METHOD FOR MEASURING GLYCOPROTEIN, METHOD FOR EXAMINING LIVER DISEASE, REAGENT FOR QUANTITATIVE DETERMINATION OF GLYCOPROTEIN, AND GLYCAN-MARKER GLYCOPROTEIN AS AN INDEX FOR CLINICAL CONDITIONS OF LIVER DISEASE
An object of the present invention is to provide a method for measuring a glycan-marker glycoprotein, by which liver disease can be detected with higher accuracy than is possible with conventional methods. Also, an object of the present invention is to provide a method for examining liver disease, by which liver disease can be detected with higher accuracy than is possible with conventional methods. Also, an object of the present invention is to provide a reagent for quantitative determination of a glycoprotein, which is used for the above measurement methods. Furthermore, an object of the present invention is to provide a glycan-marker glycoprotein as an index for clinical conditions of liver disease, which is capable of identifying the clinical conditions of liver disease depending on the progress of liver disease. The method for measuring a glycoprotein is characterized in that: the glycoprotein is at least one glycoprotein selected from alpha-1-acid glycoprotein (AGP) and Mac-2-binding protein (M2BP) contained in a sample collected from a subject; when the glycoprotein is AGP, AGP binding to a first lectin selected from AOL and MAL is measured; and when the glycoprotein is M2BP, M2BP binding to a second lectin selected from WFA, BPL, AAL, RCA120, and TJAII is measured.
This application is a continuation of U.S. application Ser. No. 14/051,729, filed Oct. 11, 2013, which is a division of U.S. application Ser. No. 13/374,807, filed Jan. 13, 2012, which is a continuation of PCT/JP2010/061891 filed on Jul. 14, 2010, which claims priority to Japanese Application Nos. 2009-165795 filed on Jul. 14, 2009 and 2009-287243 filed on Dec. 18, 2009. The entire contents of these applications are incorporated herein by reference.
BACKGROUND OF THE INVENTION 1. Field of the InventionThe present invention relates to a method for measuring at least one glycoprotein selected from alpha-1-acid glycoprotein (AGP) and Mac-2-binding protein (M2BP), a method for examining liver disease using at least one glycoprotein selected from AGP and M2BP, and a glycan-marker glycoprotein with which hepatic cell carcinoma and background liver status such as regarding inflammation-fiber formation can be detected based on glyco-alterations.
2. Description of the Related ArtLiver cancer can be roughly classified into primary liver cancer and metastatic liver cancer developed in the liver. It is said that hepatic cell carcinoma accounts for 90% of primary liver cancer cases.
Hepatic cell carcinoma patients are often infected with hepatitis type C virus or hepatitis type B virus that constitutes the underlying cause of a disease. The disease proceeds from acute viral hepatitis to chronic viral hepatitis, and then to cirrhosis. Long after the development of viral hepatitis, the disease can become cancerous for the first time. In the case of cirrhosis, normal hepatocytes decrease through repetition of inflammation and regeneration, and then the affected liver becomes an organ composed of fibrous tissue. For example, there are said to be 3 million type C hepatitis patients in Japan alone and 10 million or more in China and Africa. Also, in the case of type B and/or type C hepatitis patients, the carcinogenic rate from chronic hepatitis is an annual rate of 0.8% for mild chronic hepatitis (F1), an annual rate of 0.9% for moderate chronic hepatitis (F2), and an annual rate of 3.5% for severe chronic hepatitis (F3). Furthermore, the probability of cirrhosis (F4) becoming cancerous increases to an annual rate of as high as 7% (
Early detection of cancer is important for cancer treatment. Also, in the case of hepatic cell carcinoma, early detection of cancer significantly influences treatment and postoperative prognosis. The 5-year survival rate after hepatic resection is 80% for stage I cancer and only 38% for stage IV cancer.
As liver cancer markers, α-fetoprotein (AFP) and a protein induced by Vitamin K absence or antagonist-II (PIVKA-II) are currently known (patent documents 1 and 2), but both the specificity and the sensitivity thereof are insufficient. Hence, physical examination for early detection of liver cancer is currently conducted with the use of liver cancer markers and imaging studies such as ultrasonography, computed tomography (CT), and magnetic resonance imaging (MRI).
Also, non-patent document 1 describes an attempt to measure fucosylated AGP in serum using AAL lectin so as to detect cirrhosis. However, the technique described in non-patent document 1 is unsatisfactory in view of liver disease detection performance, since the specificity is about 87% and the accuracy is about 77%, although the sensitivity is about 66%, as understood from the results described in Table 2.
Also, non-patent document 2 describes an experiment conducted by measuring asialo AGP in sera of healthy subjects, acute hepatitis patients, chronic hepatitis patients, cirrhosis patients, and hepatic cell carcinoma patients by immunochromatography using RCA lectin, so as to reveal whether each liver disease could be determined to be positive or not. However, the technique described in non-patent document 2 is unsatisfactory in view of liver disease detection performance, since the sensitivity of cirrhosis detection, for example, is about 88%, but the false positive rate for chronic hepatitis patients is 63%, as understood from the results described in Table 2.
PRIOR ART DOCUMENTS Patent Documents
- Patent document 1: JP Patent Publication (Kokai) No. 10-26622 A (1998)
- Patent document 2: JP Patent Publication (Kokai) No. 8-184594 A (1996)
- Non-patent document 1: Ingvar Ryden et al., Diagnostic Accuracy of α1-Acid Glycoprotein Fucosylation for Liver Cirrhosis in Patients Undergoing Hepatic Biopsy, Clinical Chemistry 48: 12, 2195-2201 (2002)
- Non-patent document 2: Eun Young Lee et al., Development of a rapid, immunochromatographic strip test for serum asialo α1-acid glycoprotein in patients with hepatic disease, Journal of Immunological Methods 308 (2006) 116-123
An object of the present invention is to provide a method for measuring a glycan-marker glycoprotein, by which liver disease can be detected with higher accuracy than conventional methods. Also, an object of the present invention is to provide a method for examining liver disease, by which liver disease can be detected with higher accuracy than conventional methods. Also, an object of the present invention is to provide a reagent(s) for quantitative determination of a glycoprotein(s) to be used for the above measurement methods. Moreover, an object of the present invention is to provide a glycan-marker glycoprotein as an index for clinical conditions of liver disease, with which clinical conditions of liver disease can be distinguished from one another according to the progress of liver disease.
The method for measuring at least one glycoprotein selected from alpha-1-acid glycoprotein (AGP) and Mac-2-binding protein (M2BP) contained in a sample collected from a subject is characterized in that: when the glycoprotein is AGP, AGP that binds to first lectin selected from AOL and MAL is measured; and when the glycoprotein is M2BP, M2BP that binds to second lectin selected from WFA, BPL, AAL, RCA120, and TJAII is measured.
According to the measurement method of the present invention, a glycan-marker glycoprotein, with which liver disease such as cirrhosis can be examined with high reliability, can be conveniently measured.
Furthermore, according to the glycan-marker glycoprotein as an index for clinical conditions of liver disease of the present invention, examination becomes possible with higher accuracy than is possible with existing markers and with minute amounts of serum. Thus, monitoring of the progress of liver fiber formation becomes possible, so that not only the understanding of the development of clinical conditions but also the evaluation of improvement in fiber formation in the liver or liver inflammation after antiviral therapy using interferon, for example, become possible.
The patent or application file contains at least one drawing executed in color. Copies of this patent or patent application publication with color drawing(s) will be provided by the Office upon request and payment of the necessary fee.
After infection with hepatitis type B virus or hepatitis type C virus, transition from acute-stage inflammation to chronic-stage inflammation takes place for 5-15 years. In particular, type C hepatitis that has transitioned to the chronic stage is merely cured naturally, and the liver functions decrease to result in cirrhosis. The time course from infection with type C hepatitis to hepatic cell carcinoma and changes in liver status are shown in
The medical benefits project in Japan for type B and type C hepatitis patients are exclusively intended for fiber formation at the stages ranging from F1 to F3 as determined by histopathological diagnosis on liver biopsy specimens. On the other hand, when diseases are diagnosed at the F4 stage, they are classified as cirrhosis. Hence, only some type B and type C hepatitis patients are aided by interferon treatment in the medical benefits project. In such cases, satisfactory treatment results cannot be obtained.
1-2. Evaluation of Suppression of Fiber Formation by Antiviral TherapyIn the case of type C chronic hepatitis, PEG-IFN+RBV therapy is applied. In the case of a type C cirrhosis compensatory period, sole administration of interferon is applied. Meanwhile, in the case of type B hepatitis (chronic hepatitis or cirrhosis), treatment is mainly performed with a nucleic acid analog and inflammation and fiber formation evaluation markers are thought to be essential. In particular, clinical application of serum biomarkers is broadly expected for diagnostic and evaluation purposes.
1-3. Hepatic Cell CarcinomaIt is considered that microbiological factors (through infection with hepatitis type B virus or hepatitis type C virus) and environmental factors alternately have significant impact on hepatic cell carcinoma. In Japan, it is known that about 90% of hepatic cell carcinoma patients have a history of infection with hepatitis type B or hepatitis type C virus and that chronic hepatitis patients and cirrhosis patients develop hepatic cell carcinoma. In addition to the presence of viruses, being male, being elderly, alcoholism, tobacco, the presence of aflatoxin (a fungal toxin), and the like are suggested as hepatic cell carcinoma risk factors (Clinical guidelines for liver cancer, International Medical Information Center (Foundation)).
1-4. Early Diagnosis of Hepatic Cell CarcinomaHepatic cell carcinoma is currently detected by mainly the measurement of liver cancer markers such as AFP and PIVKA-II in a serum sample from a subject and diagnostic imaging performed mainly by ultrasonography (echo test). Diagnostic imaging is generally performed by a first test using ultrasonography or CT and then by MRI or angiography when some abnormalities are found.
1-5. Discrimination of Groups at High Risk of Cancer in View of Prevention of Hepatic Cell CarcinomaAbout 90% of hepatic cell carcinoma patients have experienced transition from hepatitis due to infection with hepatitis type B virus or hepatitis type C virus in Japan. Hence, patients to be subjected to detailed examination can be discriminated using viral infection and decreased liver functions as indices.
