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  • wri_ichp
    Junior Member
    • Feb 2016
    • 1

    Total RNAseq multiple mapping issue

    We are running paired-end total RNA (using blood) on HiSeq and after adapter and quality trimming (Q>30), we use tophat2 for alignment. We are getting about 90% overall mapping, but around 80% of those are mapping to multiple locations.

    I am pretty sure this is way too high, but don't know what the issue is. Are there any recommendations for how we can reduce the multi-mapping or ideas on what might have caused it. Thanks!
  • Brian Bushnell
    Super Moderator
    • Jan 2014
    • 2709

    #2
    Mapping to a transcriptome will have a high rate of multiple mapping because the same references occur multiple times. If you want unique mapping, map to the genome instead, using a splice-aware aligner.

    Also, trimming to Q30 will reduce the length of your reads and bias your data with no real advantage. Q10-12 will give you much better results. Short reads will multi-map more because they contain less information.

    Comment

    • Michael.Ante
      Senior Member
      • Oct 2011
      • 127

      #3
      I would rather guess, that you have rRNA contamination in your sample, or highly expressed transcripts originating from a cluster of similar genes. Check your reads with FastQC and if detected, blast your over-represented sequences. You can also use the repeat-masker to analyse your alignment towards rRNA and other elements.

      Comment

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