t.test to determine the P-value in DESeq2
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@4fedfa78
Last seen 2.1 years ago
Japan

Hello,

For running the DESeq2 I am using the below command to do the t.test for determining the p-value, to separate those genes which are "significant" expressed, I also used the Excell sheet for determining the "Significant" genes expression, but in both cases, some of the genes which are significantly expressed in the original data, are expressing "Non-significantly" in my analysis. is there someone to advise me where would be the problems? Many thanks


Pvalue=c()
carrierindex=which(CountsNorm$condition=="carrier")
noncarrierindex=which(CountsNorm$condition=="noncarrier")
for (i in 1:nrow(Counts)){
  Pvalue=c(Pvalue,t.test(Counts[i,carrierindex],Counts[i,noncarrierindex])$p.value)
}
DESeq2 • 2.9k views
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That command has nothing to do with DESeq.

Applying a simple t-test to RNAseq counts is wrong.

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so could you please advise me what kinds of test should I apply?

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Can you explain why you won't use DESeq2? Why are you tagging your questions with it and not using it?

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I used the below commands for running the DESEq2,

library(DESeq2)

count_matrix <- as.matrix(read.csv("~/Desktop/sample.csv", row.names = 1))

head(count_matrix, 2)

View(count_matrix)

condition <- factor(c(rep("carrier",3), rep("noncarrier", 3)))

sampleTable <- data.frame(condition = as.factor(condition))

rownames(sampleTable) <- colnames(count_matrix)

sampleTable

deseq <- DESeqDataSetFromMatrix(countData = count_matrix,

                            colData = sampleTable,

                            design = ~condition)

deseq$condition <- relevel(dds$condition, ref = "noncarrier")

d.deseq <- DESeq(deseq)

res<- results(d.deseq)

res<- results(d.deseq, alpha = 0.05 )

summary(res)

but the results are as below, and the DEGs are very less:

out of 32159 with nonzero total read count

adjusted p-value < 0.05

LFC > 0 (up) : 23, 0.072%

LFC < 0 (down) : 10, 0.031%

outliers [1] : 168, 0.52%

low counts [2] : 2542, 7.9%

(mean count < 0)

[1] see 'cooksCutoff' argument of ?results

[2] see 'independentFiltering' argument of ?results

could you please help me to know where my mistake is, it is about 6 months since I am trying different ways to solve the problems, that is why I thought maybe by using t.test I would be able to solve the problem, I would really appreciate your advise and help in my this tough time.

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This is likely not a DESeq2 problem. Either your study is underpowered (3 vs 3 definitely is) or batch effects make things difficult. The vignette covers diagnosis of batch effects via PCA. In any case, switching to underpowered tests like t or Wilcox-test is not going to provide any benefit.

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Many thanks for your answer. sorry, I did not get what it means by underpowered or batch effects, could you please make it clear? Thanks in advance

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In this case I recommend taking courses or tutorials on basics of RNA-seq and stats/experimental design so you get a background before going into analysis. Among other resources, HBC has great tutorials: https://hbctraining.github.io/DGE_workshop/lessons/04_DGE_DESeq2_analysis.html

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You can Google those terms. You can't expect a discussion board to do everything for you.

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ATpoint ★ 4.6k
@atpoint-13662
Last seen 1 day ago
Germany

I am not sure what you are asking. You do two completely different types of statistical tests and find that they disagree. Of course they do, specialized software like DESeq2 would not have been developed if simple tests would do just as fine. There is an extensive stack of literature motivating the use of testing frameworks like DESeq2, please read the underlying papers from Michael Love (Love 2014) and others for example the literature on limma and edgeR from Gordon Smyth lab. There are also plenty of forum and community posts highlighting why t-tests are inferior and do not apply here, especially in the presence of low sample size (replicates).

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Many thanks for your kind reply. I understand, could you please advise me what kind of test should I apply? if possible could you please give me the commands?

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