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  • #1

    fastq quality check with Q=33 or Q=64?

    Hi all,

    I'm trying do quality checking with FASTX toolkit,
    FASTX-Toolkit - Command Line Usage
    http://hannonlab.cshl.edu/fastx_toolkit/commandline.html#fastq_quality_filter_usage


    Now I'm confused with different fastq. I list some samples as following, Is there anyone know which Q (33/64) I should used for data analysis?

    @SRR036482.94 SOLEXA8_1:2:1:0:1735 length=51
    AAAATAAAATATTGGCACAAAGAGATTTCAAAAATATCACTGCATCCTATA
    +SRR036482.94 SOLEXA8_1:2:1:0:1735 length=51
    =HCHHHEC@EHHHHHHHHDCGGBGHHHHHFHHHHHEEHHHHHFHHHHHHHD
    @SRR036482.95 SOLEXA8_1:2:1:1:1455 length=51
    ATTATAGAAAGCCAGAGGGAACTAATCACTTCAGTGCAACTGCAGCAGGTA
    +SRR036482.95 SOLEXA8_1:2:1:1:1455 length=51
    HHDDC=C7?D??DDD8ECC0ACGEGHHEDHHEHE@A8GC?:C4;D=CA@53

    Many thanks.
    Tags: None
  • #2
    This definitely looks like Sanger quality values (Phred+33).

    See FastQ for more information on the FastQ data format.

    Comment

    • #3
      fkrueger is correct, they are Sanger (Phred+33) encodings. The accession numbers (SRR) indicate that this is data downloaded from the the NCBI SRA. SRA data will always be Phred+33.

      Comment

      • #4
        Feng,


        How are you? There is an excelent paper that describes the FASTQ encoding. But kmcarr is correct, all the FASTQ sequences from ncbi are Phred+33.

        http://www.ncbi.nlm.nih.gov/pubmed/20015970

        Comment

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