Functional role of IL-22 in psoriatic arthritis

This study was approved by the Institutional Review Board (IRB) of Veterans Affairs Medical Centre (VAMC), Sacramento. After obtaining IRB approved informed consent form, specimens were collected from patients with active PsA, RA and OA. RA and OA patients were recruited according to the clinical, laboratory and radiographic classification criteria of the American College of Rheumatology (ACR). Patients with PsA had either oligoarthritis or symmetric polyarthritis as described by Moll and Wright [31]. All patients with PsA fulfilled the CASPAR classification criteria for PsA [32]. Before enrolling in this study, patients had undergone complete physical examination, evaluation of severity of psoriasis and arthritis, appropriate blood tests and radiological studies. Active PsA or RA was defined by the presence of at least 3 swollen and 3 tender joints. In patients with PsA, in addition to the above, presence of plaque psoriasis with a qualifying lesion of at least 2 cm in diameter was checked. All patients were evaluated for the swollen joint count, the tender joint count, patient's assessment of pain, ESR and CRP.

SF and blood were collected from patients with PsA (n = 15), RA (n = 15) and OA (n = 15). Synovial fluid mononuclear cells (SFMC) and peripheral blood mononuclear cells (PBMC) were isolated from SF and blood respectively. SF and synovial tissues were collected from one or both knees of PsA, RA and OA patients. Synovial tissues were studied from PsA (n = 5), RA (n = 5) and OA (n = 5) patients. These subjects had an arthroscopic procedure or joint replacement for treatment of their arthritis. All enrolled patients were on NSAID or Acetaminophen except two RA patients were on low dose oral steroid (≤ 7.5 mg/day), six RA patients were on hydroxychloroquine; six RA and five PsA patients were on low dose methotrexate (< 10 mg/week). None of the PsA patients was on steroid. None of the RA or PsA patients was on biologics for at least 3 months before the enrollment for this study.

Peripheral blood and SF from the knee joints of patients with PsA (n = 15), RA (n = 15) and OA (n = 15) were collected. The SF was immediately centrifuged at 1600 rpm for 20 min at 4°C to remove cells and debris. SF supernatants were carefully removed and stored at -20°C for ELISA of IL-22 (Human IL-22 ELISA Kit, eBioscience, San Diego, CA, USA). Serum was stored at -20°C for ELISA of IL-22. Sensitivity for IL-22 detection by this kit is 8-1000 pg/ml.

FLS of PsA, RA and OA were grown in T75 flask and upon 70-80% confluence, cells were scrapped with a cell scrapper, then centrifuged for 8 min at 1600 rpm, 22°C. Lysis buffer containing 150 mM NaCl (Fischer Scientific, Houston, TX, USA), 50 mM Tris-HCL of pH 7.2 (Sigma-Aldrich, St. Louis, MO, USA), 1% w/v Triton X-100 (Sigma-Aldrich, St. Louis, MO, USA), 1% w/v sodium deoxycholate (Sigma-Aldrich, MO, USA), 0.1% w/v SDS (Fischer Scientific, Houston, TX, USA) with protease inhibitor (Roche, Indianapolis, IN, USA) was added and incubated for 40 min at 4°C. Supernatants were collected after centrifugation at 4°C, 13000 rpm for 20 min and the protein concentration was estimated using BCA Protein Assay Reagent Kit (Thermo-Fisher scientific, Houston, TX, USA). Cell lysate protein (30 μg) was used for western blot analysis. Cell lysate was run in a 10% acrylamide gel (BIO-RAD, CA, USA). The Immuno-Blot PVDF membrane (BIO-RAD, Richmond, CA, USA) was blocked with 5% nonfat dried milk in TBST (50 ml of 1 M Tris, 30 ml of 3 M NaCl, 20 ml of 10% Tween, ddH2O, total volume 1L) for 2 hour at room temperature. Then blots were incubated overnight at 4°C with the primary antibody, IL-22Rα1 (R&D Sytems, Minneapolis, MN, USA) at 3 μg/ml concentrations; αtubulin (Cell signaling Technologies, Danvers, MA, USA), 1:250 concentrations. Blots were washed 5x in TBST and secondary antibody (Jackson Immunoresearch Labs, PA, USA) was added at 1:5000 dilution. After keeping the blot in secondary antibody for 1 hr, it was washed 5x in TBST and then developed using ECL western blotting detection reagents solution (Thermo-Fisher Scientific, Houston, TX, USA) for chemiluminescent detection. Band density was measured using Image J software (NIH, Bethesda, MD, USA).

