CA2532866A1

CA2532866A1 - Use of protein sahh as a marker for colorectal cancer

Info

Publication number: CA2532866A1
Application number: CA002532866A
Authority: CA
Inventors: Michael Tacke; Peter Berndt; Marie-Luise Hagmann; Johann Karl; Hanno Langen; Stefan Palme; Markus Roessler; Wolfgang Rollinger; Werner Zolg
Original assignee: Individual
Current assignee: F Hoffmann La Roche AG
Priority date: 2003-08-07
Filing date: 2004-08-05
Publication date: 2005-02-17
Also published as: EP1654539A1; WO2005015221A1

Abstract

The present invention relates to the diagnosis of colorectal cancer. It discloses the use of protein SAHH (S-adenosylhomocysteine hydrolase) in the diagnosis of colorectal cancer. It relates to a method for diagnosis of colorectal cancer from a stool sample, derived from an individual by measuring SAHH in said sample. Measurement of SAHH can, e.g. be used in the early detection or diagnosis of colorectal cancer.

Description

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Use of protein SAHH as a marker for colorectal cancer The present invention relates to the diagnosis of colorectal cancer. It discloses the use of the protein SAHH (= S-adenosylhomocysteine hydrolase) in the diagnosis of colorectal cancer. Furthermore, it especially relates to a method for diagnosis of colorectal cancer from a stool sample, derived from an individual by measuring SAHH in said sample: Measurement of SAHH can, e.g., be used in the early detection or diagnosis of colorectal cancer.
Cancer remains a major public health challenge despite progress in detection and therapy. Amongst the various types of cancer, colorectal cancer (= CRC) is one of the most frequent cancers in the Western world.
The earlier cancer can be detected/diagnosed, the better is the overall survival rate.
This is especially true for CRC. The prognosis in advanced stages of tumor is poor.
More than one third of the patients will die from progressive disease within five years after diagnosis, corresponding to a survival rate of about 40% for five years.
Current treatment is only curing a fraction of the patients and clearly has the best effect on those patients diagnosed in an early stage of disease.
With regard to CRC as a public health problem, it is essential that more effective screening and preventative measures for colorectal cancer be developed.
The earliest detection procedures available at present for colorectal cancer involve using tests for fecal blood or endoscopic procedures. However, significant tumor size must typically exist before fecal blood is detected. With regard to detection of CRC from a stool sample, the current state of the art is the guaiac-based fecal occult blood test.
In the recent years a tremendous amount of so-called colon specific or even so-called colorectal cancer specific genes has been reported. The vast majority of the corresponding research papers or patent applications are based on data obtained by analysis of RNA expression patterns in colon (cancer) tissue versus a different tissue or an adjacent normal tissue, respectively. Such approaches may be summarized as differential mRNA display techniques.

