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  • Bowtie not mapping (even) perfect matches ?

    Hello everybody,

    I am a little worried since about half of my reads do not align, although they have exact full-length matches in the my dataset.

    I run bowtie with the command line:

    ./bowtie-0.12.9/bowtie myindex -a -S -p 32 -r ibis100.raw ibis100.sam

    As the command line says, I used raw reads without quality scores as an input.

    Typical sam line for a read that matches 100% the reference:

    10423427 4 * 0 0 * * 0 0 GTTATTCATTCACTACTACAGCTGAGCGTGAAATTGTAAGAGATATTAAAGAGAAACTTAGTTATGTAGCCT IIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIIII XM:i:0

    The vast majority of reads are perfect alignments when checked using blast, my understanding is that the -a option should cause them to be reported all, and still, they do not align properly.

    Has anybody any thought about what could be the cause of that? I find it really weird and have not been able to find an explanation so far.

    All the best,

    Yvan

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