质粒RP4的接合转移系统:通过转座子7插入进行分析
Conjugal transfer system of plasmid RP4: analysis by transposon 7 insertion.
作者信息
Barth P T, Grinter N J, Bradley D E
出版信息
J Bacteriol. 1978 Jan;133(1):43-52. doi: 10.1128/jb.133.1.43-52.1978.
Abstract
We have begun an analysis in Escherichia coli of the conjugal transfer functions of the broad-host-range plasmid RP4. We have isolated 19 tra mutants of RP4, generated by insertion of transposon 7, and mapped their insertion sites by restriction endonuclease analysis. These sites fall into two separate regions on either side of the kanamycin resistance determinant. The transfer rates of the mutants range from 10% of that of RP4 to an undetectable level. Spot tests with the P-1 pilus-specific phages PRR1, Pf3, and PR4 and electron microscopic examination for pili have classified the mutants into several phenotypes consistent with their having normal, retracted, or no pili. Analysis of transient plasmid heterozygotes, created by P1 transduction, divided the tra mutants into a minimum of five complementation groups. Some of these groups contain more than one phenotypic class and may represent more than one gene because of the possible polar and deletion effects of Tn7 insertion.
摘要
我们已开始对广宿主范围质粒RP4的接合转移功能在大肠杆菌中进行分析。我们分离出了19个由转座子7插入产生的RP4的tra突变体,并通过限制性内切酶分析确定了它们的插入位点。这些位点位于卡那霉素抗性决定簇两侧的两个不同区域。突变体的转移率从RP4的10%到检测不到的水平不等。用P-1菌毛特异性噬菌体PRR1、Pf3和PR4进行斑点试验以及对菌毛进行电子显微镜检查,已将突变体分为几种表型,这与它们具有正常菌毛、缩回菌毛或无菌毛的情况一致。对通过P1转导产生的瞬时质粒杂合子的分析,将tra突变体至少分为五个互补群。其中一些群包含不止一种表型类别,由于Tn7插入可能产生的极性和缺失效应,可能代表不止一个基因。
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