Staining of cells for flow cytometry
| FACS buffer: | 1xPBS
FCS (heat-inactivated, final concentration: 5%) 5% Natriumazid (final concentration: 0.1%) |
||
| 1st antibody: | primary antibody (approx. dilution 1:200) | ||
| 2nd antibody: | secondary antibody (approx. dilution 1:500)
fluorescence- labelled |
||
| controls: | sample with irrelevant primary antibody and secondary antibody
sample with secondary antibody only if possible untransfected cells stained with both antibodies |
Procedure
Preparation of cells:
§ aspirate medium and wash twice with 5-10 mL 1xPBS
§ detach cells with 1 mL Trypsin/EDTA
§ inactivate Trypsin/EDTA with 3 mL fresh medium
§ transfer the cells into a 15 mL centrifuge tube and centrifuge 3 min at 600 rpm
§ discard supernatant and resuspend the cell pellet in FACS buffer
§ centrifuge again, resuspend cells in FACS buffer and determine cell count
§ distribute into Eppendorf tubes (106 cells/tube)
Staining (perform all steps on ice):
§ pellet the cells by centrifugation 2 min, 2500 rpm, 4°C
§ resuspend pelled in 300 µL FACS buffer
§ add 1st antibody at desired concentration
§ incubate 1-1.5h on ice, centrifuge 2 min, 2500 rpm, 4°C
§ discard supernatant and resuspend the pellet in 600 µL FACS buffer, centrifuge again as above
§ wash 3 times with 300 µL FACS buffer, at the end resuspend in 300 µL FACS buffer
§ add 2nd antibody at desired concentration
§ incubate max. 30 min on ice (keep samples dark!)
§ wash twice with 600 µL FACS buffer
§ during centrifugation prepare FACS tubes with 600 µL FACS buffer
§ resuspend pellet in 600 µL FACS buffer and transfer to prepared FACS tubes
§ measure samples