Freezing and Thawing S2 Cells: Difference between revisions

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==SOP==
*[[SOP- Cryogenic Materials]]
*[[SOP- Biosafety Cabinets]]
==METHOD==
#Use and early passage (1-10) of exponentially growing (about ~10^7 cells).
#Use and early passage (1-10) of exponentially growing (about ~10^7 cells).
#Detach by pipeting a stream of media over the cells
#Detach by pipeting a stream of media over the cells

Latest revision as of 14:28, 5 June 2020

SOP

METHOD

  1. Use and early passage (1-10) of exponentially growing (about ~10^7 cells).
  2. Detach by pipeting a stream of media over the cells
  3. Transfer into a 15 mL falcon tube
  4. Spin at 500g for 10 min, save the supernatant
  5. Prepare freezing media:
    1. Add 4.5 mL supernatant
    2. Add 4.5 mL fresh media
    3. Add 100 uL sterile DMSO
  6. Resuspend to 1/10th original culture volume
  7. Dispense 0.5 mL into sterile cryovials
  8. Place in isopropanol freezing chamber and store at -80 for about a day
  9. Transfer to liquid nitrogen
  10. Cells should be viable for >5 years

see PMID 18388942

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