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单纯疱疹病毒 DNA 包装终止酶 pUL15 核酸酶结构域的结构表明真核生物和原核生物病毒之间存在进化谱系。

The structure of the herpes simplex virus DNA-packaging terminase pUL15 nuclease domain suggests an evolutionary lineage among eukaryotic and prokaryotic viruses.

机构信息

Department of Molecular Biosciences, University of Kansas, Lawrence, Kansas, USA.

出版信息

J Virol. 2013 Jun;87(12):7140-8. doi: 10.1128/JVI.00311-13. Epub 2013 Apr 17.

Abstract

Herpes simplex virus 1 (HSV-1), the prototypic member of herpesviruses, employs a virally encoded molecular machine called terminase to package the viral double-stranded DNA (dsDNA) genome into a preformed protein shell. The terminase contains a large subunit that is thought to cleave concatemeric viral DNA during the packaging initiation and completion of each packaging cycle and supply energy to the packaging process via ATP hydrolysis. We have determined the X-ray structure of the C-terminal domain of the terminase large-subunit pUL15 (pUL15C) from HSV-1. The structure shows a fold resembling those of bacteriophage terminases, RNase H, integrases, DNA polymerases, and topoisomerases, with an active site clustered with acidic residues. Docking analysis reveals a DNA-binding surface surrounded by flexible loops, indicating considerable conformational changes upon DNA binding. In vitro assay shows that pUL15C possesses non-sequence-specific, Mg(2+)-dependent nuclease activity. These results suggest that pUL15 uses an RNase H-like, metal ion-mediated catalysis mechanism for cleavage of viral concatemeric DNA. The structure reveals extra structural elements in addition to the RNase H-like fold core and variations in local architecture of the nuclease active site, which are conserved in herpesvirus terminases and bear great similarity to the phage T4 gp17 but are distinct from podovirus and siphovirus orthologs and cellular RNase H, delineating a new evolutionary lineage among a large family of eukaryotic viruses and simple and complex prokaryotic viruses.

摘要

单纯疱疹病毒 1(HSV-1)是疱疹病毒的原型成员,它利用一种称为末端酶的病毒编码分子机器将病毒双链 DNA(dsDNA)基因组包装到预先形成的蛋白质壳中。末端酶包含一个大亚基,该亚基被认为在每个包装周期的包装起始和完成时切割连接的病毒 DNA,并通过 ATP 水解为包装过程提供能量。我们已经确定了 HSV-1 末端酶大亚基 pUL15(pUL15C)的 C 末端结构域的 X 射线结构。该结构显示出一种类似于噬菌体末端酶、RNase H、整合酶、DNA 聚合酶和拓扑异构酶的折叠,具有一个聚集了酸性残基的活性位点。对接分析显示出一个 DNA 结合表面,周围是柔性环,表明在 DNA 结合时会发生相当大的构象变化。体外测定表明,pUL15C 具有非序列特异性、Mg2+依赖性核酸酶活性。这些结果表明,pUL15 利用类似于 RNase H 的金属离子介导的催化机制切割病毒连接的 DNA。该结构揭示了除 RNase H 样折叠核心之外的额外结构元素,以及核酸酶活性位点的局部结构变化,这些变化在疱疹病毒末端酶中保守,并与噬菌体 T4 gp17 非常相似,但与 Podovirus 和 Siphovirus 同源物以及细胞 RNase H 不同,在一个大型真核病毒家族和简单和复杂的原核病毒中划定了一个新的进化谱系。

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