rennin controversy, 143
Pepsinogen, 6, 141, 144

differentiation of, from pepsin, 141, 145
formation of, 141
extract of, preparation of, 144
Peptases, 5

Peptic activity, Fuld and Levison's method for,
determination of, 167
Mett's method for the determination of,
165

Peptic activity, Rose's method for determination

of, 167
Peptic proteolysis, 141

products of, 141

relation of, to tryptic proteolysis, 142
Peptides, 66, 71, 95, 120
Peptone, 6s, 7i. 95. "8
ampho, 95, 119
anti, 119

differentiation of, from proteoses, 119
experiments on, 119, 120
in urine, 412, 426
tests for, 427
separation of, from proteoses, 120
Peptone test for bile acids (Oliver), 209, 435
Periodide test for choline, 357
Peroxidases, 5, 14, is, 321
Peters' method for sugar determination, 525
Pettenkofer's test for bile acids, 208, 434

Mylius's modification of, 208,

434
Neukomm's modification of,
209, 435
Phenaceturic acid, 370, 398
Phenol, 213, 387

excretion of, 387, 545

quantitative determination of, in urine, 543
tests for, 219
Phenolphthalein as indicator, 153, 157, 158, 162,
479
preparation of, 158,. 605
test for blood in feces, 234
Phenolsulphonephthalein test for kidney effi-
ciency, 455
Phenol-sulphuric acid, 369, 385
Phenylacetic acid, 214
Phenyl-a-amino propionic acid, 69, 73
Phenylalanine, 65, 67, 69, 73
Phenylethylamine, 214
Phenylglucosazone, 22 and plate opposite
Phenylhydrazine, 22

acetate solution, preparation of, 23
mixture, preparation of, 22
reaction, 22, 23, 413

Cipollina's modification of, 23, 414
Phenyllactosazone, crystalline form of, Plate III,

opposite p. 22
Phenylmaltosazone, crystalline form of Plate III,

opposite p. 22
Phenylpotassium sulphate, 386
Phenylpropionic acid, 214
Phloroglucinol-HCl reaction, 36. 38, 443. 446
Phosphate solutions and hydrogen ion concen-
tration, 154, 156, 157. 159. 361, 481
Phosphates in urine, 361, 406, 553
detection of, 408
experiments on, 408
quantitative determination of, 552
Phosphatase, 9
Phosphatese, 9
Phosphatides, 203, 296, 353
Phosphocarnic acid, 341, 346, 370, 399
Phosphonuclease, 136
Phosphoproteins, 94, 95, 113, 318
Phosphorized compounds in urine, 370, 399
Phosphorus in urine, determination of, 552

organic, test for, 129
Phosphotungstic acid reaction (Folin), 381

INDEX

631

Phosphotungstic precipitation test for proteose

(v. Aldor), 427
Physiological constituents of urine. 369
Phytase, s
Phytin, s

Picric acid reaction for creatinine Qaffe), 385
Pigments of urine, 359. 370, 399i 4Si
Pine wood test for indole, 219
Piria's test for tyrosine, 86
Plasma of blood, 245, 268

of muscle, 339, 347
Plasmaphaeresis, 249
Polariscope, use of, 31

in detection of conjugate glycuronates,

443
in determination of dextrose, 31, 531
0-hydroxybutyric acid, 442, S4i
Polypeptides, 66, 71, 95
Polysaccharides, 20, 43
classification of, 20
properties of, 43
Posner's modification of biuret test, 100
Potassium in urine, 370, 409

quantitative determination of, 562
Potassium hydroxide test for blood in urine
(Heller), 429
indoxyl-sulphate (see Indican, pp. 212, 387,
S42)
formula for, 212, 387
origin of, 212, 386
tests for, 387
Primary protein derivatives, 94, 114
Primary proteoses, 119
Products of protein hydrolysis, 66, 67, 71
Prolamins, 93, ill

classification of, 93
preparation of, 112
tests on, 112
Proline, 65, 67, 68, 83, ill, 142, 186

crystalline form of copper salt of, 84
crystalline form of laevo-a-, 84
Prosecretin, 185
Protagon, 353, 354

preparation of, 356
structure of, 355
Protamines, classification of, 93, 93
Proteans, 94, 114
Protease, gastric, 5, 12, 141

experiments on, 12, 144
pancreatic, 5, 12, 186

experiments on, 12, 189
vegetable, 5, 13
Proteases, 5, 12

experiments on, 12
Protective enzymes (see defensive enzymes), 3
Protein content of foods, 569

derivatives, primary, 65, 94, 114

secondary, 65, 94, 118
metabolism, time relations of, 569

influence of water on, 575
utilization, determination of, 590
Protein-coagulating enzymes, s. i43. 189, 256. 315
Protein-cystine, 77
Protein-sparing action of fat and carbohydrate,

