Using HTseq and DEseq2 for RNAseq quantitation, format of input data?

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Question: Using HTseq and DEseq2 for RNAseq quantitation, format of input data?

0

20 months ago by

reubenmcgregor88 • 50

reubenmcgregor88 • 50 wrote:

Hi all,

For clarities sake my experimental setup is: 2 conditions (treated + non treated), with 3 replicated per condition.

This was sequenced using paired end Hiseq.

I mapped to reference genome using TopHat2 and counted the reads using htseq-count for all of the alignments separately.

I am about to run DESeq2 on these outputs.

Clearly my Factor1 and Factor 2 are treated and non treated respectively.

My qyesiotnv is ca I use a dataset collection as an input. So can I input the replicates as three input files, or do I have to somehow merge the replicated form the treatment and then the replicates from non-treated before inputting into DESeq2?

Please help!?

Thanks,

Rueben]

rna-seq collections htseq_count deseq2 htseq • 1.5k views

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modified 11 months ago by Jennifer Hillman Jackson ♦ 25k • written 20 months ago by reubenmcgregor88 • 50

1

11 months ago by

Jennifer Hillman Jackson ♦ 25k

United States

Jennifer Hillman Jackson ♦ 25k wrote:

Hello,

Collections can be used (and is an accepted input type of the tool form). How-to is explained in the Galaxy tutorials here: https://galaxyproject.org/learn/

Thanks, Jen, Galaxy team

ADD COMMENT • link written 11 months ago by Jennifer Hillman Jackson ♦ 25k

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