Background
Interleukin (IL)-37 is a member of the IL-1 family, discovered by computational cloning, and previously termed IL-1 family member 7 [
1]. Quite distinct from most IL-1 family members, which are characterized by proinflammatory functions, IL-37 has emerged as a fundamental inhibitor of the innate immune response by shifting the cytokine equilibrium away from excessive inflammation [
2]. The function of IL-37 is also caspase-1-dependent. Caspase-1 processing is required not only for maturation of the intracellular IL-37 precursor and translocation of the cytokine to the nucleus, but also for the secretion of mature IL-37. IL-37 is reported to be a dual-function cytokine with intracellular and extracellular properties. IL-37 interacts intracellularly with mammalian homologs of the drosophila Mad gene 3 (Smad3), whereas the IL-1R8–IL-18Rα complex acts as the cell surface receptor for IL-37, and IL-37 uses IL-1R8 to trigger multiple intracellular switches to block inflammation [
3,
4].
Gout is a typical innate immune response triggered by monosodium urate crystal (MSU); IL-1β is critical to the acute gouty inflammation [
5], while transforming growth factor β1 (TGF-β1) plays an important role in limiting inflammation [
6]. As IL-37 functions as a natural suppressor of innate immunity, whether and how IL-37 downregulates inflammation induced by the danger signal MSU is not known. Although IL-37 exhibits the opposite function to IL-1β, there are many similarities between them: first, they are both first synthesized as precursor molecules and are processed to their mature forms by NACHT-LRR-PYD-containing protein 3 (NLRP3)-activated caspase-1 cleavage [
3]; second, toll-like receptor (TLR) ligands can induce their intracellular precursor expression and cause inflammasome priming. IL-37 shares the same intracellular inhibitory conduction signal Smad3 with the immunoregulatory cytokine TGF-β1. Interestingly, IL-1β and low concentrations of TGF-β1 have been shown effective in inducing endogenous IL-37, which is relevant to the interaction of IL-37 with Smad3 [
2]. Based on these findings, we speculated that upon stimulation by MSU, macrophages produce not only the proinflammatory cytokine IL-1β, but also the anti-inflammatory cytokine IL-37 through NLRP3 activation, to initiate a negative feedback mechanism to curb excessive inflammation.
In the current study, we investigated the expression of IL-37 in patients with active and inactive gouty arthritis. We also assessed the effect of recombinant human IL-37 (rhIL-37) in different human and murine gouty models: a human monocyte cell line (THP-1), human synovial cells (containing macrophage-like and fibroblast-like synoviocytes), a peritoneal murine model of gout and a murine gouty arthritis model. Our results support the idea that the presence of rhIL-37 attenuates the inflammatory process in gout, and it has both preventive and therapeutic effects. To our knowledge, this is the first study to show the anti-inflammatory properties of rhIL-37 in human and murine gouty models.
Methods
Patients and healthy controls
A total of 31 patients with gout were included in the current study. The classification of gout fulfilled the 1977 American Rheumatism Association (now the American College of Rheumatology (ACR)) preliminary criteria for the classification of the acute arthritis of primary gout and the 2015 ACR/European League Against Rheumatism (EULAR) gout classification criteria [
7,
8]. Gouty patients were divided into acute (
n = 16) and non-acute (
n = 15) groups. Healthy controls (
n = 18) with no hyperuricemia, no metabolic syndrome or other chronic diseases were recruited. Peripheral blood samples were obtained from patients with gout and healthy controls. Serum samples were stored at −80 °C until cytokine levels were determined. Peripheral blood mononuclear cells (PBMCs) from patients and healthy controls were isolated using Ficoll-Paque PLUS (GE Healthcare, Piscataway, NJ, USA), according to the manufacturer’s instructions. The collected cells were used for cell cultures or stored at −80 °C until RNA extraction. Synovial fluids were collected from five patients with acute gout and stored at −80 °C prior to assay. Synovial tissue from patients with active gouty arthritis and subcutaneous tophus from patients with chronic tophaceous gout were subjected to immunohistochemical analysis.
