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Hi all,
I ran Bioanalyser on the PCR products of my RNA-Seq library prep, and there are adaptor dimers contamination in all my samples. Some are more serious (sample 1) than the others (sample 3) as the starting amount of RNA varies among my samples. Pls see attached pic.
Should I do a AMPure beads purification on all? Or should I do a gel purification instead? Do all my samples (sample 1,2 and 3) all warrant 2nd purification in order to get rid of the adaptor dimers? I am going to run a multi-plex Hi-Seq run, 8-12 samples per lane, so it will be ~25M per sample.
Thanks a lot!
I ran Bioanalyser on the PCR products of my RNA-Seq library prep, and there are adaptor dimers contamination in all my samples. Some are more serious (sample 1) than the others (sample 3) as the starting amount of RNA varies among my samples. Pls see attached pic.
Should I do a AMPure beads purification on all? Or should I do a gel purification instead? Do all my samples (sample 1,2 and 3) all warrant 2nd purification in order to get rid of the adaptor dimers? I am going to run a multi-plex Hi-Seq run, 8-12 samples per lane, so it will be ~25M per sample.
Thanks a lot!
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