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  • Mammoth
    Junior Member
    • Jun 2019
    • 2

    Bowtie1: Reads don't get randomly distributed on direct repeat

    Hi all,

    I am mapping small RNA sequencing reads with bowtie1.2.2 to a locus that encodes a direct repeat with the exactly(!) the same sequence repeated 19 times. I don't allow mismatches, and ask to get back only one alignment:

    bowtie index clippedreads.fq --best --strata -M 1 -v 0 -S | \
    samtools view -Sb -F 4 - |\
    samtools sort - -o outfile.bam

    (or alternatively --best -k 1 -v 0; however, it does not really make a difference in my hands)

    A couple of thousand reads are mapping to that locus (all these reads have the same sequence of course), and based on the bowtie1 manual I would assume they are randomly (and roughly equally) distributed across the 19 repeat units. However, what I get is one or two of the repeat units are highly covered, and the rest is distributed as expected (see picture):
    Click image for larger version

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    Weirdly, the peak shifts with different libraries, but is otherwise nicely reproducible.
    I was wondering what is going on, why the repeat units are not equally covered, or how this can be handled?

    Thanks a ton! Any suggestion is highly appreciated.
  • pmiguel
    Senior Member
    • Aug 2008
    • 2328

    #2
    Looks more-or-less random to me. How many standard deviations from the mean number of hits/repeat are the high and low-hit repeat counts?

    --
    Phillip

    Comment

    • Mammoth
      Junior Member
      • Jun 2019
      • 2

      #3
      Dear Phillip,

      Thank you for your reply. The biggest peak is around 4 standard deviations larger than the mean, the lowest one 2 SD. That seems quite a bit for a random distribution, or not?

      Comment

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