首页> 外文期刊>Molecular Microbiology >Dissection of a functional interaction between the DNA translocase, FtsK, and the XerD recombinase.
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Dissection of a functional interaction between the DNA translocase, FtsK, and the XerD recombinase.

机译:解剖了DNA转位酶,F​​tsK和XerD重组酶之间的功能相互作用。

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摘要

Successful bacterial circular chromosome segregation requires that any dimeric chromosomes, which arise by crossing over during homologous recombination, are converted to monomers. Resolution of dimers to monomers requires the action of the XerCD site-specific recombinase at dif in the chromosome replication terminus region. This reaction requires the DNA translocase, FtsK(C), which activates dimer resolution by catalysing an ATP hydrolysis-dependent switch in the catalytic state of the nucleoprotein recombination complex. We show that a 62-amino-acid fragment of FtsK(C) interacts directly with the XerD C-terminus in order to stimulate the cleavage by XerD of BSN, a dif-DNA suicide substrate containing a nick in the 'bottom' strand. The resulting recombinase-DNA covalent complex can undergo strand exchange with intact duplex dif in the absence of ATP. FtsK(C)-mediated stimulation of BSN cleavage by XerD requires synaptic complex formation. Mutational impairment of the XerD-FtsK(C) interaction leads to reduction in the in vitro stimulation of BSN cleavage by XerD and a concomitant deficiency in the resolution of chromosomal dimers at dif in vivo, although other XerD functions are not affected.
机译:成功的细菌圆染色体分离要求将在同源重组过程中交叉产生的任何二聚体染色体转化为单体。将二聚体分解为单体需要XerCD位点特异性重组酶在染色体复制末端区域的dif处起作用。此反应需要DNA转位酶FtsK(C),该酶通过在核蛋白重组复合体的催化状态下催化ATP水解依赖性开关来激活二聚体分辨率。我们显示FtsK(C)的62个氨基酸的片段直接与XerD C末端相互作用,以刺激BSN的XerD裂解,Dif-DNA自杀底物在“底部”链中含有缺口。在不存在ATP的情况下,所得的重组酶-DNA共价复合物可与完整的双链体dif进行链交换。由XerD的FtsK(C)介导的BSN切割刺激需要突触复合物形成。 XerD-FtsK(C)相互作用的突变损伤导致XerD对BSN裂解的体外刺激减少,并伴随着体内dif染色体二聚体分辨率的降低,尽管其他XerD功能并未受到影响。

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