Preparation of MSU crystals
MSU crystals were prepared as described by Denko and Whitehouse [
9]. Briefly, 4 g uric acid was dissolved in 800 ml of deionized water, heated to 60 °C, adjusted to pH 8.9 with 0.5 N NaOH, and crystallized overnight at room temperature. MSU crystals were recovered by centrifugation, washed with distilled water and dried at 40 °C for 24 h. Crystal shape and birefringence were assessed by compensated polarized light microscopy. MSU crystals were milled and then sterilized by heating at 180 °C for 2 h before each experiment. We measured <0.015 EU/ml endotoxin in MSU crystal preparations using a Limulus amebocyte lysate assay (Sigma-Aldrich, St Louis, MO, USA).
Induction of gout models in vitro and rhIL-37/Mertk inhibitor treatment
THP-1-derived macrophages
THP1 monocytes were suspended in complete medium, consisting of RPMI 1640, 2 mM L-glutamine, 100 units/ml of penicillin, 100 μg/ml of streptomycin, supplemented with 10% fetal bovine serum (FBS) (Gibco BRL, Grand Island, NY, USA) and were seeded in 24-well culture plates (2 × 10
5 cells/ml/well). Cells then were treated with 50 ng/ml phorbol myristate acetate (PMA) for 24 h to generate THP-1-derived macrophages [
2]. THP-1-derived macrophages were treated with or without 10 ng/ml recombinant human IL-37 (rhIL-37; R&D Systems, Minneapolis, MN, USA) for 3 h, followed by incubation for 1 h with or without a small-molecule inhibitor of Mertk (Mertk inhibitor UNC2250, 20 nM; Selleckchem, Houston, TX, USA) and then incubated with either 1 μg/ml lipopolysaccharide (LPS) (Sigma), 5 mM ATP (Sigma), or MSU (50 μg/ml, 100 μg/ml) separately for a further 18 h. Culture supernatants were harvested and frozen at −80 °C for later cytokine analysis by ELISA.
Synoviocytes
Synovial tissue specimens were obtained from patients with osteoarthritis, who were undergoing surgical joint replacements. Synovial cells (containing macrophage-like and fibroblast-like synoviocytes) were isolated from tissue explants and cultured as previously described [
10]. Briefly, tissues were minced and incubated with a solution containing 0.15 mg/ml DNase, 0.15 mg/ml hyaluronidase (type I-S), and 1 mg/ml collagenase (type IA) (Sigma-Aldrich) in Dulbecco’s modified Eagle’s medium (DMEM; Invitrogen, Carlsbad, CA, USA) for 1 h at 37 °C. Cells were washed and resuspended in DMEM supplemented with 10% FBS, 30 mg/ml glutamine, 250 μg/ml amphotericin B (Sigma-Aldrich), and 20 μg/ml gentamicin (Invitrogen). After overnight culture, non-adherent cells were removed, and adherent cells were cultured and seeded in 6-well culture plates (1 × 10
6 cells/ml/well).
All experiments were performed with cells obtained after passage 2. Cell-specific markers were used to identify synoviocyte populations. Macrophage-like synoviocytes (MLS) were CD68+, as demonstrated by specific fluorescence antibody staining (Biolegend, San Diego, CA, USA) and flow cytometry analysis. Synovial cells were treated with or without rhIL-37 (R&D Systems) 10 ng/ml for 3 h and incubated with LPS 1 μg/ml, ATP 5 mM, or MSU (50 μg/ml, 100 μg/ml) separately for a further 6 h or 18 h. The supernatants were harvested and frozen at −80 °C for later cytokine analysis by ELISA.
In vivo experiments and IL-37/Mertk inhibitor treatment
MSU crystal-induced murine peritonitis
Male C57BL/6 mice, 6–8 weeks old, were injected intraperitoneally (IP) with MSU crystals suspended in phosphate-buffered saline (PBS) (3 mg/0.5 ml). rhIL-37 (1000 ng/mouse) was given IP once either 72 h, 48 h and 24 h prior to MSU crystal administration or 1 h after it. All controls received vehicle alone. At 3 h after MSU crystal administration, mice were killed and monitored for cell recruitment in the peritoneal lavage fluid, and chemokine expression and production. Cells collected by peritoneal lavage were retained for subsequent flow cytometry analysis. Peritoneal lavage fluid was stored at −80 °C for later chemokine analysis by LEGENDplex™ Muti-Analyte Flow Assays (Biolegend).
