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玉米黑粉菌Brh2蛋白形成D环。

D-loop formation by Brh2 protein of Ustilago maydis.

作者信息

Mazloum Nayef, Zhou Qingwen, Holloman William K

机构信息

Department of Microbiology and Immunology, Cornell University Weill Medical College, New York, NY 10065, USA.

出版信息

Proc Natl Acad Sci U S A. 2008 Jan 15;105(2):524-9. doi: 10.1073/pnas.0707031105. Epub 2008 Jan 3.

Abstract

Brh2, the ortholog of the BRCA2 tumor suppressor in Ustilago maydis, works hand in hand with Rad51 to promote repair of DNA by homologous recombination. Previous studies established that Brh2 can stimulate DNA strand exchange by enabling Rad51 nucleoprotein filament formation on replication protein A-coated ssDNA. But, more recently, it was noted that Brh2 has an inherent DNA annealing activity, raising the notion that it might have roles in recombination in addition to or beyond the mediator function. Here, we found that Brh2 can autonomously promote the formation of D-loops in reactions with plasmid DNA and homologous single-stranded oligonucleotides. The reaction differs from that catalyzed by Rad51 in having no requirement for cofactors or preloading phase on ssDNA. D-loop formation was most effective when Brh2 was mixed with plasmid DNA before addition of single-stranded oligomer. D-loop formation catalyzed by Rad51 was also enhanced when Brh2 was premixed with plasmid DNA. Brh2 rendered defective in Rad51 interaction by mutation in the BRC element was still capable of promoting D-loop formation. However, the mutant protein was unable to enhance the Rad51-catalyzed reaction. The results suggest a model in which Brh2 binding to plasmid DNA attracts and helps capture Rad51-coated ssDNA.

摘要

Brh2是玉米黑粉菌中BRCA2肿瘤抑制因子的直系同源物,它与Rad51协同作用,通过同源重组促进DNA修复。先前的研究表明,Brh2可通过使Rad51在复制蛋白A包被的单链DNA上形成核蛋白丝来刺激DNA链交换。但是,最近有研究指出,Brh2具有内在的DNA退火活性,这引发了一种观点,即它可能在重组中除了介导功能之外或超越介导功能还发挥作用。在这里,我们发现Brh2在与质粒DNA和同源单链寡核苷酸的反应中能够自主促进D环的形成。该反应与Rad51催化的反应不同,它不需要辅助因子,也不需要在单链DNA上进行预加载阶段。当在添加单链寡聚物之前将Brh2与质粒DNA混合时,D环形成最为有效。当Brh2与质粒DNA预混合时,Rad51催化的D环形成也会增强。通过BRC元件突变而导致与Rad51相互作用缺陷的Brh2仍然能够促进D环的形成。然而,突变蛋白无法增强Rad51催化的反应。结果提示了一种模型,即Brh2与质粒DNA的结合会吸引并帮助捕获Rad51包被的单链DNA。

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