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  • #1

    Removing duplicate reads for tophat?

    Hello.

    I have two human single end RNA seq data generated from Solexa.
    Yesterday, I ran fastqc using my data and the program reported that two data have a little amount of duplicated reads.

    Should I remove this before processing Tophat?
    And is there any programs which can be used for such purpose?

    Thanks!!
    Tags: None
  • #2
    A small amount of duplication is going to be present in almost any RNA-Seq library. I would not remove these before running TopHat or any other aligners.

    There are threads on this forum where this issue has been discussed in great detail, inncluding one which has a link to a mathematically rigorous treatment of the question by lh3, a senior user. Searching the forum with "duplicate reads" should point you in the right direction.

    Best of luck,

    Shurjo

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    • #3
      Thanks shurjo!

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