The FHA domain of PNKP is essential for its recruitment to DNA damage sites and maintenance of genome stability

IF 1.5 4区 医学 Q4 BIOTECHNOLOGY & APPLIED MICROBIOLOGY
Kaima Tsukada , Mikio Shimada , Rikiya Imamura , Kotaro Saikawa , Masamichi Ishiai , Yoshihisa Matsumoto
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引用次数: 9

Abstract

Polynucleotide kinase phosphatase (PNKP) has dual enzymatic activities as kinase and phosphatase for DNA ends, which are the prerequisite for the ligation, and thus is involved in base excision repair, single-strand break repair and non-homologous end joining for double-strand break (DSB) repair. In this study, we examined mechanisms for the recruitment of PNKP to DNA damage sites by laser micro-irradiation and live-cell imaging analysis using confocal microscope. We show that the forkhead-associated (FHA) domain of PNKP is essential for the recruitment of PNKP to DNA damage sites. Arg35 and Arg48 within the FHA domain are required for interactions with XRCC1 and XRCC4. PNKP R35A/R48A mutant failed to accumulate on the laser track and siRNA-mediated depletion of XRCC1 and/or XRCC4 reduced PNKP accumulation on the laser track, indicating that PNKP is recruited to DNA damage sites via the interactions between its FHA domain and XRCC1 or XRCC4. Furthermore, cells expressing PNKP R35A/R48A mutant exhibited increased sensitivity toward ionizing radiation in association with delayed SSB and DSB repair and genome instability, represented by micronuclei and chromosome bridges. Taken together, these findings revealed the importance of PNKP recruitment to DNA damage sites via its FHA domain for DNA repair and maintenance of genome stability.

Abstract Image

PNKP的FHA结构域对其招募DNA损伤位点和维持基因组稳定性至关重要
多核苷酸激酶磷酸酶(PNKP)具有DNA末端激酶和磷酸酶的双重酶活性,这是DNA连接的先决条件,因此参与碱基切除修复、单链断裂修复和双链断裂(DSB)修复的非同源末端连接。在这项研究中,我们通过激光微照射和共聚焦显微镜下的活细胞成像分析,研究了PNKP在DNA损伤部位的招募机制。我们发现PNKP的叉头相关(FHA)结构域对于将PNKP招募到DNA损伤位点至关重要。与XRCC1和XRCC4相互作用需要FHA域中的Arg35和Arg48。PNKP R35A/R48A突变体未能在激光轨迹上积累,sirna介导的XRCC1和/或XRCC4的缺失减少了PNKP在激光轨迹上的积累,表明PNKP通过其FHA结构域与XRCC1或XRCC4之间的相互作用被募集到DNA损伤位点。此外,表达PNKP R35A/R48A突变体的细胞对电离辐射的敏感性增加,与SSB和DSB修复延迟和基因组不稳定有关,以微核和染色体桥为代表。综上所述,这些发现揭示了PNKP通过其FHA结构域招募到DNA损伤位点对DNA修复和维持基因组稳定性的重要性。
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来源期刊
CiteScore
4.90
自引率
0.00%
发文量
24
审稿时长
51 days
期刊介绍: Mutation Research (MR) provides a platform for publishing all aspects of DNA mutations and epimutations, from basic evolutionary aspects to translational applications in genetic and epigenetic diagnostics and therapy. Mutations are defined as all possible alterations in DNA sequence and sequence organization, from point mutations to genome structural variation, chromosomal aberrations and aneuploidy. Epimutations are defined as alterations in the epigenome, i.e., changes in DNA methylation, histone modification and small regulatory RNAs. MR publishes articles in the following areas: Of special interest are basic mechanisms through which DNA damage and mutations impact development and differentiation, stem cell biology and cell fate in general, including various forms of cell death and cellular senescence. The study of genome instability in human molecular epidemiology and in relation to complex phenotypes, such as human disease, is considered a growing area of importance. Mechanisms of (epi)mutation induction, for example, during DNA repair, replication or recombination; novel methods of (epi)mutation detection, with a focus on ultra-high-throughput sequencing. Landscape of somatic mutations and epimutations in cancer and aging. Role of de novo mutations in human disease and aging; mutations in population genomics. Interactions between mutations and epimutations. The role of epimutations in chromatin structure and function. Mitochondrial DNA mutations and their consequences in terms of human disease and aging. Novel ways to generate mutations and epimutations in cell lines and animal models.
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