首页> 外文期刊>Nucleic Acids Research >RecG helicase activity at three- and four-strand DNA structures.
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RecG helicase activity at three- and four-strand DNA structures.

机译:RecG解旋酶在三链和四链DNA结构上的活性。

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The RecG helicase of Escherichia coli is necessary for efficient recombination and repair of DNA in vivo and has been shown to catalyse the unwinding of DNA junctions in vitro. Despite these findings, the precise role of RecG remains elusive. However, models have been proposed in which RecG promotes the resolution of linked duplexes by targeting three-strand junctions present at D-loops. One such model postulates that RecG catalyses the formation of four-strand (Holliday) junctions from three-strand junctions. To test this model, the DNA binding and unwinding activities of RecG were analysed using synthetic three- and four-strand junctions. The substrate specificity of RecG was found to depend critically on the concentrations of ATP and MgCl(2)and under certain conditions RecG preferentially unwound three-strand junction DNA. This was at least partly due to the larger inhibitory effect of MgCl(2)on the binding of four-strand as opposed to three-strand junctions by RecG. Thus RecG may be targeted to three-strand junctions in vivo whilst still being able to branch migrate the four-strand junctions formed as a result of the initial helicase reaction. The increase in the dissociation constant of RecG on conversion of a three-strand into a four-strand junction may also facilitate resolution of the four-strand junction by the RuvABC complex.
机译:大肠杆菌的RecG解旋酶是体内有效重组和修复DNA所必需的,并已显示出其在体外催化DNA连接解旋的作用。尽管有这些发现,RecG的确切作用仍然难以捉摸。但是,已经提出了模型,其中RecG通过靶向D环处的三链结来提高连接的双链体的分辨率。一种这样的模型假定RecG催化三链结形成四链(霍利迪)结。为了测试该模型,使用合成的三链和四链接头分析了RecG的DNA结合和解链活性。发现RecG的底物特异性主要取决于ATP和MgCl(2)的浓度,在某些条件下RecG优先解绕三链结DNA。这至少部分是由于MgCl(2)对四链结合的较大抑制作用,而与RecG的三链结合相反。因此,RecG可以靶向体内的三链连接,同时仍然能够分支迁移由于初始解旋酶反应而形成的四链连接。将三链转换为四链结时,RecG的解离常数增加,也可能有助于RuvABC复合物拆分四链结。

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