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肺炎链球菌中质粒pMV158的ssoA起始位点的滞后链复制:两个保守ssoA区域突变的体内和体外影响

Lagging-strand replication from the ssoA origin of plasmid pMV158 in Streptococcus pneumoniae: in vivo and in vitro influences of mutations in two conserved ssoA regions.

作者信息

Kramer M G, Khan S A, Espinosa M

机构信息

Centro de Investigaciones Biológicas, CSIC, Madrid, Spain.

出版信息

J Bacteriol. 1998 Jan;180(1):83-9. doi: 10.1128/JB.180.1.83-89.1998.

Abstract

The streptococcal plasmid pMV158 replicates by the rolling-circle mechanism. One feature of this replication mechanism is the generation of single-stranded DNA intermediates which are converted to double-stranded molecules. Lagging-strand synthesis initiates from the plasmid single-stranded origin, sso. We have used the pMV158-derivative plasmid pLS1 (containing the ssoA type of lagging-strand origin) and a set of pLS1 derivatives with mutations in two conserved regions of the ssoA (the recombination site B [RS(B)] and a conserved 6-nucleotide sequence [CS-6]) to identify sequences important for plasmid lagging-strand replication in Streptococcus pneumoniae. Cells containing plasmids with mutations in the RS(B) accumulated 30-fold more single-stranded DNA than cells containing plasmids with mutations in the CS-6 sequence. Specificity of lagging-strand synthesis was tested by the development of a new in vitro replication system with pneumococcal cell extracts. Four major initiation sites of lagging-strand DNA synthesis were observed. The specificity of initiation was maintained in plasmids with mutations in the CS-6 region. Mutations in the RS(B) region, on the other hand, resulted in the loss of specific initiation of lagging-strand synthesis and also severely reduced the efficiency of replication.

摘要

链球菌质粒pMV158通过滚环机制进行复制。这种复制机制的一个特点是产生单链DNA中间体,这些中间体随后会转变为双链分子。滞后链的合成起始于质粒单链起始位点sso。我们使用了pMV158衍生质粒pLS1(包含ssoA类型的滞后链起始位点)以及一组在ssoA的两个保守区域(重组位点B [RS(B)]和一个保守的6核苷酸序列[CS-6])发生突变的pLS1衍生物,以确定对肺炎链球菌中质粒滞后链复制重要的序列。含有在RS(B)发生突变的质粒的细胞积累的单链DNA比含有在CS-6序列发生突变的质粒的细胞多30倍。通过开发一种新的肺炎球菌细胞提取物体外复制系统,对滞后链合成的特异性进行了测试。观察到了滞后链DNA合成的四个主要起始位点。在CS-6区域发生突变的质粒中,起始的特异性得以维持。另一方面,RS(B)区域的突变导致滞后链合成的特异性起始丧失,并且还严重降低了复制效率。

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