Abstract
Osteoarthritis (OA) is a full-joint, multifactorial, degenerative and inflammatory disease that seriously affects the quality of life of patients due to its disabling and pain-causing properties. ER stress has been reported to be closely related to the progression of OA. The inositol-requiring enzyme 1α/X-box-binding protein-1 spliced (IRE1α/XBP1s) pathway, which is highly expressed in the chondrocytes of OA patients, promotes the degradation and refolding of abnormal proteins during ER stress and maintains the stability of the ER environment of chondrocytes, but its function and the underlying mechanisms of how it contributes to the progression of OA remain unclear. This study investigates the role of IRE1α/ERN1 in OA. Specific deficiency of ERN1 in chondrocytes spontaneously resulted in OA-like cartilage destruction and accelerated OA progression in a surgically induced arthritis model. Local delivery of AdERN1 relieved degradation of the cartilage matrix and prevented OA development in an ACLT-mediated model. Mechanistically, progranulin (PGRN), an intracellular chaperone, binds to IRE1α, promoting its phosphorylation and splicing of XBP1u to generate XBP1s. XBP1s protects articular cartilage through TNF-α/ERK1/2 signaling and further maintains collagen homeostasis by regulating type II collagen expression. The chondroprotective effect of IRE1α/ERN1 is dependent on PGRN and XBP1s splicing. ERN1 deficiency accelerated cartilage degeneration in OA by reducing PGRN expression and XBP1s splicing, subsequently decreasing collagen II expression and triggering collagen structural abnormalities and an imbalance in collagen homeostasis. This study provides new insights into OA pathogenesis and the UPR and suggests that IRE1α/ERN1 may serve as a potential target for the treatment of joint degenerative diseases, including OA.
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Introduction
Osteoarthritis refers to a group of chronic degenerative bone diseases involving various tissues, including articular cartilage, subchondral bone, and synovial tissue around the joint1,2,3. Under normal physiological conditions, the degradation and synthesis of cartilage components maintain a dynamic balance. Any damage and degeneration of articular cartilage causes an imbalance in cartilage metabolism, leading to progressive tissue loss and dysfunction4,5. The cartilage extracellular matrix (ECM) is mainly composed of collagen fibers, proteoglycans and glycosaminoglycans. The accumulation of misfolded and unfolded ECM proteins, such as collagen types II, IX, X and XI and aggrecan, can influence growth plate development and cause cartilage-related diseases, including chondrodysplasia6. The synthesis of these ECM mutant proteins can trigger endoplasmic reticulum (ER) stress to induce an unfolded protein response (UPR), which leads to the activation of canonical ER stress sensors, including inositol-requiring enzyme-1α (IRE1α), PERK, and ATF67. The assembly and folding of secreted proteins in the ER are complex and exquisitely regulated processes that maintain ER homeostasis. Stable ER stress and UPR signals and effects are essential for normal chondrogenic differentiation and hypertrophic maturation8.
Human IRE1α, encoded by the endoplasmic reticulum to nucleus signaling 1 (ERN1) gene, is equipped with a serine/threonine protein kinase domain and a ribonuclease domain and participates in regulating the folding of proteins and maintaining ER homeostasis9. IRE1α is closely associated with cartilage or bone growth and development. Tohmonda et al. reported that specific inactivation of IRE1α in hematopoietic stem cells leads to increased bone mass and decreased osteoclast number in vivo10. Cameron et al. analyzed the role of the IRE1α/XBP1 pathway in the pathology of Schmid-type metaphyseal achondroplasia (MCDS) and proposed that the pathology of MCDS is supported by XBP1-independent UPR-induced dysregulation of C/EBP-β-mediated chondrocyte differentiation11. Tohmonda et al. proposed that the IRE1α-XBP1 signaling pathway is involved in osteoblast differentiation by facilitating the transcription of osterix12. Furthermore, myofiber-specific defects in IRE1α weakened skeletal muscle regeneration in adult mice13 and activated ER stress, and the UPR signaling pathway component IRE1α in the body’s immune cells can increase the release of inflammatory cytokines and further promote the production of inflammation14. We previously reported that IRE1α enhances chondrocyte viability and inhibits cell apoptosis in chondrocytes, whereas IRE1α deficiency increases the apoptosis of chondrocytes by upregulating the proapoptotic factors caspase 3, pJNK1, and CHOP15. We also designed and constructed a novel siERN1-nanoprodrug with universal biocompatibility, long-term drug release responsiveness, superior targeting properties, and strong anti-inflammatory therapeutic effects in mouse collagen-induced arthritis and inflammatory bowel disease models16. Although some studies have reported the potential efficacy of IRE1α regulation in skeletal development and related diseases, as Huang noted, IRE1α plays an important role in chondrocytes, and the understanding of IRE1α responses and cell death fate remains controversial17. Given the uncertainties in the regulation of cartilage function by IRE1α and the remarkable complexity and heterogeneity exhibited by osteoarthritis, it is important to elaborate on the mechanism of ERN1/IRE1α in the occurrence and development of osteoarthritis.
