Immunohistochemistry: Fluorescence Protocol 2.0

• R&D Systems 'AF' or 'BAF' series ) or selected monoclonal antibodies.

Secondary Antibodies and Secondary Reagents

• Biotinylated donkey anti-goat IgG (Jackson Immuno Research Lab Catalog # 705-066-147)
• Biotinylated goat anti-mouse IgG₁ ( Caltag Lab Catalog # M32115)
• FITC-labeled goat anti-mouse IgG₁ ( Caltag Lab Catalog # M32001)
• FITC-labeled anti-mouse IgG_2A ( Caltag Lab Catalog # M32201)
• FITC-labeled anti-mouse IgG_2B ( Caltag Lab Catalog # M32401)
• Oregon Green coupled anti-mouse IgG (Molecular Probes Catalog # 06380)
• Oregon Green-avidin D(Molecular Probes Catalog # A6374)
• FITC-Avidin D ( Sigma Catalog # A-2001)

Buffers and Additional Supplies

• Fixation Buffer Formaldehyde (37% v/v Sigma ) is diluted in PBS to a final formaldehyde concentration of 2% (v/v) and adjust pH to 7.4. Light sensitive, store at 4°C in the dark; prepare working dilution just prior to fixation
• Wash Buffer Earls Buffered Salt Solution (EBSS) (Gibco BRL)
• Wash Buffer-Saponin EBSS with 0.1% (w/v) Saponin ( Sigma Catalog # S4521) and adjust pH to 7.2-7.4 with NaOH.
• Endogenous Peroxidase Blocking Buffer 3M NaN₃ in EBSS with 1% H₂ O₂ and 0.1% (w/v) Saponin.
• Endogenous Biotin Blocking Buffer Avidin/Biotin Blocking Kit (Vector Lab Catalog # SP2001). Both Avidin D and Biotin should be supplemented with 0.1% (w/v) Saponin.
• Fluorescence Anti Fading Mounting Medium Carbonate/bicarbonate buffered glycerol (1:1 v/v) containing 2 % 1,4-Diazobicyclo 2.2 octane (Sigma Catalog # D2522) and adjust pH to 7.4.
• Saponin stock Prepare a stock of 10 % (w/v) Saponin in EBSS. Prepare fresh, since crude saponin powder batches are generally fungi infected.
• Intracellular transport inhibitor Brefeldin A ( Sigma Catalog # B7651)
• Microscope slides Adhesion slides ( BioRad Catalog # 12550-15) (smeared cells); TC microscope glass slides (tissue sections); HTC slides (Cel-line Assoc. Catalog # 10-618)
• Frozen tissue embedding OCT-compound ( VWR Catalog # 25608-930)
• Humidified Chamber A plastic light protected box lined with wet paper towels.

Controls
Positive staining controls

• Stain fixed, permeabilized cytokine-cDNA transfected eukaryotic cells expressing the intra-cellular target cytokine protein.
• Stain cultured blood mononuclear cells or spleen cells that have been harvested, fixed and permeabilized at the peak of cytokine production after in vitro stimulation with strong polyclonal activators such as phorbol 12-myristate 13 acetate/ionomycin, anti-CD3⁺ CD28 monoclonal antibody, LPS or bacterial superantigens such as staphylococcal enterotoxin A (SEA), staphylococcal enterotoxin B (SEB) or streptococcal pyrogenic exotoxin A (SPE-A).

Negative staining controls

• Ligand blocking control : to study the specificity of the cytokine staining by a preincubation of the cytokine-specific antibody with its target cytokine at a molar ratio of 1:10 prior to addition to the cells.
• Isotype matched control immunoglobulin : Stain the cells by a primary isotype pre-matched immunoglobulin of irrelevant antigen-specificity at the same concentration as the cytokine-specific antibodies.
• Unlabeled antibody control : Cells that will be stained by a fluorochrome or a biotinylated primary cytokine-specific antibody will be incubated initially with the unconjugated version of the same antibody.
• Non transfected eukaryotic cells and unstimulated PBMNC are good negative controls.

