β-Arrestin1 mediates nicotinic acid–induced flushing, but not its antilipolytic effect, in mice
Robert W. Walters, … , Erin J. Whalen, Robert J. Lefkowitz
Robert W. Walters, … , Erin J. Whalen, Robert J. Lefkowitz
Published April 6, 2009
Citation Information: J Clin Invest. 2009;119(5):1312-1321. https://doi.org/10.1172/JCI36806.
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Research Article Cardiology

β-Arrestin1 mediates nicotinic acid–induced flushing, but not its antilipolytic effect, in mice

Abstract

Nicotinic acid is one of the most effective agents for both lowering triglycerides and raising HDL. However, the side effect of cutaneous flushing severely limits patient compliance. As nicotinic acid stimulates the GPCR GPR109A and Gi/Go proteins, here we dissected the roles of G proteins and the adaptor proteins, β-arrestins, in nicotinic acid–induced signaling and physiological responses. In a human cell line–based signaling assay, nicotinic acid stimulation led to pertussis toxin–sensitive lowering of cAMP, recruitment of β-arrestins to the cell membrane, an activating conformational change in β-arrestin, and β-arrestin–dependent signaling to ERK MAPK. In addition, we found that nicotinic acid promoted the binding of β-arrestin1 to activated cytosolic phospholipase A2 as well as β-arrestin1–dependent activation of cytosolic phospholipase A2 and release of arachidonate, the precursor of prostaglandin D2 and the vasodilator responsible for the flushing response. Moreover, β-arrestin1–null mice displayed reduced cutaneous flushing in response to nicotinic acid, although the improvement in serum free fatty acid levels was similar to that observed in wild-type mice. These data suggest that the adverse side effect of cutaneous flushing is mediated by β-arrestin1, but lowering of serum free fatty acid levels is not. Furthermore, G protein–biased ligands that activate GPR109A in a β-arrestin–independent fashion may represent an improved therapeutic option for the treatment of dyslipidemia.

Authors

Robert W. Walters, Arun K. Shukla, Jeffrey J. Kovacs, Jonathan D. Violin, Scott M. DeWire, Christopher M. Lam, J. Ruthie Chen, Michael J. Muehlbauer, Erin J. Whalen, Robert J. Lefkowitz

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Figure 9

MK-0345–induced G protein signaling, β-arrestin conformational changes, and recruitment.

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MK-0345–induced G protein signaling, β-arrestin conformational changes, ...
(A) Cells expressing GPR109A and the ICUE2 biosensor were treated with forskolin and MK-0354 (MK). MK-0354 (open circles) decreased cAMP in a dose-dependent fashion, and this response was inhibited by pertussis toxin (filled circles). (B) Cells expressing GPR109A and the BRET reporter Luc–β-arr–YFP were treated with nicotinic acid (open squares) or MK-0354 (open circles). MK-0354 failed to induce conformational changes in β-arrestin2. Data are mean ± SEM of 3 independent experiments. (C) Cells expressing GPR109A β-arrestin1–mYFP were treated with nicotinic acid, MK-0354, or both. Prior to nicotinic acid stimulation, β-arrestin1 resided in the cytosol; it translocated to bind GPR109A in the membrane in response to 10 μM nicotinic acid. No translocation was noted in cells stimulated with 200 μM MK-0354 or in cells treated with 10 μM nicotinic acid in the presence of 200 μM MK-0354. Images are representative of 4 independent experiments. Original magnification, ×100.