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  • Extract perfectly mapped reads from SAM/BAM file

    Hi,
    Given a SAM or BAM file, does anyone know how to identify which paired-sequences map perfectly to the reference? By perfectly mapped, I mean that the query is identical to the the reference (or its reverse complement).
    I'm fine using either command-line tools or programming.
    Many thanks,
    Graham

  • #2
    Hi,
    I think you can look at the NM tag in the SAM/BAM file. If both reads of a pair have NM:i:0 than the match is perfect.

    Dario

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    • #3
      Make sure that there is also no soft-clipping in the cigar if you want the full read aligned.

      Comment

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