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Microarray-based estimation of SNP allele-frequency in pooled DNA using the Langmuir kinetic model

机译:使用朗格缪尔动力学模型基于池的DNA中基于微阵列的SNP等位基因频率估计

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Background High throughput genotyping of single nucleotide polymorphisms (SNPs) for genome-wide association requires technologies for generating millions of genotypes with relative ease but also at a reasonable cost and with high accuracy. In this work, we have developed a theoretical approach to estimate allele frequency in pooled DNA samples, based on the physical principles of DNA immobilization and hybridization on solid surface using the Langmuir kinetic model and quantitative analysis of the allelic signals. Results This method can successfully distinguish allele frequencies differing by 0.01 in the actual pool of clinical samples, and detect alleles with a frequency as low as 2%. The accuracy of measuring known allele frequencies is very high, with the strength of correlation between measured and actual frequencies having an r2 = 0.9992. These results demonstrated that this method could allow the accurate estimation of absolute allele frequencies in pooled samples of DNA in a feasible and inexpensive way. Conclusion We conclude that this novel strategy for quantitative analysis of the ratio of SNP allelic sequences in DNA pools is an inexpensive and feasible alternative for detecting polymorphic differences in candidate gene association studies and genome-wide linkage disequilibrium scans.
机译:背景技术用于全基因组关联的单核苷酸多态性(SNP)的高通量基因分型需要用于相对容易地以合理的成本和高精度产生数百万个基因型的技术。在这项工作中,我们基于Langmuir动力学模型和等位基因信号的定量分析,基于DNA固定化和在固体表面杂交的物理原理,开发了一种理论方法来估计合并的DNA样品中的等位基因频率。结果该方法可以成功地区分出实际样本中的等位基因频率相差0.01,并检测出频率低至2%的等位基因。测量已知等位基因频率的准确性非常高,测量频率与实际频率之间的相关强度为r 2 = 0.9992。这些结果表明,该方法可以以可行且廉价的方式准确估算合并的DNA样品中的绝对等位基因频率。结论我们得出结论,这种定量分析DNA池中SNP等位基因序列比率的新颖策略是一种用于检测候选基因关联研究和全基因组连锁不平衡扫描中多态性差异的廉价且可行的替代方法。

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