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  • #1

    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.
    Tags: None
  • #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?

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    • #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

      • #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

        • #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.

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