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  • #1

    Convert Maq's out put to fasta/fastq?

    Hi!

    I would like to know whether it's possible to convert Maq's out put (out.aln.txt file, after running maq mapview or the unmapped reads files, by incorporating the u option in maq map) back to a fasta/fastq format so that it can be re-used in Maq/ other assemblers.

    Thanks
    Tags: fasta, maq
  • #2
    Not totally sure, but I know that the Vancouver Short Read Analysis Package has a tool for converting Maq to BED (http://vancouvershortr.wiki.sourcefo...t/ConvertToBed) and that Aaron Quinlan's BEDTools have a script for generating BED --> fasta.

    Hope that helps! Definitely not the most direct way though for sure. :P

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    • #3
      R/BioConductor can do this easily, by importing the MAQ output into an AlignedRead object, creating a ShortReadQ object from that, and then exporting a fastq file.
      @1
      NNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN
      +
      """"""""""""""""""""""""""""""""""""

      Comment

      • #4
        mapview to fastq:

        maq mapview maq_map_file |awk '{print "@"$1"\n"$15"\n+\n"$16}' > fastq_file

        mapview to fasta:

        maq mapview maq_map_file |awk '{print ">"$1"\n"$15}'> fasta_file

        unmapped reads file to fastq

        awk '{print "@"$1"\n"$3"\n+\n"$4}' unmapped_reads_file > fastq_file

        Comment

        • #5
          I've tried your suggetions. I'm able to create the fastq files with awk and convert that to bfq format required for MAQ. But running MAQ with the bfq files gives me a error:
          Assertion failed: (fp_bfq_l), function ma_match.cc, line 557.
          Any suggestions why this might happen?
          Last edited by bea; 06-04-2009, 12:50 AM.

          Comment

          • #6
            If your fastq name is too long, >35 characters, Maq will delete the front exceed characters, so at this situation, you can't get the actual primary fastq back.
            And the primary fastq paired-end reads, every reads in pe1.fastq file should be corresponding to the same line of pe2.fastq file, so you should sort the name of reads in mapview file at first.

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