A Cell-Based Double Reporter Gene Splicing Assay for Therapeutic Screening in Myotonic Dystrophy

IF 1.2 Q3 MULTIDISCIPLINARY SCIENCES
I. Udosen, J. Granados, J. Brook
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引用次数: 0

Abstract

Abstract The study has developed a model splicing construct assay system based on splicing misregulation, one of the major molecular features associated with myotonic dystrophy. The splicing construct assay has double reporters for intron 2 splicing in chloride channel (CLCN1). The CLCN1 transgene splicing construct assay was used to transfect wild type and DM fibroblast cell lines and the clones generated showed that it enabled quantification of splicing efficiency in transgene construct. Validation of the DM fibroblasts containing transgene splicing construct was performed by differentiating the DM fibroblasts into myoblasts which exhibited a switch in CLCN1 splicing construct which was consistent with that associated with myotonic dystrophy (DM) condition. The myoblast derived from fibroblasts cell-based gene-splicing assay was subsequently applied in therapeutic screening in small throughput screens of 113 compounds which identified Protein Kinase C inhibitors- hypericin and Ro-31-8220 as potential therapeutic agents. The CLCN1 gene-splicing assay is a good model system for application in therapeutic screening in myotonic dystrophy because its double reporters facilitated quantification of effect putative drug on correction of misregulated splicing.
基于细胞的双报告基因剪接试验用于肌强直性营养不良的治疗筛选
摘要本研究开发了一种基于剪接失调的模型剪接构建物检测系统,剪接失调是强直性肌营养不良的主要分子特征之一。剪接构建物分析具有氯通道内含子2剪接的双报告子(CLCN1)。CLCN1转基因剪接构建体测定用于转染野生型和DM成纤维细胞系,所产生的克隆表明它能够量化转基因构建体中的剪接效率。通过将DM成纤维细胞分化为成肌细胞来验证含有转基因剪接构建体的DM成纤维纤维细胞,该成肌细胞在CLCN1剪接构建体中表现出与强直性肌营养不良(DM)状况相关的转换。衍生自成纤维细胞的成肌细胞基于细胞的基因剪接分析随后应用于113种化合物的小通量筛选中的治疗性筛选,这些化合物鉴定了蛋白激酶C抑制剂金丝桃素和Ro-31-8220作为潜在的治疗剂。CLCN1基因剪接分析是一个很好的模型系统,可用于强直性肌营养不良的治疗性筛选,因为它的双报告子有助于量化推定药物对纠正错误剪接的作用。
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来源期刊
The EuroBiotech Journal
The EuroBiotech Journal Agricultural and Biological Sciences-Food Science
CiteScore
3.60
自引率
0.00%
发文量
17
审稿时长
10 weeks
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