In Vivo Visualization of Delta Opioid Receptors Upon Physiological Activation Uncovers a Distinct Internalization Profile

Lauren Faget, Eric Erbs, Julie Le Merrer, Gregory Scherrer, Audrey Matifas, Nadia Benturquia, Florence Noble, Marion Decossas, Marc Koch, Pascal Kessler, Jean-Luc Vonesch, Yannick Schwab, Brigitte L. Kieffer, Dominique Massotte

Research output: Contribution to journalArticlepeer-review

39 Scopus citations

Abstract

G-protein-coupled receptors (GPCRs) mediate numerous physiological functions and represent prime therapeutic targets. Receptor trafficking upon agonist stimulation is critical for GPCR function, but examining this process in vivo remains a true challenge. Using knock-in mice expressing functional fluorescent delta opioid receptors under the control of the endogenous promoter, we visualized in vivo internalization of this native GPCR upon physiological stimulation. We developed a paradigm in which animals were made dependent on morphine in a drug-paired context. When re-exposed to this context in a drug-free state, mice showed context-dependent withdrawal signs and activation of the hippocampus. Receptor internalization was transiently detected in a subset of CA1 neurons, uncovering regionally restricted opioid peptide release. Importantly, a pool of surface receptors always remained, which contrasts with the in vivo profile previously established for exogenous drug-induced internalization. Therefore, a distinct response is observed at the receptor level upon a physiological or pharmacological stimulation. Altogether, direct in vivo GPCR visualization enables mapping receptor stimulation promoted by a behavioral challenge and represents a powerful approach to study endogenous GPCR physiology.
Original languageAmerican English
JournalJournal of Neuroscience
Volume32
Issue number21
DOIs
StatePublished - 23 May 2012
Externally publishedYes

EGS Disciplines

  • Biology

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