As an example for data available from mRNA-display techniques, WO 01/96390 shall be mentioned arid discussed. This application describes and claims more than two hundred isolated polynucleotides and the corresponding polypeptides as such, as well as their use in the detection of CRC. However, it is general knowledge that differences on the level of mRNA are not mirrored by the level of the corresponding proteins. A protein encoded by a rare mRNA may be found in very high amounts and a protein encoded by an abundant rnRNA may nonetheless be hard to detect and find at all. This lack of correlation between mRNA-level and protein level is due to reasons like mRNA stability, efficiency of translation, stability of the protein, Z O etc.
There also are recent approaches investigating the differences in protein patterns between different tissues or between healthy and diseased tissue in order to identify candidate marker molecules which might be used in the diagnosis of CRC.
Briinagel, G., et al., Cancer Research 62 (2002) 2437-2442, have identified seven nuclear matrix proteins which appear to be more abundant in CRC tissue as compared to adjacent normal tissue. No data from liquid and stool samples obtained from an individual are reported.
WO 02/078636 reports about nine colorectal cancer-associated spots as found by surface-enhanced laser desorption and ionization (SELDI). These spots are seen more frequently in sera obtained from patients with CRC as compared to sera obtained from healthy controls. However, the identity of the molecules) comprised in such spot, e.g., its (their sequence), is not known.
Despite the large and ever growing list of candidate protein markers in the field of CRC, to date clinical/diagnostic utility of these molecules is not known. In order to be of clinical utility a new diagnostic marker as a single marker should be at least as good as the best single marker known in the art. Or, a new marker should lead to a progress in diagnostic sensitivity and/or specificity either if used alone or in combination with one or more other markers, respectively. The diagnostic sensitivity and/or specificity of a test is best assessed by its receiver-operating characteristics, which will be described in detail below.
At present, for example, diagnostic blood tests based on the detection of carcinoembryonic antigen (CEA), a tumor-associated glycoprotein, are available to assist diagnosis in the field of CRC. CEA is increased in 95% of tissue samples obtained from patients with colorectal, gastric, and pancreatic cancers and in the majority of breast, lung, and head and neck carcinomas (Goldenberg, D.M., et al., J.
Natl. Cancer Inst. (Bethesda) 57 (1976) 11-22). Elevated CEA levels have also been reported in patients with nonmalignant disease, and many patients with colorectal cancer have normal CEA levels in the serum, especially during the early stage of the disease (Carriquiry, L.A., and Pineyro, A., Dis. Colon Rectum 42 (1999) 921-929;
Herrera, M.A., et al., Ann. Surg. 183 ( 1976) 5-9; Wanebo, H.J., et al., N.
Engl. J.
Med. 299 (1978) 448-451). The utility of CEA as measured from serum or plasma in detecting recurrences is reportedly controversial and has yet to be widely applied (Martell, R.E., et al., Int. J. Biol. Markers 13 (1998) 145-149; Moertel, C.G., et al., JAMA 270 ( 1993) 943-947).
In light of the available data, serum CEA determination possesses neither the sensitivity nor the specificity to enable its use as a screening test for colorectal cancer in the asymptomatic population (Reynoso, G., et al., JAMA 220 (1972) 365; Sturgeon, C., Clinical Chemistry 48 (2002) 1151-1159).
Samples taken from stool have the advantage that such sampling is easily possible by non-invasive means.
As mentioned above, the guaiac test is currently most widely used as a screening assay for CRC from stool. The guaiac test, however, has both poor sensitivity as well as poor specificity. The sensitivity of the guaiac-based fecal occult blood tests is ~26%, which means 74% of patients with malignant lesions will remain undetected (Ahlquist, D.A., Gastroenterol. Clin. North Am. 26 ( 1997) 41-55). The visualization of precancerous and cancerous lesions represents the best approach to early detection, but colonoscopy is invasive with significant costs, risks, and complications (Silvis, S.E., et al., JAMA 235 ( 1976) 928-930; Geenen, J.E., et al., Am. J. Dig. Dis. 20 ( 1975) 231-235; Anderson, W.F., et al., J. Natl. Cancer Institute 94 (2002) 1126-1133).
The sensitivity and specificity of diagnostic alternatives to the guaiac test have been recently investigated by Sieg, A., et al., Int. J. Colorectal Dis. 14 ( 1999) 267-271.
Especially the measurement of hemoglobin and of the hemoglobin-haptoglobin complex from stool specimen have been compared. It has been noted that the hemoglobin assay has an unsatisfactory sensitivity for the detection of colorectal neoplasms. Whereas cancer in its progressed carcinoma stage is detected with a sensitivity of about 87% the earlier tumor stages are not detected with a sufficient sensitivity. The hemoglobin-haptoglobin complex assay was more sensitive in the detection of earlier stages of CRC. This more sensitive detection was accompanied by a poor specificity. Since poor specificity, however, translates to a high number of unnecessary secondary investigations, like colonoscopy, an assay with a poor accuracy also does not meet the requirements of a generally accepted screening assay.
A further alternative method to the guaiac test for detection of CRC in stool has been published recently and consists in the detection of the colorectal cancer-specific antigen, "minichromosome maintenance protein 2" (MCM2) by immunohistochemistry in colonic cells shed into stool. Due to the small study size, conclusion on the diagnostic value for detection of colorectal cancer is preliminary.
However, the test seems to have only limited sensitivity to detect right-sided colon cancer. (Davies, R.J., et al., Lancet 359 (2002) 1917-1919).
The identification of an early CRC tumor marker that would allow reliable cancer detection or provide early prognostic information by non-invasive means from a stool specimen could lead to a diagnostic assay that would greatly aid in the diagnosis and in the management of this disease. Therefore, an urgent clinical need exists to improve the diagnosis of CRC, especially from stool. It is especially important to improve the early diagnosis of CRC, since for patients diagnosed early on chances of survival are much higher as compared to those diagnosed at a progressed stage of disease.
It was the task of the present invention to investigate whether a new marker can be identified which may aid in CRC diagnosis. Preferably such marker would be present in stool and allow for a non-invasive diagnosis.
Surprisingly, it has been found that use of protein SAHH can at least partially overcome the problems known from the state of the art.
The present invention therefore relates to a method for the diagnosis of colorectal cancer comprising the steps of a) providing a stool sample obtained from an individual, b) contacting said sample with a specific binding agent for SAHH
under conditions appropriate for formation of a complex between said binding agent and SAHH, and c) correlating the amount of complex formed in (b) to the diagnosis of colorectal cancer.
In a preferred embodiment the stool sample is processed to obtain a processed sample liquid which is more convenient to handle than a stool specimen. Such processed sample is then incubated with the specific binding agent for SAHH.
The present invention therefore also relates to a method for the diagnosis of colorectal cancer comprising the steps of a) providing a stool sample obtained from an individual, b) processing said sample to obtain a processed liquid sample, c) contacting said processed liquid sample with a specific binding agent for SAHH
under conditions appropriate for formation of a complex between said binding agent and SAHH, and d) correlating the amount of complex formed in (c) to the diagnosis of colorectal cancer. A preferred method uses a stool sample obtained from an individual.
Another preferred embodiment of the invention is a method for the diagnosis of colorectal cancer comprising the steps of a) processing a stool sample obtained from an individual to obtain a processed liquid sample b) contacting said processed liquid sample with a specific binding agent for SAHH under conditions appropriate for formation of a complex between said binding agent and SAHH, and c) correlating the amount of complex formed in (b) to the diagnosis of colorectal cancer.
In another preferred embodiment the stool sample is processed to retrieve colonycytes which are then smeared on a microscopic slide. Such processed sample is then incubated with the specific binding agent for SAHH. The present invention therefore also relates to a method for the diagnosis of colorectal cancer comprising the steps of a) providing a stool sample obtained from an individual, b) processing said sample to retrieve colonycytes, c) contacting said processed sample with a specific binding agent for SAHH under conditions appropriate for formation of a complex between said binding agent and SAHH, and d) correlating the amount of complex formed in (c) to the diagnosis of colorectal cancer.

The protein SAHH (S-adenosylhomocysteine hydrolase; SWISS-PROT: P23526) is characterized by the sequence given SEQ ID NO: 1. The corresponding cloned human cDNA encodes for a 48-kDa protein which catalyzes the following rerversible reaction: S-adenosyl-L-homocysteine + H2O ~ adenosine + L-homocysteine (Cantoni, G.L., Annu. Rev. Biochem. 44 (1975) 435-451).
Hershfield, M.S., and Francke, U., Science 216 (1982) 739-742, located the corresponding gene to chromosome 20 and later on Coulter-Karis, D.E., and Hershfield, M.S., Ann.
Hum. Genet. 53 ( 1989) 169-175, sequenced the full-length cDNA. Recently, the structure of SAHH has been resolved (Turner, M.A., et al., Cell. Biochem.
Biophys.
33 (2000) 101-125).
S-adenosyl-L-homocysteine is formed by the donation of a methyl group of S-adenosylmethionine, a universal methyl donor, to a methyl acceptor (e.g. DNA).
Subsequently, it is hydrolyzed to adenosine and L-homocysteine by SAHH.
Inhibition of SAHH results in accumulation of cellular S-adenosyl-L-homocysteine, which acts as feedback inhibitor on most methylation reactions (Chiang, P.K., Pharmacol. Ther. 77 (1998) 115-134). Since methylation of nucleic acids and phospholipids is crucial in cellular growth, differentiation and carcinogenesis (Chiang, P.K., et al., FASEB J. 10 (1996) 471-480; Cui, Z., et al., J. Biol.
Chem. 269 ( 1994) 24531-24533; Szyf, M., et al., Pharmacol. Ther. 70 ( 1996) 1-37), inhibitors of SAHH are an interesting pharmacological target. Consequently, there are a number of inhibitors of SAHH described as reviewed in Chiang, P.K., Pharmacol. Ther.

