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酵母中缺乏RAD51时的双链断裂修复:断裂诱导的DNA复制的可能作用。

Double-strand break repair in the absence of RAD51 in yeast: a possible role for break-induced DNA replication.

作者信息

Malkova A, Ivanov E L, Haber J E

机构信息

Rosenstiel Center and Department of Biology, Brandeis University, Waltham, MA 02254-9110, USA.

出版信息

Proc Natl Acad Sci U S A. 1996 Jul 9;93(14):7131-6. doi: 10.1073/pnas.93.14.7131.

Abstract

In wild-type diploid cells of Saccharomyces cerevisiae, an HO endonuclease-induced double-strand break (DSB) at the MAT locus can be efficiently repaired by gene conversion using the homologous chromosome sequences. Repair of the broken chromosome was nearly eliminated in rad52delta diploids; 99% lost the broken chromosome. However, in rad51delta diploids, the broken chromosomes were repaired approximately 35% of the time. None of these repair events were simple gene conversions or gene conversions with an associated crossover, instead, they created diploids homozygous for the MAT locus and all markers in the 100-kb region distal to the site of the DSB. In rad51delta diploids, the broken chromosome can apparently be inherited for several generations, as many of these repair events are found as sectored colonies, with one part being repaired and the other part being lost the broken chromosome. Similar events occur in about 2% of wild-type cells. We propose that a broken chromosome end can invade a homologous template in the absence of RAD51 and initiate DNA replication that may extend to the telomere, 100 or more kb away. Such break-induced replication appears to be similar to recombination-initiated replication in bacteria.

摘要

在酿酒酵母的野生型二倍体细胞中,MAT位点处由HO核酸内切酶诱导产生的双链断裂(DSB)可通过利用同源染色体序列的基因转换有效修复。在rad52δ二倍体细胞中,断裂染色体的修复几乎完全消除;99%的细胞丢失了断裂的染色体。然而,在rad51δ二倍体细胞中,断裂染色体约有35%的时间得到修复。这些修复事件均不是简单的基因转换或伴有交换的基因转换,相反,它们产生了MAT位点以及DSB位点远端100 kb区域内所有标记均为纯合的二倍体细胞。在rad51δ二倍体细胞中,断裂染色体显然可以遗传几代,因为许多这样的修复事件表现为扇形菌落,一部分得到修复,另一部分丢失了断裂的染色体。类似事件在约2%的野生型细胞中也会发生。我们提出,在没有RAD51的情况下,断裂的染色体末端可以侵入同源模板并启动DNA复制,该复制可能延伸至100 kb或更远的端粒。这种断裂诱导的复制似乎类似于细菌中重组起始的复制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e2d1/38948/08cc6a44ab32/pnas01518-0297-a.jpg

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