In the current study, we not only elucidated the role of ERN1/IRE1α in OA but also revealed the mechanism by which ERN1 deficiency leads to the structural abnormality of collagen through PGRN and XBP1 splicing and proposed a possible functional compensatory mechanism in the absence of ERN1. This study provides a new strategy for the precise treatment of clinical OA.
Materials and methods
Human subjects
All biomedical studies involving humans in this study were reviewed and approved by the Ethics Committee of Chongqing Medical University, and full written consent was obtained before the operative procedure. In this study, 12 clinical samples were collected and used for Western blotting and RT‒qPCR: 3 normal and 9 osteoarthritic cartilage tissues. All samples were stored in liquid nitrogen for a long time.
Mice
All animal studies were performed in accordance with institutional guidelines and approval by the Ethics Committee of Chongqing Medical University. ERN1flox/+ mice were purchased from Shanghai Biomodel Organism Science & Technology Development Co., Ltd (Shanghai, China). Col2a1-Cre mice on a C57BL6/J background were gifted by Dr. Lin Chen (Army Medical University, Chongqing, China). ERN1flox/flox, Col2a1-Cre mice (ERN1cKO) and ERN1flox/flox mice (Cre-negative control mice) were obtained in accordance with previously described methods1,2. GRN−/− mice were purchased from the Jackson Laboratory.
Cell culture
The human chondrocyte cell line C28/I2 was kindly provided by Professor Liu Chuanju (New York University, USA). RAW 264.7 cells were purchased from the Cell Bank of the Chinese Academy of Sciences (Shanghai, China). All cells were routinely assessed every 2 months for mycoplasma contamination using the EZ-PCR mycoplasma test kit (Biological Industries, Israel) according to the manufacturer’s protocol. C28/I2 cells, HEK 293 cells and 293T cells were maintained in Dulbecco’s modified Eagle’s medium (DMEM) with 100 units/ml streptomycin and penicillin and 10% fetal bovine serum (FBS). RAW 264.7 cells were cultured in Dulbecco’s modified Eagle’s medium alpha (α-MEM) containing 10% FBS and 100 units/ml streptomycin and penicillin. All cells were cultured at 37 °C in a humidified incubator with 5% CO2.
Primary mouse chondrocytes
Immature murine articular chondrocytes were isolated by enzymatic digestion of articular cartilage from the knee joints of 6-day-old newborn ERN1 control and cKO mice. Briefly, after sacrificing the mice, we dislocated the femoral heads, femoral condyles and tibial plateau. The cartilage samples from one mouse were isolated under a microscope and then rinsed in PBS buffer. The cartilage samples were kept in a digestion buffer containing 0.25% collagenase II in DMEM for 12–16 h. After digestion, the cells were seeded in a 60 mm dish and allowed to grow in DMEM/F12 with 10% FBS and 100 units/ml streptomycin and penicillin for 3 days. Then, the medium was replaced with fresh medium.