(1998) 115-134.
A deficiency in SAHH is one of the different causes of hypermethioninemia, a disease associated with failure to thrive, mental and motor retardation, facial dysmorphism, and myocardiopathy (Labrune, P., et al., J. Pediatr. 117 ( 1990) 226).
Immunoblotting techniques were used to determine SAHH levels in hepatic tissues (Bethin, K.E., et al., J. Biol. Chem. 270 ( 1995) 20698-20702).
As obvious to the skilled artisan, the present invention shall not be construed to be limited to the full-length protein SAHH of SEQ ID NO:1. Physiological or artificial fragments of SAHH, secondary modifications of SAHH, as well as allelic variants of SAHH are also encompassed by the present invention. Artificial fragments preferably encompass a peptide produced synthetically or by recombinant techniques, which at least comprises one epitope of diagnostic interest consisting of at least 6 contiguous amino acids as derived from the sequence disclosed in SEQ ID
NO:1. Such fragment may advantageously be used for generation of antibodies or as a standard in an immunoassay. More preferred the artificial fragment comprises at least two epitopes of interest appropriate for setting up a sandwich immunoassay.
In preferred embodiments, the novel marker SAHH may be used for monitoring as well as for screening purposes. Its use for screening purposes is most preferred.
When used in patient monitoring the diagnostic method according to the present invention may help to assess tumor load, efficacy of treatment and tumor recurrence in the follow-up of patients. Increased levels of SAHH are directly correlated to tumor burden. After chemotherapy a short term (few hours to 14 days) increase in SAHH may serve as an indicator of tumor cell death. In the follow-up of patients (from 3 months to 10 years) an increase of SAHH can be used as an indicator for tumor recurrence in the colorectum.
In a preferred embodiment the diagnostic method according to the present invention is used for screening purposes. Le., it is used to assess subjects without a prior diagnosis of CRC by measuring the level of SAHH in a stool sample and correlating the level measured to the presence or absence of CRC.
Colorectal cancer most frequently progresses from adenomas (polyps) to malignant carcinomas. The different stages of CRC used to be classified according to Dukes' stages A to D.
The staging of cancer is the classification of the disease in terms of extent, progression, and severity. It groups cancer patients so that generalizations can be made about prognosis and the choice of therapy.
Today, the TNM system is the most widely used classification of the anatomical extent of cancer. It represents an internationally accepted, uniform staging system.
There are three basic variables: T (the extent of the primary tumor), N (the status of regional lymph nodes) and M (the presence or absence of distant metastases).
The TNM criteria are published by the UICC (International Union Against Cancer), _g_ Sobin, L.H., Wittekind, Ch. (eds): TNM Classification of Malignant Tumours, fifth edition, 1997.
What is especially important is, that early diagnosis of CRC translates to a much better prognosis. Malignant tumors of the colorectum arise from benign tumors, i.e. from adenoma. Therefore, best prognosis have those patients diagnosed at the adenoma stage. Patients diagnosed as early as in stage Tis, N0, MO or T1-3;
N0; M0, if treated properly have a more than 90% chance of survival 5 years after diagnosis as compared to a 5-years survival rate of only 10% for patients diagnosed when distant metastases are already present.
In the sense of the present invention early diagnosis of CRC refers to a diagnosis at a pre-malignant state (adenoma) or at a tumor stage where no metastases at all (neither proximal nor distal), i.e., adenoma, T;S, N0, MO or T1-4; N0; MO are present. T;S denotes carcinoma iii situ.
In a preferred embodiment the detection of SAHH is used to diagnose CRC as early as in the adenoma stage.
It is further preferred, that CRC is diagnosed when it has not yet fully grown through the bowel wall and thus neither the visceral peritoneum is perforated nor other organs or structures are invaded, i.e., that diagnosis is made at stage T;S, N0, MO or T1-3; N0; MO (=T;~-3; N0; MO).
The diagnostic method according to the present invention is based on a stool sample which is derived from an individual. The stool sample is extracted and SAHH is specifically measured from this processed stool sample by use of a specific binding agent.
A specific binding agent is, e.g., a receptor for SAHH, a lectin binding to SAHH or an antibody to SAHH. A specific binding agent has at least an affinity of 10' 1/mol for its corresponding target molecule. The specific binding agent preferably has an affinity of 108 1/mol or even more preferred of 1091/mol for its target molecule. As the skilled artisan will appreciate the term specific is used to indicate that other biomolecules present in the sample do not significantly bind to with the binding agent specific for SAHH. Preferably, the level of binding to a biomolecule other than the target molecule results in a binding affinity which is only 10%, more preferably only 5% of the affinity of the target molecule or less. A most preferred specific binding agent will fulfill both the above minimum criteria for affinity as well as for specificity.
A specific binding agent preferably is an antibody reactive with SAHH. The term antibody refers to a polyclonal antibody, a monoclonal antibody, fragments of such antibodies, as well as to genetic constructs comprising the binding domain of an antibody.
Any antibody fragment retaining the above criteria of a specific binding agent can be used. Antibodies are generated by state of the art procedures, e.g., as described in Tijssen (Tijssen, P., Practice and theory of enzyme immunoassays 11 ( 1990) the whole book, especially pages 43-78; Elsevier, Amsterdam). In addition, the skilled artisan is well aware of methods based on immunosorbents that can be used for the specific isolation of antibodies. By these means the quality of polyclonal antibodies and hence their performance in immunoassays can be enhanced. (Tijssen, P., supra, pages 108-115).
For the achievements as disclosed in the present invention polyclonal antibodies raised in rabbits have been used. However, clearly also polyclonal antibodies from different species , e.g. rats or guinea pigs, as well as monoclonal antibodies can also be used. Since monoclonal antibodies can be produced in any amount required with constant properties, they represent ideal tools in development of an assay for clinical routine. The generation and use of monoclonal antibodies to SAHH in a method according to the present invention is yet another preferred embodiment.
As the skilled artisan will appreciate now, that SAHH has been identified as a marker which is useful in the diagnosis of CRC, alternative ways may be used to reach a result comparable to the achievements of the present invention. For example, alternative strategies to generate antibodies may be used. Such strategies comprise amongst others the use of synthetic peptides, representing an epitope of SAHH for immunization. Alternatively, DNA Immunization also known as DNA
vaccination may be used.

