CA1039650A - Cancer associated polypeptide antigen, process for its preparation, process for preparing antibodies, process of cancer diagnosis and composition useful as an immunizing agent - Google Patents

Cancer associated polypeptide antigen, process for its preparation, process for preparing antibodies, process of cancer diagnosis and composition useful as an immunizing agent

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CA1039650A
CA1039650A CA175,995A CA175995A CA1039650A CA 1039650 A CA1039650 A CA 1039650A CA 175995 A CA175995 A CA 175995A CA 1039650 A CA1039650 A CA 1039650A
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cancer
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Knut B. Bjorklund
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    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/53Immunoassay; Biospecific binding assay; Materials therefor
    • G01N33/574Immunoassay; Biospecific binding assay; Materials therefor for cancer
    • G01N33/57484Immunoassay; Biospecific binding assay; Materials therefor for cancer involving compounds serving as markers for tumor, cancer, neoplasia, e.g. cellular determinants, receptors, heat shock/stress proteins, A-protein, oligosaccharides, metabolites
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K39/0005Vertebrate antigens
    • A61K39/0011Cancer antigens
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders

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Abstract

Abstract: A process for the isolation of cancer associated polypeptide antigen mainly by sveral steps of gel filtration and pH-gradient elution; a cancer associated polypeptide antigen hased on a single peptide chain and denaturating irreversibly at pHs exceeding about 4.5; a composition comprising such antigen and a stabilizing amount of albumen in admixture therewith and a method of making such composition; a diagnostic composition comprising a particulate material labelled with albumen-stabilized antigen; process for preparing antibodies monospecific with regard to the cancer associated polypeptide antigen comprising preparing an oil emulsion, wherein an acid aqueous solution of the polypeptide is enclosed phase protected by a surrounding oil phase; a cancer diagnosis method based on determining the presence of cancer associated polypeptide antigen in a living animal body under examination; and composition useful as an immunizing agent containing as an active ingredient the cancer associated polypeptide antigen.

Description

` --The present invention refers to the problem of isolating cancer associated antigen showing monospecificity and being present in a wide variety of human cancers of different localizations.
Many attempts have been made to demonstrate the presence of tumor-reactive antibodies in sera obtained from animals to which preparations of human cancer tumors have been administered. If such demonstrations would turn out to be consistently reproducible, that would indicate the presence in human cancer tissue of important antigens not present in the normal tissues and might thus lead to a better understanding of the nature o~ the neoplastic process. For the purpose of a better understanding of cancer diseases, human cancer tissue has been studied in order to find out the existence of monospecific cancer associated antigen and above all to find out a reproducible way of isolating and purifying such antigen.
The presence of antigens associated with adeno-carcinoma of the colon and the digestive system has been shown by Gold et al: J.expt. Med. 121 (1965) 439-462 and J.expt.
Med. 122, 1965 467-487. In these reports reference is had to even earlier works by B. B~orklund indicating the existence of human cancer associated antigen common to the ma~or part of all known malignant tumors of epithelial origing Internat.
Arch. Allergy and Appl. Immunol. 1966J 8~ 179 and Internat.
Arch. Allergy and Appl. Immunol. 1958~ 12, 241. In U.S. patent 3,663~ 684 to Freedman et al there is described a carcinom-embryonic antigen showing so ^alled 'ICEA-activity'i. This antigen is, however, completely different from the antigen of this ~nvention, which will be shown in detail below in this disclosure.
-2-.

-\

A practical and commercially useful isolation of antigen per se as well as its association with various car-clnomatous diseases has not hitherto been achieved. Thus, it has hitherto not been possible to isolate and characterize human cancer associated antigen by practical and reproducible methods, neither has it been possible to establish or even to indicate the presence of the antigen in the blood of persons suffering from hidden or overt cancerous disease by means of a diagnostic test suitable for the investigation in a large scale.
For the purpose of fully utilizing the presence of antibodies specific to tumor associated antigen in animal antisera as a diagnostic agent a test must be developed which shows the existence of the tumor antigen in the blood of the patient. Procedures suggested up to now have not proved to be effective when trying to make a certain diagnosis with regard to the presence of cancer disease.
One of the main objects of the invention is to provide a process for isolating and purifying cancer associated antigen starting from human tumor tissue or other tissue containing such antigen.
Another object of the invention is to characterize such antigen after its isolation.
A further object of the invention is to provide diagnostic test procedures based on the use or existence of such human cancer associated antigen.
A further object of the invention is to provide a process for preparing antibodies specific to said cancer associated polypeptide antigen.
Still a further object Or the invention is to provide a composition useful as an immunizing agent.
-3-Yet another object of the invention is to provide a composition comprising such antigen and a stabilizing amount of albumen in admixture therewith and a method of making such composition.
A further object of the invention is to provide a diagnostic composition comprising a particulate material labelled with albumen-stabilized antigen.
In this disclosure including the claims the expression "cancer associated polypeptide antigen'~ is abbreviated CAPA.
Accordingly, the invention provides i.a. practical processes for:
a) Purifying, isolating, characterizing and confirming the identity and specificity of CAPA;
b) Use of such CAPA for diagnosing the presence of cancer by indicating the presence of circulating CAPA; and c) A process for the preparation of antibodies mono-specific to such C~PA.
Other objects and characterizing features of the invention will be obvious from the following description of the invention in general terms as well as by specific examples.
A material possessing CAPA activity is isolated and purified by means of the process of the present invention by homogenizlng malignant tissues from autopsiesg carcinoma tissues of various types and sites being collected to make up a tumor pool. An alternative starting material is tissue from human placenta or cultures of malignant cells in vitro (for details on such cultures see B. Bjorklund, V. Bjorklund and I. Hedlof, J.Nat. Cancer Inst. 26: 533-545, 1961, "Antigenicity of Pooled Human Malignant and Normal Tissues by Cytoimmunological Technique. III. Distribution of Tumor Antigen. Normal tissues are also collected in parallel with malignant tissues, and to arrive at a useful sequence of process steps leading to the isolation of a pure antigen a new test procedure has been developed as per the enclosed Fig. 1. Thusg the application of biochemical separation methods was guided by a sensitive immunological assay procedure permitting the detection of less than 1 ng (nano-grams) of antigen. The greatest value of the assay technique as per Fig. 1 is based on its selectivity. Antigenic differences between extracts to be compared were manifested against a background of insignificant similarities3 the assay arrangement serving as a feedback control of an array of chemical procedures which were varied to result in tumor fractions of 1) maximum antigenic reactivity with anti-tumor sera which had been absorbed by normal antigens; and of 2) minimum antigenic reactivity with anti-tumor sera which had been absorbed by tumor antigens. For additional control purposes there were also established tumor fractions of minimum reactivity with anti-normal sera which had been absorbed by normal or tumor antigens.
Carcinoma and normal tissues while in the frozen state are separately mixed with water having a temperature of about 0C and are homogenized in such a way as not to generate excess friction heat which will cause inactivation .. . . . . . . . . . ... -1()39650 of th~ pertinent CAPA. The temperature of the suspension should not be allowed to rise above about 0C.
The resulting cold mixture of liquid homogenate and solids i8 mixed with an organic solvent having the ability of dissolving lipids, such as neutral fats, for instance acetone or ethyl ether, at a temperature below about 0C, the solvent treatment having for its purpose the removal of i.aO lipoidic substances and resulting in increased exposure of antigenic groups. The solids are separ~ted fr~m the mixture, suitably by centrifugationg the water and solvent layers being discarded. The temperature should not exceed about +4C.
The recovered solids are lyophilized and the lyophilized tissue powder is ground, as in a stainless steel ball millg at a low temperature, preferably below about 0C and suitably at a temperature below about -70C.
The grinding results in a fine, grayish-brown powder.
If desired, the resulting powder is extracted with a salt solution, such as saline, at neutral pH at low temperature, suitably about 0Cg the supernatant after centrifugation being discarded. The resulting sediment may be resuspended in cold water, the sediment being recovered and lyophilized. The resulting powder may be stored for years in closed bottles at about 4Co When extracting the above polypeptide-containing tumor and normal powders with H20 at an alkaline pH the extracts become turbid upon the addition of NaCl at neutral or slightly alkaline pHs. This turbidity is due mainly to the presence of impurities of nucleic acid character. After ~0 centrifugation of the saline-treated extracts all activity . :' :' .. .:

