The present invention relates to a method for immunoassay for measuring an autoantibody against Ku86 and a kit for the immunoassay. In particular, an autoantibody against Ku86 occurs specifically in the blood of a patient with primary hepatocellular carcinoma. Thus, the present invention not only provides a method of measuring the autoantibody, but also may be utilized for determination of primary hepatocellular carcinoma.
Ku86 is a protein which is involved in cleavage of double-stranded DNA, and, together with Ku70, forms a heterodimer, referred to as Ku. The Ku heterodimer has been described to be capable of repairing double-stranded DNA breaks in cooperation with a DNA dependent protein kinase and the like (Non Patent Literature 1).
Meanwhile, it has been revealed that according to a modified agarose two-dimensional electrophoresis in which 2D-DIGE technique (two-dimensional fluorescence difference gel electrophoresis) is applied to agarose two-dimensional electrophoresis (Non Patent Literature 2), by comparing the protein expression levels between a cancerous part of primary hepatocellular carcinoma and a peripheral non-cancerous tissue using proteomic analysis, a protein Ku86 is expressed at a higher level in the cancerous part (Non Patent Literature 3).
Non Patent Literature 1: Li et al., Proc. Natl. Acad. Sci. USA, Vol.9, No.2, 832-837, 2002
Non Patent Literature 2: Takeshi Tomonaga et al., Clin. Cancer Res. 2004;10:2007-2014
Non Patent Literature 3: Masanori Seimiya et al., Hepatology 2008;48:519-30
The present inventors have found that, by measuring an expression level of Ku86 present in a tissue specimen derived from a patient suspected of having carcinoma or a patient with carcinoma, a cancerous part can be distinguished from a non-cancerous part in those tissues. The present inventors have further carried on the study on the presence of Ku86 in a blood specimen, and surprisingly found that an autoantibody against Ku86 may be present in a blood specimen, and the amount of the autoantibody is specifically abundant in a case of a patient with primary hepatocellular carcinoma. Therefore, an object of the present invention is to provide a method of measuring an autoantibody against Ku86, which can be applied to the determination of primary hepatocellular carcinoma.
The present inventors have found that an autoantibody against Ku86 can be measured by reacting the autoantibody in a specimen with a Ku86 antigen as a reagent, and measuring the resulting immune complex between the autoantibody and the Ku86 antigen with a labeled anti-human immunoglobulin antibody, thereby allowing the determination of carcinoma, and then completed the present invention.
Thus, the present invention relates to a method for immunoassay of an autoantibody against Ku86 characterized in that the autoantibody is measured by reacting the autoantibody against Ku86 in a specimen with a Ku86 antigen as a reagent, and measuring the resulting immune complex between the autoantibody against Ku86 and the Ku86 antigen.
Furthermore, the present invention relates to a kit for immunoassay of an autoantibody against Ku86, characterized by comprising at least a Ku86 antigen as a reagent component.
Furthermore, the present invention relates to a method of determining primary hepatocellular carcinoma, wherein the primary hepatocellular carcinoma is determined by measuring an autoantibody against Ku86.
Furthermore, the present invention relates to a marker for determination of primary hepatocellular carcinoma, comprising an autoantibody against Ku86.
The present invention can easily measure an autoantibody against Ku86 present in a specimen, in particular, a specimen derived from blood, and it is effective for determination of a patient with primary hepatocellular carcinoma.
The method for immunoassay of autoantibody against Ku86 of the present invention is characterized in that the autoantibody against Ku86 is measured by reacting the autoantibody against Ku86 in a specimen with a Ku86 antigen as a reagent, and measuring the resulting immune complex between the autoantibody against Ku86 and the Ku86 antigen.
In the present invention, a specimen is preferably a sample derived from an organism, in particular, a specimen derived from blood is preferred, and examples of a specimen derived from blood may include whole blood, blood plasma, and serum.
The subject to be measured by the method for immunoassay of the present invention is an autoantibody against Ku86. As described above, Ku86 is a protein which is involved in cleavage of double-stranded DNA, its formal name being ATP-dependent DNA helicase 2 subunit 2. It is otherwise referred to as XRCC5. Additionally, Ku86 is an 82 kDa protein consisting of 732 amino acids, and its accession number (accession No.) in the US National Center for Biotechnology Information (NCBI) is gi-10863945.