579
Proteins, 63, 93, 412, 422

acetic acid and potassium ferro-cyanide test
for, 104

Proteins. Acree-Rosenheim test on, 100
action of alkaloidal reagents on, 103

of metallic salts on, 103

mineral acids, alkalies and organic acids
on, 103
Bardach's reaction on, loi
biuret test on, 98
chart for use in review of, 121
chemical composition of, 63
classification of, 93, 95
coagulated, 94, 116

biuret test on, 118

formation of, 116

Hopkins-Cole reaction on, 118

Millon's reaction on, 118

solubility of, 118

xanthoproteic reaction on, 118

quantitative determination of, 327
coagulation, influence of salts upon, 117
coagulation or boiling test for, 105
color reactions of, 97
conjugated, 94, 93, 112, 123

classes of, 94, 112

experiments on, 59, 113, 128, 296, 321

nomenclature of, 94, 112

occurrence of, 94, 112
decomposition of, 64, 67, 68

by hydrolysis, 63

by oxidation, 64

products of, 64, 67, 68, 71
experiments on, 85
separation of, 85
study of, 64, 67, 85
derived, 94, 114
formation of fat from, 179
formulas of, 64
Heller's ring test on, 103
Hopkins-Cole reaction on, 98
importance of, to life, 63
in urine, 412, 422

determination of, 331

test for, 423
Liebermann's reaction on, 100
Millon's reaction on, 97
of milk, 315, 318
molecular weights of, 64
Posner's reaction on, 100
precipitation of, by alcohol, 106

alkaloidal reagents, 103

metallic salts, 103

mineral acids, 103
precipitation reactions of, 102
quantitative determination of, in milk, 328
review of, 121
Robert's ring test on, 104
salting-out experiments on, 103
salts of, 103

scheme for separation of, 122
simple, 93, 95
synthesis of. 66, 70
xanthoproteic reaction on, 98
Proteolysis, peptic, 142

tryptic. 142, 186
Proteolj-tic enzymes (see Proteases, p. 13)
Proteose, 64, 94, 93. 118

V. Aider's method for detection of, 437
biuret test on, i30
coagulation test on, 120

632

INDEX

Proteose, deutero, 94, 95, 120

differentiation of, from peptone, 120
experiments on, 119, 120
hetero, 95, 120
in urine, 412, 426
test for, 427
potassium ferrocyanide and acetic test on,

120
powder, preparation of, 120
precipitation of, by nitric acid, 120
by picric acid, 120
by potassio-mercuric iodide, 120
by trichloracetic acid, 120
primary, 120
proto, 95, 96, 120

Schulte's method for detection of, 427
secondary, 120

separation of, from peptones, 120
Protoproteose, 95, 96, 120
Proteoses and peptones, 95, 96, 119, 120
separation of, 120
tests on, 120
Proteose-peptone, 119

Proteose-peptone, coagulation test on, 120
experiments on, 119
Millon's reaction on, 119
precipitation of, by nitric acid, 120
by picric acid, 120
Prothrombin, 256, 257
Pseudo-globulin, 246

Ptomaines and leucomaines in urine, 370, 401
Ptyalin (see Salivary amylase, i, 4, 10, 55, 187)
Purinases, 127, 134

experiments on, 134
Purine bases, 125, 126, 132, 346, 370, 401
formulas for, 127
in urine, quantitative determination of, 513

tests on, 132, 133
content of foods, 572
excretion, rate of, 574
oxidases, s, 127, 134
Purines, amino, 127, 132

oxy, 127, 132
Purine-free and high purine diets, influence of, 571
Pus casts in urinary sediments, 465, 472
cells in urinary sediments, 472
in urine, 431

tests for, 431, 432
Putrefaction, control of, by carbohydrate, 213

indican as an index of, 212, 386
Putrefaction mixture, preparation of a, 214
products, 212

experiments on, 214
most important, 212
tests for, 218
Putrescine, 212
Pyloric glands, 138
Pyrimidine bases, 125, 126, 128
experiments on, 133
formulas for, 128
Pyrocatechol-sulphuric acid, 369, 386
a-pyrrolidine-carboxylic acid (see Proline, pp. 65,

