Replication of a Bacillus subtilis oriC plasmid in vitro

脱氧核糖核酸 生物 复制的起源 dnaB解旋酶 枯草芽孢杆菌 DNA复制 质粒 复制前复合体 分子生物学 原核DNA复制 原点识别复合体 自主复制序列 体外 基因 细胞生物学 遗传学 真核细胞DNA复制 解旋酶 核糖核酸 细菌
作者
Shigeki Moriya,William Firshein,Hiroshi Yoshikawa,Naotaka Ogasawara
出处
期刊:Molecular Microbiology [Wiley]
卷期号:12 (3): 469-478 被引量:40
标识
DOI:10.1111/j.1365-2958.1994.tb01035.x
摘要

Summary We constructed an in vitro replication system specific for a Bacillus subtilis oriC plasmid using a soluble fraction derived from cell extracts of B. subtilis. DNA polymerase III and two initiation proteins, DnaA and DnaB, were required for in vitro replication as observed in vivo. Both upstream and downstream DnaA box regions of the dnaA gene were required as cis‐elements for in vitro synthesis of the B. subtilis oriC plasmid as well as for in vivo activity. The replication was semi‐conservative and only one round of replication occurred within 15min. These results indicate that in vitro replication faithfully reproduced in vivo replication. To elucidate the site of initiation and the direction of replication, we analysed replicative intermediates generated in vitro in the presence of various concentrations of ddGTP by two methods. First, analysis of restriction fragments around the dnaA gene showed a high level of incorporation of the radioactive substrate, indicating that replication began within the vicinity of the dnaA gene. Second, using 2‐dimensional gel electrophoresis, bubble arcs were detected only on fragments containing the DnaA box region downstream of the dnaA gene, indicating that the initiation site resided within this region. The distribution of the bubble arcs suggested that both bidirectional and unidirectional replication occurred in vitro.
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