~75,995 remains in the clear supern~tant. The supernatant may be precipitated iso-electrically at acidic pH, suitably about .~, and the resulting precipitates are dissolved in an aqueous phosphate buffered solution of pH about 7Ø
The solutions resulting from the above procedure are filtered ~ith a suitable molecular sieve type gel in bead form permitting fractionation of compounds having a MW
range including 10-106 to 20-1069 especially about 15-106, the filtering gel being eluted with a buffer of about neutral pH and the MW fraction 10-106 to 20-106, especially about 15-106 being recovered. The gel or sieve may be selected from polyacrylamide gels, cross-linked dextran gels, agar and agarose gels and equivalent gels or molecular sieves, such as Bio-Gel A-50m (Trademark for an agarose gel from Bio-Rad Laboratories, Munchen, West Germany; 100-200 mesh, exclusion limit (Daltons) 50-106, fractionation range (Daltons) 105 to 50-106, appr. content of agarose 2 %) or -Sepharose 2B (Trademark for an agarose gel from Pharmacia Fine Chemicals, Uppsala, Sweden; 60-300 microns, beads, fractionation range 105 to 20-106, appr~ agarose content 2 %), the gel being equilibrated with a suitable buffer solution at pH about 7.0, such as Sorensen's buffer (a 1/15 ~1 buffer solution based on sodium and potassium phosphates) diluted 1:10. The type of sieve or gel used for this gel filtration is not critical and the only requirement in this regard is that it should have the ability of providing fractionation ~ ;
of compounds within the above-identified molecular weight ~-range~ Another useful gel for the purpose of the invention ~ :
is Bio-Gel A-150m, (Bio-Rad Laboratories; 100-200 mesh, -exclusion limit (Daltons) 150-106~ fractionation range (Daltons) 10 to ~150-10 ). For further details on gel . .

filtration techni~ue see H.Determann "Gelchromatographie", Springer-Verlag, BerllnoHeldelbergoNew York 1967. The eluant used for the filtration is a buffer solution of pH about 7, and in the effluent the antigen activity is found in the fraction containing said MW range, said fraction being recovered.
The sedimented active fractions from the above gel filtration is dissolved in a suitable buffer of pH
about 7O0, such as Sorensen's buffer diluted 1:10, and the resulting solutions are filtered through a column loaded with a weak ion exchanger molecular sieve type gel having weak ion exchanging properties, for instance a polyacrylamide gel, such as Bio-Gel P-2 (defined below), the column being equilibrated with a similar buffer of pH about 7Ø The fraction showing antigen activity is found to be the first fraction of the solution leaving the column, said fraction being recovered.
The recovered fraction from the chromatography on Bio-Gel P-2 above is subjected to a particular procedure developed for the purpose of further purification of the CAPA. In principle, this procedure comprises the following steps: A mixture of proteins or conjugated proteins is precipitated by isoelectric adjustment of pH. The precipitate hereby obtained is mixed with a suitable gel selected while considering the protein mixture at handO The resulting mixture of precipitate and gel is layered on top of a column containing an identical gel of the same isoelectric pH9 iOe. the pH
which is isoelectric for the proteins to precipitate same in the previous stepO The column is then subjected to elution under gradually increasing or decreasing pH~ In the eluate the fraction or fractions recovered are those containing ~he desired protein or proteins. Although the process of the invention is not to be bound by any particular theory -it is believed that the separation of molecular species of the protein mixture can be explained in the following way:
The precipitated proteins are exposed to a flow of ions which brings one protein after another in solution.
The time required for solubilization of the various proteins will depend on the ionic strength, pH, temperature, and the flow rate. Since the distribution coefficient of each dissolved protein is lower than that of the ionic gradient, the protein will travel faster in the gel than will the gradient. In consequence, the protein will reprecipitate and become stationary until redissolved by the approaching ionic front. Tnis process repeats itself an idefinite number of time~ thus effecting separation of molecular species differing only slightly from each other.
Bio-Gel P2 is a crosslinked polyacrylamide (100-200 ;
mesh) having a molecular weight exclusion limit of about 2000, but this exclusion limit is not critical. Other useful gels are cross-linked dextran gels, such as Sephadex G-25, -which has a molecular weight exclusion limit of about 25,000, but this exclusion limit is not cri~tical. These gels are of the molecular sieve type and are as usual employed in bead form. Any such molecular sieve type gel having molecular weight exclusion limits of at least about 2-3000 may be employed satisfactorilyO For a review of molecular sieve type gels suitable for gel filtration in combination with --gradient elutlonJ in accord with the invention, see Gellotte, Fractionation of Proteins3 Peptides and Amino Acids by Gel Filtration, in "Mew Biochemical Separations", Van Nostrand, London/New York 1964 _9_ . . . . , . ", . , . , :
. - , . . , , . :, ~ . ~ .

. ].75,~'35 The normal and CAPA Fractions recovered from ~he chromatography above are subJected to active substance precipitation at pH about 5, the sediment being recovered and dissolved in water having a pH of about ~.5. The pH
of the clear solutions is then brought to an acidic pH, suitably about 5.0 with formic acid, this treatment resulting in precipitation. Each precipitate is mixed with a slurry of a ~ ~
similar gel as above equilibrated with HCOOH-HCOONH4 at a pH ;-of about 5Ø Each of these mixtures is placed on top of a gel column equilibrated as above.
For the elution of the precipitates a pH gradient was used, in this case having a progressively decreasing pH.
A suitable buffer system is HCOOH-HCOONH~ and NH4HC03-N~3.
The antigen activity is found in the effluent within the pH
range from the initial pH to about 3.
The effluent fraction recovered within the above-identified pH-range contains the desired CAPA, ~irhich may be recovered by freeze drying. In order to establish the molecular weight of the CAPA of said effluent fraction the fraction may be subjected to filtration on a gel column equilibrated with HCOOH-HCOONHL~ at a pH of about 3.0, the gel being selected from those mentioned above, Bio-Gel P-30 (Trademark for a polyacrylamide gel from Bio-Rad Laboratories, Munchen, West Germany; 100-200 mesh exclusion limit (Daltons) 40,000, fractionation range (Daltons) 2,500-40,000), and Sephadex G-75 or G-50 (Trademarks for dextran gels from Pharmacia Fine Chemicals, Uppsala, Sweden; ~0-120 and 50-150 microns, fractionation range 3-70,000 and 1-30,000, respectively) being particularly suitable gels for carrying out this filtration. The eluted fractions of CAPA having a spectrophotometric absorption peak wavelength within the range about 229 to about 233 nm and a molecular weight of from about 20,000 to about 27,000 are recovered.
The CAPA may be recovered from the active fraction after filtratlon by freeze drying and may be stored for a long time in vacuum, cold and in the dark.
The isolated material consists of a polypeptide based on a single peptide chain as shown by treatment with performic acid. The CAPA shows basic reaction and is soluble at a pH within the range of about 1-3.5. The unprotected polypeptide denaturates irreversibly at neutral pHs, namely at pHs exceeding about ~ 5. The antigen is hygroscopic, turns yellow and becomes inactivated and smeary when it takes up moisture.
The purified CAPA contains a fluorescent group, said group being subject to activation at a wavelength of about 2g~ nm while emitting light at a wavelength of about 350 nm. The fluorescence is proportional to the CAPA
quantity and may be used to determine the presence of polypeptide during the procedure for its isolation.
The CAPA shows spectrophotometric peak absorption at a wavelength within the range from about 229 to about 233 nm. Moreover, it shows great ten~encies to aggregation and is not filtratable on normal filter media used for sterilization. It has been established that the CAPA
originates from the cancer cell walls, since antibodies generated by injecting the CAPA into a living animal body cause complete lysis or decomposition of cancer cells in -vivo when such cells are subjected to the effect of such antibodies.
As indicated above the polypeptide has a molecular weight within the range 20,000 to 27,000, more particularly :.
, : :

