4.8 Article

RNASEQR-a streamlined and accurate RNA-seq sequence analysis program

Journal

NUCLEIC ACIDS RESEARCH
Volume 40, Issue 6, Pages -

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/nar/gkr1248

Keywords

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Funding

  1. Institute for Systems Biology-University of Luxemburg
  2. National Institutes of Health Center for Systems Biology [P50 [GM076547]]
  3. Republic of China National Science Council [97-2221-E-126-012-MY3]
  4. Republic of China National Health Research Institute [NHRI-EX100-10004NI]
  5. Chang-Gung Memorial Hospital [CMRPG 380621, CMRPG 392101]

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Next-generation sequencing (NGS) technologies-based transcriptomic profiling method often called RNA-seq has been widely used to study global gene expression, alternative exon usage, new exon discovery, novel transcriptional isoforms and genomic sequence variations. However, this technique also poses many biological and informatics challenges to extracting meaningful biological information. The RNA-seq data analysis is built on the foundation of high quality initial genome localization and alignment information for RNA-seq sequences. Toward this goal, we have developed RNASEQR to accurately and effectively map millions of RNA-seq sequences. We have systematically compared RNASEQR with four of the most widely used tools using a simulated data set created from the Consensus CDS project and two experimental RNA-seq data sets generated from a human glioblastoma patient. Our results showed that RNASEQR yields more accurate estimates for gene expression, complete gene structures and new transcript isoforms, as well as more accurate detection of single nucleotide variants (SNVs). RNASEQR analyzes raw data from RNA-seq experiments effectively and outputs results in a manner that is compatible with a wide variety of specialized downstream analyses on desktop computers.

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