ACLT OA induction and intra-articular injection
OA was surgically induced in 10- to 12-week-old males by unilateral (right) anterior cruciate ligament transection (ACLT) surgery3,4. The ACL was transected to establish the ACLT model. The mice were sacrificed at the designated time points, and the knee joints were collected for analysis. The designated expression products were intra-articularly injected into the knee joints 4 weeks after surgery for 4 weeks. In the single treatment group, adenovirus expressing ERN1 (AdERN1), XBP1s (AdXBP1s) or control (AdGFP) was injected 1 time/week 4 times at 1 × 109 PFU/time (<15 µl/joint). The combined treatment group, the AdERN1+siPGRN group, was injected with AdERN1 two weeks after the surgery and then with PGRN siRNA (2.5 nm/10 μl/time, 1 time/week) 4 days later. The AdXBP1s+rhPGRN group was injected with AdXBP1s two weeks after the surgery and then with recombinant PGRN protein (4 μg/time, 1 time/week) 4 days later. The PGRN knockout (GRN−/−) mice were divided into three groups. The control group (AdGFP) was injected 1 time/week 4 times and 1 × 109 PFU/time (<15 μl/joint). The AdERN1 group was injected 1 time/week 4 times and 1 × 109 PFU/time (<15 μl/joint). The AdERN1+rhPGRN group was injected with AdERN1 1 time/week 4 times after surgery and then with recombinant PGRN protein (4 μg/time, 1 time/week) simultaneously.
CRISPR-Cas9 technique
The oligonucleotide sequences used for the generation of single guide RNAs (sgRNAs) are listed in Supplementary Table 1. The ERN1-KO and PGRN-KO cell lines were generated via the CRISPR‒Cas9 system. ERN1-KO and PGRN-KO monoclonal cell lines (KO1 and KO2) were generated using single-guide RNAs (Supplementary Table 1). Single-guide RNAs targeting human ERN1 and PGRN were designed using E-CRISP (www.e-crisp.org/E-CRISP/designcrispr.html). Pairs of forward and reverse oligonucleotides for sgRNAs were annealed and then inserted into the plasmid vector LentiCRISPR v2, and 293T cells were transfected with sgRNA vector and two packaging plasmids (psPAX2 and pVSVG) using 100 mM PEI, pH 7.0 (Sigma #408727) diluted in ddH2O (pVSVG:psPAX2:lentiCRISPR=1:2:3). Supernatants were collected at 48 h post-transfection and passed through a 0.45 μm filter. Subsequently, the lentivirus supernatants were transduced into C28/I2 cells with 5 μg/ml polybrene. Forty-eight hours later, the cells were transferred and selected by 0.5 μg/ml puromycin for 3 days. Puromycin-resistant clones were sorted and confirmed by western blotting.
Reverse transcription-PCR (RT‒PCR)
RT‒PCR and real-time PCR analyses were performed as previously described16. The relative mRNA expression was quantified using the comparative cycle threshold (CT) method, as previously described16. The full list of primers is listed in Supplementary Table 2.
Immunofluorescence (IF) and immunohistochemistry (IHC)
IF and IHC analyses were performed to detect the expression of IRE1α, phosphorylated IRE1α, Col2, Aggrecan, MMP13, PGRN, XBP1s, and p-ERK1/2 in chondrocytes and cartilage as previously described16. The full list of primary antibodies is listed in Supplementary Table 3.
Mass spectrometry analysis
C28/I2 cells were seeded in 10 cm dishes. When the cell density reached 90%, the medium was changed to serum-free medium, and the eukaryotic expression plasmid pcDNA3.1(−)-Myc-IRE1α was transfected into C28/I2 cells using Lipo2000. The serum-free medium was replaced with fresh DMEM containing 10% FBS after coincubation for 6–8 h. Then, after the culture was continued for 48 h, the original medium was removed, and the cells were washed three times with precooled PBS. Then, 400.0 μl of IP buffer was added, and the cells were lysed for 30 min on ice and shaken every 10 min during this time. The samples were centrifuged at 15,000 rpm and 4 °C for 15 min, the supernatant was collected, anti-Myc antibody was added, and the samples were incubated overnight on a 4 °C rotary mixer. Magnetic beads were then collected and washed five times with prechilled IP buffer for 5 min each. The beads were collected and analyzed for the label-free quantitative proteomics assay to assess the IRE1α-enriched proteins by Shanghai Bioprofile Technology Co., Ltd., Shanghai, China.
Co-immunoprecipitation (Co-IP)
Cells were lysed with cold IP-lysis buffer (50 mM Tris-HCl, 150 mM NaCl, 2 mM EDTA, 0.5% NP40, pH 7.5) with protease inhibitors (1 mM PMSF) for 30 min as described previously16.
RNA-seq library preparation and sequencing
RNA-seq library preparation and sequencing were performed in accordance with previous reports7,18.
