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利用携带katG'::lux融合基因的大肠杆菌进行氧化应激检测。

Oxidative stress detection with Escherichia coli harboring a katG'::lux fusion.

作者信息

Belkin S, Smulski D R, Vollmer A C, Van Dyk T K, LaRossa R A

机构信息

Desert Research Institute, Ben-Gurion University of the Negev, Sede-Boqer, Israel.

出版信息

Appl Environ Microbiol. 1996 Jul;62(7):2252-6. doi: 10.1128/aem.62.7.2252-2256.1996.

Abstract

A plasmid containing a transcriptional fusion of the Escherichia coli katG promoter to a truncated Vibrio fischeri lux operon (luxCDABE) was constructed. An E. coli strain bearing this plasmid (strain DPD2511) exhibited low basal levels of luminescence, which increased up to 1,000-fold in the presence of hydrogen peroxide, organic peroxides, redox-cycling agents (methyl viologen and menadione), a hydrogen peroxide-producing enzyme system (xanthine and xanthine oxidase), and cigarette smoke. An oxyR deletion abolished hydrogen peroxide-dependent induction, confirming that oxyR controlled katG'::lux luminescence. Light emission was also induced by ethanol by an unexplained mechanism. A marked synergistic response was observed when cells were exposed to both ethanol and hydrogen peroxide; the level of luminescence measured in the presence of both inducers was much higher than the sum of the level of luminescence observed with ethanol and the level of luminescence observed with hydrogen peroxide. It is suggested that this construction or similar constructions may be used as a tool for assaying oxidant and antioxidant properties of chemicals, as a biosensor for environmental monitoring and as a tool for studying cellular responses to oxidative hazards.

摘要

构建了一个质粒,该质粒包含大肠杆菌katG启动子与截短的费氏弧菌lux操纵子(luxCDABE)的转录融合体。携带此质粒的大肠杆菌菌株(DPD2511菌株)表现出低水平的基础发光,在过氧化氢、有机过氧化物、氧化还原循环剂(甲基紫精和甲萘醌)、产过氧化氢酶系统(黄嘌呤和黄嘌呤氧化酶)以及香烟烟雾存在的情况下,发光增加高达1000倍。oxyR缺失消除了过氧化氢依赖性诱导,证实oxyR控制katG'::lux发光。乙醇也通过一种不明机制诱导发光。当细胞同时暴露于乙醇和过氧化氢时,观察到明显的协同反应;在两种诱导剂存在下测得的发光水平远高于单独使用乙醇时观察到的发光水平与单独使用过氧化氢时观察到的发光水平之和。有人提出,这种构建体或类似构建体可作为一种工具,用于测定化学品的氧化和抗氧化特性,作为环境监测的生物传感器,以及作为研究细胞对氧化危害反应的工具。

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