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  • ramirob
    Member
    • Apr 2012
    • 16

    [sam_read1] reference 'chrN.fa' is recognized as '*'

    Hello,

    I aligned some human samples with Casava, and then converted the alignments to SAM using samtools:

    llumina_export2sam.pl --read1=file_R1.export.txt.gz --read2=file_R2.export.txt.gz > file.sam

    Then I try to convert to bam:

    samtools view -bt genome.fa.fai file.sam > file.bam

    but I get a lot of

    [sam_read1] reference 'chr8.fa' is recognized as '*'.
    [sam_read1] reference 'chr11.fa' is recognized as '*'.
    etc.

    There was a similar thread that suggested changing the header as follows:

    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:1771885


    where do I get all of that information? I also might have to do this over and over again so I was looking for some software or precise ways so that I can write a script to do it.

    Thanks in advance,

    Ramiro
  • naman.neoanderson007
    Junior Member
    • Mar 2013
    • 1

    #2
    Hi, Ramiro

    I have just entered in 'seqanswers' and saw your question

    I suggest you to check your GENOME file - "genome.fa.fai"
    Is it in proper FASTA format ?

    Correct FASTA formated GENOME file will solve your problem.

    Comment

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