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Molecular Dissection of Phage Endolysin

赖氨酸 周质间隙 支原体 肽聚糖 生物 大肠杆菌 自溶素 噬菌体 溶解 微生物学 溶解循环 分枝杆菌 细菌细胞结构 生物化学 细胞壁 结核分枝杆菌 细菌 基因 遗传学 医学 肺结核 病毒 病理
作者
Amol Arunrao Pohane,Himanshu Joshi,Vikas Jain
出处
期刊:Journal of Biological Chemistry [Elsevier BV]
卷期号:289 (17): 12085-12095 被引量:43
标识
DOI:10.1074/jbc.m113.529594
摘要

Mycobacterium tuberculosis has always been recognized as one of the most successful pathogens. Bacteriophages that attack and kill mycobacteria offer an alternate mechanism for the curtailment of this bacterium. Upon infection, mycobacteriophages produce lysins that catalyze cell wall peptidoglycan hydrolysis and mycolic acid layer breakdown of the host resulting in bacterial cell rupture and virus release. The ability to lyse bacterial cells make lysins extremely significant. We report here a detailed molecular dissection of the function and regulation of mycobacteriophage D29 Lysin A. Several truncated versions of Lysin A were constructed, and their activities were analyzed by zymography and by expressing them in both Escherichia coli and Mycobacterium smegmatis. Our experiments establish that Lysin A harbors two catalytically active domains, both of which show E. coli cell lysis upon their expression exclusively in the periplasmic space. However, the expression of only one of these domains and the full-length Lysin A caused M. smegmatis cell lysis. Interestingly, full-length protein remained inactive in E. coli periplasm. Our data suggest that the inactivity is ensued by a C-terminal domain that interacts with the N-terminal domain. This interaction was affirmed by surface plasmon resonance. Our experiments also demonstrate that the C-terminal domain of Lysin A selectively binds to M. tuberculosis and M. smegmatis peptidoglycans. Our methodology of studying E. coli cell lysis by Lysin A and its truncations after expressing these proteins in the bacterial periplasm with the help of signal peptide paves the way for a large scale identification and analysis of such proteins obtained from other bacteriophages.

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