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RecBC DNA解旋酶的易位步长及机制

Translocation step size and mechanism of the RecBC DNA helicase.

作者信息

Bianco P R, Kowalczykowski S C

机构信息

Section of Microbiology, University of California at Davis, 95616, USA.

出版信息

Nature. 2000 May 18;405(6784):368-72. doi: 10.1038/35012652.

Abstract

DNA helicases are ubiquitous enzymes that unwind double-stranded DNA. They are a diverse group of proteins that move in a linear fashion along a one-dimensional polymer lattice--DNA--by using a mechanism that couples nucleoside triphosphate hydrolysis to both translocation and double-stranded DNA unwinding to produce separate strands of DNA. The RecBC enzyme is a processive DNA helicase that functions in homologous recombination in Escherichia coli; it unwinds up to 6,250 base pairs per binding event and hydrolyses slightly more than one ATP molecule per base pair unwound. Here we show, by using a series of gapped oligonucleotide substrates, that this enzyme translocates along only one strand of duplex DNA in the 3'-->5' direction. The translocating enzyme will traverse, or 'step' across, single-stranded DNA gaps in defined steps that are 23 (+/-2) nucleotides in length. This step is much larger than the amount of double-stranded DNA that can be unwound using the free energy derived from hydrolysis of one molecule of ATP, implying that translocation and DNA unwinding are separate events. We propose that the RecBC enzyme both translocates and unwinds by a quantized, two-step, inchworm-like mechanism that may have parallels for translocation by other linear motor proteins.

摘要

DNA解旋酶是一类能解开双链DNA的普遍存在的酶。它们是一组多样的蛋白质,通过一种将核苷三磷酸水解与易位和双链DNA解旋相偶联的机制,沿着一维聚合物晶格——DNA——以线性方式移动,从而产生单链DNA。RecBC酶是一种持续性DNA解旋酶,在大肠杆菌的同源重组中发挥作用;它每次结合事件能解开多达6250个碱基对,每解开一个碱基对水解略多于一个ATP分子。在这里,我们通过使用一系列有缺口的寡核苷酸底物表明,这种酶仅沿着双链DNA的一条链在3'→5'方向上易位。易位的酶会以确定的步长穿过或“跨越”单链DNA缺口,步长为23(±2)个核苷酸。这个步长比利用一分子ATP水解产生的自由能所能解开的双链DNA量要大得多,这意味着易位和解旋是两个独立的事件。我们提出,RecBC酶通过一种量化的、两步的、类似尺蠖的机制进行易位和解旋,这种机制可能与其他线性运动蛋白的易位有相似之处。

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