67, 68, 83, III, 142, 186)
Pyuria, 431

Quadriurate, 461

Qualitative analysis of the products of salivary
digestion, 60

Quantitative analysis of blood, 270

of gastric juice, 148

of milk, 324

of urine, 479
Quevenne lactometer, determination of specific
gravity of milk by, 324

RafEnose, 19, 42

Raiziss and Dubin's volumetric methods for total

sulphur, 551
Rancid fat, 178

Raw and heated milk tests, 320
Reaction of the urine, 361, 479, 580
Reagents and solutions, 594-610,
Reduced alkali-hematin, 299
Reduced hemoglobin, 296
Reductases, 319
Rehfuss stomach tube, cut of IJ9

use of, 149, 159
Reichert's method for crystallization of oxy-
hemoglobin, 266
Reinsch test for arsenic, 449

for mercury, 450
Remont's method for detection of salicylic acid

and salicylates, 323
Rennin, gastric, 139, 143, 147, 315, 321

action of, upon casein, 143, 147, 315, 321

experiments on, 147, 321

influence of, upon milk, 147, 321

in gastric juice, absence of, 143

nature of action of, 143, 315

occurrence of, 143
Rennin, pancreatic, s, 189, 194

experiments on, 194
Rennin-pepsin controversy, 143
Resorcinol-HCl reaction, 35, 447
Respiration, chemistry of, 255
Retention meal in gastric analysis, 161
Reticulin, 112

Reversibility of enzyme action, 8, 57
Reynolds-Gunning test for acetone, 438
Rhamnose, 19, 38

Rhubarb, influence of, on color of feces, 238
Ricin, 13, 262
Riegler's reaction, 23, 414
Rigor mortis, 339, 340
Ring test for urobilin, 400
Roaf's method for crystallizing hippuric acid, 390,

587
Robert's ring test for protein, 104. 424

reagent, preparation of, 104, 424
Robin's reaction for urorosein, 453
Rosolic acid, use of, as indicator, 158, 513
Rosenheim's bismuth test for choline, 358
Rosenheim's periodide test for choline, 357
Rosenheim and Drummond's volumetric methods

for sulphates and total sulphur, 550-551
Rose's method for determination of pepsin, 167
Rothera's reaction for acetone, 438
Rubner's test for lactose in urine, 445
Ruhemann's uricometer, cut of, 513

use of, 5 13
Russo's reaction, 455

Ruttan and Hardisty's orthotolidin test for blood,
171. 233, 263. 430

Saccharide group, 20
Saccharose (see Sucrose, 19, 41)

INDEX

633

Sahli's desmoid reaction, 146

reagent, 164
Salicyl aldehyde reaction for acetone (Frommer),

438
Saliva, S4

alkalinity of, 55
amount of, 55
bacteria in, 58
biuret test on, 58
calcium in, sp
chlorides in, 59
constituents of, ss
digestion of dry starch by, 60
digestion of inulin by, 60
digestion of starch paste by, 56, 59
dilution of, influence on digestion, 60
enzymes contained in, 55
excretion of potassium iodide in, 61
inorganic matter in, tests for, 59
Millon's reaction on, 58
mucin from, preparation of, 59
nitrites in, test for, 59
phosphates in, test for, 59
potassium thiocyanate in, 59
reaction of, ss, 58
secretion of, S4
specific gravity of, 55, s8
sulphates in, test for, S9
tests on, 58
thiocyanates in, ss, S9
tripeptide-splitting enzymes in, 57
Salivary amylase, i, 4, 10, 55. 187

activity of, in stomach, 57, 188
inhibition of actixaty of, 57
nature of action of, s6, 57
products of action of, 56
scheme showing, 56
Salivary digestion, 54

graphic representation of, 56
influence of acids and alkalis on, 56, 61
dilution on, 57, 60
metallic salts on, 6x
temperature on, 60
nature of action of acids and alkalis on, 6i
qualitative analysis of products of, 60
Salivary digestion in stomach, 57, 188
glands. 54
stimuli, 54
Salkowski-Autenrieth-Barth method for deter-
mination of oxalic acid in urine, 54s
Salkowski's method for determination of purine

bases, 516
Salkowski-Schippers reaction for bile pigments,

208, 433
Salkowski's test for cholesterol, 210, 357

for creatinine, 385
Salmine, bi, 68, 69, 94, 95
"Salt-free" diet, metabolism on a, 576
Salted plasma, preparation of, 268
Salting-out experiments on proteins, 105, 122
Santonin, influence of on color of feces, 238
Saponification, 177, 181, 182
of bayberry tallow, 181
of lard, 182
Sarcolactic acid, 342

