CAPE was purchased from Shanghai Aladdin Biochemical Technology Co., Ltd. IL-1β was purchased from ProteinTech Group, Inc. The Cell Counting Kit-8 (CCK-8) was purchased from Beyotime Institute of Biotechnology. Griess Reagent Nitrite Measurement kit (cat. no. 13547) was purchased from Cell Signaling Technology, Inc. The ELISA kits for human PGE2 (cat. no. SEKH-0414), Toluidine Blue solution and bovine serum albumin (BSA) were purchased from Beijing Solarbio Science & Technology Co., Ltd. Penicillin/streptomycin, fetal bovine serum (FBS) and DMEM were purchased from Gibco (Thermo Fisher Scientific, Inc.).

Human chondrocytes were isolated from human articular cartilage tissues that were procured from patients with femoral neck fracture. The collection of cartilage tissues from patients was approved by the Ethics Committee of Shenzhen Second People's Hospital (Shenzhen, China). Patients with an average age of 64.8 years (aged 60-68 years, two males and three females) who were subjected to total knee replacement surgery at the Shenzhen Second People's Hospital from January to March, 2021 participated in the study. All patients provided written informed consent. The articular cartilage tissues were washed with PBS and cut into 1 mm³ pieces. The sections were then cultured with collagenase II (2 g/l) for 4 h at 37°C (31). Upon centrifugation at 108 × g for 5 min at 24°C, the cells were cultured in DMEM with 10% (v/v) FBS and 1% (v/v) antibiotics (penicillin/streptomycin) in an atmosphere containing 5% CO₂ at 37°C. The culture medium was changed every other day. Only cells from the first three passages were used in the present study. Chondrocyte morphology was examined using toluidine blue staining. In brief, the culture medium was aspirated and washed twice with PBS. Toluidine blue solution for 5 min at room temperature, and the same amount of distilled water was added and mixed evenly. Images were acquired using an Olympus microscope (Olympus Corporation) after standing for 15 min at room temperature.

Sprague-Dawley male wild-type rats (n=12; 8 weeks old; weighing 300-350 g) were acquired from Cloud-Clone Corp. The rats were maintained in a clean environment at 27°C under a 12-h light/dark cycle with 50% humidity, and had free access to adequate food and water. The animal protocols and the experimental procedures were in agreement with the Animal Care and Use Committee of Southwest Medical University (approval no. 20211124-043). The model of OA was established by the destabilization of the medial meniscus (DMM) through surgical treatment as previously described (32). Briefly, the rats were anesthetized with 2% (w/v) pentobarbital (40 mg/kg) via intraperitoneal injection. The capsule of the right knee joint was opened though the medial patellar tendon and the medial meniscus tibial ligament was cut using microsurgical scissors. The medial meniscus tibial ligament was not cut in the sham-operated control group. In the present study, the rats were randomly divided into three groups as follows: The sham-operated control group (sham), the OA group (DMM) and the CAPE-treated OA group (DMM + CAPE). Rats in the CAPE treatment group were administered 10 mg/kg/2 days CAPE, for 8 weeks. At the end of the experiment, all animals were sacrificed by cervical dislocation under anesthesia through an intraperitoneal injection of pentobarbital sodium (50 mg/kg), and respiratory arrest was used to confirm animal death. During the course of the experiment, any rats that were unable to eat or drink, had difficulty breathing and had lost 20% of their body weight before the experiment, were regarded as having reached the humane endpoint and were thus immediately euthanized. None of the rats reached the aforementioned end points in this experiment and thus none were euthanized before the end of the experiment.

Negative control (NC) siRNA and NRF2 siRNA were purchased from Shanghai GenePharma Co., Ltd. Chondrocytes were plated and cultured in six-well plates for 24 h, and then transfected with 80 nM NC and NRF2 siRNA for 48 h using Lipofectamine^® 2000 siRNA transfection reagent (Thermo Fisher Scientific, Inc.). The sequences of the NRF2 and NC siRNAs were as follows: 1#NRF2 siRNA: sense, 5′-GGG AGG AGC UAU UAU CCA UTT-3′ and antisense, 5′-AUG GAU AAU AGC UCC UCC CTT-3′; and 2#NRF2 siRNA sense, 5′-GCC CAU UGA UGU UUC UGA UTT-3′ and antisense, 5′-AUC AGA AAC AUC AAU GGG CTT-3′; and 3#NRF2 siRNA sense, 5′-GCC UGU AAG UCC UGG UCA UTT-3′ and antisense, 5′-AUG ACC AGG ACU UAC AGG CTT-3′; and NC siRNA sense, 5′-UUC UCC GAA CGU GUC ACG UTT-3′ and antisense, 5′-ACG UGA CAC GUU CGG AGA ATT-3′; NC FAM-siRNA sense, 5′-UUC UCC GAA CGU GUC AC GUT T-3′ and antisense, 5′-ACG UGA CAC GUU CGG AGA ATT-3′.