For measurement, the stool sample is obtained from an individual. An aliquot of the stool sample may be used directly. Preferably an aliquot of the stool sample is processed to yield a liquid sample.
The stool sample is preferably used or processed directly after sampling or stored cooled or more conveniently stored frozen. Frozen stool samples can be processed by thawing, followed by dilution in an appropriate buffer, mixing and centrifugation. Supernatants are used as liquid sample for subsequent measurement of marker SAHH.
An aliquot of the processed stool sample is incubated with the specific binding agent for SAHH under conditions appropriate for formation of a binding agent SAHH-complex. Such conditions need not be specified, since the skilled artisan without any inventive effort can easily identify such appropriate incubation conditions.
As a final step according to the method disclosed in the present invention the amount of complex is measured and correlated to the diagnosis of CRC. As the skilled artisan will appreciate there are numerous methods to measure the amount of specific binding agent SAHH-complex all described in detail in relevant textbooks (c~, e.g., Tijssen P., supra, or Diamandis, E.P., et al., eds.
(1996) Immunoassay, Academic Press, Boston).
Preferably SAHH is detected in a sandwich type assay format. In such assay a first specific binding agent is used to capture SAHH on the one side and a second specific binding agent, which is labeled to be directly or indirectly detectable is used on the other side.
As mentioned above, it has surprisingly been found that SAHH can be measured from a stool sample obtained from an individual sample. No tissue and no biopsy sample is required to apply the marker SAHH in the diagnosis of CRC.
Whereas application of routine proteomics methods to tissue samples, leads to the identification of many potential marker candidates for the tissue selected, the inventors of the present invention have surprisingly been able to detect protein SAHH in a stool sample. Even more surprising they have been able to demonstrate that the presence of SAHH in such stool sample obtained from an individual can be correlated to the diagnosis of colorectal cancer.
Antibodies to SAHH with great advantage can also be used in established procedures, e.g., to detect colorectal cancer cells in situ, in biopsies, or in immunohistological procedures.
Preferably, an antibody to SAHH is used in a qualitative (SAHH present or absent) or quantitative (SAHH amount is determined) immunoassay.
Measuring the level of protein SAHH has proven very advantageous in the field of CRC. Therefore, in a further preferred embodiment, the present invention relates to use of protein SAHH as a marker molecule in the diagnosis of colorectal cancer from a stool sample obtained from an individual.
The term marker molecule is used to indicate that an increased level of the analyte SAHH as measured from a bodily fluid or especially a processed stool sample obtained from an individual marks the presence of CRC.
It is especially preferred to use the novel marker SAHH in the early diagnosis of colorectal cancer.
The use of protein SAHH itself, represents a significant progress to the challenging field of CRC diagnosis from stool. Combining measurements of SAHH with other known markers, like hemoglobin or the hemoglobin-haptoglobin complex, or with other markers of CRC yet to be discovered, leads to further improvements.
Therefore in a further preferred embodiment the present invention relates to the use of SAHH as a marker molecule for colorectal cancer in combination with one or more other marker molecules for colorectal cancer in the diagnosis of colorectal cancer from a stool sample obtained from an individual. Preferred selected other CRC markers with which the measurement of SAHH may be combined are hemoglobin and/or the hemoglobin-haptoglobin complex. Very preferred the marker SAHH is used in combination with hemoglobin. Also very preferred the marker SAHH is used in combination with the hemoglobin-haptoglobin complex.

Diagnostic reagents in the field of specific binding assays, like immunoassays, usually are best provided in the form of a kit, which comprises the specific binding agent and the auxiliary reagents required to perform the assay. The present invention therefore also relates to an immunological kit comprising at least one specific binding agent for SAHH and auxiliary reagents for measurement of SAHH.
Accuracy of a test is best described by its receiver-operating characteristics (ROC) (see especially Zweig, M. H., and Campbell, G., Clin. Chem. 39 (1993) 561-577).
The ROC graph is a plot of all of the sensitivity/specificity pairs resulting from continuously varying the decision thresh-hold over the entire range of data observed.
The clinical performance of a laboratory test depends on its diagnostic accuracy, or the ability to correctly classify subjects into clinically relevant subgroups.
Diagnostic accuracy measures the test's ability to correctly distinguish two different conditions of the subjects investigated. Such conditions are for example health and disease or benign versus malignant disease.
In each case, the ROC plot depicts the overlap between the two distributions by plotting the sensitivity versus 1 - specificity for the complete range of decision thresholds. On the y-axis is sensitivity, or the true-positive fraction [defined as (number of true-positive test results) (number of true-positive + number of false-negative test results)]. This has also been referred to as positivity in the presence of a disease or condition. It is calculated solely from the affected subgroup. On the x-axis is the false-positive fraction, or 1 - specificity [defined as (number of false-positive results) / (number of true-negative + number of false-positive results)]. It is an index of specificity and is calculated entirely from the unaffected subgroup.
Because the true- and false-positive fractions are calculated entirely separately, by using the test results from two different subgroups, the ROC plot is independent of the prevalence of disease in the sample. Each point on the ROC plot represents a sensitivity/-specificity pair corresponding to a particular decision threshold. A test with perfect discrimination (no overlap in the two distributions of results) has an ROC plot that passes through the upper left corner, where the true-positive fraction is 1.0, or 100% (perfect sensitivity), and the false-positive fraction is 0 (perfect specificity). The theoretical plot for a test with no discrimination (identical distributions of results for the two groups) is a 45° diagonal line from the lower left corner to the upper right corner. Most plots fall. in between these two extremes. (If the ROC plot falls completely below the 45° diagonal, this is easily remedied by reversing the criterion for "positivity" from "greater than" to "less than" or vice versa.) Qualitatively, the closer the plot is to the upper left corner, the higher the overall accuracy of the test.
One convenient goal to quantify the diagnostic accuracy of a laboratory test is to express its performance by a single number. The most common global measure is the area under the ROC plot. By convention, this area is always > 0.5 (if it is not, one can reverse the decision rule to make it so). Values range between 1.0 (perfect separation of the test values of the two groups) and 0.5 (no apparent distributional difference between the two groups of test values). The area does not depend only on a particular portion of the plot such as the point closest to the diagonal or the sensitivity at 90% specificity, but on the entire plot. This is a quantitative, descriptive expression of how close the ROC plot is to the perfect one (area =
1.0).
Clinical utility of the novel marker SAHH has been assessed in comparison to and in combination with the established marker hemoglobin using a receiver operator curve analysis (ROC; Zweig, M. H., and Campbell, G., Clin. Chem. 39 (1993) 561-577). This analysis has been based on well-defined patient cohorts consisting of 30 samples each from patients in T1-3; N0; M0, more progressed tumor, i.e., T4 and/or various severity of metastasis (N+ and/or M+), and healthy controls, respectively.
The following examples, references, sequence listing and figures are provided to aid the understanding of the present invention, the true scope of which is set forth in the appended claims. It is understood that modifications can be made in the procedures set forth without departing from the spirit of the invention.
Description of the Figures Figure 1 Figure 1 shows a typical example of a 2D-gel, loaded with a tumor sample (left side), and a gel, loaded with a matched control sample (right side) obtained from adjacent healthy mucosa. The molecular weight inferred from the position of the protein spot in the gel is about 48 kDa, the isoelectric point is at about pH 6 (less). The circle in the enlarged section of these gels indicates the position for the protein SAHH. This protein was not detectable by the same method in healthy mucosa.
Figure 2 Typical example of a Western-Blot. A polyacrylamide gel was loaded with tissue lysates from colorectal tumor tissue and adjacent healthy control tissue from 3 patients (subject 4: colon ca (carcinoma), Dukes C; subject 7: colon ca, Dukes C; and subject 13: colon ca, Dukes B) and after electrophoresis the proteins were blotted onto a nitrocellulose membrane. Presence of SAHH in the samples was tested using a polyclonal rabbit anti-SAHH serum.
Lanes containing tumor lysates are indicated with "T", lanes containing normal control tissue with "N". The arrow indicates the position in the gel of the SAHH band. All tumor samples give a strong signal at the position of SAHH, whereas only a weale signal can be detected in the lysates from adjacent normal control tissue.
Abbreviations ABTS 2,2'-Azino-di- [3-ethylbenzthiazoline sulfonate (6)]

