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细胞表面免疫球蛋白。IX。一种研究小鼠脾细胞中合成、细胞内运输和外化的新方法。

Cell surface immunoglobulin. IX. A new method for the study of synthesis, intracellular transport, and exteriorization in murine splenocytes.

作者信息

Vitetta E S, Uhr J W

出版信息

J Exp Med. 1974 Jun 1;139(6):1599-620. doi: 10.1084/jem.139.6.1599.

Abstract

A new method for the detection of cell surface immunoglobulin labeled with isotopic precursors is described. The method consists of the aggregation of surface Ig on cells with specific antibody (heterologous) and the subsequent removal of antigen-antibody complexes by the combination of high speed centrifugation and immunoprecipitation of remaining soluble complexes using antibody to the heterologous Ig. Using this method, the kinetics of appearance of cell surface Ig and its turnover were studied in murine splenocytes. The results suggest that cell surface Ig is synthesized and transported in the same manner as secretory Ig rather than being synthesized on the plasma membrane. The turnover of intracellular and cell surface Ig in lymphocytes is slow. In contrast, intracellular Ig in plasma cells is rapidly secreted and usually without a cell surface phase. Cell surface Ig was shown to be radiolabeled with [(3)H]glucosamine, -galactose, and -fucose. The proportion of cell surface to intracellular (nonsurface) Ig labeled with these precursors suggests the same sequence of addition of sugars to Ig destined to be on the surface of lymphocytes as with Ig which will be secreted by plasma cells. Results with this new method also confirm earlier conclusions based on experiments using cell surface iodination: 8S IgM is the predominant Ig on the surface of murine splenocytes and the molecule appears to be attached by its micro-chains.

摘要

本文描述了一种检测用同位素前体标记的细胞表面免疫球蛋白的新方法。该方法包括用特异性抗体(异种)使细胞表面的Ig聚集,随后通过高速离心去除抗原 - 抗体复合物,并使用针对异种Ig的抗体对剩余的可溶性复合物进行免疫沉淀。利用这种方法,研究了小鼠脾细胞中细胞表面Ig出现的动力学及其周转情况。结果表明,细胞表面Ig的合成和运输方式与分泌型Ig相同,而不是在质膜上合成。淋巴细胞中细胞内和细胞表面Ig的周转缓慢。相比之下,浆细胞中的细胞内Ig迅速分泌,通常没有细胞表面阶段。细胞表面Ig被证明能用[³H]葡糖胺、半乳糖和岩藻糖进行放射性标记。用这些前体标记的细胞表面Ig与细胞内(非表面)Ig的比例表明,与将由浆细胞分泌的Ig一样,添加到注定位于淋巴细胞表面的Ig上的糖的顺序相同。用这种新方法得到的结果也证实了基于细胞表面碘化实验得出的早期结论:8S IgM是小鼠脾细胞表面的主要Ig,该分子似乎通过其微链连接。

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