Murine gouty arthritis
Male C57BL/6 mice, 6–8 weeks old, were anesthetized in by inhalation of 3% isoflurane (Forane; Abbot, Chicago, IL, USA) and then intra-articular injected with 50 μl (1 mg) MSU suspension into the right foot pad [
11]. PBS was injected into the left foot pad at the same time as a control. rhIL-37 was given IP once either 72 h and 24 h prior to MSU crystal administration or 1 h and 4 h after it and at different concentrations (1000 and 100 ng/mouse). For the Mertk inhibitor group, UNC2250 (60 μg UNC2250/100 μl dimethyl sulfoxide (DMSO)) was injected IP into mice prior to MSU crystal administration and rhIL-37 intervention on two successive days. All controls received the diluent alone. At 8 h after MSU crystal administration, mice were killed after monitoring for joint swelling. Joint tissues were removed and stored for further RNA and protein extraction, or fixed in formalin for histopathologic analysis.
Joint swelling was examined by digimatic caliper (Mitutoyo, Kawasaki, Japan), the minimum accuracy of which was 0.01 mm [
12]. Joint inflammation was expressed as the ratio of the foot pad thickness of the inflamed over the normal control joint; values exceeding 1.10 were categorized as inflammation.
Histological studies and immunohistochemistry
Mouse joint tissue sections were prepared and stained with H&E. Synovial tissue from patients with active gouty arthritis and subcutaneous tophus from patients with chronic tophaceous gout were subjected to immunohistochemical analysis. Rabbit anti-IL-37 antibody (ab153889; Abcam, Cambridge, MA, USA) and goat anti-rabbit IgG H&L (ab97051; Abcam) secondary antibody were used. Each sample was incubated with an isotypic antibody dilution under the same experimental conditions as the negative control. Images were acquired using a light microscope (Olympus, Tokyo, Japan) with × 10 and × 20 objectives, and analyzed with image processing software (Olympus).
ELISA
The levels of cytokines or chemokines in serum or supernatants were measured by ELISA (IL-1β, TGF-β1, IL-8 and chemokine (C-C motif) ligand 2 (CCL2) ELISAs were from R&D Systems; IL-37 ELISA was from Cloud Clone Corp®, Houston, TX, USA). The detection limits of the ELISAs were <4.8 pg/ml for IL-1β, <15.4 pg/ml for TGF-β1, <7.5 pg/ml for IL-8, <10 pg/ml for CCL2 and <3.1 pg/ml for IL-37, respectively.
Multi-analyte flow assays
The levels of proinflammatory chemokines in mouse peritoneal lavage fluid were measured by LEGENDplex™ Multi-Analyte Flow Assays (Biolegend) Mouse Proinflammatory Chemokine Panel (13-plex, Cat. No. 740007). Methods were performed as recommended by the manufacturer.
Fluorescence staining and flow cytometry analysis
For fluorescent staining of cell surface markers, mouse peritoneal cells were stained with fluorescent antibodies to the surface markers F4/80, Gr-1, and clone 7/4 (F4/80 and Gr-1 were from Biolegend; clone 7/4 was from AbD Serotec, Kidlington, UK) then washed and resuspended in fluorescence-activated cell sorting (FACS) buffer. Peritoneal cell populations were sorted based on their expression of F4/80, Gr-1, and clone 7/4. Monocytes were Gr-1
inter 7/4
+ F4/80
low, neutrophils were Gr-1
high 7/4
+ F4/80
- and macrophages with high expression of F4/80 (gate R4) were thought to be resident macrophages [
13]. FACS was performed using the Accuri C6 (BD Biosciences, San Jose, CA, USA).
