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对恶臭假单胞菌TOL质粒pWW0编码的一种底物特异性宽松的芳香环双加氧酶甲苯酸1,2-双加氧酶的遗传分析。

Genetic analysis of a relaxed substrate specificity aromatic ring dioxygenase, toluate 1,2-dioxygenase, encoded by TOL plasmid pWW0 of Pseudomonas putida.

作者信息

Harayama S, Rekik M, Timmis K N

出版信息

Mol Gen Genet. 1986 Feb;202(2):226-34. doi: 10.1007/BF00331641.

DOI:10.1007/BF00331641
PMID:3010045
Abstract

Toluate 1,2-dioxygenase is the first enzyme of a meta-cleavage pathway for the oxidative catabolism of benzoate and substituted benzoates to Krebs cycle intermediates that is specified by TOL plasmid pWW0 of Pseudomonas putida. A collection of derivatives harbouring Tn1000 insertions and defective in toluate dioxygenase have been isolated from pPL392, a pBR322-based hybrid plasmid carrying the TOL plasmid meta-cleavage pathway operon. In parallel, a series of N-methyl-N'-nitro-N-nitro-soguanidine-induced mutant plasmids defective in this enzyme activity were isolated from pNM72, a pKT231-based hybrid plasmid carrying the same operon. Pairs of mutant plasmids, consisting of one Tn1000 derivative and one nitrosoguanidine-induced derivative, were used for complementation analysis of toluate dioxygenase in Escherichia coli recA bacteria, in which the formation of 2-hydroxymuconic semialdehyde from benzoate was examined. Four cistrons for toluate 1,2-dioxygenase were thus identified. DNA fragments containing nitrosoguanidine-induced mutant cistrons plus the other meta-cleavage operon genes were cloned into pOT5, an R388-based vector, and complementation tests between different nitrosoguanidine-induced mutant cistrons were carried out in Pseudomonas putida cells, this time scoring for growth on p-toluate. This analysis also identified four cistrons. Examination of the products of these cistrons, by means of E. coli minicells containing pPL392 or its Tn1000 insertion derivatives, indicated that the first two cistrons of the operon comprise a single gene, xylX, which encodes a 57 kilodalton protein, and that the third cistron, xylY, encodes a 20 kilodalton protein.

摘要

甲苯酸1,2 - 双加氧酶是恶臭假单胞菌TOL质粒pWW0所规定的将苯甲酸和取代苯甲酸氧化分解为三羧酸循环中间体的间位裂解途径中的第一种酶。从pPL392(一种携带TOL质粒间位裂解途径操纵子的基于pBR322的杂交质粒)中分离出了一系列携带Tn1000插入且甲苯酸双加氧酶有缺陷的衍生物。同时,从pNM72(一种携带相同操纵子的基于pKT231的杂交质粒)中分离出了一系列经N - 甲基 - N' - 硝基 - N - 亚硝基胍诱导的、该酶活性有缺陷的突变体质粒。由一个Tn1000衍生物和一个亚硝基胍诱导的衍生物组成的突变体质粒对,用于在大肠杆菌recA细菌中对甲苯酸双加氧酶进行互补分析,在此分析中检测了从苯甲酸形成2 - 羟基粘康酸半醛的情况。由此确定了甲苯酸1,2 - 双加氧酶的四个顺反子。将含有亚硝基胍诱导的突变顺反子以及其他间位裂解操纵子基因的DNA片段克隆到基于R388的载体pOT5中,并在恶臭假单胞菌细胞中对不同的亚硝基胍诱导的突变顺反子进行互补测试,这次以在对甲苯酸上的生长情况作为评分标准。该分析也确定了四个顺反子。通过含有pPL392或其Tn1000插入衍生物的大肠杆菌微小细胞对这些顺反子的产物进行检测,结果表明该操纵子的前两个顺反子构成一个单一基因xylX,其编码一个57千道尔顿的蛋白质,第三个顺反子xylY编码一个20千道尔顿的蛋白质。

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