diammonium salt BSA bovine serum albumin cDNA complementary DNA

CHAPS (3-[(3-Cholamidopropyl)-dimethylammonio]-1-propane-sulfonate) DMSO dimethyl sulfoxide DTT dithiothreitol EDTA ethylene diamine tetraacetic acid ELISA enzyme-linked immunosorbent assay HRP horseradish peroxidase IAA iodoacetamid IgG immunoglobulin G

IEF isoelectric focussing IPG immobilized pH gradient LDS lithium dodecyl sulfate MALDI-TOF matrix-assisted laser desorption/ionisation-time of flight mass spectrometry MES mesityl, 2,4,6-trimethylphenyl OD optical density PAGE polyacrylamide gel electrophoresis PBS phosphate buffered saline PI isoelectric point RTS rapid translation system SDS sodium dodecyl sulfate Example 1 Identification of SAHH as a potential colorectal cancer marker Sources of tissue In order to identify tumor-specific proteins as potential diagnostic markers for colorectal cancer, analysis of three different kinds of tissue using proteomics methods is performed.
In total, tissue specimen from 10 patients suffering from colorectal cancer are analyzed. From each patient three different tissue types are collected from therapeutic resections: tumor tissue (> 80% tumor) (T), adjacent healthy tissue (N) and stripped mucosa from adjacent healthy mucosa (M). The latter two tissue types serve as matched healthy control samples. Tissues are immediately snap frozen after resection and stored at - 80°C before processing. Tumors are diagnosed by histopathological criteria.
Tissue preparation 0.8-1.2 g of frozen tissue are put into a mortar and completely frozen by liquid nitrogen. The tissue is pulverized in the mortar, dissolved in the 10-fold volume (w/v) of lysis buffer (40 mM Na-citrate, 5 mM MgCl2, 1% Genapol X-080, 0.02%
Na-azide, Complete~ EDTA-free [Roche Diagnostics GmbH, Mannheim, Germany, Cat. No. 1 873 580] ) and subsequently homogenized in a Wheaton~
glass homogenizer (20 x loose fitting, 20 x tight fitting). 3 ml of the homogenate are subjected to a sucrose-density centrifugation (10-60% sucrose) for 1 h at 4500 x g.

