THE OCCURRENCE DURING ACUTE INFECTIONS OF A
PROTEIN NOT NORMALLY PRESENT IN THE BLOOD

II~. I~OLOGICAI. PROPERTIES OF THE C-REACTIVE PROTEIN AND ITS
     DIFFERENTIATION FROM NORMAL BLOOD PROTEINS

BY COLIN M. MAcLEOD, M.D., AND OSWALD T. AVERY, M.D.
(From the Hospital of The Rockefeller Is.sti&te for Medical Research)

(Received for publication, October 7, 1940)

Previous studies from this laboratory have shown that serum obtained
from patients during the acute phase of certain infectious diseases reacts
to form a precipitate with the C polysaccharide of Pneumococcus.  In the
two preceding papers (1, 2) evidence was presented that the C-reactive
substance in "acute phase" serum is protein in nature; certain of the
chemical properties which distinguish the so called "C-protein" from normal
serum proteins were described, and some of the distinctive features of its
reactivity with the test carbohydrate were discussed. Because of these
differences in chemical properties and in view of the fact that it is not
demonstrable in the blood of convalescents and healthy individuals, the
question arose whether this particular protein might not also possess im-
munological properties specifically different from those which characterize
the proteins normally found in human serum.  With this object in mind
the following experiments were carried out.
The present paper presents the results of a study of the antigenicity and
immunological specificity of the C-protein.  It will be shown that the them-
ical individuality of this substance is reflected in the serological spec&$y
of the antibodies to which it gives rise in the rabbit, and that by means of
antisera it is possible to differentiate the C-protein from the normal protein
constituents of human serum.

EXPERIMEkTAL

Preparation of ~knwizng Antigens.-The C-protein used for the im-
munization of rabbits was prepared from blood obtained at autopsy from
fatal cases of Pneumococcus lobar pneumonia.  The reactive protein was
precipitated from the serum by the addition of an optimal concentration
of the C polysaccharide. It has been shown that in the C-reaction, floccula-
tion of the active protein is conditioned by the calcium ions normally present
                        191


192     ABNORMU PROTEIN IN BLOOD DURING INFECTION. III t

in the serum, and that the precipitate thus formed can be repeatedly washed
with a dilute solution of calcium chloride without loss of the reactive
protein. Thus a method was available for obtaining the C-protein rela-
tively free from the' normal serum proteins and in a form especially suitable
for testing its anligenicit;; in animals.

Human serum known to contain the C-precipitable protein was passed through s
Berkefeld filter to remove bacteria and cellular debris.  To the tiRered serum the C
polysaccharide was added in final concentration of 1:20,000.  The mixture was incubated
2 hours at 37'C. and overnight in the refrigerator.  The precipitate which formed was
recovered by centrifirgation. In order to remove as completely as possible any nom]
protein which may have become entrained during flocculation,. the precipitate was
thoroughly washed 3 or 4 times with large portions of aa/ calcium chloride in physio-
logical saline.  The washed precipitate containing the C-protein was then emulsified in
a volume of bf/iOO aqueous solution of calcium chloride equal to l/10 the volume of the
original serum.  This preparation of the protein in particulate form was used as immunis-
ing antigen.       
                 I
Other lots of reactive protein prepared in this same manner were further purified by

re-solution and reprecipitation. The precipitate after repeated washings with dilute
calcium was 6nely enmlsiied in physiological saline and redissolved by the dropwise
addition of the minii amount of ~/lo NaOH necessary to effect solution which occurs
at approximately pH 8.5, probably due to the splitting off of bound calcium; a small
amount of insoluble material was removed by centrifugation.  Prom the clear super-
natant, the protein was reprecipitated by adding an equivalent amount of ~/lo HCI
bringing the solution back to neutral reaction at which flocculation again occurs.  The
reprecipitated protein was recovered by centrifugation and the same procedure repeated
a second time. The precipitate was again washed in ~/20 calcium chloride in physio-
logical salt solution and then resuspended in a &ely divided state in a6/100 CalciUm
chloride in distilled water. All preparations used for immunization were standardized
as to protein content on the basis of total nitrogen present.  Merthiolate in final concen-
tration of 1:20,000 was added as preservative.

