Hi I have phenol contamination in my RNA after trizol extraction (I don't think I washed them enough). I'm looking to re-precipitate all my samples using LiCl or Sodium acetate to eventually run them on RT-qPCR. Can anyone weigh in here as to what is the best option?
Cheers
Toby
FX Reymond Sutandy
Hi,
You can repeat your procedure again with phenol extraction then followed by ethanol and sodium acetate precipitation. One sugestion you can use Phase lock gel column to help with the phenol separation. It always work best for me and never got phenol contamination.
Good luck!
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Prabodh Kumar
If your RNA concentration is not very low and they are >1kb in size, LiCl precipitation overnight is the best protocol according to me.
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