首页> 外文期刊>Nucleic Acids Research >Interaction of the resolving enzyme YDC2 with the four-way DNA junction.
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Interaction of the resolving enzyme YDC2 with the four-way DNA junction.

机译:解析酶YDC2与四向DNA连接的相互作用。

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Holliday junctions (four-way DNA junctions), formed during homologous recombination, are bound and resolved by junction-specific endonucleases to yield recombinant duplex DNA products. The junction-resolving enzymes are a structurally diverse class of proteins that nevertheless have many properties in common; in particular a high structure specificity for binding and metal-dependent, (frequently) sequence-specific cleavage activity. In Saccharomyces cerevisiae, the enzyme CCE1 is necessary for the resolution of recombining mitochondrial genomes, and in Schizosaccharomyces pombe the homologous protein YDC2 is thought to have a similar function. We have generated an inactive mutant of YDC2, D226N, that retains structure-specific junction binding and have analysed the interaction of this protein with the four-way DNA junction. YDC2 binds the four-way junction in two specific complexes (I and II), unfolding the stacked X-structure into a conformation where the arms extend to the four corners of a square. This structure is reminiscent of that of the free junction in the absence of metal ions and of the structures imposed on the Holliday junction by CCE1 and RuvA. DNase I probing reveals footprints specific for complexes I and II which extend from the junction centre on all four arms. No protection is observed with the small, hydrophobic probe DMS.
机译:在同源重组过程中形成的霍利迪接头(四向DNA接头)通过接头特异性核酸内切酶结合并分解,从而产生重组双链DNA产物。连接解析酶是结构上多样化的一类蛋白质,但是它们具有许多共同的特性。特别是对于结合和金属依赖性的(经常)序列特异性的切割活性具有高的结构特异性。在酿酒酵母中,酶CCE1对于线粒体基因组重组的解析是必需的,在粟酒裂殖酵母中,同源蛋白YDC2被认为具有类似的功能。我们已经生成了YDC2的无活性突变体D226N,该突变体保留了结构特异性的连接结合,并分析了该蛋白质与四向DNA连接的相互作用。 YDC2在两个特定的复合体(I和II)中结合四向连接,将堆叠的X结构展开为构型,其中臂延伸到正方形的四个角。这种结构让人联想到在不存在金属离子的情况下的自由结以及CCE1和RuvA施加在霍利迪结上的结构。 DNase I的探测揭示了复合物I和II特有的足迹,复合物I和II从所有四个臂的交界处开始延伸。较小的疏水探针DMS未观察到保护作用。

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