Gene editing of DNAH11 restores normal cilia motility in primary ciliary dyskinesia

原发性睫状体运动障碍 纤毛 生物 运动纤毛 转录激活物样效应核酸酶 卡塔格综合征 细胞生物学 粘液纤毛清除率 离体 遗传学 基因 分子生物学 体内 基因组编辑 支气管扩张 医学 内科学 清脆的
作者
Michele Lai,Massimo Pifferi,Andrew Bush,Martina Piras,Angela Michelucci,Maria Di Cicco,Ambra Del Grosso,Paola Quaranta,Chiara Cursi,Elena Tantillo,Sara Franceschi,Chiara Maria Mazzanti,Paolo Simi,Giuseppe Saggese,Attilio Boner,Mauro Pistello
出处
期刊:Journal of Medical Genetics [BMJ]
卷期号:53 (4): 242-249 被引量:65
标识
DOI:10.1136/jmedgenet-2015-103539
摘要

Background Primary ciliary dyskinesia (PCD) is a rare autosomal recessive genetic disorder characterised by dysfunction of motile cilia. Ciliary dysmotility causes poor mucociliary clearance and leads to impairment of pulmonary function and severe respiratory infections. PCD has no specific therapy. With the aim to permanently restore gene function and normalise ciliary motility, we used gene editing to replace mutated with wild-type sequence in defective cells. Methods The target gene was dynein heavy chain 11 ( DNAH11 ), an essential component of ciliary structure. Airway ciliated cells were collected from two patients with PCD with DNAH11 nonsense mutations and altered ciliary beating and pattern. Repair of the genetic defect was performed ex vivo by site-specific recombination using transcription activator-like effector nucleases (TALENs). Results In an epithelial cell line engineered to contain the DNAH11 target site, TALENs cleaved over 80% of the mutated DNAH11 sequence and replaced the mutated sequence with wild-type sequence in about 50% of cells. In airway ciliated cells of patients with PCD, site-specific recombination and normalisation of ciliary beating and pattern occurred in 33% and 29% of cells, respectively. Conclusion This study demonstrates that gene editing can rescue ciliary beating ex vivo, opening up new avenues for treating PCD.

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