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Disrupted CaV1.2 selectivity causes overlapping long QT and Brugada syndrome phenotypes in the CACNA1C-E1115K iPS cell model

诱导多能干细胞 美西律 Brugada综合征 电生理学 错义突变 复极 长QT综合征 膜片钳 医学 表型 药理学 内科学 细胞生物学 神经科学 QT间期 生物 基因 遗传学 胚胎干细胞
作者
Asami Kashiwa,Takeru Makiyama,Hirohiko Kohjitani,Thomas L. Maurissen,Taisuke Ishikawa,Yuta Yamamoto,Yimin Wuriyanghai,Jingshan Gao,Hai Huang,Tomohiko Imamura,Takanori Aizawa,Misato Nishikawa,Kazuhisa Chonabayashi,Hiroyuki Mishima,Seiko Ohno,Futoshi Toyoda,Seiichi Sato,Koh-ichiro Yoshiura,Kazuhiro Takahashi,Yoshinori Yoshida,Knut Woltjen,Minoru Horie,Naomasa Makita,Takeshi Kimura
出处
期刊:Heart Rhythm [Elsevier]
卷期号:20 (1): 89-99 被引量:6
标识
DOI:10.1016/j.hrthm.2022.08.021
摘要

A missense mutation in the α1c subunit of voltage-gated L-type Ca2+ channel-coding CACNA1C-E1115K, located in the Ca2+ selectivity site, causes a variety of arrhythmogenic phenotypes.We aimed to investigate the electrophysiological features and pathophysiological mechanisms of CACNA1C-E1115K in patient-specific induced pluripotent stem cell (iPSC)-derived cardiomyocytes (CMs).We generated iPSCs from a patient carrying heterozygous CACNA1C-E1115K with overlapping phenotypes of long QT syndrome, Brugada syndrome, and mild cardiac dysfunction. Electrophysiological properties were investigated using iPSC-CMs. We used iPSCs from a healthy individual and an isogenic iPSC line corrected using CRISPR-Cas9-mediated gene editing as controls. A mathematical E1115K-CM model was developed using a human ventricular cell model.Patch-clamp analysis revealed that E1115K-iPSC-CMs exhibited reduced peak Ca2+ current density and impaired Ca2+ selectivity with an increased permeability to monovalent cations. Consequently, E1115K-iPSC-CMs showed decreased action potential plateau amplitude, longer action potential duration (APD), and a higher frequency of early afterdepolarization compared with controls. In optical recordings examining the antiarrhythmic drug effect, late Na+ channel current (INaL) inhibitors (mexiletine and GS-458967) shortened APDs specifically in E1115K-iPSC-CMs. The AP-clamp using a voltage command obtained from E1115K-iPSC-CMs with lower action potential plateau amplitude and longer APD confirmed the upregulation of INaL. An in silico study recapitulated the in vitro electrophysiological properties.Our iPSC-based analysis in CACNA1C-E1115K with disrupted CaV1.2 selectivity demonstrated that the aberrant currents through the mutant channels carried by monovalent cations resulted in specific action potential changes, which increased endogenous INaL, thereby synergistically contributing to the arrhythmogenic phenotype.

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