Abstract
CaMKII is a major synaptic protein that is activated during the induction of long-term potentiation (LTP) by the Ca2+ influx through NMDARs. This activation is required for LTP induction, but the role of the kinase in the maintenance of LTP is less clear. Elucidating the mechanisms of maintenance may provide insights into the molecular processes that underlie the stability of stored memories. In this brief review, we will outline the criteria for evaluating an LTP maintenance mechanism. The specific hypothesis evaluated is that LTP is maintained by the complex of activated CaMKII with the NMDAR. The evidence in support of this hypothesis is substantial, but further experiments are required, notably to determine the time course and persistence of complex after LTP induction. Additional work is also required to elucidate how the CaMKII/NMDAR complex produces the structural growth of the synapse that underlies late LTP. It has been proposed by Frey and Morris that late LTP involves the setting of a molecular tag during LTP induction, which subsequently allows the activated synapse to capture the proteins responsible for late LTP. However, the molecular processes by which this leads to the structural growth that underlies late LTP are completely unclear. Based on known binding reactions, we suggest the first molecularly specific version of tag/capture hypothesis: that the CaMKII/NMDAR complex, once formed, serves as a tag, which then leads to a binding cascade involving densin, delta-catenin, and N-cadherin (some of which are newly synthesized). Delta-catenin binds AMPA-binding protein (ABP), leading to the LTP-induced increase in AMPA channel content. The addition of postsynaptic N-cadherin, and the complementary increase on the presynaptic side, leads to a trans-synaptically coordinated increase in synapse size (and more release sites). It is suggested that synaptic strength is stored stably through the combined actions of the CaMKII/NMDAR complex and N-cadherin dimers. These N-cadherin pairs have redundant storage that could provide informational stability in a manner analogous to the base-pairing in DNA.
Highlights
CaMKII is a major synaptic protein that is activated during the induction of long-term potentiation (LTP) by the Ca2+ influx through NMDARs
LTP induction should cause a persistent increase in the CaMKII/NMDAR complex The initial evidence that CaMKII could interact with the NMDAR came from in vitro experiments showing that a fragment of GluN2B is a substrate for purified CaMKII [7]
The CaMKII/NMDAR complex is a promising candidate as the molecular basis of memory storage
Summary
The CaMKII/NMDAR complex is a promising candidate as the molecular basis of memory storage. Much additional work is required at the behavioral level to test the role of the CaMKII and the CaMKII/NMDAR complex in the persistence of memory. An important unresolved question is whether the importance of CaMKII/NMDAR complex in LTP maintenance, as demonstrated, will be specific for CA1 or more generally applicable to synapses. One perspective on this question comes from analysis of the PSDs, which are generally isolated from whole brains. Recent work shows that the ability of activity to stabilize synaptic connections is dependent on the CaMKII/NMDAR complex [83]. Authors' contributions JL and MS contributed to writing this review.
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