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  • wynstep
    Member
    • Jan 2014
    • 11

    Correlation FPKM and RPKM

    Hi everyone!
    I'm trying to evaluate gene expression differences, in breast cancer cells before and after treatment. So I'm working on RNA-seq data (single-end reads).

    I tried to correlate FPKM (CuffDiff output) and RPKM (counts from HTSeq-count, then classic "Mortazavi et al." calculation).
    Reading the CuffLinks website, some papers and other forums, it seems that these values have to be the same for single-end reads data!

    I also filtered miRNAs and other genes shorter then 300bp (could give false FPKM high values).
    I hope that someone can help me!

    Thanks in advace
  • rboettcher
    Member
    • Oct 2010
    • 71

    #2
    You did not include a question or any findings in your post, so what exactly do you want to know?

    Comment

    • dpryan
      Devon Ryan
      • Jul 2011
      • 3478

      #3
      For single-end reads, FPRKM==RPKM. Keep in mind that, due to how it works, the RPKM values produced by cufflinks will almost never be the same as those you compute by hand. Firstly, htseq-count only count uniquely mapped reads, whereas cufflinks will distribute fractional reads counts over transcripts and genes. Also, you likely have a single pre-defined length for each gene, presumably computed by just summing the length of each exon in a "union gene model". I recall that cufflinks tries to determine the actual length and distributions of the transcripts and then uses that.

      BTW, unless you really want to discover new isoforms or genes, you might just directly use the counts from HTSeq-count in DESeq2 (or edgeR or limma).

      Comment

      • wynstep
        Member
        • Jan 2014
        • 11

        #4
        Sorry, you're right! My question is:
        Is possible to obtain equal FPKM and RPKM values? All says "yes", but deeply searching into the literature, I didn't find a protocol to do it or some correlation analysis.

        The best match I've found is this:

        but he tried to correlate crude counts to fpkm (without a great success...)

        Thanks!

        Comment

        • dpryan
          Devon Ryan
          • Jul 2011
          • 3478

          #5
          By definition, an FPKM value computed with single-end reads is also the RPKM value (in fact, this is also true for paired-end reads if you only use reads where both ends map to the same feature). As I mentioned above, the reason that you're getting different values by hand than by cufflinks is that you're using vastly different methods to arrive at both counts and lengths.

          Comment

          • wynstep
            Member
            • Jan 2014
            • 11

            #6
            Originally posted by dpryan View Post
            For single-end reads, FPRKM==RPKM. Keep in mind that, due to how it works, the RPKM values produced by cufflinks will almost never be the same as those you compute by hand. Firstly, htseq-count only count uniquely mapped reads, whereas cufflinks will distribute fractional reads counts over transcripts and genes. Also, you likely have a single pre-defined length for each gene, presumably computed by just summing the length of each exon in a "union gene model". I recall that cufflinks tries to determine the actual length and distributions of the transcripts and then uses that.

            BTW, unless you really want to discover new isoforms or genes, you might just directly use the counts from HTSeq-count in DESeq2 (or edgeR or limma).
            sorry for my ignorance, what's the meaning of FPRKM? Thanks for your answer!
            The reason why I tried to compare FPKM and RPKM, is only to have a value control!
            I believe that I have to follow only one strand of analysis...

            Comment

            • wynstep
              Member
              • Jan 2014
              • 11

              #7
              Originally posted by dpryan View Post
              By definition, an FPKM value computed with single-end reads is also the RPKM value (in fact, this is also true for paired-end reads if you only use reads where both ends map to the same feature). As I mentioned above, the reason that you're getting different values by hand than by cufflinks is that you're using vastly different methods to arrive at both counts and lengths.
              Thank you very much for your explanation!

              Comment

              • dpryan
                Devon Ryan
                • Jul 2011
                • 3478

                #8
                FPRKM was just a typo I meant FPKM

                Comment

                • wynstep
                  Member
                  • Jan 2014
                  • 11

                  #9
                  Originally posted by dpryan View Post
                  FPRKM was just a typo I meant FPKM
                  Ah ok! I was afraid I missed something important!

                  Comment

                  • dpryan
                    Devon Ryan
                    • Jul 2011
                    • 3478

                    #10
                    I should also point you to figure 3D in this paper.

                    Comment

                    • wynstep
                      Member
                      • Jan 2014
                      • 11

                      #11
                      Originally posted by dpryan View Post
                      I should also point you to figure 3D in this paper.
                      I requested the article to my university, so interested! The 3D figure (I can't see it in high resolution for now...) seems really similar to my correlation curve between FPKM and RPKM

                      Thanks a lot!

                      Comment

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