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  • BWA trim doesn’t work.

    I tried to run BWA with trimming those low-quality bases around the end of read. And command is like:
    Code:
    /share/bin/bwa aln -t 7 -I -q 20 ****.txt.gz > ****.sai
    Here -I is to convert Illumina format to sanger
    However when I check the generated sam file, I can still see lines like:
    Code:
    HWI-ST150_0131:3:1:5473:1943#0  133 X   113713314   0   35M5S   =   113713314   0   TNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN    ########################################    XC:i:35
    Shouldn't the crappy sequences trimmed? Or my command has some problems?thx

  • #2
    In here for 133 - the samtools flags: http://picard.sourceforge.net/explain-flags.html

    you get:

    Summary:
    read paired
    read unmapped
    second in pair

    So the read is unmapped:

    Also see this thread from today about bwa-mapped reads with the unmapped flag:

    Discussion of next-gen sequencing related bioinformatics: resources, algorithms, open source efforts, etc


    Chris
    Last edited by cjp; 11-28-2011, 03:58 AM. Reason: explain what 133 is

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