Cardiac hypertrophy and arrhythmia in mice induced by a mutation in ryanodine receptor 2
Francisco J. Alvarado, … , Michael J. Ackerman, Héctor H. Valdivia
Francisco J. Alvarado, … , Michael J. Ackerman, Héctor H. Valdivia
Published March 5, 2019
Citation Information: JCI Insight. 2019;4(7):e126544. https://doi.org/10.1172/jci.insight.126544.
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Research Article Cardiology

Cardiac hypertrophy and arrhythmia in mice induced by a mutation in ryanodine receptor 2

Abstract

Hypertrophic cardiomyopathy (HCM) is triggered mainly by mutations in genes encoding sarcomeric proteins, but a significant proportion of patients lack a genetic diagnosis. We identified a potentially novel mutation in ryanodine receptor 2, RyR2-P1124L, in a patient from a genotype-negative HCM cohort. The aim of this study was to determine whether RyR2-P1124L triggers functional and structural alterations in isolated RyR2 channels and whole hearts. We found that P1124L induces significant conformational changes in the SPRY2 domain of RyR2. Recombinant RyR2-P1124L channels displayed a cytosolic loss-of-function phenotype, which contrasted with a higher sensitivity to luminal [Ca2+], indicating a luminal gain of function. Homozygous mice for RyR2-P1124L showed mild cardiac hypertrophy, similar to the human patient. This phenotype, evident at 1 year of age, was accompanied by an increase in the expression of calmodulin (CaM). P1124L mice also showed higher susceptibility to arrhythmia at 8 months of age, before the onset of hypertrophy. RyR2-P1124L has a distinct cytosolic loss-of-function and a luminal gain-of-function phenotype. This bifunctionally divergent behavior triggers arrhythmias and structural cardiac remodeling, and it involves overexpression of CaM as a potential hypertrophic mediator. This study is relevant to continue elucidating the possible causes of genotype-negative HCM and the role of RyR2 in cardiac hypertrophy.

Authors

Francisco J. Alvarado, J. Martijn Bos, Zhiguang Yuchi, Carmen R. Valdivia, Jonathan J. Hernández, Yan-Ting Zhao, Dawn S. Henderlong, Yan Chen, Talia R. Booher, Cherisse A. Marcou, Filip Van Petegem, Michael J. Ackerman, Héctor H. Valdivia

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Figure 5

Cellular hypertrophy in cardiac myocytes from 1-year-old P1124L mice.

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Cellular hypertrophy in cardiac myocytes from 1-year-old P1124L mice. (A...
(A) Representative transmitted light images of ventricular myocytes (scale bar: 50 μm). Cardiac myocytes were enzymatically isolated from freshly explanted hearts. Images were obtained with a confocal microscope. Cells are delineated and colored green (measured cells) or purple (out of focus or out of frame). (B–D) Cell width (B), length (C), and surface area (D) measured from transmitted light images (left, individual measurements from n = 75 WT, 81 Het, 84 Homo cells; right, mean values for n = 3 hearts per genotype. *P < 0.05, 1-way ANOVA). (E) Box plots showing transcript expression level of 3 hypertrophic genes: natriuretic peptide A (Nppa), natriuretic peptide B (Nppb), and myosin heavy chain 7 (Myh7). Data normalized to actin (Actb) expression (n = 5 WT, 4 Het, 5 Homo hearts per genotype. **P < 0.01, **P < 0.05, 1-way ANOVA).