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CircMarker: a fast and accurate algorithm for circular RNA detection

机译:线马克:一种快速准确的圆形RNA检测算法

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While RNA is often created from linear splicing during transcription, recent studies have found that non-canonical splicing sometimes occurs. Non-canonical splicing joins 3' and 5' and forms the so-called circular RNA. It is now believed that circular RNA plays important biological roles such as affecting susceptibility of some diseases. During the past several years, multiple experimental methods have been developed to enrich circular RNA while degrade linear RNA. Although several useful software tools for circular RNA detection have been developed as well, these tools are based on reads mapping may miss many circular RNA. Also, existing tools are slow for large data due to their dependence on reads mapping. In this paper, we present a new computational approach, named CircMarker, based on k-mers rather than reads mapping for circular RNA detection. CircMarker takes advantage of transcriptome annotation files to create the k-mer table for circular RNA detection. Empirical results show that CircMarker outperforms existing tools in circular RNA detection on accuracy and efficiency in many simulated and real datasets. We develop a new circular RNA detection method called CircMarker based on k-mer analysis. Our results on both simulation data and real data demonstrate that CircMarker runs much faster and can find more circular RNA with higher consensus-based sensitivity and high accuracy ratio compared with existing tools.
机译:虽然RNA通常在转录期间从线性剪接产生,但最近的研究发现有时会发生非规范剪接。非规范拼接到3'和5'并形成所谓的圆形RNA。现在据信,圆形RNA发挥着重要的生物学作用,例如影响某些疾病的易感性。在过去几年中,已经开发了多种实验方法以富集圆形RNA,同时降解线性RNA。尽管已经开发了几种用于圆形RNA检测的软件工具,但这些工具基于读取映射可能会错过许多圆形RNA。此外,由于它们对读取映射的依赖性,现有工具对于大数据而缓慢。在本文中,我们提出了一种新的计算方法,名为Circarmarer,基于K-MERS而不是读取循环RNA检测的映射。线程矢量利用转录组注释文件来创建用于圆形RNA检测的K-MET表。经验结果表明,线程领域在许多模拟和实际数据集中的循环RNA检测中的现有工具优于现有工具。我们开发了一种基于K-MES分析的新循环RNA检测方法。我们对模拟数据和实际数据的结果表明,与现有工具相比,线程市场速度速度更快,可以达到更多圆形RNA,并与基于工具相比具有更高的普通敏感性和高精度。

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