首页> 美国卫生研究院文献>Journal of Bacteriology >Cloning and characterization of a region of Enterococcus faecalis plasmid pPD1 encoding pheromone inhibitor (ipd) pheromone sensitivity (traC) and pheromone shutdown (traB) genes.
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Cloning and characterization of a region of Enterococcus faecalis plasmid pPD1 encoding pheromone inhibitor (ipd) pheromone sensitivity (traC) and pheromone shutdown (traB) genes.

机译:粪肠球菌质粒pPD1区域的克隆和表征该区域编码信息素抑制剂(ipd)信息素敏感性(traC)和信息素关闭(traB)基因。

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摘要

Bacteriocin plasmid pPD1 in Enterococcus faecalis encodes a mating response to recipient-produced sex pheromone cPD1. Once a recipient acquires pPD1, transconjugants apparently shut off cPD1 activity in broth culture and no longer behave as recipients for pPD1. This event is performed by synthesis of the pheromone inhibitor iPD1 and also by repression of cPD1 production, the so-called "pheromone shutdown." A 5.4-kb EcoRV-HincII segment of pPD1, which expressed iPD1 in Escherichia coli, was sequenced and found to be organized as traC-traB-traA-ipd; each open reading frame is analogous to that found in other pheromone plasmids, pAD1 and pCF10, and thus is designated in accordance with the nomenclature in pAD1. The ipd gene encodes a peptide consisting of 21 amino acids, in which the C-terminal eight residues correspond to iPD1. The putative TraC product has a strong similarity to oligopeptide-binding proteins found in other bacterial species, as do pheromone-binding proteins of pCF10 and pAD1. A strain carrying traC-disrupted pPD1 required a concentration of cPD1 fourfold higher than that needed by the wild-type strain for induction of sexual aggregation. These results suggest that the TraC product contributes to pheromone sensitivity as a pheromone-binding protein. A strain transformed with traB-disrupted pPD1 produced a high level of cPD1 similar to that produced by plasmid-free recipients and underwent self-induction. Thus, the TraB product contributes to cPD1 shutdown.
机译:粪肠球菌中的细菌素质粒pPD1编码对受体产生的性信息素cPD1的交配反应。一旦接受者获得了pPD1,转导结合体显然会关闭肉汤培养中的cPD1活性,不再充当pPD1的接受者。此事件是通过合成信息素抑制剂iPD1以及通过抑制cPD1产生(所谓的“信息素关闭”)来执行的。对在大肠杆菌中表达iPD1的pPD1的5.4-kb EcoRV-HincII片段进行测序,发现其组织形式为traC-traB-traA-ipd。每个开放阅读框与在其他信息素质粒pAD1和pCF10中发现的相似,因此按照pAD1中的命名法命名。 ipd基因编码由21个氨基酸组成的肽,其中C端的8个残基对应于iPD1。推定的TraC产物与其他细菌中发现的寡肽结合蛋白具有高度相似性,pCF10和pAD1的信息素结合蛋白也是如此。携带traC破坏的pPD1的菌株所需要的cPD1浓度要比野生型菌株诱导性聚集所需的浓度高四倍。这些结果表明,TraC产物作为信息素结合蛋白有助于信息素敏感性。用traB破坏的pPD1转化的菌株产生了高水平的cPD1,类似于无质粒受体产生的cPD1,并进行了自我诱导。因此,TraB产品有助于cPD1关闭。

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