However, even in the case of cirrhosis (F4) patients for which hepatic cell carcinoma appears at an annual rate of about 7%, it must be said that repetition of expensive detailed examinations that are highly invasive every 3 months for early detection and treatment of cancer is a significant economic and physical burden for the patients. This can especially be said for the case of F3, which has an annual carcinogenic rate of 3-4%. Furthermore, in view of the about 50% success rate of the treatment of hepatitis type C virus with interferon, it is necessary to clarify the stage (between cirrhosis and the onset of hepatic cell carcinoma) of each chronic hepatitis patient and thus to perform clinical follow-up for a considerable number of the patients for which interferon treatment has failed. Specifically, current treatment for the disease that proceeds from hepatitis to hepatic cell carcinoma is in a status in which the risk of cancer should be ranked for hepatitis to cirrhosis patients by a convenient test such as a blood test and then diagnostic treatment of hepatic cell carcinoma appropriate for each result should be performed.
From the perspective of clinical pathology, the degree of fiber formation correlates with the risk of cirrhosis or the risk of hepatic cell carcinoma. Therefore, we have found that the development of an inspection technique by which the progress of fiber formation can be determined serologically and quantitatively can solve the problem. As shown in
AGP and M2BP are the new glycan-marker glycoproteins used as indices for clinical conditions of liver disease of the present invention. They are found to experience glyco-alterations that are characteristic of chronic hepatitis, cirrhosis, and hepatic cell carcinoma caused by the development and progress of diseases due to viral infection. Such marker glycoproteins capable of specifying clinical conditions of liver disease using glyco-alterations accompanying the progress of clinical conditions of viral liver disease as indices are referred to as glycan markers as indices for clinical conditions of liver disease.
Detection of glyco-alterations in AGP and M2BP that are new glycan markers as indices for clinical conditions of liver disease of the present invention is effective for distinguishing among clinical conditions of viral liver diseases such as hepatic cell carcinoma, cirrhosis, fiber formation in the liver (F3 and F4 markers), and chronic hepatitis so as to distinguish among the diseases. However, such glyco-alterations in these markers differ in type and rate depending on disease type and the degree of progress. Therefore, lectin probes reflecting disease-specific glyco-alterations should be statistically selected in order to construct detection kits specialized in each subject using the markers.
3. Verification of Liver Disease-Specific Glyco-Alterations in Glycan-Marker GlycoproteinsDisease-specific glyco-alterations existing on AGP and M2BP are verified using lectin arrays described later. More specifically, an antibody-overlay lectin array method is employed. Based on the results obtained by measurement of the above marker glycoproteins using lectin arrays, 1) the degree of changes in measured values and lectin signals at which the changes are observed depending on the progress of the disease, 2) the stage (initial or late stage) at which changes in measured value are most significant, and 3) whether or not information concerning changes in measured value contributes to disease control are examined and the usefulness thereof is evaluated, so that the appropriateness of each marker for clinical conditions of liver disease is verified.
More specific methods for selecting lectin probes appropriate for using glycan-marker glycoproteins for monitoring of the progress of fiber formation in the liver or detection of cirrhosis are as described below.
Differential glycan profiling is performed using antibody-overlay lectin microarrays or the like for glycoproteins (AGP and M2BP) collected from the sera of (viral) hepatitis patients, cirrhosis patients, and hepatic cell carcinoma patients. First, blood samples are collected from (viral) hepatitis patients, chronic hepatitis patients, cirrhosis patients, and hepatic cell carcinoma patients. Each blood sample collected is subjected to immunoprecipitation using antibodies against AGP and M2BP, thereby performing concentration and purification. Then, it is confirmed whether the use as glycan-marker glycoproteins for clinical conditions of liver disease is possible using antibody-overlay lectin arrays. More specifically, as shown in
A lectin array is prepared by immobilizing (array formation) a plurality of types of discriminant (probe) lectin, which differ in specificity, on one substrate in parallel. With a lectin array, the types of lectin that interact with complex carbohydrates to be analyzed and the degrees of the interactions can be simultaneously analyzed. Moreover, with a lectin array, information required for glycan structure estimation can be obtained by a single analysis, and, steps from sample preparation to scanning can be rapidly and conveniently performed. Glycoproteins cannot be directly analyzed by a glycan profiling system such as mass spectroscopy. When such a system is employed, glycoproteins should be converted in advance to glycopeptides or free sugar chains. Meanwhile, a lectin microarray is advantageous in that direct analysis is possible with only the direct introduction of a fluorescence substance into a core protein portion, for example. Lectin microarray technology has been developed by the present inventors and the principle and the basic concept thereof are described in Kuno A., et al. Nat. Methods 2, 851-856 (2005), for example.
Examples of lectins to be used for lectin arrays are as listed in Table 2 below.
For example, a lectin array (LecChip (GP Bioscience)) on which 45 types of lectin have been immobilized on the base is already currently commercially available.
3-2. Statistical Analysis of Glycan Profiles Using Lectin ArraysLectin array technology has been currently developed to practical technology by which quantitative differential glycan profiling can be performed not only for purified samples, but also for mixed samples such as sera and cell lysates. In particular, differential glycan profiling of sugar chains on cell surface layers has been significantly developed (Ebe, Y. et al., J. Biochem. 139, 323-327 (2006), Pilobello, K. T. et al., Proc Natl Acad Sci U.S.A. 104, 11534-11539 (2007), Tateno, H. et al., Glycobiology 17, 1138-1146 (2007)).
Also, data mining of glycan profiles by statistical analysis can be performed by methods described in “Kuno A, et al. J Proteomics Bioinform. 1, 68-72 (2008),” “The Japanese Society of Carbohydrate Research, 2008/8/18 Development of Applied Technology of Lectin Microarray—Differential Glycan Profiling and Statistical Analysis of Biological Samples—Atsushi Kuno, Atsushi Matsuda, Yoko Itakura, Hideki Matsuzaki, Hisashi Narumatsu, and Jun Hirabayashi”, and “Matsuda A, et al. Biochem Biophys Res Commun. 370, 259-263 (2008),” for example.
3-3. Antibody-Overlay Lectin Microarray MethodA lectin microarray platform is basically as described above. The antibody-overlay lectin microarray method is an applied method that enables convenient, simultaneous, and high-speed analysis of multiple analytes upon detection not by directly labeling analytes with fluorescence or the like, but by indirectly introducing a fluorescent group or the like via an antibody into analytes (“Kuno A, Kato Y, Matsuda A, Kaneko M K, Ito H, Amano K, Chiba Y, Narimatsu H, Hirabayashi J. Mol Cell Proteomics. 8, 99-108 (2009),” “Jun Hirabayashi, Atsushi Kuno, and Noboru Uchiyama, “Development of Applied Technology of Glycan Profiling using Lectin Microarray,” “Approach from Molecular Level, Cancer Diagnosis and Research—Challenge to Clinical Application—(Extra Number, Experimental Medicine), YODOSHA, Vol. 25 (17) 164-171 (2007),” “Application of Glycan Profiling System using Lectin Microarray to Search for Glycan marker (Atsushi Kuno and Jun Hirabayashi),” and “Development of Clinical Glycan marker and Elucidation of Sugar Chain Functions (see Gene and Medicien, Mook No. 11, pp. 34-39, Medical Do (2008)).
When glycoproteins (AGP and M2BP) are analytes, sugar chain (glycan) portions are recognized by lectins on a lectin microarray. Antibodies (anti-AGP antibody and anti-M2BP antibody) against core protein portions are overlaid thereon, so that the glycoproteins to be tested can be specifically detected with high sensitivity without labeling or high-level precise purification thereof.
3-4. Lectin-Overlay Antibody Microarray MethodThe lectin-overlay antibody microarray method involves the use of an antibody microarray instead of a lectin microarray, which is prepared by immobilizing in parallel (array formation) an antibody against a core protein on a substrate such as a glass substrate. The number of antibodies corresponding to the number of markers to be examined is required for the method. It is also required to confirm in advance lectins for detection of glyco-alterations.
4. Method for Detecting Liver Disease Using Disease-Specific Glyco-Alterations in Glycan Marker as an Index for Clinical Conditions of Liver DiseaseAGP and M2BP are novel glycan markers as indices for clinical conditions of liver disease, which is characterized in that the glycan structures are altered in association with clinical changes in liver disease such as the progress of fiber formation. Accordingly, a lectin (hereinafter, abbreviated as lectin “A”), the reactivity of which is altered in response to changes in the glycan structures of AGP and M2BP is reacted with markers contained in a sample collected from a subject, and then markers that have reacted with the lectin are measured. Thus, the clinical conditions of liver disease can be identified and the degree of fiber formation in the liver can be determined, for example.
For example, novel glycan markers as indices for clinical conditions of liver disease can be detected using:
(1) (i) the above lectin “A”; and (ii) an antibody for detection of a core protein portion other than the sugar chain of the above marker. Novel glycan markers as indices for clinical conditions of liver disease can also be detected using: (2) antibodies that are specific to glycan markers as indices for clinical conditions of liver disease, the epitope of which is a part containing a sugar-chain-binding portion.
For example, markers are detected using antibodies against the core proteins of markers and lectin “A”, so that liver disease patients can be distinguished from healthy subjects and detected. Preferably, an antibody overlay method using lectin array (“Kuno A, Kato Y, Matsuda A, Kaneko M K, Ito H, Amano K, Chiba Y, Narimatsu H, Hirabayashi J. Mol Cell Proteomics. 8, 99-108 (2009)) can be used. When one, two, or more optimum lectins “A” are selected for the test for verification of disease-specific glyco-alterations in 3, it is more preferable to use a 1st or 2nd rapid measurement method (described later).
A specific example of the method for examining liver disease using novel glycan markers as indices for clinical conditions of liver disease is a method for detecting liver disease comprising the steps of:
1) measuring glycan markers as indices for clinical conditions of liver disease, which have sugar chains specifically reacting with lectin “A” in a sample collected from a subject;
2) measuring glycan markers as indices for clinical conditions of liver disease, which have sugar chains specifically reacting with lectin “A” in a sample collected from a healthy subject;
3) measuring glycan markers as indices for clinical conditions of liver disease, which have sugar chains specifically reacting with lectin “A” in a sample collected from a liver disease patient; and
4) comparing the measurement results for glycan markers as indices for clinical conditions of liver disease obtained from the subject with the measurement results for glycan markers as indices for clinical conditions of liver disease obtained from the healthy subject or the liver disease patient, and then determining that the subject has liver disease when the measurement results for the subject are closer to the measurement results for the liver disease patient.
