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盘基网柄菌接触位点A蛋白的两步糖基化及不完全糖基化形式向细胞表面的转运

Two-step glycosylation of the contact site A protein of Dictyostelium discoideum and transport of an incompletely glycosylated form to the cell surface.

作者信息

Hohmann H P, Bozzaro S, Yoshida M, Merkl R, Gerisch G

机构信息

Max-Planck-Institut für Biochemie, Martinsried bei München, Federal Republic of Germany.

出版信息

J Biol Chem. 1987 Dec 5;262(34):16618-24.

PMID:3316223
Abstract

Two different types of oligosaccharides, designated type 1 and 2 carbohydrate residues, are present on the contact site A molecule, an 80-kDa glycoprotein involved in the formation of EDTA-stable cell adhesion during cell aggregation in Dictyostelium discoideum. The first precursor detected by pulse-chase labeling with [35S]methionine was a 68-kDa glycoprotein carrying type 1 carbohydrate. Conversion of the precursor into the 80-kDa form occurred simultaneously with the addition of type 2 carbohydrate. Tunicamycin inhibited type 1 glycosylation more efficiently than type 2 glycosylation. The first precursor detected in tunicamycin-treated cells by pulse-chase labeling was a 53-kDa protein lacking both carbohydrates, which was converted through addition of type 2 carbohydrate into a 66-kDa final product. Labeling of intact cells indicated that this 66-kDa glycoprotein is transported to the cell surface. Prolonged treatment with tunicamycin resulted in the accumulation within the cells of the 53-kDa precursor with no detectable exposure of this protein on the cell surface. It is concluded that type 1 carbohydrate, which is cotranslationally added in N-glycosidic linkages, is neither required for transport of the protein to the Golgi apparatus nor for type 2 glycosylation or protection of the protein against proteolytic degradation. Incapability of tunicamycin-treated cells of forming EDTA-stable cell contacts suggests a role for type 1 carbohydrate in cell adhesion. Type 2 carbohydrate is added posttranslationally. It is required in the absence of type 1 glycosylation for transport of the protein to the cell surface.

摘要

在盘基网柄菌细胞聚集过程中,参与形成EDTA稳定细胞黏附的80 kDa糖蛋白接触位点A分子上存在两种不同类型的寡糖,分别称为1型和2型碳水化合物残基。用[35S]甲硫氨酸脉冲追踪标记检测到的第一个前体是携带1型碳水化合物的68 kDa糖蛋白。前体向80 kDa形式的转化与2型碳水化合物的添加同时发生。衣霉素抑制1型糖基化比抑制2型糖基化更有效。用衣霉素处理的细胞经脉冲追踪标记检测到的第一个前体是一种缺乏两种碳水化合物的53 kDa蛋白质,通过添加2型碳水化合物将其转化为66 kDa的终产物。完整细胞的标记表明,这种66 kDa糖蛋白被转运到细胞表面。用衣霉素长时间处理导致53 kDa前体在细胞内积累,该蛋白在细胞表面未检测到暴露。得出的结论是,以N-糖苷键共翻译添加的1型碳水化合物,对于蛋白质转运到高尔基体、2型糖基化或蛋白质免受蛋白水解降解的保护都不是必需的。衣霉素处理的细胞无法形成EDTA稳定的细胞接触,这表明1型碳水化合物在细胞黏附中起作用。2型碳水化合物是在翻译后添加的。在没有1型糖基化的情况下,它是蛋白质转运到细胞表面所必需的。

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