about 2~000. Analyses indicate that it does not contain any carbohydrate and spectrophotometry indicates that the CAPA
is free from nucleic acids. Analyses made with amino acid analyzer with and without oxidation indicate agreement with the molecular weight as estimated by the gel filtration on Bio-Gel P 30 or its equivalent.
The isolated CAPA may be used in many applicationsJ
such as in the preparation of monospecific antibodies, for diagnostic purposes, for immunization procedures, as an active ingredient in compositions useful as immunizing agents.
In connection with the preparation of antibodies monospecific with regard to the cancer associated polypeptide antigen, a new process has been developed. As indicated above the unprotected CAPA denaturates irreversibly at neutral pHs, which means that injecting an acidic solution of the CAPA into a living animal body results in denaturation of the CAPA immediately when it comes into contact with the neutral body fluids. In order to prevent such denaturation an oil emulsion is prepared, wherein an aqueous solution of the CAPA at a pH within the range from about 2 to about 3 constitutes the enclosed phase surrounded by the oil phase.
On injecting suc~ oil emulsion into a living animal body the acidic aqueous solution of the CAPA is protected by the surrounding oil phase when it comes into contact with the neutral body fluids. In this way the CAPA maintains its activity in vivo and may be carried to the antibody-producing cells.
An approach of maintaining antigen activity in vitro at neutral pHs resides in complexing the CAPA with inert proteln, such as human or bovine albumin. By making use of such approach a complcx is formed which is soluble ak neutral pHs while maintaining the antigen activity in vitro.
~ith regard to cancer diagnosis a modified hemaggluti-nation inhibition technique has been developed. This technique enables determining the presence of CAPA at different stages of cancer progress by investigating materials of interest, such as patient sera, tissues, secretions and extracts from living animal bodies including e~g. biopsy material, ,urgical specimens, punctions and smears. This new modified hemagglutination inhibition technique resides in a method comprising the steps:
a) preparing a series of samples of the material subject to investigation by serial dilution;
b) adding to each of said samples a predetermined amount of antiserum containing antibodies specific to the CAPA;
c) adding, after incubation, to each of said - -incubated samples a predetermined amount of CAPA supported by a particulate carrier;
d) comparing the resulting series of treated samples with a row of control samples of decreasing known amounts of CAPA providing inhibition and predetermined amounts of antiserum containing said antibodies and thereafter adding to each of said control samples a predetermined amount of CAPA ~supported by a similar particulate carrier; -and e) establishing by comparison of said sample series and said control sample row the amount of CAPA in the material investigated to find , -~ ~. . .: , out the presence of cancer and its state of progress.
The invention also ~rovides for a compositlon useful as an immunizing agent active in vivo, said composition comprising the CAPA as defined herein together with a pharmaceutically acceptable carrier.
The invention will now be further described by means of the following non-limiting examples.
Example I.
Isolation of pure anti~en.
Since it has been shol~n (Int.Arch.Allergy 36; 191-203 (1969), "Systematic Antigenic Change in Human Carcinoma Tissues by Hemagglutination Techniques", by B. Bjorklund) that most cancer tissue contains the antigen of this invention7 cancer tissues of various types and from various sites were collected to make up a tumor pool. In this case the pool was made up from macroscopically pure, histologically verified carcinomatous tissues from the following organs (autopsy): ~reast, bronchus, caecum, colon, duodenum, gall bladder, kidney, larynx, liver, lung, oesophagus, ovary, pancreas, prostate, rectum, stomach, uterus. Normal tissues were collected from a number of individuals to establish a pool of isoantigens, tissue antigens and individual antigens. Autopsy cases were used and the tumor dia~gnoses were histologically verified. Moreover, it was established that the pertinent tumor antigen was intact because of immunological cross-reactivity with fresh tumor tissues and live tumor cells.
Aseptic precautions were maintained wherever possibleO
The carcinomatous and normal tissues from autopsies were separately trimmed clear of adjacent tissue and cut in 2-3 cm cubes which were washed in 0.9 ~ NaCl at 0C until they no longer gave off blood stain. The washed cubes were frozen and stored at -2~Co While still in the frozen state, the tissue cubes ;'', _ ~75,~'~5 were mixed with 10 ml H20 at 0C for each gram of froæen tissue and homo,enized in a chilled MSE Ato-Mix homogenizer with rotating knives at "half-speed" for three periods of one minute. In this connection it should be observed that the temperature of the suspension should be kept at about 0C, preferably slightly below said temperature.
The cold homogenate was poured into cold 1000 ml polythene bottles. L~00 ml suspension and L~00 ml ethylether at -20C ("Aether ad narcosin PH Nord., cont. diphenylamine 0.002 ~, from Skanska Bomullskrutfabriken AB, Dosjebro, Sweden) were mixed in each bottle and agitated at -2C for 120 minutes in an TM
International PR-2 centrifuge shaking-attachment at motor speed ~ ~
300 RPM. The mixture was centrifuged at 1000 x G at -2C for -5 minutes. During this step the lipid layer does not mix with the tissue layer. The ethyl ether and the lipid were discarded and a second extraction was carried out for 60 minutes followed by centrifugation for 5 minutes and removal of ether-lipid layer.
Finally, centrifugation at 1000 x G at -2C was carried out for 30 minutes and the ~er layer was removed although it contained 20 some CAPA. The remaining insolubles were saved. The residual -ethyl ether was removed by application of vacuum for 5 minutes.
The antigenic material was suspended in 50 ml H20 at 0C, transferred to 500 ml infusion bottles and shell-frozen at -70C (dry ice and ethanol).
Lyophilization was carried out in a Texvac, Type IV A (Tr~) lyophilizer (Textor, Bad Soden, Taunus, West-Germany), at controlled temperature.
The lyophilized tissue powder was ground in a stainless steel ball mill ("Cytolator",TMLars Lj~mgberg Company, Stockholm, Sweden) at a temperature of about -70C for 2 hours at L~0 RPM.
The grinding resulted in a fine, grayish-brown powder. This powder was extracted with pre-chilled ethylether at -2C in a PR-2 shaking device at 300 RP~l for 60 minutes and centrifuged at :

1000 x r at -2C for 30 minutes. The ether layer w~s removed and the sedlment ~as dried in vacuo. The resultin~ crude tissue powder (CTP) cl~n be stored for years at 4C in closed bottles without appreciable loss of activity.
Five grams of CTP were suspended at neutral PH in 500 ml of saline containing sterile cubes of ice. The suspension was homogenized in a MSE Ato-mix at "half speed" for 3 periods of 1 minute. The temperature was kept a-t 0C. The mixture was kept at 0C for 30 minutes at slow stirring. Centrifugatlon was carried out at 1009 x G at 0C ~or 49 minutes. The supernatant was discarded.
The sediment was resuspended in 500 ml cold distilled water and stirred slowly at 0C for 30 minutes, Following centri-fugation at 1090 x G at 0C for 40 minutes, the supernatant was discarded. The remainlng sediment was suspended in 25 ml cold distilled water and shell-frozen at -70C (dry ice and ethanol).
~yophilization resulted in a washed tissue powder (l~TP) which can be stored for years in closed bottles at l~C.
Aqueous extracts of CAPA and normal I~TP at pH 9.5 were made and concentrated ten tlmes by isoelectric precipitation at pH 4.~ and dissolving the precipitate in one tenth of the volume of water of pH 9.5. The resulting concentrate is stabilized by rapid heating to a temperature of 9~-100~ and maintaining said temperature for 5-10 minutes. This heat treatment destroys enzymes, which otherwise would inactivate the CAPA. The stabilized extract became turbid upon the addition of saline at pH 7.5 due to precipitation of remaining contaminants of nucleic acid characterO To precipitate such remaining contaminants ~.0 ml of CAPA and normal aqueous extracts were separately precipitated by the addition of 0.~ ml 10 ~0 solution of NaCl. After centri- ~ -1~396SO
fugation at 27~000 x G at O C for 1 hour, the clear super-natants were precipitated iso-electrically at pH 4.8 (pH
adjustment with 0.1 N HCl or 0.1 N HCOOH). The precipitates were dissolved ln 2-3 ml M/150 phosphate bufferJ pH 7Ø
The resulting solutions originating from tumor and normal WTP were filtered with Bio-Gel A-50m (as hereinbefore defined) in refrigerated columns having an inner diameter of 2.50 cm and a length of 138 cm, at a flow rate of 6.~ ml/cm2/h.
The gel was equilibrated with M/150 phosphate buffer of pH 7.0 with 2 % N butanol and eluted with the same buffer. In each run, 4-8 ml Or extract, containing a total amount of 50-100 mg of protein were used.
The antigen activity was found in the mid-fraction of the effluent of the tumor extract. 1.0 ml aliquots of this fraction, totalling 160-180 ml, were diluted three times and adjusted to various pH-values ranging from 2.0 to 9Ø After 5 minutes at room temperature the samples were transferred to cuvettes and their llght scatter at 500 nm was measured at an angle of 90. The scatter intensities plotted against pH
indicated a maximum at pH 4.8, said pH being the iso-electric polnt of the fraction. This method is a new technique developed for the purpose of determining the exact and necessary conditions for the purification of the CAPA. Conventional technique for the determination of the iso-electric point cannot be used here in view of the low concentration of peptide.
The remaining part of the active mid-fraction was pre-cipitated at pH 4.8 with the aid of 0.1 N HCl. Centrifugation at ~,80~ x G at 0C for 5 minutes resulted in a quantitative yield of activity.
~0 To effect further purification of the CAPA the sedi-mented, active mid-fractions from five Bio-Gel A-50m columns were dissolved in M/150 phosphate bu~fer solution of pH 7.0 (Sorensen's huffer in 2 % N-butanol~ to 5 % of the orlginal effluent vo]ume. This solution containing 130 mg protein in ~.5 ml was filteted through a Bio-Gel P-2 column (as herein~
before defined) with a ratio diameter/height of 1/35 and at a flow rate of 35 ml/cm2/h. The column had been equilibrated with M/150 phosphate buffer of pH 7.0 (Sorensen's buffer in 2 ~
~-butanol). For each mg of protein a bed volume of 10 ml was permitted.
The first fraction was active and was excluded with the eluting buffer of pH 7.0 while impurities were absorbed on the gel at the low ionic strength used. The active substance was precipitated at pH h.~ with 0.1 M HCOOH and centrifuged at 3,~00 x G at 0C for 5 minutes. The sediment was dissolved in ~.5 ml H20 and the pH adjusted to ~.5 with 0.1 M NH~OH. The clear solution was reprecipitated three times with 0.1 M HCOOH at pH 4.~, washed in the centrifuge at the same pH and dissolved at pH ~.5. The disappearance of M-butanol was followed by gas-liquid chromatography. The final solution was stored in ampoules, shell-frozen and lyophilized. The resulting product was a dry, almost white powder and this powder was stored at -24C in the evacuated and sealed ampoules, An identical procedure was employed with a corresponding extract originating from normal tissue and no activity was found.
For further purification of the product obtained from the previous chromatographic procedure, a pE~ gradient elution process was developedO This process resides, in principle, in the following steps: Protein mixture to be purified with regard to the active component thereof is precipitated by an isoelectric adjustment of pHo The precipitate is mixed with a suitable gel, ,, . , . - : .