The cytotoxicity of CAPE on human chondrocytes was evaluated using CCK-8 assay. In brief, chondrocytes were plated into 96-well plates in serum-free medium for 24 h, and then treated with various concentrations of CAPE (0, 1, 3, 5, 10, 20 and 40 µM) for 24 h. The chondrocytes were then washed with PBS, and 100 µl DMEM containing 10 µl CCK-8 solution was added to each well, followed by incubation at 37°C for 3 h. The optical density value of the wells was measured at a wavelength of 450 nm using a microplate reader (Thermo Fisher Scientific, Inc.).

Chondrocytes were plated and cultured in 6-well plates, and pre-treated with CAPE (0, 10 or 20 µM). After 24 h, IL-1β (10 ng/ml) was added, followed by additional 24 h of incubation at 37°C. The content of NO and PGE2 in each well was detected using the Griess reaction and ELISA kits, respectively, according to the manufacturer's protocols.

Total RNA was extracted from the chondrocytes using TRIzol^® reagent (Takara Bio, Inc.), and 1 µg total RNA was used to synthesize cDNA using the PrimeScript™ RT reagent kit with gDNA Eraser (Takara Bio, Inc.), and the conditions were as follow: 15 min at 37°C, followed by 5 sec at 85°C. The total volume of q-PCR was 10 µl, including 5 µl 2X SYBR Master Mix (Beyotime Institute of Biotechnology), 0.25 µl each primer and 4.5 µl diluted cDNA. qPCR was conducted in a CFX96Real-Time PCR System, and the thermocycling conditions were as follows: 10 min at 95°C, followed by 40 cycles of 15 sec at 95°C and 1 min at 60°C. GAPDH was used as the internal control for normalization. The relative mRNA of the target genes was calculated using the 2^−ΔΔCq method (36). The primer sequences of the target genes are presented in Table I.

The cells were lysed by radio immunoprecipitation assay (RIPA) buffer (Thermo Fisher Scientific, Inc.) containing 1 mM PMSF to extract total protein. The protein concentration was detected with a BCA protein assay kit (Beyotime Institute of Biotechnology). Subsequently, 40 µg denatured protein solution were separated by 12% SDS-PAGE (Wuhan Servicebio Technology Co., Ltd.) and transferred to a PVDF membrane (Merck KGaA), which was incubated in methanol for 1 min at room temperature. The methanol was then removed and the membrane was equilibrated in transfer buffer until ready to use. Upon transfer at 100 V for 1 h at 4°C, the membrane was blocked with 5% skimmed milk for 1 h at room temperature and then incubated with primary antibodies against GADPH (1:1,000; cat. no. AP0066; Bioworld Technology, Inc.), MMP3 (1:5,000; cat. no. 66338-1-Ig; ProteinTech Group, Inc.), MMP13 (1:1,000; cat. no. 18165-1-AP; ProteinTech Group, Inc.), a disintegrin and metalloproteinase with thrombospondin motif-5 (Adamts5; 1:500; cat. no. A2836; ABclonal Biotech Co., Ltd.), iNOS (1:500; cat. no. 18985-1-AP; ProteinTech Group, Inc.), cyclooxygenase-2 (COX-2; 1:500; cat. no. 12375-1-AP; ProteinTech Group, Inc.), lamin B1 (1:1,000; cat. no. AF1408; Beyotime Institute of Biotechnology), NRF2 (1:2,000; cat. No. 16396-1-AP; ProteinTech Group, Inc.), HO-1 (1:1,000; cat. no. 10701-1-AP; ProteinTech Group, Inc.), p65 (1:1,000; cat. no. 8242; Cell Signaling Technology Inc.), phosphorylated (p)-p65 (1:1,000; cat. no. 3033; Cell Signaling Technology Inc.), IκBα (1:1,000, cat. no. 4814; Cell Signaling Technology Inc.), p-IκBα (1:1,000, cat. no. 2859; Cell Signaling Technology Inc.) and collagen II (1:500; cat. no. PA5-99159, Thermo Fisher Scientific, Inc.) overnight at 4°C. Subsequently, the membranes were incubated with a HRP-conjugated goat anti-rabbit (1:1,000; cat. no. A0208; Beyotime Institute of Biotechnology Inc.) or goat anti-mouse IgG (1:1,000; cat. no. A0216; Beyotime Institute of Biotechnology Inc.) secondary antibody for 2 h at room temperature. Finally, an ECL reagent (cat. no. 34580; ThermoFisher Scientific, Inc.) was used to detect the blots. The ECL signal was captured using Odyssey FC Imager (Gene Company, Ltd.), and GAPDH and Lamin B1 were used as loading controls for normalization. Quantitative analysis was performed using ImageJ 1.53e software (National Institutes of Health).