Immunofluorescent staining of cytokine-producing cells in suspension

1. Harvest cells and wash twice in V-bottomed tubes with cold Wash Buffer by centrifugation (400 x g for 5 minutes) to remove extracellular proteins, including cytokines.
2. Resuspend to 1-5 x 10⁶ cells/mL in Wash Buffer.
3. Transfer 10-15 µL of the cell suspension to each reaction field on the adhesion slide.
4. Allow the cells to adhere electrostatically in a monolayer for 10 minutes at room temperature in the humidified chamber to prevent the cells from drying out.
5. Add 50 µL of ice-cold Fixation Buffer to each field to fix the cells.
6. Incubate for 20 minutes at 4°C.
7. Wash three times with Wash Buffer to remove free formaldehyde.
8. Add 25 µL of 2% fetal bovine serum in Wash Buffer to block unbound surface area on the slide.
9. Incubate for 10 minutes at 37°C.
   1. Wash slides three times in Wash Buffer-Saponin. The slides are now ready for staining.
   2. Alternatively, wash the slides in Wash Buffer and allow the slides to dry. Dried slides can be stored at -20°C several months before being stained. Prior to staining the slides should be washed in Wash Buffer-Saponin.

1. Incubate in Endogenous Peroxidase Blocking Buffer for 30 minutes at room temperature in the dark to block endogenous peroxidase activity in the cells (this step can be omitted if cells are to be stained by fluorochromes or non-peroxidase based enzymatic methods).
2. Block endogenous biotin activity with the Avidin/Biotin blocking kit in a two step procedure for 30 minutes in the presence of saponin, described in steps 3-5.
3. Incubate each cell spot on slides with Avidin for 15 minutes supplemented with saponin (0.1% w/v).
4. Wash each cell spot on slides twice in Wash Buffer-Saponin.
5. Incubate in Biotin for 15 minutes supplemented with saponin (0.1% w/v).
6. Wash each cell spot on slides twice in Wash Buffer-Saponin.
7. Incubate each cell spot on slides for 30 minutes at room temperature with 15 µL unlabeled or biotinylated cytokine-specific antibodies (0.5-5 µg/mL) diluted in Wash Buffer-Saponin.
   
8. Wash slides three times in Wash Buffer-Saponin.
   Note: If using R&D Systems biotinylated antibody skip steps 9 and 10 and continue.
9. Incubate each cell spot on slides for 30 minutes at room temperature with 15 µL of a biotinylated secondary antibody (either biotin-donkey anti-goat IgG Fab₂ diluted 1:700; or biotin-goat anti mouse IgG₁ or IgG_2A or IgG_2B diluted 1:500) in Wash Buffer-Saponin.
10. Wash slides three times in Wash Buffer-Saponin.

Cytokine-specific staining based on either biotinylated primary antibodies or unlabeled primary antibodies along with biotinylated secondary antibodies can then be developed by techniques based on immunoflourescence or immunoenzymatic methods.

1. Incubate slides for 30 minutes at room temperature with 15 µL of Oregon-Green Avidin or FITC-Avidin at a concentration of 2-5 µg/mL in Wash Buffer-Saponin.
2. Wash slides twice in Wash Buffer-Saponin.
3. Wash slides once in Wash Buffer only. Allow slides to air dry before mounting in Mounting Buffer. FITC staining, but not Oregon-Green staining, will require a mounting medium including some anti-fading substance to reduce UV quenching. It is possible to store fluorochrome-stained slides for long periods in the freezer, provided that they have not been mounted in Mounting medium.

b. Detection using fluorochrome-labeled antibodies
If cytokine producing cells are to be detected by fluorochrome-labeled primary or secondary antibodies there is no need to block endogenous peroxidase or biotin activity. Background signals are often reduced when fluorochrome-labeled antibodies are used in Wash Buffer-Saponin supplemented with 5% human AB serum.

1. Incubate each cell spot on slides for 30 minutes at room temperature with 15 µL of either unlabeled or fluorochome-labeled primary cytokine-specific antibodies (0.5-5 µg/mL) diluted in Wash Buffer-Saponin supplemented with 5% human AB serum.
2. Wash slides three times in Wash Buffer-Saponin.
3. Incubate cells for 30 minutes at room temperature with 15 µL of flurochrome-labeled secondary antibody (either FITC-labeled anti-mouse IgG₁ or IgG_2A or IgG_2B diluted 1:300) in Wash Buffer-Saponin supplemented with 5% human AB serum.
4. Wash slides three times in Wash Buffer-Saponin and air dry the slides.
5. Mount and coverslip with Fluorescence Anti Fading Mounting Medium.