Immunization of Rabbits.-Rabbits were injected intravenously on each of 5 Or 6
consecutive days with 1 cc. of a preparation of the antigen containing approximatelY 1.5
mg. of protein per cc. 7 days after the last injection the animals were bled.  Immune
sera prepared in this manner are referred to in the following proto& as anti-CP rabbit
serum.

C P&acckkde.-The C polysaccharide was prepared from an R strain derived from
Pneumococcus Type II. The methods of isolation and purification were the same as
those previously described (3).

Serok%kal fiactim.-The precipitation and complement-fixation tests were carried
out with anti-CP rabbit sera prepared as stated above; the test antigens used in *e
serological reactions were, (a) whole serum obtained from patients with acute infections
and known to contain the protein reactive with the C polysaccharide; (b) control serum
from healthy individuals; (c) purified preparations of the C-reactive protein isolated
from patients' serum by salting out with sodium sulfate according to the method de-
scribed in the preceding paper (2).


COLIN 116. lUcLEOD AND OSWALD T. AVERY        193

I,,,~~&ogicd Specificty of the C-Reactive Protek-In view of &e
chemical tierences which distinguish this protein from the norms~ serum
pmtehs it was of mterest to determine whether corresponding differences
,+t in antigenic function and serological speci&ity. For this purpose
antisera were prepared by injecting rabbits with washed precipitates of the
,.,,active protein removed from acute phase serum by the C polysaccharide.
The method Of preparing the immunizing antigen, the technique-for the
preduction of rabbit antisera, and the nature of test antigens used in the

TABLE I

Pruiidins in Sera of Rabbits Imnunized with C-Rmctivc prot&*
    I              Dflutfons of tent antfgcna

&PnbNt MNm I  Patfat's aenml; acute stnge of l&u
                   pneumonk

1:2

      1       +++
      2        +++
     3       ++++

Control: normal rabbit
seromt. . . . . . . . . . . . .    -

  1:s

+++*
+++*
++++

1:10

+++*
+++*
++++

Normal human serum

I:2  I 1:s I 1:10

f     +     +
      Tr.      Tr.
f      +       f

Tn this and the following table-s tbe degree of precipitation is expressed by the symbols:
++++ - flocculent precipitate, clear supematant.
  + - slight turbidity.
   Tr. = trace.

o Protein precipitated from acute phase serum by C polysaccbaride.
t Pooled sera of normal rabbits.

serological reactions have been described in a preceding section of this
paper.

In the following experiment various lots of anti-CP rabbit serum were
tested for the presence of precipitins for the C-protein by adding a constant
amount of immune serum to serial dilutions of patient's serum known to
contain the reactive protein as determined by previous test with the ,C
polysaccharide. As controls the same antisera were similarly tested against
normal human serum known to be free from the C-reactive protein.  The
results of the precipitin tests are presented in Table I.

As shown in Table I the precipitins in anti-CP rabbit serum are highly
specific for the C-protein and react only weakly or not at all with the pro-
teins normally present in human serum. The lack of cross-reactions is
particularly noteworthy in this instance, since the antisera had not been


194   ABNORMAL PRO- IN BLOOD DURING XNFECTION. III

previously absorbed `with normal human serum before being used' in the
test. The specificity of the antibodies under these conditions is all the
more striking in view of the' fact that the test antigens contained in common
the normal proteins of human serum.

Furthermore, the results of the precipitin tests demonstrate that the
reactive protein precipitated by the C polysaccharide is markedly antigenic
and in this form is capable of inciting in rabbits the production of antibodies
specifically reactive with the homologous protein in the native state in
which it exists in the serum of infected patients.
In the following experiment the precipitins in another lot of anti-CP
rabbit serum were titrated by the use of acute phase and normal human
sera as test antigens. For purposes of titration the immune serum was
first absorbed with normal human serum to remove any cross-reacting anti-

TABLE II

Preci#itin Reactions of AntXP Rabbit Serum with Acute Phase and Nomad Hunm Sero

serum of
rabbits imau-                        Dflutfcm of test antigem
nfzed with     Test antiga~ used
C-pIOtGiU*                       1:2    1:10 1:20 150  ~ 1:m 1:soo 1:looo
                           -------
Lot4   Acut.ephaaehumanserum ++++ +++ +++ ++zk +-I: A    -


       Normalhumanserum     l-r. l-r. - - - - -
* Precipitated from patient's serum by C polysaccharide.

bodies which if present would tend to mask the end point. The particular
specimen of acute phase serum used as test antigen was obtained from a
patient acutely ill with Type III Pneumococcus pneumonia who at the time
had high fever, a marked bacteremia, and massive puhonary involvement.
`The precipitating action of the immune serum in the presence of kreas-
ing dilutions Of the test antigens is shown in Table II.

