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在大鼠脾细胞中检测到四种白细胞介素-2表面结合蛋白。

Four interleukin-2 surface binding proteins detected in rat spleen cells.

作者信息

Chopra R K, Carroll M P, May W S, Bhatia S K, Margolick J B, Nagel J E, Adler W H

机构信息

Department of Environmental Health Sciences, School of Hygiene and Public Health, Johns Hopkins University, Baltimore, MD 21205.

出版信息

Immunology. 1992 Nov;77(3):338-44.

Abstract

Four specific interleukin-2 (IL-2) surface binding proteins can be detected by covalent cross-linking of [125I]IL-2 to rat spleen cells that have been activated with various stimuli including concanavalin A (Con A), phytohaemagglutinin (PHA), calcium ionophore, and phorbol dibutyrate (PDB) with or without calcium ionophore. These four cross-linked proteins could not be demonstrated in either unstimulated T cells or in activated T cells when binding was performed in the presence of a 20-100-fold excess of unlabelled IL-2. The molecular weights of the four cross-linked proteins, after subtraction of the molecular weight contribution of IL-2 are: 53,000, 70,000, 90,000 and 118,000. The 53,000 MW protein was identified as the rat IL-2 receptor (IL-2R) alpha-chain by immune precipitation. Additionally, results suggest that the rat IL-2R alpha-chain is tightly complexed to both the 118,000 and 90,000 MW IL-2 binding proteins. Purification of surface labelled proteins from activated cells using IL-2 affinity chromatography yields four proteins with similar molecular weight to those identified by cross-linking plus an additional non-ligand cross-linked protein of 46,000 MW. The 46,000 MW band may be a non-binding associated protein since it was not seen following [125I]IL-2 binding cross-linking. Tryptic digests and two-dimensional separation of the affinity-isolated proteins indicate that unique peptide maps are generated for the 46,000, 53,000 and 70,000 MW proteins and excludes the possibility that the bands identified by cross-linking represents cross-linking of multiple ligands to the 53,000 MW subunit. However, the 90,000 and 118,000 MW bands yield peptide maps that closely resemble each other suggesting that these binding proteins may be related. These results suggest that at least four IL-2 surface binding proteins may constitute the rat IL-2R system.

摘要

通过将[125I]白细胞介素-2(IL-2)与经多种刺激(包括伴刀豆球蛋白A(Con A)、植物血凝素(PHA)、钙离子载体以及有或无钙离子载体的佛波酯(PDB))激活的大鼠脾细胞进行共价交联,可检测到四种特异性IL-2表面结合蛋白。当在存在20 - 100倍过量未标记IL-2的情况下进行结合反应时,在未刺激的T细胞或活化的T细胞中均无法证明这四种交联蛋白的存在。扣除IL-2的分子量贡献后,这四种交联蛋白的分子量分别为:53,000、70,000、90,000和118,000。通过免疫沉淀法鉴定出53,000 MW的蛋白为大鼠IL-2受体(IL-2R)α链。此外,结果表明大鼠IL-2Rα链与118,000和90,000 MW的IL-2结合蛋白紧密结合。使用IL-2亲和层析从活化细胞中纯化表面标记蛋白,得到四种分子量与交联鉴定的蛋白相似的蛋白,外加一种46,000 MW的非配体交联蛋白。46,000 MW条带可能是一种非结合相关蛋白,因为在[125I]IL-2结合交联后未观察到该条带。亲和分离蛋白的胰蛋白酶消化产物和二维分离表明,46,000、53,000和70,000 MW的蛋白产生了独特的肽图谱,排除了交联鉴定的条带代表多个配体与53,000 MW亚基交联的可能性。然而,90,000和118,000 MW条带产生的肽图谱彼此非常相似,表明这些结合蛋白可能相关。这些结果表明,至少四种IL-2表面结合蛋白可能构成大鼠IL-2R系统。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/eafc/1421716/eb8af5771a56/immunology00102-0028-a.jpg

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