Real-time PCR and qPCR-array
Total RNA was extracted with Trizol (Invitrogen, Carlsbad, CA, USA) according to the manufacturer’s instructions. cDNAs were prepared using the iScript™ cDNA Synthesis kit (Bio-Rad, Hercules, CA, USA). PCR primers (BioTNT, Shanghai, China) used for RT-PCR were as follows: human pro-IL-37: forward 5′-AGTGAGGTCAGCGATTAGGA-3′ and reverse 5′-TTTTAGTGAGCAGGTTTGGT-3′; human β-actin: forward 5′-CCACGAAACTACCTTCAACTCC-3′, and reverse 5′-GTGATCTCCTTCTGCATCCTGT-3′. RNA samples were normalized to control housekeeping genes (human β-actin) and relative mRNA levels of target genes were calculated by the 2-ΔΔ cycle threshold (Ct) method.
For PCR array experiments, an RT2 Profiler Custom PCR array was used to simultaneously examine the mRNA levels of 89 genes, including five housekeeping genes in 96-well plates according to the protocol of the manufacturer (SABiosciences, QIAGEN, Hilden, Germany). Real-time PCR was performed using the RT2 SYBR green qPCR Master Mix (SABiosciences) on an ABI 7500 Fast 96-well real-time PCR machine (Applied Biosystems, Foster City, CA, USA). Results were analyzed using the PCR Array Data Analysis Web Portal (SABiosciences). Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and β-actin were chosen as internal loading controls for standardization between samples and relative mRNA levels of target genes were calculated by the 2-ΔΔ Ct method.
Western blot analysis
Equal amounts of whole joint tissue were lysed in lysis buffer and tissue proteins extracted. Protein levels in different groups were expressed as a ratio to that of the corresponding GAPDH. We used rabbit polyclonal anti-mouse NLRP3 antibody, anti-mouse Smad3, anti-mouse IL-1R8, anti-mouse SOCS3 (all antibodies were from Santa Cruz Biotechnology, Dallas, TX, USA) and rabbit polyclonal anti-mouse GAPDH antibody (Cell Signaling Technology, Danvers, MA, USA) as primary antibody and anti-rabbit IgG HRP-linked antibody (Cell Signaling Technology) as secondary antibody.
Statistical analysis
Experiments were performed at least three times. Data were analyzed with GraphPad Prism 5.01 (GraphPad Software, La Jolla, CA, USA) and are presented as the mean (± S.E.M) or median (range). Repeated measures analysis of variance (ANOVA) followed by the Student Newman-Keuls (S-N-K) test were used for post-hoc analysis of differences between groups. P values <0.05 were considered to indicate statistically significant differences.
Discussion
Acute gout is an inflammatory response to MSU crystals in the joints and periarticular tissue. An interesting feature of acute gout is the self-limiting nature of the inflammatory flare. The inhibition of this inflammatory response is linked to a number of regulatory events ranging from crystal coating and apoptotic cell clearance, through to proinflammatory cytokine regulation and TGF-β1 production. However, current research into the pathways involved in the resolution of inflammation remains limited. IL-37 has emerged as a fundamental inhibitor of the innate immune response by shifting the cytokine equilibrium away from excessive inflammation. IL-37 has been shown to attenuate inflammation in models of septic shock, chemical colitis, cardiac ischemia and contact dermatitis [
17‐
21]. Based on the above findings, we are greatly interested in whether and how IL-37 downregulates inflammation induced by MSU in gouty arthritis.
First, IL-37 was demonstrated to be expressed in synovial tissue and chronic tophus in patients with gouty arthritis. Diseased synovial lining contained small amounts of IL-37, whereas tissue around chronic tophus contained large amounts of IL-37. Thus, we hypothesized that IL-37 might be involved in the limitation of MSU-induced inflammation because in chronic tophus, abundant crystals do not always trigger inflammation. We also found that serum IL-37 was obviously higher in healthy controls (HC) than in patients with non-acute gout (NAG) and patients with acute gout (AG) (HC > NAG > AG). The results suggest that the expression of IL-37 is closely related to the internal inflammatory state. An elevated level of inflammation is associated with lower serum IL-37. High IL-37 in HC and NAG may protect individuals from inflammation. Furthermore, we found that the mRNA level of pro-IL-37 in PBMCs from patients with AG was much higher than that from those with NAG, which suggests that inflammation may promote pro-IL-37 mRNA expression in PBMCs to curb the excess inflammation. Accordingly, we investigated if MSU could directly induce the expression of IL-37 in PBMCs. We stimulated PBMCs with different concentrations of MSU and discovered that both protein and mRNA expression of IL-37 was increased dose dependently. Based on these findings, we thus verified our speculation that upon stimulation by MSU, macrophages produced not only the proinflammatory cytokine IL-1β, but also the anti-inflammatory cytokine IL-37. In future studies, a time-course of IL-37 vs IL-1β production would be informative to determine whether MSU-induced IL-37 is a downstream effect of MSU-induced IL-1β production (or TLR activation).