Scallops, preparation of glycogen from, 348
Schalfijew's method for preparation of hemin,
366

Schema for "blood counting," 311
Scheme for analysis of biliary calculi, 209
bone ash, 338
stomach contents, 159
urinary calculi, 477
separation of carbohydrates, 53
of proteins, 122
Scherer's coagulation method for determination

of albumin in urine, 531
Schifl's reaction for cholesterol, 210, 357

for uric acid, 381
Schmidt diet, composition of, 228
■ Schmidt's nuclei test for pancreatic insufficiency,
237
Schmidt's test for hydrobilirubin, 23s
Schulte's method for detection of proteose in

urine, 427
Schumm's modification of the guaiac test, 262
Schutz's law, statement of, 9, 166
Schweitzer's reagent, action of, on cellulose, 49

preparation of. 49
Scleroproteins, (see Albuminoids), 93. 112
Scombrine, 67. 94
Scombrone, 93. 95

Scott-Wilson apparatus, cut of, 536
Scott- Wilson method for acetone and diacetic acid
in blood. 284
in urine, 536
reagent 537
Scybala, 50, 223

Secondary protein derivatives, 65, 94. "8
Secondary proteoses, 120
Secretin, 185
SeliwanoS's reaction, 35, 447

reagent, preparation of, 35, 447
Senna, influence of, on color of feces, 238
Separation of feces, importance of, in nutrition

and metabolism experiments, 224, 587
Serine, 65. 67. 69, 73

crystalline form of, "3
formula for, 73
Serum albumin, 93, 245, 268, 412. 422
in urine, 412, 422
test for, 423
Serum, blood, 24s. 267

milk. 313
Serum globulin, 93, 246, 412, 422
in urine, 412, 422
test for, 423
Shackell's method for vacuum desiccation, 482
Shaffer and Marriott's method for acetone and

diacetic acid, 539
Shaffer and Marriott's method for determination

of ^-hydroxybutj-ric acid, 539
Sherrington's solution, preparation of, 30S
Silicates in urine. 370. 411
Silver reduction test for uric acid (Schiff), 381
Skatole, 212, 213, 214, 219

tests for, 219
Skatole-carbonic acid. 217. 220

test for. 220
Smith's test for bile pigments, 208. 433
Soap, salting-out of, 181

insoluble, preparation of, 182
Sodium and potassium in urine, 370, 409. S6i

quantitative determination of, 561
Sodium alizarin sulphonate as indicator, 153. IS4.
157. 158, 174, 481

634

INDEX

Sodium alizarin sulphonate, preparation of, 154,

158
Sodium chloride, crystalline form, 267
Sodium chloride in urine, 409, 556, 561, 576
Sodium hypobromite solution, preparation of, 601
Sodium nitrite-ferrous sulphate reaction for di-

acetic acid (Hurtley), 440
Sodium nitroprusside test for acetone, 437
Sodium sulphide solution, preparation of, 607
Solera's reaction for detection of thiocyanate in
saliva, 59
test paper, preparation of, 59
Soluble starch, 11, 43, 56

as indicator, 165, 280, 286, 524, 533
Sorensen's formol titration method for amino
nitrogen, 502
indicator method for hydrogen ion concen-
tration, 158, 480
Soxhlet apparatus for extraction of fat, 326
Soxhlet lactometer, determination of specific

gravity of milk by, 324
Specificity of enzyme action, 7
Spectroscope, use of in detection of blood, 297
Spermatozoa in urinary sediments, 473

microscopical appearance of human, 474
Spiegler's ring test for protein, 104, 424

reagent, preparation of, 104, 424
Spiro's reaction for hippuric acid, 390
Spongin, 69

Standard ammonium thiocyanate solution, prepa-
ration of, 594
creatinine solution, 599
iodine solution, 602
potassium permanganate, 605
picramic acid, 60s

silver nitrate solution, preparation of, 606
sodium alcoholate, 607
sodium thiosulphate, 604, 607
uranium acetate solution, preparation of, 609
uric acid solution, 610
Starch, 20, 43

action of alcohol on iodide of, 45
action of alkali on iodide of, 45

heat on iodide of, 46
dry, digestion of, by pancreatic amylase,

188, 192
dry, digestion of, by salivary amylase, 60
experiments on, 43
hyperglycemia produced by, 567
iodine test for, 45

ftiicroscopical characteristics of, 43, 44
microscopical examination of, 45
potato, preparation of, 43
soluble, ir, 43, 56
soluble starch as indicator, 165, 280, 286,

