Hybridoma cells in SFX media: Difference between revisions
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== | == Material == | ||
* 5 ml, 10 ml, 20 ml pipettes | |||
* Serum free media (400 mls SF media + 1% antibiotics; 4 mls P/S and 4 mls Glutamine) | |||
* 2 blue cap flasks | |||
* 1 conical tube | |||
== | == Procedure == | ||
# fill 10 mls SFX media per blue cap flask | # fill 10 mls SFX media per blue cap flask | ||
# put flask for > = 1 hour in incubator 10% CO2 @ 37 °C | # put flask for > = 1 hour in incubator 10% CO2 @ 37 °C |
Latest revision as of 14:35, 8 June 2015
Material
- 5 ml, 10 ml, 20 ml pipettes
- Serum free media (400 mls SF media + 1% antibiotics; 4 mls P/S and 4 mls Glutamine)
- 2 blue cap flasks
- 1 conical tube
Procedure
- fill 10 mls SFX media per blue cap flask
- put flask for > = 1 hour in incubator 10% CO2 @ 37 °C
- use 10 ml pipette to take up the media and blow off the cells
- check the flask in microscope to make sure that the cells have detached
- use 10 ml pipette to remove the cells from the flask into the conical tube
- spin at 1000rpm for 3 minutes
- aspirate off the media
- add 2 mls of SFX media
- resuspend the cells
- add the 2 mls of the suspension to 1flask
- ut in 10% CO2 incubator
- let cells grow until they die ( 1-2 weeks; spin cells down( 1000 rpm , 3 min. 4°C)
- collect supernatent( contains Antibody) and add @1:50 concentratin 5 x sodium azide/ 500 mM Hepes and store at 4°C