To perform the method for immunoassay of the present invention, a Ku86 antigen as a reagent is used. Though a Ku86 antigen as a reagent is not especially limited as long as it may effect an antigen-antibody reaction with an autoantibody against Ku86, examples of it may include a full length Ku86 protein, a variant of the full length Ku86 protein which is a protein having the same function as the full length protein capable of an antigen-antibody reaction with an autoantibody against Ku86, and having a homology of 90% or more to the amino acid sequence, or a protein having the amino acid sequence in which one to several amino acid residues are deleted, substituted, or added in the amino acid sequence of the full length Ku86 protein, and a fragment peptide of Ku86 that may effect an antigen-antibody reaction with the autoantibody against Ku86. Though a full length Ku86 protein is available from Abnova Corporation, the protein or its variant may also be synthesized by genetic engineering technique because its entire amino acid sequence is known as described above. When used in the present invention, a fragment peptide of Ku86 may be generated by cleaving a full length Ku86 protein into various peptide fragments by enzymatic hydrolysis and the like, or may also be easily generated using, a commercial automated peptide synthesizer. Additionally, the targeted fragment peptide of Ku86 may be generated by genetic engineering technique.
In the present invention, the thus-obtained variant or fragment peptide of the full length Ku86 protein may be reacted with an autoantibody against Ku86, then those who produce an antigen-antibody reaction may be selected to be used as a Ku86 antigen as a reagent. In the present invention, the whole of the each peptide fragment described above, as well as a part of it and the mixture thereof may be used, and are included in a Ku86 antigen as a reagent.
For the immunoassay of an autoantibody against Ku86 in the present invention, for example, a Ku86 antigen as a reagent is solid-phased onto a microplate or other carrier, and then a specimen expected to contain the autoantibody is applied to the resulting water-insolubilized carrier to allow the autoantibody to be bound thereto by an antigen-antibody reaction with the Ku86 antigen as a reagent. Then, an anti-human immunoglobulin antibody labeled with an enzyme and the like is applied to the carrier to react with and bind to the autoantibody.
The preparation of a water-insolubilized carrier may be easily carried out using a known method that binds a protein to the surface of a solid phase. As a carrier for conversion to solid-phase, for example, beads, microplates, and tubes are generally used. For a method of binding a Ku86 antigen as a reagent to these solid-phase surfaces, known immobilization techniques such as physisorption and chemical binding may be utilized as appropriate.
Upon contacting the thus solid-phased Ku86 antigen with a specimen containing its autoantibody, only the autoantibody against Ku86 binds specifically to the Ku86 antigen as a reagent. Thus, when a labeled anti-human immunoglobulin antibody is added, the anti-human immunoglobulin antibody binds to the autoantibody against Ku86, therefore this label can be utilized to carry out the measurement of the autoantibody.
As a label, routinely used labels, for example, enzymes, radioisotopes, fluorescent and chemiluminescent substances such as FITC, rhodamine, and luminol are used as appropriate. These various labels may be used to measure an autoantibody against Ku86 by a method such as enzyme-linked immunosorbent assay, radioimmunoassay, fluorescence immunoassay, and chemiluminescence immunoassay.
As a labeling enzyme used in enzyme-linked immunosorbent assay, an enzyme that is routinely used in enzyme immunoassay (EIA), such as horseradish peroxidase, calf intestine alkaline phosphatase, β-galactosidase, urease, or glucose oxidase is used as appropriate, and chromogenic substrates suitable for these enzymes and used routinely in EIA are used as appropriate. As chromogenic substrates, for example, in the case of HRP, 3,3′,5,5′-tetramethyl benzidine (TMBZ), TMBZ.HCl, TMBZ.PS, ABTS, o-phenylene diamine, and p-hydroxyphenyl acetic acid are used, in the case of alkaline phosphatase, p-nitrophenyl phosphate and 4-methylumbelliferyl phosphate are used, and in the case of β-galactosidase, o-nitrophenyl-β-D-galactopyranoside, and 4-methylumbelliferyl β-D-galactopyranoside are used.
Also in radioimmunoassay, fluorescence immunoassay, chemiluminescence immunoassay and the like, known labels generally used may be adopted.
In the method for immunoassay of the present invention, other than the above-described methods, an autoantibody against Ku86 may also be measured by western blotting, immunohistochemistry, immunoassay such as latex immunonephelometry and immunoprecipitation, and liquid chromatography.
The method for immunoassay of the present invention may be performed by a kit for immunoassay of an autoantibody against Ku86 comprising at least a Ku86 antigen as a reagent component. The Ku86 antigen may be a reagent component of the kit, for example, in the form bound to a water-insoluble carrier such as a microplate. As other reagent components of the kit, an anti-human immunoglobulin antibody is included. For this anti-human immunoglobulin antibody, those labeled with labeling substances such as enzymes, radioisotopes, fluorescent substances, or chemiluminescent substances are used depending on the measuring method adopted, such as enzyme-linked immunosorbent assay, radioimmunoassay, fluorescence immunoassay, and chemiluminescent immunoassay. As other reagent components, a surfactant and a buffer may be added as appropriate.
