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痘苗病毒哥本哈根株中的一个DNA连接酶基因对于病毒复制和重组而言并非必需。

A DNA ligase gene in the Copenhagen strain of vaccinia virus is nonessential for viral replication and recombination.

作者信息

Colinas R J, Goebel S J, Davis S W, Johnson G P, Norton E K, Paoletti E

机构信息

Department of Microbiology and Immunology, Albany Medical College, New York 12208.

出版信息

Virology. 1990 Nov;179(1):267-75. doi: 10.1016/0042-6822(90)90295-3.

Abstract

Biochemical and genetic analyses have been conducted to determine whether a vaccinia virus open reading frame (orf) with extensive homology to the Saccharomyces cerevisiae DNA ligase gene encodes a functional ligase activity. This orf in HindIII A, designated A50R, is capable of encoding a 552-amino-acid, 63.4-kDa polypeptide. Full-length A50R mRNA produced in vitro directed the synthesis of a polypeptide with an apparent molecular weight of 57 kDa. Significantly, translation reactions programmed with A50R mRNA were capable of ligating a 3-kb Notl restriction fragment into multimers. DNA ligase activity was not detectable when either truncated sense or full-length antisense mRNA was translated in vitro. In extracts prepared from cells infected with wt vaccinia virus, DNA ligase activity was detected as assayed by the formation of a 57 kDa ligase-AMP adduct which was expressed early in the viral replication cycle. In cells infected with a DNA ligase deletion mutant no equivalent AMP-labeled adduct was detected. Relative to wt virus, the DNA ligase deletion mutant exhibited no significant differences in homologous recombination. These results indicate that the vaccinia orf A50R encodes a functional DNA ligase expressed early in infection, but this DNA ligase is nonessential for either recombination or viral replication.

摘要

已进行生化和遗传分析,以确定与酿酒酵母DNA连接酶基因具有广泛同源性的痘苗病毒开放阅读框(orf)是否编码功能性连接酶活性。HindIII A中的这个orf,命名为A50R,能够编码一个552个氨基酸、63.4 kDa的多肽。体外产生的全长A50R mRNA指导合成了一个表观分子量为57 kDa的多肽。重要的是,用A50R mRNA编程的翻译反应能够将一个3 kb的Notl限制片段连接成多聚体。当体外翻译截短的正义或全长反义mRNA时,未检测到DNA连接酶活性。在用野生型痘苗病毒感染的细胞制备的提取物中,通过形成57 kDa连接酶-AMP加合物检测到DNA连接酶活性,该加合物在病毒复制周期早期表达。在用DNA连接酶缺失突变体感染的细胞中,未检测到等效的AMP标记加合物。相对于野生型病毒,DNA连接酶缺失突变体在同源重组方面没有显著差异。这些结果表明,痘苗orf A50R编码一种在感染早期表达的功能性DNA连接酶,但这种DNA连接酶对于重组或病毒复制不是必需的。

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