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The Bellerophon pipeline improving de novo transcriptomes and removing chimeras

机译:Bellerophon管线可改善从头转录组并去除嵌合体

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摘要

Transcriptome quality control is an important step in RNA‐Seq experiments. However, the quality of de novo assembled transcriptomes is difficult to assess, due to the lack of reference genome to compare the assembly to. We developed a method to assess and improve the quality of de novo assembled transcriptomes by focusing on the removal of chimeric sequences. These chimeric sequences can be the result of faulty assembled contigs, merging two transcripts into one. The developed method is incorporated into a pipeline, which we named Bellerophon, that is broadly applicable and easy to use. Bellerophon first uses the quality assessment tool TransRate to indicate the quality, after which it uses a transcripts per million (TPM) filter to remove lowly expressed contigs and CD‐HIT‐EST to remove highly identical contigs. To validate the quality of this method, we performed three benchmark experiments: (1) a computational creation of chimeras, (2) identification of chimeric contigs in a transcriptome assembly, (3) a simulated RNA‐Seq experiment using a known reference transcriptome. Overall, the Bellerophon pipeline was able to remove between 40% and 91.9% of the chimeras in transcriptome assemblies and removed more chimeric than nonchimeric contigs. Thus, the Bellerophon sequence of filtration steps is a broadly applicable solution to improve transcriptome assemblies.
机译:转录组质量控制是RNA-Seq实验中的重要一步。然而,由于缺乏用于比较组装的参考基因组,因此难以评估从头组装转录组的质量。我们开发了一种方法,通过重点研究嵌合序列的去除来评估和提高从头组装转录组的质量。这些嵌合序列可能是错误的组装重叠群的结果,将两个转录本合并为一个。所开发的方法已并入我们称为Bellerophon的管道中,该管道广泛适用且易于使用。 Bellerophon首先使用质量评估工具TransRate来指示质量,然后使用每百万笔成绩单(TPM)过滤器除去表达低的重叠群,并使用CD-HIT-EST除去高度相同的重叠群。为了验证该方法的质量,我们进行了三个基准实验:(1)嵌合体的计算创建,(2)转录组装配中嵌合重叠群的鉴定,(3)使用已知参考转录组的模拟RNA-Seq实验。总体而言,Bellerophon管道能够去除转录组装配体中40%至91.9%的嵌合体,并且比非嵌合重叠群更能去除嵌合体。因此,Bellerophon过滤步骤的顺序是改善转录组装配的广泛适用的解决方案。

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