A threshold is also determined in advance for distinguishing liver disease from the other diseases based on the measurement results for many liver disease patients and healthy subjects, and then the measurement results for the subject are compared with the threshold, so as to determine whether or not the subject is affected by liver disease.
4-1. Method for Measuring the Progress of Fiber FormationIt is known that regarding the progress of hepatitis due to hepatitis viral infection, the degree of fiber formation correlates with liver dysfunction and a risk of hepatic cell carcinoma. Therefore, the measurement of fiber formation refers to evaluation of liver dysfunction and a risk of cancer. Also, about 40% of all the hepatitis patients does not react to interferon treatment, so that viral infection persists. It is considered that whether or not these clinical conditions progress to an active mode should be determined based on the progress of fiber formation. Based on these viewpoints, measurement of the progress of fiber formation is significant for diagnostic treatment for hepatitis.
Fiber formation is currently evaluated based on pathological diagnosis on biopsy samples. In recent years, the widespread use of the method is expected as a result of introduction of Fibroscan. Also, as methods for serological evaluation of fiber formation, Fibro Test, Ford s index, Hepatoscore, and the like are clinically used, but these methods are inferior to biopsy diagnosis in terms of both sensitivity and specificity.
AGP and M2BP are subjected to the antibody-overlay lectin microarray method using a group of patients' sera differing in the degree of the progress of fiber formation, so that lectins that exhibit increased or decreased signal intensity in correlation with the degree of the progress of fiber formation are selected. Based on the information, a sandwich detection method using an antibody against a candidate marker molecule and lectin “A” exhibiting changes in signals due to the progress of fiber formation can be established, such as lectin-antibody sandwich ELISA or an antibody-overlay lectin microarray method. About 100 patients' sera (100 serum samples) subjected in advance to the staging of fiber formation by pathological diagnosis are collected and then subjected to analysis. A cut off value at each stage is then determined, so that the progress of fiber formation in the liver can be monitored using the serum sample from each patient.
An example of lectin “A” is, in the case of AGP, a first lectin selected from AOL and MAL and an example of lectin “A” in the case of M2BP is a second lectin selected from WFA, BPL, AAL, RCA120, and TJAII. Hereinafter, such a lectin selected from AOL and MAL may be referred to as a “first lectin,” and such a lectin selected from WFA, BPL, AAL, RCA120, and TJAII may be referred to as a “second lectin.”
For example, AGP binding to a first lectin can be measured using a first lectin array to which at least the first lectin has been immobilized and an anti-AGP antibody; and M2BP binding to a second lectin can be measured using a second lectin array to which at least the second lectin has been immobilized and an anti-M2BP antibody.
4-2. Detection of CirrhosisCirrhosis is defined as clinical conditions in which regenerating nodules losing hepatic lobule structures and fine fibrous diffuse connective tissues appear throughout the liver, surrounding such regenerating nodules. This is also a terminal status of progressive chronic liver disease with persistent damage to hepatocytes and fiber formation. Liver biopsy to be performed in cirrhosis is intended to perform component diagnosis. In the cases of early cirrhosis or cirrhosis with a macronodular pattern, many cases are diagnosed with difficulties (Surgical Pathology, Fourth ed., Bunkodo Co., Ltd.). Therefore, test techniques with which cirrhosis can be qualitatively and quantitatively diagnosed are required. For the purpose, candidate antibody molecules capable of monitoring the progress of fiber formation and a lectin set, found in the section, “1) Method for measuring the progress of fiber formation” can be used for detection of cirrhosis if the fiber formation stages, F3 and F4, can be distinguished from each other.
4-3. Detection of Disease-Specific Glyco-Alterations on Novel Glycan Markers as Indices for Clinical Conditions of Liver Disease in a SampleExamples of a sample include, biopsy tissue samples, body fluid samples, and a preferable example of the same is blood (e.g., serum and blood plasma).
The term “measurement” refers to both qualitative measurement and quantitative measurement.
Measurement of glycan markers as indices for clinical conditions of liver disease can be performed using (1) a column or an array to which lectin “A” has been immobilized and (2) an antibody against AGP or M2BP, for example. Preferably, an antibody-overlay lectin array method, and more preferably a 1st or 2nd rapid measurement method can be used.
The concentration of AGP or M2BP can also be measured. Examples of a method to be used therefor include an antibody-overlay lectin array method using a lectin array, immunoassay, an enzyme activity determination method, and a capillary electrophoresis method. Preferably, the following qualitative or quantitative techniques can be used, such as enzyme immunoassay, double-antibody sandwich ELISA, a gold colloid method, radioimmunoassay, enzyme chemiluminescence immunoassay, electric chemiluminescence immunoassay, latex agglutination immunoassay, fluorescence immunoassay, a Western blotting method, an immunohistochemical method, and a surface plasmon resonance method (hereinafter, referred to as an SPR method) using lectin “A” most reflecting disease-specific glyco-alterations, which is statistically selected with an antibody-overlay lectin array, and a monoclonal antibody or a polyclonal antibody specific to AGP or M2BP.
Further specifically, sub determination can also be performed by a Western blotting method using lectin “A” and antibodies against glycan markers as indices for clinical conditions of a disease. The above expression “when the measurement results for a subject are higher than . . . ” in qualitative determination refers to a case in which novel glycan markers as indices for clinical conditions of a disease are qualitatively demonstrated to be present in a sample from a subject with higher concentrations than those in a sample from a healthy subject. Furthermore, a lectin method as a direct sugar chain measurement method without mediation of an antibody is also included herein.
Examples of lectin “A” the reactivity of which is altered in response to changes (accompanying the progress of fiber formation in the liver) in the AGP gly can structure include AOL and MAL or a combined use of AOL and MAL, which are strictly selected by statistical analysis after an antibody-overlay lectin array method. AOL is a lectin that exhibits the highest significant difference among a group of lectins, the reactivity of which to AGP sugar chain increases with the progress of fiber formation in the liver. MAL is a lectin exhibits the most significant differences among a group of lectins, the reactivity of which to AGP sugar chain decreases with the progress of fiber formation in the liver. Accordingly, the use of both measured value of AGP binding to AOL and measured value of AGP binding to MAL makes it possible to more precisely distinguish the clinical conditions of the liver disease of a subject. As a method that involves the use of both the measured value of AGP binding to AOL (measured value of AOL) and the measured value of AGP (measured value of MAL) binding to MAL, a known statistical technique can be employed. For convenience, a difference between and the ratio of AOL measurement value and/to MAL measurement value can be used. In addition, when a difference between or the ratio of AOL measurement value and/to MAL measurement value is used, the same scale is preferably employed for both measured values for convenience, a difference between the cut off line values of both measured values is found and then the scales can be corrected. For example, the ratio of MAL cut-off line value to AOL cut-off line value is used and then either AOL measurement value or MAL measurement value may be corrected. AGP contained in a sample collected from a subject using AOL and/or MAL is measured, so that AGP can be used as a marker for identifying fiber formation in the liver, a cirrhosis detection marker, or a hepatic cell carcinoma detection marker. Also, AGP in a sample collected from a patient under treatment using interferon or the like is measured using the lectin “A,” so that the therapeutic effect can be monitored.
In addition, the measured values of AGP binding to AOL or MAL are preferably normalized using the measured value of AGP binding to lectins the reactivity of which substantially remains unchanged regardless of changes in AGP glycan structure. As such a lectin, DSA is preferable. Also, measured values of AGP binding to AOL or MAL can be normalized using the measured value of AGP core protein contained in a sample collected from a subject. Also, in a method that involves the use of both AOL measurement value and MAL measurement value, a normalized AOL measurement value and a normalized MAL measurement value are preferably used. For example, with the use of the above first lectin array and the above second lectin array, which are prepared by further immobilizing DSA, AGP binding to DSA is measured, measured values of AGP binding to a first lectin are normalized using measured values of AGP binding to DSA, M2BP binding to DSA is measured, the measured values of M2BP binding to a second lectin are normalized using the measured value of M2BP binding to DSA, and thus AGP and/or M2BP can be measured. Examples of lectin “A,” the reactivity of which is altered in response to changes in M2BP glycan structure accompanying changes in the clinical conditions of the liver, include WFA, BPL, AAL, RCA120, and/or TJAII strictly selected by statistical analysis after the antibody-overlay lectin array method. WFA, BPL, AAL, RCA120, and TJAII are all lectins, the reactivity of which to M2BP sugar chain increases as the clinical conditions of liver disease progress. WFA, BPL, and TJAII that are strongly reactive to M2BP of hepatic cell carcinoma patients, and particularly of cases of post-operative cancer recurrence. M2BP contained in a sample collected from a subject is measured using WFA, BPL and/or TJAII, so that M2BP can be used as a marker for discriminating a group of patients with a high risk of hepatic cell carcinoma. Also, M2BP contained in a sample collected from a subject is measured using AAL and/or RCA120, so that M2BP can be used as a marker for identifying fiber formation in the liver, a cirrhosis detection marker, or a hepatic cell carcinoma detection marker. Also, WFA is periodically used for a patient after extraction of hepatic cell carcinoma and then M2BP in a sample collected from the patient is measured, so that a risk of recurrence can be predicted. In addition, there are very few molecules capable of binding to WFA in glycoproteins contained in serum, thereby enabling the direct use of serum as a measurement sample. WFA is preferable since the degree of freedom resulting from the use of WFA is high upon construction of a measurement system.
In addition, the measured values of M2BP binding to WFA, BPL, AAL, RCA120, or TAJII are preferably normalized using the measured value of M2BP binding to a lectin the reactivity of which substantially remains unchanged regardless of changes in M2BP glycan structure. As such a lectin, DSA is preferable. Also, the measured values of M2BP binding to WFA, BPL, AAL, RCA120, or TAJII may be normalized using the measured value of M2BP core protein contained in a sample collected from a subject.
