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直接证据表明,紫外线(UV)照射损伤的单纯疱疹病毒(HSV)DNA 可以在依赖于细胞类型的方式下修复。

Direct evidence that HSV DNA damaged by ultraviolet (UV) irradiation can be repaired in a cell type-dependent manner.

机构信息

Drexel Institute for Biotechnology and Virology Research and Department of Microbiology and Immunology, Drexel University College of Medicine, Doylestown, PA 18902, USA.

出版信息

J Neurovirol. 2012 Jun;18(3):231-43. doi: 10.1007/s13365-012-0105-2. Epub 2012 May 12.

Abstract

Infection of permissive cells, in tissue culture, with herpes simplex virus (HSV) has been reported to induce host DNA damage repair responses that are necessary for efficient viral replication. However, direct repair of the damaged viral DNA has not, to our knowledge, been shown. In this report, we detect and determine the amount of damaged HSV-1 DNA, following introduction of experimentally damaged HSV genomes into tissue cultures of permissive Vero, NGF differentiated PC12 cells and primary rat neurons, using a method of detection introduced here. The results show that HSV-1 strain 17 DNA containing UV-induced DNA damage is efficiently repaired, in Vero, but not NGF differentiated PC12 cells. The primary rat neuronal cultures were capable of repairing the damaged viral DNA, but with much less efficiency than did the permissive Vero cells. Moreover, by conducting the experiments with either an inhibitor of the HSV polymerase (phosphonoacetic acid [PAA]) or with a replication defective DNA polymerase mutant virus, HP66, the results suggest that repair can occur in the absence of a functional viral polymerase, although polymerase function seems to enhance the efficiency of the repair, in a replication independent manner. The possible significance of varying cell type mediated repair of viral DNA to viral pathogenesis is discussed.

摘要

在组织培养中,允许细胞感染单纯疱疹病毒(HSV)已被报道会诱导宿主 DNA 损伤修复反应,这对于病毒的有效复制是必要的。然而,据我们所知,受损的病毒 DNA 并没有直接修复。在本报告中,我们使用这里介绍的检测方法,检测并确定在将实验性受损的 HSV 基因组引入允许的 Vero、NGF 分化的 PC12 细胞和原代大鼠神经元的组织培养物后,受损的 HSV-1 DNA 的数量。结果表明,含有 UV 诱导的 DNA 损伤的 HSV-1 株 17 DNA 在 Vero 中,但在 NGF 分化的 PC12 细胞中不能有效修复。原代大鼠神经元培养物能够修复受损的病毒 DNA,但效率远低于允许的 Vero 细胞。此外,通过用 HSV 聚合酶抑制剂(膦甲酸钠[PAA])或复制缺陷型 DNA 聚合酶突变病毒 HP66 进行实验,结果表明,尽管聚合酶功能似乎以不依赖于复制的方式增强修复的效率,但在没有功能性病毒聚合酶的情况下,修复也可以发生。讨论了不同细胞类型介导的病毒 DNA 修复对病毒发病机制的可能意义。

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