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  • By how much custom primers can overlap adapters?

    By how much 5' ends of custom sequencing primers are allowed to overlap with the P5 and P7 flow cell adapters on MiSeq cell?
    More specifically, with these sequences:
    P5: 5' AATGATACGGCGACCACCGA 3'
    P7: 5' CAAGCAGAAGACGGCATACGA 3'

    Has anyone tried complete overlap?

    Thanks

  • #2
    Hi Xaki, yes we tried a complete overlap with no success. Still not 100% why this didn't work but we gave up after about 3-4 runs (and tried a lot of things). So we ended up using a custom primer. The custom primer we use overlaps 4 bp. however our p5 is:
    P5 5'-AATGATACGGCGACCACCGAGATCTACAC-3'

    And our first 4bp of our custom primer (p5 end) is 5'-ACAC......

    in total our custom primer is 22bp and contains some LNA's to keep the size down a bit and the melt temp high.

    hope this helps, regards, Mike.

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    • #3
      Thank you bunce. This is helpful to know that complete overlap does not work. I wonder why? Do you see clusters forming at all?
      Your primer design is same as ours. We also start from ACAC...
      Has anyone tried to go a bit deeper into flow cell adapters sequence?

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      • #4
        Hi Xaki. Yes - clusters formed. I am not sure why we could never get decent sequences. I suspect it might be that the 'vision' that all the libraries are lined up as nice organised vertical strands of DNA is misleading.... and that a lot of clusters exist in a bridged form. This represents an issue when trying to sneak in a custom primer. We tried altering the run recipe (annealing temp) to try and get the sequencing primer to bind before a cluster could bridge. But eventually gave up - the sequencing efficiency was too low.

        The flow cell grafted P5 has a 'U' to enable cleavage of the strand - I think this is why it may not be possible to steal a few more bases? not really sure. Cheers Mike.

        Comment


        • #5
          There is a similar thread here. Some think you can extend custom sequencing primer into flow cell adapter with no problems, but I do not see anyone with direct experience doing that and getting good results.
          Last edited by Xaki; 11-12-2015, 12:57 PM.

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