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首页> 外文期刊>Bioinformatics >Detecting genomic indel variants with exact breakpoints in single- and paired-end sequencing data using SplazerS
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Detecting genomic indel variants with exact breakpoints in single- and paired-end sequencing data using SplazerS

机译:使用SplazerS在单端和双端测序数据中检测具有确切断点的基因组indel变体

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摘要

Motivation: The reliable detection of genomic variation in resequencing data is still a major challenge, especially for variants larger than a few base pairs. Sequencing reads crossing boundaries of structural variation carry the potential for their identification, but are difficult to map. Results: Here we present a method for 'split' read mapping, where prefix and suffix match of a read may be interrupted by a longer gap in the read-to-reference alignment. We use this method to accurately detect medium-sized insertions and long deletions with precise breakpoints in genomic resequencing data. Compared with alternative split mapping methods, SplazerS significantly improves sensitivity for detecting large indel events, especially in variant-rich regions. Our method is robust in the presence of sequencing errors as well as alignment errors due to genomic mutations/divergence, and can be used on reads of variable lengths. Our analysis shows that SplazerS is a versatile tool applicable to unanchored or single-end as well as anchored paired-end reads. In addition, application of SplazerS to targeted resequencing data led to the interesting discovery of a complete, possibly functional gene retrocopy variant. Availability: SplazerS is available from http://www.seqan.de/projects/splazers.
机译:动机:在重测序数据中可靠检测基因组变异仍然是一个重大挑战,尤其是对于大于几个碱基对的变异。跨越结构变异边界的测序读物具有识别的潜力,但难以作图。结果:在这里,我们提出了一种“拆分”读取映射的方法,其中读取的前缀和后缀匹配可能会被读取到参考的对齐方式中的较长间隙中断。我们使用这种方法来精确检测基因组重测序数据中具有精确断点的中等大小的插入和长缺失。与其他拆分映射方法相比,SplazerS显着提高了检测大indel事件的灵敏度,尤其是在变异丰富的区域。我们的方法在存在测序错误以及由于基因组突变/差异导致的比对错误时都非常可靠,并且可以用于可变长度的读取。我们的分析表明,SplazerS是一种通用工具,适用于非锚定或单端以及锚定的双端读取。此外,将SplazerS应用于有针对性的重测序数据导致有趣的发现了完整的,可能具有功能的基因逆转录变体。可用性:可从http://www.seqan.de/projects/splazers获得SplazerS。

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