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无活性的pT181起始异二聚体RepC/C能够结合,但无法诱导质粒复制起点解链。

The inactive pT181 initiator heterodimer, RepC/C, binds but fails to induce melting of the plasmid replication origin.

作者信息

Jin R, Zhou X, Novick R P

机构信息

Department of Molecular Pathogenesis, Skirball Institute of Biomolecular Medicine, New York University Medical Center, New York, New York 10016, USA.

出版信息

J Biol Chem. 1996 Dec 6;271(49):31086-91. doi: 10.1074/jbc.271.49.31086.

Abstract

Staphylococcus aureus plasmid pT181 replicates via a rolling circle mechanism. The synthesis of the pT181 initiator protein (RepC) is regulated by antisense RNAs, and RepC is inactivated after usage by the attachment of an oligonucleotide to one of its subunits. The inactivated heterodimeric RepC/C* has been shown be unable to initiate replication in vitro (Rasooly, A., and Novick, R. P. (1993) Science 262, 1048-1050). The inactive RepC/C* has been found to be very stable and constitute about 90-95% of the total RepC antigen inside the cell. We studied the specific interaction of the RepC/C and RepC/C* complex with the pT181 double strand origin. The results indicated that RepC/C and RepC/C* footprint supercoiled DNA differently although their footprints on linear DNA are similar; we also find that RepC/C is able to enhance cruciform extrusion while RepC/C* cannot. RepC/C* binds and bends the double strand origin much more weakly than does RepC/C. These results suggest that the attached oligonucleotide induces a conformational change in the RepC/C* molecule that is responsible for its lack of activity.

摘要

金黄色葡萄球菌质粒pT181通过滚环机制进行复制。pT181起始蛋白(RepC)的合成受反义RNA调控,并且RepC在使用后通过一个寡核苷酸连接到其一个亚基上而失活。已证明失活的异源二聚体RepC/C在体外无法启动复制(Rasooly, A.和Novick, R. P.(1993年)《科学》262, 1048 - 1050)。已发现无活性的RepC/C非常稳定,在细胞内占总RepC抗原的约90 - 95%。我们研究了RepC/C和RepC/C复合物与pT181双链原点的特异性相互作用。结果表明,RepC/C和RepC/C对超螺旋DNA的足迹不同,尽管它们对线性DNA的足迹相似;我们还发现RepC/C能够增强十字形结构的挤出,而RepC/C则不能。RepC/C与双链原点的结合和弯曲比RepC/C弱得多。这些结果表明,连接的寡核苷酸诱导了RepC/C*分子的构象变化,这是其缺乏活性的原因。

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