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  • Staroselec
    Junior Member
    • Jul 2012
    • 2

    RNA shearing

    Hello
    I would like to fragment RNA samples into ~30-50 bp fragments prior to making cDNA libraries and sequencing with SOLiD.
    Is it possible with the Covaris? What conditions? Could you advise other methods?
    Thank you for your time and tolerance.
  • JPC
    Senior Member
    • May 2008
    • 116

    #2
    You will have to get the whole transcription Library prep kit from ABI so I would stick with the enzyme shear that they recommend (using RNAseIII for 3 mins at 37degrees C).

    The 3 min incubation should shear your samples between 25 and 750bp with the majority of the product towards the 100bp region. It will probably take a little trial and error but I would try adding 15 seconds to the incubation and see how far the peak shifts?

    Comment

    • kandasamyalkondan
      Junior Member
      • Jun 2014
      • 3

      #3
      Hello
      I would like to fragment RNA samples into ~30-50 bp fragments prior to making cDNA libraries and sequencing with illumina.
      Is it possible with the Q800R sonicator? .is there is any protocol

      Comment

      • NextGenSeq
        Senior Member
        • Apr 2009
        • 482

        #4
        I would make cDNA and shear it. Why do you want fragments that short?
        You will lose them using Ampure bead purification as well as many column methods.

        Comment

        • jwfoley
          Senior Member
          • Jun 2009
          • 183

          #5
          Why don't you just heat your RNA in a magnesium solution? Or if you like kit science, Ambion makes a "fragmentation reagent" and that's pretty much what it is.

          But these fragments will be too short for a regular sequencing library, so I suggest you revisit your experimental design, unless there's some really good reason why you need them to be so short.

          Comment

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