Measurement of AGP binding to AOL, MAL, or DSA and measurement of M2BP binding to WFA, BPL, AAL, RCA120, or TAJII are preferably performed by the antibody-overlay lectin microarray method. In particular, the antibody-overlay lectin microarray method is capable of simultaneously measuring AGP or M2BP binding to a plurality of types of lectin. Also, when markers such as AGP and M2BP are rapidly measured using lectin “A,” measurement is preferably performed by the following 1st or 2nd rapid measurement method.
An example of the 1st rapid measurement method is a method for quantitatively determining AGP reacting with the above lectin “A” by mixing biotinylated lectin “A” prepared by binding biotin to lectin “A” with a sample, adding magnetic particles to which streptavidin has been immobilized to the mixture, so as to form a magnetic particle-lectin “A”-AGP complex, reacting the complex with a labeled anti-AGP antibody, so as to form a 2nd complex of magnetic particle-lectin “A”-AGP-labeled anti-AGP antibody, and then measuring the amount of the label of the 2nd complex. In addition, M2BP can be measured in a manner similar to that in the above method for measuring AGP except for the use of a labeled anti-M2BP antibody. With the 1st rapid measurement method, AGP or M2BP in a sample can be quantitatively determined within about 60 minutes. With the use of biotinylated lectin “A” and streptavidin-immobilized magnetic particles, the reactivity of lectin “A” to AGP or M2BP in a sample can be improved and the reaction time of lectin “A” with AGP or M2BP can be shortened to about 30 minutes.
Furthermore, an example of the 2nd rapid measurement method is a method for quantitatively determining AGP reacting with lectin “A” by mixing magnetic particles to which lectin “A” has been immobilized with a sample, capturing AGP sugar chains in the sample using lectin “A,” reacting AGP captured by the magnetic particles with a labeled anti-AGP antibody, so as to form a magnetic particle-lectin “A”-AGP-labeled anti-AGP antibody complex, and then measuring the amount of the label of the complex. Also with the 2nd rapid measurement method, M2BP can be measured in a manner similar to the above method for measuring AGP except for the use of a labeled anti-M2BP antibody. With the 2nd rapid measurement method, AGP or M2BP in a sample can be quantitatively determined within about 20 minutes. Specifically with the use of lectin “A”-immobilized magnetic particles, the reactivity of lectin “A” to AGP or M2BP in a sample is significantly improved and thus the reaction time of lectin “A” with AGP or M2BP can be shortened to about 5 minutes.
The 1st and the 2nd rapid measurement methods are suitable for automation. In particular, the 2nd rapid measurement method can be appropriately performed with full automatic measuring equipment. Automation of the 2nd rapid measurement method makes it possible to easily perform consecutive measurement of multiple specimens. Also, automation makes it possible to perform measurement of a single specimen for multi test items (measurements using different lectins) within a short period of time.
As labels for labeled anti-AGP antibodies or labeled anti-M2BP antibodies, fluorescent substances or enzymes can be used. Examples of a fluorescent substance include fluorescein isothiocyanate (FITC), a green fluorescent protein (GFP), and luciferin. Examples of an enzyme include alkaline phosphatase (ALP), peroxidase, glucose oxidase, tyrosinase, and acid phosphatase. When alkaline phosphatase is used as an enzyme, a known luminescent substrate, a known chromogenic substrate, and the like can be used. Examples thereof include chemiluminescent substrates such as CDP-star (registered trademark)(4-chloro-3-(methoxyspiro{1,2-dioxetane-3,2′-(5′-chloro) tricyclo [3.3.1.13,7]decane}-4-yl) phenylphosphate disodium), and CSPD (registered trademark) (3-(4-methoxyspiro{1,2-dioxetane-3,2-(5′-chloro) tricyclo [3.3.1.13,7]decane}-4-yl) phenylphosphate disodium), and chromogenic substrates such as p-nitrophenyl phosphate, 5-bromo-4-chloro-3-indolyl-phosphoric acid (BCIP), 4-nitroblue tetrazolium chloride (NBT), and iodonitrotetrazolium (INT). Furthermore, an antibody is labeled with biotin, and then the above fluorescent substance to which streptavidin has been bound or the above enzyme may be bound to the antibody via biotin-avidin binding.
A blood sample contains a trace amount of AGP or M2BP having glycan structural changes due to fiber formation in the liver. Hence, it is preferable to use an enzyme as a label and a luminescent substrate in view of high sensitivity and more rapid detection of the label.
In addition, an enzyme such as ALP has sugar chains. Hence, a deglycosylated enzyme is preferably used to prevent a nonspecific reaction between the sugar chains and a lectin. As such a deglycosylated enzyme, deglycosylated ALP can be used, such as Recombinant AP, EIA Drade, and CR 03535452 (Roche Diagnostics).
Also, an anti-AGP antibody or an anti-M2BP antibody also has sugar chains. Hence, a deglycosylated antibody is preferably used to prevent a nonspecific reaction between sugar chains and lectins. For example, an anti-AGP antibody or an anti-M2BP antibody converted to Fab′ as a result of pepsin digestion and reduction is preferably used.
A labeled antibody reagent is prepared as follows. According to a known method, an anti-AGP antibody or an anti-M2BP antibody is mixed with a maleimidized label using a cross-linking agent such as EMCS [N-(6-Maleimidocaproyloxy)succinimido] (DOJINDO LABORATORIES) for reaction, so that a labeled antibody can be prepared. For example, deglycosylated ALP is maleimidized using a cross-linking agent, followed by reaction with an anti-AGP antibody or an anti-M2BP antibody converted to Fab′. The use of the thus prepared antibody is preferable in view of prevention of nonspecific reaction.
5. Novel Specific Polyclonal Antibodies and/or Monoclonal Antibodies Using Novel Glycan Markers as Indices for Clinical Conditions of Liver Disease
In the method for detecting hepatic cell carcinoma using novel glycan markers as indices for clinical conditions of liver disease, when a polyclonal antibody and/or a monoclonal antibody specific to glycan markers as indices for clinical conditions of liver disease can be easily obtained, these antibodies can be used. However, when the antibodies cannot be easily obtained, they can be prepared as follows, for example.
5-1. Preparation of AntibodiesThe novel glycan markers as indices for clinical conditions of liver disease of the present invention can be used for preparing a polyclonal antibody or a monoclonal antibody for detection of liver disease.
For example, antibodies against novel glycan markers as indices for clinical conditions of liver disease can be prepared by a known method. Freund's complete adjuvant is administered at the same time, so that the generation of an antibody can be boosted. Also, a peptide including a binding position to which sugar chain X has bound is synthesized, the peptide is covalently bound to commercially available keyhole limpet hemocyanin (KLH), and then the conjugate is administered to an animal. In addition, a granulocyte-macrophage colony stimulating factor (GM-CSF) is administered at the same time, so that antibody production can be boosted.
Also, for example, monoclonal antibodies against novel glycan markers as indices for clinical conditions of liver disease can be prepared by the methods of Keller and Milstein (Nature Vol. 256, pp. 495-497 (1975)). For example, a hybridoma is prepared by cell fusion of antibody-producing cells obtained from an animal immunized with an antigen with myeloma cells, and then clones producing an anti-X antibody are selected from the thus obtained hybridoma.
Specifically, an adjuvant is added to the thus obtained glycan markers as indices for clinical conditions of liver disease for antigens. Examples of an adjuvant include Freund's complete adjuvant and Freund's incomplete adjuvant. Any of these adjuvants may be mixed.
An antigen obtained as described above is administered to a mammal such as a mouse, a rat, a horse, a monkey, a rabbit, a goat, or sheep. Any immunization method can be employed herein, as long as it is an existing method. Immunization is mainly performed by intravenous injection, subcutaneous injection, intraperitoneal injection, or the like. Also, the immunization interval is not particularly limited and immunization is performed at intervals of several days to several weeks and preferably at intervals of 4 to 21 days.
On days 2 to 3 after the final immunization date, antibody-producing cells are collected. Examples of antibody-producing cells include spleen cells, lymph node cells, and peripheral blood cells.
As myeloma cells to be fused to antibody-producing cells, cells of established cell lines from various animals (e.g., mice, rats, and humans), which are generally available for persons skilled in the art, are used. Cell lines to be used herein have properties such that they have drug resistance and are unable to survive in an unfused state, but are able to survive only in a fused state in a selective medium (e.g., HAT medium). In general, an 8-azaguanine-resistant strain is used. This cell line is deficient in hypoxanthine-guanine-phosphoribosyltransferase and is unable to grow in a hypoxanthine.aminopterin.thymidine (HAT) medium.
Myeloma cells of various known cell lines are appropriately used, such as P3 (P3x63Ag8.653) (J. Immunol. 123, 1548-1550 (1979)), P3x63Ag8U.1 (Current Topics in Microbiology and Immunology 81, 1-7 (1978)), NS-1 (Kohler, G. and Milstein, C., Eur. J. Immunol. 6, 511-519 (1976)), MPC-11 (Margulies, D. H. et al., Cell 8, 405-415 (1976)), SP2/0 (Shulman, M. et al., Nature 276, 269-270 (1978)), FO (de St. Groth, S. F. et al., J. Immunol. Methods 35, 1-21 (1980)), 5194 (Trowbridge, I. S., J. Exp. Med. 148, 313-323 (1978)), and R210 (Galfre, G. et al., Nature 277, 131-133 (1979)).
Next, the above myeloma cells are fused to antibody-producing cells. Cell fusion is performed by bringing myeloma cells into contact with antibody-producing cells at a mixture ratio ranging from 1:1 to 1:10 in the presence of a fusion accelerator at 30° C. to 37° C. for 1 to 15 minutes in a medium for culturing animal cells, such as MEM, DMEM, or RPME-1640 medium. A fusion accelerator with an average molecular weight between 1,000 and 6,000 such as polyethylene glycol or polyvinyl alcohol, or a fusion virus such as Sendai virus can be used for acceleration of cell fusion. Also, antibody-producing cells can also be fused to myeloma cells using a commercially available cell fusion apparatus using electrical stimulation (e.g., electroporation).
