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Analysis of GPCR dimerization using acceptor photobleaching resonance energy transfer techniques

Academic Article
Publication Date:
2013
abstract:
The ability of GPCRs to assemble into multimeric complexes is one of the most recently studied and discussed topics for many reasons, including the possibility that GPCR assemblies show a distinct pharmacological profile offering an innovative avenue for the drug synthesis. In addition, the possible differential coupling of monomeric versus multimeric GPCRs to G proteins and other downstream partners, as well as the signaling, the regulation through desensitization and internalization, and the subcellular localization can well represent additional factors that contribute to GPCR-mediated physiopathological states. The standard biochemical techniques used to identify GPCR interactions, such as coimmunoprecipitation, have obvious limitations owing to the use of nonphysiological buffers and detergents that disrupt the natural cell environment and biological interactions and preclude the analysis of subcellular localization and compartmentalization. In the past decade, new biophysical proximity assays based on the resonance energy transfer (RET) between two chromophores allow the study of dimerization in intact living cells, thus proving more information on GPCR physiological roles. In this chapter, we detail the application of two RET techniques based on fluorescence (FRET) and bioluminescence (BRET) to the study of GPCR dimerization and describe the results that can be obtained.
Iris type:
01.01 Articolo in rivista
Keywords:
BRET; FRET; Receptor dimerization; Thromboxane receptor; Oxytocin receptor
List of contributors:
Busnelli, Marta; Chini, Bice
Authors of the University:
BUSNELLI MARTA
CHINI BICE
Handle:
https://iris.cnr.it/handle/20.500.14243/127252
Published in:
METHODS IN ENZYMOLOGY
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