首页> 美国卫生研究院文献>Applied and Environmental Microbiology >Identification of a p-Coumarate Degradation Regulon in Rhodopseudomonas palustris by Xpression an Integrated Tool for Prokaryotic RNA-Seq Data Processing
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Identification of a p-Coumarate Degradation Regulon in Rhodopseudomonas palustris by Xpression an Integrated Tool for Prokaryotic RNA-Seq Data Processing

机译:通过Xpression原核RNA-Seq数据处理的集成工具鉴定了Phodopseudomonas palustris中的p-香豆酸降解调节子。

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摘要

High-throughput sequencing of cDNA prepared from RNA, an approach known as RNA-seq, is coming into increasing use as a method for transcriptome analysis. Despite its many advantages, widespread adoption of the technique has been hampered by a lack of easy-to-use, integrated, open-source tools for analyzing the nucleotide sequence data that are generated. Here we describe Xpression, an integrated tool for processing prokaryotic RNA-seq data. The tool is easy to use and is fully automated. It performs all essential processing tasks, including nucleotide sequence extraction, alignment, quantification, normalization, and visualization. Importantly, Xpression processes multiplexed and strand-specific nucleotide sequence data. It extracts and trims specific sequences from files and separately quantifies sense and antisense reads in the final results. Outputs from the tool can also be conveniently used in downstream analysis. In this paper, we show the utility of Xpression to process strand-specific RNA-seq data to identify genes regulated by CouR, a transcription factor that controls p-coumarate degradation by the bacterium Rhodopseudomonas palustris.
机译:从RNA制备的cDNA的高通量测序(一种称为RNA-seq的方法)正越来越多地用作转录组分析的方法。尽管具有许多优点,但由于缺乏易于使用的,集成的,开放源代码的工具来分析所生成的核苷酸序列数据,因此该技术的广泛采用受到了阻碍。在这里,我们描述Xpression,一种用于处理原核RNA序列数据的集成工具。该工具易于使用且完全自动化。它执行所有必不可少的处理任务,包括核苷酸序列提取,比对,定量,归一化和可视化。重要的是,Xpression处理多重和链特异性核苷酸序列数据。它从文件中提取并修剪特定序列,并分别量化最终结果中的有义和反义读物。该工具的输出还可以方便地用于下游分析。在本文中,我们展示了Xpression实用程序来处理链特异的RNA-seq数据,以鉴定受CouR调控的基因,该转录因子可控制p-香豆酸盐被细菌红假单胞菌降解。

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