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转座子插入揭示了蒙氏立克次体的一种质粒pRM。

Transposon insertion reveals pRM, a plasmid of Rickettsia monacensis.

作者信息

Baldridge Gerald D, Burkhardt Nicole Y, Felsheim Roderick F, Kurtti Timothy J, Munderloh Ulrike G

机构信息

Department of Entomology, University of Minnesota, St Paul, MN 55108, USA.

出版信息

Appl Environ Microbiol. 2007 Aug;73(15):4984-95. doi: 10.1128/AEM.00988-07. Epub 2007 Jun 15.

Abstract

Until the recent discovery of pRF in Rickettsia felis, the obligate intracellular bacteria of the genus Rickettsia (Rickettsiales: Rickettsiaceae) were thought not to possess plasmids. We describe pRM, a plasmid from Rickettsia monacensis, which was detected by pulsed-field gel electrophoresis and Southern blot analyses of DNA from two independent R. monacensis populations transformed by transposon-mediated insertion of coupled green fluorescent protein and chloramphenicol acetyltransferase marker genes into pRM. Two-dimensional electrophoresis showed that pRM was present in rickettsial cells as circular and linear isomers. The 23,486-nucleotide (31.8% G/C) pRM plasmid was cloned from the transformant populations by chloramphenicol marker rescue of restriction enzyme-digested transformant DNA fragments and PCR using primers derived from sequences of overlapping restriction fragments. The plasmid was sequenced. Based on BLAST searches of the GenBank database, pRM contained 23 predicted genes or pseudogenes and was remarkably similar to the larger pRF plasmid. Two of the 23 genes were unique to pRM and pRF among sequenced rickettsial genomes, and 4 of the genes shared by pRM and pRF were otherwise found only on chromosomes of R. felis or the ancestral group rickettsiae R. bellii and R. canadensis. We obtained pulsed-field gel electrophoresis and Southern blot evidence for a plasmid in R. amblyommii isolate WB-8-2 that contained genes conserved between pRM and pRF. The pRM plasmid may provide a basis for the development of a rickettsial transformation vector.

摘要

直到最近在猫立克次体中发现pRF之前,立克次体属(立克次体目:立克次体科)的专性细胞内细菌一直被认为不具有质粒。我们描述了来自蒙氏立克次体的pRM质粒,通过脉冲场凝胶电泳和Southern印迹分析检测到该质粒,这两种分析方法针对的是来自两个独立的蒙氏立克次体群体的DNA,这些群体通过转座子介导将偶联的绿色荧光蛋白和氯霉素乙酰转移酶标记基因插入pRM中进行转化。二维电泳显示pRM以环状和线性异构体的形式存在于立克次体细胞中。通过对经限制酶消化的转化体DNA片段进行氯霉素标记拯救,并使用源自重叠限制片段序列的引物进行PCR,从转化体群体中克隆出了23,486个核苷酸(G/C含量为31.8%)的pRM质粒。对该质粒进行了测序。基于对GenBank数据库的BLAST搜索,pRM包含23个预测基因或假基因,并且与较大的pRF质粒非常相似。在已测序的立克次体基因组中,这23个基因中有两个是pRM和pRF所特有的,pRM和pRF共有的4个基因仅在猫立克次体或祖先群立克次体贝利立克次体和加拿大立克次体的染色体上发现。我们获得了脉冲场凝胶电泳和Southern印迹证据,证明在嗜吞噬细胞无形体分离株WB - 8 - 2中存在一种质粒,该质粒含有在pRM和pRF之间保守的基因。pRM质粒可能为开发立克次体转化载体提供基础。

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