Relative Abundance of Transcripts ( RATs): Identifying differential isoform abundance from RNA-seq

The biological importance of changes in RNA expression is reflected by the wide variety of tools available to characterise these changes from RNA-seq data. Several tools exist for detecting differential transcript isoform usage (DTU) from aligned or assembled RNA-seq data, but few exist for DTU dete...

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Autores principales: Froussios, Kimon, Mourão, Kira, Simpson, Gordon, Barton, Geoff, Schurch, Nicholas
Formato: Online Artículo Texto
Lenguaje:English
Publicado: F1000 Research Limited 2019
Materias:
Method Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6426083/
https://www.ncbi.nlm.nih.gov/pubmed/30906538
http://dx.doi.org/10.12688/f1000research.17916.1
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author Froussios, Kimon
Mourão, Kira
Simpson, Gordon
Barton, Geoff
Schurch, Nicholas
author_facet Froussios, Kimon
Mourão, Kira
Simpson, Gordon
Barton, Geoff
Schurch, Nicholas
author_sort Froussios, Kimon
collection PubMed
description The biological importance of changes in RNA expression is reflected by the wide variety of tools available to characterise these changes from RNA-seq data. Several tools exist for detecting differential transcript isoform usage (DTU) from aligned or assembled RNA-seq data, but few exist for DTU detection from alignment-free RNA-seq quantifications. We present the RATs, an R package that identifies DTU transcriptome-wide directly from transcript abundance estimates. RATs is unique in applying bootstrapping to estimate the reliability of detected DTU events and shows good performance at all replication levels (median false positive fraction < 0.05). We compare RATs to two existing DTU tools, DRIM-Seq & SUPPA2, using two publicly available simulated RNA-seq datasets and a published human RNA-seq dataset, in which 248 genes have been previously identified as displaying significant DTU. RATs with default threshold values on the simulated Human data has a sensitivity of 0.55, a Matthews correlation coefficient of 0.71 and a false discovery rate (FDR) of 0.04, outperforming both other tools. Applying the same thresholds for SUPPA2 results in a higher sensitivity (0.61) but poorer FDR performance (0.33). RATs and DRIM-seq use different methods for measuring DTU effect-sizes complicating the comparison of results between these tools, however, for a likelihood-ratio threshold of 30, DRIM-Seq has similar FDR performance to RATs (0.06), but worse sensitivity (0.47). These differences persist for the simulated drosophila dataset. On the published human RNA-seq dataset the greatest agreement between the tools tested is 53%, observed between RATs and SUPPA2. The bootstrapping quality filter in RATs is responsible for removing the majority of DTU events called by SUPPA2 that are not reported by RATs. All methods, including the previously published qRT-PCR of three of the 248 detected DTU events, were found to be sensitive to annotation differences between Ensembl v60 and v87.
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spelling pubmed-64260832019-03-21 Relative Abundance of Transcripts ( RATs): Identifying differential isoform abundance from RNA-seq Froussios, Kimon Mourão, Kira Simpson, Gordon Barton, Geoff Schurch, Nicholas F1000Res Method Article The biological importance of changes in RNA expression is reflected by the wide variety of tools available to characterise these changes from RNA-seq data. Several tools exist for detecting differential transcript isoform usage (DTU) from aligned or assembled RNA-seq data, but few exist for DTU detection from alignment-free RNA-seq quantifications. We present the RATs, an R package that identifies DTU transcriptome-wide directly from transcript abundance estimates. RATs is unique in applying bootstrapping to estimate the reliability of detected DTU events and shows good performance at all replication levels (median false positive fraction < 0.05). We compare RATs to two existing DTU tools, DRIM-Seq & SUPPA2, using two publicly available simulated RNA-seq datasets and a published human RNA-seq dataset, in which 248 genes have been previously identified as displaying significant DTU. RATs with default threshold values on the simulated Human data has a sensitivity of 0.55, a Matthews correlation coefficient of 0.71 and a false discovery rate (FDR) of 0.04, outperforming both other tools. Applying the same thresholds for SUPPA2 results in a higher sensitivity (0.61) but poorer FDR performance (0.33). RATs and DRIM-seq use different methods for measuring DTU effect-sizes complicating the comparison of results between these tools, however, for a likelihood-ratio threshold of 30, DRIM-Seq has similar FDR performance to RATs (0.06), but worse sensitivity (0.47). These differences persist for the simulated drosophila dataset. On the published human RNA-seq dataset the greatest agreement between the tools tested is 53%, observed between RATs and SUPPA2. The bootstrapping quality filter in RATs is responsible for removing the majority of DTU events called by SUPPA2 that are not reported by RATs. All methods, including the previously published qRT-PCR of three of the 248 detected DTU events, were found to be sensitive to annotation differences between Ensembl v60 and v87. F1000 Research Limited 2019-02-24 /pmc/articles/PMC6426083/ /pubmed/30906538 http://dx.doi.org/10.12688/f1000research.17916.1 Text en Copyright: © 2019 Froussios K et al. http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution Licence, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Method Article
Froussios, Kimon
Mourão, Kira
Simpson, Gordon
Barton, Geoff
Schurch, Nicholas
Relative Abundance of Transcripts ( RATs): Identifying differential isoform abundance from RNA-seq
title Relative Abundance of Transcripts ( RATs): Identifying differential isoform abundance from RNA-seq
title_full Relative Abundance of Transcripts ( RATs): Identifying differential isoform abundance from RNA-seq
title_fullStr Relative Abundance of Transcripts ( RATs): Identifying differential isoform abundance from RNA-seq
title_full_unstemmed Relative Abundance of Transcripts ( RATs): Identifying differential isoform abundance from RNA-seq
title_short Relative Abundance of Transcripts ( RATs): Identifying differential isoform abundance from RNA-seq
title_sort relative abundance of transcripts ( rats): identifying differential isoform abundance from rna-seq
topic Method Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6426083/
https://www.ncbi.nlm.nih.gov/pubmed/30906538
http://dx.doi.org/10.12688/f1000research.17916.1
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