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链球菌质粒pMV158及其衍生物在大肠杆菌无细胞提取物中的复制

Replication of the streptococcal plasmid pMV158 and derivatives in cell-free extracts of Escherichia coli.

作者信息

del Solar G, Diaz R, Espinosa M

出版信息

Mol Gen Genet. 1987 Mar;206(3):428-35. doi: 10.1007/BF00428882.

DOI:10.1007/BF00428882
PMID:3035343
Abstract

pMV158 is a 5.4 kb broad host range multicopy plasmid specifying tetracycline resistance. This plasmid and two of its derivatives, pLS1 and pLS5, are stably maintained and express their genetic information in gram-positive and gram-negative hosts. The in vitro replication of plasmid pMV158 and its derivatives was studied in extracts prepared from plasmid-free Escherichia coli cells and the replicative characteristics of the streptococcal plasmids were compared to those of the E. coli replicons, ColE1 and the mini-R1 derivative pKN182. The optimal replicative activity of the E. coli extracts was found at a cellular phase of growth that corresponded to 2 g wet weight of cells per litre. Maximal synthesis of streptococcal plasmid DNA occurred after 90 min of incubation and at a temperature of 30 degrees C. The optimal concentration of template DNA was 40 micrograms/ml. Higher plasmid DNA concentrations resulted in a decrease in the incorporation of dTMP, indicating that competition of specific replication factor(s) for functional plasmid origins may occur. In vitro replication of plasmid pMV158 and its derivatives required the host RNA polymerase and de novo protein synthesis. The final products of the streptococcal plasmid DNAs replicated in the E. coli in vitro system were monomeric supercoiled DNA forms that had completed at least one round of replication, although a set of putative replicative intermediates could also be found. The results suggest that a specific plasmid-encoded factor is needed for the replication of the streptococcal plasmids.

摘要

pMV158是一种5.4 kb的广宿主范围多拷贝质粒,赋予四环素抗性。该质粒及其两个衍生物pLS1和pLS5能在革兰氏阳性和革兰氏阴性宿主中稳定维持并表达其遗传信息。在从无质粒的大肠杆菌细胞制备的提取物中研究了质粒pMV158及其衍生物的体外复制,并将链球菌质粒的复制特性与大肠杆菌复制子ColE1和mini-R1衍生物pKN182的复制特性进行了比较。发现大肠杆菌提取物的最佳复制活性出现在细胞生长阶段,相当于每升2克湿重的细胞。链球菌质粒DNA在孵育90分钟后且温度为30℃时合成量最大。模板DNA的最佳浓度为40微克/毫升。较高的质粒DNA浓度导致dTMP掺入量减少,表明可能存在特定复制因子对功能性质粒起始位点的竞争。质粒pMV158及其衍生物的体外复制需要宿主RNA聚合酶和从头合成蛋白质。在大肠杆菌体外系统中复制的链球菌质粒DNA的最终产物是已完成至少一轮复制的单体超螺旋DNA形式,不过也能发现一组假定的复制中间体。结果表明,链球菌质粒的复制需要一种特定的质粒编码因子。

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