524, 533
solubility of, 43
various forms of, 44
Starch group, 20

Starch paste, action of tannic acid on, 45
diffusibility of, 45

digestion of, by pancreatic amylase, 188
191
by salivary amylase, 10, 56, 59
Fehling's test on, 45
hydrolysis of, 45
iodic acid paper, 59
preparation of, 45

Steapsin (see Pancreatic lipase, 5, 13, 178, 188,

193
Stearic acid, 177, 354
Stearin, 177, 178, 313
Stellar phosphate, 322, j6o
Stercobilin, 222
Stokes' reagent, action of, 296

preparation of, 296
Stomach contents, lactic acid in tests for, 170
examination of, 159
pepti de-splitting enzyme in, 142, 199
removal of, 161
tube, Rehfuss, 149
Stomach, motor and functional activities of, 159
Stone-cystine, 77
Sturine, 67, 68, 93
Sublingual glands, characteristics of saliva

secreted by, 54
Submaxillary glands, characteristics of saliva

secreted by, 54
Substrate, 3
Succinic acid, 214
Sucrase, 4, 14, ips. 200

experiments on, 14, 200
vegetable, 14
Sucrose, 19, 41

experiments on, 42
inversion of, 42
production of alcohol from, 42
structure of, 41
Sucrose-H2S04 test (Pettenkofer), 208, 434
Sulphanilic acid, 455
Sulphates in saliva, test for, 59
Sulphates in urine, 370, 403, 546
ethereal, 404, 551

quantitative determination of, 547
experiments on, 404
inorganic, 404, 550

quantitative determination of, 547
total, quantitative determination of, 546,
551
Sulphocyanides (see Thiocyanates, 55, 59. 369,

392)
Sulphur in protein, 63, 108
acid, io8
in urine, gravimetric determination of, 546

volumetric determination of, 550
lead blackening, 108
loosely combined, 108
mercaptan, 108
neutral, 108, 404
oxidized, 108
"partition," in urine, 577
tests for, 108
unoxidized, 108
Sulphuric acid test (Piria), 86
Surface tension test for bile acids (Hay), 209, 434
Suspension of manganese dioxide, 513
Synthesis of hippuric acid, 585

demonstration of, 585

Tallow bayberry, saponification of, 181
Tallquist's hemoglobin scale, determination of

hemoglobin by, 304
Tannic acid, influence of, on dextrin, 48
on starch, 45

precipitation test for proteose (Ott),
429

INDEX

635

Tannin test for carbon monoxide hemoglobin,

298
Tanret's reagent, preparation of, 104, 425
Tanret's test, 104, 425
Tartar, formation of, 55
Taurine, 204, 210, 341, 346, 369, 392
derivatives. 369, 392
formula for, 204
microscopical appearance, 211
preparation of, 210
Taurocholic acid, 204

group, 204
Teichmann's crystals, form of (see Hemm
crystals, p. 265)
test. 264, 266, 429
Tendomucoid, 94. 113. 332
biuret test on, 332
chemical composition of, 113
hydrolysis of, 332

loosely combined sulphur in. test for, 332
preparation of. 332
solubility of. 332
Test meals. i6i

Ewald, 161
water. i6r
retention. i6r
Tetrapeptides, 66. 95
Tetramethylene-diamine, 214
Tetranucleotide, 123

Thiocyanates in saliva, significance of. 53
ferric chloride test for. 39
Solera's reaction for. 59
Thiocyanates in urine, 369. 392
Thiophene reaction. 171
Thoma-Zeiss hemocj'tometer, 304
Thrombin, 247. 257
Thromboplastine, 257
Thymol, formula for, 367

interference in Heller's ring test, 423

determination of sugar, acetone bodies,
phosphates and magnesium in urine,
367
interference of, in Lieben's acetone test, 437
vise of, as preservative, 367
Thymolphthalein, use of, as indicator, 137, 138
Thymus histone. 93
Thymus nucleic acid. 124. 131

preparation of. 131
tests on, 132
Time relations of protein metabolism, 369
Tincture of iodine, preparation of. 608
Tissue, adipose, experiments on, 176. 338
connective, 330

white fibrous. 331

composition of, 331
experiments on, 332
yellow elastic, 333

composition of, 334
experiments on. 334
epithelial, 330

experiments on 331
muscular, 339

experiments on. 347
nervous. 353

experiments on. 336
osseous. 336

experiments on, 337
Tissue debris in urinar>' sediments, 463, 473

Titanium tetrachloride as cellulose solvent, 49
Toison's solution, preparation of, 608
o-Tolidin test for blood, 233. 263, 430
ToUen's reaction for conjugate glycuronates, 442
arabinose. 37
galactose. 36. 446
pentoses in urine, 443
Tdpfer's method for quantitative analysis of

gastric juice. 174
Tfipfer's reagent, as indicator, 133. 134, 164, 173

preparation of, 173
Total solids, of milk, quantitative determination
of, 327
of urine, quantitative determination of,
483
Total sulphur of urine, quantitative determina-
tion of, 348
phosphorus of urine, quantitative deter-
mination of, 334
Trichloracetic acid, precipitation of protein by,