Luciferase assay
For generation of the pGL3-Col2-luc reporter plasmid, the promoter region of the human Col2A1 gene was amplified by PCR using the genomic DNA of healthy adult volunteers’ peripheral venous blood as a template. The gene fragment was located between −1267 bp upstream and +285 bp downstream of the start of transcription, and PCR products were inserted into the pGL3 vector after digestion with the restriction endonucleases MluI and BglII. The primers are shown in Supplementary Table 1. For the luciferase assay, cells were cultured in 24-well plates and cotransfected with 0.5 μg of Col2A1 gene-responsive luciferase reporter (pGL3-Col2) and XBP1s eukaryotic expression plasmid (pcDNA3.1-XBP1s) using PEI (Sigma) following the manufacturer’s instructions. The pRL-SV40 plasmid (Promega) was added as an internal control. Cells were harvested 48 h post-transfection and subjected to the Dual-Luciferase® Reporter Assay (Promega #E1910). Each assay was performed in triplicate and repeated three times.
Chromatin immunoprecipitation (ChIP)
C28/I2 cells were cultured and then treated with formaldehyde (final 1%) at 37 °C for 10 min to crosslink the target protein and the corresponding genomic DNA. Glycine solution (final 0.125 M) was added to stop crosslinking. Cells were washed with cold PBS and lysed with ChIP lysis buffer (50 mM HEPES, 150 mM NaCl, 1 mM EDTA, 0.1% SDS, 0.1% sodium deoxycholate, 1% Triton X-100, pH 7.5). The lysate was sonicated to shear DNA to a length between 200 and 1000 bp. The sonicated supernatant was incubated with either antibody against XBP1s (Biolegend, USA) or control IgG overnight at 4 °C with rotation. For the collection of the DNA-XBP1s-antibody complex, Magrose Protein A/G (BEAVER) was added to the mixture and incubated for 1 h at 4 °C with rotation, and the DNA/Magrose Protein A/G complex was pelleted by a magnetic stand. After extensive washing of the pellet in a series of washing buffers, the pellet was dissolved in elution buffer (10 mM EDTA, 50 mM Tris, 1% SDS, pH 7.5), and the magnetic beads were removed. The supernatant was treated with NaCl (final 0.2 M) and heated to 65 °C for 4 h to reverse the protein‒DNA crosslinking. After treatment with EDTA and proteinase K, the supernatant was extracted with phenol/chloroform and precipitated with ethanol to recover the DNA. The DNA pellet was resuspended in a small amount of water for qPCR detection of the target gene. The full list of primers is listed in Supplementary Table 2.
Western blot analysis
Western blot analysis was performed as described previously16. The full list of primary antibodies is listed in Supplementary Table 3.
Scanning electron microscopy (SEM) and transmission electron microscopy (TEM)
Femoral heads were isolated from 12-month-old control mice and ERN1 cKO mice. Femoral heads were treated with 0.1% (w/v) trypsin (Sigma #T7409) and 0.1% (w/v) hyaluronidase (Sigma #H3506) at 37 °C for 24 h each to remove proteoglycans, fixed with Karnovsky’s fixative at room temperature for 3 h, and sequentially dehydrated in graded water–ethanol and tert-butyl alcohol. The freeze dryer was precooled to approximately −50 °C, and the samples with tert-butanol were placed in and defrosted for 15–30 min. The samples were vacuumed until the tert-butanol was completely sublimated, approximately 3–8 h. The samples were then coated with platinum and imaged using a scanning electron microscope (SU8010, Hitachi).
Then, costal cartilage was isolated from 12-month-old control mice and ERN1 cKO mice. All samples were fixed with 2% glutaraldehyde solution and decalcified with 15% (w/v) EDTA at pH 7.4 for 14 days. After dehydration with an alcohol gradient series, each sample was doubly replaced with propylene oxide, soaked with epoxy resin, and embedded in an oven at 60 °C for 48 h. The specimens were then sectioned into ultrathin slices, dyed with citric acid lead, and examined under a transmission electron microscope (JEM-1400Plus, JEOL).
