一种支持小型RK2质粒在大肠杆菌中进行体外复制的内膜衍生亚组分的分离。
Isolation of an inner membrane-derived subfraction that supports in vitro replication of a mini-RK2 plasmid in Escherichia coli.
作者信息
Kim P D, Firshein W
机构信息
Department of Molecular Biology and Biochemistry, Wesleyan University, Middletown, Connecticut 06459, USA.
出版信息
J Bacteriol. 2000 Mar;182(6):1757-60. doi: 10.1128/JB.182.6.1757-1760.2000.
Previous results have demonstrated that the inner, but not the outer, membrane fraction of Escherichia coli is the site of membrane-associated DNA replication of plasmid RK2, a broad-host-range plasmid capable of replication in a wide variety of gram-negative hosts (K. Michaels, J. Mei, and W. Firshein, Plasmid 32:19-31, 1994). To resolve the inner membrane replication site further, the procedure of Ishidate et al. (K. Ishidate, E. S. Creeger, J. Zrike, S. Deb, G. Glauner, T. J. MacAlister, and L. I. Rothfield, J. Biol. Chem. 261:428-443, 1986) was used to separate the inner membrane into a number of subfractions, of which only one, a small subfraction containing only 10% of the entire membrane, was found to synthesize DNA inhibited by antibody prepared against the plasmid-encoded initiation protein TrfA. This is the same subfraction that was also found to bind oriV and TrfA to the greatest extent in filter binding assays (J. Mei, S. Benashski, and W. Firshein, J. Bacteriol. 177:6766-6772, 1995).
先前的研究结果表明,大肠杆菌的内膜(而非外膜)部分是质粒RK2膜相关DNA复制的位点,RK2是一种广宿主范围的质粒,能够在多种革兰氏阴性宿主中复制(K. 迈克尔斯、J. 梅和W. 菲尔申,《质粒》32:19 - 31,1994年)。为了进一步确定内膜复制位点,采用了石idate等人的方法(K. 石idate、E. S. 克里格、J. 齐里克、S. 德布、G. 格劳纳、T. J. 麦卡利斯特和L. I. 罗斯菲尔德,《生物化学杂志》261:428 - 443,1986年)将内膜分离成多个亚组分,其中只有一个亚组分,即仅占整个膜10%的小亚组分,被发现能合成受针对质粒编码的起始蛋白TrfA制备的抗体抑制的DNA。在滤膜结合试验中,同样也是这个亚组分被发现与oriV和TrfA的结合程度最高(J. 梅、S. 贝纳什斯基和W. 菲尔申,《细菌学杂志》177:6766 - 677 , 1995年)。
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