DESeq2 object problem with padj
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7.7 years ago
pennakiza ▴ 60

Hello all,

RNA-seq DE analysis noob here so please bear with my silly question!

So, I have tximported my salmon data of paired-end RNA seq reads and I am trying to use DESeq2 to analyze the differential expression for two conditions (screen and treatment) in 8 different patients.

I use this bit of code:

coldata<-data.frame(con=s2c$condition)
rownames(coldata)<-colnames(txi)
dds <- DESeqDataSetFromTximport(txi, colData=coldata, design= ~con)
dds <- dds[ rowSums(counts(dds)) > 1, ] 
dds<-DESeq(dds)
res<-results(dds)

but I get padj values in all my genes around 0.9!

On the other hand, if I use replicates (patient1, patient2 and so on) I got some significant padjs but my MA plot is a small vertical line!

Maybe I shouls use both factors (replicate and condition) on my design? How can I do that?

Could someone please help me understand what I am doing wrong?

Thank you very much!

Pen

DESeq2 padj • 2.9k views
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What do you mean by "if I use replicates"? I presume there are replicates in the example you posted.

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I mean if I use replicates as a comparison in design, instead of condition. So if instead of comparing "treated" and "screen" samples, I compare "patient 1" to "patient 2" and so on, regardless the condition?

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1) please list all the samples names and the organism they come from. 2) then tell us what you are comparing

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So, my table looks like that: [https://ibb.co/npWGfa]

where replicates is the patient the sample comes from, so P1= patient 1, P2= patient2 and so on. They are samples from human cancer patients, taken before and after treatment.

What I am looking for is to compare the gene expression between the patients, before and after treatment.

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Were you able to find a solution to this? I am in a similar situation with my data currently!

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