Miniatura

Fitxers

691049.pdf (6.52 MB)

Tipus de document

Article

Versió

Versió publicada

Data de publicació

2018-09-19

Llicència de publicació

cc-by (c) Luján, Rafael et al., 2018
Si us plau utilitzeu sempre aquest identificador per citar o enllaçar aquest document: https://hdl.handle.net/2445/148836

SK2 Channels Associate With mGlu1α Receptors and CaV2.1 Channels in Purkinje Cells

Títol de la revista

Autors

Director/Tutor

ISSN de la revista

Títol del volum

Recurs relacionat

https://doi.org/10.3389/fncel.2018.00311

Resum

The small-conductance, Ca2+-activated K+ (SK) channel subtype SK2 regulates the spike rate and firing frequency, as well as Ca2+ transients in Purkinje cells (PCs). To understand the molecular basis by which SK2 channels mediate these functions, we analyzed the exact location and densities of SK2 channels along the neuronal surface of the mouse cerebellar PCs using SDS-digested freeze-fracture replica labeling (SDS-FRL) of high sensitivity combined with quantitative analyses. Immunogold particles for SK2 were observed on post- and pre-synaptic compartments showing both scattered and clustered distribution patterns. We found an axo-somato-dendritic gradient of the SK2 particle density increasing 12-fold from soma to dendritic spines. Using two different immunogold approaches, we also found that SK2 immunoparticles were frequently adjacent to, but never overlap with, the postsynaptic density of excitatory synapses in PC spines. Co-immunoprecipitation analysis demonstrated that SK2 channels form macromolecular complexes with two types of proteins that mobilize Ca2+: CaV2.1 channels and mGlu1α receptors in the cerebellum. Freeze-fracture replica double-labeling showed significant co-clustering of particles for SK2 with those for CaV2.1 channels and mGlu1α receptors. SK2 channels were also detected at presynaptic sites, mostly at the presynaptic active zone (AZ), where they are close to CaV2.1 channels, though they are not significantly co-clustered. These data demonstrate that SK2 channels located in different neuronal compartments can associate with distinct proteins mobilizing Ca2+, and suggest that the ultrastructural association of SK2 with CaV2.1 and mGlu1α provides the mechanism that ensures voltage (excitability) regulation by distinct intracellular Ca2+ transients in PCs.

Matèries

Molècules, Cerebel, Receptors cel·lulars

Matèries (anglès)

Molecules, Cerebellum, Cell receptors

Citació

Col·leccions

Articles publicats en revistes (Patologia i Terapèutica Experimental)
<b>Publicacions de projectes de recerca finançats per la UE</b>
Articles publicats en revistes (Institut d'lnvestigació Biomèdica de Bellvitge (IDIBELL))

Citació

LUJÁN, Rafael, AGUADO, Carolina, CIRUELA ALFÉREZ, Francisco, MORATÓ ARÚS, Xavier, MARTÍN-BELMONTE, Alejandro, ALFARO RUIZ, Rocío, MARTÍNEZ GÓMEZ, Jesús, OSSA, Luis de la, WATANABE, Masahiko, ADELMAN, John p., SHIGEMOTO, Ryuichi, FUKAZAWA, Yugo. SK2 Channels Associate With mGlu1α Receptors and CaV2.1 Channels in Purkinje Cells. _Frontiers in Cellular Neuroscience_. 2018. Vol. 12, núm. 311. [consulta: 23 de gener de 2026]. ISSN: 1662-5102. [Disponible a: https://hdl.handle.net/2445/148836]

Exportar metadades

JSON - METS

Compartir registre