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  • smurugesan
    Junior Member
    • Aug 2017
    • 8

    Customprimers-SampleSheet error during secondary analysis

    Hi everyone,

    Yesterday i did a 16s MiSeq run using custom primers, when i tried to demultiplex using samplesheet generated through IEM, i found error during secondary analysis to generate Fastq files. I replaced the illumina index sequences with custom index sequences during samplesheet generation. But still I could not overcome the issue. It would be great help, if any one can help to sort this issue. Many thanks in advance.
  • pmiguel
    Senior Member
    • Aug 2008
    • 2328

    #2
    What was the error?

    --
    Phillip

    Comment

    • smurugesan
      Junior Member
      • Aug 2017
      • 8

      #3
      Dear Phillip, Sorry I was not clear in my message. The error was during the demultiplex execution according to the analysis error log. When MSR executes the secondary analysis, the error message was "aborting analysis. Please check error log and sample sheet issues". For your information please find the below link for sample sheet. Thank you.

      Comment

      • pmiguel
        Senior Member
        • Aug 2008
        • 2328

        #4
        Nothing leaps out at me as being wrong with that sample sheet. You will probably need to take this up with Illumina.

        --
        Phillip

        Comment

        • pmiguel
          Senior Member
          • Aug 2008
          • 2328

          #5
          Well, one thing. You mentioned you changed the sample sheet after the run. What sample sheet was used by the MiSeq during the run?

          The length of the i7 index read is determined by the length of the sequences in the sample sheet. So if you did not have 12 base indexes in the run sample sheet, then that index read would be whatever length the indexes you did use were. And, if you didn't provide any indexes, then no index read would have been done and it would likely be impossible to demultiplex you run.

          --
          Phillip

          Comment

          • GenoMax
            Senior Member
            • Feb 2008
            • 7142

            #6
            Following up @Phillip's suggestion, post this part from your ReadInfo.xml file for this run. It should look something like this
            Code:
            <Read Number="1" NumCycles="151" IsIndexedRead="N"/>
            <Read Number="2" NumCycles="8" IsIndexedRead="Y"/>
            <Read Number="3" NumCycles="152" IsIndexedRead="N"/>

            Comment

            • thermophile
              Senior Member
              • Apr 2015
              • 243

              #7
              Look for WorkflowLog.txt (I demultiplex in basespace where it's in fastqc/files), scroll to the bottom and it will tell you exactly what has caused the sample sheet failure.
              Microbial ecologist, running a sequencing core. I have lots of strong opinions on how to survey communities, pretty sure some are even correct.

              Comment

              • athuyvo
                Junior Member
                • Jul 2017
                • 3

                #8
                I'm experiencing a similar problem. Was this resolved?

                I ran a MiSeq run with 16s custom libraries/primers and got the same error "abort analysis. Please check error log and sample sheet." No fastq files were produced for my run, but the overall quality of the run was good. I also noticed the base call intensity for the i7 read was pretty low. Could this be a software issue or maybe a primer issue? PhiX was also spiked in at 15%.
                Last edited by athuyvo; 03-13-2018, 04:08 PM. Reason: added more details

                Comment

                • thermophile
                  Senior Member
                  • Apr 2015
                  • 243

                  #9
                  Here's how my header looks for custom amplicon sequencing.

                  Code:
                  Workflow	GenerateFASTQ
                  Application	FASTQ Only
                  Assay	Nextera
                  Description	
                  Chemistry	Amplicon
                  Microbial ecologist, running a sequencing core. I have lots of strong opinions on how to survey communities, pretty sure some are even correct.

                  Comment

                  • athuyvo
                    Junior Member
                    • Jul 2017
                    • 3

                    #10
                    Thanks @thermophile. I have same exact format for my sample sheet. I was able to requeue the analysis by essentially ignoring the i7 reads and demultiplex using only i5 barcodes. We think the problem was suboptimal custom i7 primers so the MiSeq couldn't demultiplex using i7 reads.

                    Comment

                    • thermophile
                      Senior Member
                      • Apr 2015
                      • 243

                      #11
                      you reverse complimented your i7 barcodes right?
                      Microbial ecologist, running a sequencing core. I have lots of strong opinions on how to survey communities, pretty sure some are even correct.

                      Comment

                      • athuyvo
                        Junior Member
                        • Jul 2017
                        • 3

                        #12
                        i7 barcodes were reverse complimented. We were able to salvage our data by mining the adapter reads and found the i7 barcodes.

                        Comment

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