The data presented in Table II again demonstrate the selective specificity
of the precipitins in anti-CP rabbit serum.  The results also show that the
presence of the reactive protein could still be detected in the patient's serum
when the latter was diluted 1 part in 500. In the absence of quantitative
data as to the actual amount of reactive protein present in the test serum
it is of course obvious that the result does not represent the true titre cf
precipitins in the immune rabbit serum. The reactions do indicate, how-
ever, the relative sensitivity of the precipitb test as a means of demonstrst-
ing the reactive protein when present in amounts too small to be detected
by the precipitation test with C polysac&ride. In a par&l series of
tests the latter reaction was completely negative in all dilutions of the same


COLIN M. MM!LEOD AND OSWALD T. AVERY        195

Serum above 1: 20.  Because of inherent differences in the nature of the
two reactions the use of the polysaccharide test alone may be misleading.
ln the precipitin reaction the precipitate is composed largely of the antibody
Sl&ulin from the immune rabbit serum, while in the flocculation test with
C pelysaccharide, the precipitate consists chiefly of the reactive protein
present in the albumin fraction of the patient's serum.  Consequently in
be latter test a negative result does not necessarily imply the complete
absence of the react& protein since it may be present in amounts too small
to yield a visible precipitate with the test carbohydrate.  This diEerence
in the sensitiyity of the two tests has both theoretical and practical interest;
for example, the use of specific antiserum would be the method of choice
in any attempt to trace the origin and fate of the reactive protein in the
tissues and fluids of the body.
              .
                        TABLE III

p&pith Reactions of Anti-CP Rabbit Serum with Ptijied Pre@mtim of Reactive Proteilt

Anti-CP rabbit
E%.

   Dflutio~ of tat a&em

Purfssd pnpurtion of rencth protein*

   4 y;; 1 :% 1 lY@ j 1:1;, 1 1::;
* Isolated from patient's serum by salting out reactive protein with sodium sulfate,
followed by dialysis and reprecipitation (2).

In the following experiment the same lot of anti-CP rabbit serum as that
used in the preceding test was titrated against a purified preparation of the
reactive protein. In this instance the test antigen was prepared by salting
out the reactive protein from acute phase human serum with sodium sulfate
followed by dialysis and reprecipitation as described in the preceding paper
(2). The dilutions of test antigen are expressed in terms of protein based
on the content of total nitrogen in the preparation.  The results of the
precipitin titration are given in Table III.
As shown in Table III the titre of precipitins in this particular antiserum
was 1: 240,000 when a highly purified preparation of reactive protein was
used. The immune serum was the same lot as that used in the preceding .
experiment and had been absorbed with normal human serum prior to use
in these tests.

The immunizing antigen used in preparing the antiserum consisted of the
reactive protein precipitated from patients' serum by C pclysaccharide
whereas the test antigen was prepared by salting out the serum albumin
and subsequently isolating the reactive protein as previously described (2).


196   ABNOl& PROTEIN IN BLOOD DURING INTECTION. KU

The difkences in the preparative methods and the fact that the immunizing
and test antigens were derived from sera of different patients serve to
emphasize the immu~~ological identity of the reactive protein and its
differentiation from the proteins of normal human serum.  The antigenic
quality of the C-precipitable protein is reflected in the high titre of pre+
itins in the serum of rabbits which had received during a single course of
five daily injections a total of only 6.5 mg. of the reactive protein.

As pointed out in the preceding experiment, the greater sensitivity of the
precipitin reaction as contrasted with that of the flocculation test with C
polysaccharide is again evident in the present instance where the quanti-
tative relationships are more adequately defined. Although not shown
in the protocol, it was found in a parallel series that the reaction with the
C polysaccharide was completely negative in dilutions of the test antigen
above 1: 15,000, whereas with immune rabbit serum the presence of the
homologous protein could be detected in dilutions as high as 1: 240,000.

