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Counting Rad51 Proteins Disassembling From Nucleoprotein Filaments Under Tension

机译:计数从张力下从核蛋白丝分解的Rad51蛋白

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The central catalyst in eukaryotic ATP-dependent homologous recombination consists of RAD51 proteins, polymerized around single-stranded DNA. This nucleoprotein filament recognizes and invades a homologous duplex DNA segment. After strand exchange, the nucleoprotein filament should disassemble so that the recombination process can be completed. The molecular mechanism of RAD51 filament disassembly is poorly understood. Here we show, by combining optical tweezers with single-molecule fluorescence microscopy and microfluidics, that disassembly of human RAD51 nucleoprotein filaments results from the interplay between ATP hydrolysis and the release of the tension stored in the filament. By applying external tension to the DNA, we found that disassembly slows down and can even be stalled. We quantified the fluorescence of RAD51 patches and found that disassembly occurs in bursts interspersed by long pauses. After relaxation of a stalled complex, pauses were suppressed resulting in a large burst. These results indicate that tension-dependent disassembly takes place only from filament ends, after tension-independent ATP hydrolysis. This integrative single-molecule approach allowed us to dissect the mechanism of this principal homologous recombination reaction step, which in turn clarifies how disassembly can be influenced by accessory proteins.
机译:真核ATP依赖的同源重组中的中心催化剂由RAD51蛋白组成,其围绕单链DNA聚合。该核蛋白丝识别并侵入同源双链DNA片段。链交换后,核蛋白细丝应分解,以便完成重组过程。 RAD51灯丝拆卸的分子机理了解甚少。在这里,我们显示,通过将光镊与单分子荧光显微镜和微流控技术相结合,人类RAD51核蛋白细丝的拆卸是由于ATP水解和细丝中存储的张力释放之间的相互作用而导致的。通过对DNA施加外部张力,我们发现拆卸速度减慢,甚至可能停止。我们对RAD51贴片的荧光进行了定量,发现在长暂停之间散布的突发中发生了拆卸。停顿的复合体放松之后,停顿被抑制,从而导致大量爆发。这些结果表明,在不依赖于张力的ATP水解之后,仅在细丝末端发生了依赖于张力的拆卸。这种整合的单分子方法使我们能够剖析该主要同源重组反应步骤的机制,从而阐明了辅助蛋白如何影响拆卸。

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