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依托泊苷诱导的痘苗病毒端粒分辨率阻滞依赖于病毒编码的DNA连接酶。

An etoposide-induced block in vaccinia virus telomere resolution is dependent on the virus-encoded DNA ligase.

作者信息

DeLange A M, Carpenter M S, Choy J, Newsway V E

机构信息

Department of Human Genetics, University of Manitoba, Winnipeg, Canada.

出版信息

J Virol. 1995 Apr;69(4):2082-91. doi: 10.1128/JVI.69.4.2082-2091.1995.

Abstract

Etoposide, an inhibitor of the breakage-reunion reaction associated with cellular type II DNA topoisomerases, was shown to inhibit plaque formation of vaccinia virus. This drug had a major effect on the segregation of newly replicated DNA concatemers. Gene expression and the initiation and elongation phases of viral DNA replication were essentially unaffected. Pulsed-field gel electrophoresis of viral DNA replicated in the presence of etoposide revealed two major classes of DNA: the mature monomeric linear genome and DNA that failed to enter the gel (the relative proportions depending on the concentrations of drug). Restriction enzyme analysis showed a severe defect in telomere resolution. In addition, slowly migrating restriction fragments were suggestive of a general recombination defect. We have isolated several etoposide-resistant mutants and used marker rescue and DNA sequencing to localize the resistance-causing mutation to the amino terminus of the viral DNA ligase gene. Inactivation of the DNA ligase also resulted in an etoposide-resistant phenotype, but to a lesser extent. The telomere resolution and segregation defects were corrected both in the drug-resistant mutants and in the DNA ligase knockout mutants. Reinsertion of wild-type or mutant DNA ligase in the viral thymidine kinase locus confirmed the role of the viral DNA ligase in conferring sensitivity not only to etoposide but also to another topoisomerase II inhibitor, 4'-(9-acridinylamino) methanesulphon-m-anisidide (mAMSA). The data suggest that the nonessential DNA ligase is involved in telomere resolution, possibly as part of a general recombinase.

摘要

依托泊苷是一种与细胞II型DNA拓扑异构酶相关的断裂-重连反应抑制剂,已被证明能抑制痘苗病毒的蚀斑形成。该药物对新复制的DNA串联体的分离有重大影响。基因表达以及病毒DNA复制的起始和延伸阶段基本未受影响。在依托泊苷存在的情况下复制的病毒DNA的脉冲场凝胶电泳显示出两类主要的DNA:成熟的单体线性基因组和未能进入凝胶的DNA(相对比例取决于药物浓度)。限制性内切酶分析显示端粒分辨率存在严重缺陷。此外,缓慢迁移的限制性片段提示存在普遍的重组缺陷。我们分离出了几个对依托泊苷耐药的突变体,并使用标记拯救和DNA测序将导致耐药的突变定位到病毒DNA连接酶基因的氨基末端。DNA连接酶的失活也导致了对依托泊苷的耐药表型,但程度较轻。在耐药突变体和DNA连接酶敲除突变体中,端粒分辨率和分离缺陷均得到了纠正。在病毒胸苷激酶基因座中重新插入野生型或突变型DNA连接酶证实了病毒DNA连接酶不仅在赋予对依托泊苷的敏感性方面起作用,而且在赋予对另一种拓扑异构酶II抑制剂4'-(9-吖啶基氨基)甲磺基间茴香胺(mAMSA)的敏感性方面也起作用。数据表明,非必需的DNA连接酶参与端粒分辨率,可能作为一般重组酶的一部分。

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