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Just an FYI for anyone still using the XL+. It's a bad idea to run any FLX samples on the XL+ chemistry. From what was sort of explained to me by a 454 rep, the emPCR master mix and thermocycling conditions are optimized for one or the other, and cause problems when the protocols are mixed. I had some issues running PTPs of mixed samples with XL+ kits (some regions with 16s amplicons and some with Rapid libraries) where the amplicon data was quite poor and unexpected. When the same libraries were repeated with FLX chemistry and emPCR, the results were great. Not sure exactly what the cause(s) were, but I know it caused some bioinformatic headaches for our customers.
Best of luck! I'll see you on the Illumina forums!
Anthony
Best of luck! I'll see you on the Illumina forums!
Anthony
You can use Lib-L primer sequences to create amplicons, which is what all of my previous 16s customers were doing. You end up with uni-directional reads but twice the coverage of Lib-A. This is the same kit used for rapid, PE and cDNA libraries.
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