After this centrifugation step three fractions are obtained. The fraction on top of the gradient contains the soluble proteins and is used for further analysis.
Isoelectric focussing (IEF) and SDS-PAGE
For IEF, 3 ml of the suspension are mixed with 12 ml sample buffer (7 M urea, thiourea, 2% CHAPS, 0.4% IPG buffer pH 4-7, 0.5% DTT) and incubated for 1 h.
The samples are concentrated in an Amicon° Ultra-15 device (Millipore GmbH, Schwalbach, Germany) and the protein concentration is determined using the Bio-Rad~ protein assay (Cat.No. 500-0006; Bio-Rad Laboratories GmbH, Miinchen, Germany) following the instructions of the supplier's manual. To a volume corresponding to 1.5 mg of protein sample buffer is added to a final volume of 350 ~tl. This solution is used to rehydrate IPG strips pH 4-7 (Amersham Biosciences, Freiburg, Germany) overnight. The IEF is performed using the following gradient protocol: 1.) 1 minute to 500 V; 2.) 2 h to 3,500 V; 3.) 22 h at constant 3,500 V giving rise to 82 kVh. After IEF, strips are stored at -80°C or directly used for SDS-PAGE.
Prior to SDS-PAGE the strips are incubated in equilibration buffer (6 M urea, 50 mM Tris/HCI, pH 8.8, 30% glycerol, 2% SDS), for reduction DDT (15 min, +
50 mg DTT/10 ml), and for alkylation IAA (15 min, + 235 mg iodacetamide/10 ml) is added. The strips are put on 12.5% polyacrylamide gels and subjected to electrophoresis at 1 W/gel for 1 h and thereafter at 17 W/gel. Subsequently, the gels are fixed (50% methanol, 10% acetate) and stained overnight with NoveX M
Colloidal Blue Staining Kit (Invitrogen, Karlsruhe, Germany, Cat No. LC6025, 7101).
Detection of SAHH as a potential marker for colorectal cancer Each patient is analyzed separately by image analysis with the ProteomeWeaver~
software (Definiens AG, Germany, Miinchen). In addition, all spots of the gel are excised by a picking robot and the proteins present in the spots are identified by MALDI-TOF mass spectrometry (UltraflexTM Tof/Tof, Bruker Daltonik GmbH, Bremen, Germany). For each patient, 4 gels from the tumor sample are compared with 4 gels each from adjacent normal and stripped mucosa tissue and analyzed for distinctive spots corresponding to differentially expressed proteins. By this means, protein SAHH is found to be specifically expressed or strongly overexpressed in tumor tissue and not detectable or less strongly expressed in healthy control tissue.
It therefore - amongst many other proteins - qualifies as a candidate marker for use in the diagnosis of colorectal cancer.
Example 2 Generation of antibodies to the colorectal cancer marker protein SAHH
Polyclonal antibody to the colorectal cancer marker protein SAHH is generated for further use of the antibody in the measurement of serum and plasma and blood and stool levels of SAHH by immunodetection assays, e.g. Western Blotting and ELISA.
Recombinant protein expression in E. coli In order to generate antibodies to SAHH, recombinant expression of the protein is performed for obtaining immunogens. The expression is done applying a combination of the RTS 100 expression system and E.coli. In a first step, the DNA
sequence is analyzed and recommendations for high yield cDNA silent mutational variants and respective PCR-primer sequences are obtained using the "ProteoExpert RTS E.coli HY" system. This is a commercial web based service (www.proteoexpert.com). Using the recommended primer pairs, the "RTS 100 E.
coli Linear Template Generation Set, His-tag" (Roche Diagnostics GmbH, Mannheim, Germany, Cat.No. 3186237) system to generate linear PCR templates from the cDNA and for in-vitro transcription and expression of the nucleotide sequence coding for the SAHH protein is used. For Western-blot detection and later purification, the expressed protein contains a His-tag. The best expressing variant is identified. All steps from PCR to expression and detection are carried out according to the instructions of the manufacturer. The respective PCR product, containing all necessary T7 regulatory regions (promoter, ribosomal binding site and T7 terminator) is cloned into the pBAD TOPO° vector (Invitrogen, Karlsruhe, Germany, Cat. No. K 4300/01) following the manufacturer's instructions. For expression using the T7 regulatory sequences, the construct is transformed into E.
coli BL 21 (DE 3) (Studier, F.W., et al., Methods Enzymol. 185 (1990) 60-89) and the transformed bacteria are cultivated in a 11 batch for protein expression.

Purification of His-SAHH fusion protein is done following standard procedures on a Ni-chelate column. Briefly, 11 of bacteria culture containing the expression vector for the His-SAHH fusion protein is pelleted by centrifugation. The cell pellet is resuspended in lysis buffer, containing phosphate, pH 8.0, 7 M guanidium chloride, imidazole and thioglycerole, followed by homogenization using a Ultra-Turrax ~t .
Insoluble material is pelleted by high speed centrifugation and the supernatant is applied to a Ni-chelate chromatographic column. The column is washed with several bed volumes of lysis buffer followed by washes with buffer, containing phosphate, pH 8.0 and Urea. Finally, bound antigen is eluted using a phosphate buffer containing SDS under acid conditions.
Production of monoclonal antibodies against the SAHH
a) Immunization of mice 12 week old A/J mice are initially immunized intraperitoneally with 100 ~g SAHH.
This is followed after 6 weeks by two further intraperitoneal immunizations at monthly intervals. In this process each mouse is administered 100 ~.g SAHH
adsorbed to aluminum hydroxide and 109 germs of Bordetella pertussis.
Subsequently the last two immunizations are carried out intravenously on the 3rd and 2nd day before fusion using 100 ~g SAHH in PBS buffer for each.
b) Fusion and cloning Spleen cells of the mice immunized according to a) are fused with myeloma cells according to Galfre, G., and Milstein, C., Methods in Enzymology 73 ( 1981 ) 3-46.
In this process ca. 1*10$ spleen cells of the immunized mouse are mixed with 2x10' myeloma cells (P3X63-Ag8-653, ATCC CRL1580) and centrifuged (10 min at 300 x g and 4°C.). The cells are then washed once with RPMI 1640 medium without fetal calf serum (FCS) and centrifuged again at 400 x g in a 50 ml conical tube. The supernatant is discarded, the cell sediment is gently loosened by tapping, 1 ml PEG
(molecular weight 4000, Merck, Darmstadt) is added and mixed by pipetting.
After 1 min in a water-bath at 37°C., 5 ml RPMI 1640 without FCS is added drop-wise at room temperature within a period of 4-5 min. Afterwards 5 ml RPMI 1640 containing 10% FCS is added drop-wise within ca. 1 min, mixed thoroughly, filled to 50 ml with medium (RPMI 1640+10% FCS) and subsequently centrifuged for min at 400 x g and 4°C. The sedimented cells are taken up in RPMI 1640 medium containing 10% FCS and sown in hypoxanthine-azaserine selection medium (100 mmol/1 hypoxanthine, 1 ~.g/ml azaserine in RPMI 1640+10% FCS).
Interleukin 6 at 100 U/ml is added to the medium as a growth factor.
5 After ca. 10 days the primary cultures are tested for specific antibody.
SAHH-positive primary cultures are cloned in 96-well cell culture plates by means of a fluorescence activated cell sorter. In this process again interleukin 6 at 100 U/ml is added to the medium as a growth additive.
c) Immunoglobulin isolation from the cell culture supernatants 10 The hybridoma cells obtained are sown at a density of 1x105 cells per ml in RPMI
1640 medium containing 10% FCS and proliferated for 7 days in a fermenter (Thermodux Co., Wertheim/Main, Model MCS-104XL, Order No. 144-050). On average concentrations of 100 ~.g monoclonal antibody per ml are obtained in the culture supernatant. Purification of this antibody from the culture supernatant is carried out by conventional methods in protein chemistry (e.g. according to Bruclc, C., et al., Methods in Enzymology 121 (1986) 587-695).
Generation of polyclonal antibodies a) Immunization For immunization, a fresh emulsion of the protein solution ( 100 ~g/ml protein SAHH) and complete Freund's adjuvant at the ratio of 1:1 is prepared. Each rabbit is immunized with 1 ml of the emulsion at days 1, 7, 14 and 30, 60 and 90.
Blood is drawn and resulting anti-SAHH serum used for further experiments as described in examples 3 and 4.
b) Purification of IgG (immunoglobulin G) from rabbit serum by sequential precipitation with caprylic acid and ammonium sulfate One volume of rabbit serum is diluted with 4 volumes of acetate buffer (60 mM, pH 4.0). The pH is adjusted to 4.5 with 2 M Tris-base. Caprylic acid (25 ~1/ml of diluted sample) is added drop-wise under vigorous stirring. After 30 min the sample is centrifuged ( 13,000 x g, 30 min, 4°C), the pellet discarded and the supernatant collected. The pH of the supernatant is adjusted to 7.5 by the addition of 2 M Tris-base and filtered (0.2 ~tm).
The immunoglobulin in the supernatant is precipitated under vigorous stirring by the drop-wise addition of a 4 M ammonium sulfate solution to a final concentration of 2 M. The precipitated immunoglobulins are collected by centrifugation (8,000 x g, 15 min, 4°C).
The supernatant is discarded. The pellet is dissolved in 10 mM NaH2P04/NaOH, pH 7.5, 30 mM NaCI and exhaustively dialyzed. The dialysate is centrifuged (13,000 x g, 15 min, 4°C) and filtered (0.2 ~tm).
Biotinylation of polyclonal rabbit I~G
Polyclonal rabbit IgG is brought to 10 mg/ml in 10 mM NaHZPO4/NaOH, pH 7.5, 30 mM NaCI. Per ml IgG solution 50 ~.1 Biotin -N-hydroxysuccinimide (3.6 mg/ml in DMSO) are added. After 30 min at room temperature, the sample is chromatographed on Superdex 200 ( 10 mM NaHZPO4/NaOH, pH 7.5, 30 mM
NaCI). The fraction containing biotinylated IgG are collected. Monoclonal antibodies are biotinylated according to the same procedure.
Digoxy enylation of polyclonal rabbit Ig_G
Polyclonal rabbit IgG is brought to 10 mg/ml in 10 mM NaHZPOø/NaOH, 30 mM
NaCI, pH 7.5. Per ml IgG solution 50 ~.1 digoxigenin-3-O-methylcarbonyl-E-aminocaproic acid-N-hydroxysuccinimide ester (Roche Diagnostics, Mannheim, Germany, Cat. No. 1 333 054) (3.8 mg/ml in DMSO) are added. After 30 min at room temperature, the sample is chromatographed on Superdex~ 200 ( 10 mM
NaH2P04/NaOH, pH 7.5, 30 mM NaCI). The fractions containing digoxigenylated IgG are collected. Monoclonal antibodies are labeled with digoxigenin according to the same procedure.

