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  • bwa question: quality discrepancy between a color-space alignment and its csfastq

    I am using bwa to perform color-space alignments. I found that the quality line of a mapped read is totally different from its original value in the csfastq file.

    ==================================
    Here is an example:

    The record in the sam file:
    solid_XX:853_13_240 0 18 48162088 37 48M * 0
    0 TCATGAATATAAAACAAGGCCCCTGCAGTCTGGTCCACAGGCCCCCAT VLZ][!!]]]!!TT]ZWSW]]]PO]VOBIRV]UOPQXQEFKNIP]O8
    3 XT:A:U CM:i:3 X0:i:1 X1:i:0 XM:i:2 XO:i:0 XG:i:0 MD:Z:6T3T0C36

    And the original csfastq record is as follows:
    @solid_XX:853_13_240/1
    GGCTCGNATTANCACCAGATAAAGCTCGCGGCACGACCCGATAAAACTC
    +
    =03>>4"7=>:"</<;682<;=>)=851(81<;15269/-023-:<*%%
    ======================================

    I am a bit confused by this discrepancy. Can anyone help? Thanks.

  • #2
    Which version is this? It should be fixed in the latest version. If the latest still produces alignment like this, please let me know. Thanks.

    Comment


    • #3
      bwa 0.5.7 (just downloaded from SF)

      Comment


      • #4
        I see. I misread the email. The quality in fastq is color quality. The quality in SAM is nucleotide quality. They are different. Please read the bwa paper. This is not a bug, but an essential feature.

        Comment


        • #5
          Many thanks.

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