Characterization of the regulon controlled by the leucine-responsive regulatory protein in Escherichia coli.

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J Bacteriol. 1992 February; 174(4): 1109-1118

research-article

Characterization of the regulon controlled by the leucine-responsive regulatory protein in Escherichia coli.

B R Ernsting, M R Atkinson, A J Ninfa and R G Matthews

Biophysics Research Division, University of Michigan, Ann Arbor 48109.

ABSTRACT

The leucine-responsive regulatory protein (Lrp) has been shownto regulate, either positively or negatively, the transcriptionof several Escherichia coli genes in response to leucine. Wehave used two-dimensional gel electrophoresis to analyze thepatterns of polypeptide expression in isogenic lrp+ and lrpmutant strains in the presence or absence of leucine. The absenceof a functional Lrp protein alters the expression of at least30 polypeptides. The expression of the majority of these polypeptidesis not affected by the presence or absence of 10 mM exogenousleucine. Outer membrane porins OmpC and OmpF, glutamine synthetase(GlnA), the small subunit of glutamate synthase (GltD), lysyl-tRNAsynthetase form II (LysU), a high-affinity periplasmic bindingprotein specific for branched-chain amino acids (LivJ), W protein,and the enzymes of the pathway converting threonine to glycine,namely, threonine dehydrogenase (Tdh) and 2-amino-3-ketobutyratecoenzyme A ligase (Kbl), were identified as members of the Lrpregulon by electrophoretic analysis. We have shown that Lrpis a positive regulator of glutamate synthase and glutaminesynthetase and that exogenous leucine has little or no effecton the expression of these proteins. In strains carrying a glnLdeletion and in strains carrying the glnL2302 allele, whichdirects the synthesis of a GlnL protein that is constitutivelyactive, expression of glutamine synthetase is no longer regulatedby Lrp, demonstrating that the effect of Lrp on glutamine synthetaselevels is indirect and requires an intact glnL gene. lrp::Tn10strains grow poorly when arginine or ornithine is present asthe sole nitrogen source in the medium. On the bases of presentstudies and previous research, we propose that Lrp is involvedin the adaptation of E. coli cells to major shifts in environment,such as those which occur when E. coli leaves the intestinaltract of its animal host. Several genes required for amino acidand peptide transport and catabolism are negatively regulatedby Lrp, and other genes required for amino acid biosynthesisand ammonia assimilation in a nitrogen-poor environment arepositively regulated by Lrp.

J Bacteriol. 1992 February; 174(4): 1109-1118

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