Question: How to merge replicates of mapped reads out of Tophat for pathview and gage

Parharn · 07-07-2014, 01:27 AM

Hi, I have three biological replicates for my experiment. I wonder how should I merge the accepted_hits.bam out of Tophat for doing Pathview/gage analysis for "RNA-seq Pathway and Gene-set analysis workflow"? Let's name the accepted_hits.bam replicates as 1.bam 2.bam and 3.bam for the sake of short writing.

I have a thread on biostars.org
https://www.biostars.org/p/105503/

TiborNagy · 07-07-2014, 05:09 AM

The documentation suggest you need to use a differential expression analysis solution: DESeq2, Cufflinks, Limma and after that use gage. These packages handle the replicates.

bigmw · 07-28-2014, 12:31 PM

You would need to index all of them and get .bam.bai file for each one of them. Then collect all .bam and .bam.bai files into the same directory (i.e. tophat_all as in the demo code). Then all samples will be scanned in by function summarizeOverlaps at step 1: Count the reads mapped to each gene.
If you read carefully, actually all details are covered in Section 3.1 Preparation: read mapping and package installation:
http://www.bioconductor.org/packages...eqWorkflow.pdf

Quote:

Originally Posted by Parharn

Hi, I have three biological replicates for my experiment. I wonder how should I merge the accepted_hits.bam out of Tophat for doing Pathview/gage analysis for "RNA-seq Pathway and Gene-set analysis workflow"? Let's name the accepted_hits.bam replicates as 1.bam 2.bam and 3.bam for the sake of short writing.

I have a thread on biostars.org
https://www.biostars.org/p/105503/

bigmw · 10-27-2014, 01:29 PM

That’s the joint workflow for the users’ convenience. But GAGE/Pathview does not really require a external differential expression analysis step, as shown in the native workflow. For details:
http://bioconductor.org/packages/rel...eqWorkflow.pdf

Quote:

Originally Posted by TiborNagy

The documentation suggest you need to use a differential expression analysis solution: DESeq2, Cufflinks, Limma and after that use gage. These packages handle the replicates.

Parharn · 10-27-2014, 02:03 PM

Yes, later I discovered it but thanks to saying anyway

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07-07-2014, 01:27 AM	#1
Parharn Member Location: Sweden Join Date: Jul 2013 Posts: 84	Question: How to merge replicates of mapped reads out of Tophat for pathview and gage Hi, I have three biological replicates for my experiment. I wonder how should I merge the accepted_hits.bam out of Tophat for doing Pathview/gage analysis for "RNA-seq Pathway and Gene-set analysis workflow"? Let's name the accepted_hits.bam replicates as 1.bam 2.bam and 3.bam for the sake of short writing. I have a thread on biostars.org https://www.biostars.org/p/105503/

07-07-2014, 05:09 AM	#2
TiborNagy Senior Member Location: Budapest Join Date: Mar 2010 Posts: 329	The documentation suggest you need to use a differential expression analysis solution: DESeq2, Cufflinks, Limma and after that use gage. These packages handle the replicates.

10-27-2014, 02:03 PM	#5
Parharn Member Location: Sweden Join Date: Jul 2013 Posts: 84	Yes, later I discovered it but thanks to saying anyway