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Cloning of a gene cluster encoding biphenyl and chlorobiphenyl degradation in Pseudomonas pseudoalcaligenes.

机译:假单胞菌假产碱菌中编码联苯和氯联苯降解的基因簇的克隆。

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摘要

A gene cluster encoding biphenyl- and chlorobiphenyl-degrading enzymes was cloned from a soil pseudomonad into Pseudomonas aeruginosa PAO1161. Chromosomal DNA from polychlorinated biphenyl-degrading Pseudomonas pseudoalcaligenes KF707 was digested with restriction endonuclease XhoI and cloned into the unique XhoI site of broad-host-range plasmid pKF330. Of 8,000 transformants tested, only 1, containing the chimeric plasmid pMFB1, rendered the host cell able to convert biphenyls and chlorobiphenyls to ring meta cleavage compounds via dihydrodiols and dihydroxy compounds. The chimeric plasmid contained a 7.9-kilobase XhoI insert. Subcloning experiments revealed that the genes bphA (encoding biphenyl dioxygenase), bphB (encoding dihydrodiol dehydrogenase), and bphC (encoding 2,3-dihydroxybiphenyl dioxygenase) were coded for by the 7.9-kilobase fragment. The gene order was bphA-bphB-bphC. The hydrolase activity, which converted the intermediate meta cleavage compounds to the final product, chlorobenzoic acids, and was encoded by a putative bphD gene, was missing from the cloned 7.9-kilobase fragment.
机译:从土壤假单胞菌中将编码联苯和氯联苯降解酶的基因簇克隆到铜绿假单胞菌PAO1161中。用限制性内切核酸酶XhoI消化多氯联苯降解假单胞菌拟杯假单胞菌KF707的染色体DNA,并将其克隆到宽宿主范围质粒pKF330的独特XhoI位点。在测试的8000个转化子中,只有1个包含嵌合质粒pMFB1,使宿主细胞能够通过二氢二醇和二羟基化合物将联苯和氯联苯转化为环间裂解化合物。嵌合质粒包含一个7.9碱基对的XhoI插入片段。亚克隆实验表明,7.9碱基对的片段编码了bphA(编码联苯双加氧酶),bphB(编码二氢二醇脱氢酶)和bphC(编码2,3-二羟基联苯双加氧酶)基因。基因顺序为bphA-bphB-bphC。克隆的7.9碱基碱基片段缺少水解酶活性,该水解酶活性将中间的间位裂解化合物转化为最终产物氯苯甲酸,并由推定的bphD基因编码。

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    Furukawa, K; Miyazaki, T;

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  • 年度 1986
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