J Bacteriol. 1993 Sep;175(17):5585-94.

Sequencing and characterization of a gene cluster encoding the enzymes for L-rhamnose metabolism in Escherichia coli.

Moralejo P, Egan SM, Hidalgo E, Aguilar J.

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Department of Biochemistry, School of Pharmacy, University of Barcelona, Spain.

Abstract

The sequencing of the EcoRI-HindIII fragment complementing mutations in the structural genes of the L-rhamnose regulon of Escherichia coli has permitted identification of the open reading frames corresponding to rhaB, rhaA, and rhaD. The deduced amino acid sequences gave a 425-amino-acid polypeptide corresponding to rhamnulose kinase for rhaB, a 400-amino-acid polypeptide corresponding to rhamnose isomerase for rhaA, and a 274-amino-acid polypeptide corresponding to rhamnulose-1-phosphate aldolase for rhaD. Transcriptional fusions of the three putative promoter regions to lacZ showed that only the rhaB leader region acted as a promoter, as indicated by the high beta-galactosidase activity induced by rhamnose, while no significant activity from the rhaA and rhaD constructions was detected. The rhaB transcription start site was mapped to -24 relative to the start of translation. Mutations in the catabolic genes were used to show that L-rhamnose may directly induce rhaBAD transcription.

PMID:: 8396120; [PubMed - indexed for MEDLINE]
PMCID:: PMC206615

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Cited by 18 PubMed Central articles

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Structures reported by this article

L-Rhamnulose-1-Phosphate Aldolase From Escherichia Coli (Mutant E192a)

PDB: 1OJR

Source: Escherichia coli

Method: X-Ray Diffraction

Resolution: 1.35 Å

See all 2 structures...

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Sequencing and characterization of a gene cluster encoding the enzymes for L-rhamnose metabolism in Escherichia coli.
J Bacteriol. 1993 Sep ;175(17):5585-94.

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