Difference between revisions of "Splitting Cells"

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m (Cell Specific Notes)
(Protocol)
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#Warm PBS and Media in water bath
 
#Warm PBS and Media in water bath
 
#Wash cells twice with 10 mL (per 10 cm dish) PBS -/-
 
#Wash cells twice with 10 mL (per 10 cm dish) PBS -/-
#Add 1 mL trypsin and sit in the hood
+
#Add 1 mL trypsin and sit in the hood for 2-5 min
 
#Add 10 mL media to each new dish
 
#Add 10 mL media to each new dish
 
#Check cells for trypsinization, and if necessary tap the cells
 
#Check cells for trypsinization, and if necessary tap the cells
Line 13: Line 13:
 
#Add 1 mL cells to each dish (for 10X dilution; 0.5 mL for 20X)
 
#Add 1 mL cells to each dish (for 10X dilution; 0.5 mL for 20X)
 
#Replace plates in the incubator
 
#Replace plates in the incubator
 +
 
==Cell Specific Notes==
 
==Cell Specific Notes==
 
*3T3-L1 fibroblasts have special considerations regarding confluence.  See [[Differentiation of 3T3-L1 Cells]]
 
*3T3-L1 fibroblasts have special considerations regarding confluence.  See [[Differentiation of 3T3-L1 Cells]]

Revision as of 17:29, 26 October 2009

Materials

  • Media (L1-FBS for 3T3-L1, COS-FBS for others): Prepare by filtering together 5 mL PSG, 50 mL COS-FBS and one bottle of DMEM
  • PBS -/-
  • 0.05% Trypsin

Protocol

  1. Warm PBS and Media in water bath
  2. Wash cells twice with 10 mL (per 10 cm dish) PBS -/-
  3. Add 1 mL trypsin and sit in the hood for 2-5 min
  4. Add 10 mL media to each new dish
  5. Check cells for trypsinization, and if necessary tap the cells
  6. Add 9 mL media to trypsinized cells
  7. Add 1 mL cells to each dish (for 10X dilution; 0.5 mL for 20X)
  8. Replace plates in the incubator

Cell Specific Notes

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