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针对人膀胱癌相关抗原的单克隆抗体。II. 通过免疫沉淀和SDS-PAGE分析鉴定细胞靶结构。

Monoclonal antibodies to antigens associated with transitional cell carcinoma of the human urinary bladder. II. Identification of the cellular target structures by immunoprecipitation and SDS-PAGE analysis.

作者信息

Paulie S, Koho H, Ben-Aissa H, Hansson Y, Lundblad M L, Perlmann P

出版信息

Cancer Immunol Immunother. 1984;17(3):173-9. doi: 10.1007/BF00205482.

Abstract

The cellular target structures for six monoclonal antibodies raised against cultured human bladder carcinoma cells (TCC) were investigated. The specificities of these antibodies when tested against a large panel of cells have been described in the companion paper. Radiolabeled cell lysates were precipitated with the different monoclonal antibodies bound to protein A (Staphylococcus aureus) on a matrix of Sepharose beads. The precipitates were separated by sodium dodecyl sulfate- gel electrophoresis (SDS-PAGE) and analyzed by autoradiography. The antibodies 4B5, 7E9, and 14B11 have previously been found to react in a similar way with TCC-targets and some non-TCC tumor cells, but not with normal urothelial cells or cells of hematopoietic origin. When tested with lysates of a TCC-cell line (TCCSuP) a strong 92K band and a weak 23K band were precipitated with any one of these antibodies. These polypeptides were expressed on the cell surface and were not linked by disulfide bonds. Depletion experiments confirmed that the three antibodies recognized the same antigens. Another antibody (4E8) probably directed to a differentiation antigen present on both urothelial and melanoma cells detected two high molecular polypeptides, 190K and 170K. Antibodies from the S2C6 hybridoma, which displayed a distinct dual specificity for TCC- targets and for malignant or transformed cells of B cell origin, precipitated a 50K component from extracts of either TCC- or B cell-derived cell lines. Antibodies produced by the S2A9 hybridoma were shown to bind to a framework epitope of the HLA-A, B, C heavy chain.

摘要

研究了针对培养的人膀胱癌细胞(TCC)产生的六种单克隆抗体的细胞靶结构。这些抗体在针对大量细胞进行测试时的特异性已在配套论文中描述。用与蛋白A(金黄色葡萄球菌)结合的不同单克隆抗体在琼脂糖珠基质上沉淀放射性标记的细胞裂解物。沉淀物通过十二烷基硫酸钠-凝胶电泳(SDS-PAGE)分离并通过放射自显影分析。先前已发现抗体4B5、7E9和14B11与TCC靶标和一些非TCC肿瘤细胞以类似方式反应,但不与正常尿路上皮细胞或造血来源的细胞反应。当用TCC细胞系(TCCSuP)的裂解物进行测试时,用这些抗体中的任何一种都沉淀出一条强的92K带和一条弱的23K带。这些多肽在细胞表面表达,并且不通过二硫键连接。去除实验证实这三种抗体识别相同的抗原。另一种抗体(4E8)可能针对尿路上皮细胞和黑色素瘤细胞上都存在的一种分化抗原,检测到两条高分子量多肽,190K和170K。来自S2C6杂交瘤的抗体对TCC靶标以及B细胞来源的恶性或转化细胞表现出明显的双重特异性,从TCC或B细胞来源的细胞系提取物中沉淀出一个50K的成分。S2A9杂交瘤产生的抗体显示与HLA-A、B、C重链的一个框架表位结合。

相似文献

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Isolation and characterization of two bladder carcinoma-associated antigens.两种膀胱癌相关抗原的分离与鉴定
J Immunol Methods. 1986 Nov 20;94(1-2):145-51. doi: 10.1016/0022-1759(86)90227-9.

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