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An integrative approach for efficient analysis of whole genome bisulfite sequencing data

机译:一种有效分析全基因组亚硫酸氢盐测序数据的综合方法

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Background Whole genome bisulfite sequencing (WGBS) is a high-throughput technique for profiling genome-wide DNA methylation at single nucleotide resolution. However, the applications of WGBS are limited by low accuracy resulting from bisulfite-induced damage on DNA fragments. Although many computer programs have been developed for accurate detecting, most of the programs have barely succeeded in improving either quantity or quality of the methylation results. To improve both, we attempted to develop a novel integration of most widely used bisulfite-read mappers: Bismark, BSMAP, and BS-seeker2. Results A comprehensive analysis of the three mappers revealed that the mapping results of the mappers were mutually complementary under diverse read conditions. Therefore, we sought to integrate the characteristics of the mappers by scoring them to gain robustness against artifacts. As a result, the integration significantly increased detection accuracy compared with the individual mappers. In addition, the amount of detected cytosine was higher than that by Bismark. Furthermore, the integration successfully reduced the fluctuation of detection accuracy induced by read conditions. We applied the integration to real WGBS samples and succeeded in classifying the samples according to the originated tissues by both CpG and CpH methylation patterns. Conclusions In this study, we improved both quality and quantity of methylation results from WGBS data by integrating the mapping results of three bisulfite-read mappers. Also, we succeeded in combining and comparing WGBS samples by reducing the effects of read heterogeneity on methylation detection. This study contributes to DNA methylation researches by improving efficiency of methylation detection from WGBS data and facilitating the comprehensive analysis of public WGBS data.
机译:背景技术全基因组亚硫酸氢盐测序(WGBS)是一种高通量技术,用于以单核苷酸分辨率分析全基因组DNA甲基化。但是,WGBS的应用受到亚硫酸氢盐诱导的DNA片段损伤而导致的低准确性的限制。尽管已经开发了许多用于精确检测的计算机程序,但是大多数程序在提高甲基化结果的数量或质量方面几乎没有成功。为了改善两者,我们尝试开发一种最广泛使用的重亚硫酸盐读取映射器的新颖集成:Bismark,BSMAP和BS-seeker2。结果对这三个作图者的综合分析表明,在不同的阅读条件下,作图者的作图结果是相互补充的。因此,我们试图通过对映射器进行评分以对伪像获得鲁棒性来整合其特征。结果,与单个映射器相比,集成显着提高了检测精度。另外,胞嘧啶的检出量高于Bismark。此外,该集成成功地减少了读取条件引起的检测精度波动。我们将整合应用于实际的WGBS样本,并通过CpG和CpH甲基化模式根据来源组织成功地对样本进行了分类。结论在这项研究中,我们通过整合三个重亚硫酸盐读取的绘图仪的绘图结果,提高了WGBS数据的甲基化结果的质量和数量。此外,我们通过减少读取异质性对甲基化检测的影响,成功地组合和比较了WGBS样品。这项研究通过提高WGBS数据中的甲基化检测效率并促进对WGBS公开数据的综合分析,为DNA甲基化研究做出了贡献。

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