A hybridoma of interest is selected from cells after cell fusion. An example of a method for selection is a method using selective growth of cells in a selective medium. Specifically, cell suspension is diluted with an appropriate medium and then spread over a microtiter plate. A selective medium (e.g., HAT medium) is added to each well, and then cells are cultured while appropriately exchanging selective media. As a result, cells that have grown can be obtained as hybridoma cells.
Screening for a hybridoma is performed by limiting dilution, a fluorescence excitation cell sorter method, or the like, and then finally a monoclonal-antibody-producing hybridoma is obtained. Examples of a method for collecting a monoclonal antibody from the thus obtained hybridoma include a general cell culture method and a method for forming ascites.
Also, an antibody to be used in the present invention may be a monoclonal antibody or a polyclonal antibody. Examples of such an antibody include single-chain Fvs (scFv), a single-chain antibody, a Fab fragment, a F(ab′) fragment, and disulfide linkage Fvs (sdFv). Furthermore, as an antibody to be used in not only the 1st or the 2nd rapid measurement method, but also the present invention, a deglycosylated antibody is preferably used to prevent a nonspecific reaction between a sugar chain and a lectin. For example, an anti-AGP antibody or an anti-M2BP antibody converted to Fab′ as a result of pepsin digestion and reduction can be used.
EXAMPLES Example 1: Use of Glycan-Marker Glycoproteins as Indices for Clinical Conditions of Liver Disease for Detection of Liver DiseaseLiver disease was detected by antibody-overlay lectin array performed for glycan-marker glycoproteins as indices for clinical conditions of liver disease, AGP and Mac2BP (M2BP), as follows. In addition,
1. Enrichment of Marker Proteins from Serum
Enrichment of the marker glycoproteins derived from the sera of (viral) hepatitis patients (CH), cirrhosis patients (LC), hepatic cell carcinoma patients (HCC), and healthy subjects (HV) was performed according to “Kuno A, Kato Y, Matsuda A, Kaneko M K, Ito H, Amano K, Chiba Y, Narimatsu H, Hirabayashi J. Mol Cell Proteomics. 8, 99-108 (2009).” In addition, five cases each were used for analysis of each clinical condition in order to clarify the dependence of the obtained results on clinical conditions. Each patient's serum was diluted 10-fold with a 0.2% SDS-containing PBS buffer and then heated for 10 minutes at 95° C. Five (5) μL of the resultant was dispensed in the case of AGP and 20 μL of the same was dispensed in the case of Mac2BP to reaction tubes, and then 500 ng of an antibody (biotinylated antibody) against each antigen was added to the reaction tubes. Each reaction solution was adjusted with a reaction buffer (1% Triton X-100-containing Tris-buffered saline (TBSTx)) to 45 μL, followed by 2 hours of shaking reaction at 4° C. Immediately after antigen-antibody reaction, 5 μL (corresponding to 10 μL of the original beads solution) of a solution of magnetic beads with streptavidin immobilized thereto (Dynabeads MyOne Streptavidin T1, DYNAL Biotech ASA), which had been washed 3 times in advance with a reaction buffer and then concentrated 2-fold for adjustment, was added to the above reaction solution, followed by further 1 hour of reaction. As a result of the reaction, the glycoproteins formed complexes with magnetic beads via the biotinylated antibody. The complexes were adsorbed to magnet for recovery of magnetic beads and then the solution was discarded. The thus recovered complexes were washed 3 times with 500 μL of a reaction buffer and then suspended in 10 μL of an elution buffer (0.2% SDS-containing TBS). The suspension solution was heated at 95° C. for 5 minutes, so as to dissociate and elute the glycoproteins from magnetic beads. The thus obtained solution was designated an eluate. At this time, heat-denatured biotin antibodies are also mixed thereinto. Hence, 10 μL (corresponding to 20 μl of the original beads solution) of a magnetic beads solution that had been concentrated 2-fold for adjustment by the above-mentioned technique was added to the eluate, followed by 1 hour of reaction. Thus, adsorption removal of biotinylated antibodies was performed. The thus obtained solution was designated as a serum-derived glycoprotein solution and used for the following experiments.
2. Antibody-Overlay Lectin ArrayAn appropriate amount of the above-obtained glycoprotein solution was adjusted with a lectin array reaction buffer (1% Triton X-100-containing phosphate-buffered saline (PBSTx)) to 60 μL. The solution was added to each reaction vessel (8 reaction vessels were formed per glass slide) for a lectin microarray, followed by 10 or more hours of reaction at 20° C. The lectin microarray base comprising 8 reaction vessels was prepared according to the techniques of Uchiyama et al., (Proteomics 8, 3042-3050 (2008)). Thus, a binding reaction between sugar chains on the glycoproteins and 43 types of lectin immobilized on the array substrate reached an equilibrium state. Subsequently, to prevent sugar chains on antibodies for detection from binding to unreacted lectins on the base, so as to generate noise, 2 μL of a human serum-derived IgG solution (Sigma) was added and then reaction was performed for 30 minutes. Each reaction vessel was washed 3 times with 60 μL of PBSTx and then 2 μL of a human serum-derived IgG solution was added again. After slight stirring, a 100 ng equivalent of an antibody (biotinylated antibody for detection) against each glycoprotein to be detected, was added to the solution, followed by 1 hour of reaction at 20° C. After antigen-antibody reaction, each reaction vessel was washed 3 times with 60 μL of PBSTx, and then a PBSTx solution containing a 200 ng equivalent of Cy3-labeled streptavidin was added, followed by further 30 minutes of reaction at 20° C. After reaction, each reaction vessel was washed 3 times with 60 μL of PBSTx, and then array scanning was performed using an array scanner GlycoStation (MORITEX Corporation).
Of the thus obtained results, a typical example of each clinical condition resulting from the use of AGP is shown in
As shown in Example 1, glycoproteins were chosen by statistical analysis from the lectin signal information obtained by the antibody-overlay lectin array analysis of glycoproteins. The use of the thus selected optimum glycoprotein leads to the possibility of detecting liver disease with each type of clinical condition.
Accordingly, an experiment was conducted with the following procedures using AGP as a target molecule.
1. Narrowing Down the Number of Lectins for Distinguishing Between Cirrhosis and HepatitisTo narrow down the number of lectin groups exhibiting signal fluctuations with the progress of fiber formation, firstly antibody-overlay lectin array analysis was conducted for AGP using sera of clinically diagnosed HCC, LC, and CH patients (10 cases each). To perform more objective narrowing down, Student T test was performed for HCC-LC and LC-CH. Lectins with a risk of 0.1% or less were designated as useful lectins. The results are shown in Table 3. As understood from the previous experimental results (
Next, antibody-overlay lectin microarray was performed for 125 cases of a group of patients infected by hepatitis virus and pathologically diagnosed by liver biopsy for staging of fiber formation according to the procedures of Example 1. In addition, the results of staging for fiber formation in the liver in 125 cases are as follows: F0 and F1 (33 cases), F2 (32 cases), F3 (31 cases), and F4 (29 cases). According to the above procedures, lectins statistically useful for identification were narrowed down. As a result, the results for top 6 types of lectin are shown in Table 4. The thus obtained 6 lectins ranked high and particularly LEL, AOL, and MAL were selected as the most effective lectins for identification. Hence, detailed data analysis was conducted for the 3 types of lectin.
The results of measuring with time AOL, MAL, and LEL signal fluctuations in the same patient are shown in
It was demonstrated by the above results that the independent use of or a combined use of AOL and MAL signal fluctuations makes it possible to identify the progress of fiber formation in the liver.
Example 3: Detection of Cirrhosis by Antibody-Overlay Lectin Array Analysis for AGP Glycan-Marker Glycoprotein as an Index for Clinical Conditions of Liver DiseaseIt was considered based on the results of Example 2 that determination of a cut-off value of each lectin (signals) or a combination of lectin signals on the basis of the progress of fiber formation in the liver enables detection of cirrhosis. Hence, an experiment was conducted with the following procedures.
1. Determination of Lectin Signal⋅Cut-Off Values for Detection of cirrhosis
First, a cut-off value was determined for each lectin in order to detect a patient with cirrhosis from among patients infected by hepatitis virus. For this purpose, a receiver operating characteristic curve (ROC curve) for distinguishing F4 (cirrhosis) from the other stages (F1-F3) was created for 80 cases of pathologically diagnosed patients (F1, F2, F3, and F4 (20 cases each)) with the use of data obtained by normalization of 2 types of lectin signal narrowed down in Example 2 with DSA lectin signals. The results are shown on the left in
Antibody-overlay lectin array was performed for 45 cases of clinically diagnosed chronic hepatitis patients and 43 cases of clinically diagnosed cirrhosis patients according to the procedures in Example 2 using AGP as a target molecule. All signals were normalized with the signal of DSA lectin, which had been designated as 100%. The numerical values were determined to be positive or negative using the above-mentioned cut-off values, so that cirrhosis detection was tested. As a result, when AOL signals were used, the detection ability was represented by the sensitivity of 86.1%, the specificity of 91.1%, and the accuracy of 88.6%. When MAL signals were used, the detection ability was represented by the sensitivity of 90.7%, the specificity of 88.9%, and the accuracy of 89.8%. Significantly high-level detection was possible in both cases, such that the accuracy exceeded 85%. Moreover, the detection ability was examined using an equation with a combined use of two signals ((relative signal intensity of AOL)×1.5−(relative signal intensity of MAL)). Thus, the most reliable cirrhosis detection result was obtained, such that the sensitivity was 95.4%, the specificity was 91.1%, and the accuracy was 93.2%. It is particularly worth noting that the detection ability was overwhelmingly higher than those of known techniques for detection of disease-specific glyco-alterations in AGP using AAL lectin or RCA lectin. These results agree with the result of the narrowing-down step using antibody-overlay lectin array in which AAL and RCA120 were inferior to AOL and MAL (see Table 3 and Table 4).
