Annotation different expressed exon. results from DESeq
1
0
Entering edit mode
@fabrice-tourre-4394
Last seen 10.2 years ago
Dear list, When I use DESeq find different expressed exon in tow conditions. e.g, id baseMean baseMeanA baseMeanB 1 ENSMUSG00000079102:009 851.0096 1697.09604 4.9231156 2 ENSMUSG00000026727:016 239.6701 478.35562 0.9846231 3 ENSMUSG00000026727:004 155.8972 311.79442 0.0000000 How can know the Alternative Splicing Event for ENSMUSG00000079102:009, ENSMUSG00000026727:016 and ENSMUSG00000026727:004? for example, Cassette exon (skipped exon), Intron retention, Mutually exclusive exons, Alternative 3' sites, Alternative 5' sites, Alternative first exon. Thank you very much in advance.
DESeq DESeq • 1.4k views
ADD COMMENT
0
Entering edit mode
Alejandro Reyes ★ 1.9k
@alejandro-reyes-5124
Last seen 4 months ago
Novartis Institutes for BioMedical Reseā€¦
Dear Fabrice, I think you meant DEXSeq. To classify events into alternative splicing types it is useful to go back to the alignment files and visualize the exon-exon junction reads, then it becomes obvious which are the events that are giving rise to the differences in exon usage. Best regards, Alejandro > Dear list, > > When I use DESeq find different expressed exon in tow conditions. e.g, > > id baseMean baseMeanA baseMeanB > 1 ENSMUSG00000079102:009 851.0096 1697.09604 4.9231156 > 2 ENSMUSG00000026727:016 239.6701 478.35562 0.9846231 > 3 ENSMUSG00000026727:004 155.8972 311.79442 0.0000000 > > How can know the Alternative Splicing Event for > ENSMUSG00000079102:009, ENSMUSG00000026727:016 and > ENSMUSG00000026727:004? > for example, Cassette exon (skipped exon), Intron retention, Mutually > exclusive exons, Alternative 3' sites, Alternative 5' sites, > Alternative first exon. > > Thank you very much in advance. > > _______________________________________________ > Bioconductor mailing list > Bioconductor at r-project.org > https://stat.ethz.ch/mailman/listinfo/bioconductor > Search the archives: http://news.gmane.org/gmane.science.biology.informatics.conductor >
ADD COMMENT
0
Entering edit mode
Alejandro, Thank you. It is from DESeq. I have added GeneSymbol to the last column. Here how should I understand ENSMUSG00000026727:016, ENSMUSG00000026727:004?does it mean there are two exon 016 and 004 in gene ENSMUSG00000026727 are different expressed in tow conditions? id baseMean baseMeanA baseMeanB 1 ENSMUSG00000022150+ENSMUSG00000079102:009 851.0096 1697.09604 4.9231156 2 ENSMUSG00000026727:016 239.6701 478.35562 0.9846231 3 ENSMUSG00000026727:004 155.8972 311.79442 0.0000000 4 ENSMUSG00000022150+ENSMUSG00000079102:015 698.9853 1348.73940 49.2311562 5 ENSMUSG00000025730:010 703.3964 56.87455 1349.9183017 6 ENSMUSG00000005836:007 302.9137 590.07349 15.7539700 foldChange log2FoldChange pval padj GeneSymbol 1 0.002900906 -8.429281 3.160644e-18 3.750609e-13 Dab2 2 0.002058350 -8.924296 1.458392e-12 8.653076e-08 Rsu1 3 0.000000000 -Inf 2.943669e-11 1.164378e-06 Rsu1 4 0.036501607 -4.775896 1.217087e-09 3.610671e-05 Dab2 5 23.735013823 4.568945 4.029933e-09 9.564321e-05 Rab40c 6 0.026698319 -5.227107 6.754638e-09 1.335910e-04 Gata6 On Mon, Mar 3, 2014 at 3:35 AM, Alejandro Reyes <alejandro.reyes at="" embl.de=""> wrote: > Dear Fabrice, > > I think you meant DEXSeq. > To classify events into alternative splicing types it is useful to go back > to the alignment files and visualize the exon-exon junction reads, then it > becomes obvious which are the events that are giving rise to the differences > in exon usage. > > Best regards, > Alejandro > > > >> Dear list, >> >> When I use DESeq find different expressed exon in tow conditions. e.g, >> >> id baseMean baseMeanA baseMeanB >> 1 ENSMUSG00000079102:009 851.0096 1697.09604 4.9231156 >> 2 ENSMUSG00000026727:016 239.6701 478.35562 0.9846231 >> 3 ENSMUSG00000026727:004 155.8972 311.79442 0.0000000 >> >> How can know the Alternative Splicing Event for >> ENSMUSG00000079102:009, ENSMUSG00000026727:016 and >> ENSMUSG00000026727:004? >> for example, Cassette exon (skipped exon), Intron retention, Mutually >> exclusive exons, Alternative 3' sites, Alternative 5' sites, >> Alternative first exon. >> >> Thank you very much in advance. >> >> _______________________________________________ >> Bioconductor mailing list >> Bioconductor at r-project.org >> https://stat.ethz.ch/mailman/listinfo/bioconductor >> Search the archives: >> http://news.gmane.org/gmane.science.biology.informatics.conductor >> >
ADD REPLY
0
Entering edit mode
