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  • Save truseq stranded mRNA polyA(-) supernatant for small RNAseq?

    Has anyone tried to save and sequence the polyA(-) supernatant from Illumina's TruSeq stranded mRNA library prep kit? If so, any advice or insight into things to consider using the supernatant - ie: would I do another phenol extraction or something to pellet out the polyA(-) RNA then suspend in H2O?

    I'm interested in small RNAs (miRNA, piRNA) in particular so I assume I'd need to clean up the supernatant on a gel to size select for 20-30 nt or maybe use another rRNA depletion to clean up the samples.

    Thanks!

    This kit:
    Prepare sequencing libraries from mRNA to get a clear view of the coding transcriptome with strand-specific information.

  • #2
    It is a good idea to try. Simplest way would be to dilute the bead supernatant to reduce salts concentration coming from binding buffer and then use a Zymo RNA Clean & Concentrator column which gives options to purify the required size range including small RNA for follow up application.

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    • #3
      I have a bunch of Qiagen miRNeasy columns as well (> 20 nt) - any reason to use the Zymo over the Qiagen?

      Thanks!

      Comment


      • #4
        Zymo kit is designed for purification and elution volume can be as low as 5 ul. miRNeasy is for RNA extraction from tissue and cells and has to be modified for purification with risk of loosing material.

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