Molecular characterization of the Entner-Doudoroff pathway in Escherichia coli: sequence analysis and localization of promoters for the edd-eda operon.

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J Bacteriol. 1992 July; 174(14): 4638-4646

research-article

Molecular characterization of the Entner-Doudoroff pathway in Escherichia coli: sequence analysis and localization of promoters for the edd-eda operon.

S E Egan, R Fliege, S Tong, A Shibata, R E Wolf Jr and T Conway

School of Biological Sciences, University of Nebraska, Lincoln 68588-0118.

ABSTRACT

The nucleotide sequence of the entire Escherichia coli edd-edaregion that encodes the enzymes of the Entner-Doudoroff pathwaywas determined. The edd structural gene begins 236 bases downstreamof zwf. The eda structural gene begins 34 bases downstream ofedd. The edd reading frame is 1,809 bases long and encodes the602-amino-acid, 64,446-Da protein 6-phosphogluconate dehydratase.The deduced primary amino acid sequences of the E. coli andZymomonas mobilis dehydratase enzymes are highly conserved.The eda reading frame is 642 bases long and encodes the 213-amino-acid,22,283-Da protein 2-keto-3-deoxy-6-phosphogluconate aldolase.This enzyme had been previously purified and sequenced by otherson the basis of its related enzyme activity, 2-keto-4-hydroxyglutaratealdolase. The data presented here provide proof that the twoenzymes are identical. The primary amino acid sequences of theE. coli, Z. mobilis, and Pseudomonas putida aldolase enzymesare highly conserved. When E. coli is grown on gluconate, theedd and eda genes are cotranscribed. Four putative promoterswithin the edd-eda region were identified by transcript mappingand computer analysis. P1, located upstream of edd, appearsto be the primary gluconate-responsive promoter of the edd-edaoperon, responsible for induction of the Entner-Doudoroff pathway,as mediated by the gntR product. High basal expression of edais explained by constitutive transcription from P2, P3, and/orP4 but not P1.

J Bacteriol. 1992 July; 174(14): 4638-4646

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