Example 4: Determination of Therapeutic Effects of an Interferon Using a Marker Capable of Monitoring the Progress of Fiber Formation in the LiverIt was demonstrated based on the results of Example 2 that the progress of fiber formation can be monitored through observation of AOL and MAL signal fluctuations. Hence, the therapeutic effects of an interferon that is an antiviral agent were experimentally determined using AOL/DSA or MAL/DSA as a parameter indicating the progress of fiber formation. The following experiment was conducted for type C hepatitis patients of a sustained virological responder (SVR) group for which the therapeutic effects of the interferon had been confirmed and a non-virological responder (NVR) group for which no therapeutic effect thereof had been confirmed. After interferon treatment, patients' sera from blood collected with time were subjected to enrichment of AGP in serum and antibody-overlay lectin microarray analysis by techniques similar to those in Example 1. After normalization with DSA signals, relative signal values of AOL and MAL were calculated. The time course changes in each signal (typical results of the SVR group and the NVR group (2 cases each)) are shown in
Preparation of R1 reagent: R1 reagent 1 was prepared by adding 5 μg/mL biotinylated DSA (J-OIL MILLS, INC.) to buffer A (PBS-1% TritonX, pH7.4). R1 reagent 2 was prepared by adding 5 μg/mL biotinylated MAL (Vector) to buffer A. R1 reagent 3 was prepared by adding 2.5 μg/mL biotinylated AOL to buffer A. In addition, biotinylated AOL used herein was prepared by biotinylation of AOL (Tokyo Kasei Kogyo Co., Ltd.) using a biotin labeling kit (DOJIDO).
Preparation of R2 reagent: An R2 reagent was prepared by adding magnetic particles (number average particle size: 2 μm) to which streptavidin had been immobilized to buffer A to 0.5 w/v %.
Preparation of R3 reagent: A solution containing a 0.025 U/mL ALP-labeled mouse anti-AGP monoclonal antibody, 0.1 M MES (2-(N-Morpholino)ethanesulfonic acid, pH6.5), 0.15 M sodium chloride, 1 mM magnesium chloride, 0.1 mM zinc chloride, 0.1 w/v % NaN3, and 0.5 w/v % casein Na was prepared and then designated as R3 reagent 1. R3 reagent 2 was prepared in a manner similar to that for R3 reagent 1 except for the use of a 0.5 U/mL ALP-labeled mouse anti-AGP monoclonal antibody instead of a 0.025 U/mL ALP-labeled mouse anti-AGP monoclonal antibody.
Preparation of R4 reagent: A solution containing 0.1 M 2-amino-2-methyl-1-propanol (AMP, pH 9.6), 1 mM magnesium chloride, and 0.1 w/v % NaN3 was prepared and then designated as an R4 reagent.
Preparation of R5 reagent: CDP-Star with Sapphirine-II (luminescent substrate for ALP, Applied Biosystems) was designated as an R5 reagent.
Preparation of washing reagent: A solution containing 20 mM tris (pH7.4), 0.1 w/v % Tween20, 0.1 w/v % NaN3, and 0.8 w/v % sodium chloride was prepared, and then designated as a washing reagent.
1-2. Confirmation of Dilution Linearity of DSAAGP in Consera (normal human serum, Nissui Pharmaceutical Co., Ltd.) was recovered in buffer B (TBS-0.5% TritonX-0.1% SDS) using an anti-AGP antibody in a manner similar to that for enrichment in Example 1 and then used as a sample. The thus recovered sample was diluted 1-fold, ½-fold, ¼-fold, ⅛-fold, and 1/16-fold, respectively, with buffer B so that diluted samples were prepared.
R1 reagent 1 (110 μL) was added to 30 μL of each diluted sample. After 2 minutes of reaction at room temperature, 30 μL of the R2 reagent was added and then reaction was performed for 30 minutes at room temperature. Magnetic particles bearing the complex of DSA and AGP were collected for B/F separation, the separated magnetic particles were washed using a washing reagent, and then the solution was discarded. This treatment was performed 4 times. R3 reagent 1 (100 μL) was added to the washed magnetic particles, followed by 20 minutes of reaction at room temperature, so that AGP in the complex on magnetic particles was reacted with the ALP-labeled mouse anti-AGP monoclonal antibody. Collected magnetic particles bearing the complex of the ALP-labeled mouse anti-AGP monoclonal antibody, AGP, and DSA were subjected to the removal of liquid components (B/F separation), the thus separated magnetic particles were washed with a washing reagent, and then the solution was discarded. This treatment was performed 4 times. Complex-bearing magnetic particles were dispersed in 50 μL of the R4 reagent, 100 μL of the R5 reagent was added, and then chemiluminescence intensity due to ALP was measured as a photo count value using a luminescence measurement apparatus. The results are shown in
An experiment was conducted for confirmation of dilution linearity in a MAL measurement system in a manner similar to that in “confirmation of dilution linearity of DSA” except for the use of R1 reagent 2 instead of R1 reagent 1 and the use of R3 reagent 2 instead of R3 reagent 1. The results are shown in
An experiment was conducted for confirmation of dilution linearity in an AOL measurement system in a manner similar to that in “confirmation of dilution linearity of DSA” except for the use of HCV-positive blood plasma 2 (Millenium Biotech) instead of Consera and the use of R1 reagent 3 instead of R1 reagent 1. The results are shown in
Consera (normal human serum, Nissui Pharmaceutical Co., Ltd.), normal human serum (TRINA), and HCV-positive blood plasma 1 and 2 (Millenium Biotech) were each subjected to AGP separation using an anti-AGP antibody in a manner similar to that for enrichment in Example 1. The resultants were then each recovered in a buffer (TBS-0.5% TritonX-0.1% SDS) and then used as samples for measurement. Also, a buffer alone was used as a sample (NC) for blank measurement.
R1 reagent 1 (110 μL) was added to 30 μL of each measurement sample. After 2 minutes of reaction at room temperature, 30 μL of the R2 reagent was added and then reaction was performed at room temperature for 30 minutes. Magnetic particles bearing the complex of DSA and AGP were collected for B/F separation, the separated magnetic particles were washed with a washing reagent, and then the solution was discarded. This treatment was performed 4 times. R3 reagent 1 (100 μL) was added to the washed magnetic particles, reaction was performed at room temperature for 20 minutes, and then AGP in the complex on magnetic particles was reacted with the ALP-labeled mouse anti-AGP monoclonal antibody. Magnetic particles bearing the complex of the ALP-labeled mouse anti-AGP monoclonal antibody, AGP, and DSA were collected for B/F separation, the separated magnetic particles were washed with a washing reagent, and then the solution was discarded. This treatment was performed 4 times. Complex-bearing magnetic particles were dispersed in 50 μL of the R4 reagent and then 100 μL of the R5 reagent was added. Chemiluminescence intensity in the DSA measurement system was measured as a photo count value using a luminescence measurement apparatus. The time required for measurement was 65 minutes. Measurement results are shown in Table 5.
Also, chemiluminescence in the MAL measurement system was measured in a manner similar to that in the DSA measurement system except for the use of R1 reagent 2 instead of R1 reagent 1 and the use of R3 reagent 3 instead of R3 reagent 1. The results are shown in Table 5. Also, chemiluminescence in the AOL measurement system was measured in a manner similar to that in the DSA measurement system except for the use of R1 reagent 3 instead of R1 reagent 1. The results are shown in Table 5. Also, measurement results obtained using MAL and AOL are normalized with the measurement result obtained using DSA and then the thus obtained values are shown in Table 5, in addition to
Each measurement sample in the above 1-5 was subjected to measurement by an antibody overlay method using lectin arrays used in Example 1. The time for measurement required by the lectin arrays method was about 18 hours. The results are shown in Table 6, in addition to
Regarding measurement results for MAL subjected to normalization with DSA, it was demonstrated that the measurement results obtained by the Pt measurement method shown in the embodiment (shown in
Preparation of R1 reagent: Buffer A (PBS-1% TritonX, pH7.4) was designated as an R1 reagent.
Preparation of R2 reagent: Magnetic particles (number average particle size: 2 μm) to which streptavidin had been immobilized was added to buffer A to 0.5 w/v % and then 2.5 μg/mL biotinylated DSA (J-OIL MILLS, INC.) was added, followed by 30 minutes of stirring at room temperature. After stirring, the magnetic particles were collected and then precipitated, so that solution components were discarded. Buffer A was added to the resultant and then stirred. Magnetic particles were collected and then precipitated, so that solution components were discarded. This procedure was repeated 3 times. Buffer A was added to the resultant so that the concentration of magnetic particles was 0.5 w/v %. The thus obtained solution containing DSA-bearing magnetic particles was designated as R2 reagent 1. R2 reagent 2 containing MAL-bearing magnetic particles was prepared in a manner similar to that for R2 reagent 1 except for the use of 25 μg/mL biotinylated MAL (Vector) instead of 2.5 μg/mL biotinylated DSA (J-OIL MILLS, INC.). R2 reagent 3 containing AOL-bearing magnetic particles was prepared in a manner similar to that for R2 reagent 1 except for the use of 25 μg/mL biotinylated AOL instead of 2.5 μg/mL biotinylated DSA (J-OIL MILLS, INC). In addition, biotinylated AOL used herein was prepared by biotinylation of AOL (Tokyo Kasei Kogyo Co., Ltd.) using a biotin-labeling kit (DOJIDO).
Preparation of R3 reagent: A solution containing 0.1 U/mL ALP (Recombinant AP, EIA Drade, CR 03535452)-labeled mouse anti-AGP monoclonal antibody-Fab′, 0.1 M MES (2-(N-Morpholino) ethanesulfonic acid, pH6.5), 0.15 M sodium chloride, 1 mM magnesium chloride, 0.1 mM zinc chloride, 0.1 w/v % NaN3, and 0.25 w/v % casein Na was prepared and designated as R3 reagent 1. R3 reagent 2 was prepared in a manner similar to that for R3 reagent 1 except for the use of 0.1 w/v % BSA instead of 0.25 w/v % casein Na.
In addition, in the above 1st rapid measurement method (manual method), ALP that had not been deglycosylated was used, but in the 2nd rapid measurement method, deglycosylated ALP was used.
Preparation of R4 reagent: A solution containing 0.1 M 2-amino-2-methyl-1-propanol (AMP, pH9.6), 1 mM magnesium chloride, and 0.1 w/v % NaN3 was prepared and designated as an R4 reagent.
Preparation of R5 reagent: CDP-Star with Sapphirine-II (luminescent substrate for ALP, Applied Biosystems) was designated as an R5 reagent.
