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首页> 外文期刊>Journal of Bioinformatics and Computational Biology >Analysis of context-dependent errors for Illumina sequencing
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Analysis of context-dependent errors for Illumina sequencing

机译:Illumina测序的上下文相关错误分析

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摘要

The new generation of short-read sequencing technologies requires reliable measures of data quality. Such measures are especially important for variant calling. However, in the particular case of SNP calling, a great number of false-positive SNPs may be obtained. One needs to distinguish putative SNPs from sequencing or other errors. We found that not only the probability of sequencing errors (i.e. the quality value) is important to distinguish an FP-SNP but also the conditional probability of "correcting" this error (the "second best call" probability, conditional on that of the first call). Surprisingly, around 80% of mismatches can be "corrected" with this second call. Another way to reduce the rate of FP-SNPs is to retrieve DNA motifs that seem to be prone to sequencing errors, and to attach a corresponding conditional quality value to these motifs. We have developed several measures to distinguish between sequence errors and candidate SNPs, based on a base call's nucleotide context and its mismatch type. In addition, we suggested a simple method to correct the majority of mismatches, based on conditional probability of their "second" best intensity call. We attach a corresponding second call confidence (quality value) of being corrected to each mismatch.
机译:新一代的短读测序技术需要可靠的数据质量度量。此类措施对于变量调用特别重要。但是,在SNP调用的特定情况下,可能会获得大量的假阳性SNP。人们需要将推定的SNP与测序或其他错误区分开。我们发现,不仅序列错误的概率(即质量值)对于区分FP-SNP很重要,而且“纠正”此错误的条件概率(“第二最佳呼叫”概率,以第一个条件为条件)也很重要。呼叫)。令人惊讶的是,第二次调用可以“纠正”大约80%的不匹配。降低FP-SNP速率的另一种方法是检索似乎易于测序错误的DNA模体,并将相应的条件质量值附加到这些模体上。我们基于碱基检出的核苷酸背景及其错配类型,开发了几种区分序列错误和候选SNP的方法。此外,我们基于其“第二”最佳强度调用的条件概率,提出了一种校正大多数不匹配的简单方法。我们为每个不匹配项附加了一个相应的被纠正的第二呼叫置信度(质量值)。

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