Chondrocytes were seeded in a glass plate, cultured for 12 h, pre-treated with or without CAPE (20 µM) for 24 h, and then co-incubated with or without IL-1β (10 ng/ml) for 24 h. Subsequently, the cells were washed with PBS and fixed with 4% paraformaldehyde for 15 min. The cells were then treated with 0.1% TritonX-100 for 5 min and blocked with 5% BSA for 1 h at room temperature. The cells were then incubated with primary antibodies against collagen II (1:100; cat. no. PA5-99159, Thermo Fisher Scientific, Inc.), MMP3 (1:100; cat. no. 66338-1-Ig; ProteinTech Group, Inc.), p65 (1:400; cat. no. 8242; Cell Signaling Technology Inc.) and NRF2 (1:500; cat. no. 16396-1-AP; ProteinTech Group, Inc.) overnight at 4°C. The following day, the cells were incubated with Alexa Fluor^® 647-conjugated goat anti-rabbit IgG (1:500; cat. no. A0468; Beyotime Institute of Biotechnology) and Alexa Fluor^® 647-conjugated goat anti-mouse IgG secondary antibodies (1:500; cat. no. A0473; Beyotime Institute of Biotechnology) for 1 h at room temperature in the dark and exposed to DAPI (Beyotime Institute of Biotechnology) for 5 min at room temperature. Finally, the cells were observed under a confocal microscope (ZEISS GmbH) and analyzed using ImageJ 1.53e software.

The structure data file (SDF) of CAPE (Pubchem ID: 5281787) was downloaded from the PubChem website (https://pubchem.ncbi.nlm.nih.gov/) and converted to PDB format on OpenBabel 3.1.1. The structure of Keap1-NRF2 complex was downloaded from the RCSB Protein Data Bank (https://www.rcsb.org/). AutoDockTools1.5.7 software was used to modify the receptor protein, such as water removal and hydrogenation, and also to modify ligand small molecule, such as hydrogenation. Next, the molecular docking analysis of receptor protein and ligand small molecule was performed using AutoDockTools. Eventually, ligand binding flexibility with the binding pocket residues were drawn using PYMOL 2.5.2.

The knee joint tissue was fixed with 4% paraformaldehyde for 24 h at 4°C and then decalcified with 10% EDTA solution for 2 weeks. The tissue was then dehydrated, cleared, embedded in paraffin blocks and sliced to obtain frontal serial sections at a thickness of 5 µm. The slides were then stained with Safranin O/Fast Green (S/O) (cat. no. G1053; Beijing Solarbio Science & Technology Co., Ltd.). In brief, the slides were strained with Fast Green for 2 min, washed with water, and soaked in 1% hydrochloric acid and alcohol for 10 sec at room temperature. Then strained with Safranin O for 5 sec, rapid dehydrated in absolute ethanol for 5 sec, 2 sec and 10 sec, and sealed with neutral resin (Sinopharm Group Chemical Reagent Co., Ltd.) at room temperature. The extent of cartilage degeneration was assessed using a Nikon E100 microscope (Nikon Corporation) and evaluated using the Osteoarthritis Research Society International (OARSI) scoring system as described previously (37).