Sulfated glycosaminoglycan assay (sGAG)
Mouse knee joint cartilage samples were collected at 4 weeks after ACLT surgery and lyophilized. Explants (20–50 mg) were digested with papain (20 mg/ml) in 0.2 M sodium phosphate buffer (Na2HPO4–NaH2PO4, pH 6.4), 8 mg/ml sodium acetate, 4 mg/ml EDTA and 0.8 mg/ml L-cysteine-HCl at 65 °C for 18 h. The tubes were centrifuged at 10,000×g for 10 min. The supernatant was decanted for use with a Blyscan sGAG assay (Blyscan, Biocolor, Ltd., Carrickfergus, UK) with a chondroitin sulfate standard and normalized against the explants’ wet weight. sGAG absorbance readings were carried out for each cartilage sample in duplicate in 96-well plates at 656 nm. The S-glycosaminoglycan concentrations were obtained from the standard curve.
Statistical analysis
All statistical analyses were analyzed using GraphPad Prism software (version 7.0; GraphPad, Inc., La Jolla, CA, USA). Student’s t-test was used to establish statistical significance between the two groups. One-way or two-way analysis of variance (ANOVA) was performed. Experimental data are expressed as the mean ± standard error of the mean (S.E.M.). A P value <0.05 was considered statistically significant.
Results
The expression profile of IRE1α in OA patients and mice with surgically induced OA
To identify the potential role of IRE1α/XBP1s in OA, we isolated primary cartilage tissues from human osteoarthritic and control articular cartilage, and the protein expression levels of IRE1α, p-IRE1α and XBP1s in the articular cartilage of patients with OA were significantly higher than those in the non-OA cartilage (Supplementary Fig. 1). Furthermore, the expression of IRE1α and phosphorylated IRE1α in the articular cartilage of the mice in the ACLT model group was also notably higher and more widely distributed than that in the sham group (Supplementary Fig. 2). The data indicate that the articular cartilage microenvironment of OA exists in a state of ER stress. The expression profile of IRE1α/XBP1s is associated with the occurrence and development of OA, and thus, it was further investigated.
Specific deficiency of ERN1 in chondrocytes generates an OA-like phenotype in aging mice
We then generated mice with cartilage-specific defects in ERN1 (ERN1flox/floxCol2Cre+, ERN1 cKO mice) (Supplementary Fig. 3a, b) and observed spontaneous OA development and symptoms in aging ERN1 cKO mice (Supplementary Video). The hind limb joints of 4-month-old and 12-month-old mice were collected. As shown in Fig. 1a–d, in the 12-month-old mouse group, proteoglycans, chondrocyte number and cartilage thickness in the articular cartilage of the ERN1 cKO mice were significantly lower than those of the control littermates, and the Osteoarthritis Research Society International (OARSI) score indicated more severe OA symptoms in the ERN1 cKO mice than in the control mice, although there was no significant difference in the 4-month-old mice. In addition, IHC results showed that compared with those of control mice, articular cartilage anabolic markers, including Col2 and Aggrecan, were decreased in the ERN1 cKO mice, whereas the catabolic marker MMP13 was increased (Fig. 1e, f).
Simultaneously, the expression of osteogenesis-related markers, such as DMP, RUNX2, OPG, and Col1, was upregulated in primary chondrocytes isolated from the cartilage of the ERN1 cKO mice compared to that in control primary chondrocytes from the cartilage of the wild-type mice (Fig. 1g). Pearson correlation analysis showed that the mRNA level of ERN1 was positively associated with the mRNA levels of Col2 and Aggrecan and negatively related to the levels of MMP13 and ADAMTS5 in the mouse cartilage tissues (Fig. 1h). The gait analysis of 12-month-old ERN1 cKO mice and control mice further indicated that the print area, swing speed, mean intensity, step cycle, run average speed, stand, max contact and max intensity of the ERN1 cKO mice were clearly reduced, whereas the run duration, stride length and swing of the ERN1 cKO mice were obviously increased compared with those of the control mice. These findings indicated that ERN1 cKO mice may suffer from OA-related pain (Fig. 1i, j, Supplementary Fig. 4). These data confirm that ERN1 plays a protective role in OA progression.