Hi Alejandro and list, Since this is a recurrent topic about alternative splicing with RNA- Seq and the robust DEXSeq software, are you planning to include some 'downstream' tool to guide on the classification of the AS events based on the bam alignments? I known there are some tools like splicegrapher.py and other few out there but it would be a perfect end point for the R/DEXSeq package. Thanks again Jose 2014-03-03 9:35 GMT+01:00 Alejandro Reyes <alejandro.reyes@embl.de>: > Dear Fabrice, > > I think you meant DEXSeq. > To classify events into alternative splicing types it is useful to go > back to the alignment files and visualize the exon-exon junction reads, > then it becomes obvious which are the events that are giving rise to the > differences in exon usage. > > Best regards, > Alejandro > > > > > Dear list, > > > > When I use DESeq find different expressed exon in tow conditions. e.g, > > > > id baseMean baseMeanA baseMeanB > > 1 ENSMUSG00000079102:009 851.0096 1697.09604 4.9231156 > > 2 ENSMUSG00000026727:016 239.6701 478.35562 0.9846231 > > 3 ENSMUSG00000026727:004 155.8972 311.79442 0.0000000 > > > > How can know the Alternative Splicing Event for > > ENSMUSG00000079102:009, ENSMUSG00000026727:016 and > > ENSMUSG00000026727:004? > > for example, Cassette exon (skipped exon), Intron retention, Mutually > > exclusive exons, Alternative 3' sites, Alternative 5' sites, > > Alternative first exon. > > > > Thank you very much in advance. > > > > _______________________________________________ > > Bioconductor mailing list > > Bioconductor@r-project.org > > https://stat.ethz.ch/mailman/listinfo/bioconductor > > Search the archives: > http://news.gmane.org/gmane.science.biology.informatics.conductor > > > > _______________________________________________ > Bioconductor mailing list > Bioconductor@r-project.org > https://stat.ethz.ch/mailman/listinfo/bioconductor > Search the archives: > http://news.gmane.org/gmane.science.biology.informatics.conductor > -- Jose M. Garcia Manteiga PhD Research Assistant - Data Analysis in Functional Genomics Center for Translational Genomics and BioInformatics Dibit2-Basilica, 3A3 San Raffaele Scientific Institute Via Olgettina 58, 20132 Milano (MI), Italy Tel: +39-02-2643-4751 e-mail: garciamanteiga.josemanuel@hsr.it [[alternative HTML version deleted]]
ADD REPLY
0
Entering edit mode
Hi Jose, Thanks for your input, will definitely add it to the "to do" list. There are things around BioC, like SplicingGraphs, I will have a closer look to the recent updates and think how to integrate DEXSeq results with this and other packages. Bests regards, Alejandro > Hi Alejandro and list, > Since this is a recurrent topic about alternative splicing with > RNA-Seq and the robust DEXSeq software, are you planning to include > some 'downstream' tool to guide on the classification of the AS events > based on the bam alignments? I known there are some tools like > splicegrapher.py and other few out there but it would be a perfect end > point for the R/DEXSeq package. > Thanks again > Jose > > > > 2014-03-03 9:35 GMT+01:00 Alejandro Reyes <alejandro.reyes at="" embl.de=""> <mailto:alejandro.reyes at="" embl.de="">>: > > Dear Fabrice, > > I think you meant DEXSeq. > To classify events into alternative splicing types it is useful to go > back to the alignment files and visualize the exon-exon junction > reads, > then it becomes obvious which are the events that are giving rise > to the > differences in exon usage. > > Best regards, > Alejandro > > > > > Dear list, > > > > When I use DESeq find different expressed exon in tow > conditions. e.g, > > > > id baseMean baseMeanA baseMeanB > > 1 ENSMUSG00000079102:009 851.0096 1697.09604 4.9231156 > > 2 ENSMUSG00000026727:016 239.6701 478.35562 0.9846231 > > 3 ENSMUSG00000026727:004 155.8972 311.79442 0.0000000 > > > > How can know the Alternative Splicing Event for > > ENSMUSG00000079102:009, ENSMUSG00000026727:016 and > > ENSMUSG00000026727:004? > > for example, Cassette exon (skipped exon), Intron retention, > Mutually > > exclusive exons, Alternative 3' sites, Alternative 5' sites, > > Alternative first exon. > > > > Thank you very much in advance. > > > > _______________________________________________ > > Bioconductor mailing list > > Bioconductor at r-project.org <mailto:bioconductor at="" r-project.org=""> > > https://stat.ethz.ch/mailman/listinfo/bioconductor > > Search the archives: > http://news.gmane.org/gmane.science.biology.informatics.conductor > > > > _______________________________________________ > Bioconductor mailing list > Bioconductor at r-project.org <mailto:bioconductor at="" r-project.org=""> > https://stat.ethz.ch/mailman/listinfo/bioconductor > Search the archives: > http://news.gmane.org/gmane.science.biology.informatics.conductor > > > > > -- > Jose M. Garcia Manteiga PhD > Research Assistant - Data Analysis in Functional Genomics > Center for Translational Genomics and BioInformatics > Dibit2-Basilica, 3A3 > San Raffaele Scientific Institute > Via Olgettina 58, 20132 Milano (MI), Italy > > Tel: +39-02-2643-4751 > e-mail: garciamanteiga.josemanuel at hsr.it > <mailto:garciamanteiga.josemanuel at="" hsr.it="">
ADD REPLY

Login before adding your answer.

Similar Posts
Loading Similar Posts
Traffic: 978 users visited in the last hour
Content Search
Users
Tags
Badges
Help About
FAQ
Access RSS
API
Stats

Use of this site constitutes acceptance of our User Agreement and Privacy Policy.

Powered by the version 2.3.6