Amplify PGx

This step adds the DNA samples and reagents to the plates to prepare them for PCR amplification.

MA1
PGP (PGx Primer Pool)
PGM (PGx Master Mix)
96-well 200 μl skirted PCR plate
DNA plate (20 ng/μl per well)
Microseal 'B' adhesive seals
1. Prepare the following consumables:

Reagent

Storage

Instructions

PGM

-25°C to -15°C

Thaw at room temperature. Vortex or invert 10 times to mix. Pulse centrifuge at 280 × g.

PGP

-25°C to -15°C

Thaw at room temperature. Vortex or invert 10 times to mix. Pulse centrifuge at 280 × g for 1 minute.
2. Thaw samples to room temperature. 
3. In the post-amp area, save the following PCR program on the thermal cycler:
Set the reaction volume to 35 μl and the lid temperature to 105°C
98°C for 30 seconds
11 cycles of:
98°C for 30 seconds
76°C for 30 seconds
72°C for 20 seconds
21 cycles of:
98°C for 30 seconds
66°C for 30 seconds
72°C for 20 seconds
72°C for 5 minutes
Hold indefinitely at 12°C
4. Apply a PGx barcode label to a new PCR plate.
1. Add 10 µl MA1 to each well of the PGx plate.
2. Add 10 µl PGP to each well of the PGx plate.
3. Add 10 µl PGM to each well of the PGx plate.
4. Transfer 5 µl DNA sample from the DNA plate to the corresponding wells of the PGx plate.
5. Apply Microseal 'B' to the PGx plate. Make sure that each well is tightly sealed with no bubbles or gaps in the film.
6. Vortex at 1600 rpm for 15 seconds, and then pulse centrifuge at 280 × g for 1 minute.
7. Perform the remaining protocol steps for the PGx plate in the post-amplification area.