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DNA-tension dependence of restriction enzyme activity reveals mechanochemical properties of the reaction pathway

机译:限制酶活性的DNA张力依赖性揭示了反应途径的机械化学性质

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Type II restriction endonucleases protect bacteria against phage infections by cleaving recognition sites on foreign double-stranded DNA (dsDNA) with extraordinary specificity. This capability arises primarily from large conformational changes in enzyme and/or DNA upon target sequence recognition. In order to elucidate the connection between the mechanics and the chemistry of DNA recognition and cleavage, we used a single-molecule approach to measure rate changes in the reaction pathway of EcoRV and BamHI as a function of DNA tension. We show that the induced-fit rate of EcoRV is strongly reduced by such tension. In contrast, BamHI is found to be insensitive, providing evidence that both substrate binding and hydrolysis are not influenced by this force. Based on these results, we propose a mechanochemical model of induced-fit reactions on DNA, allowing determination of induced-fit rates and DNA bend angles. Finally, for both enzymes a strongly decreased association rate is obtained on stretched DNA, presumably due to the absence of intradomain dissociation/re-association between non-specific sites (jumping). The obtained results should apply to many other DNA-associated proteins.
机译:II型限制性核酸内切酶通过以非凡的特异性切割外来双链DNA(dsDNA)上的识别位点来保护细菌免受噬菌体感染。这种能力主要来自靶序列识别后酶和/或DNA的构象变化较大。为了阐明DNA识别和裂解的机理与化学之间的联系,我们使用了单分子方法来测量EcoRV和BamHI的反应路径中速率随DNA张力的变化。我们表明,这种张力极大地降低了EcoRV的诱导拟合率。相反,发现BamHI不敏感,这提供了底物结合和水解均不受此力影响的证据。基于这些结果,我们提出了对DNA进行诱导拟合反应的机械化学模型,从而可以确定诱导拟合速率和DNA弯曲角度。最后,对于这两种酶,在拉伸的DNA上获得的结合率大大降低,这大概是由于非特异性位点之间没有域内解离/再结合(跳跃)。所得结果应适用于许多其他与DNA相关的蛋白质。

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