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. 2004 Nov;186(21):7196-204.
doi: 10.1128/JB.186.21.7196-7204.2004.

Characterization of the Escherichia coli AaeAB efflux pump: a metabolic relief valve?

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Characterization of the Escherichia coli AaeAB efflux pump: a metabolic relief valve?

Tina K Van Dyk et al. J Bacteriol. 2004 Nov.

"VSports注册入口" Abstract

Treatment of Escherichia coli with p-hydroxybenzoic acid (pHBA) resulted in upregulation of yhcP, encoding a protein of the putative efflux protein family. Also upregulated were the adjacent genes yhcQ, encoding a protein of the membrane fusion protein family, and yhcR, encoding a small protein without a known or suggested function. The function of the upstream, divergently transcribed gene yhcS, encoding a regulatory protein of the LysR family, in regulating expression of yhcRQP was shown. Furthermore, it was demonstrated that several aromatic carboxylic acid compounds serve as inducers of yhcRQP expression. The efflux function encoded by yhcP was proven by the hypersensitivity to pHBA of a yhcP mutant strain. A yhcS mutant strain was also hypersensitive to pHBA. Expression of yhcQ and yhcP was necessary and sufficient for suppression of the pHBA hypersensitivity of the yhcS mutant VSports手机版. Only a few aromatic carboxylic acids of hundreds of diverse compounds tested were defined as substrates of the YhcQP efflux pump. Thus, we propose renaming yhcS, yhcR, yhcQ, and yhcP, to reflect their role in aromatic carboxylic acid efflux, to aaeR, aaeX, aaeA, and aaeB, respectively. The role of pHBA in normal E. coli metabolism and the highly regulated expression of the AaeAB efflux system suggests that the physiological role may be as a "metabolic relief valve" to alleviate toxic effects of imbalanced metabolism. .

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Figures

FIG. 1.
FIG. 1.
Bioluminescent response of three gene fusions to salicylate. A. E. coli strain DPD1675 carrying plasmid pDEW655 with a yhcRQP-luxCDABE gene fusion. B. E. coli strain DPD1675 carrying plasmid pDEW215 with a yciG-luxCDABE gene fusion. C. E. coli strain DPD1675 carrying plasmid pDEW558 with a lysU-luxCDABE gene fusion. Diamonds, no addition. Squares, 0.6 mM sodium salicylate added at zero time. Circles, 5 mM sodium salicylate added at zero time. RLU, relative light units.
FIG. 2.
FIG. 2.
Bioluminescent response of three gene fusions to acetate. A. E. coli strain DPD1675 carrying plasmid pDEW655 with a yhcRQP-luxCDABE gene fusion. B. E. coli strain DPD1675 carrying plasmid pDEW215 with a yciG-luxCDABE gene fusion. C. E. coli strain DPD1675 carrying plasmid pDEW558 with a lysU-luxCDABE gene fusion. Diamonds, no addition. Squares, 80 mM sodium acetate added at zero time. Circles, 160 mM sodium acetate added at zero time. RLU, relative light units.
FIG. 3.
FIG. 3.
Metabolic relief valve model for AaeAB efflux pump expression. A. In normal E. coli cellular metabolism, pHBA is an intermediate in ubiquinone biosynthesis, and its intracellular concentration is likely very low. In this situation, the regulatory gene aaeR is expressed, but the positive regulator is in an inactive form as depicted by the circle. Accordingly, expression of the genes encoding the efflux pump, aaeA and aaeB, which requires the active form of the regulatory protein for expression, is very low. B. In a situation of a metabolic upset when the intracellular concentration of pHBA is abnormally high, the AaeR regulator binds pHBA and is converted to the active form as depicted by the square, thus activating transcription of the efflux pump genes. Expression of the efflux pump proteins thus results in removal of excess pHBA and hence in restoration of cellular homeostasis.

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