Second, different gouty arthritis models were used to investigate the inhibitory effect of IL-37 in vitro and in vivo. As IL-37 was identified in the diseased synovial tissue from patients with gouty arthritis, synovial cells containing both MLS and FLS were exposed to MSU in studies in vitro. Our previous study revealed that exposure of FLS to MSU crystals only transiently induced an increase in IL-1β expression, which was apparently not sufficient to initiate the inflammatory cascade as seen in resident macrophages [
22]. Therefore, besides observing the inhibitory effect of rhIL-37 in vitro, we also hypothesized that MLS may play the role of resident macrophages to initiate inflammation in gouty arthritis. Our results showed that rhIL-37 was prominent in suppressing the production of IL-1β, IL-8, and CCL2 in THP-1 macrophages and synovial cells stimulated with MSU, and this anti-inflammatory effect was TGF-β independent.
We also confirmed our previous hypothesis that MLS could play a key role in the initiation of the inflammatory cascade upon MSU stimulation by releasing major proinflammatory cytokines and chemokines in joints to recruit neutrophil and monocyte infiltration. Accumulating evidence indicates that chemokines, which are powerful leukocyte chemoattractants and activators, contribute to acute gout inflammation [
23]. Recent studies have shown that MSU crystals induce FLS to release CCL2, thus, diminishing CCL2 production may limit the inflammatory process and monocyte recruitment in joints [
24]. The recruitment and activation of neutrophils is central to acute gouty inflammation. The CXC family of chemokines plays an important role in neutrophil chemotaxis. Indeed, increased levels of CXCL8 (IL-8), CXCL1 (KC) and CXCL10 (IP-10) have been detected in synovial fluid in patients with gouty arthritis [
25,
26]. In our in vivo studies, rhIL-37 consistently exerted an effective inhibitory role in decreasing neutrophil and monocyte infiltration by dramatically reducing the expression of major proinflammatory cytokines including CXCL1, CXCL10 and MCP-1, but not affecting the level of IL-10 and TGF-β (data not shown). This finding is in line with what has been described in experimental colitis, in which an antibody to the IL-10 receptor did not affect the anti-inflammatory properties of transgenic mice expressing human IL-37 [
27]. In our study, we also found that the effects of rhIL-37 were both preventive and therapeutic. In the arthritis model, reduced foot swelling and attenuated pathological joint inflammation were observed in both the rhIL-37 preventive and therapeutic groups.
Third, in the murine acute gouty arthritis model, qPCR-array and western blot analysis indicated that IL-1R8, Smad3 and SOCS3 were highly expressed, whereas NLRP3 was suppressed in the rhIL-37 intervention groups. These findings suggest that rhIL-37 can suppress MSU-induced inflammation by inhibiting NLRP3 and enhancing expression of IL-1R8 and SOCS3 for anti-inflammatory signal transduction. Similar results were shown in a murine model of invasive pulmonary aspergillosis [
28]. In that study, rhIL-37 markedly reduced NLRP3-dependent neutrophil recruitment and steady-state mRNA levels of IL-1β, and mitigated lung inflammation and damage. Besides NLRP3 inhibition, in our study rhIL-37 also enhanced expression of IL-1R8, Smad3 and SOCS3.
The anti-inflammatory activity of IL-37 requires IL-1R8 (TIR-8/SIGIRR). Studies by Nold-Petry et al. [
4] demonstrate that IL-37 requires the receptors IL-18Rα and IL-1R8 to suppress innate immunity in vitro and in vivo (using the IL-1R8-knockout (KO) mice). In future studies, IL-1R8 silencing and IL-1R8-KO mice studies will be necessary to confirm the contribution of IL-1R8 in rhIL-37 anti-inflammatory properties.
