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  • TruSeq small RNA final products Peaks

    Hi everyone,

    I have tried to make small RNA libraries from insect RNAs and I should say that it was my first experience. I used TruSeq small RNA kit. I have attached my final products (samples 1-3, 4 is just water) run in Experion DNA 1K chip from Bio-Rad after gel purification and ethanol precipitation. I appreciate if you guys let me know if you think they look good to send for sequencing.
    My ultimate goal is discovering known and novel viruses in insect. So, I am looking for any kind of small RNAs (18-30 nt).

    Thanks
    Attached Files

  • #2
    Your libraries look perfect! The goal of the gel cut is to remove the primer and adapter dimer bands at ~125 and 135bp while keeping your small RNA libraries, which in your case are ~153-165bp. Looking from these traces you have nothing but the library peak. The yields also look good enough for pooling and sequencing.
    Last edited by kcchan; 03-10-2013, 09:05 PM. Reason: Derp, didn't read the initial post fully. Sample 4 is NTC.

    Comment


    • #3
      Thanks so much for your reply

      Comment


      • #4
        Hi,
        Which method did you use for isolating the small RNA fragment from the adapter dimer.

        Thanks

        Comment


        • #5
          HI F2000,

          I did gel purification. I followed the TruSeq protocol

          Comment

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