Evaluation of Stromal Cytokine-Induced Intracellular Protein Phosphorylation Using Phospho-Flow Cytometry
Published: November 30, 2023
Abstract
Source: Coats, J. S., et al. Expression of Exogenous Cytokine in Patient-derived Xenografts via Injection with a Cytokine-transduced Stromal Cell Line. J. Vis. Exp. (123) (2017).
This video demonstrates the evaluation of stromal cytokine-induced intracellular phosphorylation of proteins in leukemia cells. These intracellular phosphorylated proteins are quantified using the phospho-flow cytometry technique.
Protocol
1. Phospho-flow Cytometry Assays to Evaluate the Activity of Cytokine Produced by Stroma
NOTE: Assess the supernatant from the engineered stroma before the first experiment to verify the relevant bio-activity of the stroma-generated cytokine for the individual experiment. Once the engineered stroma is validated, further testing is not necessary unless stroma are introduced that were produced with a new vector.
- Purchase MUTZ5 and/or MHH-CALL4 leukemia cell lines (TSLP responsive), recombinant human cytokine, and antibodies approved for use in phospho-flow cytometry assays to detect appropriate downstream phosphorylation targets.
- Thaw harvested supernatant from control and cytokine-expressing stroma.
- Plate the leukemia cell lines in R20 medium (see Table of Materials) at a concentration of 0.2 x 106 cells per well in a 96-well tissue culture plate. Plate 3 wells per condition to allow for triplicate assays. Incubate for 2 h at 37 °C. This time allows for the loss of any phosphorylation that occurred during prior culture conditions.
NOTE: 12 wells per cell line provides triplicate assays for each experimental condition shown in step 1.4. - After 2 h in culture, transfer the cells from each well to separate 4 mL tubes and centrifuge at 500 x g for 5 min, at 4 °C. Decant the supernatant.
- Resuspend the cells in 200 µL for each of the following experimental conditions (perform assays in triplicate): 1) negative control-media only, 2) positive control-media with recombinant cytokine at saturating concentration(s) (TSLP at 15 ng/mL, etc.), 3) control stroma-supernatant from control stroma, and 4) cytokine-stroma-supernatant from cytokine-producing stroma.
- Incubate the cells for the duration specified by specific commercial phospho-assay (e.g. 30 min for phospho-STAT5 in MUTZ5 or MHH-CALL4 in response to TSLP).
- Centrifuge at 500 x g for 5 min at 4 °C and decant the supernatant.
- Perform phospho-flow cytometry staining per the manufacturer's protocol and collect flow cytometry data.
- Analyze flow cytometry data.
- Gate on intact cells based on forward (FSC, indicates cell size) and side (SSC, indicates cell granularity) light scatter.
- Determine the median fluorescent intensity (MFI) of the intact cells in each sample. Compare the average MFI obtained from the triplicate values of stromal cell supernatant to that of positive and negative media controls.
Disclosures
The authors have nothing to disclose.
Materials
| 10 mL serological pipettes | Falcon | 357551 | |
| 15 mL polypropylene conical tubes | Fisher | 05-539-12 | |
| 50 mL polypropylene conical tubes | Falcon | 352098 | |
| 1 mL pipette tips | Fisher | 2707509 | |
| 200 μL pipette tips | Denville Scientific | P3020-CPS | |
| 10 μL pipette tips | Denville Scientific | P-1096-CP | |
| “R20” cell culture medium, % of total volume (makes 195 mL) | Lab Recipe | ||
| RPMI, 76.84% (150 mL) | Mediatech | 10-040-CV | |
| FBS, 20.49% (40 mL) | Mediatech | 35-011-CV | |
| 2mM L-glutamine, 1.02% (2 mL) | Mediatech | 35-011-CV | |
| 1 mM Na pyruvate, 1.02% (2 mL ) | |||
| Penicillin-Streptomycin, 0.51% (1 mL | Mediatech | 30-002-Cl | |
| 2-Mercaptoethanol, 0.10% (0.1 M), 0.10% (200 µL) | MP | 190242 | |
| Biologics | |||
| "CALL-4" MHH-CALL-4 cell line, human B cell precursor leukemia | DSMZ | ACC 337 | |
| MUTZ-5 cell line, human B cell precursor leukemia | DSMZ | ACC 490 | |
| Recombinant Human TSLP protein | R&D Systems | 1398-TS-010 | |
| Flow cytomery antibodies (clone)* | |||
| Anti-mouse CD45 FITC (30F11) | Miltenyi Biotec | 130-102-778 | |
| CD127 PE (MB15-18C9) (alternate name is IL-7Rα) | Miltenyi Biotec | 130-098-094 | |
| CD34 APC (8G12) | BD Biosciences | 340667 | |
| CD45 PE-Cy7 (HI30) | eBioscience | 25-0459 | |
| "FVD" Fixable viability dye eFluor 780 | eBioscience | 65-0865 | |
| Ig κ light chain FITC (G20-193) | BD Pharmingen | 555791 | |
| Ig λ light chain FITC (JDC-12) | BD Pharmingen | 561379 | |
| IgD PE (IA6-2) | BioLegend | 348203 | |
| IgM PE-Cy5 (G20-127) | BD Biosciences | 551079 | |
| pSTAT5 PE, mouse anti-STAT5 (pY694) | BD PhosphoFlow | 612567 | |
| Other materials & equipment | |||
| FlowJo flow cytometry analysis software | FlowJo, LLC | Version 10 | |
| *All antibodies are anti-human unless otherwise stated. |
Cite This Article
Evaluation of Stromal Cytokine-Induced Intracellular Protein Phosphorylation Using Phospho-Flow Cytometry. J. Vis. Exp. (Pending Publication), e21808, doi: (2023).