Cloning and sequence analysis of a gene (pchR) encoding an AraC family activator of pyochelin and ferripyochelin receptor synthesis in Pseudomonas aeruginosa.

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J Bacteriol. 1993 September; 175(18): 5882-5889

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Cloning and sequence analysis of a gene (pchR) encoding an AraC family activator of pyochelin and ferripyochelin receptor synthesis in Pseudomonas aeruginosa.

D E Heinrichs and K Poole

Department of Microbiology and Immunology, Queen's University, Kingston, Ontario, Canada.

ABSTRACT

Pseudomonas aeruginosa K372 is deficient in the production ofboth the 75-kDa ferripyochelin receptor protein and pyochelin.A 1.8-kb EcoRI-SalI fragment which restored production of boththe receptor protein and pyochelin was cloned. Nucleotide sequencingof the fragment revealed an open reading frame of 888 bp, designatedpchR (pyochelin), capable of encoding a 296-amino-acid proteinof a 32,339-Da molecular mass. By using a phage T7-based expressionsystem, a protein of ca. 32 kDa was produced off the 1.8-kbfragment, confirming that this open reading frame was indeedexpressed. A region exhibiting homology to the consensus Fur-bindingsite of Escherichia coli was identified upstream of the pchRcoding region overlapping a putative promoter. In addition,the C-terminal 80 amino acid residues of PchR showed approximately50% homology (identity, 31%; conserved changes, 19%) to thecarboxy terminus of AraC, a known transcriptional activatorof gene expression in E. coli, Salmonella typhimurium, Citrobacterfreundii, and Erwinia chrysanthemi. Within the C-terminal regionof PchR, AraC, and a number of other members of the AraC familyof transcriptional activators, there exists a highly conserved17-residue domain where, in fact, two residues are strictlymaintained and two others exhibit only conserved changes, suggestinga common functional significance to this region in all of theseproteins. These data are consistent with a role for PchR asa transcriptional activator of pyochelin and ferripyochelinreceptor synthesis in P. aeruginosa. In agreement with this,a PchR mutant obtained by in vitro mutagenesis and gene replacementwas deficient in production of the ferripyochelin receptor andpyochelin.

J Bacteriol. 1993 September; 175(18): 5882-5889

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