Leaky Ca2+ release channel/ryanodine receptor 2 causes seizures and sudden cardiac death in mice
Stephan E. Lehnart, … , Gregory Morley, Andrew R. Marks
Stephan E. Lehnart, … , Gregory Morley, Andrew R. Marks
Published May 15, 2008
Citation Information: J Clin Invest. 2008;118(6):2230-2245. https://doi.org/10.1172/JCI35346.
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Research Article Cardiology

Leaky Ca2+ release channel/ryanodine receptor 2 causes seizures and sudden cardiac death in mice

Abstract

The Ca2+ release channel ryanodine receptor 2 (RyR2) is required for excitation-contraction coupling in the heart and is also present in the brain. Mutations in RyR2 have been linked to exercise-induced sudden cardiac death (catecholaminergic polymorphic ventricular tachycardia [CPVT]). CPVT-associated RyR2 mutations result in “leaky” RyR2 channels due to the decreased binding of the calstabin2 (FKBP12.6) subunit, which stabilizes the closed state of the channel. We found that mice heterozygous for the R2474S mutation in Ryr2 (Ryr2-R2474S mice) exhibited spontaneous generalized tonic-clonic seizures (which occurred in the absence of cardiac arrhythmias), exercise-induced ventricular arrhythmias, and sudden cardiac death. Treatment with a novel RyR2-specific compound (S107) that enhances the binding of calstabin2 to the mutant Ryr2-R2474S channel inhibited the channel leak and prevented cardiac arrhythmias and raised the seizure threshold. Thus, CPVT-associated mutant leaky Ryr2-R2474S channels in the brain can cause seizures in mice, independent of cardiac arrhythmias. Based on these data, we propose that CPVT is a combined neurocardiac disorder in which leaky RyR2 channels in the brain cause epilepsy, and the same leaky channels in the heart cause exercise-induced sudden cardiac death.

Authors

Stephan E. Lehnart, Marco Mongillo, Andrew Bellinger, Nicolas Lindegger, Bi-Xing Chen, William Hsueh, Steven Reiken, Anetta Wronska, Liam J. Drew, Chris W. Ward, W.J. Lederer, Robert S. Kass, Gregory Morley, Andrew R. Marks

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Figure 5

Electrical and Ca2+ cycling abnormalities in Ryr2RS/WT cardiomyocytes are consistent with Ca2+-triggered afterdepolarizations and are reduced by the RyR2-stabilizing drug S107.

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Electrical and Ca2+ cycling abnormalities in Ryr2RS/WT cardiomyocytes ar...
(A) Representative examples of whole-cell current (Em) recordings from Ryr2RS/WT cardiomyocytes paced continuously at 1 Hz (recording started after 2 minutes; pacing stimuli as indicated) under control (left) and ISO-stimulated conditions (1 μM; right). Following ISO, aberrant membrane depolarizations (asterisks) increased in frequency and became self-sustained when pacing was stopped (not shown). (B) Intracellular Ca2+ transients from Ryr2RS/WT cardiomyocytes field-paced continuously at 1 Hz under control (left) and ISO-stimulated conditions (1 μM, right; recording started after 2 minutes continuous pacing). Aberrant spontaneous Ca2+ waves (asterisks) occurred irregularly and became self-sustained when pacing was stopped (not shown). (C) Representative current traces from Ryr2RS/WT cardiomyocytes recorded during an 0.5-Hz depolarization train in the absence (left) and presence of ISO (1 μM; right). ISO-treated Ryr2RS/WT cardiomyocytes showed frequent ITI (asterisks) during and after pacing. The figure illustrates currents recorded during and following the first 2 and last 5 pulses from a continuous 10-pulse (1 Hz) conditioning train. A 5.5-second-long period of the recording during the train was omitted for display purposes, and the time scale is expanded in the ISO-treated examples in the rights panels of AC. (D) Normalized ITI density in ISO-treated cells. ISO-treated Ryr2RS/WT cardiomyocytes (n = 7) showed significantly increased ITI densities (*P < 0.05 vs. control; n = 6); in vivo S107 treatment significantly decreased ITI density in ISO-treated Ryr2RS/WT cells (#P < 0.05; n = 4). (E) Simultaneous confocal Ca2+ imaging of a small region of interest and ITI recording from an ISO-stimulated Ryr2RS/WT cardiomyocyte. Following regular pacing-induced Ca2+ release (last cycle shown on left side), intracellular Ca2+ and membrane current rapidly normalized to the resting (diastolic) state. Ryr2RS/WT cardiomyocytes showed abnormal intracellular Ca2+ release events, which became organized as Ca2+ waves, coinciding with secondary arrhythmogenic ITI. Scale bar: 10 μm; time and normalized F/F0 fluorescence signal are as indicated. (F) Representative confocal Ca2+ spark images from WT and Ryr2RS/WT cardiomyocytes before (–ISO) and after (+ISO; 1 μM) treatment. Bar graphs show significant differences (*P < 0.05) in average spark frequencies and average spatial area dimensions, indicating increased intracellular Ca2+ leak in Ryr2RS/WT cardiomyocytes following ISO stimulation as the subcellular origin of arrhythmogenic diastolic DADs (A), Ca2+ waves (B and E), and ITI (C and E) events.