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恶臭假单胞菌P111因基因改变导致氯苯甲酸分解代谢的变化。

Variation in chlorobenzoate catabolism by Pseudomonas putida P111 as a consequence of genetic alterations.

作者信息

Brenner V, Hernandez B S, Focht D D

机构信息

Department of Soil and Environmental Sciences, University of California, Riverside 92521.

出版信息

Appl Environ Microbiol. 1993 Sep;59(9):2790-4. doi: 10.1128/aem.59.9.2790-2794.1993.

Abstract

Pseudomonas putida P111 is able to utilize a broad range of monochlorinated, dichlorinated, and trichlorinated benzoates. The involvement of two separate dioxygenases was noted from data on plasmid profiles and DNA hybridization. The benzoate dioxygenase, which converts 3-chlorobenzoate (3-CB), 4-CB, and benzoate to the corresponding catechols via reduction of a dihydrodiol, was shown to be chromosomally coded. The chlorobenzoate-1,2-dioxygenase that converts ortho-chlorobenzoates to the corresponding catechols without the need of a functional dioldehydrogenase was shown to be encoded on plasmid pPB111 (75 kb). Cured strains were unable to utilize ortho-chlorobenzoates for growth. DNA hybridization data indicated that catabolism of the corresponding chlorocatechols was coded on chromosomal genes. Maintenance of plasmid pPB111 was dependent on the presence of ortho-chlorobenzoates in the growth media. A unique variant of P111 (P111D), able to grow on 3,5-dichlorobenzoate (3,5-DCB), was obtained by continuous subculturing from media containing progressively lower and higher concentrations of 3-CB and 3,5-DCB, respectively. The low frequency of segregants able to grow on 2,5-DCB, 2,3-DCB, and 2,3, 5-trichlorobenzoate was evident by lag periods greater than 200 h. Continued subculture on 3,5-DCB resulted in the formation of new plasmid pPH111 (120 kb), which was homologous to pPB111. A probe from the clc operon, which encodes for the chlorocatechol pathway, hybridized to plasmid pPH111 and to the chromosome of the wild-type strain P111 but not to its plasmid pPB111 nor to the chromosome of strain P111A, which had lost the ability to utilize chlorobenzoates.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

恶臭假单胞菌P111能够利用多种一氯代、二氯代和三氯代苯甲酸酯。从质粒图谱和DNA杂交数据中发现有两种不同的双加氧酶参与其中。将3-氯苯甲酸酯(3-CB)、4-CB和苯甲酸酯通过二氢二醇还原转化为相应儿茶酚的苯甲酸双加氧酶被证明是由染色体编码的。将邻氯苯甲酸酯转化为相应儿茶酚而无需功能性二醇脱氢酶的氯苯甲酸-1,2-双加氧酶被证明是由质粒pPB111(75 kb)编码的。治愈菌株无法利用邻氯苯甲酸酯进行生长。DNA杂交数据表明,相应氯代儿茶酚的分解代谢是由染色体基因编码的。质粒pPB111的维持依赖于生长培养基中邻氯苯甲酸酯的存在。通过分别从含有浓度逐渐降低和升高的3-CB和3,5-DCB的培养基中连续传代培养,获得了一种能够在3,5-二氯苯甲酸酯(3,5-DCB)上生长的P111独特变体(P111D)。能够在2,5-DCB、2,3-DCB和2,3,5-三氯苯甲酸酯上生长的分离子频率较低,这通过大于200小时的延迟期明显体现出来。在3,5-DCB上继续传代培养导致形成了与pPB111同源的新质粒pPH111(120 kb)。来自编码氯代儿茶酚途径的clc操纵子的探针与质粒pPH111以及野生型菌株P111的染色体杂交,但不与其质粒pPB111杂交,也不与已失去利用氯苯甲酸酯能力的菌株P111A的染色体杂交。(摘要截断于250字)

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2cea/182367/197b413e6556/aem00038-0038-b.jpg

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