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  • #1

    lost RNA

    I am using ScriptSeq Complete Kit (Bacteria) to prepare RNA-Seq library. I finished rRNA depletion step and I checked RNA concentration with Nanodrop. I found I might lose RNA from several samples. There RNA concentrations are very low with incorrect 260/280 compared with the other samples.
    I think the RNA might be lost in the step of ethanol precipitation and washing. I want to reprocess these samples. I calculate the remaining reagents and I found I have enough reagents except for the magnetic beads. The kit containing is just too expensive. Anything else I can do? Thank you!
    Tags: None
  • #2
    Hello-

    First, Nanodrop is not sensitive enough to be able to quantify output from the rRNA depletion steps; we recommend either a Qubit with Ribo-Green and a Bioanalyzer using a Pico chip.

    What did you use to purify the remaining RNA after depletion and post-streptavidin bead processing?

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    • #3
      I used ethanol precipitation.
      The samples are from the same strains as the good samples. So, even nanodrop is not accurate, they should not have so bog difference.
      I am wondering I lost RNA during ethanol washing

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      • #4
        what is the typical yield of the Ribo-Zero rRNA Removal Kits say starting with 5 ug E. coli total RNA?

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        • #5
          The Illumina user guide reports 8% recovery; from 5 µg of RNA, up to 400 ng of non-ribosomal RNA - to include tRNAs, non-coding RNAs and mRNA (mRNA give the lowest of the recovered RNA in terms of percentages).

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          • #6
            I started from 2.5 ug
            For some samples which I though they are good gave the concentrations of 20~ 80 ng/ul and I have 10 ul for each samples. So, it looks I should worry about rRNA removal in these "good" samples rather than RNA losing of the "bad" samples

            Originally posted by Olaf Blue View Post
            The Illumina user guide reports 8% recovery; from 5 µg of RNA, up to 400 ng of non-ribosomal RNA - to include tRNAs, non-coding RNAs and mRNA (mRNA give the lowest of the recovered RNA in terms of percentages).

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            • #7
              Best thing to do is two-fold: 1) Check the RNA post-Ribo-Zero on a Bioanalyzer (if the total RNA was of high quality to start with, you should see disappearance of the two major rRNA peaks (16/23s or 18/28s) and if the RNA was of less that good quality, check with RT-PCR if you are concerned.

              You will never eliminate all of the rRNA - Ribo-Zero is to minimize it as much as possible.

              The small rRNA (5s/5.8s) can be reduced using a Qiagen or Zymo RNAClean column, and following the procedure to recover RNAs >200 nt.

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