Cellular ELISA Protocol

Author: Nanci Donacki

Source: Contributed by Nanci Donacki

Date Added: 2002-05-14
Date Modified: 2004-04-28

 Formalin Fixed Cell Plates

  1.  Trypsinize confluent flasks
  2. Pool and count cells
  3. Centrifuge at 1500 rpm for 10 minutes
  4.  Resuspend to the appropriate concentration in complete medium
    4 x 105 cells/ml for epithelial cells
    2 x 105 cells/ml for fibroblast cells
  5.  Add 100 æl/cell to 96 well culture plates.
  6. Incubate overnight at 37oC.
  7. Wash plates twice with PBS
  8.  Add 125 æl/well 10% Buffered Formalin
  9.  Fix for 15 minutes at room temperature
  10. Wash three times with di-H2O.
  11. Blot dry.
  12. Store at 2-8oC.

 Reagents

  1.  PBS:1% BSA
  2. PBS:2% BSA
  3. Carbonate Buffer
    1.59 g      Na2CO3
    2.93 g      NaHCO3
    Dissolve in 900 ml di-H2O.  Check pH and adjust to 9.6 necessary.  Qs. to 1 liter.
  4. 10X Substrate Buffer, pH 6.0
    36.6 g      Citric Acid, monohydrate
    113.5 g      Potassium dibasic phosphate
    Dissolve in 900 ml di-H2O.  Check pH and adjust to 6.0 if necessary.  Qs. to 1 liter.
  5.  0.3% H2O2
    Dilute 30% stock Peroxide 1:100 in di-H2O.
  6. OPD Stock, 4.0%
    4 g OPD in 100 ml di-H2O.  Aliquot and store at -20oC.  Protect from light.
  7.  4.5N H2SO4
    12.0 ml      Concentrated Sulfuric Acid
    88.0 ml      di-H2O

Procedure

  1. Wash ELISA plates once with di-H2O.
  2. Add 250 æl/well PBS:2% BSA.
  3.  Incubate 1 hour at 37oC.
  4. Wash 3 times with di-H2O.
  5.  Add 50 æl/well supe, ascites, or controls diluted in PBS:1%BSA.
  6.  Incubate for 2 hr at 37oC.
  7. Wash 5 times with di-H2O.
  8. Add 50 æl/well anti-mouse IgG:HRP diluted in PBS:1% BSA.
  9.  Incubate for 1 hr at 37oC.
  10. Wash 5 times with di-H2O.  Wash once with carbonate buffer.
  11. Add 50 æl/well working substrate solution
    0.5 ml      4.0% OPD
    5 æl      30% H2O2
    1.0 ml      10X Substrate buffer
    8.5 ml      di-H2O.
  12. Incubate for 20 minutes at room temperature.
  13. Add 25 æl/well 4.5N Sulfuric Acid
  14. Read A490

Notes

  1.  Test all supernatants at 1:5 dilution.
  2.  Test ascites at 1:100


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