103, 120. 272
Tricresol-peroxidase reaction (Kastle). 320
Trimethyl-oxyethyl-ammonium hydroxide (see

Choline, 212. 354, 337)
Trioses. 19
Tripeptides. 66, 93
Triple phosphate. 362. 408, 438, 476
crystalline form of, 408
formation of. 408
Trisaccharides, 19. 42
Trommer's test. 25
Tropaeolin O. use of, as indicator, 137

preparation of, 138
Tropaeolin OO, use of. as indicator, 133, 154. 135,
157. 159
preparation of. 133. 138
Tropaeolin 000, use of, as indicator, 137

preparation of, 138
Trypsin (see also Pancreatic protease. 3, 12, 186)
action of, upon proteins, 66, 186, 189
experiments on, 190
influence of alkalis and mineral acids upon,

186
in stomach, 131, 169

determination of, 169
nature of, 186
Trypsinogen. 6. 186

activation of, 6, 186, 196
Tryptic digestion, 66, 186

influence of bile on, 190

most favorable reaction for, 19 r

temperature for, 192
products of, 66, 186, 189
Tryptic proteolysis, 142, i86
Tryptophane, 63, 67, 68, 77. 98, 199
bromine water test for, 199
formula for, 77

group in the protein molecule, 98
Hopkins-Cole reaction for, 98
mercury compound of, preparation of, 190
occurrence of, as a decomposition product of

protein, 65, 67. 68. 77
occurrence of. as an end-product of pan»
creatic digestion, 186, 189
Tuberculosis, urochromogen reaction for, 433
Tussah silk fibroin, 68
Tyrosinase, 3
Tyrosine, 3, 65, 67. 69. 74. 86, 97. i86, 463

6s6

INDEX

Tyrosine, crystalline form of, 76

experiments on, 86

formula for, 77

Hoffmann's reaction for, 86

in urinary sediments, 463

microscopical examination of, 86

Morner's test for, 86

occurrence of, 6s, 67, 69, I86

Piria's test for, 86

salts of, 77

separation of, from leucine, 85

solubility of, 86

sublimation of, 86
Tyrosine-sulphuric acid, 86

V. Udrdnsky's test for bile acids, 208, 434
Uffelmann's reagent, preparation of, 170

reaction for lactic acid, 170
Unknown substances in urine, 454
Unorganized ferments, i

sediments in urine, 457, 458
Unsaturated acids, 177
Uranium acetate method for determination of

total phosphates in urine, 552
Uracil, 125, 128, 133

Wheeler-Johnson reaction for, 133
Urate, ammonium, crystalline form of, Plate VI,
opposite p. 462
sodium, crystalline form of, 462
Urates in urinary sediments, 461
Urea, 248, 274, 341, 372, 491
crystalline form of, 372
decomposition of, by sodium hypobromite,

374. 496
excretion of, 372, 374
experiments on, 37s
formation of, 373
formula for, 372
furfural test for, 377
isolation of, from the urine, 375
melting-point of, 37s

quantitative determination of, in blood, 274
in urine, 491-499
Urea nitrate, 374, 376

crystalline form of, 374
formula for, 374
oxalate, 374, 376

crystalline form of, 376
formula for, 374
Urease, 4

decomposition of urea by, 491

preparation of, 491
quantitative determination of urea by, 274,
491
Uremia, blood in, 270, 271
Urethral filaments in urinary sediments, 46s,

473
Uric acid, 26, 127, 133, 137, 248, 270, 274, 341, 369,
377-381, 460, 476. 510, 57 1. 573
calculi, 476

crystalline form of, pure, 380
endogenous, 378, 573
exogenous, 378, 571
experiments on, 380
formula for, 377
Ganassini's test, 381
in blood, 248, 270, 274
in leukaemia, 379

Uric acid in urinary sediments, 460

crystalline form of, Plate V, oppo-
site p. 380, 461
isolation of, from the urine, 380
metabolism, 571, 573
murexide test for, 380
origin of, 378

quantitative determination of, in blood,
Benedict's method, 275
Folin-Denis method, 274
in urine, microchemical colo-
rimetric method, 510
Folin-Shafler method, 5 1 1
Heintz method, s 12
Kruger- Schmidt method,

