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小型RK2质粒在大肠杆菌提取物中的复制需要质粒编码的蛋白质TrfA以及宿主编码的蛋白质DnaA、B、G、DNA旋转酶和DNA聚合酶III。

Replication of mini RK2 plasmid in extracts of Escherichia coli requires plasmid-encoded protein TrfA and host-encoded proteins DnaA, B, G DNA gyrase and DNA polymerase III.

作者信息

Pinkney M, Diaz R, Lanka E, Thomas C M

机构信息

Department of Genetics, University of Birmingham, England.

出版信息

J Mol Biol. 1988 Oct 20;203(4):927-38. doi: 10.1016/0022-2836(88)90118-0.

Abstract

Soluble extracts of Escherichia coli capable of carrying out replication of the mini-RK2 derivative pCT461 have been prepared from cells carrying this plasmid or from plasmid-free bacteria. The latter are dependent upon exogenously added plasmid-encoded replication protein (TrfA) and require additional DnaA protein for optimum activity. This dependence upon DnaA was confirmed by the failure of DnaA-deficient cell extracts to support replication of pCT461 in the absence of added DnaA protein. Replication is unidirectional and begins at or near oriV, the vegetative replication origin of RK2. DNase I protection studies with purified TrfA indicate that this protein acts by binding to short (17 base-pairs) directly repeated DNA sequences present in oriV. The in vitro replication is resistant to rifampicin but can be abolished by antibodies against DnaG protein (E. coli primase) or DnaB protein (helicase) and by DNA gyrase inhibitors. Inhibition by arabinosyl-CTP suggests that DNA polymerase III is responsible for elongation of nascent DNA strands. These results are discussed in relation to the mechanism of RK2 replication and in the context of the host range of the plasmid.

摘要

已从携带该质粒的细胞或无质粒细菌中制备出能够进行mini-RK2衍生物pCT461复制的大肠杆菌可溶性提取物。后者依赖于外源添加的质粒编码复制蛋白(TrfA),并且需要额外的DnaA蛋白以实现最佳活性。在没有添加DnaA蛋白的情况下,缺乏DnaA的细胞提取物无法支持pCT461的复制,这证实了对DnaA的这种依赖性。复制是单向的,起始于RK2的营养复制起点oriV或其附近。用纯化的TrfA进行的DNase I保护研究表明,该蛋白通过与oriV中存在的短(17个碱基对)直接重复DNA序列结合而起作用。体外复制对利福平有抗性,但可被抗DnaG蛋白(大肠杆菌引发酶)或DnaB蛋白(解旋酶)的抗体以及DNA回旋酶抑制剂所消除。阿拉伯糖基-CTP的抑制作用表明DNA聚合酶III负责新生DNA链的延伸。结合RK2复制机制以及质粒的宿主范围对这些结果进行了讨论。

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