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恶臭假单胞菌HS12中硝基苯分解代谢质粒pNB1和pNB2的鉴定与特性分析

Identification and characterization of the nitrobenzene catabolic plasmids pNB1 and pNB2 in Pseudomonas putida HS12.

作者信息

Park H S, Kim H S

机构信息

Department of Biological Sciences, Korea Advanced Institute of Science and Technology, 373-1, Kusung-dong, Yusong-gu, Taejon 305-701, Korea.

出版信息

J Bacteriol. 2000 Feb;182(3):573-80. doi: 10.1128/JB.182.3.573-580.2000.

Abstract

Pseudomonas putida HS12, which is able to grow on nitrobenzene, was found to carry two plasmids, pNB1 and pNB2. The activity assay experiments of wild-type HS12(pNB1 and pNB2), a spontaneous mutant HS121(pNB2), and a cured derivative HS124(pNB1) demonstrated that the catabolic genes coding for the nitrobenzene-degrading enzymes, designated nbz, are located on two plasmids, pNB1 and pNB2. The genes nbzA, nbzC, nbzD, and nbzE, encoding nitrobenzene nitroreductase, 2-aminophenol 1,6-dioxygenase, 2-aminomuconic 6-semialdehyde dehydrogenase, and 2-aminomuconate deaminase, respectively, are located on pNB1 (59.1 kb). Meanwhile, the nbzB gene encoding hydroxylaminobenzene mutase, a second-step enzyme in the nitrobenzene catabolic pathway, was found in pNB2 (43.8 kb). Physical mapping, cloning, and functional analysis of the two plasmids and their subclones in Escherichia coli strains revealed in more detail the genetic organization of the catabolic plasmids pNB1 and pNB2. The genes nbzA and nbzB are located on the 1.1-kb SmaI-SnaBI fragment of pNB1 and the 1.0-kb SspI-SphI fragment of pNB2, respectively, and their expressions were not tightly regulated. On the other hand, the genes nbzC, nbzD, and nbzE, involved in the ring cleavage pathway of 2-aminophenol, are localized on the 6.6-kb SnaBI-SmaI fragment of pNB1 and clustered in the order nbzC-nbzD-nbzE as an operon. The nbzCDE genes, which are transcribed in the opposite direction of the nbzA gene, are coordinately regulated by both nitrobenzene and a positive transcriptional regulator that seems to be encoded on pNB2.

摘要

恶臭假单胞菌HS12能够在硝基苯上生长,被发现携带两个质粒,即pNB1和pNB2。野生型HS12(pNB1和pNB2)、自发突变体HS121(pNB2)和治愈衍生物HS124(pNB1)的活性测定实验表明,编码硝基苯降解酶的分解代谢基因(命名为nbz)位于两个质粒pNB1和pNB2上。分别编码硝基苯硝基还原酶、2-氨基苯酚1,6-双加氧酶、2-氨基粘康酸6-半醛脱氢酶和2-氨基粘康酸脱氨酶的基因nbzA、nbzC、nbzD和nbzE位于pNB1(59.1 kb)上。同时,在pNB2(43.8 kb)中发现了编码羟基氨基苯变位酶的nbzB基因,它是硝基苯分解代谢途径中的第二步酶。对这两个质粒及其在大肠杆菌菌株中的亚克隆进行物理图谱分析、克隆和功能分析,更详细地揭示了分解代谢质粒pNB1和pNB2的遗传组织。基因nbzA和nbzB分别位于pNB1的1.1 kb SmaI-SnaBI片段和pNB2的1.0 kb SspI-SphI片段上,它们的表达不受严格调控。另一方面,参与2-氨基苯酚环裂解途径的基因nbzC、nbzD和nbzE位于pNB1的6.6 kb SnaBI-SmaI片段上,并作为一个操纵子按nbzC-nbzD-nbzE的顺序聚集。nbzCDE基因与nbzA基因转录方向相反,受硝基苯和一个似乎由pNB2编码的正转录调节因子共同调控。

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