M-current preservation contributes to anticonvulsant effects of valproic acid
Hee Yeon Kay, … , Anastasia Kosenko, Naoto Hoshi
Hee Yeon Kay, … , Anastasia Kosenko, Naoto Hoshi
Published September 8, 2015
Citation Information: J Clin Invest. 2015;125(10):3904-3914. https://doi.org/10.1172/JCI79727.
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Research Article Neuroscience

M-current preservation contributes to anticonvulsant effects of valproic acid

Abstract

Valproic acid (VPA) has been widely used for decades to treat epilepsy; however, its mechanism of action remains poorly understood. Here, we report that the anticonvulsant effects of nonacute VPA treatment involve preservation of the M-current, a low-threshold noninactivating potassium current, during seizures. In a wide variety of neurons, activation of Gq-coupled receptors, such as the m1 muscarinic acetylcholine receptor, suppresses the M-current and induces hyperexcitability. We demonstrated that VPA treatment disrupts muscarinic suppression of the M-current and prevents resultant agonist-induced neuronal hyperexcitability. We also determined that VPA treatment interferes with M-channel signaling by inhibiting palmitoylation of a signaling scaffold protein, AKAP79/150, in cultured neurons. In a kainate-induced murine seizure model, administration of a dose of an M-channel inhibitor that did not affect kainate-induced seizure transiently eliminated the anticonvulsant effects of VPA. Retigabine, an M-channel opener that does not open receptor-suppressed M-channels, provided anticonvulsant effects only when administered prior to seizure induction in control animals. In contrast, treatment of VPA-treated mice with retigabine induced anticonvulsant effects even when administered after seizure induction. Together, these results suggest that receptor-induced M-current suppression plays a role in the pathophysiology of seizures and that preservation of the M-current during seizures has potential as an effective therapeutic strategy.

Authors

Hee Yeon Kay, Derek L. Greene, Seungwoo Kang, Anastasia Kosenko, Naoto Hoshi

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Figure 7

Lipid modification of AKAP150 is required for muscarinic suppression of the M-current.

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Lipid modification of AKAP150 is required for muscarinic suppression of ...
(A) Representative current traces showing muscarinic response of the M-current in AKAP150-silenced rat SCG neurons. Silencing of endogenous AKAP150 attenuated 1 μM oxo-M induced suppression of the M-current. Coexpression of WT AKAP79, AK79(wt), but not palmitoylation-deficient AKAP79(C36S/C129S), AK79(C36S/C129S), rescued oxo-M induced suppression of the M-current. (B) Summary of the ability of AKAP79 mutants to restore muscarinic M-current suppression in AKAP150-silenced neurons. Open bars indicate P < 0.001 from AKAP150-silenced control evaluated by one-way ANOVA followed by Dunnett’s multiple comparisons test. AKAP79(C36S/C129S) did not restore AKAP150-mediated muscarinic signaling. Attachment of a myristoylation site to AKAP79(C36S/C129S) restored signaling. Error bars show ± SEM. Numbers to the right of bars represent n.