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  • gigigou
    Member
    • May 2012
    • 31

    about MACS

    I am using MACS to find peaks of chip seq data.
    I get a question about the P value.
    General MACS gets many peaks from a sample, much more than SISSRs. But not all the peaks are reliable. So I want to filter the peaks MACS found.
    In the command line there is an option -p followed by a p value. If it is set too strictly, e.g. 1e-50, there may be no peaks found, otherwise, e.g. 1e-10, there may be too many peaks.
    So I want to ask generally which P value is suitable, i.e., on which P value the peaks found are reliable?
    Thank you!
  • ishmael
    Member
    • Jul 2008
    • 17

    #2
    I would surggest you generate the tdf file of the coverage of genome, and load the tdf and peak lists of different p cutoff of MACS and SISSRs.
    And I think the shapes of the peaks of coverage will give you more clues.

    Comment

    • gigigou
      Member
      • May 2012
      • 31

      #3
      Originally posted by ishmael View Post
      I would surggest you generate the tdf file of the coverage of genome, and load the tdf and peak lists of different p cutoff of MACS and SISSRs.
      And I think the shapes of the peaks of coverage will give you more clues.
      Thank you.
      I'm new in chip seq. And I don't quite understand what is "tdf file of the coverage of genome". Could you please tell me how to generate this file?

      Comment

      • ishmael
        Member
        • Jul 2008
        • 17

        #4
        Sorry I didn't explain clearly. tdf is the coverage file format of IGV, a genome browser.
        I think you'd better to generate the coverage files of chip-seq, and load them into the browser. And than you may load the peak lists you got from different p-value cutoffs and different softwares. Your eyes will give you some clues which peak list is the better choice from the shape of the peaks.

        Comment

        • gigigou
          Member
          • May 2012
          • 31

          #5
          Originally posted by ishmael View Post
          Sorry I didn't explain clearly. tdf is the coverage file format of IGV, a genome browser.
          I think you'd better to generate the coverage files of chip-seq, and load them into the browser. And than you may load the peak lists you got from different p-value cutoffs and different softwares. Your eyes will give you some clues which peak list is the better choice from the shape of the peaks.
          I see.
          But what I want is to have a general p value to ensure that I can indeed get some peaks which are reliable. Cause this is automatically done by my pipeline.
          According to your words I think there may be no such fixed p value, so I think I'd better make the p value as a parameter for users to determine.
          Thank you very much for your patient explaine!

          Comment

          • ishmael
            Member
            • Jul 2008
            • 17

            #6
            The quality and nature of different chip are different, I think.
            So it is alway not bad to check the coverage manually.
            If you want a reliable peak list, think about IDR or MAnorm if the replicate samples are availble.

            PS, check your private message box

            Originally posted by gigigou View Post
            I see.
            But what I want is to have a general p value to ensure that I can indeed get some peaks which are reliable. Cause this is automatically done by my pipeline.
            According to your words I think there may be no such fixed p value, so I think I'd better make the p value as a parameter for users to determine.
            Thank you very much for your patient explaine!

            Comment

            • DNASpeaks
              Junior Member
              • Oct 2012
              • 5

              #7
              Hi Everyone
              I am doing chip seq analysis using galaxy. I have paired end data and I am having trouble running MACS on my bam file -
              Looks like galaxy takes only eland multi format as input and I am not sure of the format -

              Do you think converting my bam files to bed files (by creating a BEDPE format) would help? I do not have bed tools installed, I also would like to know if the BAM files need to be sorted before I convert them into BED files -
              I appreciate any help or suggestions.
              Thanks.

              Comment

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