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一种新型的 RNA 病毒多蛋白中的信号肽切割位点被鉴定出来。

A new type of signal peptidase cleavage site identified in an RNA virus polyprotein.

机构信息

Institut für Immunologie, Friedrich-Loeffler-Institut, Paul-Ehrlich-Strasse 28, D-72001 Tübingen, Germany.

出版信息

J Biol Chem. 2010 Mar 19;285(12):8572-84. doi: 10.1074/jbc.M109.083394. Epub 2010 Jan 21.

Abstract

Pestiviruses, a group of enveloped positive strand RNA viruses belonging to the family Flaviviridae, express their genes via a polyprotein that is subsequently processed by proteases. The structural protein region contains typical signal peptidase cleavage sites. Only the site at the C terminus of the glycoprotein E(rns) is different because it does not contain a hydrophobic transmembrane region but an amphipathic helix functioning as the E(rns) membrane anchor. Despite the absence of a hydrophobic region, the site between the C terminus of E(rns) and E1, the protein located downstream in the polyprotein, is cleaved by signal peptidase, as demonstrated by mutagenesis and inhibitor studies. Thus, E(rns)E1 is processed at a novel type of signal peptidase cleavage site showing a different membrane topology. Prevention of glycosylation or introduction of mutations into the C-terminal region of E(rns) severely impairs processing, presumably by preventing proper membrane interaction or disturbing a conformation critical for the protein to be accepted as a substrate by signal peptidase.

摘要

瘟病毒,一组包裹在正链 RNA 病毒属于黄病毒科,通过多蛋白表达其基因,随后由蛋白酶进行加工。结构蛋白区域包含典型的信号肽切割位点。只有糖蛋白 E(rns) 末端的位点不同,因为它不含疏水区跨膜区,而是一个作为 E(rns) 膜锚的两亲性螺旋。尽管没有疏水区,但 E(rns)和 E1 之间的位点,即在多蛋白下游的蛋白质,被信号肽酶切割,如突变和抑制剂研究所示。因此,E(rns)E1 在一种新型的信号肽切割位点进行加工,表现出不同的膜拓扑结构。糖基化的阻止或 E(rns)的 C 末端区域的突变严重损害了加工,可能是通过阻止适当的膜相互作用或扰乱对蛋白质被信号肽酶接受为底物至关重要的构象。

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