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Trichloroethylene and chloroform degradation by a recombinant pseudomonad expressing soluble methane monooxygenase from Methylosinus trichosporium OB3b.

机译:三氯乙烯和氯仿被重组假单胞菌降解该假单胞菌表达了来自甲烷单孢菌OB3b的可溶性甲烷单加氧酶。

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摘要

Soluble methane monooxygenase (sMMO) from Methylosinus trichosporium OB3b can degrade many halogenated aliphatic compounds that are found in contaminated soil and groundwater. This enzyme oxidizes the most frequently detected pollutant, trichloroethylene (TCE), at least 50 times faster than other enzymes. However, slow growth of the strain, strong competition between TCE and methane for sMMO, and repression of the smmo locus by low concentrations of copper ions limit the use of this bacterium. To overcome these obstacles, the 5.5-kb smmo locus of M. trichosporium OB3b was cloned into a wide-host-range vector (to form pSMMO20), and this plasmid was electroporated into five Pseudomonas strains. The best TCE degradation results were obtained with Pseudomonas putida F1/pSMMO20. The plasmid was maintained stably, and all five of the sMMO proteins (alpha, beta, and gamma hydroxylase proteins, reductase, and component B) were observed clearly by both sodium dodecyl sulfate-polyacrylamide gel electrophoresis and Western immunoblotting. TCE degradation rates were quantified for P. putida F1/pSMMO20 with a gas chromatograph (Vmax = 5 nmol per min per mg of protein), and the recombinant strain mineralized 55% of the TCE (10 microM) as indicated by measuring chloride ion concentrations with a chloride ion-specific electrode. The maximum TCE degradation rate obtained with the recombinant strain was lower than that of M. trichosporium OB3b but greater than other TCE-degrading recombinants and most well-studied pseudomonads. In addition, this recombinant strain mineralizes chloroform (a specific substrate for sMMO), grows much faster than M. trichosporium OB3b, and degrades TCE without competitive inhibition from the growth substrate.
机译:产自甲基毛孢菌OB3b的可溶性甲烷单加氧酶(sMMO)可以降解在污染的土壤和地下水中发现的许多卤代脂肪族化合物。这种酶氧化最常见的污染物三氯乙烯(TCE),比其他酶快至少50倍。但是,菌株生长缓慢,TCE和甲烷之间对sMMO的激烈竞争以及低浓度铜离子对smmo基因座的抑制作用限制了该细菌的使用。为了克服这些障碍,将毛孢霉OB3b的5.5-kb smmo基因座克隆到一个宽宿主范围的载体中(形成pSMMO20),并将该质粒电穿孔入5个假单胞菌菌株中。使用恶臭假单胞菌F1 / pSMMO20获得最佳的TCE降解结果。质粒保持稳定,十二烷基硫酸钠-聚丙烯酰胺凝胶电泳和Western免疫印迹均清楚地观察到所有五个sMMO蛋白(α,β和γ羟化酶蛋白,还原酶和B组分)。用气相色谱仪(Pmax)恶臭假单胞菌F1 / pSMMO20的TCE降解速率进行定量分析(Vmax =每毫克蛋白质每分钟5 nmol),重组菌株矿化了55%的TCE(10 microM),方法是测量氯离子浓度带有氯离子专用电极。重组菌株获得的最大TCE降解率低于毛孢霉OB3b,但高于其他降解TCE的重组子和研究最深入的假单胞菌。另外,该重组菌株使氯仿矿化(sMMO的特定底物),比毛孢霉菌OB3b的生长快得多,并且降解了TCE,而没有来自生长底物的竞争性抑制。

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