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  • Sample quality for RNA_SEQ

    Dear all,

    I am preparing samples for RNA-SEQ - total RNA was isolated from OCT-Embedded frozen tissue using trizol - I run a RNA integrity check today but there's a lot degradation in some of my samples (See attached, band 1-6). I wonder if these samples could still be used or I have to get some high quality RNA?

    BTW, Would too much OCT in the samples affect the isolation process and Quality of RNA?

    Thanks.

    Cub
    Attached Files

  • #2
    Hi,

    If you have degraded RNA, then you might want to consider using a method other than poly-A based enrichment (which is what most kits use, including Illumina's sample prep kit) for removing structural RNA and other highly abundant species. There is a method that utilises time- and concentration-dependant rehybridisation and a duplex-specific nuclease to remove highly abundant transcripts. If you're using Illumina sequencing, there is a tech note on it on their website. A google search should turn up the documentation that you need.

    Cheers,

    Scott.

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    • #3
      Hi Scott,

      Thanks of the information. I was not able to locate the document you mentioned - wondering if you can post a link? Thank you.

      Cub

      Comment


      • #4
        Search for DSN Normalization SamplePrep Application Note

        Comment

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