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“天然未折叠”的VPg对田菁花叶病毒丝氨酸蛋白酶活性至关重要。

"Natively unfolded" VPg is essential for Sesbania mosaic virus serine protease activity.

作者信息

Satheshkumar Panayampalli Subbian, Gayathri Pananghat, Prasad Kasaragod, Savithri Handanahal Subbarao

机构信息

Department of Biochemistry, Indian Institute of Science, Bangalore.

出版信息

J Biol Chem. 2005 Aug 26;280(34):30291-300. doi: 10.1074/jbc.M504122200. Epub 2005 Jun 7.

DOI:10.1074/jbc.M504122200
PMID:15944159
Abstract

Polyprotein processing is a major strategy used by many plant and animal viruses to maximize the number of protein products obtainable from a single open reading frame. In Sesbania mosaic virus, open reading frame-2 codes for a polyprotein that is cleaved into different functional proteins in cis by the N-terminal serine protease domain. The soluble protease domain lacking 70-amino-acid residues from the N terminus (deltaN70Pro, where Pro is protease) was not active in trans. Interestingly, the protease domain exhibited trans-catalytic activity when VPg (viral protein genome-linked) was present at the C terminus. Bioinformatic analysis of VPg primary structure suggested that it could be a disordered protein. Biophysical studies validated this observation, and VPg resembled "natively unfolded" proteins. CD spectral analysis showed that the deltaN70Pro-VPg fusion protein had a characteristic secondary structure with a 230 nm positive CD peak. Mutation of Trp-43 in the VPg domain to phenylalanine abrogated the positive peak with concomitant loss in cis- and trans-proteolytic activity of the deltaN70Pro domain. Further, deletion of VPg domain from the polyprotein completely abolished proteolytic processing. The results suggested a novel mechanism of activation of the protease, wherein the interaction between the natively unfolded VPg and the protease domains via aromatic amino acid residues alters the conformation of the individual domains and the active site of the protease. Thus, VPg is an activator of protease in Sesbania mosaic virus, and probably by this mechanism, the polyprotein processing could be regulated in planta.

摘要

多聚蛋白加工是许多动植物病毒采用的一种主要策略,用于使从单个开放阅读框中获得的蛋白质产物数量最大化。在田菁花叶病毒中,开放阅读框2编码一种多聚蛋白,该多聚蛋白在顺式作用下被N端丝氨酸蛋白酶结构域切割成不同的功能蛋白。缺少N端70个氨基酸残基的可溶性蛋白酶结构域(δN70Pro,其中Pro代表蛋白酶)在反式作用中无活性。有趣的是,当VPg(病毒蛋白基因组连接蛋白)存在于C端时,蛋白酶结构域表现出反式催化活性。对VPg一级结构的生物信息学分析表明它可能是一种无序蛋白。生物物理研究证实了这一观察结果,并且VPg类似于“天然未折叠”蛋白。圆二色光谱分析表明,δN70Pro-VPg融合蛋白具有特征性二级结构,在230 nm处有一个正的圆二色峰。VPg结构域中的色氨酸-43突变为苯丙氨酸消除了正峰,同时δN70Pro结构域的顺式和反式蛋白水解活性丧失。此外,从多聚蛋白中删除VPg结构域完全消除了蛋白水解加工。结果提示了一种蛋白酶激活的新机制,即天然未折叠的VPg与蛋白酶结构域之间通过芳香族氨基酸残基的相互作用改变了各个结构域的构象以及蛋白酶的活性位点。因此,VPg是田菁花叶病毒中蛋白酶的激活剂,可能通过这种机制,多聚蛋白加工在植物体内得以调控。

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