_ 175,995 such as Sephadex G-25 ~as hereinbefore defined) or Bio-Gel P-2 ~as hereinbefore defined). This mixture is layered on top of a column containing an identical gel Or the same iso-electric pH. The column is then subjected to pH-gradient elution under constant flow rate and tempera~ure. Thus~ the column-is eluted with a medium of continuously or stepwise increasing or decreasing pH.
The instant case gradient elution was carried ou~ with 15 mg of lyophilized and salt-free CAPA powder and normal antigen powder purlf~ed as described in the preceding seckion, in this case by decreasing pHs. The powders ~ere separately dissolvred in H20~ the pH being adjusted to 8.5 with 0.1 N NH~OH. The pH
of the clear solutions was then brought to 5.0 with 0.1 M HCOOH
which resulted in precipitation. Each precipitate was mixed with 10 ml Bio-Gel P-2 slurry equilibrated with an aqueous solution prepared from 0.02 M HCOOH and 0.02 M HCOONH4 to make a pH of 5Ø Each of these mixtures was placed on top of a 15 ml Bio-Gel P-2, silicon-treated column, having an inner diameter - ` of 16 mm and a length of 150 mm~ equilibrated as above. The gel was supported by a small piece of glass-wool.

A pH-gradient was used for elution of the precipitates.
TM
By means of a gradient mixer (Ultrograd,LKB9 Sweden) the pH was kept at about 5 for 2 short period of time to wash the precipitate and then the pH was gradually lowered to 2.8.
Finally, the pH was raised to 9. The buffer system comprised 0.02 M HCOOH - HCOONH4 and 0.02 M NH4HCO~ - NH~ and the elution was made at room temperature. The flow rate was held at 27.2 mls per square cm column cross-section per hour.
The effluent from the tumor extract was assayed by fluo-rescence spectrometry (activation at 288 nm~ fluorescence emitted at 350 nm). The fraction eluted between the initial pH and .~ .

- . -- .. -- - . .......... . .. ... ....... .

about ~ was recovered for furth~r use. After lyophilization and freeze-drying the product could be stored in sealed ampoules after removal of air at -24C.
For characterization of molecular size and to con-firm the purity9 the antigenic material in the form cf solutions thereof were filtered with Bio-Gel P-~O (as here~
inbefore defined) which had been equilibrated with a buffer 0.02 M HCOOH - HCOONH49 pH 3Ø The pH-eluted CAPA was dissolved in a small amount of the same bufferO The flow rate was ~.25 ml/cm2/hour and the fractions collected comprised 1.24 ml. The active fractions showed a spectrophotometric absorption maximum at a wavelength of 229-2~3 nm and a fluorescence of 350 nm when activated at 2~8 nm.
In a typical run, 10.4 mg of CAPA dissolved in 3 ml of the above buffer on a siliconized Bio-Gel P-30 column (i.d. 2.54 cm9 length 50 cm), resulted in complete recovery of both substance and activity. The elution volume was compatible with a MW within the range 22gOO0~249000~ These molecular weight figures were obtained by comparing the elution volumes with those of compounds of known MWs, such as ribonuclease and insulin. Rfter freeze-drying there is obtained a white hygroscopic powder which can be stored in the cold and in the absence of light and oxygen. Upon analyzing the product no carbohydrate and no nucleic acids are found. Analyses by amino acid analyzer indicated agreement with molecular weight as estimated by gel filtration. Analyses of the amino acids show the following mole percentages3 the figures being of an accuracy of + 5 %: The calculated molecular weight was 2~9200 + 2,500 (Standard deviation).

: . : ., .: , . . .

.
Al,~nine ~.62 Arginine L~.57 Asp~rtic acid10.3~
Cystelne 0.95 Glut~mic acidL7.0 Glycine 6~7 Histidine 1.00 Isoleucine L~.75 Leucine 10.49 Lysine 3.69 Methionine 1.91 Phenylalanine2.75 Proline 3.79 Serine 7.7L~
Threonine 5.92 Tyrosine 3.21 Valine ~,3~ -This amino acid content corresponds to a theoretical nitrogen content of 1~.2 - 17.g ~. Determination of total nitrogen according to Dumas' points to a value of 17.0 + 0.5 %. ~ ~
As shown by treatment with performic acid the polypeptide is -based on a single peptide chain. Moreover, the polypeptide, if not protected by complexing with albumen, denaturates irreversibly at pHs exceeding about 50 ~-Exa,m,p,l,e Ia.
In exactly the same manner as described in Example I
above the polypeptide is prepared from human placenta tissue.
Example Ib.
Preparation of CAPA-albumen complexO
An aliquot of the CAPA as prepared under Example I is dissolved in formic acid (for instance 0.05M; the pH should be within the range 2-3). A clear solution is obt~ined. To said solution there is added albumen powder or a solution of albumen at the same pH as of the above formic acid solution (200 parts by weight of albumen per 1 part by weight of 5APA) resulting in a clear solution of CAPA and albumen. Then the pH of the solution is slowly increased by adding a base (for instance an aqueous sodium hydroxide solution or ammonia) until pH
reaches about 7.5. This results in a clear solution containing CAPA and albumen in the form of a complex.
This solution containing 12 ~g CAPA/ml may be used directly in the diagnostic procedure described below or the complex may be isolated in the form of a white powder by freeze-drying. The powder is stable in the cold (+~C) for a long period of time.
It has been shown by experiments that maximum utilization of the CAPA activity is obtained at a weight ratio of albumen to CAPA equal to about or exceeding 200 Example Ic.
;::
Preparation of tanned and labelled red blood cells! ~
.
Fresh sheep blood (1 part by volume) are added to sterile Alsever's solution tlo2 part by volume) (Alsever's -~
solution is prepared from 250 g glucose, ~0 g sodium citrate dihydrate, ~2 g NaCl~ add water to make up to 10 liters~ -pH adjusted to 6.1 with 10 % citric acid monohydrate)O The mixture is centrifuged and the red blood cells are resuspended once in Alsever's solution and twice in a buffer solution of pH 6~o Finally, a suspension of the red blood cells is made up in the buffer 6.~ at a concentration of 109 cells/ml.
1 volume of red blood cell suspension prepared as above is added to 1 volume of buffer solution of pH 6.

containing about 1~ lug tannic acid/ml under stirring. The thus tanned/blood cells are centrifuged and resuspended twice in buffer of pH 7.5. Finally, the red blood cells are suspended in buffer of pH 7.5 at a concentration of 109 cells/ml.
An aliquot of the CAPA complex prepared under Example Ib above is dissolved in a buffer solution of pH 7.5 to give a concentration of 3 lug CAPA per ml (calculated on pure CAPA). l part by volume of the suspension of tanned red blood cells prepared above is added dropwise at 0C to l part by volume of the CAPA complex solution for a period of time of lO minutes. The labelled cells are centrifuged and resuspended in a buffer solution of pH 7.5 containing a stabilizing amount (about 1.2 volume/volume) of inert human serum to give a suspension containing 1.6 x lO~ labelled cells per ml. These labelled cells are used as shown below in the diagnostic procedure of the invention.
Example II.
Preparation of antibodies.
In view of the fact that the CAPA of the invention denaturates irreversibly at neutral pHs as hereinbefore indicated, it was suspected that parenteral injection of the polypeptide would not result in the production of antibodies.