The amount of reactive protein in the blood during acute bacterial
infections is relatively small and varies in individual cases depending to
some extent at least upon the nature and severity of the pathological
process. AS pointed out in earlier studies (4) the concentration of the
C-precipitable substance in patients' serum is maximal during the height
of the disease and progressively diminishes following the onset of recovery.
Abemethy and Francis (5) have shown that in severe cases of pneumonia,
the serum may give a positive flocculation reaction when the test carbo-
hydrate is added in dilutions as high as 1: 640,000.  Reactions of this order
compare favorably in sensitivity to precipitin reactions involving the
combination of an antigen with its specific antibody.  The flocculation of
the reactive protein in the presence of the C polysaccharide affords a means
of determining roughly the amount of reactive protein present in a give*
serum; however, for the detection of minute quantities of the protein the
immunological reaction with anti-(X rabbit serum is far more sensitive.

Co??#e??k%t Fixation by Reactive Protein and $pecijc A&sew@.-
In order to compare further the antigenic specificity of the C-reactive pro-
tein with that of normal serum proteins, the corresponding antisera were
prepared in rabbits and tested for the capacity to bind complement in the
presence of varying dilutions of the C-reactive protein.
          .
The technique used in the complement-iixation test was the -e as that described
by Pittman and Goodnerl (6). The anti-CP rabbit serum was prepared as described

l The authors take pleasure in thanking Dr. Go&xx for his kindness in carrying Out
these tests.


COLIN MM. IUcLEOD AND OSWALD T. AVERY       197

llnd was absorbed with nod human serum. The immune sera to the normal proteins
in human blood were produced by injecting rabbits intravenously on each of 5 consecutive
days with 0.2 CC. of whole serum obtained from a healthy individual.  The total amount
of normal serum injected was 1.0 CC. per rabbit.  7 days after the last injection the
Bnimals were bled and their sera tested for precipitins and complement-fixing antibodies.
In precipitin tests the latter antisera reacted with normal human serum diluted as high
as 1:80,000.

The C-reactive Protein used as test antigen was prepared from patient's serum by
salting out with sodium sulfate, followed by dialysis and reprecipitation (2). The
amount of protein Present was estimated by determination of the total nitrogen.  The
dilutions of the protein used in tests were made in physiological saline.  Results of the
complement-fixation tests are shown in Table IV.

TABLE Iv

ComQk~~ Fistic &Y Anti-CP Rabbit Serum ad Reactive Protein Isolated jrm
                Patient's Serum

    Sem of rabbits immunized with          Purihd preparation of reactive pmteill*

                                1:5000        l:so,ooo       1250,000
C-proteinf _ . . . . . . . . . . . . . . . . . . . . . _ . . .   +++     ++++     +++
Normalhumanserum . . . . . . . . . . . . . . . .._      -

Degree of fixation expressed by the symbols:
+ + + + = complete fixation of complement.
    - = no kation of complement.
* Isolated from patient's serum by salting out reactive protein with sodium sulfate,
followed by dialysis and reprecipitation (2).
t Prepared by precipitating the reactive protein from acute phase sefum with C
polysaccharide.

As shown in Table IV a purified preparation of the reactive protein
in dilutions of 1: 5000 to 1: 250,000 bed complement in the presence of an
antiserum prepared by immunizing rabbits with the reactive protein in the
form precipita,ted by C. On the other hand mixtures of the reactive protein
and an antiserum to normal human serum failed entirely to 6.x complement.
These results confirm those of the precipitin tests and afford further evi-
dence that the C-reactive protein is immunologically distinct from the
proteins of normal human serum.

Reactivity of Anti-CP Serum witk Acute Phase Moltkey Semcna.-It has
been shown by Abemethy (7) that the serum of moqkeys (Macacus cylso-
molgos) acutely ill with experimental Type III Pneumococcus pneumonia
precipitates with the C carbohydrate in high dilutions, but that the serum
from normal or recovered monkeys fails to react.  It was of interest to
determine whether the se&m of acutely ill monkeys would react specifically  ,
with antiserum to the C-reactive protein of acute. phase human serum.