Immunohistochemical assay was performed as previously described (38). Briefly, the slides were deparaffinized and rehydrated. For antigen repair, the slides were incubated with 0.4% pepsin (Sangon Biotech Co., Ltd.) in 5 mM HCl at 37°C for 20 min, and then blocked with 5% BSA for 30 min. The slides were then incubated with primary antibodies against collagen Ⅱ (1:50; cat. no. PA5-99159, Thermo Fisher Scientific, Inc.), MMP3 (1:500; cat. no. 66338-1-Ig; ProteinTech Group, Inc.), MMP13 (1:500; cat. no. 18165-1-AP; ProteinTech Group, Inc.) and NRF2 (1:500; cat. no. 16396-1-AP; ProteinTech Group, Inc.) overnight at 4°C. Finally, the slides were incubated with HRP-conjugated goat anti-rabbit (1:50; cat. no. A0208; Beyotime Institute of Biotechnology, Inc.) or goat anti-mouse IgG (1:50; cat. no. A0216; Beyotime Institute of Biotechnology, Inc.) secondary antibody for 50 min at room temperature, and images were captured using an Olympus BX51 microscope (Olympus Corporation).

Data are expressed as the mean ± SD. All experiments were repeated at least three times. Statistical analyses were performed using GraphPad Prism version 8.0 software (GraphPad Software, Inc.). Comparisons between two groups were performed using an unpaired two-tailed Student's t-test. Comparisons among multiple groups were done using one-way ANOVA test followed by a post-hoc Test (Bonferroni). A value of P<0.05 was considered to indicate a statistically significant difference.

The molecular chemical structure of CAPE is illustrated in Fig. 1A, and the morphology of the human chondrocytes are illustrated in Fig. 1B and C, respectively. To measure the cytotoxic effect of CAPE on human chondrocytes, the chondrocytes were treated with various concentrations of CAPE (0, 1, 3, 5, 10, 20 and 40 µmol/l) for 24 h. CAPE cytotoxicity was detected using CCK-8 assay. The results revealed that there was no obvious cytotoxic effect of CAPE on human chondrocytes when the cells were incubated with 1, 3, 5, 10 or 20 µM CAPE (Fig. 1D). However, the viability of the chondrocytes was significantly inhibited following treatment with 40 µM CAPE (Fig. 1D). Therefore, CAPE was used at 10 and 20 µM in the subsequent experiments.

To examine the effects of CAPE on the IL-1β-induced inflammation of chondrocytes, the expression and production levels of COX-2, iNOS, NO and PGE2 were measured using RT-qPCR, western blot analysis and ELISA. The results revealed that CAPE at the concentrations of 10 and 20 µM inhibited the expression of COX-2 and iNOS stimulated by IL-1β at the protein and mRNA level (Fig. 2A-C). In addition, the results of Griess reaction and ELISA revealed that CAPE at concentrations of 10 and 20 µM suppressed the production of NO and PGE2 stimulated by IL-1β (Fig. 2D and E). Therefore, these results indicated that CAPE inhibited the expression and production of IL-1β-induced inflammatory mediators in human chondrocytes, particularly at the concentrations of 10 and 20 µM.

To determine the effects of CAPE on IL-1β-induced ECM synthesis and degradation in chondrocytes, the effects of CAPE on the expression of collagen II, aggrecan, MMP3, MMP13 and Adamts5 were examined using RT-qPCR, western blot analysis and immunofluorescence. The results revealed that the mRNA expression levels of collagen II and aggrecan were increased by CAPE at 10 and 20 µM under IL-1β stimulation, while the mRNA expression levels of MMP3, MMP13 and Adamts5 were inhibited (Fig. 3A). In addition, the protein level of collagen II was increased by CAPE at 10 and 20 µM following IL-1β stimulation, while the protein levels of MMP3, MMP13 and Adamts5 were inhibited (Fig. 3B). The immunofluorescence staining of collagen II and MMP3 revealed that CAPE activated collagen II expression and inhibited MMP3 expression following IL-1β stimulation (Fig. 3C and D). Therefore, these data indicated that CAPE attenuated the IL-1β-induced ECM degradation in human chondrocytes by preventing the degradation of collagen II and the production of ECM degradative enzymes.

To explore the anti-inflammatory mechanisms of CAPE in IL-1β-stimulated chondrocytes, the expression of p65, p-p65, IκBα and p-IκBα was detected using western blot analysis and immunofluorescence. The results revealed that the phosphorylation of p65 was significantly increased by IL-1β stimulation, while it was significantly inhibited by pre-treatment with CAPE (Fig. 4A and B). Additionally, pre-treatment with CAPE inhibited the protein level of IkBα and the phosphorylation level of IkBα in IL-1β-stimulated chondrocytes (Fig. 4A and B). The immunofluorescence staining of p65 revealed that pre-treatment with CAPE decreased the expression of p65 in the nucleus of IL-1β-stimulated chondrocytes (Fig. 4C). Therefore, these data suggested that CAPE prevented the IL-1β-induced NF-κB activation by inhibiting the translocation of p65 and the degradation of IκBα in human chondrocytes.

