Polyunsaturated fatty acyl coenzyme a suppress the glucose-6-phosphatase promoter activity by modulating the DNA binding of hepatocyte nuclear factor 4α

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Abstract

Glucose-6-phosphatase confers on gluconeogenic tissues the capacity to release endogenous glucose in blood. The expression of its gene is modulated by nutritional mechanisms dependent on dietary fatty acids, with specific inhibitory effects of polyunsaturated fatty acids (PUFA). The presence of consensus binding sites of hepatocyte nuclear factor 4 (HNF4) in the -1640/+60 bp region of the rat glucose-6-phosphatase gene has led us to consider the hypothesis that HNF4α could be involved in the regulation of glucose-6-phosphatase gene transcription by long chain fatty acid (LCFA). Our results have shown that the glucose-6-phosphatase promoter activity is specifically inhibited in the presence of PUFA in HepG2 hepatoma cells, whereas saturated LCFA have no effect. In HeLa cells, the glucose-6-phosphatase promoter activity is induced by the co-expression of HNF4α or HNF1α. PUFA repress the promoter activity only in HNF4α-cotransfected HeLa cells, whereas they have no effects on the promoter activity in HNFla-cotransfected HeLa cells. From gel shift mobility assays, deletion, and mutagenesis experiments, two specific binding sequences have been identified that appear able to account for both transactivation by HNF4α and regulation by LCFA in cells. The binding of HNF4α to its cognate sites is specifically inhibited by polyunsaturated fatty acyl coenzyme A in vitro. These data strongly suggest that the mechanism by which PUFA suppress the glucose-6-phosphatase gene transcription involves an inhibition of the binding of HNF4α to its cognate sites in the presence of polyunsaturated fatty acyl-CoA thioesters.

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Rajas, F., Gautier, A., Bady, I., Montano, S., & Mithieux, G. (2002). Polyunsaturated fatty acyl coenzyme a suppress the glucose-6-phosphatase promoter activity by modulating the DNA binding of hepatocyte nuclear factor 4α. Journal of Biological Chemistry, 277(18), 15736–15744. https://doi.org/10.1074/jbc.M200971200

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