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Hi, all,
I just prepared couple of libraries with the NEBNext® Ultra™ II FS DNA Library Prep Kit for Illumina. After run them on a Qiaxcel system, I saw a visible ~35bp peak.(15bp and 3000bp are alignment markers) Could it be primer-dimer or adaptor-dimer? Should I perform another round of beads clean-up? Or I can just send them for sequencing?
Thank
I just prepared couple of libraries with the NEBNext® Ultra™ II FS DNA Library Prep Kit for Illumina. After run them on a Qiaxcel system, I saw a visible ~35bp peak.(15bp and 3000bp are alignment markers) Could it be primer-dimer or adaptor-dimer? Should I perform another round of beads clean-up? Or I can just send them for sequencing?
Thank
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