Hi,
I have extracted total RNA and then treated with DNase I (NEB) to remove any DNA contamination and then heat inactivated. My questions are:
1. Can I use this RNA for RNA seq? OR
2. Do I need to use phenol to remove DNA, precipitate with 100% ethanol and wash with 70% ethanol?
Thanks
Samuel A. Logan
Yes, that should be fine. You'll need to quantify your RNA before sending it for RNAseq though. Run it through a BioAnalyser or something similar (nanodrop might be ok). The RNA needs to be a certain RIN (RNA Intregity Number). Illumina hi-seq, I think should be RIN of 7... Maybe different RIN for different methods... Illumina mi-seq, Bio Rad, Ion Torrent..
Good luck..
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