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首页> 外文期刊>Analytical Biochemistry: An International Journal of Analytical and Preparative Methods >Identification of coding single nucleotide polymorphisms and mutations by combination of genome tiling arrays and enrichment/depletion of mismatch cDNAs
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Identification of coding single nucleotide polymorphisms and mutations by combination of genome tiling arrays and enrichment/depletion of mismatch cDNAs

机译:通过组合基因组切片阵列和错配cDNA的富集/缺失,鉴定编码的单核苷酸多态性和突变

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摘要

Genome tiling array technology combined with a method for both enrichment and depletion of mismatch-containing cDNA fragments offers a useful approach for detecting coding single nucleotide polymorphisms (cSNPs) and mutations in pooled cDNA samples. Enriched mismatch and perfect match cDNA samples from human primary melanoma cells and normal melanocytes were obtained by selection using mismatch repair thyrnine DNA glycosylase-bound beads. These cDNA samples were then labeled and hybridized to Encyclopedia of DNA Elements genome tiling arrays. The results revealed that the hybridization intensity values of potential cDNA variation regions of the enriched mismatch samples increased, whereas the hybridization intensity values of corresponding regions of the enriched perfect match samples decreased. Six potential mutations were confirmed by polymerase chain reaction product sequencing, including two novel heterozygous mutations in melanoma cells. We suggest that this strategy should increase the efficiency of both cSNP and mutation detection throuiahout the entire human genome and decrease the cost and complexity of genomewide analysis of cDNA variations. (c) 2006 Elsevier Inc. All rights reserved.
机译:基因组切片阵列技术与富集和消除含错配的cDNA片段的方法相结合,为检测编码的单核苷酸多态性(cSNPs)和合并的cDNA样品中的突变提供了一种有用的方法。通过使用错配修复的胸腺嘧啶脱氧核糖核酸结合糖基化酶进行筛选,从人原发性黑素瘤细胞和正常黑素细胞中获得了丰富的错配和完全匹配的cDNA样品。然后将这些cDNA样品标记并与DNA Elements基因组切片阵列百科全书杂交。结果表明,富集错配样品的潜在cDNA变异区的杂交强度值增加,而富集完全匹配样品的相应区域的杂交强度值降低。通过聚合酶链反应产物测序确认了六个潜在的突变,包括黑素瘤细胞中的两个新的杂合突变。我们建议该策略应通过整个人类基因组提高cSNP和突变检测的效率,并降低cDNA变异的全基因组分析的成本和复杂性。 (c)2006 Elsevier Inc.保留所有权利。

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