Poor dispersion fit in DESeq2
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Entering edit mode
10 weeks ago
Ben ▴ 20

I am attempting to run DESeq2, edgeR, and limma-voom to find DEGs between a condition sensitivity with factors 'lineage'.

My dispersion model doesn't seem to fit well to my data, but I wanted to check if it was acceptable, here is my code:

keep <- edgeR::filterByExpr(y = counts, group = sensitivity) # default filterByExpr settings
counts <- counts[keep, ]
dds <- DESeqDataSetFromMatrix(counts, metadata, design = ~ lineage + sensitivity)
dds <- DESeq(dds, fitType = fit_type, minReplicatesForReplace = Inf)
plotDispEsts(dds)

Here is my dispersion model fitted to my data using parametric fit type.

parametric

And here is the model with the local fit type.

local | 200

Any thoughts?

deseq2 RNA-seq edgeR limma • 454 views
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Yep. Thats a pretty weird looking fit.

One thing that is noticable is that the gene-est dispersions look to be bimodel in the mid-ranges. One of your factors is "lineage". Is it possible that there are different cell types, and the genes with lower dispersion represent genes expressed in both cell types, and those with low dispersion represent those that are only expressed in one cell type?

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Yes, agreed definitely looks bimodal. Lineage is actually about 4 or 5 different cell lineages. I couldn't think of a quick way to determine which genes were differentially expressed between these, so I just individually ran a couple of lineages with the design ~ sensitivity.

My dispersions still look quite bimodal. Any ideas?

Bowel:

bowel dispersion

Lung (ymin = 1e-03 as there as several outliers at 1e-08):

lung dispersion

CNS (ymin = 1e-04 as there as several outliers at 1e-08):

cns dispersion

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Entering edit mode

I think you probably need input from Mike Love (@mikelove). He hangs around here sometimes, but is more active on support.bioconductor.org, so you might try cross posting there.

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I have cross-posted, thanks for your help!

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