Procedure
1
Pulse centrifuge the MSA1 plate at 280 × g.
2
Carefully remove the cap mat.
3
Add 50 µl FMS to each well of the MSA1 plate.
4
Reseal with the cap mat using the original orientation.
5
Vortex at 1600 rpm for 1 minute, and then centrifuge the plate at 280 × g.
6
Incubate on the preheated heat block for 1 hour.
If you are continuing, you can leave the plates on the heat block until you have completed preparation for
the next step, no longer than 2 hours.
SAFE STOPPING POINT
If you are stopping, seal the plate, and store at -25°C to -15°C for up to 24 hours.
Precipitate DNA
This step uses 100 % 2-propanol and PM1 to precipitate the DNA.
Consumables
u
100% 2-propanol
u
PM1(2 tubes)
u
Cap mat
Preparation
1
Do one of the following:
u
If proceeding immediately from
, leave the MSA1 plate on the heat block until
preparation is complete.
u
If the MSA1 plate was stored at -25°C to -15°C, thaw at room temperature, pulse centrifuge
at 280 × g, and preheat the heat block to 37°C.
2
Prepare the following consumable.
Item
Storage
Instructions
PM1
2°C to 8°C
Thaw to room temperature and invert 10 times to mix.
3
Remove the cap mat.
Procedure
1
Add 100 μl PM1 to each well of the MSA1 plate.
2
Reseal with the cap mat using the original orientation.
3
Vortex the plate at 1600 rpm for 1 minute.
4
Incubate on the preheated heat block for 5 minutes.
5
Pulse centrifuge at 280 × g for 1 minute.
6
Set the centrifuge at 4°C in preparation for the next centrifuge step.
Document # 11322427 v03
For Research Use Only. Not for use in diagnostic procedures.
11
Infinium HD Super Assay Reference Guide