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首页> 外文期刊>Plasmid: An International Journal Devoted to Extrachromosomal Gene Systems >Plasmid rolling-circle replication: highlights of two decades of research.
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Plasmid rolling-circle replication: highlights of two decades of research.

机译:质粒滚环复制:二十年研究的重点。

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This review provides a historical perspective of the major findings that contributed to our current understanding of plasmid rolling-circle (RC) replication. Rolling-circle-replicating (RCR) plasmids were discovered approximately 20 years ago. The first of the RCR plasmids to be identified were native to Gram-positive bacteria, but later such plasmids were also identified in Gram-negative bacteria and in archaea. Further studies revealed mechanistic similarities in the replication of RCR plasmids and the single-stranded DNA bacteriophages of Escherichia coli, although there were important differences as well. Three important elements, a gene encoding the initiator protein, the double strand origin, and the single strand origin, are contained in all RCR plasmids. The initiator proteins typically contain a domain involved in their sequence-specific binding to the double strand origin and a domain that nicks within the double strand origin and generates the primer for DNA replication. The double strand origins include the start-site of leading strand synthesis and contain sequences that are bound and nicked by the initiator proteins. The single strand origins are required for synthesis of the lagging strand of RCR plasmids. The single strand origins are non-coding regions that are strand-specific, and contain extensive secondary structures. This minireview will highlight the major findings in the study of plasmid RC replication over the past twenty years. Regulation of replication of RCR plasmids will not be included since it is the subject of another review.
机译:这篇综述提供了主要发现的历史观点,这些发现有助于我们对质粒滚环(RC)复制的当前了解。大约20年前发现了滚转复制(RCR)质粒。首先要鉴定的RCR质粒对革兰氏阳性菌是天然的,但后来在革兰氏阴性菌和古细菌中也鉴定出了此类质粒。进一步的研究表明,尽管RRC质粒的复制和大肠杆菌的单链DNA噬菌体的复制机制相似,但也存在重要差异。所有RCR质粒均包含三个重要元素,即编码起始蛋白,双链起源和单链起源的基因。引发剂蛋白通常包含一个域,该域参与其与双链起点的序列特异性结合,以及一个在双链起点内形成切口并生成用于DNA复制的引物的域。双链起源包括前导链合成的起始位点,并包含由引发剂蛋白结合和形成切口的序列。 RCR质粒的落后链的合成需要单链起源。单链起源是链特异性的非编码区,并且包含广泛的二级结构。这份小型综述将突出过去20年中质粒RC复制研究的主要发现。由于这是另一篇综述的主题,因此不包括RCR质粒复制的调控。

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