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J. Bacteriol. doi:10.1128/JB.00767-08
Copyright (c) 2008, American Society for Microbiology and/or the Listed Authors/Institutions. All Rights Reserved.

Glucose and glucokinase-controlled mal gene expression in Escherichia coli

Department of Biology, University of Konstanz, 78457 Konstanz, Germany

^* To whom correspondence should be addressed. Email: winfried.boos{at}uni-konstanz.de.

	Abstract

MalT is the central transcriptional activator of all mal genes in Escherichia coli. Its activity is controlled by the inducer maltotriose. It can be inhibited by the interaction with certain proteins and its expression can be controlled. Here we report a novel aspect of mal gene regulation: the effect of cytoplasmic glucose and glucokinase (Glk) on the activity and the expression of MalT. Amylomaltase (MalQ) is essential for the metabolism of maltose. It forms maltodextrins and glucose from maltose or maltodextrins. We found that glucose above a concentration of 0.1 mM blocked the activity of the enzyme. malQ mutants when grown in the absence of maltodextrins are endogenously induced by maltotriose that is derived from the degradation of glycogen. Therefore, the fact that glk malQ⁺ mutants showed elevated mal gene expression finds its explanation in the reduced ability to remove glucose from MalQ-catalyzed maltodextrin formation and is caused by a metabolically induced MalQ^- phenotype. However, even in mutants lacking glycogen glucokinase controls endogenous induction. We found that overexpressed glucokinase due to its structural similarity with Mlc, the repressor of malT, binds to the glucose transporter (PtsG) releasing Mlc thus increasing malT repression. In addition, even in mutants lacking Mlc (and glycogen) the overexpression of glk leads to a reduction in mal gene expression. We interpret this repression by a direct interaction of GlK with MalT concomitant with MalT inhibition. This repression was dependent on the presence of either maltodextrin phosphorylase or amylomaltase and led to the inactivation of MalT.