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大肠杆菌噬菌体λ DNA 复制起点的转录激活受宿主 DnaA 起始功能调控。

Transcriptional activation of the origin of coliphage lambda DNA replication is regulated by the host DnaA initiator function.

作者信息

Wegrzyn G, Szalewska-Pałasz A, Wegrzyn A, Obuchowski M, Taylor K

机构信息

Department of Molecular Biology, University of Gdańsk, Poland.

出版信息

Gene. 1995 Feb 27;154(1):47-50. doi: 10.1016/0378-1119(94)00849-n.

Abstract

The initiator of phage lambda DNA replication, the lambda O protein, is considered to be an analogue of the initiator of DNA replication (DnaA) of its host, Escherichia coli. Both specifically recognize their origins of replication, ori lambda and oriC, respectively, and organize the assembly of specific replication complexes. However, DnaA has an additional activation function, acting on oriC-proximal DnaA-boxes, and regulating transcription initiated at promoters in and around oriC. Here, we demonstrate that lambda plasmid replication can be synchronized by a temperature shift-down that caused renaturation of the previously denatured DnaAts protein. Moreover, we show that elimination of the activating DnaA function affects transcriptional activation at ori lambda. DnaA may act by binding to DnaA-boxes, situated around the lambda pR promoter; there are no such sequences in ori lambda. Our results being to explain in molecular terms why lambda plasmid replication is DnaA-dependent [Kur et al., J. Mol. Biol. 198 (1987) 203-210] and why the initiation of phage lambda DNA replication is blocked (in E. coli devoid of prophage Rac) after inactivation of DnaA [Wegrzyn et al., Genetics (1995) in press].

摘要

噬菌体λ DNA复制的起始蛋白λ O蛋白,被认为是其宿主大肠杆菌DNA复制起始蛋白(DnaA)的类似物。二者分别特异性识别各自的复制起点,即ori λ和oriC,并组织特定复制复合物的组装。然而,DnaA具有额外的激活功能,作用于oriC近端的DnaA框,并调节在oriC及其周围启动子处起始的转录。在此,我们证明λ质粒复制可通过温度下调实现同步,温度下调会使先前变性的DnaAts蛋白复性。此外,我们表明消除DnaA的激活功能会影响ori λ处的转录激活。DnaA可能通过结合位于λ pR启动子周围的DnaA框发挥作用;ori λ中不存在此类序列。我们用分子术语解释了为什么λ质粒复制依赖于DnaA[Kur等人,《分子生物学杂志》198(1987)203 - 210],以及为什么在DnaA失活后(在不含原噬菌体Rac的大肠杆菌中)噬菌体λ DNA复制的起始被阻断[Wegrzyn等人,《遗传学》(1995)待发表]。

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