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  • SEQanswer
    Junior Member
    • Jun 2011
    • 2

    Trouble converting SAM to BAM, all 'chrM' recognized as '*'?

    Hello
    I'm trying to convert GERALD output, export.txt files, to BAM.
    I used samtools export2sam.pl to convert export.txt to SAM but when using samtools -bt to convert SAM to BAM, all the chrM are being recognized as '*'.
    such as
    [sam_read1] reference 'chrM' is recognized as '*'.

    Can anyone help on why are chrM's causing issues here?

    Thanks in advance
    Jay
  • ECO
    --Site Admin--
    • Oct 2007
    • 1360

    #2
    Hey Jay,

    Let me know what new username you'd like (via PM, or email admin@), as that one ain't gonna work.

    Thanks,
    -=Eric

    Comment

    • SEQanswer
      Junior Member
      • Jun 2011
      • 2

      #3
      Issue solved, thanks for help SEQanswers.

      Comment

      • ECO
        --Site Admin--
        • Oct 2007
        • 1360

        #4
        Jay...posting your solution is helpful too...it may help others in the future.

        Comment

        • jjpurwar
          Junior Member
          • Jun 2011
          • 9

          #5
          How did you resolve this issue? Please help!

          Comment

          • jjpurwar
            Junior Member
            • Jun 2011
            • 9

            #6
            I figured out the solution to my problem. Turns out that my sam file header had to be in the right format:

            The first line needs to be header.
            The second line needs to be a dummy read group line
            The next lines need to contain the chromosomes and their lengths.

            An example of a good header is as follows:

            @HD VN:1.0 SO:unsorted
            @RG ID:unknownReadGroup SM:unknownSample
            @SQ SN:chrI AS:ce6_32r_index LN:15072421
            @SQ SN:chrII AS:ce6_32r_index LN:15279323
            @SQ SN:chrIII AS:ce6_32r_index LN:13783681
            @SQ SN:chrIV AS:ce6_32r_index LN:17493785
            @SQ SN:chrM AS:ce6_32r_index LN:13794
            @SQ SN:chrV AS:ce6_32r_index LN:20919568
            @SQ SN:chrX AS:ce6_32r_index LN:17718854

            Once I deleted all the @SQ , @PG, @HD lines from my sam file and appended the above header text file to my sam file and tried to convert it to a bam - it worked beautifully.

            Comment

            • jdilts
              Member
              • May 2012
              • 10

              #7
              What was wrong with the original header?

              What was wrong with the original header?

              Comment

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