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首页> 外文期刊>Scientific reports. >Repair of the TGFBI gene in human corneal keratocytes derived from a granular corneal dystrophy patient via CRISPR/Cas9-induced homology-directed repair
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Repair of the TGFBI gene in human corneal keratocytes derived from a granular corneal dystrophy patient via CRISPR/Cas9-induced homology-directed repair

机译:通过CRISPR / Cas9诱导的同源性定向修复修复来自粒状角膜营养不良患者的人角膜角膜细胞中的TGFBI基因

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Granular corneal dystrophy (GCD) is an autosomal dominant hereditary disease in which multiple discrete and irregularly shaped granular opacities are deposited in the corneal stroma. GCD is caused by a point mutation in the transforming growth factor-β-induced (TGFBI) gene, located on chromosome 5q31. Here, we report the first successful application of CRISPR-Cas9-mediated genome editing for the correction of a TGFBI mutation in GCD patient-derived primary corneal keratocytes via homology-directed repair (HDR). To correct genetic defects in GCD patient cells, we designed a disease-specific guide RNA (gRNA) targeting the R124H mutation of TGFBI, which causes GCD type 2 (GCD2). An R124H mutation in primary human corneal keratocytes derived from a GCD2 patient was corrected by delivering a CRISPR plasmid expressing Cas9/gRNA and a single-stranded oligodeoxynucleotide HDR donor template in vitro. The gene correction efficiency was 20.6% in heterozygous cells and 41.3% in homozygous cells. No off-target effects were detected. These results reveal a new therapeutic strategy for GCD2; this method may also be applicable to other heredity corneal diseases.
机译:颗粒性角膜营养不良(GCD)是常染色体显性遗传性疾病,其中多个离散且形状不规则的颗粒混浊沉积在角膜基质中。 GCD是由位于5q31号染色体上的转化生长因子-β诱导(TGFBI)基因中的点突变引起的。在这里,我们报道了CRISPR-Cas9介导的基因组编辑在通过同源性定向修复(HDR)来纠正GCD患者来源的原发性角膜角化细胞中的TGFBI突变中的首次成功应用。为了纠正GCD患者细胞中的遗传缺陷,我们设计了针对TGFBI的R124H突变的疾病特异性向导RNA(gRNA),该突变导致GCD 2型(GCD2)。通过在体外递送表达Cas9 / gRNA的CRISPR质粒和单链寡脱氧核苷酸HDR供体模板,可以纠正源自GCD2患者的原代人角膜角膜细胞中的R124H突变。基因校正效率在杂合细胞中为20.6%,在纯合细胞中为41.3%。没有检测到脱靶效应。这些结果揭示了GCD2的新治疗策略。这种方法也可能适用于其他遗传性角膜疾病。

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