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Truncated titin proteins and titin haploinsufficiency are targets for functional recovery in human cardiomyopathy due to TTN mutations

提丁 默默林 心肌病 收缩性 单倍率不足 肌节 生物 扩张型心肌病 分子生物学 细胞生物学 化学 内科学 遗传学 心肌细胞 医学 内分泌学 心力衰竭 表型 基因
作者
Andrey Fomin,Anna Gärtner,Lukas Cyganek,Malte Tiburcy,Izabela Tuleta,Luisa Wellers,Lina Folsche,Anastasia J. Hobbach,Marion von Frieling-Salewsky,Andreas Unger,Anna Hucke,Franziska Koser,Astrid Kassner,Katharina Sielemann,Katrin Streckfuß‐Bömeke,Gerd Hasenfuß,Alexander Goedel,Karl‐Ludwig Laugwitz,Alessandra Moretti,Jan Gummert
出处
期刊:Science Translational Medicine [American Association for the Advancement of Science (AAAS)]
卷期号:13 (618) 被引量:101
标识
DOI:10.1126/scitranslmed.abd3079
摘要

Heterozygous truncating variants in TTN (TTNtv), the gene coding for titin, cause dilated cardiomyopathy (DCM), but the underlying pathomechanisms are unclear and disease management remains uncertain. Truncated titin proteins have not yet been considered as a contributor to disease development. Here, we studied myocardial tissues from nonfailing donor hearts and 113 patients with end-stage DCM for titin expression and identified a TTNtv in 22 patients with DCM (19.5%). We directly demonstrate titin haploinsufficiency in TTNtv-DCM hearts and the absence of compensatory changes in the alternative titin isoform Cronos. Twenty-one TTNtv-DCM hearts in our cohort showed stable expression of truncated titin proteins. Expression was variable, up to half of the total titin protein pool, and negatively correlated with patient age at heart transplantation. Truncated titin proteins were not detected in sarcomeres but were present in intracellular aggregates, with deregulated ubiquitin-dependent protein quality control. We produced human induced pluripotent stem cell–derived cardiomyocytes (hiPSC-CMs), comparing wild-type controls to cells with a patient-derived, prototypical A-band-TTNtv or a CRISPR-Cas9–generated M-band-TTNtv. TTNtv-hiPSC-CMs showed reduced wild-type titin expression and contained truncated titin proteins whose proportion increased upon inhibition of proteasomal activity. In engineered heart muscle generated from hiPSC-CMs, depressed contractility caused by TTNtv could be reversed by correction of the mutation using CRISPR-Cas9, eliminating truncated titin proteins and raising wild-type titin content. Functional improvement also occurred when wild-type titin protein content was increased by proteasome inhibition. Our findings reveal the major pathomechanisms of TTNtv-DCM and can be exploited for new therapies to treat TTNtv-related cardiomyopathies.
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