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Gene induction for the treatment of methylmalonic aciduria

机译:基因诱导治疗甲基丙二酸尿症

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Background Methylmalonic aciduria is an autosomal recessive inborn error of the propionate metabolic pathway. One form of this disorder is caused by mutations in methylmalonyl-coenzyme A mutase (MCM), resulting in reduced levels of enzyme activity. The pharmacological up-regulation of residual mutase activity is one approach to advance treatment strategies for individuals affected by this disorder. We describe the construction,characterization and use of a cellular genomic reporter assay for MCM expression that will potentially identify therapeutic pharmacological agents for methylmalonic aciduria treatment. Methods Homologous recombination was used to insert an enhanced green fluorescent protein (EGFP) cassette inframe before the last codon of exon 13 of the MCM gene (MUT) in a BAC clone. The construct was used to generate stable HeLa cell lines. EGFP expression was measured by flow cytometry and the real-time reverse transcriptase-polymerase chain reaction was used to quantify changes in MUT gene mRNA levels. Results The genomic reporter assay used to screen a selection of compounds. Cisplatin, zidovudine and adefovir were found to increase the levels of MCM mRNA and EGFP expression, providing support for the possible efficacy of these pharmacological compounds in treating methylmalonic aciduria. Conclusions This assay has the potential of being used in high-throughput screening of chemical libraries for the identification of novel compounds that specifically modulate the expression of MCM.
机译:背景甲基丙二酸尿症是丙酸代谢途径的常染色体隐性先天性错误。这种疾病的一种形式是由甲基丙二酰辅酶A突变酶(MCM)突变引起的,导致酶活性水平降低。残留突变酶活性的药理学上调是一种改善受该疾病影响的个体治疗策略的方法。我们描述了MCM表达的细胞基因组报告基因测定法的构建,表征和用途,该方法可能会确定甲基丙二酸尿症的治疗药理剂。方法采用同源重组技术在BAC克隆中,在MCM基因(MUT)第13外显子的最后一个密码子前插入一个增强的绿色荧光蛋白(EGFP)盒。该构建体用于产生稳定的HeLa细胞系。通过流式细胞仪测量EGFP的表达,实时逆转录聚合酶链反应用于量化MUT基因mRNA水平的变化。结果用于筛选化合物的基因组报告基因分析。发现顺铂,齐多夫定和阿德福韦可增加MCM mRNA和EGFP表达水平,为这些药理化合物治疗甲基丙二酸尿症的可能功效提供了支持。结论该测定法有可能用于化学文库的高通量筛选中,以鉴定特异性调节MCM表达的新型化合物。

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