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伯氏疏螺旋体BlyA和BlyB蛋白的特性:一种原噬菌体编码的类孔蛋白系统。

Characterization of Borrelia burgdorferi BlyA and BlyB proteins: a prophage-encoded holin-like system.

作者信息

Damman C J, Eggers C H, Samuels D S, Oliver D B

机构信息

Department of Molecular Biology and Biochemistry, Wesleyan University, Middletown, Connecticut 06459, USA.

出版信息

J Bacteriol. 2000 Dec;182(23):6791-7. doi: 10.1128/JB.182.23.6791-6797.2000.

Abstract

The conserved cp32 plasmid family of Borrelia burgdorferi was recently shown to be packaged into a bacteriophage particle (C. H. Eggers and D. S. Samuels, J. Bacteriol. 181:7308-7313, 1999). This plasmid encodes BlyA, a 7.4-kDa membrane-interactive protein, and BlyB, an accessory protein, which were previously proposed to comprise a hemolysis system. Our genetic and biochemical evidence suggests that this hypothesis is incorrect and that BlyA and BlyB function instead as a prophage-encoded holin or holin-like system for this newly described bacteriophage. An Escherichia coli mutant containing the blyAB locus that was defective for the normally cryptic host hemolysin SheA was found to be nonhemolytic, suggesting that induction of sheA by blyAB expression was responsible for the hemolytic activity observed previously. Analysis of the structural features of BlyA indicated greater structural similarity to bacteriophage-encoded holins than to hemolysins. Consistent with holin characteristics, subcellular localization studies with E. coli and B. burgdorferi indicated that BlyA is solely membrane associated and that BlyB is a soluble protein. Furthermore, BlyA exhibited a holin-like function by promoting the endolysin-dependent lysis of an induced lambda lysogen that was defective in the holin gene. Finally, induction of the cp32 prophage in B. burgdorferi dramatically stimulated blyAB expression. Our results provide the first evidence of a prophage-encoded holin within Borrelia.

摘要

最近研究表明,伯氏疏螺旋体保守的cp32质粒家族被包装进噬菌体颗粒中(C. H. 埃格斯和D. S. 塞缪尔斯,《细菌学杂志》181:7308 - 7313, 1999年)。该质粒编码BlyA,一种7.4 kDa的膜相互作用蛋白,以及BlyB,一种辅助蛋白,之前有人提出它们构成一个溶血系统。我们的遗传学和生物化学证据表明这个假说是错误的,BlyA和BlyB的功能相反,是这个新描述的噬菌体的原噬菌体编码的孔蛋白或类孔蛋白系统。发现含有blyAB基因座的大肠杆菌突变体,其对通常隐性的宿主溶血素SheA有缺陷,该突变体不溶血,这表明blyAB表达诱导sheA是之前观察到的溶血活性的原因。对BlyA结构特征的分析表明,它与噬菌体编码的孔蛋白的结构相似性大于与溶血素的相似性。与孔蛋白特征一致,用大肠杆菌和伯氏疏螺旋体进行的亚细胞定位研究表明,BlyA仅与膜相关,而BlyB是一种可溶性蛋白。此外,BlyA通过促进在孔蛋白基因有缺陷的诱导型λ溶原菌的内溶素依赖性裂解,表现出类孔蛋白功能。最后,伯氏疏螺旋体中cp32原噬菌体的诱导显著刺激了blyAB的表达。我们的结果提供了伯氏疏螺旋体中原噬菌体编码孔蛋白的首个证据。

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