Identification and cloning of a fur homolog from Neisseria gonorrhoeae.

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Infect Immun. 1993 November; 61(11): 4599-4606

Identification and cloning of a fur homolog from Neisseria gonorrhoeae.

S A Berish, S Subbarao, C Y Chen, D L Trees and S A Morse

Division of Sexually Transmitted Diseases Laboratory Research, Centers for Disease Control and Prevention, Atlanta, Georgia 30333.

ABSTRACT

The promoter region of the major iron-regulated protein of Neisseriagonorrhoeae, Fbp, has two regions that exhibit homology withthe Escherichia coli consensus Fur-binding sequences. Gel retardationassays suggested that purified E. coli Fur bound to two siteswithin the Fbp promoter. The presence of a gonococcal Fur homologwas suggested by Southern hybridization under conditions oflow stringency, which revealed a DNA locus that exhibited homologyto the E. coli fur gene. Oligonucleotides derived from the conservedregions of fur genes of extremely diverse bacteria were usedto amplify a 140-bp fragment of a putative gonococcal fur gene.This fragment was used to identify clones containing the entiregonococcal fur gene. After sequencing the gonococcal fur geneand its promoter region, we found that gonococcal Fur exhibited50% identity with E. coli Fur at the amino acid level; however,it complemented two E. coli Fur- mutants. The presence of aFur homolog in N. gonorrhoeae suggests that Fur-regulated genesare widely distributed among extremely diverse bacteria.

Infect Immun. 1993 November; 61(11): 4599-4606

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