Nucleotide sequencing and transcriptional mapping of the genes encoding biphenyl dioxygenase, a multicomponent polychlorinated-biphenyl-degrading enzyme in Pseudomonas strain LB400.

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J Bacteriol. 1992 May; 174(9): 2903-2912

research-article

Nucleotide sequencing and transcriptional mapping of the genes encoding biphenyl dioxygenase, a multicomponent polychlorinated-biphenyl-degrading enzyme in Pseudomonas strain LB400.

B D Erickson and F J Mondello

Bioremediation Laboratory, General Electric Co., Schenectady, New York 12301.

ABSTRACT

The DNA region encoding biphenyl dioxygenase, the first enzymein the biphenyl-polychlorinated biphenyl degradation pathwayof Pseudomonas species strain LB400, was sequenced. Six openreading frames were identified, four of which are homologousto the components of toluene dioxygenase from Pseudomonas putidaF1 and have been named bphA, bphE, bphF, and bphG. From thiscomparison, biphenyl dioxygenase was found to be a multicomponentenzyme containing a two-subunit iron-sulfur protein, a ferredoxin,and a reductase. Comparison of the large subunit of the iron-sulfurprotein and the ferredoxin with other multicomponent dioxygenasesidentified amino acid sequences similar to Rieske iron-sulfurproteins for binding a [2Fe-2S] cluster. Sequences have alsobeen identified in the reductase component that match the consensussequence for FAD or NAD binding. Transcription of the biphenyldioxygenase region was examined, and three transcription initiationsites were identified. Transcription initiating at the sitefurthest upstream is greatly increased when the LB400 cellsare grown on biphenyl as the sole carbon source.

J Bacteriol. 1992 May; 174(9): 2903-2912

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