Article ID | Journal | Published Year | Pages | File Type |
---|---|---|---|---|
1993702 | Methods | 2011 | 8 Pages |
Abstract
The biophysical characterization of purified membrane proteins typically requires detergent mediated extraction from native lipid membrane environments. In the case of human G protein-coupled receptors (GPCRs), this process has been complicated by their conformational heterogeneity and the general lack of understanding the composition and interactions within the diverse human cellular membrane environment. Several successful GPCR structure determination efforts have shown that the addition of cholesterol analogs is often critical for maintaining protein stability. We have identified sterols that substantially increase the stability of the NOP receptor (ORL-1), a member of the opioid GPCR family, in a mixed micelle environment. Using dynamic light scattering and small-angle X-ray scattering, we have determined that the most thermal stabilizing sterol, cholesteryl hemisuccinate, induces the formation of a bicelle-like micelle architecture when mixed with dodecyl maltoside detergent. Together with mutagenesis studies and recent GPCR structures, our results provide indications that stabilization is attained through a combination of specific sterol binding to GPCRs and modulation of micelle morphology.
Keywords
IMACβ2ARDPHSf9SAXSLCPβ1ARDLSMβCDGPCRDPPCCHSPDCORL-1CPMDDMCMC1,6-diphenyl-1,3,5-hexatrieneCCmn-dodecyl β-d-maltosideOpioidThermostabilitydipalmitoylphosphatidylcholineRadius of gyrationHydrodynamic radiuscritical micelle concentrationLipidic Cubic Phasetransmembranemethyl-β-cyclodextrinwild typeSmall-angle X-ray scatteringDynamic Light Scatteringimmobilized metal ion affinity chromatographycholesterolcholesterol consensus motifCholesteryl hemisuccinateβ1-Adrenergic receptorβ2-adrenergic receptorOpioid receptorG protein-coupled receptor
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Authors
Aaron A. Thompson, Jeffrey J. Liu, Eugene Chun, Daniel Wacker, Huixian Wu, Vadim Cherezov, Raymond C. Stevens,