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Establishment and application of a real-time loop-mediated isothermal amplification system for the detection of CYP2C19 polymorphisms

机译:CYP2C19基因多态性实时定量环介导等温扩增系统的建立与应用

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摘要

Single-nucleotide polymorphisms (SNPs) represent the most widespread type of genetic variation (approximately 90%) in the human genome, and the demand to overcome such variation has received more attention now than ever before. The capacity to rapidly assess SNPs that correlate with disease predisposition, drug efficacy and drug toxicity is a key step for the development of personalized medicine. In this work, a rapid one-step SNP detection method, real-time loop-mediated isothermal amplification (RT-LAMP), was first applied for CYP2C19 polymorphisms testing. The optimized method was established with specifically designed primers for target amplification by real-time detection in approximately 30 min under isothermal conditions. RT-LAMP amplified few copies of template to produce significant amounts of product and quantitatively detected human DNA with compatible specificity and sensitivity. The success in the establishment of this RT-LAMP protocol for CYP2C19 polymorphism testing is significant for the extension of this technique for the detection of other SNPs, which will further facilitate the development of personalized medicine.
机译:单核苷酸多态性(SNP)代表了人类基因组中最广泛的遗传变异类型(大约90%),克服这种变异的需求现在比以往任何时候都受到了更多的关注。快速评估与疾病易感性,药物功效和药物毒性相关的SNP的能力是开发个性化药物的关键步骤。在这项工作中,一种快速的单步SNP检测方法,即实时环介导的等温扩增(RT-LAMP),首先被用于CYP2C19多态性测试。优化的方法是使用专门设计的引物建立的,该引物用于在等温条件下约30分钟内通过实时检测进行靶标扩增。 RT-LAMP扩增了几份模板,以产生大量产物,并以兼容的特异性和敏感性定量检测了人类DNA。建立用于CYP2C19多态性测试的RT-LAMP协议的成功对扩展该技术以检测其他SNP具有重要意义,这将进一步促进个性化药物的开发。

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