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来自美人鱼发光杆菌的pMJ101质粒复制区域的定位

Localization of the replication region of the pMJ101 plasmid from Vibrio ordalii.

作者信息

Bidinost C, Crosa J H, Actis L A

机构信息

Departamento de Bioquimica Clinica, Facultad de Ciencias Quimicas, Universidad Nacional de Cordoba, Argentina.

出版信息

Plasmid. 1994 May;31(3):242-50. doi: 10.1006/plas.1994.1026.

Abstract

The 30-kb pMJ101 plasmid is found as a high-copy-number pool in all the pathogenic strains of Vibrio ordalii examined so far. The replication functions of pMJ101 were localized within a 2.4-kb EcoRV-HindIII restriction fragment by using different subclones in combination with Bal31 exonuclease deletions and Tn5 insertion mutants. Recombinant clones carrying this fragment were able to replicate in Escherichia coli cells deficient in either DNA Polymerase I (PolA-) or integration host factor functions. However, the viability of recombinant plasmids containing the pMJ101 origin of replication was dependent on the expression of the gene encoding the DnaA protein. Electrophoretic analysis of plasmid-encoded proteins in an in vitro transcription-translation coupled system revealed that the replication region of pMJ101 encodes a 36-kDa protein. The expression of this protein was correlated with the ability of different recombinant plasmids harboring this pMJ101 DNA region to replicate in the PolA- E. coli strain. Replication typing showed that pMJ101 is not related to any of the plasmid incompatibility groups contained in the bank of rep probes described by M. Couturier et al. (Microbiol. Rev. 52, 375-395, 1988).

摘要

在迄今为止检测的所有奥尔氏弧菌致病菌株中,30 kb的pMJ101质粒以高拷贝数形式存在。通过使用不同的亚克隆,结合Bal31核酸外切酶缺失和Tn5插入突变体,将pMJ101的复制功能定位在一个2.4 kb的EcoRV - HindIII限制片段内。携带该片段的重组克隆能够在缺乏DNA聚合酶I(PolA-)或整合宿主因子功能的大肠杆菌细胞中复制。然而,含有pMJ101复制起点的重组质粒的活力依赖于编码DnaA蛋白的基因的表达。在体外转录 - 翻译偶联系统中对质粒编码蛋白进行的电泳分析表明,pMJ101的复制区域编码一种36 kDa的蛋白。该蛋白的表达与携带此pMJ101 DNA区域的不同重组质粒在PolA-大肠杆菌菌株中复制的能力相关。复制分型显示,pMJ101与M. Couturier等人(《微生物学评论》52,375 - 395,1988)描述的rep探针库中包含的任何质粒不相容群均无关。

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