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De novo clustering of long reads by gene from transcriptomics data

机译:通过转录组织数据基因的长读取的Novo聚类

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Long-read sequencing currently provides sequences of several thousand base pairs. It is therefore possible to obtain complete transcripts, offering an unprecedented vision of the cellular transcriptome. However the literature lacks tools for de novo clustering of such data, in particular for Oxford Nanopore Technologies reads, because of the inherent high error rate compared to short reads. Our goal is to process reads from whole transcriptome sequencing data accurately and without a reference genome in order to reliably group reads coming from the same gene. This de novo approach is therefore particularly suitable for non-model species, but can also serve as a useful pre-processing step to improve read mapping. Our contribution both proposes a new algorithm adapted to clustering of reads by gene and a practical and free access tool that allows to scale the complete processing of eukaryotic transcriptomes. We sequenced a mouse RNA sample using the MinION device. This dataset is used to compare our solution to other algorithms used in the context of biological clustering. We demonstrate that it is the best approach for transcriptomics long reads. When a reference is available to enable mapping, we show that it stands as an alternative method that predicts complementary clusters.
机译:读取测序目前提供几千个碱基对的序列。因此,可以获得完整的转录物,提供细胞转录组的前所未有的视觉。然而,文献缺乏用于DE Novo聚类这些数据的工具,特别是对于牛津纳米孔技术读取,因为与短读取相比固有的高误码率。我们的目标是精确地处理整个转录组测序数据的读数,而没有参考基因组,以便可靠地群体来自同一基因的读数。因此,该DE Novo方法特别适用于非模型物种,但也可以作为改善读取映射的有用预处理步骤。我们的贡献都提出了一种新的算法,适用于基因的读数和实用和自由访问工具,允许展示真核转录om的完全处理。我们使用碎片装置测序小鼠RNA样品。此数据集用于将我们的解决方案与在生物聚类上下文中使用的其他算法进行比较。我们证明它是转录组织长读数的最佳方法。当参考可用于启用映射时,我们将显示它作为预测互补群集的替代方法。

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