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采用抗β2微球蛋白(β2m)抗血清通过亲和层析法分离HLA和肿瘤抗原。

Isolation of HLA and tumor antigens by means of affinity chromatography employing anti-beta2-microglobulin (beta2m) antiserum.

作者信息

Rauch J E, Shuster J, Thomson D M, Gold P

出版信息

Cancer. 1978 Sep;42(3 Suppl):1601-5. doi: 10.1002/1097-0142(197809)42:3+<1601::aid-cncr2820420838>3.0.co;2-v.

Abstract

A method for the isolation of HLA antigen molecules from normal and cancerous solid human tissue is described. The method employs anti-beta2-microglobulin (beta2m) antiserum coupled to Sepharose beads as an immunosorbent affinity medium. The anti-beta2m affinity chromatography procedure greatly purifies and selectively enriches HLA and any material that copurifies by affinity, with beta2m and/or HLA molecules. The HLA isolated by this purification procedure was used to immunize rabbits. The antisera obtained were absorbed on beta2m to remove all anti-beta2m antibody activity. The use of such anti-HLA antisera in radioimmunoassays, immunoprecipitation studies, and F(ab')2 blocking experiments demonstrated that these antisera are directed against a common HLA determinant present on the heavy (alloantigen-bearing) chain of all HLA molecules. The use of an identical procedure employing human tumor tissues has resulted in the isolation of HLA-like or HLA-associated tumor-specific antigens as demonstrated by the leukocyte adherence inhibition (LAI) assay.

摘要

本文描述了一种从正常和癌性人体实体组织中分离HLA抗原分子的方法。该方法采用与琼脂糖珠偶联的抗β2-微球蛋白(β2m)抗血清作为免疫吸附亲和介质。抗β2m亲和层析程序可极大地纯化并选择性富集HLA以及任何通过亲和作用与β2m和/或HLA分子共纯化的物质。通过该纯化程序分离得到的HLA用于免疫兔子。所获得的抗血清在β2m上进行吸附以去除所有抗β2m抗体活性。在放射免疫测定、免疫沉淀研究和F(ab')2阻断实验中使用此类抗HLA抗血清表明,这些抗血清针对所有HLA分子重链(携带同种异体抗原的链)上存在的共同HLA决定簇。采用相同程序处理人肿瘤组织已导致分离出HLA样或HLA相关的肿瘤特异性抗原,白细胞黏附抑制(LAI)试验证明了这一点。

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