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  • fznajar
    Member
    • Jan 2012
    • 35
    #1

    Blast to SAM

    I converted my BlasyN to SAM using:

    blast2sam.pl <blastN file> > <output file>

    I then tried to generate a "bam" file using:

    samtools view -bT <reference.fasta> <sam file> -o <bam output>


    I got the following output:
    [sam_header_read2] 0 sequences loaded.
    [samopen] no @SQ lines in the header.
    [sam_read1] missing header? Abort!

    Any help?

    Thanks in advance
    Tags: None
  • seqeve
    Junior Member
    • Oct 2012
    • 4
    #2
    If the header is absent from the SAM file use the command below, where reference.fa is the reference fasta file used to map the reads:
    samtools view -bT reference.fa test.sam > test.bam

    If the header information is available:
    samtools view -bS test.sam > test.bam
    Dave's Wiki | SAMTools
    http://davetang.org/wiki/tiki-index.php?page=SAMTools
    Dave's Wiki


    I would suggest trying -bS, even though this is opposite to what this wiki says?

    Comment

    • fznajar
      Member
      • Jan 2012
      • 35
      #3
      Thank you seqeve.
      I am still getting the same error above.
      Best

      Comment

      • kmcarr
        Senior Member
        • May 2008
        • 1181
        #4
        Originally posted by fznajar View Post
        I converted my BlasyN to SAM using:

        blast2sam.pl <blastN file> > <output file>

        I then tried to generate a "bam" file using:

        samtools view -bT <reference.fasta> <sam file> -o <bam output>


        I got the following output:
        [sam_header_read2] 0 sequences loaded.
        [samopen] no @SQ lines in the header.
        [sam_read1] missing header? Abort!

        Any help?

        Thanks in advance
        Try providing a reference index file instead of the reference fasta itself.

        Code:
        samtools faidx <reference.fasta> [Creates reference.fasta.fai]

samtools view -bt <reference.fasta.fai> -o <bam.out> <sam.in>

        Comment

        • fznajar
          Member
          • Jan 2012
          • 35
          #5
          Thanks all. It turned out my fasta reference sequence from illumina has a format problem as each sequences is one single long line. I just had to reformat it and it worked.

          Thanks again for your help

          Comment

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