~xperiments carried out on rabbits confirmed this and it was found that no antibody production occurred after the injection of polypeptide complexed ~ith albumen into rabbits. ~11 hemmaggluti-nation reactions were negative.
In order to be able to transfer the polypeptide in an active condition to the antibody producing cells it is necessary to maintain the polypeptide in the solution at pHs lower than about 3 (0.02 m HCOOH, pH 2.~) and to emulgate the solution in oil to the formation of extremely small drops surrounded by a protecting oil layer. The injection of the emulsion resulted in production of satisfactory quantities of antibodies, which reacted specifically with the CAPA in hemagglutination reactions, wherein blood cells had been labelled with CAPA.
Preparation of immunizin~ ~ent. ~16 micrograms of pure CAPA prepared from pooled human cancer tumors were dissolved in 1.0 ml 0002 m HCOOH of pH 2.g. To the resultin~ solution there was added dropwise 1.0 ml adjuvant oil (commercial preparation from Difco Laboratories, De-troit, Mic~gan, USA; Bacto-Adjuvant9 Freund) under simultaneous emulsificationO The emulsification was carried out according to Freund by means of an injectlon syringe, the mixture beinO drawn up and down in the syringe to the formation of a uniform, white emulsion having about the same consistency as wipped cream. One drop of said emulsion was tested with ice water to confirm that it floated separately and maintained intact. The resulting, semi-liquid emulsion was used for subcutaneous and intramuscular injections on rabbits Immunization of five rabbits. In the first injection a so-called complete adjuvant was used and in the subsequent injections a so-called incomplete adjuvant was used. After initial drain of blood from each of five rabbits to establish O-values, -2~-- . ~ . , ~ ; . , ~ , totally ll0~ micro~rams of enu]sified C~PA at pH 2.~ were injected subcutaneously on each rlght and left hand side. At ten days intervals additionally three injections were given, the first one intramuscularly in each hind leg and the second and the third subcutaneOUSly on both front sides and both backs, respectively.
The selection of the injection sites was made in order to utilize the admission areas of the regional lymphatic glands. In total, each rabbit received about 106 mgs of CAPA in the form of emulsion. 14 and 24 days after the last injection test samples of blood were taken, which were subjected to hemagglutination analysis with regard to the presence of specific antibodies against CAPA. Two days after the last sample a maximum amount of blood was drained, which was recovered in the form oF serum that was sterile filtered and transferred in small portions to sterile tubes. These tubes could be stored in the cold while maintaining the speci~icity.
Example III.
Dia~nostic procedure.
a) Single blind study.
Blood samples were obtained from the Central Hospital -of Eskilstuna, SwedenJ of which ~2 originated from patients of the infection clinic;one from the surgical clinic; two from radiotherapy; ten from post partus women; ten from ~mbilical cord blood and ten from women pregnant in l-trimester and six in 2-trimester. Moreover, blood was obtained from twenty 10 year old children from Slottsskolan and ten samples from older healthy adults from the private clinic of DrO Iundstrom in ~skilstuna, SwedenO From the surgical and medical clinics of Ersta Sjukhus in Stockholm, Sweden, there were obtained samples from fortyfour patients, from Akeshovs Hospital, samples were obtained from fortyfive pat;ents and from the surgical clinic of Karolinska Sjukhuset in Stockholm-, Sweden, there were obtained blood samples from seventytwo patients admitted for ~, possible surgery. The Blood Donor Department of Karolinska Sjukhuset in Stockholm, Sweden9 provided llg samples from donors of ages ranging from 20-67 years9 average age 37.2 years (SD + 11.3 years), and from the Clinical Central Laboratory of said hospital sera were obtained from 29 patients subject to care within the general divisions of ~adiumhemmet in Stockholm, Sweden, and from twelve patients within its gynaecological divisions. -The total number of blood samples was 431. With ~ ~ ;
regard to the 111 cases from Eskilstuna a clinical investigation was made and a medical record was drafted except for the participants of obvious health. As regards the medical records were Stockholm cases, detailed studies of patients~/made with regard to 101 cases. In the remaining cases other clinical diagnoses than malignancy were at hand and there was no suspicion of malignant disease.
Venous blood l~as transferred to Wassermann tubes without additive and was transferred to the laboratory, in and some cases after the removal of coagulum /blood cells by means of centrifugation.
The blood analysis was based on indication of the -existence of 5APA by means of a modified hemagglutination inhibition technique (micromethod). In principle, the following procedure was used:
which had been absorbed with sheep red cells, 25 ~1 of patient serum,/was titrated in g steps 2-dilution in Linbro IS-MRC-96 dilution plates, and then 25 ~1 of specific antiserum in limit dilution (about 1:2000) was added to each cavity. After incubation at 225 for .~
-26- ~ ~

, 10 minutes there was added to each cavity 50 ~1 of a suspension of about 6-~ million sheep blood red ce]ls tanned and labelled with isolated CAPA linked to human albumen as shown under Example Ic above (about 2-~ ~g ~er 109 blood cells). Other particulate carriers, such as latex~
bentonite, and collodion, can be employed instead of the -~
red blood cells. The reaction was recorded by means of an inclined mirror and a standard series after 4-24 hours incubation at 1-2C. For control purposes, use was made of:
1. CAPA labelled blood cells plus antiserum;
2. CAPA labelled blood cells without antiserum;
3. Patient serum plus blood cells labelled with human albumen;
4. Patient serum and untreated blood cells;
5. CAPA labelled blood cells and antibodies in one ~ -row where inhibition is provided by stepwise decreasing known amounts of CAPA.
The dilution liquids used contained -pooled (i.e. combined from many individuals) inactivated neutral human serum for the stabilization of the blood cellsO
CAPA-reagent was prepared from pooled human carcinoma tissues and was purified as described above by means of gel filtration, pH-gradient elution, filtering through Bio-Gel P-30 and complexing with albumen.
As antiserum there was used horse anti-HeLa from 19 November,1962, absorbed by normal tissues and pooled human serumO The immunization was made with washed fragments of HeLa-cells grown in Eagle's medium containing 20 % inactivated human serum in flat glass bottlesO The cells had been harvested with EDTA, centrifused and washed three times with water.

:

1039~50 In the pr~-~sence of CAP~ in patlent serum, the horse ' ~ntibodie~ were neutrali~ed resulting in the absence of agglutinatlon when the po1ypeptide labelled blood cells were subsequently added. Recording was rnade after an increasing score from 0-6, wherein 0 indicates absence of inhibition and
6 indicates maximum inhibition of the agglutination. The , ~ -relation between the scores and the concentration of CAPA
per ml of serum is seen from Table 1 obtained by calibration of dilutions of predetermined amounts of CAPA in neutral serum.
Table 1.
Approximative calibration of scores and quantit~ of CAPA.
Score ~g CAPA/ml ... . . ~ . _ _ ....... . .
0 ~ 0003 ~',' 1 O.OL~ - O.Og 2 0.09 - 0.12 ' 3 0.13 - 0.2 0~25 - 0.~9 0.50 ~ -99 6 > 1.0 The recordings were made without knowledge of the health con- ~-ditions of the patients. The material subject to investigation ' has been grouped as seen from Table 2 below. ~ ' Table 2.
The presence of CAPA in ~31 sera from individuals of different groups according to an integer score from 0 to 6 and average scores (M) and standard deviations (SD)o ' --2g--... _ . . .. . .
Groups Integer score 0 1 2 3 4 5 6Number M +SD -1. Primary cancer 5 4 1 2 12 3.00 + 1.13 with metastases 2. Extended cancer 4 2 1 4 8 2 1 22 2.91 + 1.82 3. Cancer not 6 10 15 8 39 1.64 +0.99 radically treated 4. Primary cancer 3 1 4 2 10 1.50 + 1.18 untreated 5. Cancer radi-cally removed 19 1 1 21 0.14 ~ 0.19 -6. Malignant 7 3 1 11 0.45 +0.68 :- -disease other :
than cancer ~ '
7. Non-malignant 118 3 3 7 1 132 0.26 + 0.22 disease
8. Healthy adults 8 2 10 0.20 + 0.42 (M = 71 years)
9. Blood donors 116 2 118 0.02 + 0.13 (M = 39 years)
10. 10-year old19 1 20 0.10 +0.44 individuals
11. Newly born 1 1 1 4 2 1 10 2.80 +1.48 (umbilical cord blood)
12. Pregnant women 12 2 2 16 0.38 ~ 0.72
13. Women post 8 1 1 10 0.40 +0.97 partus It is clear from the results that the highest scores have been obtained with the groups comprising "primary cancer and metastasses"
(local) and by "extended cancer" and group "newly born"
(umbilical cord blood).
Low scores have been obtained for blood donors. An intermediate position is taken by the group "Primary cancer untreated" and the group "cancer not radically treated". Scores about the same as those of the blood donors are found within the group "cancer radically removed".
The average values as to CAPA in all groups have been compared pair-wise and are shown in Table 3 below.
Table 3.
Statistic significance a)of differences between scores for presence in sera of CAPA of nine categories of individuals.

