The HNH endonuclease domain of the giant virus MutS7 specifically binds to branched DNA structures with single-stranded regions

IF 3 3区 生物学 Q2 GENETICS & HEREDITY DNA Repair Pub Date : 2025-01-01 DOI:10.1016/j.dnarep.2024.103804
Satoshi Yoshioka , Hirochika Kurazono , Koki Ohshita , Kenji Fukui , Masaharu Takemura , Shin-Ichiro Kato , Kouhei Ohnishi , Takato Yano , Taisuke Wakamatsu
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Abstract

Most giant viruses including Mimiviridae family build large viral factories within the host cytoplasms. These giant viruses are presumed to possess specific genes that enable the rapid and massive replication of their large double-stranded DNA genomes within viral factories. It has been revealed that a functionally uncharacterized protein, MutS7, is expressed during the operational phase of the viral factory. MutS7 contains an N-terminal mismatched DNA-binding domain, which is similar to the mismatched DNA-recognizing protein MutS1, and a unique C-terminal HNH endonuclease domain absent in other MutS family proteins. MutS7 gene of the genus Mimivirus of the family Mimiviridae is encoded in the locus that is responsible for resistance against infection of a virophage. In the present study, we characterized the MutS7 HNH domain of Mimivirus shirakomae. The HNH domain preferentially bound to branched DNA structures containing single-stranded regions, especially the displacement-loop structure, which is a primary intermediate in homologous/homeologous recombination, rather than to linear DNAs and branched DNAs lacking single-stranded regions. However, the HNH domain exhibited no endonuclease activity. The site-directed mutagenesis analysis revealed that the Cys4-type zinc finger of the HNH domain was not essential, but was important for the DNA binding. Given that giant virus MutS7 contains a mismatch-binding domain in addition to the HNH domain, we propose that giant virus MutS7 may suppress homeologous recombination in the viral factory.
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巨型病毒MutS7的HNH内切酶结构域特异性地与单链区域的支链DNA结构结合。
包括迷你病毒科在内的大多数巨型病毒在宿主细胞质内建立大型病毒工厂。据推测,这些巨型病毒拥有特定的基因,使其大型双链DNA基因组能够在病毒工厂内快速大量复制。已经发现在病毒工厂的操作阶段表达了一种功能上未表征的蛋白MutS7。MutS7含有一个与错配dna识别蛋白MutS1相似的n端错配dna结合结构域,以及一个其他MutS家族蛋白所缺乏的独特的c端HNH内切酶结构域。米米病毒科米米病毒属的MutS7基因编码在负责抵抗病毒噬菌体感染的位点上。在本研究中,我们对shirakomae Mimivirus的MutS7 HNH结构域进行了表征。HNH结构域优先与含有单链区域的支链DNA结构结合,特别是作为同源/同源重组初级中间体的位移环结构,而不是与缺乏单链区域的线性DNA和支链DNA结合。然而,HNH结构域没有表现出内切酶活性。位点突变分析表明,HNH结构域的cys4型锌指不是必需的,但对DNA结合很重要。鉴于巨型病毒MutS7除了HNH结构域外还含有一个错配结合结构域,我们提出巨型病毒MutS7可能抑制病毒工厂中的同源重组。
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来源期刊
DNA Repair
DNA Repair 生物-毒理学
CiteScore
7.60
自引率
5.30%
发文量
91
审稿时长
59 days
期刊介绍: DNA Repair provides a forum for the comprehensive coverage of DNA repair and cellular responses to DNA damage. The journal publishes original observations on genetic, cellular, biochemical, structural and molecular aspects of DNA repair, mutagenesis, cell cycle regulation, apoptosis and other biological responses in cells exposed to genomic insult, as well as their relationship to human disease. DNA Repair publishes full-length research articles, brief reports on research, and reviews. The journal welcomes articles describing databases, methods and new technologies supporting research on DNA repair and responses to DNA damage. Letters to the Editor, hot topics and classics in DNA repair, historical reflections, book reviews and meeting reports also will be considered for publication.
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