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痘苗病毒F12L蛋白是肌动蛋白尾形成、正常噬斑大小和毒力所必需的。

Vaccinia virus F12L protein is required for actin tail formation, normal plaque size, and virulence.

作者信息

Zhang W H, Wilcock D, Smith G L

机构信息

Sir William Dunn School of Pathology, University of Oxford, Oxford OX1 3RE, United Kingdom.

出版信息

J Virol. 2000 Dec;74(24):11654-62. doi: 10.1128/jvi.74.24.11654-11662.2000.

Abstract

Vaccinia virus gene F12L is shown to encode a 65-kDa protein that is synthesized early and late during infection and that is not modified by glycosylation. Computational sequence comparison revealed that related proteins are encoded by all sequenced chordopoxviruses. A virus deletion mutant lacking the F12L gene (vDeltaF12L) and a revertant virus with the F12L gene reinserted into the deletion mutant (vF12L-rev) were constructed and analyzed. A version of the F12L gene with a C-terminal amino acid tag derived from the influenza virus hemagglutinin and that is recognized by a monoclonal antibody was also inserted into the F12L locus of vDeltaF12L. Loss of the F12L protein reduced the formation of IMV 2-fold, but there was a dramatic (99.5%) reduction in actin tail formation, and the levels of cell-associated enveloped virus and extracellular enveloped virus were reduced 8- to 11-fold and 7-fold, respectively. Consistent with the lack of actin tail formation, vDeltaF12L produced a very small plaque. The vDeltaF12L virus was severely attenuated in vivo, such that a dose of vDeltaF12L 10,000-fold greater than the dose of wild-type virus that induced severe disease was unable to induce disease in mice infected intranasally.

摘要

痘苗病毒基因F12L被证明编码一种65kDa的蛋白质,该蛋白质在感染的早期和晚期均有合成,且未发生糖基化修饰。通过计算序列比较发现,所有已测序的脊索痘病毒均编码相关蛋白质。构建并分析了缺失F12L基因的病毒缺失突变体(vDeltaF12L)和将F12L基因重新插入缺失突变体中的回复病毒(vF12L-rev)。还将一个带有源自流感病毒血凝素的C末端氨基酸标签且能被单克隆抗体识别的F12L基因版本插入到vDeltaF12L的F12L基因座中。F12L蛋白的缺失使胞内成熟病毒(IMV)的形成减少了2倍,但肌动蛋白尾的形成显著减少(99.5%),细胞相关包膜病毒和细胞外包膜病毒的水平分别降低了8至11倍和7倍。与肌动蛋白尾形成的缺失一致,vDeltaF12L产生的噬斑非常小。vDeltaF12L病毒在体内严重减毒,以至于鼻内感染小鼠时,剂量比诱导严重疾病的野生型病毒剂量大10000倍的vDeltaF12L也无法诱导疾病。

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