.
Significance bJ of difference Groups between categories number M + SD 2 3 4 5 6 7 8 9 :
1. Primary Cancer 3.00 + 1.13 0 ~x~x ~x~ ~x~ xxx xx~ xx~
with metastases 2. Extended cancer 2. 91 + 1.82 3~3~ x3~ 3~x3~ 3~x3~ xx3~ 3~xX

3. Cancer, not radi- 1. 64 + 0.99 0 xxx xx xxx xxx xxx cally treated 4. Primary cancer, 1. 50 + 1.18 xxx x xxx xx xxx untreated 5. Cancer radically 0.14 -+ 0.19 0 0 0 0 removed 6. Malignant disease 0.45 -+ 0.68 0 0 0 other than cancer 7. Non-malignant 0. 26 -+ 0.22 0 xxxC) disease 8. Old healthy 0.20 +- 0.42 0 adults 9. Blood donors 0.02 +- 0.13 a) Significance tests of differences were made by means of an approximatively normal distributed variable, Z, defined as:

Z = `- :

\ / SD1 SD2 V n1 ~2 b) if Z > 1.96 the significance of difference is ~, which means 0.01 < P < 0.05 " Z > 2.6 " " " " is ~, which means O.001 < P < O.01 " Z > 3.5 " " ~' " is ~x-, P < 0.001 c) This group includes 11 positive tests of which 8 refer to suspected but not verified cancer.
It is clear from the table above that with regard to "primary cancer with metastases" as well as for "extended cancer"
there are significantly higher average scores relative to all of the other groups with the exception, however, for newly born (see also Table 2).
Fo~ the groups "cancer not radically treated" as well as "primary cancer untreated" the average scores are significantly higher relative to all groups except the two first-mentioned and relative to "malignan~ disease other than cancer" relative to which the difference is significant (0.01 < P < 0.05).
-Groups 5-9 do not show mutual significant differences except for the significant differences between 7 and 9. This difference may be explained by the fact that genuine, hidden cancer causes may be present among the cases showing sc~res between 1 and 4.
The positive indication in umbilical cord blood deserves certain attention. In order to establi~sh whether the CAPA
originates from placenta, pieces of such tissue were extracted.
Amounts of 300 mgs of frozen placenta tissue per ml buffered physiological NaCl solution at pH 7.5 were homogeni~ed at 0C and centrifuged at 1000 x G for 30 minutes at 0C in conically extended tubes (according to Markham). The super-natants were tested for presence of CAPA by means of the hemagglutination tec'lni~ue descril)e(l ,lbove, To exlclldc the por;sihility -that -the in}libi-tion reactinns obtained ~ere causecl by unsl?ecific ;nactivation of the pure C~A applied to the hlood cclls, said hlood cells were s}laken a~ter each recording and a standard amount of antibodies specific to -the CArA wasadded~ .~io anti~oen inacti-vation could be indicated in any of the cases. ~s control material there was used an extract of ant;gen powder produced from human cancer tissues of different origin and from different localizations.
The results show, that out of 26 placentas from as many indi-viduals all without exception contained significant quantities of C~PA. The average figure (geometrical) for the 26 placentae was 297 ~ 8 micrograms per gram wet tissue (0.0390).
Since as is clear from the above investi~ation that the ~:
C~PA of this invention is synthetized in the placenta, and since the genes contained in the placenta must be present also in the ;ndividual originating from the same ovum cell, it follows that the ability or capacity to ~enerate the CAPA is a normal phenomenon. Normally, this capacity is repressed since normal cells do not contain the CAPA in measurable amounts. In cancer cells, however, an activation of the capacity has occurred characterized by a significant presence of CAPA within and about the cells. The antigenic and to some extent functional similarity between trophoblast cells of the placenta and cancer cells and the difference with regard to the other cells of the individual seems compatible with the view that the cancer diseases are due to `-changed control of inherent properties.
A statistical analysis of the experimental results shows that there is a highly significant correlation between the presence of cancer diagnosis and increased CAP~ concentration (P ~C 0.001). The same holds true for the relation between the -~

_ 32 :. ' , . .

`- 1039650 size of the -tu~r ~ass considere(l ~nd the increa~sed !'~
concentration wit}lin the same a~e groups (P C 0.001). The increased concen-tration of CAPA has been follnd in connection w;th a large variety of difFerent localizations of cancer.
Irrespective of tvpe and localization cancer tumors have been found to contain the CAPA in view of which said CAPA seems to be common to all known types of cancer, i.e mali~nant tumors of epithelial ori~in.
b) Double blind study.
In order to attest further to the validity of the above conclusions, a double blind study was performed under the most rigidly controlled conditions. Coded blood specimens were obtained from the various depar-tments of the Central Hospital of Eskilstuna, Sweden. In this case quantita-tive measurements of the CAP~ level of the patient's sera were made.
The results from this double blind study as well as the results from the fore-~,oing s1ngle blind study are summarized in tables 4-8 below. In said tables:
Table 4 shows the total number of examined individuals and the number of individuals showing cancer dia~nosis;
Table 5 shows the numbers of individuals of the different ~roups to~ether with their average ages and the deviations thereof;
Table 6 shows the presence of CAPA in the sera from all examined patients;
Table 7 shows the percentage of individuals havin~ a CAPA concentration of ~O.l5~g/ml serum while excluding ~roups 9, 10 and 12 of table 5.
Table~8 shows the presence of C~PA in relation to tumor localizations for groups ]-3 of table 5. The site numbers refer to _ 33 "Cancer Incidence in Sweden 1968"

Table 4.
Number of examined individuals. : .
....

Studies Number of Number of individuals individuals s~lowing cancer diagnosis .,, ,~,. . . .
Single blind 431 104 Double blind 503 49 -~
._ . :
934 153 .. : :
: , .:

. , , - ,~ ~ . -. . .

Table 5 Number of individuals of different groups and average ages and deviations thereof.

Groups Single blind study Double blind study Num- Average Devi- Num- Average + Devi-ber age -+ ation ber age - ation 1. Cancer with 34 72 -+ 9 14 66 -+ 10 metastases 2. Untreated cancer 49 67-+ 11 14 66 -+ 12 without metastase indications and cancer not radi-cally treated 3. Cancer radically 21 66+ 15 21 64 -+ 12 removed 4. Malignant disease 11 70-+ 7 5 58 -+ 18 other than cancer 5. Non-malignant132 61 -+22 186 46 -+ 21 disease 6. Healthy adults 10 71+ 5 46 36 -+ 14 7. Blood donors118 38 -+11 8. 10 year old and 20 1û + 0 62 2 -+ 1.5 younger indi-viduals 9. umbilical cord 10 0 - 0 20 0 - 0 blood 10. Women post partus 10 21 - 3 20 25 - 4 + 4 110 26 -+ 4.5 11. Pregnant women 16 26 12. Cancer in situ - - - 5 27 + 6 Total431 503 , .

Table 6 :.
Presence of CAPA in sera from 934 individuals.

