Overexpression of the NEK8 kinase inhibits homologous recombination

IF 2.7 3区 生物学 Q2 GENETICS & HEREDITY
Joshua L. Turner, Georgia Moore, Tyler J. McCraw, Jennifer M. Mason
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引用次数: 0

Abstract

Homologous recombination proteins maintain genome stability by repairing double strand breaks and protecting replication fork stability. Defects in homologous recombination results in cancer predisposition but can be exploited due to increased sensitivity to certain chemotherapeutics such as PARP inhibitors. The NEK8 kinase has roles in the replication response and homologous recombination. NEK8 is overexpressed in breast cancer, but the impact of NEK8 overexpression on homologous recombination has not been determined. Here, we demonstrate NEK8 overexpression inhibits RAD51 focus formation resulting in a defect in homologous recombination and degradation of stalled replication forks. Importantly, NEK8 overexpression sensitizes cells to the PARP inhibitor, Olaparib. Together, our results suggest NEK8 overexpressing tumors may be recombination-deficient and respond to chemotherapeutics that target defects in recombination such as Olaparib.
NEK8激酶过表达抑制同源重组
同源重组蛋白通过修复双链断裂和保护复制叉的稳定性来维持基因组的稳定性。同源重组的缺陷导致癌症易感性,但由于对某些化疗药物(如PARP抑制剂)的敏感性增加,可以利用。NEK8激酶在复制反应和同源重组中起作用。NEK8在乳腺癌中过表达,但NEK8过表达对同源重组的影响尚未确定。在这里,我们证明NEK8过表达抑制RAD51焦点形成,导致同源重组缺陷和停滞复制分叉的降解。重要的是,NEK8过表达使细胞对PARP抑制剂Olaparib敏感。总之,我们的研究结果表明NEK8过表达的肿瘤可能是重组缺陷的,并且对靶向重组缺陷的化疗药物(如奥拉帕尼)有反应。
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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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