To investigate the role of the NRF2/HO-1 signaling pathway in the anti-inflammatory effects of CAPE, the expression of NRF2 and HO-1 in IL-1β-stimulated human chondrocytes was detected using western blot analysis and immunofluorescence. The results revealed that CAPE increased the expression of NRF2 in a concentration-dependent manner (Fig. S1). Additionally, the results revealed that the protein levels of NRF2 and HO-1 were increased by 10 and 20 µM CAPE under IL-1β stimulation (Fig. 5A and B). The immunofluorescence staining of NRF2 revealed that pre-treatment with CAPE increased the expression of NRF2 in the nuclei of IL-1β-stimulated chondrocytes (Fig. 5C). Therefore, these data suggested that CAPE exerted anti-inflammatory effects in IL-1β-stimulated chondrocytes through the activation of the NRF2/HO-1signaling pathway.

To further confirm that the anti-inflammatory effects of CAPE are mediated via the NRF2/HO-1 signaling pathway in IL-1β-stimulated chondrocytes, NRF2 siRNA was transfected into chondrocytes to silence the expression of NRF2 (Fig. S2). The results revealed that the silencing of NRF2 inhibited the protein levels of NRF2 and HO-1 which had been increased by pre-treatment with CAPE in the IL-1β-stimulated chondrocytes, which suggested that the CAPE-induced activation of the NRF2/HO-1 signaling activation was inhibited by the silencing of NRF2 (Fig. 6A and B). The silencing of NRF2 increased the phosphorylation levels of p65 in the nuclei of IL-1β-stimulated chondrocytes which had been decreased by pre-treatment with CAPE; this suggested that the CAPE-mediated suppression of NF-κB signaling was abolished by the silencing of NRF2 (Fig. 6A and B). Furthermore, downregulation of NRF2 could inhibit the protein levels of iNOS and COX-2 by pre-treatment with CAPE in IL-1β-induced chondrocytes, which suggested that the CAPE-mediated suppression of inflammation was abolished by downregulation of NRF2 (Fig 6A and B). In addition, the silencing of NRF2 in IL-1β-stimulated chondrocytes increased the protein levels of MMP3, MMP13 and Adamts5, whereas it decreased the protein levels of collagen II upon pre-treatment with CAPE (Fig. 6C and D). Therefore, these data indicated that CAPE regulated NF-κB signaling and the inflammatory response though the NRF2/HO-1 signaling pathway in IL-1β-stimulated chondrocytes.

In order to evaluate whether there is any affinity between CAPE and Keap1-NRF2 complex, computational molecular docking analysis was performed. The structures of CAPE and the Keap1-NRF2 complex (PDB ID: 2FLU) were obtained and analyzed (Fig. 7A and B). It was found that CAPE interacted with and docked at the Keap1-NRF2 complex binding site. High-affinity (-7.39 kcal/mol) hydrogen binding events were observed between the residues of Arg415, Val465 and Val512 in CAPE and Keap1-NRF2 complex (Fig. 7C). Therefore, these results indicated that CAPE probably inhibited the development of OA by interacting with the Keap1-NRF2 complex, inhibiting ubiquitination and promoting nuclear translocation of NRF2.

To examine the effects of CAPE on OA progression in vivo, a model of OA was established using rats, followed by an intra-peritoneal injection of 10 mg/kg CAPE. S/O staining revealed that the articular cartilage exhibited a normal, red-dyed area and a smooth surface in the sham control group, whereas the thickness of the articular cartilage was significantly reduced in the DMM group (Fig. 8A). Compared with that in the DMM group, the red-dyed area was thicker and the surface of articular cartilage was smoother in the CAPE-treated group (Fig. 8A), which suggested that CAPE played a role in attenuating the degradation of cartilage matrix. The immunohistochemistry of MMP3, MMP13, collagen Ⅱ and NRF2 was also performed in the OA model. In the DMM group, the expression of MMP3 and MMP13 was markedly increased compared with that in the sham group, while the DMM + CAPE group exhibited a decreased expression of MMP3 and MMP13 (Fig. 8B). In the DMM group, the expression of collagen Ⅱ was markedly decreased compared with that in the sham group, while the DMM + CAPE group exhibited a high expression (Fig. 8B). In the DMM group, the expression of NRF2 was not markedly different from that in the sham group, while the DMM + CAPE group showed increased expression in the cell nuclei (Fig. 8B).