| Literature DB >> 32457152 |
Jade Degrandmaison1,2,3,4,5, Khaled Abdallah2,3,4, Véronique Blais2,3,4, Samuel Génier1,3,4, Marie-Pier Lalumière1,3,4, Francis Bergeron2,3,4,5, Catherine M Cahill6,7,8, Jim Boulter6,7,8, Christine L Lavoie2,3,4,9, Jean-Luc Parent10,3,4,9, Louis Gendron11,3,4,9,12,13.
Abstract
With over 30% of current medications targeting this family of proteins, G-protein-coupled receptors (GPCRs) remain invaluable therapeutic targets. However, due to their unique physicochemical properties, their low abundance, and the lack of highly specific antibodies, GPCRs are still challenging to study in vivo. To overcome these limitations, we combined here transgenic mouse models and proteomic analyses in order to resolve the interactome of the δ-opioid receptor (DOPr) in its native in vivo environment. Given its analgesic properties and milder undesired effects than most clinically prescribed opioids, DOPr is a promising alternative therapeutic target for chronic pain management. However, the molecular and cellular mechanisms regulating its signaling and trafficking remain poorly characterized. We thus performed liquid chromatography-tandem mass spectrometry (LC-MS/MS) analyses on brain homogenates of our newly generated knockin mouse expressing a FLAG-tagged version of DOPr and revealed several endogenous DOPr interactors involved in protein folding, trafficking, and signal transduction. The interactions with a few identified partners such as VPS41, ARF6, Rabaptin-5, and Rab10 were validated. We report an approach to characterize in vivo interacting proteins of GPCRs, the largest family of membrane receptors with crucial implications in virtually all physiological systems.Entities:
Keywords: G-protein–coupled receptors; GPCR interactome; mass spectrometry; mouse model; δ-opioid receptor
Year: 2020 PMID: 32457152 PMCID: PMC7293596 DOI: 10.1073/pnas.1917906117
Source DB: PubMed Journal: Proc Natl Acad Sci U S A ISSN: 0027-8424 Impact factor: 11.205