Aboussekhra A, Chanet R, Adjiri A, Fabre F
Section de Biologie, Instiut Curie, Centre Universitaire, Orsay, France.
Mol Cell Biol. 1992 Jul;12(7):3224-34. doi: 10.1128/mcb.12.7.3224-3234.1992.
Eleven suppressors of the radiation sensitivity of Saccharomyces cerevisiae diploids lacking the Srs2 helicase were analyzed and found to contain codominant mutations in the RAD51 gene known to be involved in recombinational repair and in genetic recombination. These mutant alleles confer an almost complete block in recombinational repair, as does deletion of RAD51, but heterozygous mutant alleles suppress the defects of srs2::LEU2 cells and are semidominant in Srs2+ cells. The results of this study are interpreted to mean that wild-type Rad51 protein binds to single-stranded DNA and that the semidominant mutations do not prevent this binding. The cloning and sequencing of RAD51 indicated that the gene encodes a predicted 400-amino-acid protein with a molecular mass of 43 kDa. Sequence comparisons revealed homologies to domains of Escherichia coli RecA protein predicted to be involved in DNA binding, ATP binding, and ATP hydrolysis. The expression of RAD51, measured with a RAD51-lacZ gene fusion, was found to be UV- and gamma-ray-inducible, with dose-dependent responses.
对11个酿酒酵母二倍体辐射敏感性的抑制子进行了分析,这些二倍体缺乏Srs2解旋酶,结果发现它们在RAD51基因中含有共显性突变,已知该基因参与重组修复和基因重组。这些突变等位基因在重组修复中几乎造成了完全阻断,就像RAD51缺失一样,但杂合突变等位基因抑制了srs2::LEU2细胞的缺陷,并且在Srs2+细胞中呈半显性。本研究结果被解释为意味着野生型Rad51蛋白与单链DNA结合,并且半显性突变不会阻止这种结合。RAD51的克隆和测序表明,该基因编码一种预测的400个氨基酸的蛋白质,分子量为43 kDa。序列比较揭示了与大肠杆菌RecA蛋白预测参与DNA结合、ATP结合和ATP水解的结构域的同源性。用RAD51 - lacZ基因融合体测量发现,RAD51的表达可被紫外线和γ射线诱导,具有剂量依赖性反应。