Affiliation:
1. Department of Medicine/Infectious Diseases, University of Florida, Gainesville, Florida 32610
2. Department of Pathobiological Sciences, School of Veterinary Medicine, University of Wisconsin-Madison, Madison, Wisconsin 53706
Abstract
ABSTRACT
The flagellar transcriptional regulator FleQ appears to be the highest-level regulator in the hierarchical regulatory cascade of flagellar biogenesis in
Pseudomonas aeruginosa
. Except for the posttranslational downregulation of FleQ activity by FleN, an antiactivator, not much is known about the regulation of the
fleQ
gene or its gene product. Some FleQ homologs in other bacterial species either are positively regulated by another regulator (e.g., CtrA, the master regulator regulating FlbD in
Caulobacter crescentus
) or are expressed from a σ
70
-dependent promoter (e.g., FlgR of
Helicobacter pylori
). In this study we demonstrated that Vfr, an
Escherichia coli
CRP homolog known to function as an activator for various genes, including
lasR
,
regA
, and
toxA
, in
P. aeruginosa
, is capable of repressing
fleQ
transcription by binding to its consensus sequence in the
fleQ
promoter. In a DNase I footprint assay, purified Vfr protected the sequence 5′-AATTGACTAATCGTTCACATTTG-3′. When this putative Vfr binding site in the
fleQ
promoter was mutated, Vfr was unable to bind the
fleQ
promoter fragment and did not repress
fleQ
transcription effectively. Primer extension analysis of the
fleQ
transcript revealed two transcriptional start sites, t1 and t2, that map within the Vfr binding site. A putative −10 region (TAAAAT) for the t2 transcript, with a five-of-six match with the
E. coli
σ
70
binding consensus, overlaps with one end of the Vfr binding site. A 4-bp mutation and an 8-bp mutation in this −10 region markedly reduced the activity of the
fleQ
promoter. The same mutations led to the disappearance of the 203-nucleotide
fleQ
transcript in an in vitro transcription assay. Vfr probably represses
fleQ
transcription by binding to the Vfr binding site in the
fleQ
promoter and preventing the sigma factor from binding to the −10 region to initiate transcription.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
Cited by
105 articles.
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