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Nucleosome resection at a double-strand break during Non-Homologous Ends Joining in mammalian cells - implications from repressive chromatin organization and the role of ARTEMIS

机译:非同源末端连接哺乳动物细胞时在双链断裂处进行核小体切除-抑制性染色质组织和ARTEMIS的作用

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摘要

BackgroundThe S. cerevisiae mating type switch model of double-strand break (DSB) repair, utilizing the HO endonuclease, is one of the best studied systems for both Homologous Recombination Repair (HRR) and direct ends-joining repair (Non-Homologous Ends Joining - NHEJ). We have recently transposed that system to a mammalian cell culture model taking advantage of an adenovirus expressing HO and an integrated genomic target. This made it possible to compare directly the mechanism of repair between yeast and mammalian cells for the same type of induced DSB. Studies of DSB repair have emphasized commonality of features, proteins and machineries between organisms, and differences when conservation is not found. Two proteins that stand out that differ between yeast and mammalian cells are DNA-PK, a protein kinase that is activated by the presence of DSBs, and Artemis, a nuclease whose activity is modulated by DNA-PK and ATM. In this report we describe how these two proteins may be involved in a specific pattern of ends-processing at the DSB, particularly in the context of heterochromatin.
机译:背景技术利用HO核酸内切酶的双链断裂(DSB)酿酒酵母交配型开关模型是同源重组修复(HRR)和直接末端连接修复(非同源末端连接)研究最多的系统之一-NHEJ)。我们最近已将该系统转换为利用表达HO和整合基因组靶标的腺病毒的哺乳动物细胞培养模型。这使得可以直接比较酵母和哺乳动物细胞对相同类型的诱导DSB的修复机制。 DSB修复的研究强调了生物之间的特征,蛋白质和机制的共性,以及在未发现保守性时的差异。在酵母和哺乳动物细胞之间脱颖而出的两种蛋白质是DNA-PK(一种被DSB激活的蛋白激酶)和Artemis(一种核酸酶,其活性受DNA-PK和ATM调节)。在本报告中,我们描述了这两种蛋白质如何与DSB末端加工的特定模式有关,特别是在异染色质的情况下。

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