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黑腹果蝇中的mei-W68编码一种Spo11同源物:启动减数分裂重组的机制具有保守性的证据。

mei-W68 in Drosophila melanogaster encodes a Spo11 homolog: evidence that the mechanism for initiating meiotic recombination is conserved.

作者信息

McKim K S, Hayashi-Hagihara A

机构信息

Waksman Institute, Rutgers University, Piscataway, New Jersey 08854-8020, USA.

出版信息

Genes Dev. 1998 Sep 15;12(18):2932-42. doi: 10.1101/gad.12.18.2932.

Abstract

Meiotic recombination requires the action of several gene products in both Saccharomyces cerevisiae and Drosophila melanogaster. Genetic studies in D. melanogaster have shown that the mei-W68 gene is required for all meiotic gene conversion and crossing-over. We cloned mei-W68 using a new genetic mapping method in which P elements are used to promote crossing-over at their insertion sites. This resulted in the high-resolution mapping of mei-W68 to a <18-kb region that contains a homolog of the S. cerevisiae spo11 gene. Molecular analysis of several mutants confirmed that mei-W68 encodes an spo11 homolog. Spo11 and MEI-W68 are members of a family of proteins similar to a novel type II topoisomerase. On the basis of this and other lines of evidence, Spo11 has been proposed to be the enzymatic activity that creates the double-strand breaks needed to initiate meiotic recombination. This raises the possibility that recombination in Drosophila is also initiated by double-strand breaks. Although these homologous genes are required absolutely for recombination in both species, their roles differ in other respects. In contrast to spo11, mei-W68 is not required for synaptonemal complex formation and does have a mitotic role.

摘要

在酿酒酵母和黑腹果蝇中,减数分裂重组需要几种基因产物的作用。黑腹果蝇的遗传学研究表明,mei-W68基因是所有减数分裂基因转换和交叉互换所必需的。我们使用一种新的遗传定位方法克隆了mei-W68,该方法利用P因子在其插入位点促进交叉互换。这导致将mei-W68高分辨率定位到一个小于18 kb的区域,该区域包含酿酒酵母spo11基因的一个同源物。对几个突变体的分子分析证实,mei-W68编码一个spo11同源物。Spo11和MEI-W68是类似于新型II型拓扑异构酶的蛋白质家族成员。基于这一证据及其他证据,有人提出Spo11是产生启动减数分裂重组所需双链断裂的酶活性。这增加了果蝇中的重组也由双链断裂启动的可能性。尽管这两个同源基因在两个物种的重组中都是绝对必需的,但它们在其他方面的作用有所不同。与spo11不同,mei-W68不是联会复合体形成所必需的,并且确实具有有丝分裂作用。

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