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  • library prep by transposition



    what are thoughts on this new method? no need for a covaris, and low input. interested in using before capture protocol, i am concerned the transposome complex will not yield fragments representative of entire genome.

  • #2
    Moving this to the library prep forum as it's applicable to 454 (and probably solid) as well.

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    • #3
      size distribution using transposition

      I heard about the new technology as well. I was just wondering what the size distribution looks like afterwards. As far as I know there is no need to do it. Thanks.

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      • #4
        here is the distribution with bioanalyzer for a full reaction with 10 pcr cycles:



        and for 1/5 scaled down reaction with 15 pcr cycles:

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        • #5
          here is the distribution with bioanalyzer for a full reaction with 10 pcr cycles:

          [IMG][/IMG]

          and for 1/5 scaled down reaction with 15 pcr cycles:

          http://www.postimage.org/image.php?v=PqE_Lh9[IMG][/IMG]

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          • #6
            You should check with your capture reagent vendor -- one of the problems seen with Illumina libraries is "daisy-chaining" of fragments via the adapters which brings in off-target material. Nextera uses custom adapters, so any blocking oligos supplied in the kit won't be correct.

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            • #7
              @upenn_ngs: Were this size distributions for Illumina libraries?

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              • #8
                what about ends fragments ?

                Hi all,
                This fragmentation seems very interesting by its low input DNA and its relative simplicity!
                I am wondering about the non representativity of ends fragments with this fragmentation except with a previous step like circularization or adding primers.
                Is that makes sense ?

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                • #9
                  yes, this is illumina library prep. although there is a great time saving, a fragmentation and ligation protocol with NEB enzyme is still much more cost effective.

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