Working Copy: Can cells be fixed and then processed with LUTHOR HD?

We recommend that cells are fixed prior to isolation in order to preserve their transcriptomic state (importantly, dead cells will not be compatible with LUTHOR HD library preparation).

Cell fixation guidelines are below which have been validated internally.

Buffers

Specific Reagents

*Mix 1:1 nuclease-free water with 99% Glycerol, filter through a 0.2 μm filter and store at room temperature in LoBind tubes

Fixation Temperature and Time

• 1 h at 20ᵒC – for samples processed immediately after fixation

• 12-24 h at 4ᵒC – for samples to be stored

Sample Fixation (tested with 1 M DU145 cells/ml)

1. Pass cells through 40 μm strainer.

2. Centrifuge at 500g for 3 min at 4-8ᵒC.

3. Remove the supernatant without disturbing the pellet.

4. Add 1 ml of freshly prepared Fixation Buffer (FB). Note: always prepare a fresh FB.

5. Gently pipette-mix 5x

6. Incubate for 12-24 h at 4ᵒC (for storage or shipment), or 1 h at 20ᵒC for immediate use

7. Centrifuge at 500g for 3 min at 4-8ᵒC.

8. Remove the supernatant without disturbing the pellet.

9. Add 1 ml cold Quenching Buffer (QB), gently resuspend cells. Keep on ice for 5 min.

See storage guidelines.

10.    Centrifuge at 500g for 3 min at 4-8ᵒC.

11.    Resuspend cells in 1 ml Resuspension Buffer (RB)

12.    Pass cells through 40 μm strainer.

13.    Count and determine viability of cells. Strongly recommended to stain cells with a fluorescent dye such Acridine Orange/Propidium Iodide. >95% of fixed cells appear non-viable.

Fixed Sample Storage Guidelines

• Fixed samples can be stored at 4ᵒC for up to 1 week.

• For long-term storage at -80ᵒC or shipment on dry ice, proceed as follow:

• Add 0.05 volume of DMSO to fixed sample in QB buffer (step 9, e.g. 50 μl DMSO to 1000 ul fixed sample). Gently pipette mix 5x.

• Add 50% Glycerol for a final conc. of 10%.

• Store at -80ᵒC for up to 6 months