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catBCA启动子的激活:通过体外转录探究CatR与RNA聚合酶的相互作用。

Activation of the catBCA promoter: probing the interaction of CatR and RNA polymerase through in vitro transcription.

作者信息

Chugani S A, Parsek M R, Hershberger C D, Murakami K, Ishihama A, Chakrabarty A M

机构信息

Department of Microbiology and Immunology, University of Illinois College of Medicine, Chicago 60612, USA.

出版信息

J Bacteriol. 1997 Apr;179(7):2221-7. doi: 10.1128/jb.179.7.2221-2227.1997.

Abstract

The soil bacterium Pseudomonas putida is capable of degrading many aromatic compounds, including benzoate, through catechol as an intermediate. The catabolism of catechol is mediated by the catBCA operon, whose induction requires the pathway intermediate cis,cis-muconate as an inducer and the regulatory protein, CatR. CatR also regulates the plasmid-borne pheBA operon of P. putida PaW85, which is involved in phenol catabolism. We have used an in vitro transcription system to study the roles of CatR, cis,cis-muconate, Escherichia coli RNA polymerase, and promoter sequences in expression of the cat and phe operons. The assay confirmed the requirement of both CatR and cis,cis-muconate for transcript formation. We also examined the in vitro transcription of three site-directed mutants of the catBCA promoter; the results obtained compared favorably with previous in vivo data. The requirement of the alpha subunit of RNA polymerase for expression of the catBCA and the pheBA transcripts was also examined. The C-terminal region of the alpha subunit of RNA polymerase has been implicated in direct protein-protein contact with transcriptional regulatory proteins and/or direct contact with the DNA. We show that the carboxyl terminus of the alpha subunit is required for the expression of the catBCA and the pheBA operons because RNA polymerases with truncated alpha subunits were deficient in activation. Further experiments demonstrated the arginine at position 265 and the asparagine at position 268 of the alpha subunit as possible amino acids involved in activation. On the basis of these and previous results, we propose a model to explain the interaction of the different regulatory components leading to CatR-dependent activation of the catBCA operon.

摘要

土壤细菌恶臭假单胞菌能够通过儿茶酚作为中间体来降解许多芳香族化合物,包括苯甲酸盐。儿茶酚的分解代谢由catBCA操纵子介导,其诱导需要途径中间体顺,顺-粘康酸作为诱导剂以及调节蛋白CatR。CatR还调节恶臭假单胞菌PaW85的质粒携带的pheBA操纵子,该操纵子参与苯酚的分解代谢。我们使用了体外转录系统来研究CatR、顺,顺-粘康酸、大肠杆菌RNA聚合酶和启动子序列在cat和phe操纵子表达中的作用。该测定证实了CatR和顺,顺-粘康酸对于转录物形成的必要性。我们还检查了catBCA启动子的三个定点突变体的体外转录;所获得的结果与先前的体内数据相比良好。还研究了RNA聚合酶α亚基对catBCA和pheBA转录物表达的必要性。RNA聚合酶α亚基的C末端区域与转录调节蛋白的直接蛋白质-蛋白质接触和/或与DNA的直接接触有关。我们表明,α亚基的羧基末端是catBCA和pheBA操纵子表达所必需的,因为具有截短α亚基的RNA聚合酶在激活方面存在缺陷。进一步的实验证明,α亚基第265位的精氨酸和第268位的天冬酰胺可能是参与激活的氨基酸。基于这些以及先前的结果,我们提出了一个模型来解释不同调节成分之间的相互作用,这种相互作用导致catBCA操纵子的CatR依赖性激活。

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