Groups CAPA CAPA Total ::
c 0.08 ,ug/m æ~ O.09 ~ug/ml Number (Do) ` Number (O) Number (O) ~ :.
~' 1. Cancer with 9 (19) 39 (81) 48 (100) metastases 2. Untreated cancer 28 (44) 35 (56) 63 (100) without metastase indications and cancer not radi-cally treated 3. Cancer radi- 36 (86) 6 (14) 42 (100) ~ .
cally removed 4. Malignant disease15 (94) 1 (6) 16 (100) other than cancer 5. Non-malignant269(85) 49 (15) 318 (100) ~ .
disease 6. Healthy adults 54 (96) 2 (4) 56 (100) 7. Blood donors118(100) 0 (0) 118 (100) ~ :

8. 10 year old 7g (96) 3 (4) 82 (100) :-and younger individuals 9. umbilical cord blood 21 (70) 9 (30) 30 (100) ~ :-10. Women post partus25 (83) 5 (17) 30 (100) 11. Pregnant women 123 (98) 3 (2) 126 (100) 12. Cancer in situ 4 (80) 1 (20) 5 (100) -. .
Total781 (84) 153 (16) 934 (100) Table 7 Percentage of individuals showing a CAPA concentration of O.15.
Groups 9, 10 and 12 of Table 5 have been excluded.

Groups O Number -1. Cancer with metastases 64 48 2 . Untreated cancer without 21 63 metastase indications and cancer not radically treated 3. Cancer radically 10 42 removed _ . _ . . .
4. Malignant disease 0 16 other than cancer 5. Non-malignant 6 318 disease 6. Healthy adults 0 56 7. Blood donors 0 118 8. 10 year old and 0 82 yoynger individuals 11. Pregnant women 1 12 6 Total 869 ..
.

l~?a;~e6~ii.0 Presence of CAPA in relation to tumor localizations of groups 1-3.
. . Site l.Cancer 2.Untreated 3. Cancer Total Locallzatlon xx with cancer radically No meta- without meta- removed stases stases indi-cations and cancer not radically treated _ - -<0 08`0.09 ~0.08 ~o.og c 0.08 ~0.09 Gingivae Mandib. 144 1 _ 1 _2 Nasopharynx 146 2 1 3 Oesophagus 150 _ 1 3 1 1 6 Ventricle 151 12 1 2 2 8 Intestinum 152 tenui Colon 153 2 1 _ 7 _6 16 Rectum 154 4 1 5 3 1 14 Ves.Fellea,etc. 155 1 1 1 3 --Hepar 156 Pancreas 157 3 1 2 6 Vestibul. 160 1 1 2 nasi, etc.
. -Trachea, 162 4 2 3 5 14 -pulm etc.
Mamae 170 27 1 3 3 2 ~8 -Cervix uteri 229 2 3 1 6 CorPus uteri 198 11 1 1 1 2 7 Ovarii, etc. 175 14 1 1 2 9 Prostate 177 23 3 i 9 Testis 178 1 1 1 3 Penis, etc. 179 1 1 2 Renes 180 1 _ 3 _ 1 5 Ves.urinaria, 181 1 2 3 3 1 10 , .
Malignant 190 I 1 2 melanoma _ , .
Th~eoidRa 194 ~ 1 1 2 _ 5 Primary tumor origin unknown _1 1 ~i Total 939 28 35 36 6 153 .
x) According to "Cancer Incidence in Sweden 1968". :

~39650 A thorough statistical analysis of the data obtained in this double blind study again shows the highly signiricant correlation between the presence of cancer diagnosis and increased CAPA concentration (P ~ O~OOl)o This double blind study also confirms the relation between the size of the tumor rnass considered and the increased CAPA concentration within the same age groups (P ~ 0.001). The increased serum level of CAPA has been found in connection with about 20 different types and localizations of cancer. Thus, the double blind study fully confirms the validity of the new findings and tneir practical use~ulnessO
In the introductory part of this disclosure it has been indicated that the antigen disclosed in U.S. patent 3,663,684 is clearly different from the antigen of this invention. To demonstrate the diff'erence between the prior art antigen and the antigen of the invention there is given below a detailed sur~ey on some specific differences both with regard to the process of antigen isolation and with regard to the characteristics of the antigen.

~039650 CEA . . CAPA
_ . _ . _ _ . . _ . _ . . .
Source: C~ncer of the colon Source All czncers, cancer Fetus (Mekonium, gut) cell lines in vitro, placenta.
(Little if any in fetus).
. . _ Extraction from the Washing the tissue with water antigen-containing tissues at neutral pHg extraction by glycoprotein solvent at with ethyl tther (optional)g low pH at room temperatureo throw away the extract~
Keep extract. Extraction of solids at high pH (9.5), keep the extract, temperature in the water treatmento ~C 0C.
Isoelectric point: Isoelectric point:
Not given or non-existing About 5 (before final step) . _ . _ . . _ 15 Absorption of UV-light at Absorption of UV-light at 280 ~m 2~0 nm (very little at 280 nm) Fluorescence: Fluorescenceo Not mentioned Activation at 288 nm Emission at 350 nm _ _ _ _ .. _ . . . .... . ...... _ . _ Molecular weight 200,000 Molecular weight 2~200 + 2g500 (may be as low as 70,000) .~. . . __ . , Active at neutral pH Destroyed at neutral pH
. _ ~
Contains sugar No sugar by gas-liquid (glycoprotein) chromatography and mass spectroscopy and oth~r analyses . .
No inhibition of antibodies Inhibits specific antibody to CAPA by hemagglutination by hemagglutination . _ . .. . .. .. _ ~039650 CEA CAPA
Does not label sheep red Does label such cells.
cells treated with tannic acid.
. _ _ _ _ _ Is present ln cancer disease Present in serum in in concentrations from some concentrations of o.og-8 nanograms to 100-200 nm per ml 1ug/ml (equivalent of 90-8,000 ng/ml), i.eO
approximately 20 times higher than CEA.
. _ . . . . _ Assayo Expensive, time-con- Easy, rapidg inexpensive, sumingg requires radioactive no isotopesg no expensive isotopes. equipment required.

To summarize there are given below brief definitions of cancer associated polypeptide antigen and the diagnostic test of this invention.
Definition of CAPA.
HeLa cells (originating from a case of cancer in 1952) are grown in vitro. These cells are used as 2 source Gf antigen. The harvested cells are injected into horses resulting in the production of specific antibody which is used to identify the antigen in tumorsg serumg placenta etc.
The latter antigen must have and does have an identical immunological reaction site (as compared to the HeLa-antigen) but can, of course9 be different in other respects when present in a natural state.
Definition of diagnostic test. -Antigen from HeLa cell cultures in vitro is used to produce antibody in horses. After absorption of unwanted 0 antibodies, the horse serum is used to agglutinate red cells - . - . . - , ... .... .. . . . . .

labelled by antigen taken out of tumors (or placenta or cell cultures of HeLa or HEp-2 or Detroit-6). This is the indicator system. If an unknown sample contains antigenic activity it will interfere with the antib3dy and does inhibit agglutination.
Various mGdif~ications and equivalents will be apparent to those skilled in the art and can be made in the processes and the products of the present invention without departing fro~ the spirit of scope thereof~ and it is, therefore, to be understood that the invention is to be limited only by the scope of the appended claims.

TB/On -42-Fig. 1 Purification of tumor associated antigen Flow chart with conditional branching illustrat~ng the general approach of purification.

