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错配修复蛋白在酵母有丝分裂重组过程中调节异源双链体的形成。

Mismatch repair proteins regulate heteroduplex formation during mitotic recombination in yeast.

作者信息

Chen W, Jinks-Robertson S

机构信息

Graduate Program in Genetics and Molecular Biology and Department of Biology, Emory University, Atlanta, Georgia 30322, USA.

出版信息

Mol Cell Biol. 1998 Nov;18(11):6525-37. doi: 10.1128/MCB.18.11.6525.

DOI:10.1128/MCB.18.11.6525
PMID:9774668
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC109238/
Abstract

Mismatch repair (MMR) proteins actively inhibit recombination between diverged sequences in both prokaryotes and eukaryotes. Although the molecular basis of the antirecombination activity exerted by MMR proteins is unclear, it presumably involves the recognition of mismatches present in heteroduplex recombination intermediates. This recognition could be exerted during the initial stage of strand exchange, during the extension of heteroduplex DNA, or during the resolution of recombination intermediates. We previously used an assay system based on 350-bp inverted-repeat substrates to demonstrate that MMR proteins strongly inhibit mitotic recombination between diverged sequences in Saccharomyces cerevisiae. The assay system detects only those events that reverse the orientation of the region between the recombination substrates, which can occur as a result of either intrachromatid crossover or sister chromatid conversion. In the present study we sequenced the products of mitotic recombination between 94%-identical substrates in order to map gene conversion tracts in wild-type versus MMR-defective yeast strains. The sequence data indicate that (i) most recombination occurs via sister chromatid conversion and (ii) gene conversion tracts in an MMR-defective strain are significantly longer than those in an isogenic wild-type strain. The shortening of conversion tracts observed in a wild-type strain relative to an MMR-defective strain suggests that at least part of the antirecombination activity of MMR proteins derives from the blockage of heteroduplex extension in the presence of mismatches.

摘要

错配修复(MMR)蛋白可有效抑制原核生物和真核生物中不同序列之间的重组。尽管MMR蛋白发挥抗重组活性的分子基础尚不清楚,但推测这可能涉及对异源双链重组中间体中存在的错配的识别。这种识别可能发生在链交换的初始阶段、异源双链DNA的延伸过程中或重组中间体的拆分过程中。我们之前使用基于350 bp反向重复底物的检测系统,证明了MMR蛋白可强烈抑制酿酒酵母中不同序列之间的有丝分裂重组。该检测系统仅检测那些逆转重组底物之间区域方向的事件,这些事件可能是由于染色单体内交叉或姐妹染色单体转换导致的。在本研究中,我们对94%相同底物之间的有丝分裂重组产物进行了测序,以便绘制野生型与MMR缺陷型酵母菌株中的基因转换片段。序列数据表明:(i)大多数重组通过姐妹染色单体转换发生;(ii)MMR缺陷型菌株中的基因转换片段明显长于同基因野生型菌株中的片段。与MMR缺陷型菌株相比,在野生型菌株中观察到的转换片段缩短表明,MMR蛋白的抗重组活性至少部分源于在存在错配的情况下对异源双链延伸的阻断。

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本文引用的文献

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Mitotic intragenic recombination in the yeast Saccharomyces: marker-effects on conversion and reciprocity of recombination.酵母属中染色体内有丝分裂基因重组:转化和重组互逆的标记效应。
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Enhancement of MSH2-MSH3-mediated mismatch recognition by the yeast MLH1-PMS1 complex.酵母MLH1-PMS1复合物增强MSH2-MSH3介导的错配识别。
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Role of Saccharomyces cerevisiae Msh2 and Msh3 repair proteins in double-strand break-induced recombination.酿酒酵母Msh2和Msh3修复蛋白在双链断裂诱导的重组中的作用。
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