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酿酒酵母单倍体细胞中MMS诱导的DNA双链断裂的修复,这需要存在一个重复的基因组。

Repair of MMS-induced DNA double-strand breaks in haploid cells of Saccharomyces cerevisiae, which requires the presence of a duplicate genome.

作者信息

Chlebowicz E, Jachymczyk W J

出版信息

Mol Gen Genet. 1979 Jan 2;167(3):279-86. doi: 10.1007/BF00267420.

Abstract

The formation and repair of double-strand breaks induced in DNA by MMS was studied in haploid wild type and MMS-sensitive rad6 mutant strains of Saccharomyces cerevisiae with the use of the neutral and alkaline sucrose sedimentation technique. A similar decrease in average molecular weight of double-stranded DNA from 5--6 X 10(8) to 1--0.7 X 10(8) daltons was observed following treatment with 0.5% MMS in wild type and mutant strains. Incubation of cells after MMS treatment in a fresh drug-free growing medium resulted in repair of double-strand breaks in the wild type stain, but only in the exponential phase of growth. No repair of double-strand breaks was found when cells of the wild type strain were synchronized in G-1 phase by treatment with alpha factor, although DNA single-strand breaks were still efficiently repaired. Mutant rad6 which has a very low ability to repair MMS-induced single-strand breaks, did not repair double-strand breaks regardless of the phase of growth. These results suggest that (1) repair of double-strand breaks requires the ability for single-strand breaks repair, (2) rejoining of double-strand breaks requires the availability of two homologous DNA molecules, this strongly supports the recombinational model of DNA repair.

摘要

利用中性和碱性蔗糖沉降技术,研究了在酿酒酵母的单倍体野生型和对甲磺酸甲酯(MMS)敏感的rad6突变株中,由MMS诱导的DNA双链断裂的形成和修复情况。在用0.5% MMS处理后,在野生型和突变株中均观察到双链DNA的平均分子量有类似的下降,从5 - 6×10⁸道尔顿降至1 - 0.7×10⁸道尔顿。MMS处理后的细胞在新鲜的无药物生长培养基中孵育,野生型菌株中的双链断裂得以修复,但仅在生长的指数期。当野生型菌株的细胞通过α因子处理同步于G-1期时,未发现双链断裂的修复,尽管DNA单链断裂仍能被有效修复。修复MMS诱导的单链断裂能力非常低的突变体rad6,无论处于生长的哪个阶段,都不能修复双链断裂。这些结果表明:(1)双链断裂的修复需要单链断裂修复的能力;(2)双链断裂的重新连接需要两个同源DNA分子的存在,这有力地支持了DNA修复的重组模型。

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