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  • Trimming paired end RNAseq - Trimmomatic

    Hello --

    I've begun pre-processing of my paired-end RNA seq data (run on Illumina HiSeq).

    After running fastqc on my samples, I noticed some have overrepresented sequences corresponding to adaptors.

    I've been trying to use Trimmomatic to remove the adaptors, however, after Trimming I get MORE over represented reads than I do before trimming! I'm not sure what's going on.

    For instance, in my unprocessed read, I'll have a single overpresented sequence corresponding to adapter index 1. Once trimmed and processed by trimmomatic, I'll have 25 overrepresented sequences, all corresponding to different variants of the adapter index 1 sequence.

    Here is my command line:

    Code:
    TrimmomaticPE -phred33 /R1_001.fastq.gz /R2_001.fastq.gz /R1_pairedout /R1_unpairedout /R2_pairedout /R2_unpairedout ILLUMINACLIP:/TruSeq3-PE.fa:2:30:10 LEADING:5 TRAILING:5 AVGQUAL:20
    Any idea what I'm doing wrong? The same thing occurs even if I leave out the ILLUMINACLIP line.

  • #2
    cross posted https://www.biostars.org/p/106516/

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