Tweet
Is there any reason why you can't use MinElute columns instead of Ampure beads during a TruSeq DNA library prep? I can't see any reason for using beads instead of columns after the end repair and A tailing reactions. I can see maybe using beads after adapter ligation to remove adapter dimers, but couldn't you accomplish the same thing by using a MinElute purification followed by gel purification to remove dimers? I know that if you have a lot of adapter dimers that some of those may contaminate larger gel fractions, but is that contamination much of a problem during the limited cycle enrichment PCR?
I am new to TruSeq library preps, so I am trying to understand the reliance on Ampure beads when MinElute purifications are so much faster (compared to the bead steps in the TruSeq protocol.)
Thanks for any thoughts/info.
I am new to TruSeq library preps, so I am trying to understand the reliance on Ampure beads when MinElute purifications are so much faster (compared to the bead steps in the TruSeq protocol.)
Thanks for any thoughts/info.
Comment