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大肠杆菌中拓扑异构酶IV与DNA促旋酶的酶活性对比

Contrasting enzymatic activities of topoisomerase IV and DNA gyrase from Escherichia coli.

作者信息

Ullsperger C, Cozzarelli N R

机构信息

Department of Molecular and Cellular Biology, Division of Biochemistry and Molecular Biology, University of California, Berkeley, California 94720, USA.

出版信息

J Biol Chem. 1996 Dec 6;271(49):31549-55. doi: 10.1074/jbc.271.49.31549.

Abstract

DNA gyrase and topoisomerase IV (Topo IV) have distinct roles as unlinking enzymes during DNA replication despite 40% sequence identity between them. DNA gyrase unlinks replicating DNA by introducing negative supercoils while Topo IV decatenates the two daughter molecules. For this study, we measured the rates of unlinking of various topoisomers of DNA by DNA gyrase and Topo IV. Each enzyme has marked preferences for certain strand-passage reactions. DNA gyrase is a relatively poor decatenase, catalyzing strand-passage events that result in supercoiling at rates several orders of magnitude faster than those causing decatenation. Topo IV, in contrast, decatenates linked circles 10-40 times more quickly than it removes the intramolecular crossings from supercoiled DNA. Supercoiled catenanes are unlinked at an even more increased rate by Topo IV. Thus, the supercoils augment decatenation rather than compete with catenane crossings for their removal. Knot crossings and the crossings of multiply interlinked catenanes are also preferentially removed by Topo IV. This ability of Topo IV to selectively unlink catenated molecules mirrors its key role in decatenation of replicating chromosomes in vivo.

摘要

尽管DNA促旋酶和拓扑异构酶IV(Topo IV)之间有40%的序列一致性,但它们在DNA复制过程中作为解链酶具有不同的作用。DNA促旋酶通过引入负超螺旋来解开正在复制的DNA,而Topo IV则使两个子代分子解连环。在本研究中,我们测量了DNA促旋酶和Topo IV对各种拓扑异构体DNA的解链速率。每种酶对某些链通过反应都有明显的偏好。DNA促旋酶是一种相对较差的解连环酶,催化导致超螺旋的链通过事件的速率比导致解连环的速率快几个数量级。相比之下,Topo IV解连环状环的速度比从超螺旋DNA中去除分子内交叉点的速度快10到40倍。Topo IV以更高的速率解开超螺旋连环体。因此,超螺旋增强了解连环作用,而不是与连环体交叉竞争以将其去除。结交叉点和多重相互连接的连环体的交叉点也优先被Topo IV去除。Topo IV这种选择性解开连环分子的能力反映了其在体内复制染色体解连环中的关键作用。

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