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Cloning and characterization of Pseudomonas sp. strain DNT genes for 2,4-dinitrotoluene degradation.

机译:假单胞菌(Pseudomonas sp。)的克隆和鉴定。菌株DNT基因降解2,4-二硝基甲苯。

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摘要

The degradation of 2,4-dinitrotoluene (DNT) by Pseudomonas sp. strain DNT is initiated by a dioxygenase attack to yield 4-methyl-5-nitrocatechol (MNC) and nitrite. Subsequent oxidation of MNC by a monooxygenase results in the removal of the second molecule of nitrite, and further enzymatic reactions lead to ring fission. Initial studies on the molecular basis of DNT degradation in this strain revealed the presence of three plasmids. Mitomycin-derived mutants deficient in either DNT dioxygenase only or DNT dioxygenase and MNC monooxygenase were isolated. Plasmid profiles of mutant strains suggested that the mutations resulted from deletions in the largest plasmid. Total plasmid DNA partially digested by EcoRI was cloned into a broad-host-range cosmid vector, pCP13. Recombinant clones containing genes encoding DNT dioxygenase, MNC monooxygenase, and 2,4,5-trihydroxytoluene oxygenase were characterized by identification of reaction products and the ability to complement mutants. Subcloning analysis suggests that the DNT dioxygenase is a multicomponent enzyme system and that the genes for the DNT pathway are organized in at least three different operons.
机译:假单胞菌(Pseudomonas sp。)降解2,4-二硝基甲苯(DNT)。 DNT菌株是由双加氧酶攻击引发的,产生4-甲基-5-硝基邻苯二酚(MNC)和亚硝酸盐。 MNC随后被单加氧酶氧化导致亚硝酸盐的第二个分子被去除,进一步的酶促反应导致环裂变。关于该菌株中DNT降解的分子基础的初步研究表明存在三种质粒。分离出仅缺乏DNT双加氧酶或缺乏DNT双加氧酶和MNC单加氧酶的丝裂霉素衍生的突变体。突变菌株的质粒图谱表明,突变是由于最大质粒中的缺失引起的。将被EcoRI部分消化的总质粒DNA克隆到一个宽宿主范围的粘粒载体pCP13中。含有编码DNT双加氧酶,MNC单加氧酶和2,4,5-三羟基甲苯加氧酶的基因的重组克隆通过鉴定反应产物和互补突变体的能力来表征。亚克隆分析表明,DNT双加氧酶是一种多组分酶系统,DNT途径的基因至少组织在三个不同的操纵子中。

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    Suen, W C; Spain, J C;

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  • 年度 1993
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