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针对人类白细胞抗原-DRw决定簇的单克隆抗体。

Monoclonal antibodies to HLA--DRw determinants.

作者信息

Brodsky F M, Parham P, Bodmer W F

出版信息

Tissue Antigens. 1980 Jul;16(1):30-48. doi: 10.1111/j.1399-0039.1980.tb00285.x.

Abstract

Two monoclonal antibodies recognizing HLA-DRw (human la) antigens were produced. The DA2 antibody binds a monomorphic determinant, common to all specificities and Genox3.53 antibody binds to a cross-reacting site on the HLA-DRw1,2 and 6 specificities. Both antibodies are IgG1 and show complement dependent cytotoxicity only in the presence of rabbit anti-mouse IgG serum. Specificity of both antibodies for the HLA-DRw molecule was shown by inhibition of antibody binding by preincubation of antibody with detergent solubilized Ia from JY (HLA-DRw4,6) cells and by preincubation of target cells with F(ab')2 fragments of a rabbit anti-la serum. DA2 antibody reacted with all cells of human B cell origin tested and with peripheral blood lymphocytes of several primate species tested. Genox3.53 antibody bound only to human cells expressing HLA-DRw1,2 or 6 antigens, giving a negative reaction with all primates tested. Genox3.53 antibody detected a split in the HLA-DRw6 specificity, showing reduced binding to the Daudi cell (HLA-DRw6) in comparison with binding to several other cell lines typed as HLA-DRw6, under saturating conditions. This low reactivity with Daudi was confirmed by absorption experiments. The ratio of DA2 binding to Genox3.53 binding to homozygous and heterozygous cell lines under saturation conditions was compared. Results suggested that, on some cell lines, DA2 might be reacting with a second population of human Ia antigens in addition to the HLA-DRw antigens. When a mixture of saturating concentrations of DA2 and Genox3.53 antibodies was tested for binding to cells under saturating conditions, the number of counts bound suggested the antibodies could bind simultaneously. Direct binding experiments showed that when each antibody was iodinated, its binding was not inhibited by preincubation with the other antibody, confirming that the DA2 and Genox3.53 determinants are distinct on the Ia molecule.

摘要

制备了两种识别HLA - DRw(人类淋巴细胞抗原)抗原的单克隆抗体。DA2抗体结合一种单态决定簇,该决定簇为所有特异性所共有,且Genox3.53抗体结合HLA - DRw1、2和6特异性上的一个交叉反应位点。两种抗体均为IgG1,且仅在存在兔抗小鼠IgG血清时才显示补体依赖性细胞毒性。通过将抗体与经去污剂溶解的来自JY(HLA - DRw4,6)细胞的Ia进行预孵育来抑制抗体结合,以及通过用兔抗Ia血清的F(ab')2片段对靶细胞进行预孵育,证明了两种抗体对HLA - DRw分子的特异性。DA2抗体与所测试的所有人类B细胞来源的细胞以及所测试的几种灵长类物种的外周血淋巴细胞发生反应。Genox3.53抗体仅与表达HLA - DRw1、2或6抗原的人类细胞结合,对所有测试的灵长类动物均呈阴性反应。Genox3.53抗体检测到HLA - DRw6特异性的一个分裂,与在饱和条件下与其他几种分型为HLA - DRw6的细胞系相比,其与Daudi细胞(HLA - DRw6)的结合减少。吸收实验证实了与Daudi细胞的这种低反应性。比较了饱和条件下DA2与Genox3.53对纯合和杂合细胞系的结合比率。结果表明,在某些细胞系上,除了HLA - DRw抗原外,DA2可能还与另一群人类Ia抗原发生反应。当在饱和条件下测试饱和浓度的DA2和Genox3.53抗体混合物与细胞的结合时,结合的计数表明抗体可以同时结合。直接结合实验表明,当每种抗体碘化后,其结合不会被与另一种抗体的预孵育所抑制,证实了DA2和Genox3.53决定簇在Ia分子上是不同的。

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