Farnesoid X receptor is essential for normal glucose homeostasis
Ke Ma, … , Lawrence Chan, David D. Moore
Ke Ma, … , Lawrence Chan, David D. Moore
Published April 3, 2006
Citation Information: J Clin Invest. 2006;116(4):1102-1109. https://doi.org/10.1172/JCI25604.
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Research Article Endocrinology

Farnesoid X receptor is essential for normal glucose homeostasis

Abstract

The bile acid receptor farnesoid X receptor (FXR; NR1H4) is a central regulator of bile acid and lipid metabolism. We show here that FXR plays a key regulatory role in glucose homeostasis. FXR-null mice developed severe fatty liver and elevated circulating FFAs, which was associated with elevated serum glucose and impaired glucose and insulin tolerance. Their insulin resistance was confirmed by the hyperinsulinemic euglycemic clamp, which showed attenuated inhibition of hepatic glucose production by insulin and reduced peripheral glucose disposal. In FXR–/– skeletal muscle and liver, multiple steps in the insulin signaling pathway were markedly blunted. In skeletal muscle, which does not express FXR, triglyceride and FFA levels were increased, and we propose that their inhibitory effects account for insulin resistance in that tissue. In contrast to the results in FXR–/– mice, bile acid activation of FXR in WT mice repressed expression of gluconeogenic genes and decreased serum glucose. The absence of this repression in both FXR–/– and small heterodimer partner–null (SHP–/–) mice demonstrated that the previously described FXR-SHP nuclear receptor cascade also targets glucose metabolism. Taken together, our results identify a link between lipid and glucose metabolism mediated by the FXR-SHP cascade.

Authors

Ke Ma, Pradip K. Saha, Lawrence Chan, David D. Moore

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Figure 5

Impaired hepatic insulin signaling and expression of fatty acid metabolism and gluconeogenesis in the livers of FXR–/– mice.

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Impaired hepatic insulin signaling and expression of fatty acid metaboli...
Liver tissue homogenates from 4–5 mice per group were pooled together and subjected to IP and IB using antibodies as indicated. Northern blot analysis was performed on individual mice. Results are representative of — and quantitation was derived from — at least 3 independent experiments. (A) Phosphorylation of IR after insulin stimulation (1U/kg). Liver homogenates were subjected to IP by anti-phosphotyrosine antibody 4G10 and IB by IR antibody. Total IR level was analyzed by IP followed by IB using the IR antibody. Quantitation was derived from 3 independent experiments. (B) PI3K-associated IRS-2 level. (C) PI3K activity assay using immunopricipitates by anti-phosphotyrosine antibody. Liver homogenates from individual mice were subjected to IP by anti-phosphotyrosine antibody followed by PI3K assay. Quantitation was derived from individual mice. (D) Hepatic expression of genes involved in fatty acid transport and oxidation. L-FABP, liver type FFA–binding protein. (E) Hepatic expression of genes involved in gluconeogenesis. **P < 0.01.