Seqanswers Leaderboard Ad

Collapse

Announcement

Collapse
No announcement yet.
X
Collapse
 
  • Page of 1
  • Filter
  • Time
  • Show
Clear All
new posts
Previous template Next
  • #1

    DESq2 lrt with multiple factors and batch effect

    Dear all,
    I have a question concerning a multiple factor analysis with a batch effect reflecting the day of the library preparation (2 dates). I am using the likrlihood ratio test in DESeq2. My variable of interest is a continious variable indicating how much a person is exposed. Further I want to control for possible confounders sex, age and BMI.

    My first question would be if the design makes sense:

    Code:
    dds <- DESeqDataSetFromMatrix(countData = MyCounts,
                                colData = MyData,
                                design = ~libbatch + sex + age + BMI + Exposure)

dds<-DESeq(dds,test= "LRT",full = design(dds),reduced = ~libbatch)

res<-results(dds,name = "Exposure" ,pAdjustMethod = "fdr")
    or would I need to do something like this:


    Code:
    dds<-DESeq(dds,test= "LRT",full = design(dds),reduced = ~libbatch + sex + age + BMI +)
    And the second question concerning the results:
    Why are so many NAs among the adjusted pvalues? and why are many of them equal?


    res<-results(dds,name = "Expo.delta" ,pAdjustMethod = "fdr")
    baseMean log2FoldChange lfcSE stat pvalue padj
    gene1 13009.48564 -0.0005561894 0.001880162 25.89735 0.0002326616 0.01561069
    gene2 163.28590 -0.0043968404 0.003520945 25.21172 0.0003119647 0.01561069
    gene4 88.93107 -0.0074868961 0.006939026 26.88819 0.0001519605 0.01561069
    gene5 121.15589 -0.0092059826 0.004727699 25.50741 0.0002749380 0.01561069
    ... ... ... ... ... ... ...
    genex 24.22494 -0.0117729650 0.011910591 5.048386 0.5376224 NA
    geney 23.03576 0.0070158920 0.010191693 5.260325 0.5108840 NA

    Many thanks for your help!
    Last edited by krausezuhause; 01-25-2017, 05:09 AM.
    Tags: batch effect, deseq2, lrt, rnaseq
  • #2
    Your reduced design should be "~libbatch + sex + age + BMI", though I'm curious why you explicitly want an LRT.

    The NAs are probably due to independent filtering. I'd have to look up which method the "fdr" correction is using, I only ever use the standard BH method.

    Comment

    • #3
      I did not know you can also correct for a batch effect using the Wald test.
      How would the model look like then? the reduced model is ignored in a Wald test.

      Comment

      • #4
        Your full design is the same for Wald and LRT, only the latter needs a reduced design.

        Code:
        dds <- DESeqDataSetFromMatrix(countData = MyCounts,
                                colData = MyData,
                                design = ~libbatch + sex + age + BMI + Exposure)
dds<-DESeq(dds)
res <- resuls(dds) # I think this will default to Exposure, being the last variable in the design

        Comment

        • #5
          and what would be the interpretation of this model?

          dds <- DESeqDataSetFromMatrix(countData = MyCounts,
          colData = MyData,
          design = ~libbatch + sex + age + BMI + Exposure)

          dds<-DESeq(dds,test= "LRT",full = design(dds),reduced = ~libbatch)
          Only correcting for batch effect and the other confounders are ignored?

          Thanks for your reply!

          Comment

          • #6
            ? It's the same model, you're still correcting for the batch and accounting for changes in the confounders. You're just getting your p-value according to whether the log2FC of "Exposure" is different from 0 (Wald test) as opposed to whether the full or reduced models fit better (LRT).

            Comment

            • #7
              So If I understand correctly now, with the LRT above I account for batch and confounders but can not relate the significant genes to exposure?

              I get about 300 significant hits with the LRT (reduced = ~libbatch) model, but 0 hits with the Wald or LRT (reduced = ~libbatch + sex + age + BMI )

              Comment

              • #8
                Your confounders are masking any effect of exposure. Sorry your results didn't turn out better.

                Comment

                • #9
                  Many thanks for the explanation!

                  Comment

                  Previous template Next

                  Latest Articles

                  Collapse
                  • seqadmin
                    Best Practices for Single-Cell Sequencing Analysis
                    by seqadmin



                    While isolating and preparing single cells for sequencing was historically the bottleneck, recent technological advancements have shifted the challenge to data analysis. This highlights the rapidly evolving nature of single-cell sequencing. The inherent complexity of single-cell analysis has intensified with the surge in data volume and the incorporation of diverse and more complex datasets. This article explores the challenges in analysis, examines common pitfalls, offers...
                    Yesterday, 07:15 AM
                  • seqadmin
                    Latest Developments in Precision Medicine
                    by seqadmin



                    Technological advances have led to drastic improvements in the field of precision medicine, enabling more personalized approaches to treatment. This article explores four leading groups that are overcoming many of the challenges of genomic profiling and precision medicine through their innovative platforms and technologies.

                    Somatic Genomics
                    “We have such a tremendous amount of genetic diversity that exists within each of us, and not just between us as individuals,”...
                    05-24-2024, 01:16 PM
                  View All

                  ad_right_rmr

                  Collapse

                  News

                  Collapse
                  Topics Statistics Last Post
                  New Method for DNA Sequence Amplification by seqadmin
                  Started by seqadmin, Yesterday, 08:18 AM
                  0 responses
                  13 views
                  0 likes
                  		 Last Post seqadmin
                  by seqadmin
                  Yesterday, 08:18 AM  
                  New Tools Enhance Single-Molecule DNA Analysis with Minimal Samples by seqadmin
                  Started by seqadmin, Yesterday, 08:04 AM
                  0 responses
                  12 views
                  0 likes
                  		 Last Post seqadmin
                  by seqadmin
                  Yesterday, 08:04 AM  
                  SIX2 Protein Identified as a Key Player in Prostate Cancer Treatment Resistance by seqadmin
                  Started by seqadmin, 06-03-2024, 06:55 AM
                  0 responses
                  13 views
                  0 likes
                  		 Last Post seqadmin
                  by seqadmin
                  06-03-2024, 06:55 AM  
                  Genetic Mosaicism More Prevalent Than Previously Thought by seqadmin
                  Started by seqadmin, 05-30-2024, 03:16 PM
                  0 responses
                  27 views
                  0 likes
                  		 Last Post seqadmin
                  by seqadmin
                  05-30-2024, 03:16 PM  
                  View All
                  Working...
                  X