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A simple and fast two-locus quality control test to detect false positives due to batch effects in genome-wide association studies.

机译:一种简单快速的两基因座质量控制测试,可检测全基因组关联研究中由于批次效应引起的假阳性。

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摘要

The impact of erroneous genotypes having passed standard quality control (QC) can be severe in genome-wide association studies, genotype imputation, and estimation of heritability and prediction of genetic risk based on single nucleotide polymorphisms (SNP). To detect such genotyping errors, a simple two-locus QC method, based on the difference in test statistic of association between single SNPs and pairs of SNPs, was developed and applied. The proposed approach could detect many problematic SNPs with statistical significance even when standard single SNP QC analyses fail to detect them in real data. Depending on the data set used, the number of erroneous SNPs that were not filtered out by standard single SNP QC but detected by the proposed approach varied from a few hundred to thousands. Using simulated data, it was shown that the proposed method was powerful and performed better than other tested existing methods. The power of the proposed approach to detect erroneous genotypes was ∼80% for a 3% error rate per SNP. This novel QC approach is easy to implement and computationally efficient, and can lead to a better quality of genotypes for subsequent genotype-phenotype investigations.
机译:通过标准质量控制(QC)的错误基因型的影响在​​全基因组关联研究,基因型归因,遗传力估计以及基于单核苷酸多态性(SNP)的遗传风险预测中可能非常严重。为了检测这种基因分型错误,基于单个SNP和一对SNP之间关联的测试统计差异,开发并应用了一种简单的两基因座QC方法。即使标准的单个SNP QC分析未能在实际数据中检测到它们,所提出的方法也可以检测到许多具有统计意义的有问题的SNP。根据使用的数据集,未被标准的单个SNP QC过滤掉但被建议的方法检测到的错误SNP的数量从几百到数千不等。使用模拟数据表明,所提出的方法功能强大且性能优于其他经过测试的现有方法。对于每个SNP而言,错误率3%时,所提出的检测错误基因型的方法的功效约为80%。这种新颖的质量控制方法易于实施且计算效率高,可为后续的基因型-表型研究带来更高质量的基因型。

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