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通过表面增强共振拉曼散射进行简单的多重基因分型。

Simple multiplex genotyping by surface-enhanced resonance Raman scattering.

作者信息

Graham Duncan, Mallinder Benjamin J, Whitcombe David, Watson Nigel D, Smith W Ewen

机构信息

Department of Pure and Applied Chemistry, University of Strathclyde, Glasgow, UK.

出版信息

Anal Chem. 2002 Mar 1;74(5):1069-74. doi: 10.1021/ac0155456.

Abstract

The accurate detection of DNA sequences is essential for a variety of post human genome projects including detection of specific gene variants for medical diagnostics and pharmacogenomics. A specific DNA sequence detection assay based on surface-enhanced resonance Raman scattering (SERRS) and an amplification refractory mutation system (ARMS) is reported. Initially, generation of PCR products was achieved by using specifically designed allele-specific SERRS active primers. Detection by SERRS of the PCR products confirmed the presence of the sequence tested for by the allele-specific oligonucleotides. This lead directly to the multiplex genotyping of human DNA samples for the deltaF508 mutational status of the cystic fibrosis transmembrane conductance regulator gene using SERRS active primers in an ARMS assay. Removal of the unincorporated primers allowed fast and accurate analysis of the three genotypes possible in this system in a multiplex format without any separation of amplicons. The results indicate that SERRS can be used in modern genetic analysis and offers an opportunity for the development of novel assays. This is the first demonstration of the use of SERRS in multiplex genotyping and shows potential advantages over fluorescence as a detection technique with considerable promise for future development.

摘要

准确检测DNA序列对于人类基因组计划后的各种项目至关重要,这些项目包括用于医学诊断和药物基因组学的特定基因变异检测。本文报道了一种基于表面增强共振拉曼散射(SERRS)和扩增不应突变系统(ARMS)的特定DNA序列检测方法。最初,通过使用专门设计的等位基因特异性SERRS活性引物来实现PCR产物的生成。通过SERRS对PCR产物进行检测,证实了等位基因特异性寡核苷酸所检测序列的存在。这直接导致在ARMS分析中使用SERRS活性引物对人类DNA样本进行囊性纤维化跨膜传导调节因子基因的deltaF508突变状态的多重基因分型。去除未掺入的引物后,可以以多重形式快速准确地分析该系统中可能存在的三种基因型,而无需对扩增子进行任何分离。结果表明,SERRS可用于现代遗传分析,并为新型检测方法的开发提供了机会。这是首次证明SERRS在多重基因分型中的应用,并且显示出作为一种检测技术相对于荧光具有潜在优势,具有很大的未来发展前景。

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