This is the advice we got from Illumina about sequencing our library; it is low diversity so we will need to also sequence PhiX.

Read1 = can use the Illumina primers in the cartridge* but would see better results with a custom primer 5'-CGACAGGTTCAGAGTTCTACAGTCCGACGATC-3' If your library is low diversity and you also need to sequence PhiX, you would spike this into the Illumina well.

I'm sending two libraries and would like to sequence both on one lane. Could you do QC on both and combine them together? They each contain 96 unique dual barcoded individuals, and they can be combined with no issues. Thanks!