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  • #1

    trimming paired end reads using Trim galore

    Dear all

    im trying to trim paired-end RRBS illumina reads using Trim galore. as far as i understood, paired end reads must be trimmed using --paired option following by file names. i tried : trim_galore --paired r1.fastq.gz r2.fastq.gz. however at the end, im getting only trimmed file for read 1 and nothing for read 2. any idea why?

    thank you so much in advance
    Tags: illumina, paired end read, rrbs, trim galore
  • #2
    Hi Hedi86,

    for RRBS the command would be:

    Code:
    trim_galore --rrbs --paired r1.fastq.gz r2.fastq.gz
    Which version of Trim Galore were you using (the latest one is v0.5.0, https://github.com/FelixKrueger/TrimGalore/releases).

    Trim Galore will trim R1 first, R2 second, and then perform a validation step which p0roduces 2 new files that contain _val_ in their file names (for validated). Once this is done, the files called _trimmed_ ... are being deleted. If there are any error messages on the screen they might help identify where the problem lies.

    Comment

    • #3
      thank you for your replay

      for downstream analyses in Bismark i used both Val-trimmed-R1 and Val-trimmed-R2 files (because libraries prepared using NuGEN kit). however, bismark produced only one BAM file with R1 extension name. is it normal for pair end alignment?

      Best

      Comment

      • #4
        Yes, this is normal. Paired-end BAM files have Read 1 and Read 2 on consecutive lines, so there is only one file per read pair.

        Comment

        • #5
          These are steps to work on trimming process.

          Step 1: Quality*Trimming. In the first step, low-quality base calls are*trimmedoff from the 3'*end*of the*reads*before adapter removal.
          Step 2: Adapter*Trimming.
          Step 3: Removing Short Sequences.
          Step 4: Specialised*Trimming.
          Clinical Research

          Comment

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