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首页> 外文期刊>Mutation Research: International Journal on Mutagenesis, Chromosome Breakage and Related Subjects >UV but not X rays stimulate homologous recombination between sister chromatids and homologs in a Saccharomyces cerevisiae mec1 (ATR) hypomorphic mutant.
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UV but not X rays stimulate homologous recombination between sister chromatids and homologs in a Saccharomyces cerevisiae mec1 (ATR) hypomorphic mutant.

机译:紫外线而不是X射线会刺激酿酒酵母mec1(ATR)亚型突变体中姐妹染色单体和同源物之间的同源重组。

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摘要

MEC1, the essential yeast ATM/ATR homolog, prevents replication fork collapse and is required for the cellular response to DNA damage. We had previously observed higher rates of spontaneous SCE, heteroallelic recombination and translocations in mec1-21 mutants, which still retain some G2 checkpoint function, compared to mec1 null mutants, which are completely defective in checkpoint function, and wild type. However, the types of DNA lesions that are more recombinogenic in mec1-21, compared to wild type, are unknown. Here, we measured DNA damage-associated SCE, homolog (heteroallelic) recombination, and homology-directed translocations in mec1-21, and characterized types of DNA damage-associated chromosomal rearrangements that occur in mec1-21. Although frequencies of UV-associated recombination were higher in mec1-21, the mutant was defective in double-strand break-associated SCE and heteroallelic recombination. Over-expression of Rad53 in mec1-21 reduced UV-associated recombination but did not suppress the defect in X-ray-associated recombination. Both X ray and UV exposure increased translocation frequencies in mec1-21, but the majority of the UV-associated products were non-reciprocal translocations. We suggest that although recombinational repair of double-stand breaks is less efficient in mec1 mutants, recombinants may be generated by other mechanisms, such as break-induced replication.
机译:MEC1是必需的酵母ATM / ATR同源物,可防止复制叉崩溃,是细胞对DNA损伤的反应所必需的。我们之前曾观察到与保留了G2检查点功能的野生型相比,仍保留某些G2检查点功能的mec1-21突变体的自发SCE,异位基因重组和易位的比率更高。但是,与野生型相比,在mec1-21中重组产生更多的DNA损伤的类型尚不清楚。在这里,我们测量了mec1-21中与DNA损伤相关的SCE,同源(杂等位基因)重组和同源性定向易位,并表征了在mec1-21中发生的与DNA损伤相关的染色体重排的类型。尽管在mec1-21中与UV相关的重组频率更高,但该突变体在双链断裂相关SCE和异源等位基因重组中存在缺陷。 mec1-21中Rad53的过度表达减少了与UV相关的重组,但没有抑制与X射线相关的重组中的缺陷。 X射线和紫外线照射都增加了mec1-21中的易位频率,但是大多数与紫外线相关的产物都是不可逆的易位。我们建议,尽管双支架断裂的重组修复在mec1突变体中效率较低,但重组体可能是由其他机制产生的,例如断裂诱导的复制。

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