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N-糖基化在人血小板活化因子受体功能表达中的作用。糖基化是高效膜运输所必需的。

The role of N-glycosylation for functional expression of the human platelet-activating factor receptor. Glycosylation is required for efficient membrane trafficking.

作者信息

García Rodríguez C, Cundell D R, Tuomanen E I, Kolakowski L F, Gerard C, Gerard N P

机构信息

Ina Sue Perlmutter Laboratory, Children's Hospital, Boston, Massachusetts, USA.

出版信息

J Biol Chem. 1995 Oct 20;270(42):25178-84. doi: 10.1074/jbc.270.42.25178.

DOI:10.1074/jbc.270.42.25178
PMID:7559653
Abstract

Streptococcus pneumoniae has been shown to utilize the platelet activating factor receptor for binding and invasion of host cells (Cundell, D. R., Gerard, N. P., Gerard, C., Idanpaan-Heikkila, I., and Tuomanen, E. I. (1995) Nature, in press). Because bacterial binding is in part carbohydrate dependent, and the human platelet-activating factor (PAF) receptor bears a single N-linked glycosylation sequence in the second extracellular loop, we undertook studies to determine the role of this epitope in PAF receptor function. Binding of pneumococci to COS cells transfected with the human PAF receptor is greatly reduced for a receptor mutant that bears no N-linked glycosylation site. Immunohistochemical and binding analyses show decreased expression of the non-glycosylated molecule on the cell membrane relative to the wild type receptor; however, metabolic labeling and immunopurification indicate it is synthesized intracellularly at a level similar to the native molecule. A mutant receptor encoding a functional glycosylation site at the NH2 terminus is better expressed at the cell surface compared with the non-glycosylated form, indicating that trafficking to the cell surface is facilitated by glycosylation, but its location is relatively unimportant. The binding affinity for PAF is not significantly effected by the presence or location of the carbohydrate, and variations in cell surface expression have little influence on signal transduction, as the non-glycosylated PAF receptor is equally effective for activation of phospholipase C as the native molecule. These data are supportive of pneumococcal binding on protein moiety(ies) of the PAF receptor and indicate that N-glycosylation facilitates expression of the protein on the cell membrane.

摘要

肺炎链球菌已被证明可利用血小板活化因子受体来结合并侵入宿主细胞(Cundell, D. R., Gerard, N. P., Gerard, C., Idanpaan-Heikkila, I., and Tuomanen, E. I. (1995) 《自然》,即将发表)。由于细菌结合部分依赖碳水化合物,且人血小板活化因子(PAF)受体在第二个细胞外环带有一个单一的N-连接糖基化序列,我们开展了研究以确定该表位在PAF受体功能中的作用。对于一个没有N-连接糖基化位点的受体突变体,肺炎球菌与转染了人PAF受体的COS细胞的结合大幅减少。免疫组织化学和结合分析表明,相对于野生型受体,非糖基化分子在细胞膜上的表达降低;然而,代谢标记和免疫纯化表明它在细胞内的合成水平与天然分子相似。与非糖基化形式相比,在NH2末端编码功能性糖基化位点的突变受体在细胞表面的表达更好,这表明糖基化促进了向细胞表面的转运,但其位置相对不重要。碳水化合物的存在或位置对PAF的结合亲和力没有显著影响,细胞表面表达的变化对信号转导影响很小,因为非糖基化的PAF受体激活磷脂酶C的效果与天然分子相同。这些数据支持肺炎球菌与PAF受体的蛋白质部分结合,并表明N-糖基化促进了该蛋白质在细胞膜上的表达。

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