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首页> 外文期刊>Analytical chemistry >Quantification of Relative Gene Dosage by Single-Base Extension and High-Performance Liquid Chromatography: Application to the SMN1/SMN2 Gene
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Quantification of Relative Gene Dosage by Single-Base Extension and High-Performance Liquid Chromatography: Application to the SMN1/SMN2 Gene

机译:单碱基延伸和高效液相色谱法定量相对基因剂量:在SMN1 / SMN2基因中的应用

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摘要

One of the most commonly used techniques for genotyping of single-nucleotide polymorphism (SNP) is detection of single-base extensions (SBEs). We present a new, rapid, simple, and highly reliable method for accurate quantification of SNP variants in a single reaction. Our approach is based on SBE detection coupled with high-performance liquid chromatography (HPLC) quantification. To demonstrate the utility of our approach, we report data to determine the gene dosage for relative amounts of alleles in a homologous gene, allowing detection of mutation causing exon skipping in human SMN genes to determine the ratio between the copy numbers of the SMN1/SMN2 gene. We successfully determined the relative ratio of the SMN1 and SMN2 genes and showed assay characteristics using the SBE reaction coupled with HPLC. This assay approach readily scaled to high parallelization with multiplex SBE reactions in a single sample screened in one analysis. By screening for particular SNP genotypes, this assay can be used to determine the relative gene dosage that correlates highly with the patient's disease state. The next challenge is to apply this novel methodology in a clinical screening and quantification setting for special gene regions within highly homologous genes.
机译:用于单核苷酸多态性(SNP)基因分型的最常用技术之一是检测单碱基延伸(SBE)。我们提出了一种新的,快速,简单且高度可靠的方法,可在单个反应中准确定量SNP变体。我们的方法基于SBE检测和高效液相色谱(HPLC)定量分析。为了证明我们方法的实用性,我们报告了数据以确定同源基因中等位基因相对量的基因剂量,从而允许检测导致人SMN基因外显子跳​​跃的突变,从而确定SMN1 / SMN2拷贝数之间的比率基因。我们成功确定了SMN1和SMN2基因的相对比率,并使用SBE反应与HPLC结合显示了测定特征。这种分析方法很容易扩展到在一个分析中筛选出的单个样品中与多重SBE反应高度平行的情况。通过筛选特定的SNP基因型,该测定法可用于确定与患者疾病状态高度相关的相对基因剂量。下一个挑战是将这种新颖的方法应用于高度同源基因中特殊基因区域的临床筛查和量化设置中。

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