Freezing of feeder-free hPSCs

hPSCs are ready to be frozen when the culture reaches 50-80% confluency.

Before starting:

a. Prepare Freezing Medium I and II and keep on ice.

b. Pre-label appropriate number of cryovials (freeze approx. 2 vials/well of a 6-well plate)

Freezing Medium I

A	B
Feeder-free medium*	5 ml
FB essence**	5 ml

*The formulation of feeder-free medium can be found in below**We have used successfully frozen feeder-free hPSCs using KSR instead of FB essence. Final volume: 10ml

Freezing Medium II

A	B
FB essence*	8 ml
DMSO	2 ml

*We have used successfully frozen feeder-free hPSCs using KSR instead of FB essence. Final volume: 10ml

Feeder-free Medium (version A)

A	B
StemFlex basal medium	450 ml
StemFlex supplement	50 ml

Final volume: 500ml

Feeder-free Medium (version B)

A	B
mTeSR-plus basal medium	400 ml
mTeSR-plus supplement	100 ml

Final volume: 500ml

Wash hPSCs with DPBS.

Use 1 ml Accutase/well of a 6-well plate.

Incubate 0h 5m 0s 37°C

Add 2 ml DMEM/F12 to each well.

Collect all cells into 15 ml conical tube.

Add 7 ml DMEM/F12.

Centrifuge 200-300x g

Aspirate supernatant

Gently re-suspend the pellet in 500 µl Freezing Medium I per vial to be frozen, triturate 5-10 times to achieve single cell suspension using a P1000 tip

In each cryovial, add 500 µl pre-chilled Freezing Medium II.

Dispense 500 µl cell suspension into each cryovial using P1000, mix

Temporarily keep cryovials on ice until all cells dispensed.

Place cryovials into Styrofoam microtube freezer box or pre-cooled (4°C on ice) NALGENE™ Cryo 1°C Freezing Container filled with 250 ml of Isopropanol.

Freeze at -80°C

For long term storage, store cryovials in liquid nitrogen (-196ºC).

hPSCs are ready to be frozen when the culture reaches 50-80% confluency.

Before starting:

a. Prepare Freezing Medium I and II and keep on ice.

b. Pre-label appropriate number of cryovials (freeze approx. 2 vials/well of a 6-well plate)

Freezing Medium I

A	B
Feeder-free medium	5 ml
FB essence*	5 ml

*We have used successfully frozen feeder-free hPSCs using KSR instead of FB essence . Final volume: 10ml

Freezing Medium II

A	B
FB essence*	8 ml
DMSO	2 ml

*We have used successfully frozen feeder-free hPSCs using KSR instead of FB essence . Final volume: 10ml

Wash the plates twice with DPBS

Add 1 ml/well of ReLeSR to a 6-well plate and incubate for 0h 1m 0s Room temperature

Remove the solution and let it sit at Room temperature for 0h 2m 0s

Add 2 ml of Feeder-free medium/well.

Gently scrape the cells from the bottom of the well by using a Corning cell lifter.

Collect the cells in a 15 ml conical tube and add 3 ml of Feeder-free medium.

Gently mix by inversion and gravity precipitate for 0h 5m 0s

Remove the supernatant down to 1 ml and add 5 ml of Feeder-free medium.

Pellet the cells at 150x g and aspirate the supernatant.

Gently re-suspend the pellet in 500 µl Freezing Solution I per vial to be frozen.

Carefully add 500 µl Freezing Medium II per vial to be frozen.

Dispense 1ml aliquots in pre-labeled cryovials and keep on ice.

Place cryovials into Styrofoam microtube freezer box or pre-cooled (4°C on ice) NALGENE™ Cryo 1°C Freezing Container filled with 250 ml of Isopropanol.

Freeze -80°C

For long term storage, store cryovials in liquid nitrogen (-196ºC).