GeneRead Clonal Amp Q Kit

• Generation of sequencing-ready amplified libraries
• Multiplex clonal amplification: each library pool can include up to 12 uniquely bar coded DNA library samples
• Automated on the GeneRead QIAcube
• Proven performance with the GeneReader NGS System

Library concentration normalization and pooling

• Manual normalization of the DNA library sample(s) concentration and pooling (if multiplexing is to be performed) are performed.

Emulsion making

• The emulsion PCR beads are denatured in preparation for binding to the DNA library pool to eliminate bead clumping.
• Automated emulsion droplet formation is carried out on the GeneRead QIAcube.
• Upon completion of emulsion making, the PCR plate containing the emulsions is removed from the GeneRead QIAcube workdeck and manually loaded onto a stand-alone thermal cycler for clonal amplification.

Breaking and pooling

• The PCR plate containing the clonally amplified emulsions is loaded back onto the GeneRead QIAcube for the automated processes of pooling, breaking and cleaning of the emulsified library pools.

Enrichment

• Super A Beads are manually washed prior to the enrichment of live beads.
• Automated enrichment of live beads is conducted on the GeneRead QIAcube.
• Enriched beads are recovered and manually transferred from the GeneRead QIAcube into sample tubes.

Manual determination of bead concentration using OD

• Following the clonal amplification workflow, a standard curve is created using Primer Loaded PCR Beads that have not been through the clonal amplification process.
• The optical density of the enriched beads is measured so that the concentration can be extrapolated using the standard curve.
• Enriched beads (clonally amplified and enriched library pools) are then ready for sequencing.