NosR, a membrane-bound regulatory component necessary for expression of nitrous oxide reductase in denitrifying Pseudomonas stutzeri.

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J Bacteriol. 1992 August; 174(16): 5332-5339

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NosR, a membrane-bound regulatory component necessary for expression of nitrous oxide reductase in denitrifying Pseudomonas stutzeri.

H Cuypers, A Viebrock-Sambale and W G Zumft

Lehrstuhl für Mikrobiologie, Universität Karlsruhe, Germany.

ABSTRACT

The regulatory element NosR was identified within the nos regionof the denitrification gene cluster of Pseudomonas stutzeriZoBell (ATCC 14405) and characterized. It is essential for expressionof the N2O reductase encoded by nosZ immediately downstreamof nosR. The nosR region was initially identified by Tn5 mutagenesis(W. G. Zumft, K. Döhler, and H. Körner, J. Bacteriol.163:918-924, 1985). It consists of a single open reading frameof 2,172 nucleotides and has the coding capacity for an 81.9-kDaprotein. The codon usage for nosR, with its high G + C contentof 62.4 mol% and a preference for G or C at the third position,is characteristic for a Pseudomonas gene. Hydropathy analysisclassified NosR as an integral membrane protein with at leastseven membrane-spanning segments. No similarity to known bacterialregulator proteins was found in a data bank search. However,the C terminus of NosR shows sequence similarity to the cysteineclusters of several 2[4Fe-4S] bacterial ferrodoxins. A monocistronicmRNA for nosZ which allowed us to monitor NosR function wasidentified. Complementation of Nos- mutant MK418 (nosR::Tn5)with the nosR gene supplied in trans restored nosZ transcriptionand expression of a catalytically active N2O reductase. In additionto evidence of the requirement for NosR, indirect evidence forinvolvement of the transcriptional regulator Fnr is presented.

J Bacteriol. 1992 August; 174(16): 5332-5339

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