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酿酒酵母中RAD52表达调控对修复和重组的影响。

Effects of controlled RAD52 expression on repair and recombination in Saccharomyces cerevisiae.

作者信息

Dornfeld K J, Livingston D M

机构信息

Department of Biochemistry, University of Minnesota, Minneapolis 55455.

出版信息

Mol Cell Biol. 1991 Apr;11(4):2013-7. doi: 10.1128/mcb.11.4.2013-2017.1991.

Abstract

We have examined the effects of RAD52 overexpression on methyl methanesulfonate (MMS) sensitivity and spontaneous mitotic recombination rates. Cells expressing a 10-fold excess of RAD52 mRNA from the ENO1 promoter are no more resistant to MMS than are wild-type cells. Similarly, under the same conditions, the rate of mitotic recombination within a reporter plasmid does not exceed that measured in wild-type cells. This high level of expression is capable of correcting the defects of rad52 mutant cells in carrying out repair and recombination. From these observations, we conclude that wild-type amounts of Rad52 are not rate limiting for repair of MMS-induced lesions or plasmid recombination. By placing RAD52 under the control of the inducible GAL1 promoter, we find that induction results in a 12-fold increase in the fraction of recombinants within 4 h. After this time, the fraction increases less rapidly. When RAD52 expression is quickly repressed during induction, the amount of RAD52 mRNA decreases rapidly and no nascent recombinants are formed. This result suggests a short active half-life for the protein product. Induction of RAD52 in G1-arrested mutant cells also causes a rapid increase in recombinants, suggesting that replication is not necessary for plasmid recombination.

摘要

我们研究了RAD52过表达对甲磺酸甲酯(MMS)敏感性和自发有丝分裂重组率的影响。从ENO1启动子表达过量10倍RAD52 mRNA的细胞对MMS的抗性并不比野生型细胞更强。同样,在相同条件下,报告质粒内的有丝分裂重组率不超过在野生型细胞中测得的水平。这种高水平的表达能够纠正rad52突变细胞在进行修复和重组方面的缺陷。从这些观察结果中,我们得出结论,野生型数量的Rad52对于MMS诱导损伤的修复或质粒重组不是限速因素。通过将RAD52置于可诱导的GAL1启动子控制下,我们发现诱导在4小时内导致重组体比例增加12倍。在此之后,比例增加得较慢。当在诱导过程中迅速抑制RAD52表达时,RAD52 mRNA的量迅速减少,并且没有形成新生的重组体。这一结果表明该蛋白质产物的活性半衰期较短。在G1期停滞的突变细胞中诱导RAD52也会导致重组体迅速增加,这表明质粒重组不需要复制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3e29/359887/5ca2c3e53480/molcellb00138-0250-a.jpg

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