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A sensitive method for rapid detection of alkyl halides and dehalogenase activity using a multistep enzyme assay

机译:使用多步酶测定法快速检测卤代烷和脱卤酶活性的灵敏方法

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摘要

A method for the detection of haloalkane conversion to the corresponding alcohols by haloalkane dehalogenases is described. It is based on a multistage enzyme reaction which allows for the analysis of alkyl halides in buffered systems. Irreversible hydrolytic dehalogenation catalyzed by haloalkane dehalogenase DhaA from Rhodococcus erythropolis transfers an alkyl halide into a corresponding alcohol that is further oxidized by alcohol oxidase AOX from Pichia pastoris yielding a respective aldehyde and hydrogen peroxide easily detectable via the horseradish peroxidase catalyzed oxidation of chromogenic molecules. Due to its high sensitivity (0.025 mM, 0.43 ppm for 1,3-dibromopropane), low expenditure and the ability of handling a large number of samples in parallel, this method is an attractive alternative to existing procedures for the monitoring of both haloalkanes and dehalogenases.
机译:描述了一种通过卤代烷脱卤酶检测卤代烷转化为相应醇的方法。它基于多阶段酶反应,可分析缓冲系统中的烷基卤。来自红球红球菌的卤代烷脱卤酶DhaA催化的不可逆水解脱卤作用将烷基卤转移到相应的醇中,再由巴斯德毕赤酵母中的醇氧化酶AOX进一步氧化该相应的醇,产生易于通过辣根过氧化物酶催化的氧化作用被氧化的相应的醛和过氧化氢。由于它的高灵敏度(0.025 µmM,对于1,3-二溴丙烷为0.43 µppm),较低的费用以及能够并行处理大量样品的能力,因此该方法是目前监测卤代烷烃和卤代烷烃的现有方法的一种有吸引力的替代方法。脱卤素酶。

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