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  • cutadapt or trim galore on color space data.

    1. I download the sra files and get the .qual & .csfasta.
    2. get the fastq file using solid2fastq.py.
    3. running fastqc on the fastq indicating high content of solid smallRNA adapter.
    4. tried both cutadapt and trim galore! on the fastq file:In read named 'SRR1510896.1 1_16_1976_F3': length of quality sequence (50) and length of read (51) do not match
    step 4 was run on galaxy!
    how can I solve the problem? am I using the wrong trim software?

  • #2
    Cutadapt can deal with your data, this is taken from the Cutadapt help:

    Code:
     Colorspace options:
        -c, --colorspace    Enable colorspace mode
        -d, --double-encode
                            Double-encode colors (map 0,1,2,3,4 to A,C,G,T,N).
        -t, --trim-primer   Trim primer base and the first color
        --strip-f3          Strip the _F3 suffix of read names
        --maq, --bwa        MAQ- and BWA-compatible colorspace output. This
                            enables -c, -d, -t, --strip-f3 and -y '/1'.
        -z, --zero-cap      Change negative quality values to zero. Enabled by
                            default in colorspace mode since many tools have
                            problems with negative qualities
        --no-zero-cap       Disable zero capping
    Trim Galore does not allow using the colour space switch, so please use Cutadapt instead.

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