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Parallel single nucleotide polymorphism genotyping by surface invasive cleavage with universal detection

机译:表面侵入性切割与通用检测的平行单核苷酸多态性基因分型

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Large-scale investigations of sequence variation within the human species will provide information about the basis of heritable variation in disease susceptibility and human migration. The surface invader assay (an adaptation of the invasive cleavage reaction to an array format) is capable of exquisitely sensitive and specific detection of genetic variation. It is shown here that this genotyping technology can be multiplexed in a DNA array format, permitting the parallel analysis of a panel of single nucleotide polymorphisms (SNPs) directly from an unamplified genomic DNA target. In addition, a "universal" mode of detection was developed that makes use of a mixture of degenerate templates for DNA ligation to the surface-bound cleaved oligonucleotides and thereby makes this strategy amenable to any desired SNP site or combination of SNP sites, without regard to their particular DNA sequences. This approach was demonstrated on a proof-of-principle scale using small DNA arrays to genotype 6 SNP markers in the PTPN1 gene and 10 mutations in the cystic fibrosis transmembrane conductance regulator gene. Ibis ability to analyze many different genetic variations in parallel, directly from unamplified human genomic DNA samples, lays the groundwork for the development of high-density arrays able to analyze hundreds of thousands or even millions of SNPs.
机译:对人类内部序列变异的大规模研究将提供有关疾病易感性和人类迁移的遗传变异基础的信息。表面入侵者测定(侵袭性裂解反应适应阵列形式)能够精确灵敏地检测遗传变异。此处显示,该基因分型技术可以DNA阵列格式进行多路复用,从而可以直接从未扩增的基因组DNA靶标中对一组单核苷酸多态性(SNP)进行并行分析。此外,开发了一种“通用”检测模式,该模式利用简并模板的混合物将DNA连接至表面结合的裂解寡核苷酸,从而使该策略适用于任何所需的SNP位点或SNP位点的组合,而无需考虑特定的DNA序列。使用小DNA阵列对PTPN1基因中的6个SNP标记和囊性纤维化跨膜电导调节基因中的10个突变进行基因分型,在原则上证明了该方法。 Ibis能够直接从未扩增的人类基因组DNA样本中并行分析许多不同遗传变异的能力,为开发能够分析成千上万甚至数百万个SNP的高密度阵列奠定了基础。

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