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Detecting actively translated open reading frames in ribosome profiling data
Author(s) -
Lorenzo Calviello,
Neelanjan Mukherjee,
Emanuel Wyler,
Henrik Zauber,
Antje Hirsekorn,
Matthias Selbach,
Markus Landthaler,
Benedikt Obermayer,
Uwe Ohler
Publication year - 2015
Publication title -
nature methods
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 19.469
H-Index - 318
eISSN - 1548-7105
pISSN - 1548-7091
DOI - 10.1038/nmeth.3688
Subject(s) - orfs , ribosome profiling , open reading frame , biology , ribosome , computational biology , gene , encode , proteome , genetics , transcriptome , gene expression , rna , peptide sequence
RNA-sequencing protocols can quantify gene expression regulation from transcription to protein synthesis. Ribosome profiling (Ribo-seq) maps the positions of translating ribosomes over the entire transcriptome. We have developed RiboTaper (available at https://ohlerlab.mdc-berlin.de/software/), a rigorous statistical approach that identifies translated regions on the basis of the characteristic three-nucleotide periodicity of Ribo-seq data. We used RiboTaper with deep Ribo-seq data from HEK293 cells to derive an extensive map of translation that covered open reading frame (ORF) annotations for more than 11,000 protein-coding genes. We also found distinct ribosomal signatures for several hundred upstream ORFs and ORFs in annotated noncoding genes (ncORFs). Mass spectrometry data confirmed that RiboTaper achieved excellent coverage of the cellular proteome. Although dozens of novel peptide products were validated in this manner, few of the currently annotated long noncoding RNAs appeared to encode stable polypeptides. RiboTaper is a powerful method for comprehensive de novo identification of actively used ORFs from Ribo-seq data.

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