513
Uricometer method, 5 13
quantitative determination of, Kruger

and Schmidt's method for, s 13
Hunter and Givens' modification of, 5 15
reducing power of, 26, 379, 416, 417
Ruhemann's uricometer method for, 5 13
Schiff's reaction for, 381
Uricase, 5, 127

experiments on, 137
Uricolytic enzymes, 3, 5, 127
experiments on, 137
Urinary calculi, 475

calcium carbonate in, 476
oxalate in, 476
cholesterol in, 478
compound, 475
cystine in, 476
fibrin in, 478
indigo in, 478
phosphates in, 476
scheme for chemical analysis of, 477
simple, 475

uric acid and urates in, 476
urostealiths in, 478
xanthine in, 476
Urinary concrements (see Urinary calculi, p. 475)
Urinary sediments, 457

ammonium magnesium phosphate in,

458
animal parasites in, 465, 474
calcium carbonate in, 458, 459
oxalate in, 458
phosphate in, 458, 460
sulphate in, 458, 460
casts in, 465, 467
cholesterol in, 458, 463
collection of, 457
cylindroids in, 465, 472
cystine in, 458, 462
epithelial cells in, 465
erythrocytes in, 465, 472
fibrin in, 465, 474
foreign substances in, 465, 474
hematoidin and bilirubin in, 458, 464
hippuric acid in, 458, 463
indigo in, 458, 464
leucine and tyrosine in, 458, 463
magnesium phosphate in, 458, 464
melanin in, 458, 465
micro-organisms in, 465, 474
organized, 457, 465
pus cells in, 4<>5, 466

INDEX

637

Urinary sediments, spermatozoa in, 46s, 474

tissue debris in, 465, 473

unorganized, 4S7. 4S8

urates in, 458, 461

urethral filaments in, 465, 473

uric acid in, 458, 460

xanthine in, 458, 464
Urination, frequency of, 36 i
Urine, 359-563

acetoacetic acid in, 412, 438, 539

acetone in, 412, 435, 538

acidity of, 361, 479, 577. S8o, 582

acid fermentation of, 363

albumin in, 412, 422, S3i

alkaline fermentation of, 362, 408

allantoin in, 369. '392, 5 18

amino-acids in, 369, 394, 502

ammonia in, 369, 402, 499

aromatic oxyacids in, 369, 394

benzoic acid in, 369, 39s

bile in, 412, 432

blood in, 412, 429

calcium in, 370, 409, 559

carbonates in, 370, 410

chlorides in, 370, 405

collection of, 367

collection and preservation of, in metabolism

tests, 367, 565
color of, 359

complete analysis of, 565
conjugate glycuronates in, 412, 442
creatine in, 369, 384, 508, 509
creatinine in, 369, 381, 506, 574
dextrose in (see glucose, 412, 413, S22)
diacetic acid in (see acetoacetic acid, 412, 438,

539)
electrical conductivity of, 366
enzymes in, 370, 397
ethereal sulphuric acid in, 369, 385, 547
fat in, 4 12, 444
fluorides in, 370, 411
freezing-point of, 365
fructose in, 412, 446
galactose in, 412, 446
general characteristics of, 359
globulin in, 412, 426
glucose in, 412, 413, 522
Haser's coefficient for solids in, 364, 483
hematoporphyrin in, 412, 444
hippuric acid in, 369, 388, 5 19
hydrogen ion concentration of, 36 I, 480, 580
as influenced by diet, 580
by acid and alkali, 582
hydrogea peroxide in, 370, 411
|8-hydroxybutyric acid in, 412, 440, 539
inorganic physiological constituents of, 370,

402
inositol in, 412, 450
iron in, 370, 410, 562
lactose in, 4 12, 444
levulose in (see fructose, 412, 446)
laiose in, 412, 451
leucomaines in, 370, 401
Long's coefficient for solids in, 364, 483
magnesium in, 370, 409, 559
melanin in, 412, 451

neutral sulphur compounds in, 369, 393, 55 i,
578

Urine, nitrates in, 370, 411

nucleoprotein in, 369, 396, 412, 428

odor of, 36 I

organic physiological constituents of, 369

oxalic acid in, 369, 391

oxaluric acid in, 369. 397

/9-oxybutyric acid in (see hydroxybutyric
acid, 412, 440, S39)

