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单纯疱疹病毒1型编码的蛋白激酶UL13使病毒的Us3蛋白激酶磷酸化,并调节病毒包膜因子UL34和UL31的核定位。

Herpes simplex virus 1-encoded protein kinase UL13 phosphorylates viral Us3 protein kinase and regulates nuclear localization of viral envelopment factors UL34 and UL31.

作者信息

Kato Akihisa, Yamamoto Mayuko, Ohno Takashi, Tanaka Michiko, Sata Tetsutaro, Nishiyama Yukihiro, Kawaguchi Yasushi

机构信息

Department of Infectious Disease Control, International Research Center for Infectious Diseases, The Institute of Medical Science, The University of Tokyo, 4-6-1 Shirokanedai, Minato-ku, Tokyo 108-8639, Japan.

出版信息

J Virol. 2006 Feb;80(3):1476-86. doi: 10.1128/JVI.80.3.1476-1486.2006.

Abstract

UL13 and Us3 are protein kinases encoded by herpes simplex virus 1. We report here that Us3 is a physiological substrate for UL13 in infected cells, based on the following observations. (i) The electrophoretic mobility, in denaturing gels, of Us3 isoforms from Vero cells infected with wild-type virus was slower than that of isoforms from cells infected with a UL13 deletion mutant virus (DeltaUL13). After treatment with phosphatase, the electrophoretic mobility of the Us3 isoforms from cells infected with wild-type virus changed, with one isoform migrating as fast as one of the Us3 isoforms from DeltaUL13-infected cells. (ii) A recombinant protein containing a domain of Us3 was phosphorylated by UL13 in vitro. (iii) The phenotype of DeltaUL13 resembles that of a recombinant virus lacking the Us3 gene (DeltaUs3) with respect to localization of the viral envelopment factors UL34 and UL31, whose localization has been shown to be regulated by Us3. UL34 and UL31 are localized in a smooth pattern throughout the nuclei of cells infected with wild-type virus, whereas their localization in DeltaUL13- and DeltaUs3-infected cells appeared as nuclear punctate patterns. These results indicate that UL13 phosphorylates Us3 in infected cells and regulates UL34 and UL31 localization, either by phosphorylating Us3 or by a Us3-independent mechanism.

摘要

UL13和Us3是由单纯疱疹病毒1编码的蛋白激酶。基于以下观察结果,我们在此报告Us3是感染细胞中UL13的生理底物。(i)在变性凝胶中,感染野生型病毒的Vero细胞中Us3亚型的电泳迁移率比感染UL13缺失突变病毒(DeltaUL13)的细胞中Us3亚型的电泳迁移率慢。用磷酸酶处理后,感染野生型病毒的细胞中Us3亚型的电泳迁移率发生了变化,其中一种亚型的迁移速度与感染DeltaUL13的细胞中的一种Us3亚型一样快。(ii)含有Us3结构域的重组蛋白在体外被UL13磷酸化。(iii)就病毒包膜因子UL34和UL31的定位而言,DeltaUL13的表型类似于缺乏Us3基因的重组病毒(DeltaUs3),其定位已被证明受Us3调节。UL34和UL31在感染野生型病毒的细胞的整个细胞核中呈平滑模式定位,而它们在感染DeltaUL13和DeltaUs3的细胞中的定位则呈现为核点状模式。这些结果表明,UL13在感染细胞中使Us3磷酸化,并通过使Us3磷酸化或通过不依赖Us3的机制调节UL34和UL31的定位。

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