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膜系连使乙酰胆碱受体α亚基的细胞外结构域能够形成一个异二聚体配体结合位点。

Membrane tethering enables an extracellular domain of the acetylcholine receptor alpha subunit to form a heterodimeric ligand-binding site.

作者信息

Wang Z Z, Hardy S F, Hall Z W

机构信息

Department of Physiology, University of California School of Medicine, San Francisco 94143, USA.

出版信息

J Cell Biol. 1996 Nov;135(3):809-17. doi: 10.1083/jcb.135.3.809.

Abstract

The first step of assembly of the nicotinic acetylcholine receptor (AChR) of adult skeletal muscle is the specific association of the alpha subunit with either delta or epsilon subunits to form a heterodimer with a ligand-binding site. Previous experiments have suggested that het erodimer formation in the ER arises from interaction between the luminal, NH2-terminal domains of the subunits. When expressed in COS cells with the delta subunit, however, the truncated NH2-terminal domain of the subunit folded correctly but did not form a heterodimer. Association with the delta subunit occurred only when the NH2-terminal domain was retained in the ER and was tethered to the membrane by its own M1 transmembrane domain, by the transmembrane domain of another protein, or by a glycolipid link. In each case, the ligand-binding sites of the resulting heterodimers were indistinguishable from that formed when the full-length alpha subunit was used. Attachment to the membrane may promote interaction by concentrating or orienting the subunit; alternatively, a membrane-bound factor may facilitate subunit association.

摘要

成年骨骼肌烟碱型乙酰胆碱受体(AChR)组装的第一步是α亚基与δ或ε亚基特异性结合,形成具有配体结合位点的异二聚体。先前的实验表明,内质网中异二聚体的形成源于亚基腔内NH2末端结构域之间的相互作用。然而,当与δ亚基一起在COS细胞中表达时,该亚基截短的NH2末端结构域正确折叠,但未形成异二聚体。只有当NH2末端结构域保留在内质网中,并通过其自身的M1跨膜结构域、另一种蛋白质的跨膜结构域或糖脂连接与膜相连时,才会与δ亚基发生结合。在每种情况下,所得异二聚体的配体结合位点与使用全长α亚基时形成的配体结合位点没有区别。与膜的附着可能通过使亚基浓缩或定向来促进相互作用;或者,膜结合因子可能促进亚基缔合。

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