FLS (20,000/well) were seeded in a 24-well plate with 1 ml of complete DMEM (DMEM, 10%FBS, antibiotics). Cells were pre-treated with IL-22R Ab (1000 ng/ml) for 1 hr at 37°C then human rIL-22 (100 ng/ml) was added and incubated at 37°C in CO2 incubator for 5 days. MTT assay was done to determine the inhibitory effect of IL-22R Ab on IL-22 induced FLS proliferation.

To determine the source of IL-22, SFMC and PBMC isolated from SF and peripheral blood of PsA (n = 15), RA (n = 15) and OA (n = 15) were examined. PBMCs were isolated by Ficoll-hypaque gradient (GE Healthcare, Piscataway, NJ, USA) centrifugation of peripheral blood. Synovial fluid was treated with hyaluronidase enzyme (Sigma-Aldrich, MO, USA) at 1 mg/ml concentration for 5 mins at room temperature, then centrifuged at 2000 rpm for 20 min at 4°C. Cell pellet were resuspended in 1 ml of RPMI 1640 (Mediatech, Manassas, VA, USA) complete media (RPMI-1640 containing 10%FBS, antibiotics). Then the CD3⁺ T cells were separated magnetically from SFMC and PBMC using Easy Sep negative selection human T cell enrichment kit (Stem Cell Technology, Vancouver, BC, Canada) according to manufacturer's protocol and the purity was determined by flow cytometry using human anti CD3 antibody (BD pharmingen, San Diego, CA, USA). In a 24-well tissue culture plate, 1 × 10⁶ synovial CD3⁺ T cells and peripheral blood CD3⁺ T cells were seeded separately and stimulated with 50 ng/ml of phorbol myristate acetate (PMA) and 1 μg/ml of ionomycin (Sigma-Aldrich, MO, USA) for 24 hrs and 10 μg/ml of phytoheamagglutinin (PHA, Invitrogen, CA, USA) for 48 hrs. For mimicking physiological stimulation, FLS were cultured in 24-well plates coated with human anti CD3 and anti CD28 (5 μg/ml each) (BD Biosciences, San Diego, CA, USA) at 37°C. After 24 and 48 hrs, supernatant was collected and IL-22 was measured in the supernatant by ELISA.

All experiments were done in triplicate. Results were expressed as Mean ± SEM. For analysis of flow cytometric data, we considered the % of divided cells of each treatment group using the FlowJo software (TreeStar Inc, Ashland, OR, USA). All data were analyzed statistically using the GraphPad Prism software version 5.0 (GraphPad Software Inc, La Jolla, CA, USA). Non-parametric tests (Wilcoxon matched pairs signed rank test, Mann Whitney test, Friedman's ANOVA, Kruskal Wallis ANOVA with Dunn's multiple comparison test) were used to determine the statistical significance. A p value < 0.05 was considered statistically significant.

IL-22 levels in SF of PsA (17.75 ± 3.46 pg/ml) were significantly higher compared to that in OA (5.03 ± 0.39 pg/ml, p < 0.001, Kruskal-Wallis ANOVA with Dunn's multiple comparison test) (Figure 1). In SF of RA, highest concentration of IL-22 (21.06 ± 3.55 pg/ml) was observed. However, there was no significant difference of IL-22 levels between SF of PsA (17.75 ± 3.46 pg/ml) and RA (21.06 ± 3.55 pg/ml). Serum IL-22 levels in PsA, RA and OA were 9.22 ± 0.54 pg/ml, 9.64 ± 1.20 pg/ml and 4.45 ± 0.25 pg/ml respectively, p = ns, Kruskal Wallis ANOVA with Dunn's multiple comparison test (Figure 1). We found significantly higher levels of IL-22 in SF of PsA (17.75 ± 3.46 pg/ml) and RA (21.06 ± 3.55 pg/ml) compared to that in serum of PsA (9.22 ± 0.54 pg/ml) and RA (9.64 ± 1.20 pg/ml) (p < 0.01, Mann Whitney test). In OA, there was no significant difference of IL-22 levels between SF (5.03 ± 0.39 pg/ml) and serum (4.45 ± 0.25 pg/ml).

MTT and CFSE dilution assay were done to determine the proliferative effect of human rIL-22 in FLS of PsA, RA and OA. In MTT assay, significantly higher proliferation of PsA derived FLS were observed with rIL-22 (OD: 1.27 ± 0.06) compared to media (OD: 0.53 ± 0.02, p < 0.001, Friedman's ANOVA with Dunn's multiple comparison test) (Figure 2A). In this experiment we used rTNF-α as a positive control [11, 12] and significant proliferation were found with rTNF-α (OD: 1.53 ± 0.05) compared to media (OD: 0.53 ± 0.02, p < 0.001, Friedman's ANOVA with Dunn's multiple comparison test). There was no significant difference of proliferation between the rIL-22 (OD: 1.27 ± 0.06) and rTNF-α (OD: 1.53 ± 0.05) treated FLS. Here we observed a novel finding that rIL-22 induced significantly more proliferation in presence of rTNF-α (OD: 2.06 ± 0.11) than rIL-22 alone (OD: 1.27 ± 0.06, p < 0.01) (Figure 2A).

