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氨氯地平敏感型上皮钠通道的膜拓扑结构。

Membrane topology of the amiloride-sensitive epithelial sodium channel.

作者信息

Snyder P M, McDonald F J, Stokes J B, Welsh M J

机构信息

Howard Hughes Medical Institute, Department of Internal Medicine, University of Iowa College of Medicine, Iowa City 52242.

出版信息

J Biol Chem. 1994 Sep 30;269(39):24379-83.

PMID:7929098
Abstract

The amiloride-sensitive epithelial sodium channel (ENaC) is involved in fluid and electrolyte absorption across a number of epithelia, and cloning of several ENaC subunits has begun to facilitate investigation of the structure, function, and regulation of this channel. Analysis of the amino acid sequence has revealed two potential membrane-spanning domains, but little else is known about the structure of ENaC. To investigate the membrane topology of one subunit, alpha rENaC, we used in vitro transcription, translation, and translocation into microsomal membranes. This generated a glycosylated protein of 93 kDa. Sequence analysis also revealed eight potential sites for N-glycosylation, six of which were found to be glycosylated (Asn190, Asn259, Asn320, Asn339, Asn424, and Asn538), indicating that they are extracellular. The C terminus was localized as intracellular based on antibody recognition and protease sensitivity of a tagged epitope at the C terminus. The N terminus was also found to be intracellular, based on its protease sensitivity. Similar results were obtained by expression in Xenopus oocytes. Together, these results support a model of alpha rENaC consisting of an intracellular N terminus and C terminus, a large N-glycosylated extracellular domain, and two membrane-spanning domains that each pass once through the plasma membrane. Because of their sequence similarity, it is likely that this structure is shared by other ENaC subunits and possibly the degenerins of Caenorhabditis elegans as well.

摘要

氨氯地平敏感的上皮钠通道(ENaC)参与多种上皮细胞的液体和电解质吸收,多个ENaC亚基的克隆已开始促进对该通道的结构、功能及调节的研究。对氨基酸序列的分析揭示了两个潜在的跨膜结构域,但关于ENaC的结构了解甚少。为了研究其中一个亚基αrENaC的膜拓扑结构,我们采用了体外转录、翻译并转运至微粒体膜的方法。这产生了一个93 kDa的糖基化蛋白。序列分析还揭示了8个潜在的N-糖基化位点,其中6个被发现发生了糖基化(Asn190、Asn259、Asn320、Asn339、Asn424和Asn538),表明它们位于细胞外。基于C端标记表位的抗体识别和蛋白酶敏感性,C端被定位在细胞内。基于其蛋白酶敏感性,N端也被发现位于细胞内。在非洲爪蟾卵母细胞中表达也获得了类似结果。这些结果共同支持了αrENaC的模型,该模型由细胞内的N端和C端、一个大的N-糖基化细胞外结构域以及两个各穿过质膜一次的跨膜结构域组成。由于它们的序列相似性,其他ENaC亚基以及秀丽隐杆线虫的退化蛋白可能也具有这种结构。

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