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DNA looping by FokI: the impact of twisting and bending rigidity on protein-induced looping dynamics

机译:FokI进行DNA环化:扭曲和弯曲刚度对蛋白质诱导的环化动力学的影响

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摘要

Protein-induced DNA looping is crucial for many genetic processes such as transcription, gene regulation and DNA replication. Here, we use tethered-particle motion to examine the impact of DNA bending and twisting rigidity on loop capture and release, using the restriction endonuclease FokI as a test system. To cleave DNA efficiently, FokI bridges two copies of an asymmetric sequence, invariably aligning the sites in parallel. On account of the fixed alignment, the topology of the DNA loop is set by the orientation of the sites along the DNA. We show that both the separation of the FokI sites and their orientation, altering, respectively, the twisting and the bending of the DNA needed to juxtapose the sites, have profound effects on the dynamics of the looping interaction. Surprisingly, the presence of a nick within the loop does not affect the observed rigidity of the DNA. In contrast, the introduction of a 4-nt gap fully relaxes all of the torque present in the system but does not necessarily enhance loop stability. FokI therefore employs torque to stabilise its DNA-looping interaction by acting as a 'torsional' catch bond.
机译:蛋白质诱导的DNA循环对于许多遗传过程(例如转录,基因调控和DNA复制)至关重要。在这里,我们使用限制核酸内切酶FokI作为测试系统,使用束缚粒子运动来检查DNA弯曲和扭曲刚度对环捕获和释放的影响。为了有效地切割DNA,FokI桥接了两个不对称序列的拷贝,始终将这些位点平行排列。由于固定比对,通过沿着DNA的位点的方向来设置DNA环的拓扑。我们表明,FokI位点的分离及其方向,分别改变并置位点所需的DNA的扭曲和弯曲,都对环相互作用的动力学产生了深远的影响。出人意料的是,环内切口的存在不影响所观察到的DNA的刚度。相比之下,引入4 nt的间隙将完全缓解系统中存在的所有扭矩,但不一定会增强回路稳定性。因此,FokI使用扭矩通过充当“扭转”捕获键来稳定其DNA环相互作用。

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