Proteasomal degradation of retinoid X receptor α reprograms transcriptional activity of PPARγ in obese mice and humans
Bruno Lefebvre, … , Bart Staels, Philippe Lefebvre
Bruno Lefebvre, … , Bart Staels, Philippe Lefebvre
Published April 1, 2010
Citation Information: J Clin Invest. 2010;120(5):1454-1468. https://doi.org/10.1172/JCI38606.
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Research Article Endocrinology

Proteasomal degradation of retinoid X receptor α reprograms transcriptional activity of PPARγ in obese mice and humans

Abstract

Obese patients have chronic, low-grade inflammation that predisposes to type 2 diabetes and results, in part, from dysregulated visceral white adipose tissue (WAT) functions. The specific signaling pathways underlying WAT dysregulation, however, remain unclear. Here we report that the PPARγ signaling pathway operates differently in the visceral WAT of lean and obese mice. PPARγ in visceral, but not subcutaneous, WAT from obese mice displayed increased sensitivity to activation by its agonist rosiglitazone. This increased sensitivity correlated with increased expression of the gene encoding the ubiquitin hydrolase/ligase ubiquitin carboxyterminal esterase L1 (UCH-L1) and with increased degradation of the PPARγ heterodimerization partner retinoid X receptor α (RXRα), but not RXRβ, in visceral WAT from obese humans and mice. Interestingly, increased UCH-L1 expression and RXRα proteasomal degradation was induced in vitro by conditions mimicking hypoxia, a condition that occurs in obese visceral WAT. Finally, PPARγ-RXRβ heterodimers, but not PPARγ-RXRα complexes, were able to efficiently dismiss the transcriptional corepressor silencing mediator for retinoid and thyroid hormone receptors (SMRT) upon agonist binding. Increasing the RXRα/RXRβ ratio resulted in increased PPARγ responsiveness following agonist stimulation. Thus, the selective proteasomal degradation of RXRα initiated by UCH-L1 upregulation modulates the relative affinity of PPARγ heterodimers for SMRT and their responsiveness to PPARγ agonists, ultimately activating the PPARγ-controlled gene network in visceral WAT of obese animals and humans.

Authors

Bruno Lefebvre, Yacir Benomar, Aurore Guédin, Audrey Langlois, Nathalie Hennuyer, Julie Dumont, Emmanuel Bouchaert, Catherine Dacquet, Luc Pénicaud, Louis Casteilla, Francois Pattou, Alain Ktorza, Bart Staels, Philippe Lefebvre

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Figure 2

RXRα protein, but not mRNA, expression is downregulated in visWAT from obese mice and from obese diabetic patients.

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RXRα protein, but not mRNA, expression is downregulated in visWAT from o...
(A and B) RXR mRNA steady-state levels in mouse WAT. mRNAs from scWAT or visWAT were extracted, and Rxra, Rxrb, and Rxrg cDNAs were quantified by QPCR. (C) RXRα protein (arrowheads) in WAT sections. Original magnification, ×10. (D) RXRα protein in mouse WAT. visWAT and scWAT from OB/OB mice, C57BL/6 mice fed LFD or HFD, or ob/ob mice were probed for their content in RXRα and RXRβ by Western blot analysis. (E and F) Quantification of data in D. The intensity of each RXR band was normalized to actin. The first sample was arbitrarily set to 100%, and each sample was quantified relative to sample 1. Data represent mean ± SEM. ***P < 0.005. (G and H) RXR mRNA steady-state levels in human WAT. mRNAs from scWAT and visWAT were analyzed as in A. LN, lean normoglycemic; ON, obese normoglycemic; OI, obese glucose intolerant; OD, obese diabetic. (I) RXRα, RXRβ, and PPARγ protein levels in human scWAT and visWAT. visWAT from lean or obese diabetic patients was probed for their RXRα, RXRβ, and PPARγ content by Western blot analysis. (JL) Quantification of data in I. The intensity of each RXR or PPARγ band was normalized to β-actin. The first sample was arbitrarily set to 100%, and each sample was quantified relative to sample 1. Data represent mean ± SEM. ***P < 0.005.