We also did this experiment in RA FLS and observed similar results; human rIL-22 (OD: 1.58 ± 0.05) and rTNF-α (OD: 1.96 ± 0.04) induced significant proliferation compared to media (OD: 0.65 ± 0.04, p < 0.001, Friedman's ANOVA with Dunn's multiple comparison test). In RA also, rIL-22 in presence of rTNF-α (OD: 2.37 ± 0.11) induced significantly more proliferation than rIL-22 alone (OD: 1.58 ± 0.05, p < 0.01). In OA FLS, rIL-22 (OD: 0.73 ± 0.12) as well rTNF-α (OD: 0.90 ± 0.16) induced significant proliferation compared to media (OD: 0.38 ± 0.05, p < 0.05, Friedman's ANOVA with Dunn's multiple comparison test).

We further confirmed the proliferative effect of human rIL-22 on FLS by CFSE dilution assay. In this assay, similar results were found regarding proliferation of FLS with rIL-22. In FLS of PsA, human rIL-22 (19.64 ± 3.13%) and human rTNF-α (24.60 ± 4.95%) induced significantly more proliferation compared to that in media only (5.58 ± 0.98%, p < 0.01, Friedman's ANOVA with Dunn's multiple comparison test) (Figure 2B and 2C). Here also, rTNF-α (24.60 ± 4.95%) showed more proliferation of FLS than rIL-22 (19.64 ± 3.13%), but there was no significant difference in proliferation of FLS between these two groups. In this assay also, rIL22 in presence of rTNF-α (30.76 ± 4.17%) showed more proliferation than rIL-22 alone (19.64 ± 3.13%, p < 0.05) (Figure 2B and 2C).

In RA patients also, rIL-22 (21.57 ± 3.33%) and rTNF-α (27.45 ± 3.29%) induced significant proliferation compared to that in media (6.43 ± 1.61%, p < 0.01, Friedman's ANOVA with Dunn's multiple comparison test). There was no significant difference of proliferation between rIL-22 and rTNF-α treated FLS. In RA also, we observed that rIL-22 induced significantly more proliferation of FLS in presence of rTNF-α (33.11 ± 2.42%) compared to rIL-22 alone (21.57 ± 3.33, p < 0.05).

IL-22Rα1 expression at protein level was done by western blotting. Expressions of IL-22Rα1 were found in FLS of PsA, RA and OA patients (Figure 3A). The relative intensity (R.I) of IL-22Rα1 in FLS of PsA, RA and OA patients was 0.92 ± 0.07, 0.94 ± 0.16 and 0.69 ± 0.18 respectively. There was no significant difference (Kruskal Wallis ANOVA with Dunn's multiple comparison test) in expressions of IL-22Rα1 between FLS of PsA, RA and OA patients (Figure 3B).

In MTT assay, there was a significant difference of proliferation between media (OD: 0.53 ± 0.02) and IL-22 + IL-22R Ab (OD: 0.76 ± 0.03, p < 0.05) treated FLS (Figure 4). Anti IL-22R (IL-22R Ab) antibody (OD: 0.76 ± 0.03) significantly inhibited the rIL-22 induced FLS proliferation in PsA (1.27 ± 0.06, p < 0.01, Friedman's ANOVA with Dunn's multiple comparison test) (Figure 4). There was no significant difference of proliferation between media (OD: 0.53 ± 0.02) and only IL-22R Ab (OD: 0.63 ± 0.03) treated FLS.

In FLS of RA also, IL-22R Ab (OD: 0.71 ± 0.03) significantly inhibited rIL-22 induced FLS proliferation (OD: 1.58 ± 0.05, p < 0.001, Friedman's ANOVA with Dunn's multiple comparison test. There was no significant difference of proliferation between media (OD: 0.65 ± 0.04) and only IL-22R Ab. (OD: 0.71 ± 0.03) treated FLS. In OA FLS, IL-22R Ab (OD: 0.49 ± 0.02) inhibited the rIL-22 induced proliferation (OD: 0.73 ± 0.12, p = ns), but there was no significant difference.

CD3⁺ T cells were obtained from synovial fluid and peripheral blood of PsA, RA and OA by magnetic bead sorting. The purity of enriched T cells was > 90% by flow cytometric analysis. Activated synovial T cells of PsA and RA produced significantly more IL-22 than that of OA. Moreover in PsA and RA, activated synovial T cells produced significantly more IL-22 than peripheral blood T cells of same patients [Table 1].