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DNA cleavage and opening reactions of human topoisomerase IIα are regulated via Mg2+-mediated dynamic bending of gate-DNA

机译:人类拓扑异构酶IIα的DNA裂解和打开反应通过Mg2 +介导的Gate-DNA的动态弯曲来调控

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摘要

Topoisomerase II resolves intrinsic topological problems of double-stranded DNA. As part of its essential cellular functions, the enzyme generates DNA breaks, but the regulation of this potentially dangerous process is not well understood. Here we report single-molecule fluorescence experiments that reveal a previously uncharacterized sequence of events during DNA cleavage by topoisomerase II: nonspecific DNA binding, sequence-specific DNA bending, and stochastic cleavage of DNA. We have identified unexpected structural roles of Mg2+ ions coordinated in the TOPRIM (topoisomerase-primase) domain in inducing cleavage-competent DNA bending. A break at one scissile bond dramatically stabilized DNA bending, explaining how two scission events in opposing strands can be coordinated to achieve a high probability of double-stranded cleavage. Clamping of the protein N-gate greatly enhanced the rate and degree of DNA bending, resulting in a significant stimulation of the DNA cleavage and opening reactions. Our data strongly suggest that the accurate cleavage of DNA by topoisomerase II is regulated through a tight coordination with DNA bending.
机译:拓扑异构酶II解决了双链DNA固有的拓扑问题。作为其基本细胞功能的一部分,该酶会产生DNA断裂,但对该潜在危险过程的调节尚不甚了解。在这里,我们报告单分子荧光实验,揭示了拓扑异构酶II在DNA切割过程中以前未知的事件序列:非特异性DNA结合,序列特异性DNA弯曲和DNA的随机切割。我们已经确定了TOPRIM(拓扑异构酶-引发酶)域中协调的Mg2 +离子在诱导裂解型DNA弯曲中具有意想不到的结构作用。一个易断裂键的断裂极大地稳定了DNA弯曲,这解释了如何协调相对链中的两个断裂事件以实现高概率的双链裂解。蛋白质N门的夹紧大大提高了DNA弯曲的速率和程度,从而显着刺激了DNA裂解和打开反应。我们的数据强烈表明,拓扑异构酶II对DNA的精确切割是通过与DNA弯曲的紧密配合来调节的。

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