Difference between revisions of "Electroporation of 3T3-L1 Adipocytes"

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(changed default siRNA to 5 uL (500 pmoles) and made some extra notes)
 
(One intermediate revision by the same user not shown)
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==Materials==
 
==Materials==
*Differentiated cells FBS day 3 or less.
+
*Differentiated cells FBS day 3 or less.  If cells are difficult to trypsinize, they will not recover well.
 +
**To calculate the number of cells, use 1 - 15cm dish per final dish (10cm/6well/12well).
 +
**For example for 2 knockdowns, each being seeded in 6 - 12 well sized wells, use 1 dish, and 2 electroporations.
 
*Gene Pulser cuvette
 
*Gene Pulser cuvette
 
*DNA:  CsCl Purified or siRNA (resuspended to 0.1 nmol/uL with 200 uL water)
 
*DNA:  CsCl Purified or siRNA (resuspended to 0.1 nmol/uL with 200 uL water)
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==Protocol==
 
==Protocol==
 
#Warm media and PBS but not trypsin in water bath
 
#Warm media and PBS but not trypsin in water bath
#Wash cells twice with PBS (-/-), then trypsinize and with 2 mL 0.25% trypsin in the incubate
+
#Wash cells twice with PBS (-/-), then trypsinize and with 2 mL 0.25% trypsin in the incubator
 
#When cells have fallen off the plate, add 9 mL Media and pipet into a 15 mL falcon tube
 
#When cells have fallen off the plate, add 9 mL Media and pipet into a 15 mL falcon tube
 
#Spin at 2000 RPM for 5 min.
 
#Spin at 2000 RPM for 5 min.
 
#Wash cells with PBS +/+
 
#Wash cells with PBS +/+
 
#Reuspend cells to a final volume of 0.5 mL per electroporation in PBS +/+  
 
#Reuspend cells to a final volume of 0.5 mL per electroporation in PBS +/+  
#500 uL of cells is mixed with 50-200 ug of DNA (or 10 uL siRNA) in a 0.4 cm cuvette
+
#500 uL of cells is mixed with 50-200 ug of DNA (or 5 uL siRNA) in a 0.4 cm cuvette.  These volumes are for half of a final plate of cells.  Scale up or down accordingly.
#Electroporate at 260V and 950 uF
+
#Electroporate at 160V and 950 uF
#Add 1 mL media to cuvette and transfer to a 15 mL tube with media for 10 min.   
+
#Add 1 mL media to cuvette and transfer to a 15 mL tube with media for 10 min.  The amount of media should correspond to the final volume of plated cells (ie one electroporation of half a plate of cells would go into 6 mL final volume of media).   
 
#Aspirate floating debris before replating
 
#Aspirate floating debris before replating
 
#Bring up tube to final required volume, mix and plate
 
#Bring up tube to final required volume, mix and plate

Latest revision as of 18:45, 17 February 2010

Materials

  • Differentiated cells FBS day 3 or less. If cells are difficult to trypsinize, they will not recover well.
    • To calculate the number of cells, use 1 - 15cm dish per final dish (10cm/6well/12well).
    • For example for 2 knockdowns, each being seeded in 6 - 12 well sized wells, use 1 dish, and 2 electroporations.
  • Gene Pulser cuvette
  • DNA: CsCl Purified or siRNA (resuspended to 0.1 nmol/uL with 200 uL water)
  • PBS +/+
  • PBS -/-
  • 0.25% Trypsin
  • L1 FBS Media


Protocol

  1. Warm media and PBS but not trypsin in water bath
  2. Wash cells twice with PBS (-/-), then trypsinize and with 2 mL 0.25% trypsin in the incubator
  3. When cells have fallen off the plate, add 9 mL Media and pipet into a 15 mL falcon tube
  4. Spin at 2000 RPM for 5 min.
  5. Wash cells with PBS +/+
  6. Reuspend cells to a final volume of 0.5 mL per electroporation in PBS +/+
  7. 500 uL of cells is mixed with 50-200 ug of DNA (or 5 uL siRNA) in a 0.4 cm cuvette. These volumes are for half of a final plate of cells. Scale up or down accordingly.
  8. Electroporate at 160V and 950 uF
  9. Add 1 mL media to cuvette and transfer to a 15 mL tube with media for 10 min. The amount of media should correspond to the final volume of plated cells (ie one electroporation of half a plate of cells would go into 6 mL final volume of media).
  10. Aspirate floating debris before replating
  11. Bring up tube to final required volume, mix and plate