In the present invention, primary hepatocellular carcinoma can be determined by measuring an autoantibody against Ku86. Measuring an autoantibody against Ku86 by the method of measuring of the present invention is effective for distinguishing a cancerous disease in a patient. Utilization of the method of measuring of the present invention is effective for distinguishing, for example, a patient with initial primary hepatocellular carcinoma and a patient with recurrent primary hepatocellular carcinoma from a healthy individual. Additionally, by utilizing the method of measuring of the present invention, it is possible to distinguish a patient with initial primary hepatocellular carcinoma and a patient with recurrent primary hepatocellular carcinoma from a patient with carcinoma such as a patient with colorectal carcinoma, a patient with gastric carcinoma, a patient with pancreas, a patient with breast carcinoma, a patient with lung carcinoma or a patient with esophageal carcinoma. Furthermore, by utilizing the method of measuring of the present invention, it is possible to distinguish a patient with primary hepatocellular carcinoma such as a patient with initial primary hepatocellular carcinoma or a patient with recurrent primary hepatocellular carcinoma from a patient with hepatitis C or a patient with liver disease such as liver cirrhosis type C.
As apparent from the description above, an autoantibody against Ku86 serves as a marker for determination of primary hepatocellular carcinoma, and may be used as the marker for determination of primary hepatocellular carcinoma. An autoantibody against Ku86 is also preferred as a marker for determining primary hepatocellular carcinoma using a specimen derived from blood such as whole blood, blood plasma, and serum.
Hereinafter, the present invention will be described in more detail with reference to Examples, but the present invention is not to be limited to these Examples in any way.
For serum specimens collected from a healthy individual, a patient with hepatitis C, a patient with liver cirrhosis type C, a patient with initial primary hepatocellular carcinoma, a patient with recurrent primary hepatocellular carcinoma, a patient with colorectal carcinoma, a patient with gastric carcinoma, a patient with pancreatic carcinoma, a patient with breast carcinoma, a patient with lung carcinoma, and a patient with esophageal carcinoma, an autoantibody against Ku86 was measured with enzyme-linked immunosorbent assay (ELISA method) which is specifically described below.
Using an ELISA plate (manufactured by Nalge Nunc International, Maxisorp) as a water-insoluble carrier, full length XRCCS (recombinant protein GST-tagged: manufactured by Abnova Corporation, 5 μg/mL, 100 μL/well) as Ku86 was placed standstill onto the plate overnight at 4° C. to sensitize it, followed by washing the plate with PBS containing 0.05% Tween 20 (200 μL/well) three times. The plate was then coated overnight with PBS containing 1.5% BSA and 10% saccharose (200 μL/well) to generate a Ku86-bound ELISA plate.
Each sample serum was diluted 100 times with PBS, the dilution was added to the Ku86-bound ELISA plate in an amount of 100 μL/well, and placed standstill for 1 hour at 37° C., and the plate was then washed with PBS containing 0.05% Tween 20 (200 μL/well) three times. To the plate, an HRP labeled immunoglobulin (an HRP-labeled anti-Human IgG (manufactured by Zymed Laboratories Inc.) diluted 4000 times with PBS containing 0.05% Tween 20) was added in an amount of 100 μL/well, and the mixture was placed standstill for 30 minutes at 37° C. Then, after washing the plate with PBS containing 0.05% Tween 20 (200 μL/well) three times, TMBZ was added to the plate in an amount of 100 μL/well. After placing the plate standstill for 10 minutes at room temperature, 100 μL/well of 1 N sulfuric acid as a quencher was added to the plate. Absorbance was measured using a microplate reader (manufactured by Bio-Rad Laboratories, Inc.) at the wavelength of 450 nm.
It is noted that specimens from 48 healthy individuals, 16 hepatitis C patients, 21 liver cirrhosis type C patients, 35 specimens from initial primary hepatocellular carcinoma patients, 52 recurrent primary hepatocellular carcinoma patients, 16 specimens from colorectal carcinoma patients, 16 gastric carcinoma patients, 16 pancreatic carcinoma patients, 20 breast carcinoma patients, 10 lung carcinoma patients, and 18 esophageal carcinoma patients were used.
Results of the measurement of an autoantibody against Ku86 using the Ku86-bound ELISA plate are shown in
As shown in
As shown in
As described in detail hereinbefore, an autoantibody against Ku86 can be measured by reacting the autoantibody in a specimen such as a specimen derived from blood with a Ku86 antigen as a reagent, and measuring the resulting immune complex between the autoantibody and the Ku86 antigen, thereby allowing determination of primary hepatocellular carcinoma.
Number | Date | Country | Kind |
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2010-012976 | Jan 2010 | JP | national |
Filing Document | Filing Date | Country | Kind | 371c Date |
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PCT/JP2011/050720 | 1/18/2011 | WO | 00 | 7/9/2012 |