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Development of an assay to measure mutagenic non-homologous end-joining repair activity in mammalian cells

机译:测量哺乳动物细胞中诱变的非同源末端连接修复活性的测定方法的开发

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摘要

Double-strand break (DSB) repair pathways are critical for the maintenance of genomic integrity and the prevention of tumorigenesis in mammalian cells. Here, we present the development and validation of a novel assay to measure mutagenic non-homologous end-joining (NHEJ) repair in living cells, which is inversely related to canonical NHEJ and is based on the sequence-altering repair of a single site-specific DSB at an intrachromosomal locus. We have combined this mutagenic NHEJ assay with an established homologous recombination (HR) assay such that both pathways can be monitored simultaneously. In addition, we report the development of a ligand-responsive I-SceI protein, in which the timing and kinetics of DSB induction can be precisely controlled by regulating protein stability and cellular localization in cells. Using this system, we report that mutagenic NHEJ repair is suppressed in growth-arrested and serum-deprived cells, suggesting that end-joining activity in proliferating cells is more likely to be mutagenic. Collectively, the novel DSB repair assay and inducible I-SceI will be useful tools to further elucidate the complexities of NHEJ and HR repair.
机译:双链断裂(DSB)修复途径对于维持基因组完整性和预防哺乳动物细胞中的肿瘤发生至关重要。在这里,我们介绍了一种新颖的测定方法的开发和验证,该测定方法用于测量活细胞中的诱变非同源末端连接(NHEJ)修复,这与规范NHEJ呈反相关,并且基于单个位点的序列更改修复-染色体内基因座的特定DSB。我们已经将这种诱变的NHEJ检测与已建立的同源重组(HR)检测结合在一起,从而可以同时监控两个途径。此外,我们报告了配体反应性I-SceI蛋白的发展,其中可以通过调节蛋白质的稳定性和细胞在细胞中的定位来精确控制DSB诱导的时间和动力学。使用该系统,我们报告说诱变的NHEJ修复在生长停滞和血清缺乏的细胞中被抑制,这表明增殖细胞中的末端连接活性更可能是诱变的。总的来说,新颖的DSB修复测定和可诱导的I-SceI将成为进一步阐明NHEJ和HR修复的复杂性的有用工具。

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