On the Mechanism of Synaptic Depression Induced by CaMKIIN, an Endogenous Inhibitor of CaMKII

Belen Aburto,Magdalena Sanhueza,Cecilia Vergara,Camilo Gouet

doi:10.1371/journal.pone.0049293

Belen Aburto, Magdalena Sanhueza + Show 2 more

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https://doi.org/10.1371/journal.pone.0049293

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Abstract

Activity-dependent synaptic plasticity underlies, at least in part, learning and memory processes. NMDA receptor (NMDAR)-dependent long-term potentiation (LTP) is a major synaptic plasticity model. During LTP induction, Ca2+/calmodulin-dependent protein kinase II (CaMKII) is activated, autophosphorylated and persistently translocated to the postsynaptic density, where it binds to the NMDAR. If any of these steps is inhibited, LTP is disrupted. The endogenous CaMKII inhibitor proteins CaMKIINα,β are rapidly upregulated in specific brain regions after learning. We recently showed that transient application of peptides derived from CaMKIINα (CN peptides) persistently depresses synaptic strength and reverses LTP saturation, as it allows further LTP induction in previously saturated pathways. The treatment disrupts basal CaMKII-NMDAR interaction and decreases bound CaMKII fraction in spines. To unravel CaMKIIN function and to further understand CaMKII role in synaptic strength maintenance, here we more deeply investigated the mechanism of synaptic depression induced by CN peptides (CN-depression) in rat hippocampal slices. We showed that CN-depression does not require glutamatergic synaptic activity or Ca2+ signaling, thus discarding unspecific triggering of activity-dependent long-term depression (LTD) in slices. Moreover, occlusion experiments revealed that CN-depression and NMDAR-LTD have different expression mechanisms. We showed that CN-depression does not involve complex metabolic pathways including protein synthesis or proteasome-mediated degradation. Remarkably, CN-depression cannot be resolved in neonate rats, for which CaMKII is mostly cytosolic and virtually absent at the postsynaptic densities. Overall, our results support a direct effect of CN peptides on synaptic CaMKII-NMDAR binding and suggest that CaMKIINα,β could be critical plasticity-related proteins that may operate as cell-wide homeostatic regulators preventing saturation of LTP mechanisms or may selectively erase LTP-induced traces in specific groups of synapses.

Highlights

The multifunctional holoenzyme calmodulindependent protein kinase II (CaMKII) plays a critical role in NMDA receptor (NMDAR)-dependent long-term potentiation (LTP) and memory formation [1,2]
This study was directed to investigate the function of the endogenous CaMKII inhibitor proteins CaMKIIN and thereby to further understand the complex CaMKII participation in synaptic plasticity
Our results point to an activity-independent, direct CN action on PSDattached CaMKII, presumably on kinase binding to NR2B

Summary

Introduction

The multifunctional holoenzyme CaMKII plays a critical role in NMDAR-dependent LTP and memory formation [1,2]. LTP induction involves Ca2+ influx through NMDARs and activation of CaMKII, that translocates to stimulated spines and postsynaptic densities (PSD) [3,4,5], regulating AMPA-receptor (AMPAR) localization and function. A key binding partner of CaMKII at PSD is the NMDAR subunit NR2B [6,7]. If CaMKII activation or T286 autophosphorylation are blocked by pharmacological or genetic means, LTP induction is prevented [9,10,11], and disruption of CaMKII binding to NR2B impairs LTP and learning [12,13,14]. CaMKII autophosphorylation at T305/306 negatively regulates Ca2+-dependent activity and PSD association, suggesting a complex CaMKII modulation during synaptic potentiation and learning [15]

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