Example 3 Western Blotting for the detection of SAHH in human colorectal cancer tissue using polyclonal antibody as generated in Example 2.
Tissue lysates from tumor samples and healthy control samples are prepared as described in Example 1, "Tissue preparation".
SDS-PAGE and Western-Blotting are carried out using reagents and equipment of Invitrogen, Karlsruhe, Germany. For each tissue sample tested, 10 ~g of tissue lysate are diluted in reducing NuPAGE~ (Invitrogen) SDS sample buffer and heated for ZO min at 95°C. Samples are run on 4-12% NuPAGE~ gels (Tris-Glycine) in the MES running buffer system. The gel-separated protein mixture is blotted onto nitrocellulose membranes using the Invitrogen XCell IITM Blot Module (Invitrogen) and the NuPAGE° transfer buffer system. The membranes are washed 3 times in PBS/0.05% Tween-20 and blocked with Roti~-Block blocking buffer (A151.1; Carl Roth GmbH, Karlsruhe, Germany) for 2 h. The primary antibody, polyclonal rabbit anti-SAHH serum (generation described in Example 2), is diluted 1:10,000 in Roti~-Bloclc blocking buffer and incubated with the membrane for 1 h. The membranes are washed 6 times in PBS/0.05% Tween-20. The specifically bound primary rabbit antibody is labeled with a POD-conjugated polyclonal sheep anti-rabbit IgG antibody, diluted to 10 mU/ml in 0.5 x Roti~-Block blocking buffer.
After incubation for 1 h, the membranes are washed 6 times in PBS/0.05% Tween-20. For detection of the bound POD-conjugated anti-rabbit antibody, the membrane is incubated with the Lumi-LightPLUS Western Blotting Substrate (Order-No. 2015196, Roche Diagnostics GmbH, Mannheim, Germany) and exposed to an autoradiographic film.

