TY - JOUR
T1 - A Discrete Presynaptic Vesicle Cycle for Neuromodulator Receptors
AU - Jullié, Damien
AU - Stoeber, Miriam
AU - Sibarita, Jean Baptiste
AU - Zieger, Hanna L.
AU - Bartol, Thomas M.
AU - Arttamangkul, Seksiri
AU - Sejnowski, Terrence J.
AU - Hosy, Eric
AU - von Zastrow, Mark
N1 - Funding Information:
We thank Robert Edwards and members of his laboratory for discussions and reagents, David Perrais for valuable discussions and technical advice, and Stefan Schulz for valuable discussions and important reagents. We thank Roger Nicoll, Tim Ryan, John Williams, Gregory Scherrer, and members of the von Zastrow laboratory for valuable discussions and suggestions. Some of the imaging experiments were carried out in the UCSF Nikon Imaging Center directed by DeLaine Larsen. This study was supported by research grants from the NIH / NIDA ( DA010711 and DA012864 ). M.S. was supported by the Swiss National Science Foundation ( P2EZP3_152173 and P300PA_164712 ). D.J. received support from the UCSF Program for Breakthrough Biomedical Research . S.A. received support from NIH / NIDA DA048136 .
Funding Information:
We thank Robert Edwards and members of his laboratory for discussions and reagents, David Perrais for valuable discussions and technical advice, and Stefan Schulz for valuable discussions and important reagents. We thank Roger Nicoll, Tim Ryan, John Williams, Gregory Scherrer, and members of the von Zastrow laboratory for valuable discussions and suggestions. Some of the imaging experiments were carried out in the UCSF Nikon Imaging Center directed by DeLaine Larsen. This study was supported by research grants from the NIH/NIDA (DA010711 and DA012864). M.S. was supported by the Swiss National Science Foundation (P2EZP3_152173 and P300PA_164712). D.J. received support from the UCSF Program for Breakthrough Biomedical Research. S.A. received support from NIH/ NIDA DA048136. D.J. and M.v.Z. conceived the experiments and wrote the manuscript. D.J. H.L.Z. and E.H. performed the experiments and analyzed the data. M.S. and S.A. provided essential reagents. J.-B.S. T.M.B. and T.J.S. provided software and support for data analysis and interpretation. The authors declare no competing interests.
Publisher Copyright:
© 2019 Elsevier Inc.
PY - 2020/2/19
Y1 - 2020/2/19
N2 - A major function of GPCRs is to inhibit presynaptic neurotransmitter release, requiring ligand-activated receptors to couple locally to effectors at terminals. The current understanding of how this is achieved is through receptor immobilization on the terminal surface. Here, we show that opioid peptide receptors, GPCRs that mediate highly sensitive presynaptic inhibition, are instead dynamic in axons. Opioid receptors diffuse rapidly throughout the axon surface and internalize after ligand-induced activation specifically at presynaptic terminals. We delineate a parallel regulated endocytic cycle for GPCRs operating at the presynapse, separately from the synaptic vesicle cycle, which clears activated receptors from the surface of terminals and locally reinserts them to maintain the diffusible surface pool. We propose an alternate strategy for achieving local control of presynaptic effectors that, opposite to using receptor immobilization and enforced proximity, is based on lateral mobility of receptors and leverages the inherent allostery of GPCR-effector coupling.
AB - A major function of GPCRs is to inhibit presynaptic neurotransmitter release, requiring ligand-activated receptors to couple locally to effectors at terminals. The current understanding of how this is achieved is through receptor immobilization on the terminal surface. Here, we show that opioid peptide receptors, GPCRs that mediate highly sensitive presynaptic inhibition, are instead dynamic in axons. Opioid receptors diffuse rapidly throughout the axon surface and internalize after ligand-induced activation specifically at presynaptic terminals. We delineate a parallel regulated endocytic cycle for GPCRs operating at the presynapse, separately from the synaptic vesicle cycle, which clears activated receptors from the surface of terminals and locally reinserts them to maintain the diffusible surface pool. We propose an alternate strategy for achieving local control of presynaptic effectors that, opposite to using receptor immobilization and enforced proximity, is based on lateral mobility of receptors and leverages the inherent allostery of GPCR-effector coupling.
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UR - http://www.scopus.com/inward/citedby.url?scp=85079211903&partnerID=8YFLogxK
U2 - 10.1016/j.neuron.2019.11.016
DO - 10.1016/j.neuron.2019.11.016
M3 - Article
C2 - 31837915
AN - SCOPUS:85079211903
SN - 0896-6273
VL - 105
SP - 663-677.e8
JO - Neuron
JF - Neuron
IS - 4
ER -