pathological constituents of, 412

paralactic acid in, 370, 398

pentoses in, 412, 443

peptone in, 412, 426

phenaceturic acid in, 370, 398

phosphates in, 370, 406, 552

phosphorized compounds in, 370, 399

physiological constituents of, 369

pigments of, 359, 370, 399

potassium in, 370, 409, s6i

proteins in, 412, 422

proteoses in, 412, 422, 426

ptomaines in, 370, 401

purine bases in, 370, 401, Si3

quantitative analysis of, 479-5^3

reaction of, 361, 479, S8o

as influenced by diet, 580

by acids and alkalies, 582

silicates in, 370, 411

sodium in, 370, 409, 56 I

solids of, 364, 483

specific gravity of, 363

sulphates in, 370, 403» S46

transparency of, 360

unknown substances in, 412, 454

urea in, 369, 372, 491

uric acid in, 369, 377, 5 10

urinod in, 361

urorosein in, 412, 452

volatile fatty acids in, 370, 397

volume of, 359
Urinod, 361
Urobilin, 359, 370, 399

tests for, 400
Urobilinogen, 399
Urocanic acid, 398
Urochrome, 359, 3"0, 399, 4^1
Urochromogen, 412, 453

reaction (Weisz) for tuberculosis, 453
Uroerythrin, 359, 370, 399. 421
Uroferric acid, 369, 392, 454
Uroleucic acid, 369, 395
Urorosein, 412, 452

reaction, 452

tests for, 452

Valine, 65, 67, 69, 78

Van Slyke's method for determination of total
amino-acid nitrogen,
in urine, 505
in blood, 377
in protein hydrolysis,
88
Van Slyke and CuUea's method for urea in blood,
274
for urea in urine, 49a
Van Slyke and McLeans method for chlorides in

blood, 286
Vegetable amylase, 4, 11
lipase, 5, 13

638

INDEX

Vegetable protease, 13

sucrase, 14, 195, 199
Vegetable globulins, 93, 95, 108
Vegetable gums, 20
Veith lactometer, determination of specific

gravity of milk by, 324
Viscosity test, 59
Vitamines, 313
Vitellin, 94, 95

Volatile fatty acids, 212, 215, 370, 397
Volhard-Arnold method for determination of

chlorides, 556
Volhard-Harvey method for determination of

chlorides, 557
Volume of the urine, 359

Water at meals, influence of, 138, i8s, 402, 574

softened, 57
Water test meal, 161
Water, influence of on metabolism, 574
Wax myrtle, 181

Waxy casts in urinary sediments, 465, 470
Weber's guaiac test for blood in feces, 235
Weinland, formation of fat from protein, 179
Weisz's urochromogen reaction for tuberculosis,

453
Welker's electrical bath, 494

modified method for purine bases, s 15
Welker and Marsh method for deproteinizing milk,

329
Welker and Tracy method for deproteinizing

urine, 485
Weyl's test for creatinine, 385
Wheeler- Johnson reaction for uracil and cytosine,

133
White fibrous connective tissue, 331

experiments on, 332
Wiechowski-Handovsky method for determi-
nation of allantoin in urine, 518
Wilkinson and Peters' test, 321
Wirsing's test for urobilin, 401
Witchs' milk, 317

Wohlgemuths' method for quantitative deter-
mination of amylolytic activity, 192
Author's modification of, 239

Wolter's method for determination of iron in
urine, 562

Xanthine, 126, 127, 132, 346, 354, 401

bases (see Purine bases, pp. 126, 346, 401)

crystalline form of, 344

formula for, 127, 346

in urinary sediments, 458, 464

isolation of, from meat extract, 35 1

silver nitrate, 351

crystalline form of, 351
test, 351
. tests for, 132

Weidel's reaction for, 132
Xanthophylls, 319
Xanthoproteic reaction, 98
Xanthinoxidase, s
Xylose, 20, 38

orcinol reaction on, 38

phenylhydrazine reaction on, 38

Tollens' reaction on, 38

Yeast, enzymes of, 2

fermentation by, 42
nucleoprotein of, 128
preparation of, 128
tests on, 129
nucleic acid of, 125, 130
formula for, 125
preparation of, 130
tests on, 130
Yellow elastic connective tissue, 33;^
composition of, 334
experiments on, 334

Zappert slide, 307
Zein, 67, 69, 93, 95, III

decomposition of, 67, 69
Zeller's test for melanin, 452
V. Zeynek and Nencki's hemin test, 266, 430
Zikel pektoscope, 365
Zymase, classification of, 4

preparation of, 2
Zymo-exciter, 7
Zymogen, 6, 186