In our study, the expression of Smad3 was also significantly enhanced after rhIL-37 intervention, whereas TGF-β1 was unaffected. This result suggests rhIL-37 may also have an intracellular anti-inflammatory function through interaction with Smad3. Similar results were shown in Marcel’s study [
2]. In that study, IL-37 interacted intracellularly with Smad3 and co-localized with phospho-Smad3 to form a functional complex. Furthermore, IL-37-expressing cells and transgenic mice had less cytokine suppression when endogenous Smad3 was depleted. Smad3 inhibition studies are also required in our future research to verify the contribution of Smad3 in rhIL-37 intracellular anti-inflammatory properties.
Chen et al. have shown that mononuclear cells and synovial tissue isolated from the synovium of patients with gout have significantly upregulated expression of the SOCS family proteins cytokine-inducible SH2 protein (CIS) and SOCS3 compared with patients with osteoarthritis. Increased expression of CIS and SOCS3 is observed in MSU-crystal-stimulated human monocyte-derived macrophages, indicating that macrophage activation switches on these regulatory pathways [
6]. Our data also support a role for rhIL-37 increased intracellular SOCS3 expression in the resolution of acute gout through the ability to negatively regulate proinflammatory cytokines and to switch on anti-inflammatory cytokine production.
The mRNA levels of Mertk were significantly upregulated in the IL-37 intervention groups. In a previous study by Claudia and colleagues [
4], LPS-stimulated THP-1 cells were transfected to express IL-37b, and after inhibition of Mertk the IL-37-mediated anti-inflammation effect was reduced by 81%. In our study, we further demonstrated that Mertk signaling participates in the rhIL-37 inhibitory pathway in gouty models. By inhibition of Mertk, the anti-inflammatory effect of rhIL-37 was partly abrogated, and IL-1R8, Smad3 and SOCS3 were suppressed, whereas NLRP3 expression was reactivated. Previous studies show that Mertk plays a role as an intrinsic feedback inhibitor of the TLR4-driven and inflammatory-mediator-driven immune responses [
28‐
30]. Mertk
-/- mice have macrophages deficient in the clearance of apoptotic thymocytes [
31] and are found to be characterized with polyclonal lymphocyte proliferation with autoimmune manifestations [
32‐
34]. In a mouse model of LPS-induced acute lung injury, anti-Mertk antibody enhanced LPS-induced inflammatory responses by significantly reducing expression of the TLR suppressors SOCS1 and SOCS3. MSU crystals require TLR-2, TLR-4, and MyD88 for macrophage activation [
35], and both TLR4- and P2X
7-dependent (ATP receptor) pathways are required for NLRP3 inflammasome activation [
17,
36].
Based on these results and our findings, we hypothesize that Mertk participates in limiting MSU-induced inflammation not only by enhancing macrophage phagocytosis and clearance of MSU crystals and apoptosis of inflammatory cells, but also by inducing signaling in the downregulation of TLR4-activation-driven immune responses by suppressing NLRP3 activation. In this study, the direct link between IL-37 and Mertk, and whether MSU crystals could directly induce Mertk were not demonstrated. However, further study in this area is of great interest.
Conclusion
In conclusion, our studies strongly indicate that rhIL-37 plays a potent immunosuppressive role in the pathogenesis of both experimental gout models in vitro and in vivo by downregulating proinflammatory cytokines and chemokines, markedly reducing neutrophil and monocyte recruitment, and mitigating pathological joint inflammation. In our studies, rhIL-37 suppressed MSU-induced innate immune responses by enhancing expression of Smad3 and IL-1R8 to trigger multiple intracellular switches to block inflammation, including inhibition of NLRP3 and activation of SOCS3. Mertk signaling participates in the rhIL-37 inhibitory pathway in gouty models. By inhibition of Mertk, the anti-inflammatory effect of rhIL-37 was partly abrogated, and IL-1R8, Smad3 and SOCS3 were suppressed, whereas NLRP3 expression was reactivated. Thus, our studies reveal that rhIL-37 limits runaway inflammation initiated by MSU-crystal-induced immune responses, partly in a Mertk-dependent way. Thus, rhIL-37 has both preventive and therapeutic effects in gouty arthritis.