psichomics: graphical application for alternative splicing quantification and analysis

Saraiva-Agostinho, Nuno; Barbosa‐Morais, Nuno L.

doi:10.1101/261180

Cited by 9 publications

(11 citation statements)

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“…ASCOT's user interface and associated splicing/expression data sets are openly available at http://ascot.cs.jhu.edu. Although there have been past efforts to summarize public RNA-Seq data 28,29,74 , ASCOT represents the largest effort to date to make alternative splicing and gene expression summaries of diverse data sets available to general researchers. ASCOT also demonstrates the value of using annotation-free methods to summarize publicly archived data.…”

Section: Discussionmentioning

confidence: 99%

“…Numerous algorithms for alternative splicing analysis have been developed [11][12][13][14][15][16][17][18][19][20][21][22][23][24][25][26][27] , including several recent studies that propose useful models for studying complex splicing patterns in RNA-Seq data 11,13,25 . However, there is a need for new methods that can summarize alternative splicing across thousands of public data sets in a unified manner, without relying on prior transcript annotation 28,29 .…”

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confidence: 99%

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ASCOT identifies key regulators of neuronal subtype-specific splicing

et al. 2020

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Public archives of next-generation sequencing data are growing exponentially, but the difficulty of marshaling this data has led to its underutilization by scientists. Here, we present ASCOT, a resource that uses annotation-free methods to rapidly analyze and visualize splice variants across tens of thousands of bulk and single-cell data sets in the public archive. To demonstrate the utility of ASCOT, we identify novel cell type-specific alternative exons across the nervous system and leverage ENCODE and GTEx data sets to study the unique splicing of photoreceptors. We find that PTBP1 knockdown and MSI1 and PCBP2 overexpression are sufficient to activate many photoreceptor-specific exons in HepG2 liver cancer cells. This work demonstrates how large-scale analysis of public RNA-Seq data sets can yield key insights into cell type-specific control of RNA splicing and underscores the importance of considering both annotated and unannotated splicing events.

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Section: Discussionmentioning

confidence: 99%

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confidence: 99%

ASCOT identifies key regulators of neuronal subtype-specific splicing

et al. 2020

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“…To estimate the PSI of all exons in all GTEx samples ( GTEx Consortium, 2017 ) from the proportion of reads supporting exon inclusion in the GTEx junction read counts file ( GTEx_Analysis_2016-01-15_v7_STARv2.4.2a_junctions.gct.gz ; available for download at https://www.gtexportal.org/home/datasets ), we used the quantifySplicing function from the Psichomics package in R ( Saraiva-Agostinho and Barbosa-Morais, 2019 ). The minReads argument was set to 10 (such that a splicing event requires at least 10 reads for it to be quantified) and the eventType argument was set to ‘SE’ (instructing the quantifySplicing function to quantify alternative exon events).…”

Section: Methodsmentioning

confidence: 99%

Mutations primarily alter the inclusion of alternatively spliced exons

Baeza-Centurion

Miñana

Valcárcel

et al. 2020

eLife

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Genetic analyses and systematic mutagenesis have revealed that synonymous, non-synonymous and intronic mutations frequently alter the inclusion levels of alternatively spliced exons, consistent with the concept that altered splicing might be a common mechanism by which mutations cause disease. However, most exons expressed in any cell are highly-included in mature mRNAs. Here, by performing deep mutagenesis of highly-included exons and by analysing the association between genome sequence variation and exon inclusion across the transcriptome, we report that mutations only very rarely alter the inclusion of highly-included exons. This is true for both exonic and intronic mutations as well as for perturbations in trans. Therefore, mutations that affect splicing are not evenly distributed across primary transcripts but are focussed in and around alternatively spliced exons with intermediate inclusion levels. These results provide a resource for prioritising synonymous and other variants as disease-causing mutations.

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“…S1A). Transcriptomic analysis of PDAC samples that were screened for homogenous cancer cell population [29] using the Psycomics tool [30] indicated that MEX3A, and to a lesser extent SRRM1, were expressed at significantly higher levels in basal-like tumors (Fig. 1D).…”

Section: Identification Of Rna Processing Regulators Associated With mentioning

confidence: 99%