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Concerted action at eight phosphodiester bonds by the BcgI restriction endonuclease

机译:BcgI限制性核酸内切酶对八个磷酸二酯键的协同作用

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The BcgI endonuclease exemplifies a subset of restriction enzymes, the Type IIB class, which make two double-strand breaks (DSBs) at each copy of their recognition sequence, one either side of the site, to excise the sequence from the remainder of the DNA. In this study, we show that BcgI is essentially inactive when bound to a single site and that to cleave a DNA with one copy of its recognition sequence, it has to act in trans, bridging two separate DNA molecules. We also show that BcgI makes the two DSBs at an individual site in a highly concerted manner. Intermediates cut on one side of the site do not accumulate during the course of the reaction: instead, the DNA is converted straight to the final products cut on both sides. On DNA with two sites, BcgI bridges the sites in cis and then generally proceeds to cut both strands on both sides of both sites without leaving the DNA. The BcgI restriction enzyme can thus excise two DNA segments together, by cleaving eight phosphodiester bonds within a single-DNA binding event.
机译:BcgI核酸内切酶是限制性酶IIB类的一个子集,该酶在其识别序列的每个拷贝处(该位点的任一侧)产生两个双链断裂(DSB),以从DNA的其余部分中切除该序列。 。在这项研究中,我们表明BcgI当结合到单个位点时基本上是无活性的,并且要用其识别序列的一个拷贝切割DNA,它必须以反式作用,桥接两个独立的DNA分子。我们还显示,BcgI以高度协调的方式在单个站点上制作了两个DSB。在反应过程中,在位点一侧切割的中间体不会积聚:而是将DNA直接转化为在两侧切割的最终产物。在具有两个位点的DNA上,BcgI将顺式位点桥接,然后通常在不离开DNA的情况下在两个位点的两侧切割两条链。因此,BcgI限制酶可以通过在单个DNA结合事件中切割八个磷酸二酯键将两个DNA片段一起切除。

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