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无包膜蓝舌病毒的一种衣壳蛋白具有膜融合活性。

A capsid protein of nonenveloped Bluetongue virus exhibits membrane fusion activity.

作者信息

Forzan Mario, Wirblich Christoph, Roy Polly

机构信息

Department of Infectious and Tropical Diseases, London School of Hygiene and Tropical Medicine, Keppel Street, London WC1E 7HT, United Kingdom.

出版信息

Proc Natl Acad Sci U S A. 2004 Feb 17;101(7):2100-5. doi: 10.1073/pnas.0306448101. Epub 2004 Feb 4.

Abstract

The outer capsid layer of Bluetongue virus, a member of the nonenveloped Reoviridae family, is composed of two proteins, a receptor-binding protein, VP2, and a second protein, VP5, which shares structural features with class I fusion proteins of enveloped viruses. In the replication cycle of Bluetongue virus VP5 acts as a membrane permeabilization protein that mediates release of viral particles from endosomal compartments into the cytoplasm. Here, we show that VP5 can also act as a fusion protein and induce syncytium formation when it is fused to a transmembrane anchor and expressed on the cell surface. Fusion activity is strictly pH-dependent and is triggered by short exposure to low pH. No cell-cell fusion is observed at neutral pH. Deletion of the first 40 amino acids, which can fold into two amphipathic helices, abolishes fusion activity. Syncytium formation by VP5 is inhibited in the presence of VP2 when it is expressed in a membrane-anchored form. The data indicate an interaction between the outer capsid protein VP2 and VP5 and show that VP5 undergoes pH-dependent conformational changes that render it capable of interacting with cellular membranes. More importantly, our data show that a membrane permeabilization protein of a nonenveloped virus can evolve into a fusion protein by the addition of an appropriate transmembrane anchor. The results strongly suggest that the mechanism of membrane permeabilization by VP5 and membrane fusion by viral fusion proteins require similar structural features and conformational changes.

摘要

蓝舌病毒是无包膜呼肠孤病毒科的成员,其外衣壳层由两种蛋白质组成,一种是受体结合蛋白VP2,另一种是VP5,VP5与包膜病毒的I类融合蛋白具有共同的结构特征。在蓝舌病毒的复制周期中,VP5作为一种膜通透蛋白,介导病毒颗粒从内体区室释放到细胞质中。在此,我们表明,当VP5与跨膜锚定蛋白融合并在细胞表面表达时,它也可以作为一种融合蛋白并诱导合胞体形成。融合活性严格依赖于pH值,并且通过短暂暴露于低pH值来触发。在中性pH值下未观察到细胞间融合。删除前40个氨基酸(可折叠成两个两亲性螺旋)会消除融合活性。当以膜锚定形式表达时,在VP2存在的情况下,VP5介导的合胞体形成受到抑制。这些数据表明外衣壳蛋白VP2和VP5之间存在相互作用,并表明VP5会发生pH值依赖性的构象变化,使其能够与细胞膜相互作用。更重要的是,我们的数据表明,一种无包膜病毒的膜通透蛋白可以通过添加适当的跨膜锚定蛋白演变成融合蛋白。结果强烈表明,VP5介导的膜通透机制和病毒融合蛋白介导的膜融合需要相似的结构特征和构象变化。

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