What You Need

Materials

• Indicator cell line (see Quick Guide Chart for a given cytokine)
• Culture Medium (RPMI supplemented with 10% FBS)
• Assay Medium (RPMI supplemented with 10% FBS)
• 96-well flat-bottom culture plate (Costar Cat. No. 3595)
• MTT solution (Sigma Cat. No. M5655) 5mg/ml stock in PBS kept at room temperature (protect from light)
• MTT Lysing Solution 20% SDS/50% DMF

Instruments

• Pipettes and pipettors
• Humidified incubator
• 96-well micro test spectrophotometer

Experiment Duration

• 24-48 hour incubation (see Quick Guide Chart )
• 1 hour assay preparation

Method

1. Add 50 µl/well of Assay Medium to each well of the 96-well Assay plate.
2. Dilute Functional Grade (FG) anti-cytokine antibody by 2-fold serial dilution in the Assay plate from row 3 to 12. Leave rows 1 and 2 blank (control rows).
3. Add 50 µl/well of samples and recombinant cytokine (see Quick Guide Chart for concentration) to the assay plate from row 2 to row 12 (row 2 will be indicator cells and cytokine). Leave row 1 blank (cells alone).
4. Incubate the plate at 37°C, 5% CO₂ in a humidified incubator for 2 hours.
5. Wash indicator cells 3 times with RPMI1640 and resuspend in Assay Medium at a density of 2-3.5x10⁵ cells/ml (see Quick Guide Chart ).
6. Add 100 µl of cell suspension to each well.
7. Incubate cells for 24-48 hours (see Quick Guide Chart ) at 37°C, 5% CO₂ in a humidified incubator.
8. Add 10 µl/well of 5 mg/ml MTT solution to the plate and incubate for 4 hours.
9. Add 50 µl/well of MTT Lysing Solution to the plate and incubate overnight.
10. Read plate at 570-650 nm.
11. Graph standard curve and analyze data.

What You Need

Materials

• L929 mouse fibroblast line (ATCC Cat. No. CCL-1)
• Culture Medium (RPMI supplemented with 10% FBS)
• Assay Medium (RPMI supplemented with 2% FBS)
• 96-well flat-bottom culture plate (Costar Cat. No. 3595)
• Actinomycin D, 500 µg/ml stock aliquot kept at minus 80°C (protect from light)
• MTT solution (Sigma Cat. No. M5655) 5 mg/ml stock in PBS kept at room temperature (protect from light)
• MTT Lysing solution, 20% SDS/50% DMF

Instruments

• Pipettes and pipettors
• Humidified incubator
• 96-well micro test spectrophotometer

Experiment Duration

• 48-hour incubation (see Quick Guide Chart )
• 1 hour assay preparation

Method

1. Prepare L929 cell suspension at a density of 3.5x10⁵ /ml in assay medium. Add 100 µl/well to the 96-well Assay Plate and incubate overnight at 37°C, 5% CO₂ in a humidified incubator.
2. Add 50 µl/well of Assay Medium to each well of another dilution plate.
3. Dilute Functional Grade (FG) anti-cytokine antibody by 2-fold serial dilution in the plate from row 3 to 12. Leave rows 1 and 2 blank (control rows).
4. Add 50 µl/well of samples and recombinant cytokine (see Quick Guide Chart for concentration) to the dilution plate from row 2 to row 12 (row 2 will be indicator cells and cytokine). Leave row 1 blank (cells alone).
5. Incubate the dilution plate at 37°C, 5% CO₂ in a humidified incubator for 2 hours.
6. Transfer 50 µl/well of the Ab/Ag mixed solution to the corresponding well of the Assay Plate containing cells.
7. Prepare a 4 µg/ml working solution of the Actinomycin D by diluting the 500 µg/ml stock 125 times in the Assay Medium. Keep Actinomycin D solution protected from light. Add 50 µl of this working solution of Actinomycin D to each well.
8. Incubate plate for 24 hrs at 37°C, 5% CO₂ in a humidified incubator.
9. Add 10 µl/well of 5 mg/ml MTT solution to each well and incubate for 4 hours.
10. Add 50 µl of MTT Lysing Solution to each well and incubate overnight.
11. Read plate at 570-650 nm.
12. Graph standard curve and analyze data.

What You Need

Materials

• L929 mouse fibroblast line (ATCC Cat. No. CCL-1) or A549 human lung carcinoma (ATCC Cat. No. CCL-185)
• Culture Medium (RPMI supplemented with 10% FBS)
• Assay Medium (RPMI supplemented with 2% FBS)
• 96-well flat-bottom culture plate (Costar Cat. No. 3595)
• EMC virus, 10⁷ pfu/ml aliquots stock kept at minus 80°C
• MTT solution (Sigma Cat. No. M5655) 5 mg/ml stock in PBS kept at room temperature (protect from light)
• MTT Lysing solution, 20% SDS/50% DMF

Instruments

• Pipettes and pipettors
• Humidified incubator
• 96-well micro test spectrophotometer

Experiment Duration

• 24 hour incubation (see Quick Guide Chart )
• 1 hour assay preparation

Method

1. Prepare L929 or A549 cell suspension at a density of 3.5x10⁵ /ml in assay medium. Add 100 µl/well to the 96-well Assay Plate and incubate overnight at 37°C, 5% CO₂ in a humidified incubator.
2. Add 50 µl/well of Assay Medium to each well of anther dilution plate.
3. Dilute Functional Grade (FG) anti-cytokine antibody by 2-fold serial dilution in the plate from row 3 to 12. Leave rows 1 and 2 blank (control rows).
4. Add 50 µl/well of samples and recombinant cytokine (see Quick Guide Chart for concentration) to the dilution plate from row 2 to row 12 (row 2 will be indicator cells and cytokine). Leave row 1 blank (cells alone).
5. Incubate the dilution plate at 37°C, 5% CO₂ in a humidified incubator for 2 hours.
6. Transfer 50 µl/well of the Ab/Ag mixed solution to the corresponding well of the Assay Plate containing cells.
7. Incubate the Assay Plate for 6 hours.
8. Aspirate supernatant from the wells carefully and add 100 µl/well of EMC virus solution at a density of 1-4x10⁴ pfu/ml (see Quick Guide Chart for human IFN-g: 1/250 dilution of stock of 10⁷ pfu/ml, for mouse IFN-g, 1/1000 dilution of stock of 10⁷ pfu/ml).
9. Incubate plate for 40 hours at 37°C, 5% CO₂ in a humidified incubator.
10. Add 10 µl of 5 mg/ml MTT solution to each well and incubate for 4 hours.
11. Add 50 µl of MTT Lysing Solution to each well and incubate overnight.
12. Read plate at 570-650 nm
13. Graph standard curve and analyze data.