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Comparative assessment of methods for the fusion transcripts detection from RNA-Seq data

机译:RNA-SEQ数据融合转录物检测方法的比较评估

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摘要

RNA-Seq made possible the global identification of fusion transcripts, i.e. "chimeric RNAs". Even though various software packages have been developed to serve this purpose, they behave differently in different datasets provided by different developers. It is important for both users, and developers to have an unbiased assessment of the performance of existing fusion detection tools. Toward this goal, we compared the performance of 12 well-known fusion detection software packages. We evaluated the sensitivity, false discovery rate, computing time, and memory usage of these tools in four different datasets (positive, negative, mixed, and test). We conclude that some tools are better than others in terms of sensitivity, positive prediction value, time consumption and memory usage. We also observed small overlaps of the fusions detected by different tools in the real dataset (test dataset). This could be due to false discoveries by various tools, but could also be due to the reason that none of the tools are inclusive. We have found that the performance of the tools depends on the quality, read length, and number of reads of the RNA-Seq data. We recommend that users choose the proper tools for their purpose based on the properties of their RNA-Seq data.
机译:RNA-SEQ成为融合转录物的全局鉴定,即“嵌合RNA”。尽管已经开发了各种软件包来服务此目的,但它们在不同开发人员提供的不同数据集中行事不同。对于用户来说,和开发人员对对现有融合检测工具的性能进行了无偏见的评估。对此目标,我们比较了12名众所周知的融合检测软件包的性能。我们在四个不同的数据集中评估了这些工具的灵敏度,虚假发现速率,计算时间和内存使用(正,负,混合和测试)。我们得出结论,在灵敏度,阳性预测值,时间消耗和内存使用方面,一些工具比其他工具更好。我们还观察到由实际数据集中的不同工具检测到的融合器的小重叠(测试数据集)。这可能是由于各种工具的虚假发现,但也可能是由于没有任何工具都是包容性的原因。我们发现工具的性能取决于RNA-SEQ数据的质量,读取长度和数量。我们建议用户根据其RNA-SEQ数据的属性选择适当的工具,以其目的的目的。

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