Ubiquitin-specific protease 15 interacts directly with the HSV-1 alkaline nuclease and facilitates viral recombination and replication fork stability.

IF 3.8 2区医学 Q2 VIROLOGY

Journal of Virology Pub Date : 2025-09-23 Epub Date: 2025-08-18 DOI:10.1128/jvi.00893-25

Yee Vue, Patrick J Mullon, Alexander Leehangin, Emiliano Maldonado-Luevano, Tyler D Hasselmann, Kavi P M Mehta, Kareem N Mohni

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引用次数: 0

Abstract

Herpes simplex virus type 1 replicates in the nucleus of the host cell and utilizes many cellular proteins to facilitate DNA replication. HSV-1 DNA replication is closely linked with homologous recombination, and HSV-1 encodes a two-subunit recombinase consisting of an exonuclease (UL12) and a single-strand DNA-binding protein (ICP8). We identified the cellular deubiquitinating enzyme USP15 as a new UL12-binding partner. USP15 is one of the most enriched proteins on viral DNA and has recently been implicated in regulating cellular homologous recombination. Utilizing isolation of proteins on nascent DNA (iPOND) to compare the proteins on wild-type and UL12-deficient viruses, we observed that USP15 is not recruited to newly replicated DNA in the absence of UL12. We also observed that UL12 and USP15 interact directly in vitro using purified proteins. Together, these data suggest that UL12 directly recruits USP15 to viral DNA. UL12 stimulates a type of homology-directed repair called single-strand annealing (SSA). We generated a USP15 knockout cell line with an integrated GFP-based SSA reporter and observed that UL12 and USP15 both contribute to the maximal induction of SSA. In addition to the reporter cell line, there is a 10-fold reduction in the frequency of marker rescue, and individual replication forks move slower in the absence of USP15. These data support a role for USP15 in facilitating recombination during the virus life cycle and the maintenance of replication fork stability.IMPORTANCEHSV-1 is a ubiquitous pathogen in the global population that causes lifelong latent infection with sporadic reactivation in the host. It has long been appreciated that HSV-1 DNA replication exhibits high rates of recombination and is linked to the host DNA damage response. In this study, we show a novel interaction between UL12, a member of the HSV recombinase, and the deubiquitinating host enzyme USP15. We show that USP15 physically interacts with UL12 and is required for UL12 to maximally stimulate recombination. In the absence of USP15, we also observe an overall reduction in virus growth. This work demonstrated that host proteins facilitate viral-induced recombination. The interaction of USP15 with UL12 represents a potential target for intervention against HSV-1 infection and associated disease.

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泛素特异性蛋白酶15直接与HSV-1碱性核酸酶相互作用，促进病毒重组和复制叉的稳定性。

1型单纯疱疹病毒在宿主细胞核内复制，利用许多细胞蛋白促进DNA复制。HSV-1的DNA复制与同源重组密切相关，并且HSV-1编码由外切酶（UL12）和单链DNA结合蛋白（ICP8）组成的双亚基重组酶。我们发现细胞去泛素化酶USP15是一个新的ul12结合伙伴。USP15是病毒DNA上最富集的蛋白之一，最近被认为与调节细胞同源重组有关。利用新生DNA上的蛋白质分离（iPOND）来比较野生型和UL12缺陷病毒上的蛋白质，我们发现在缺乏UL12的情况下，USP15不会被招募到新复制的DNA上。我们还观察到UL12和USP15在体外通过纯化蛋白直接相互作用。总之，这些数据表明UL12直接将USP15招募到病毒DNA上。UL12刺激一种称为单链退火（SSA）的同源定向修复。我们利用集成gfp的SSA报告基因构建了USP15敲除细胞系，并观察到UL12和USP15都能最大程度地诱导SSA。除了报告细胞系外，在缺乏USP15的情况下，标记拯救的频率降低了10倍，单个复制分叉移动更慢。这些数据支持USP15在病毒生命周期中促进重组和维持复制叉稳定性方面的作用。hsv -1是一种在全球人群中普遍存在的病原体，可在宿主中引起终身潜伏感染并散发再激活。人们早就认识到，HSV-1 DNA复制表现出高重组率，并与宿主DNA损伤反应有关。在这项研究中，我们发现了HSV重组酶的成员UL12与去泛素化宿主酶USP15之间的一种新的相互作用。我们发现USP15与UL12物理相互作用，并且UL12需要USP15来最大限度地刺激重组。在缺乏USP15的情况下，我们还观察到病毒生长的总体减少。这项工作表明，宿主蛋白促进病毒诱导的重组。USP15与UL12的相互作用是干预HSV-1感染和相关疾病的潜在靶点。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Journal of Virology 医学-病毒学

CiteScore

10.10

自引率

7.40%

发文量

906

审稿时长

1 months

期刊介绍： Journal of Virology (JVI) explores the nature of the viruses of animals, archaea, bacteria, fungi, plants, and protozoa. We welcome papers on virion structure and assembly, viral genome replication and regulation of gene expression, genetic diversity and evolution, virus-cell interactions, cellular responses to infection, transformation and oncogenesis, gene delivery, viral pathogenesis and immunity, and vaccines and antiviral agents.