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  • #1

    Normalizing by Library Amount

    I got my Seq data back and processed with bow tie and htseq and I have my mapped gene counts... in my library I see that this is how much DNA was used for sequencing by the staff

    615 ng ---- Sample 1
    423 ng ---- Sample 2
    426 ng ----- Sample 3


    Can I divide the total mapped reads by these numbers to get a kind of weighted normalization?

    What would be the danger of doing that?
    Tags: None
  • #2
    Normalized to the total mapped reads would be more reasonable.

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    • #3
      use DESeq or edgeR ( in R ) to normalize and check for DE genes

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      • #4
        Originally posted by NicoBxl View Post
        use DESeq or edgeR ( in R ) to normalize and check for DE genes
        I use DESeq2 and I print out the normalized values then do a ttest of my own but my pvalues are nothing like in DESeq2.

        I use this code to print out normalized values.

        normalizedCounts <- t( t(counts(dds)) / sizeFactors(dds) )

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        • #5
          why do you use a ttest and not DESeq test (based on negative binomial) ? RNA-Seq data do not follow a normal distribution.

          for normalized count, you can use also : normalizedCounts <- counts(dds,normalized=TRUE)

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          • #6
            Originally posted by NicoBxl View Post
            why do you use a ttest and not DESeq test (based on negative binomial) ? RNA-Seq data do not follow a normal distribution.
            Well there we go... I guess DESeq2 doesn't perform ttest...

            Can you reference some quality sources to get familiar with negative binomial theory

            Comment

            • #7
              read DESeq paper : http://genomebiology.com/2010/11/10/R106 and also DESeq vignette that is pretty well done.
              or maybe edgeR paper also

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