Electrophoretic analysis of the novel antigen for the gastrointestinal-specific monoclonal antibody, A33

被引:16
作者
Ji, H
Moritz, RL
Reid, GE
Ritter, G
Catimel, B
Nice, E
Heath, JK
White, SJ
Welt, S
Old, LJ
Burgess, AW
Simpson, RJ
机构
[1] LUDWIG INST CANC RES, MELBOURNE BRANCH, JOINT PROT STRUCT LAB, MELBOURNE, VIC, AUSTRALIA
[2] MEM SLOAN KETTERING CANC CTR, LUDWIG INST CANC RES, NEW YORK BRANCH, NEW YORK, NY 10021 USA
[3] ROYAL MELBOURNE HOSP, WALTER & ELIZA HALL INST MED RES, PARKVILLE, VIC 3050, AUSTRALIA
关键词
monoclonal antibody A33; two-dimensional polyacrylamide gel electrophoresis; tandem mass spectrometry; peptide mass fingerprinting; human colonic proteins;
D O I
10.1002/elps.1150180345
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
The murine monoclonal antibody A33 (mAbA33) recognises a human cell membrane-associated antigen selectively expressed in epithelial cells of the lower gastrointestinal tract and > 90% of colonic cancers, but is not detected in a wide range of other normal tissues by immunohistochemical analysis. In phase I/II clinical triasl, mAbA33 has been shown to target advanced colon cancers and the humanised version is currently being evaluated in therapy studies. Although the mAbA33 has been well characterised by immunohistochemical and clinical studies, until recently, the target antigen has remained poorly defined. This nias largely attributable to the antigenic determinant recognised by mAbA33 being dependent on the native spatial conformation of the A33 antigen which impeded its identification by conventional two-dimensional electrophoresis (2-DE) and immunoblot analysis. We have developed an immunoblot method, based on nonreducing/non-urea precast a-DE gels, that has facilitated the purification of the detergent (0.3% Triton X-100) solubilised A33 antigen From the human colon cancer cell lines LIM1215 and SW1222. Under these 2-DE conditions, the A33 antigen electrophoreses with an apparent M-r similar to 41000 and pI 5.0-6.0. Attempts to isolate the A33 antigen from 2-DE gels for direct structural analysis were unsuccessful, due to its co-electrophoresis with actin and cytokeratin proteins. However, using Western blot and biosensor detection the A33 antigen has been purified chromatographically and N-terminal sequence analysis was possible. Using polyclonal antibodies raised against a synthetic peptide corresponding to the N-terminal region of the A33 antigen we have used Western blot analysis to localise the molecule in our master 2-DE protein database for normal human colon crypts and several colon carcinoma cell lines (URL address: http ://www.ludwig.edu.au). Under reducing 2-DE conditions, the A33 antigen electrophoresis as 6 differentially charged isoforms (pI 4.6-4.8) with a single molecular weight species at M-r similar to 55000.
引用
收藏
页码:614 / 621
页数:8
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