首页> 外文期刊>Proceedings of the National Academy of Sciences of the United States of America >RecQ helicase translocates along single-stranded DNA with a moderate processivity and tight mechanochemical coupling
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RecQ helicase translocates along single-stranded DNA with a moderate processivity and tight mechanochemical coupling

机译:RecQ解旋酶以适度的持续性和紧密的机械化学偶联沿着单链DNA转运

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摘要

Maintenance of genome integrity is the major biological role of RecQ-family helicases via their participation in homologous recombination (HR)-mediated DNA repair processes. RecQ helicases exert their functions by using the free energy of ATP hydrolysis for mechanical movement along DNA tracks (translocation). In addition to the importance of translocation per se in recombination processes, knowledge of its mechanism is necessary for the understanding of more complex translocation-based activities, including nucleoprotein displacement, strand separation (unwinding), and branch migration. Here, we report the key properties of the ssDNA translocation mechanism of Escherichia coli RecQ helicase, the prototype of the RecQ family. We monitored the pre-steady-state kinetics of ATP hydrolysis by RecQ and the dissociation of the enzyme from ssDNA during single-round translocation. We also gained information on the translocation mechanism from the ssDNA length dependence of the steady-state ssDNA-activated ATPase activity. We show that RecQ occludes 18 ± 2 nt on ssDNA during translocation. The hydrolysis of ATP is noncooperative in the presence of ssDNA, indicating that RecQ active sites work independently during translocation, In the applied conditions, the enzyme hydrolyzes 35 ± 4 ATP molecules per second during ssDNA translocation. RecQ translocates at a moderate processivity, with a mean run length of 100-320 nt on ssDNA. The determined tight mechanochemical coupling of 1-1±0.2 ATP consumed per nude-otide traveled indicates an inchworm-type mechanism.
机译:通过参与同源重组(HR)介导的DNA修复过程,基因组完整性的维持是RecQ家族解旋酶的主要生物学作用。 RecQ解旋酶通过利用ATP水解的自由能沿DNA轨道机械运动(易位)来发挥其功能。除了本身在重组过程中的重要性外,了解其机制对于了解更复杂的基于移位的活性(包括核蛋白置换,链分离(展开)和分支迁移)也是必要的。在这里,我们报告了RecQ家族原型Escherichia coli RecQ解旋酶的ssDNA易位机制的关键特性。我们监测了RecQ水解ATP的前稳态动力学以及在单轮易位过程中酶从ssDNA的解离。我们还从稳态ssDNA激活的ATPase活性的ssDNA长度依赖性中获得了有关转运机制的信息。我们显示,RecQ在移位过程中在ssDNA上闭塞了18±2 nt。在ssDNA存在下ATP的水解是不合作的,这表明RecQ活性位点在转运过程中独立发挥作用。在应用条件下,该酶在ssDNA转运过程中每秒水解35±4 ATP分子。 RecQ以适度的持续性易位,在ssDNA上的平均游程长度为100-320 nt。所确定的每行裸核苷酸消耗的1-1±0.2 ATP的紧密机械化学偶联表明了尺worm型机制。

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    Department of Biochemistry, Eoetvoes Lorand University - Hungarian Academy of Sciences, "Momentum" Motor Enzymology Research Group, Eoetvoes Lorand University, H-1117, Budapest, Hungary;

    Department of Biochemistry, Eoetvoes Lorand University - Hungarian Academy of Sciences, "Momentum" Motor Enzymology Research Group, Eoetvoes Lorand University, H-1117, Budapest, Hungary;

    Department of Biochemistry, Eoetvoes Lorand University - Hungarian Academy of Sciences, "Momentum" Motor Enzymology Research Group, Eoetvoes Lorand University, H-1117, Budapest, Hungary;

  • 收录信息 美国《科学引文索引》(SCI);美国《生物学医学文摘》(MEDLINE);美国《化学文摘》(CA);
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  • 正文语种 eng
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  • 入库时间 2022-08-18 00:40:26

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