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风疹病毒衣壳蛋白对p150非结构蛋白缺失的互补作用。

Complementation of a deletion in the rubella virus p150 nonstructural protein by the viral capsid protein.

作者信息

Tzeng Wen-Pin, Frey Teryl K

机构信息

Department of Biology, Georgia State University, Atlanta, Georgia 30302-4010, USA.

出版信息

J Virol. 2003 Sep;77(17):9502-10. doi: 10.1128/jvi.77.17.9502-9510.2003.

Abstract

Rubella virus (RUB) replicons with an in-frame deletion of 507 nucleotides between two NotI sites in the P150 nonstructural protein (DeltaNotI) do not replicate (as detected by expression of a reporter gene encoded by the replicon) but can be amplified by wild-type helper virus (Tzeng et al., Virology 289:63-73, 2001). Surprisingly, virus with DeltaNotI was viable, and it was hypothesized that this was due to complementation of the NotI deletion by one of the virion structural protein genes. Introduction of the capsid (C) protein gene into DeltaNotI-containing replicons as an in-frame fusion with a reporter gene or cotransfection with both DeltaNotI replicons and RUB replicon or plasmid constructs containing the C gene resulted in replication of the DeltaNotI replicon, confirming the hypothesis that the C gene was the structural protein gene responsible for complementation and demonstrating that complementation could occur either in cis or in trans. Approximately the 5' one-third of the C gene was necessary for complementation. Mutations that prevented translation of the C protein while minimally disturbing the C gene sequence abrogated complementation, while synonymous codon mutations that changed the C gene sequence without affecting the amino acid sequence at the 5' end of the C gene had no effect on complementation, indicating that the C protein, not the C gene RNA, was the moiety responsible for complementation. Complementation occurred at a basic step in the virus replication cycle, because DeltaNotI replicons failed to accumulate detectable virus-specific RNA.

摘要

风疹病毒(RUB)复制子在P150非结构蛋白的两个NotI位点之间有一个507个核苷酸的读框内缺失(DeltaNotI),不能复制(通过复制子编码的报告基因的表达检测),但可被野生型辅助病毒扩增(曾等,《病毒学》289:63 - 73,2001)。令人惊讶的是,带有DeltaNotI的病毒是有活力的,据推测这是由于病毒粒子结构蛋白基因之一对NotI缺失的互补作用。将衣壳(C)蛋白基因作为与报告基因的读框内融合引入含DeltaNotI的复制子中,或者将含DeltaNotI的复制子与RUB复制子或含有C基因的质粒构建体共转染,导致DeltaNotI复制子的复制,证实了C基因是负责互补的结构蛋白基因这一假设,并表明互补作用可顺式或反式发生。大约C基因的5'端三分之一对于互补是必需的。阻止C蛋白翻译同时最小程度干扰C基因序列的突变消除了互补作用,而改变C基因序列但不影响C基因5'端氨基酸序列的同义密码子突变对互补作用没有影响,表明是C蛋白而非C基因RNA是负责互补的部分。互补作用发生在病毒复制周期的一个基本步骤,因为DeltaNotI复制子未能积累可检测到的病毒特异性RNA。

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