198    ABNORhUL PROTEIN IN BLOOD DURING INPECTION. III

Morphinked monkeys (M. cynomolgos) were iujected intravenously with a virulent
strain of Pneumococcus Type I. A severe ihess accompanied by bactkmia resulted,
The animals were sacrificed on the 3rd day after inoculation.  &rum obtained from &ae
animals during the acute phase of the pneumococcal infection reacted strongly in pre-
cipitin tests with anti-CP serum, whereas the serum of the same animals before infection
gave negligible reactions.

' These results show that the antiserum of rabbits immunized with the
C-protein of human origin reacts specifically with the similar protein present
in the serum of infected monkeys.  The difference in the reactions before
and after infection leaves no doubt that an immunologically similar protein
occurs in the blood of man and monkeys during the course of acute infec-
tions-a protein not present in the serum of normal human beings or normal
monkeys.

DISCT.JSSION

The C-reactive protein present in acute phase human serum shows cer-
tain diRerences from the normal serum proteins. As previously described
(1, 2) the reactive protein is contained in the albumin fraction of serum,
but unlike normal serum albumin it is insoluble in water containing a trace
of calcium.  Furthermore, it has been shown that the insolubility of the
protein under these conditions is due to the presence of lipoid substances
associated with the protein, since upon removal of the lipids the protein
loses its calcium sensitivity,  However, removal of the lipids does not
affect the reactivity of the protein with the C polysaccharide.

In the present paper a further property is described which differentiates
the C-reactive protein from normal serum proteins, namely its specific
antigenicity.  It has been shown that the serum of rabbits immunized with
the C-reactive protein reacts specifically not only with purified preparations
of protein but also with this protein as it occurs in the serum obtained from
man and monkeys during the course of acute bacterial infections.  On'!
negligible reactions occur when normal human serum is mixed with a&Cl'
serum and this trace of cross-reactivity may be removed by absorption
without appreciable loss in the titre of the antibodies to the C-reactive
protein.

From these observations it may be concluded that the reactive protein
differs in both its chemical and immunological properties from the proteins
of normal human and monkey serum.

Observations on the presence of the C-reactive protein in the blood
during the acute phase of virus diseases in man are as yet too few to warrant
any conclusions as to its occurrence in infections of this nature.  Fd.her-


COLIN M. MAcLEOD AND OSWALD T. AVERY        199

more, there is available at present no evidence of relationship between this
protein and the various "soluble antigens" which, separable from the virus,
have heen found in the tissues and blood of man and animals acutely ill
,rith yellow fever (g), vaccinia (o), psittacosis (lo), itiuenza (ll), myxo-
matosis (X2), and lymphocytic choriomeningitis (13).  In this connection
              . .

it should be borne in mmd that in acute bacterial diseases of man the occur-
rence of the C-reactive protein is a general phenomenon and is h&pen&&
of the specific nature Of the etiological incitant.  Moreover, in diseases of
bacterial origin its demonstration is dependent on certain species relation-
ships, as shown by the fact that a similarly reactive protein has been found
only in the blood of immunologically related species such as man and
monkeys. An malogous substance may occur in the blood of other species
during bacterial infections but its detection would probably require in ea&
instanCe a selective test reagent.

SUMMARY

The C-reactive protein present in the albumin fraction of the serum of
patients during certain acute bacterial infections is highly antigenic upon
injection into rabbits. The antiserum thus prepared reacts specifically
with this protein and does not react with the proteins of normal human
serum. Immunological specificity has been demonstrated by both precip-
itin and complement-fixation tests.
Antiserum prepared in rabbits to the C-reactive protein from human
sources also reacts specifically with the similar protein in the serum of
monkeys acutely ill with experimental pneumococcus infection.
By means of immunological reactions it is possible to detect amounts of
reactive protein which are too small to yield a visible precipitate in tests
with the C polysaccharide.

Certain of the properties are discussed which distinguish the C-reactive
protein from the proteins of normal human serum.

BIBLIOGRAPHY

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200   ABNORldiL PROTEIN IN BLOOD DURING INFECTION. III

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