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肖普纤维瘤病毒DNA连接酶基因的特性分析

Characterization of the Shope fibroma virus DNA ligase gene.

作者信息

Parks R J, Lichty B D, Karakis C, Evans D H

机构信息

Department of Molecular Biology and Genetics, University of Guelph, Ontario, Canada.

出版信息

Virology. 1994 Aug 1;202(2):642-50. doi: 10.1006/viro.1994.1385.

DOI:10.1006/viro.1994.1385
PMID:8030229
Abstract

The Shope fibroma virus (SFV) DNA ligase gene has been cloned and sequenced, and the biochemical requirements of the gene product have been determined in vitro. The SFV ligase gene maps to the BamHI L1/L2 boundary and spans 1.7 kb. The gene is predicted to encode a 559-amino-acid protein of M(r) = 63,139 which shares 45% amino acid identity with Orthopoxvirus ligases. The C-terminal two-thirds of the protein appears to encode the catalytic domain and shares distant homology with many ligases. The N-terminal homology is shared between only Orthopoxviruses and Leporipoxviruses and suggests that DNA ligases may be composite structures consisting of two independently evolved protein domains. Although the the gene encodes features characteristic of both early and late poxviral genes, Northern analysis showed that SFV ligase is expressed as a late gene product. In order to prove the identity of the protein it was expressed as a glutathione S-transferase fusion in Escherichia coli, affinity purified, and shown to be a Mg2+.ATP-dependent ligase in vitro. The recombinant protein can also form a covalent ligase.AMP complex characteristic of ATP-dependent DNA ligases. The SFV ligase gene can be disrupted and is thus not essential for viral growth in culture. This was shown by recombining a PCR product, encoding a P7.5 promoter and E. coli guanine phosphoribosyltransferase gene (gpt) into the open reading frame, and selecting for gpt+ viruses. This work provides insights into the evolution of Orthopoxviruses and Leporipoxviruses and strains suitable for a detailed analysis of the role DNA ligases play in poxviral recombination.

摘要

肖普纤维瘤病毒(SFV)DNA连接酶基因已被克隆和测序,并在体外确定了该基因产物的生化需求。SFV连接酶基因定位于BamHI L1/L2边界,跨度为1.7 kb。该基因预计编码一个559个氨基酸的蛋白质,分子量为63,139,与正痘病毒连接酶有45%的氨基酸同一性。该蛋白质的C端三分之二似乎编码催化结构域,与许多连接酶有远缘同源性。N端同源性仅在正痘病毒和兔痘病毒之间存在,这表明DNA连接酶可能是由两个独立进化的蛋白质结构域组成的复合结构。尽管该基因编码了早期和晚期痘病毒基因的特征,但Northern分析表明SFV连接酶作为晚期基因产物表达。为了证明该蛋白质的身份,它在大肠杆菌中作为谷胱甘肽S-转移酶融合蛋白表达,经亲和纯化后,在体外显示为一种Mg2+依赖的ATP连接酶。重组蛋白还可以形成ATP依赖的DNA连接酶特有的共价连接酶-AMP复合物。SFV连接酶基因可以被破坏,因此对病毒在培养中的生长不是必需的。这是通过将编码P7.5启动子和大肠杆菌鸟嘌呤磷酸核糖转移酶基因(gpt)的PCR产物重组到开放阅读框中,并筛选gpt+病毒来证明的。这项工作为正痘病毒和兔痘病毒的进化以及适合详细分析DNA连接酶在痘病毒重组中作用的菌株提供了见解。

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