Preparation of washing reagent: A solution containing 20 mM tris (pH7.4), 0.1 w/v % Tween20, 0.1 w/v % NaN3, and 0.8 w/v % sodium chloride was prepared and designated as a washing reagent.
2-2. Confirmation of Dilution Linearity of a Measurement System Using DSAAGP in Consera (normal human serum, Nissui Pharmaceutical Co., Ltd.) was recovered in buffer B (TBS-0.5% TritonX-0.1% SDS) using an anti-AGP antibody in a manner similar to that for enrichment in Example 1 and then used as a sample. The thus recovered sample was diluted 1-fold, ½-fold, ¼-fold, ⅛-fold, and 1/16-fold, respectively, with buffer B so that diluted samples were prepared.
Conditions for the operation of a full-automatic immunoassay system HISCL2000i (Sysmex) were changed to the following conditions. Chemiluminescence (photo count value) was measured for each diluted sample using the system.
Each diluted sample (30 μL) was dispensed into a vessel. After 2.25 minutes of incubation at 42° C., 30 μL of the R2 reagent 1 was dispensed, followed by 2.5 minutes of reaction at 42° C. Furthermore, 100 μL of the R3 reagent 1 was dispensed and then a reaction was performed at 42° C. for 2.75 minutes. Magnetic particles were collected by magnetic separation, so that the solution was vacuumed and discarded. The washing reagent was dispensed, magnetic particles were dispersed in and washed with the washing reagent, magnetic particles were collected by magnetic separation, and thus the solution was vacuumed and discarded. This treatment was repeated 3 times. The R4 reagent (50 μL) was dispensed, 100 μL of the R5 reagent was dispensed, and then chemiluminescence was measured. The above measurement was performed 3 times and then the results are shown in
An experiment was conducted for confirmation of dilution linearity in the MAL measurement system in a manner similar to that in “Confirmation of dilution linearity of a measurement system using DSA” except for the use of R2 reagent 2 instead of R2 reagent 1 and the use of R3 reagent 2 instead of R3 reagent 1. The results are shown in
An experiment was conducted for confirmation of dilution linearity in the AOL measurement system in a manner similar to that in “Confirmation of dilution linearity of DSA” except for the use of HCV-positive blood plasma 2 (Millenium Biotech) instead of Consera and the use of R2 reagent 3 instead of R2 reagent 1. The results are shown in
Consera (normal human serum, Nissui Pharmaceutical Co., Ltd.), normal human serum (TRINA), and HCV-positive blood plasma 1 and 2 (Millenium Biotech) were each subjected to separation of AGP by an immunoprecipitation method using an anti-AGP antibody. Resultants were each recovered in buffer B (TBS-0.5% TritonX-0.1% SDS) and used as samples for measurement. Also, buffer B alone was used as a sample for blank measurement.
Each measurement sample was measured using a full-automatic immunoassay system HISCL2000i under conditions similar to those for “confirmation of dilution linearity of a measurement system using DSA,” “confirmation of dilution linearity of a measurement system using MAL,” and “confirmation of dilution linearity of a measurement system using AOL.” The time required for each measurement was 17 minutes. The results are shown in Table 7,
Regarding the measurement results obtained using MAL subjected to normalization with the measurement result obtained using DSA, it was demonstrated that the measurement results obtained by the 2nd rapid measurement method shown in
Serum 1 and serum 2 from patients at fiber formation stage F1, serum 3 and serum 4 from patients at fiber formation stage F2, serum 5 and serum 6 from patients at fiber formation stage F3, and serum 7 and serum 8 from patients at fiber formation stage F4 were each subjected to separation of AGP using an anti-AGP antibody in a manner similar to that for enrichment in Example 1, and then recovered in buffer B (TBS-0.5% TritonX-0.1% SDS). The resultants were used as samples for measurement. Also, buffer B alone was used as a sample for blank measurement.
Each measurement sample was measured using a full-automatic immunoassay system HISCL2000i under conditions similar to those for “confirmation of dilution linearity of a measurement system using DSA,” “confirmation of dilution linearity of a measurement system using MAL,” and “confirmation of dilution linearity of AOL.” The time required for each measurement was 17 minutes. The results are shown in Table 8,
Each measurement sample of the above 2-6 was measured by an antibody overlay method using lectin arrays used in Example 1. The time required for measurement by the lectin array method was about 18 hours. The results are shown in Table 9,
It was demonstrated based on the results shown in
It was revealed by Example 5 that the 2nd rapid measurement method exhibited a pattern similar to that of a lectin array. To demonstrate the fact in more cases, the 2nd rapid measurement method was performed according to the procedures 2-6 in Example 5 for 125 cases of the patient group (same as that in Example 2) infected with hepatitis virus and pathologically diagnosed by liver biopsy for staging for fiber formation. In addition, the results of staging for fiber formation in the liver performed for 125 cases were: 33 cases at stages F0 and F1, 32 cases at stage F2, and 31 cases at F3, and 29 cases at F4.
Detection of cirrhosis by the 2nd rapid measurement method was attempted by procedures similar to those for detection of cirrhosis using lectin arrays described in Example 3. An ROC curve for distinguishing F4 (cirrhosis) from the other (F1-F3) was created for 125 cases of the above pathologically diagnosed patients using data obtained by normalization of signals on 2 types of lectin with the signals on DSA lectin. Also, a point on a curve, which is located closest to the point of 100% sensitivity and the point of 100% specificity, in other words, a contact point between a line parallel to the line of Y=X and the ROC curve, was designated as “optimum specificity and sensitivity” and in the periphery cut-off values were determined. A combination equation (AOL/DSA×1.8−MAL/DSA) optimum for detection of cirrhosis was found based on the thus obtained cut-off value for each lectin. Accordingly, a blind test was performed for 45 cases and 43 cases of patients definitively diagnosed as having hepatitis and cirrhosis by pathological diagnosis or diagnostic imaging⋅clinical diagnosis.
As a result, the detection ability examined using the combination equation (AOL/DSA×1.8−MAL/DSA) was represented by the sensitivity of 88.3%, the specificity of 91.1%, and the accuracy of 89.8%.
Next, to examine the frequency of false-positive results from the equation, sera from 100 healthy subjects were also analyzed by the 2nd rapid measurement method. Determination of cirrhosis was performed using the equation. As shown in
As described in Example 2, a possibility was found also for M2BP, such that each type of clinical condition of liver disease can be detected based on the lectin signal information obtained by antibody-overlay lectin array analysis. Hence, an experiment for examination of a correlation with fiber formation in the liver was conducted. Antibody-overlay lectin microarray was performed according to the procedures in Example 2 for 125 cases of a group of patients (same as those in the experiment for AGP) infected with hepatitis virus and pathologically diagnosed by liver biopsy for staging for fiber formation. Graphs showing correlations between 6 lectins (out of 17 types of lectin for which binding signals had been generated), for which signal changes had been confirmed by a significance difference test with the progress of fiber formation, and the progress of fiber formation were created, as shown in
A group of lectins with signal intensities that increased with the progress of fiber formation in the liver was found in Example 7. To discriminate lectins capable of discriminating a high risk group for cancer from the group of lectins, antibody-overlay lectin microarray analysis of M2BP was conducted for sera from 7 cases of preoperative and postoperative patients with hepatic cell carcinoma. The experimental procedures were employed according to Example 1. Also, with the use of a full-automatic fluorescence immunoassay apparatus (μTAS Wako i30; Wako Pure Chemical Industries, Ltd.) and a special-purpose reagent, an amount of known hepatic cell carcinoma marker AFP in the blood and benign disorder⋅hepatic cell carcinoma distinguishing marker AFP-L 3% were also measured. The resulting lectin signal patterns are partially shown in
The best mode for detection of WFA-binding M2BP as a biomarker for discriminating a high risk group for liver cancer can be a method for detecting and identifying biomarkers contained in serum by a clinically applicable convenient means with clinically acceptable performance. The results of sandwich detection analysis using an anti-M2BP antibody overlay-WFA well plate (see
Fifty (50) μL each of biotinylated WFA (Vector, 5 μg/mL) dissolved in a PBS buffer was added to each well of a microtiter plate (Greiner Bio-One, 96-well flat-bottomed streptavidin-coated plate) and then maintained at room temperature for 2 hours, so that WFA was immobilized to a support. The plate was washed twice with a wash (0.1% Tween 20-containing PBS (300 μL)) to remove unbound WFA so that the preparation of a WFA-immobilized well plate was completed.
Each sample (1 μL) was diluted with 50 μL of the above wash and then the diluted sample was added to the WFA-immobilized well plate prepared in 1, followed by 2 hours of binding reaction at room temperature. After reaction, each well was washed 5 times with 300 μL of the above wash, so that unbound proteins were removed. A detection agent (goat anti-M2BP polyclonal antibody solution; R&D Systems) adjusted in advance with a wash to 1.0 μg/mL was added with 50 μL per well, followed by 2 hours of antigen-antibody reaction at room temperature.
After washing with 300 μL of a wash to remove unbound antibodies, an anti-goat IgG antibody-HRP solution (Jackson immuno Research) diluted 10,000-fold in advance with a wash was added with 50 μL per well and then the resultants were maintained at room temperature for 1 hour. Each well was washed 5 times with 300 μL of a wash, and then an ULTRA-TMB solution (Thermo) as a coloring reagent was added with 100 μL per well, followed by 10 minutes of coloring reaction. A 1 M H2SO4 solution was added with 100 μL per well to stop the reaction, and then absorbance was measured at 450 nm using a plate reader. The serum of a healthy subject was designated as a negative control (N), numerical conversion of the thus obtained signals was performed to find S/N ratios, and then the resulting data were used for the following analysis.
ResultsFirst, assay was performed for sera from 7 cases of the above preoperative and postoperative hepatic cell carcinoma patients. As a result, signal patterns that strongly resembled to the results in
The effects of the presence or the absence of heat treatment for specimens on the sensitivity of detection of WFA-binding M2BP by an ELISA method were confirmed.
A human liver cancer-derived cell line (HepG2 culture supernatant) was diluted 10-fold with a 0.2% SDS-containing PBS buffer, followed by 10 minutes of heat treatment at 95° C.