Tumor tissues _ . r Normal ~L ~,~
Separation ~ . .
procedure ~ ~ .
¦ Immunological ~:
comparison ~ I . ~

-1~.,. . ,~ :
/ Is there a difference \ y s No ------- ~ between tumor and normal? ~ e .~ ~ - -.;~ ~ ' .' ,~
-No ~ ~ Is the difference ~ Yes -- \ tumor plus? / I .
~ J :-No ~ Yes ~ ~
t L ~ -modify and repeat¦ 1---- LAdopt procedurq ::
,..~
/ Is the CAPA \
No ~ pure? Yes : -. 1 '','.~

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Claims (23)

What is claimed is:-
1. A process for the isolation of a cancer associated polypeptide antigen (CAPA) comprising the steps:
a) homogenizing CAPA-containing material in a liquid at a temperature not above about 0°C
b) separating solids from the mixture of liquid homogenate and solids resulting from step a) c) extracting said solids with an alkaline aqueous solution and heat stabilizing the product by rapidly heating at a temperature sufficient to destroy enzymes destructive to the CAPA but not sufficient to destroy the CAPA itself;
d) filtering the extract resulting from step c) on a filtration gel of the molecular sieve type in bead form permitting fractionation of compounds having a molecular weight range including 10.106 to 20.106, especially about 15.106, eluting the gel and re-covering the 10.106 to 15.106, fraction, especially the fraction of about 15.106 e) subjecting the fraction resulting from step d) to chromatography on a weak ion exchanger to adsorb thereon impurities and recovering the first fraction leaving said exchanger;
f) subjecting said first fraction to isoelectric precipitation;
g) mixing the resulting precipitate with a molecular sieve type gel and subjecting said gel to pH-gradient elution; and, h) while decreasing the pH, recovering the fraction down to pH about 3 containing CAPA therein having a spectrophotometric absorption peak wave length at 229-233 nm and a molecular weight within the range of about 20,000 - 27,000.
2. A process according to claim 1, wherein the fraction resulting from the pH-gradient elution is subjected to gel filtration on a gel column, the eluted fractions of antigen having a spectrophotometric absorption peak wave length at 229-233 nm and a molecular weight within the range of about 20,000 - 27,000 being recovered.
3. A process according to claim 1, wherein the homogenate resulting from step a) is subjected to organic solvent treatment in the cold before step b).
4. A process according to claim 3, wherein the solvent used is ethyl ether.
5. A process according to claim 1, wherein the homogenization is carried out in water at a temperature not above about 0°C.
6. A process according to claim 1, wherein the solids resulting from step b) are lyophilized and then ground in a steel ball mill in the cold.
7. A process according to claim 6, wherein the grinding takes place at low temperature below 0°C.
8. A process according to claim 6, wherein the grinding takes place at a temperature below the freezing point of the material under treatment.
9. A process according to claim 6, wherein the grinding takes place at a temperature of about - 70°C.
10. A process according to claim 1, wherein under step d) the filtering is carried out on a gel selected from the group consisting of polyacrylamide gels, cross-linked dextran gels, agar and agarose gels, the gel being equili-brated with phosphate buffer at about pH 7.
11. A process according to claim 1, wherein under step e) the chromatography is carried out on a column of a weak ion exchanger at neutral pH.
12. A process according to claim 11, wherein the chromatography is carried out on a weak ion exchanger polyacrylamide gel, said gel being in the form of a column at a neutral pH.
13. A process according to claim 1, wherein under step g) there is used a gel selected from the group consisting of polyacrylamide gels, cross-linked dextran gels, agar and agarose gels.
14. A process according to claim 2, wherein said gel filtration is carried out on a gel selected from the group consisting of polyacrylamide gel and cross-linked dextran gel.
15. A process according to claim 1, wherein the aqueous extract resulting from step c) is subjected to rapid heating to a temperature within the range of about 95 to about 100°C to destroy enzymes.
16. A process according to claim 15, wherein said aqueous extract is rapidly heated to a temperature within the range of about 98-100°C and maintained at said temperature for about 5-10 minutes.
17. A process for the preparation of CAPA comprising:
homogenizing antigen-containing material while still in the frozen state, in water at a temperature not above about 0°C;
subjecting the resulting homogenate to treatment with a solvent selected from the group consisting of ethyl ether and acetone;

separating solids from the resulting mixture of liquid homogenate and solids;
lyophilizing the resulting solids and grinding same in a steel ball mill at a temperature below the freezing point of the material under treatment;
extracting the resulting solids with an alkaline aqueous solution and, after centrifugation, subjecting the supernatant liquid to rapid heating to a temperature within the range of about 95 to about 100°C for a period of about 5 to about 10 minutes to destroy enzymes; treating the heated supernatant with an aqueous sodium chloride solution to precipitate contaminants and recovering the supernatant liquid;
filtering the resulting liquid on a cold column loaded with a molecular sieve type gel in bead from having a fractionation range including 10-106 to at least 20.106 and equilibrated with phosphate buffer at about pH
7.0 and recovering the active fraction of the eluate;
subjecting said active fraction to chromatography on a column loaded with a weak ion exchanger molecular sieve type gel equilibrated with phosphate buffer of about pH 7.0 and recovering the first fraction of the liquid leaving the column;
subjecting said first fraction to isoelectric pre-cipitation at about pH 5 and mixing the resulting precipitate with a molecular sieve type gel having a molecular weight exclusion limit of at least about 2000 equilibrated with HCOOH-HCOONH4 at about pH 5, applying the resulting mixture on top of a column loaded with an identical gel equilibrated in the same way, pH-gradient eluting the column and, while decreasing the pH, recovering the fraction eluted down to about pH 3 containing the CAPA having a spectrophotometric absorption peak wave length at 229-233 nm and a molecular weight of 23,200 ? 2,500 (S.D.).
18. Cancer associated polypeptide antigen (CAPA) having a spectrophotometric absorption peak wave length at 229 - 233 mm and a molecular weight within the range of about 20,000 - 27,000; whenever prepared or produced by the process defined in claim 1, 2 or 15 or by the obvious chemical equivalent.
19. Cancer associated polypeptide antigen (CAPA) having a spectrophotometric absorption peak wave length at 229 - 233 mm and a molecular weight of 23,200 ? 2,500; whenever prepared or produced by the process defined in claim 17 or by the obvious chemical equivalent.
20. A process for preparing antibodies monospecific with regard to CAPA, comprising the steps:
(a) preparing an aqueous solution at a pH less than about 3 of the CAPA as claimed in claim 18;
(b) preparing an oil emulsion, wherein the solution resulting from step a) is enclosed phase so as to be protected by the surrounding oil phase;
(c) injecting said oil emulsion into a living animal body, whereby the CAPA carried by the emulsion is transported to antibody-producing cells.
21. A process according to claim 20 wherein under step b) a Freund's adjuvant is used for preparing the oil emulsion.
22. A process according to claim 20 wherein under step a) the aqueous solution is prepared at a pH lower than about 3 using as an acidifying agent a weak acid.
23. A process according to claim 22 wherein the weak acid used is formic acid.
CA175,995A 1972-07-10 1973-07-09 Cancer associated polypeptide antigen, process for its preparation, process for preparing antibodies, process of cancer diagnosis and composition useful as an immunizing agent Expired CA1039650A (en)

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US4132769A (en) * 1974-10-30 1979-01-02 Osther Kurt B Cancer antigen, cancer therapy, and cancer diagnosis
US4146603A (en) * 1977-02-18 1979-03-27 Research Corporation Tumor specific glycoproteins and method for detecting tumorigenic cancers
US4172124A (en) * 1978-04-28 1979-10-23 The Wistar Institute Method of producing tumor antibodies
JPS56145297A (en) * 1980-04-11 1981-11-11 Kureha Chem Ind Co Ltd Preparative method of glycoprotein having immunosupressing activity
EP0087898A1 (en) * 1982-02-22 1983-09-07 Cancer Research Campaign Technology Limited Antibodies and antigens useful in the diagnosis and treatment of cancer

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BE802126A (en) 1973-11-05
DE2333740A1 (en) 1974-01-31
ZA734632B (en) 1974-06-26
CH617853A5 (en) 1980-06-30
NL7309257A (en) 1974-01-14
GB1443054A (en) 1976-07-21
IN138903B (en) 1976-04-10
ES416726A1 (en) 1976-06-16
FR2191885A1 (en) 1974-02-08
IL42594A (en) 1976-08-31
DD113918A5 (en) 1975-07-05
JPS56115954A (en) 1981-09-11
DE2366609C2 (en) 1988-02-25
SE440597B (en) 1985-08-12
JPS5817168B2 (en) 1983-04-05
DD118946A5 (en) 1976-03-20
FR2191885B1 (en) 1977-07-01
AU5728673A (en) 1975-01-09
BR7305142D0 (en) 1974-08-22
JPS6018011B2 (en) 1985-05-08
SE418186B (en) 1981-05-11
SU581842A3 (en) 1977-11-25
SE7609836L (en) 1976-09-06
IL42594A0 (en) 1973-08-29
IT1009527B (en) 1976-12-20
DE2333740C2 (en) 1987-01-22
GB1443053A (en) 1976-07-21
NO146338C (en) 1982-09-08
DK139898B (en) 1979-05-14
JPS4955823A (en) 1974-05-30
SE7609837L (en) 1976-09-06
FI60567C (en) 1982-02-10
AT336780B (en) 1977-05-25
FI60567B (en) 1981-10-30
NO146338B (en) 1982-06-01
AR197243A1 (en) 1974-03-22
SE440697B (en) 1985-08-12
ATA600773A (en) 1976-09-15
DK139898C (en) 1979-10-08

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