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  • trouble repeating a BWA alignment command

    I aligned a fastq file to a refseq data base successfully as follows:

    create an index:

    bwa index -p RefSeqbwaidx -a bwtsw /mnt/fred/home/efoss/gene_databases/refGene.txt.07Jun2010.fa

    (
    The refGene.txt.07June2010.fa file has a format like this:

    >NM_002697
    CGGAGGAGCAGCGAGTCAAGATGAGAGTTCAGCCGCGGCGGCAGCAGCAGCAGACTGGAAAAGTAAGAAGAGCTTTCCTGCCTTTTTAATTACCAAACTA
    CTCTCAGTTTTCAATGAATCAGTTCAAAGAAAGAATGCAGTCTTTCTATACCTGACTCAAGAATGAACAATCCGTCAGAAACCAGTAAACCATCTATGGA
    GAGTGGAGATGGCAACACAGGCACACAAACCAATGGTCTGGACTTTCAGAA
    )


    I align my reads:

    bwa aln -t 6 RefSeqbwaidx /mnt/fred/home/efoss/sequence_files/FASTQ_files/sequence_r1.fq > sequence_r1.fq.bwa

    and I convert the output to SAM format:

    bwa samse RefSeqbwaidx sequence_r1.fq.bwa /mnt/fred/home/efoss/sequence_files/FASTQ_files/sequence_r1.fq > sequence_r1.fq.sam

    I look into the SAM file and everything looks good. Now I go to align the corresponding "r2" file from the same experiment:

    bwa aln -t 6 RefSeqbwaidx /mnt/fred/home/efoss/sequence_files/FASTQ_files/sequence_r2.fq > sequence_r2.fq.bwa

    The alignment takes a similar amount of time, the messages reported back as the computer is working look the same, but then in the end my sequence_r2.fq.bwa file is empty. Does anyone have an idea about what is going on?

    Thank you.

    Eric

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