DMD-Associated Dilated Cardiomyopathy: Genotypes, Phenotypes, and Phenocopies

扩张型心肌病 遗传学 医学 先证者 物候学 多重连接依赖探针扩增 基因型 基因检测 外显子 心肌病 亚端粒 心力衰竭 肌营养不良蛋白 MYH7 基因 表型 生物 端粒 内科学 突变 基因亚型
作者
Renée Johnson,Robyn Otway,Ephrem Chin,Claire Horvat,Monique Ohanian,Jon A. L. Willcox,Zheng Su,Priscilla R. Prestes,Andrei Smolnikov,Magdalena Soka,Guanglan Guo,Emma M. Rath,Samya Chakravorty,Łukasz Chrzanowski,Chris Hayward,Anne Keogh,Peter S. Macdonald,Eleni Giannoulatou,Alex Chia Yu Chang,Emily C. Oates,Fadi J. Charchar,Jonathan G. Seidman,Christine E. Seidman,Madhuri Hegde,Diane Fatkin
出处
期刊:Circulation [Ovid Technologies (Wolters Kluwer)]
卷期号:16 (5): 421-430 被引量:2
标识
DOI:10.1161/circgen.123.004221
摘要

Background: Variants in the DMD gene, that encodes the cytoskeletal protein, dystrophin, cause a severe form of dilated cardiomyopathy (DCM) associated with high rates of heart failure, heart transplantation, and ventricular arrhythmias. Improved early detection of individuals at risk is needed. Methods: Genetic testing of 40 male probands with a potential X-linked genetic cause of primary DCM was undertaken using multi-gene panel sequencing, multiplex polymerase chain reaction, and array comparative genomic hybridization. Variant location was assessed with respect to dystrophin isoform patterns and exon usage. Telomere length was evaluated as a marker of myocardial dysfunction in left ventricular tissue and blood. Results: Four pathogenic/likely pathogenic DMD variants were found in 5 probands (5/40: 12.5%). Only one rare variant was identified by gene panel testing with 3 additional multi-exon deletion/duplications found following targeted assays for structural variants. All of the pathogenic/likely pathogenic DMD variants involved dystrophin exons that had percent spliced-in scores >90, indicating high levels of constitutive expression in the human adult heart. Fifteen DMD variant-negative probands (15/40: 37.5%) had variants in autosomal genes including TTN , BAG3 , LMNA , and RBM20 . Myocardial telomere length was reduced in patients with DCM irrespective of genotype. No differences in blood telomere length were observed between genotype-positive family members with/without DCM and controls. Conclusions: Primary genetic testing using multi-gene panels has a low yield and specific assays for structural variants are required if DMD -associated cardiomyopathy is suspected. Distinguishing X-linked causes of DCM from autosomal genes that show sex differences in clinical presentation is crucial for informed family management.
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