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  • GenoMax
    Senior Member
    • Feb 2008
    • 7142

    #31
    Did you also remove the corresponding Q-score value? If you used trimmomatic/bbduk they would do this but if you used some other method then you may have an extra Q-score value remaining on line 4 for each fastq record.

    I am not sure why you are having a problem but if I use the two reads you posted above I am able to demultiplex them fine (after taking the N's out).
    Last edited by GenoMax; 01-26-2016, 06:58 AM.

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    • smitra
      Member
      • May 2013
      • 20

      #32
      I haven't tried trimmomatic/bbduk yet. But this barcode splitter is playing strange with me. Yes with N's out they demultiplex but never the whole data. every time some reads remained which is completely unexplainable. If I do again with those unmatched read again some bit match. which is very strange.

      But at present i am just doing the N's out for the whole data and seems with two stage I am getting success. Thanks for helping.

      Comment

      • luc
        Senior Member
        • Dec 2010
        • 469

        #33
        You might want to try Sabre instead:
        Contribute to najoshi/sabre development by creating an account on GitHub.

        Works also on paired-end data.

        The FASTX toolkit is very old by now.

        Comment

        • smitra
          Member
          • May 2013
          • 20

          #34
          Thank you Luc. I will give it a try.

          Comment

          • sjuzhet
            Junior Member
            • Jul 2014
            • 9

            #35
            This might be a basic question, but I thought I'd hop in this topic to ask - half of my reads were read in the opposite direction, so the barcode is reverse complemented at the end of the read. Is there a way to get Fastx Toolkit to incorporate reverse complement barcodes at the end of the line as well, or do I have to do this manually?

            Comment

            • GenoMax
              Senior Member
              • Feb 2008
              • 7142

              #36
              Originally posted by sjuzhet View Post
              This might be a basic question, but I thought I'd hop in this topic to ask - half of my reads were read in the opposite direction, so the barcode is reverse complemented at the end of the read. Is there a way to get Fastx Toolkit to incorporate reverse complement barcodes at the end of the line as well, or do I have to do this manually?
              Fastx_barcode_splitter has --eol (end of line/read) option to check reads at the 3' end. Provide the barcodes appropriately in the barcode file. You will need to run --bol and --eol sequentially (with individual barcode files) since those two options can't be combined.

              Comment

              • sjuzhet
                Junior Member
                • Jul 2014
                • 9

                #37
                Originally posted by GenoMax View Post
                Fastx_barcode_splitter has --eol (end of line/read) option to check reads at the 3' end. Provide the barcodes appropriately in the barcode file. You will need to run --bol and --eol sequentially (with individual barcode files) since those two options can't be combined.
                Yeah, that's what I did. I was hoping to get a report on the number of reads that didn't match to either bol or eol, but I guess I can just calculate it.

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