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拓扑异构酶IV和DNA促旋酶在大肠杆菌复制过程中DNA解链中的作用。

Roles of topoisomerase IV and DNA gyrase in DNA unlinking during replication in Escherichia coli.

作者信息

Zechiedrich E L, Cozzarelli N R

机构信息

Department of Molecular and Cell Biology, University of California, Berkeley 94720-3204, USA.

出版信息

Genes Dev. 1995 Nov 15;9(22):2859-69. doi: 10.1101/gad.9.22.2859.

Abstract

For a cell to complete DNA replication, every link between the Watson-Crick strands must be removed by topoisomerases. Previously, we reported that the inhibition of topoisomerase IV (topo IV) leads to the accumulation of catenated plasmid replicons to a steady-state level of approximately 10%. Using pulse labeling with [3H]thymidine in Escherichia coli, we have found that in the absence of topo IV activity, nearly all newly synthesized plasmid DNA is catenated. Pulse-chase protocols revealed that catenanes are metabolized even in the absence of topo IV and that the residual turnover is carried out by DNA gyrase at a rate of approximately 0.01/sec. Using extremely short pulse-labeling times, we identified significant amounts of replication catenanes in wild-type cells. The rate of catenane unlinking in wild-type cells by the combined activities of topo IV and DNA gyrase was approximately 1/sec. Therefore, gyrase is 100-fold less efficient than topo IV in plasmid replicon decatenation in vivo. This may explain why a fully functional gyrase cannot prevent the catenation of newly synthesized plasmid DNA and the partition phenotype of topo IV mutants. We conclude that catenanes are kinetic intermediates in DNA replication and that the essential role of topo IV is to unlink daughter replicons.

摘要

为使细胞完成DNA复制,拓扑异构酶必须去除沃森-克里克链之间的每一个连接。此前,我们报道过抑制拓扑异构酶IV(topo IV)会导致连环质粒复制子积累至约10%的稳态水平。通过在大肠杆菌中用[3H]胸苷进行脉冲标记,我们发现,在缺乏topo IV活性的情况下,几乎所有新合成的质粒DNA都是连环的。脉冲追踪实验表明,即使在没有topo IV的情况下,连环体也会发生代谢,并且残余的周转由DNA促旋酶以约0.01/秒的速率进行。使用极短的脉冲标记时间,我们在野生型细胞中鉴定出了大量的复制连环体。在野生型细胞中,通过topo IV和DNA促旋酶的联合活性解开连环体的速率约为1/秒。因此,在体内质粒复制子解连环方面,促旋酶的效率比topo IV低100倍。这或许可以解释为什么功能完备的促旋酶无法阻止新合成的质粒DNA发生连环以及topo IV突变体的分配表型。我们得出结论,连环体是DNA复制过程中的动力学中间体,并且topo IV的重要作用是解开子代复制子。

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