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粪肠球菌信息素响应型接合质粒pYI17上编码的细菌素31决定簇的克隆与基因组织

Cloning and genetic organization of the bacteriocin 31 determinant encoded on the Enterococcus faecalis pheromone-responsive conjugative plasmid pYI17.

作者信息

Tomita H, Fujimoto S, Tanimoto K, Ike Y

机构信息

Department of Microbiology, Gunma University School of Medicine, Maebashi, Gunma, Japan.

出版信息

J Bacteriol. 1996 Jun;178(12):3585-93. doi: 10.1128/jb.178.12.3585-3593.1996.

Abstract

The conjugative plasmid pYI17 (57.5 kb) isolated from Enterococcus faecalis YI717 confers a pheromone response on the host and encodes the bacteriocin 31 gene. Bacteriocin 31 is active against E. hirae 9790, E. faecium, and Listeria monocytogenes. pYI17 was mapped physically by restriction enzyme analysis and the relational clone method. Deletion mutant and sequence analyses of the EcoRI fragment B cloned from pYl17 revealed that a 1.0-kb fragment contained the bacteriocin gene (bacA) and an immunity gene (bacB). This fragment induced bacteriocin activity in E. faecalis OG1X and E. hirae 9790. The bacA gene is located on the pYI17 physical map between 3.37 and 3.57 kb, and bacB is located between 3.59 kb and 3.87 kb, bacA encodes 67 amino acids, and bacB encodes 94 amino acids. The deduced amino acid sequence of the bacA protein contained a series of hydrophobic residues typical of a signal sequence at its amino terminus. The predicted mature bacA protein (43 amino acids) showed sequence homology with the membrane-active class II bacteriocins of lactic acid bacteria. Analysis of Tn5 insertion mutants and the resulting transcripts indicated that these genes are transcribed as an operon composed of bacA, bacB, and an open reading frame located downstream of bacB designated ORF3.

摘要

从粪肠球菌YI717中分离出的接合质粒pYI17(57.5 kb)赋予宿主信息素应答能力,并编码细菌素31基因。细菌素31对希氏肠球菌9790、屎肠球菌和单核细胞增生李斯特菌具有活性。通过限制酶分析和相关克隆方法对pYI17进行了物理图谱绘制。对从pYl17克隆的EcoRI片段B进行缺失突变体和序列分析,结果表明一个1.0 kb的片段包含细菌素基因(bacA)和免疫基因(bacB)。该片段在粪肠球菌OG1X和希氏肠球菌9790中诱导细菌素活性。bacA基因位于pYI17物理图谱上3.37至3.57 kb之间,bacB位于3.59 kb至3.87 kb之间,bacA编码67个氨基酸,bacB编码94个氨基酸。bacA蛋白推导的氨基酸序列在其氨基末端包含一系列典型信号序列的疏水残基。预测的成熟bacA蛋白(43个氨基酸)与乳酸菌的膜活性II类细菌素具有序列同源性。对Tn5插入突变体及其产生的转录本的分析表明,这些基因作为一个由bacA、bacB和位于bacB下游的一个开放阅读框(命名为ORF3)组成的操纵子进行转录。

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