M2BP binding to WFA was measured by a method similar to that in 2 of Example 8 except that an HepG2 culture supernatant (untreated) and an HepG2 culture supernatant (heat-treated) were used as samples so that the amount of protein per well was as listed in Table 10. Absorbance measured using a plate reader is shown in Table 10 and
It was revealed based on the results in Table 10 and
Preparation of R1 reagent: A solution (buffer C) containing 10 mM HEPES (pH 7.5), 150 mM NaCl, 0.01 mM MnCl2, 0.1 mM CaCl2, and 0.08 w/v % NaN3 was prepared and then designated as an R1 reagent.
Preparation of R2 reagent: Magnetic particles (number average particle size: 2 μm) (hereinafter, referred to as streptavidin-sensitized magnetic particles) to which commercially available streptavidin had been immobilized were added to buffer C to a concentration of 0.5 w/v %, and then a biotinylated lectin solution (WFA) was added to the solution. The mixed solution was stirred at room temperature for 30 minutes. After stirring, magnetic particles were collected with magnet for precipitation, and then solution components were discarded. After washing 3 times with buffer C, buffer D (the solution containing 10 mM HEPES (pH7.5), 150 mM NaCl, 0.01 mM MnCl2, 0.1 mM CaCl2, 0.1% W/V BSA, and 0.08 w/v % NaN3) was added so that the concentration of magnetic particles was 0.5 w/v %.
Preparation of R3 reagent: A solution containing a 0.1 U/mL recombinant ALP-labeled mouse anti-M2BP monoclonal antibody, 0.1 M MES (2-(N-Morpholino) ethanesulfonic acid, pH6.5), 0.15M NaCl, 1 mM MgCl2, 0.1 mM ZnCl2, and 0.1 w/v % NaN3 was prepared and then designated as an R3 reagent.
As an R4 reagent, an R5 reagent, and a washing reagent, the R4 reagent, the R5 reagent, and the washing reagent used in the 2nd rapid measurement method in Example 5 were used.
2. Confirmation of Dilution Linearity of a Measurement System Using WFAA human liver cancer-derived cell line culture supernatant (HepG2 culture supernatant) (100 μg/ml) was diluted 10-fold, 100-fold, 1000-fold, and 10000-fold with a buffer (PBS), so that diluted samples were prepared. Also, 5 μg/ml recombinant human galectin-3BP/MAC-2BP (R&D SYSTEMS) was diluted 2-fold, 4-fold, 8-fold, 16-fold, 32-fold, and 64-fold with a buffer (PBS), so that diluted samples were prepared.
Conditions for the operation of a full-automatic immunoassay system HISCL2000i (Sysmex) were changed to the following conditions. Chemiluminescence intensity (photo count value) was measured for each diluted sample.
The R1 reagent (30 μL) and 10 μL of each diluted sample were dispensed to a vessel. After 2.25 minutes of incubation at 42° C., 30 μL of the R2 reagent was dispensed, followed by 1.5 minutes of reaction at 42° C. Magnetic particles were collected by magnetic separation, so that the solution was vacuumed and discarded. The washing reagent was dispensed, magnetic particles were dispersed in and washed with the washing reagent and then collected by magnetic separation, so that the solution was vacuumed and discarded. This treatment was repeated 3 times. The R3 reagent (100 μL) was dispensed, followed by 2.75 minutes of reaction at 42° C. Magnetic particles were collected by magnetic separation and thus the solution was vacuumed and discarded. The washing reagent was dispensed, magnetic particles were dispersed in and washed with the washing reagent and then collected by magnetic separation, and thus the solution was vacuumed and discarded. This treatment was repeated 3 times. The R4 reagent (50 μL) was dispensed, 100 μL of the R5 reagent was dispensed, and then the chemiluminescence intensity was measured. Measurement results for the supernatant of cultured HepG2 cells are shown in Table 11 and
Sera from a healthy subject, an HBV-positive hepatic cell carcinoma patient, and an HCV-positive hepatic cell carcinoma patient were measured using a full-automatic immunoassay system HISCL2000i under conditions similar to those in “2. Confirmation of dilution linearity of a measurement system using WFA.” The time required for measurement of each specimen was 17 minutes. The results are shown in Table 13.
It could be confirmed based on the results in Table 13 that M2BP binding to WFA can be rapidly and precisely measured by the 2nd rapid measurement method.
The present invention can be used for producing apparatuses, instruments, or kits for determining liver disease or clinical conditions of liver disease, distinguishing among clinical conditions of liver disease, or detecting cirrhosis, for example.
Claims
1-30. (canceled)
31. A method for detecting cirrhosis, comprising:
- mixing a blood sample collected from a patient with liver disease, a Wisteria floribunda lectin (WFA) and an anti-Mac-2-binding protein antibody;
- assaying Mac-2-binding protein (M2BP) binding to both the WFA and the anti-M2BP antibody; and
- determining whether or not the liver disease is cirrhosis based on the assayed value of the M2BP.
32. The method according to claim 31, wherein the blood sample is a serum.
33. The method according to claim 31, wherein the mixing is performed by mixing the blood sample and the WFA, and mixing the M2BP antibody and a mixture of the blood sample and the WFA.
34. The method according to claim 31, wherein the WFA is immobilized on a particle.
35. The method according to claim 34, wherein the particle is a magnetic particle.
36. The method according to claim 35, wherein the WFA is a biotinylated WFA, and the magnetic particle is a streptavidin or an avidin immobilized magnetic particle.
37. The method according to claim 31, wherein the anti-M2BP antibody is a labeled anti-M2BP antibody, and a label of the labeled anti-M2BP antibody is a fluorescent substance or an enzyme.
38. The method according to claim 37, wherein the fluorescent substance is selected from a fluorescein isothiocyanate, a green fluorescent protein and a luciferin.
39. The method according to claim 37, wherein the enzyme is selected from an alkaline phosphatase, a peroxidase, a glucose oxidase, a tyrosinase and an acid phosphatase.
40. The method according to claim 37, wherein the enzyme is the alkaline phosphatase, which is assayed by using a luminescent substrate or a chromogenic substrate.
41. The method according to claim 31, wherein the WFA selectively binds to glycoproteins having a specific glycan structure in the blood sample, the anti-M2BP antibody binds to a core protein of Mac-2-binding protein, and a glycoprotein binding both the WFA and the anti-M2BP antibody is the glycan structure changed Mac-2-binding protein.
42. A method for distinguishing cirrhosis and hepatitis, comprising:
- providing a Wisteria floribunda lectin (WFA) and an anti-Mac-2-binding protein antibody;
- assaying Mac-2-binding protein (M2BP) which is contained in a blood sample collected from a patient with liver disease and binds to both the WFA and the anti-M2BP antibody; and
- determining whether the liver disease is cirrhosis or hepatitis based on the assayed value of the M2BP.
43. The method according to claim 42, wherein the blood sample is a serum sample.
44. The method according to claim 42, wherein the WFA is immobilized on a particle.
45. The method according to claim 44, wherein the particle is a magnetic particle.
46. The method according to claim 42, wherein the anti-M2BP antibody is a labeled anti-M2BP antibody, and a label of the labeled anti-M2BP antibody is a fluorescent substance or an enzyme.
47. The method according to claim 46, wherein the enzyme is the alkaline phosphatase, which is assayed by using a luminescent substrate or a chromogenic substrate.
48. The method according to claim 42, wherein the WFA selectively binds to glycoproteins having a specific glycan structure in the blood sample, the anti-M2BP antibody binds to a core protein of Mac-2-binding protein, and a glycoprotein sandwiched by the WFA and the anti-M2BP antibody is the glycan structure changed Mac-2-binding protein.
49. A method for detecting cirrhosis, comprising:
- providing a Wisteria floribunda lectin (WFA) and an anti-Mac-2-binding protein antibody;
- assaying Mac-2-binding protein (M2BP) which is contained in a blood sample collected from a patient with liver disease and binds to both the WFA and the anti-M2BP antibody; and
- determining whether or not the liver disease is cirrhosis based on the assayed value of the M2BP.
50. The method according to claim 49, wherein the blood sample is a serum.
51. The method according to claim 49, wherein the WFA is immobilized on a particle.
52. The method according to claim 51, wherein the particle is a magnetic particle.
53. The method according to claim 49, wherein the anti-M2BP antibody is a labeled anti-M2BP antibody, and a label of the labeled anti-M2BP antibody is a fluorescent substance or an enzyme.
54. The method according to claim 49, wherein the enzyme is the alkaline phosphatase, which is assayed by using a luminescent substrate or a chromogenic substrate.
55. A method for detecting a risk of recurrence of hepatic cell carcinoma, comprising:
- providing a Wisteria floribunda lectin (WFA) and an anti-Mac-2-binding protein antibody;
- assaying Mac-2-binding protein (M2BP) which is contained in a blood sample collected from a patient with hepatic cell carcinoma after operation and binds to both the WFA and the anti-M2BP antibody; and
- determining whether the patient has a high possibility of non-recurrence of hepatic cell carcinoma based on the assayed value of the M2BP.
56. The method according to claim 55, wherein the blood sample is a serum.
57. The method according to claim 55, wherein the WFA is immobilized on a particle.
58. The method according to claim 57, wherein the particle is a magnetic particle.
59. The method according to claim 55, wherein the anti-M2BP antibody is a labeled anti-M2BP antibody, and a label of the labeled anti-M2BP antibody is a fluorescent substance or an enzyme.
Type: Application
Filed: Nov 10, 2017
Publication Date: Apr 19, 2018
Inventors: Hisashi Narimatsu (Tsukuba-shi), Yuzuru Ikehara (Tsukuba-shi), Atsushi Kuno (Tsukuba-shi), Maki Sogabe (Tsukuba-shi), Yasuhito Tanaka (Nagoya-shi), Masashi Mizokami (Ichikawa-shi), Kiyoaki Ito (Ichikawa-shi), Shunsuke Matsubara (Kobe-shi), Chikayuki Tsuruno (Kobe-shi), Youichi Takahama (Kobe-shi), Takashi Kagawa (Kobe-shi), Shinya Nagai (Kobe-shi)
Application Number: 15/809,160