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首页> 外文期刊>Microbiology >Plasmids derived from Gifsy-1/Gifsy-2, lambdoid prophages contributing to the virulence of Salmonella enterica serovar Typhimurium: implications for the evolution of replication initiation proteins of lambdoid phages and enterobacteria
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Plasmids derived from Gifsy-1/Gifsy-2, lambdoid prophages contributing to the virulence of Salmonella enterica serovar Typhimurium: implications for the evolution of replication initiation proteins of lambdoid phages and enterobacteria

机译:来自Gifsy-1 / Gifsy-2的质粒,兰布氏植物促进型毒素肠道毒素血吸虫毒蕈毒力:对羊水噬菌体和细菌的复制起始蛋白的演变的影响

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Gifsy-1 and Gifsy-2 are lambdoid prophages which contribute to the virulence of Salmonella enterica serovar Typhimurium. The nucleotide sequence of the replication region of both prophages is identical, and similar in organization to the replication region of bacteriophage λ. To investigate the replication of the Gifsy phages and the relationship between Gifsy and host chromosome replication, a plasmid which contained all the genes and regulatory sequences required for autonomous replication in bacterial cells was constructed. This plasmid, pGifsy, was stably maintained in Escherichia coli cells. The helicase loader of the Gifsy phages is very similar to the DnaC protein of the host, a feature characteristic of a large group of prophages common in the sequenced genomes of pathogenic enterobacteria. This DnaC-like protein showed no similarity to the helicase loader of bacteriophage λ and closely related phages. Interestingly, unlike plasmids derived from bacteriophage λ (λ plasmids), pGifsy did not require a gene encoding the putative helicase loader for replication, although deletion of this gene resulted in a decrease in plasmid copy number. Under these conditions, it was shown that the plasmid utilized the helicase loader coded by the host. On the other hand, the viral protein could not substitute for DnaC in bacterial chromosome replication. The results of the current study support the hypothesis that the enterobacterial helicase loader is of viral origin. This hypothesis explains why the gene for DnaC, the protein central to both replication initiation and replication restart in E. coli, is present in the genomes of Escherichia, Shigella, Salmonella and Buchnera, but not in the genomes of related enterobacteria.
机译:Gifsy-1和Gifsy-2是抗羊毛植物的武器,这有助于Salmonella肠道毒素毒蕈醋栗的毒力。两种预脉冲的复制区域的核苷酸序列是相同的,并且在组织中与噬菌体λ的复制区域相似。为了研究Gifsy噬菌体的复制和Gifsy和宿主染色体复制之间的关系,构建了一种质粒,其包含在细菌细胞中自主复制所需的所有基因和调节序列。该质粒pGIFSY在大肠杆菌细胞中稳定地保持。 Gifsy噬菌体的螺旋酶装载机与宿主的DNAc蛋白质非常相似,该特征是致病性肠杆菌的测序基因组中常见的一大群的特征特征。该DNAC样蛋白与噬菌体λ和密切相关的噬菌体的螺旋酶装载机没有相似性。有趣的是,与源自噬菌体λ(λ质粒)的质粒不同,PGIFSY不需要编码推定的旋转酶装载机的基因以进行复制,尽管缺失该基因导致质粒拷贝数减少。在这些条件下,显示该质粒利用由宿主编码的螺旋酶负荷替床。另一方面,病毒蛋白不能替代DNAc在细菌染色体复制中。目前研究的结果支持细菌螺旋酶装载机是病毒来源的假设。该假设解释了为什么DNAC的基因,蛋白质中的复制引发和复制重新发生在大肠杆菌中,存在于大肠杆菌,志贺氏菌,沙门氏菌和Buchnera的基因组中,但不是在相关肠菌的基因组中。

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