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Flexible use of high-density oligonucleotide arrays for single-nucleotide polymorphism discovery and validation

机译:灵活使用高密度寡核苷酸阵列进行单核苷酸多态性发现和验证

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摘要

A method for identifying and validating single nucleotide polymorphisms (SNPs) with high-density oligonucleotide arrays without the need for locus-specific polymerase chain reactions (PCR) is described in this report.: Genomic DNAs were divided into subsets with complexity of similar to 10 Mb by restriction enzyme digestion and gel-based fragment size resolution, ligated to a common adaptor, and amplified with one primer in a single PCR reaction. As a demonstration of this, approach, a total of 124 SNPs were located in 190 kb of genomic sequences distributed across the entire human genome by hybridizing to high-density variant detection arrays (VDA). A set of independent validation experiments was conducted for these SNPs employing bead-based affinity selection followed by hybridization of the affinity-selected SNP-containing fragments to the same VDA that was used to identify the SNPs. A total of 98.7% (74/75) of these SNPs were confirmed using both DNA dideoxynucleotide sequencing and the VDA methodologies. With flexible sample preparation, high-density oligonucleotide arrays can be tailored for even larger scale genome-wide SNP discovery as well as validation.
机译:本报告介绍了一种无需高位基因特异性聚合酶链反应(PCR)即可鉴定和验证具有高密度寡核苷酸阵列的单核苷酸多态性(SNP)的方法。:基因组DNA分为复杂度类似于10的子集通过限制性内切酶消化和基于凝胶的片段大小解析来检测Mb,将其连接至通用的衔接子,并在单个PCR反应中用一种引物进行扩增。作为对此方法的证明,通过与高密度变异检测阵列(VDA)杂交,在整个人类基因组中分布的190 kb基因组序列中共有124个SNP。使用基于珠的亲和力选择,然后将亲和力选择的含SNP的片段与用于识别SNP的相同VDA杂交,对这些SNP进行了一组独立的验证实验。使用DNA双脱氧核苷酸测序和VDA方法均证实了这些SNP总数的98.7%(74/75)。通过灵活的样品制备,可以定制高密度寡核苷酸阵列,以进行更大规模的全基因组SNP发现和验证。

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