Results of a typical experiment are shown in Figure 2. The strong overexpression of SAHH in tumor tissue versus adjacent control tissue is found in 11 out of 14 subjects with colorectal cancer tested.
Example 4 ELISA for the measurement of SAHH in human stool specimen.
a) Processing of stool specimen About 1 g of stool per sample is collected by the patients in a special sampling device from Sarstedt, Germany, Order-No. 80.623.022, frozen and stored at -20 °C.
For analysis, the stool samples are thawed, tenfold diluted with a phosphate buffer, pH 7.4 and thoroughly mixed in order to yield a suspension of the stool sample in the extraction buffer. After centrifugation for 15 min at 12,000 x g, the upper portion of the supernatant is saved for further analysis. An aliquot of this processed stool sample is used for quantification of SAHH by ELISA.
b) Measurement of SAHH from a processed stool sample For detection of SAHH in human a processed stool sample, a sandwich ELISA is developed. For capture and detection of the antigen, aliquots of the anti-SAHH
polyclonal antibody (see example 2) are conjugated with biotin and digoxygenin, respectively.
Streptavidin-coated 96-well microtiter plates are incubated with 100 ~tl biotinylated anti-SAHH polyclonal antibody for 60 min at 10 ~.g/ml in 10 mM phosphate, pH 7.4, 1% BSA, 0.9% NaCI and 0.1% Tween-20. After incubation, plates are washed three times with 0.9% NaCI , 0.1% Tween-20. Wells are then incubated for 2 h with either a serial dilution of the recombinant protein (see Example 2) as standard antigen or with diluted stool samples from patients. After binding of SAHH, plates are washed three times with 0.9% NaCI, 0.1% Tween-20. For specific detection of bound SAHH, wells are incubated with 100 ~l of digoxygenylated anti-SAHH polyclonal antibody for 60 min at 10 ~tg/ml in 10 mM phosphate, pH 7.4, 1% BSA, 0.9% NaCI and 0.1% Tween-20. Thereafter, plates are washed three times to remove unbound antibody. In a next step, wells are incubated with 20 mU/ml anti-digoxigenin-POD conjugates (Ruche Diagnostics GmbH, Mannheim, Germany, Catalog No. 1633716) for 60 min in 10 mM phosphate, pH 7.4, 1% BSA, 0.9% NaCI and 0.1% Tween-20. Plates are subsequently washed three times with the same buffer. For detection of antigen-antibody complexes, wells are incubated with 100 ~1 ABTS solution (Ruche Diagnostics GmbH, Mannheim, Germany, Catalog No. 11685767) and OD is measured after 30-60 min at 405 nm with an ELISA reader.
Example 55 ROC analysis to assess clinical utility in terms of diagnostic accuracy Accuracy is assessed by analyzing individual stool samples obtained from well-characterized patient cohorts, i.e., 30 patients having undergone colonoscopy and found to be free of adenoma or CRC, 30 patients diagnosed and staged as Tl-3, N0, MO of CRC, and 30 patients diagnosed with progressed CRC, having at least tumor infiltration in at least one proximal lymph node or more severe forms of metastasis, respectively. SAHH is measured as described above in a stool sample obtained from each of these individuals. ROC-analysis is performed according to Zweig, M.
H., and Campbell, supra. Discriminatory power for differentiating patients in the group Tis-3, N0, MO from healthy individuals for the combination of SAHH with the established marker hemoglobin (Hemoglobin ELISA; Catalogue No.: I~7816;
Immundiagnostik AG, Wiesenstr. 4, D 64625 Bensheim, Germany) is calculated by regularized discriminant analysis (Friedman, J. H., Regularized Discriminant Analysis, Journal of the American Statistical Association 84 (1989) 165-175).

List of References Ahlquist, D.A., Gastroenterol. Clin. North Am. 26 ( 1997) 41-55 Anderson, W.F., et al., J. Natl. Cancer Inst. 94 (2002) 1126-1133 Bass, R., et al., J. Biol. Chem. 277 (2002) 46845-46848 Bethin, K.E., et al., j. Biol. Chem. 270 (1995) 20698-20702 Bruck, C., et al., Methods Enzymol. 121 ( 1986) 587-596 Briinagel, G., et al., Cancer Res. 62 (2002) 2437-2442 Cantoni, G.L., Annu. Rev. Biochem. 44 (1975) 435-451 Carriquiry, L.A., and Pineyro, A., Dis. Colon Rectum 42 (1999) 921-929 Chiang, P.K., Pharmacol. Ther. 77 (1998) 115-134 Chiang, P.K., et al., FASEB J. 10 (1996) 471-480 Coulter-Karis, D.E., and Hershfield, M.S., Ann. Hum. Genet. 53 ( 1989) 169-175 Cui, Z., et al., J. Biol. Chem. 269 ( 1994) 24531-24533 Davies, R.J., et al., Lancet 359 (2002) 1917-1919 Diamandis et al., eds., Immunoassay, Academic Press, Boston ( 1996) Friedman, J. H., Regularized Discriminant Analysis, Journal of the American Statistical Association 84 (1989) 165-175 Galfre, G., and Milstein, C., Methods Enzymol. 73 ( 1981 ) 3-46 Geenen, J.E., et al., Am. J. Dig. Dis. 20 (1975) 231-235 Goldenberg, D.M., et al., J. Natl. Cancer Inst. 57 (1976) 11-22 Herrera, M.A., et al., Ann. Surg. 183 ( 1976) 5-9 Hershfield, M.S., and Francke, U., Science 216 (1982) 739-742 Labrune, P., et al., J. Pediatr. 117 ( 1990) 220-226 Martell, R.E., et al., Int. J. Biol. Markers 13 (1998) 145-149 Moertel, C.G., et al., JAMA 270 (1993) 943-947 Reynoso, G., et al., JAMA 220 (1972) 361-365 Sieg, A., et al., Int. J. Colorectal Dis. 14 (1999) 267-271 Silvis, S.E., et al., JAMA 235 (1976) 928-930 Sobin, L.H., Wittekind, Ch. (eds), TNM Classification of Malignant Tumours, fifth edition, 1997, UICC (International Union Against Cancer) Studier, F.W., et al., Methods Enzymol. 185 (1990) 60-89 Sturgeon, C., Clin. Chem. 48 (2002) 1151-1159 Szyf, M., et al., Pharmacol. Ther. 70 (1996) 1-37 Tijssen, P., Practice and theory of enzyme immunoassays 11 ( 1990) the whole boolc, especially pages 43-78; Elsevier, Amsterdam Turner, M.A., et al., Cell. Biochem. Biophys. 33 (2000) 101-125 Wanebo, H.J., et aL, N. Engl. J. Med. 299 ( 1978) 448-451 Zou, Z., et al., Science 263 ( 1994) 526-529 Zweig, M. H., and Campbell, G., Clin. Chem. 39 (1993) 561-577 DEMANDES OU BREVETS VOLUMINEUX
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Claims

1. A method for the diagnosis of colorectal cancer comprising the steps of a) providing a stool sample obtained from an individual, b) contacting said sample with a specific binding agent for S-adenosylhomocysteine hydrolase (SAHH) under conditions appropriate for formation of a complex between said binding agent and SAHH, and c) correlating the amount of complex formed in (b) to the diagnosis of colorectal cancer.

2. Use of protein SAHH as a marker molecule in the diagnosis of colorectal cancer from a stool sample obtained from an individual.

3. Use of protein SAHH as a marker molecule in the early diagnosis of colorectal cancer from a stool sample obtained from an individual.

4. Use according to claim 3, wherein the early diagnosis is made with a sample derived from CRC patients in the adenoma stage.

5. Use according to claim 3, wherein the early diagnosis is made with a sample derived from CRC patients in stage T is -3; N0; M0

6. Use of protein SAHH as a marker molecule for colorectal cancer in combination with another marker molecule for colorectal cancer in the diagnosis of colorectal cancer from a stool sample obtained from an individual.

7. An immunological lut comprising at least one specific binding agent for SAHH and auxiliary reagents for measurement of SAHH.