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恶臭假单胞菌TOL质粒pWWO的分子与功能分析及整个调控型芳香环间位裂解途径基因的克隆

Molecular and functional analysis of the TOL plasmid pWWO from Pseudomonas putida and cloning of genes for the entire regulated aromatic ring meta cleavage pathway.

作者信息

Franklin F C, Bagdasarian M, Bagdasarian M M, Timmis K N

出版信息

Proc Natl Acad Sci U S A. 1981 Dec;78(12):7458-62. doi: 10.1073/pnas.78.12.7458.

Abstract

The genetic organization of the Pseudomonas putida plasmid pWWO-161, which encodes enzymes for the degradation of toluene and related aromatic hydrocarbons, has been investigated by transposition mutagenesis and gene cloning. Catabolic genes were localized to two clusters, one for upper pathway (hydrocarbon leads to carboxylic acid) enzymes and the other for lower pathway (carboxylic acid leads to tricarboxylic acid cycle) enzymes, that are separated by a 14-kilobase DNA segment. The physical organization of the catabolic genes thus reflects their functional organization into two regulatory blocks. The pWWO-161 DNA fragments Sst I fragment C and fragment D were cloned in a broad host range vector to produce plasmid pKT530. This hybrid encodes toluate oxygenase and all meta cleavage pathway enzymes, and it enables P. putida mt-2 and Escherichia coli K-12 cells to grow on m-toluate as sole carbon source. The pKT530 plasmid also carries xylS (a gene whose product has been postulated to regulate expression of the lower pathway genes) and the control sequences of the pathway that interact with this product, because catechol 2,3-oxygenase synthesis is specifically induced by m-toluate in both P. putida and E. coli. Evidence is presented that suggests the promoter operator of the meta pathway gene functions less effectively with the RNA polymerase or xylS product of E. coli than with the enzyme or product of P. putida.

摘要

恶臭假单胞菌质粒pWWO - 161编码甲苯及相关芳烃降解酶,已通过转座诱变和基因克隆对其遗传组织进行了研究。分解代谢基因定位于两个簇中,一个簇包含上途径(烃类转化为羧酸)酶,另一个簇包含下途径(羧酸转化为三羧酸循环)酶,这两个簇被一个14千碱基的DNA片段隔开。分解代谢基因的物理组织因此反映了它们在功能上被组织成两个调控模块。将pWWO - 161的DNA片段Sst I片段C和片段D克隆到一个广泛宿主范围的载体中,构建成质粒pKT530。这个杂种质粒编码甲苯酸加氧酶和所有间位裂解途径酶,它能使恶臭假单胞菌mt - 2和大肠杆菌K - 12细胞以间甲苯酸作为唯一碳源生长。pKT530质粒还携带xylS(其产物被推测可调控下途径基因的表达)以及与该产物相互作用的途径的控制序列,因为在恶臭假单胞菌和大肠杆菌中,间苯二酚2,3 - 加氧酶的合成均由间甲苯酸特异性诱导。有证据表明,间位途径基因的启动子操纵子与大肠杆菌的RNA聚合酶或xylS产物的作用效果不如与恶臭假单胞菌的酶或产物的作用效果好。

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