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The Journal of Neuroscience, October 15, 2008, 28(42):10549-10560; doi:10.1523/JNEUROSCI.2061-08.2008

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Cellular/Molecular
Mechanisms of Potentiation of Mossy Fiber EPSCs in the Cerebellar Nuclei by Coincident Synaptic Excitation and Inhibition

Jason R. Pugh1 and Indira M. Raman1,2

1Interdepartmental Neuroscience Program and 2Department of Neurobiology and Physiology, Northwestern University, Evanston, Illinois 60208

Correspondence should be addressed to Indira M. Raman, Department of Neurobiology and Physiology, 2205 Tech Drive, Northwestern University, Evanston, IL 60208. Email: i-raman{at}northwestern.edu

Neurons of the cerebellar nuclei receive synaptic excitation from cerebellar mossy fibers. Unlike in many principal neurons, coincident presynaptic activity and postsynaptic depolarization do not generate long-term potentiation at these synapses. Instead, EPSCs are potentiated by high-frequency trains of presynaptic activity applied with postsynaptic hyperpolarization, in patterns resembling mossy-fiber-mediated excitation and Purkinje-cell-mediated inhibition that are predicted to occur during delay eyelid conditioning. Here, we have used electrophysiology and Ca imaging to test how synaptic excitation and inhibition interact to generate long-lasting synaptic plasticity in nuclear cells in cerebellar slices. We find that the extent of plasticity varies with the relative timing of synaptic excitation and hyperpolarization. Potentiation is most effective when synaptic stimuli precede the postinhibitory rebound by ~400 ms, whereas with longer intervals, or with a reverse sequence, EPSCs tend to depress. When basal intracellular Ca is raised by spontaneous firing or reduced by voltage clamping at subthreshold potentials, potentiation is induced as long as the synaptic-rebound temporal sequence is maintained, suggesting that plasticity does not require Ca levels to exceed a threshold or attain a specific concentration. Although rebound and spike-dependent Ca influx are global, potentiation is synapse specific, and is disrupted by inhibitors of calcineurin or Ca-calmodulin-dependent protein kinase II, but not PKC. When IPSPs replace the hyperpolarizing step in the induction protocol, potentiation proceeds normally. These results lead us to propose that synaptic and inhibitory/rebound stimuli initiate separate processes, with local NMDA receptor-mediated Ca influx "priming" synapses, and Ca changes from the inhibition and rebound "triggering" potentiation at recently activated synapses.

Key words: deep cerebellar nuclei; interpositus; Purkinje cell; synaptic plasticity; eye blink; long-term potentiation; coincidence detection; non-Hebbian


Received May 5, 2008; revised Aug. 1, 2008; accepted Sept. 2, 2008.

Correspondence should be addressed to Indira M. Raman, Department of Neurobiology and Physiology, 2205 Tech Drive, Northwestern University, Evanston, IL 60208. Email: i-raman{at}northwestern.edu




This article has been cited by other articles:


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N. Zheng and I. M. Raman
Ca Currents Activated by Spontaneous Firing and Synaptic Disinhibition in Neurons of the Cerebellar Nuclei
J. Neurosci., August 5, 2009; 29(31): 9826 - 9838.
[Abstract] [Full Text] [PDF]



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