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Mapping short DNA sequencing reads and calling variants using mapping quality scores.

机译:绘制短DNA测序图,并使用绘制质量评分来调用变体。

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摘要

New sequencing technologies promise a new era in the use of DNA sequence. However, some of these technologies produce very short reads, typically of a few tens of base pairs, and to use these reads effectively requires new algorithms and software. In particular, there is a major issue in efficiently aligning short reads to a reference genome and handling ambiguity or lack of accuracy in this alignment. Here we introduce the concept of mapping quality, a measure of the confidence that a read actually comes from the position it is aligned to by the mapping algorithm. We describe the software MAQ that can build assemblies by mapping shotgun short reads to a reference genome, using quality scores to derive genotype calls of the consensus sequence of a diploid genome, e.g., from a human sample. MAQ makes full use of mate-pair information and estimates the error probability of each read alignment. Error probabilities are also derived for the final genotype calls, using a Bayesian statistical model that incorporates the mapping qualities, error probabilities from the raw sequence quality scores, sampling of the two haplotypes, and an empirical model for correlated errors at a site. Both read mapping and genotype calling are evaluated on simulated data and real data. MAQ is accurate, efficient, versatile, and user-friendly. It is freely available at http://maq.sourceforge.net.
机译:新的测序技术为DNA序列的使用开辟了一个新时代。但是,其中一些技术产生的读取非常短,通常只有几十个碱基对,要有效使用这些读取,就需要新的算法和软件。特别地,主要问题是有效地使短读与参考基因组比对以及在该比对中处理歧义或缺乏准确性。在这里,我们介绍了映射质量的概念,它是对读取实际来自映射算法所对齐位置的置信度的一种度量。我们描述了可以通过将散弹枪短读序列映射到参考基因组,使用质量得分来推导二倍体基因组的共有序列的基因型调用(例如从人类样品中)而构建程序集的软件MAQ。 MAQ充分利用配对对信息,并估计每次读取比对的错误概率。使用合并映射质量,原始序列质量得分的错误概率,两种单倍型的抽样以及站点相关错误的经验模型的贝叶斯统计模型,还可以得出最终基因型检出的错误概率。读取映射和基因型调用均在模拟数据和真实数据上进行评估。 MAQ是准确,高效,通用和用户友好的。可从http://maq.sourceforge.net免费获得。

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