ERN1 deficiency causes aggravated OA development in a surgically induced arthritis model
We first verified that the expression of IRE1α in primary chondrocytes of ERN1 cKO mice was significantly reduced by Western blotting (Fig. 2a). Then, ACLT-induced OA models were established in control and ERN1 cKO mice, and samples were collected at predetermined time points (4, 8 and 12 weeks). The OARSI score indicated that the ERN1 cKO mice displayed more severe OA symptoms than the control mice after ACLT surgery (Fig. 2b, c). The results showed that with the extension of time after surgery, more severe knee cartilage damage was observed in the ERN1 cKO mice than in the control mice, as indicated by the destruction of cartilage integrity and loss of proteoglycans. Furthermore, immunofluorescence staining was performed on the knee joint tissue samples of the mice at 12 weeks (Fig. 2d). The levels of total and phosphorylated IRE1α in the articular cartilage of mice in the ERN1 cKO group were significantly lower than those in the control group. Moreover, the expression of the cartilage anabolic marker aggrecan in the articular cartilage of the ERN1 cKO mice was significantly lower than that of the control group, while the expression of the cartilage catabolic marker MMP13 was significantly higher than that of the control group. Compared with that of the primary chondrocytes of control mice, after successful ERN1 knockout, the mRNA level of XBP1s decreased significantly. In addition, the mRNA level of the cartilage anabolic markers Col2 and DCN in the primary chondrocytes of ERN1 cKO mice were significantly reduced, while the expression of the catabolic marker ADAMTS5 was significantly increased (Fig. 2e). Moreover, under IL-1β-induced inflammatory conditions, the cartilage anabolic markers were more obviously reduced, and the catabolic marker was clearly enhanced in the primary chondrocytes of the ERN1 cKO mice (Fig. 2f). Subsequently, stable cell lines with specific ERN1 knockout (ERN1 KO1 and ERN1 KO2) were constructed and screened by CRISPR‒Cas9 in human C28/I2 cells (Supplementary Fig. 5a). The RT‒qPCR data showed that, compared with that of the control group, the cartilage anabolic marker DCN was significantly reduced after ERN1 was knocked out, while the cartilage catabolic marker MMP13 was significantly increased (Supplementary Fig. 5b). In addition, under inflammatory conditions, the decrease in the cartilage anabolic markers Col2 and DCN and the increase in the decomposition marker MMP13 were more obvious in the ERN1 null chondrocytes (Supplementary Fig. 5c).
Furthermore, we found that overexpression of ERN1 (AdERN1), with increased phosphorylation of IRE1α, induced significant increases in cartilage anabolic markers, such as Col2 and aggrecan, while the cartilage catabolic marker MMP13 was significantly decreased. This phenomenon was notable in the inflammatory microenvironment induced by IL-1β, which manifested as an obvious enhancement in cartilage anabolic markers and a decrease in cartilage catabolic markers after IL-1β induction (Supplementary Fig. 6a–d). In summary, ERN1 can protect cartilage by promoting cartilage anabolism, inhibiting catabolism, and relieving the progression of OA.
IRE1α binds to PGRN, which is required for the chondroprotective effect of IRE1α
To explore the mechanism of IRE1α in the pathogenesis of OA, we performed a proteomic analysis to detect and identify IRE1α-binding proteins. Mass spectrometry data revealed that PGRN is a protein that is highly enriched for binding to IRE1α (Fig. 3a). We then used a visual molecular dynamics (VMD) technique to predict that IRE1α interacts with the two subunits of PGRN (Fig. 3b). Subsequently, fluorescence colocalization revealed that IRE1α and PGRN were colocalized in the cytoplasm (Fig. 3c). The co-immunoprecipitation data were consistent with the VMD results, which confirmed that IRE1α and PGRN could bind to each other (Fig. 3d). A previous report showed that IRE1α contains a kinase (524 aa-827 aa) and an RNase (828 aa-977 aa) domain. We further revealed that the kinase domain of IRE1α binds to PGRN (Fig. 3e) and that the RNase domain cannot bind to PGRN (Supplementary Fig. 7). Then, we detected the interaction between p-IRE1α and PGRN. The results showed that p-IRE1α can bind to PGRN (Fig. 3f), and PGRN promotes the expression of p-IRE1α, IRE1α and XBP1s (Fig. 3g, h). Furthermore, Pearson correlation analysis showed that the mRNA level of ERN1 was positively associated with the mRNA level of PGRN in mouse cartilage tissues (Fig. 3i). Moreover, overexpression of IRE1α upregulated the mRNA and protein expression of PGRN, and the same trend was observed under IL-1β-induced inflammatory conditions (Fig. 3j, k). The protein level of PGRN was significantly decreased in the ERN1-defect primary chondrocytes and ERN1-deficient stable cell lines compared with the controls (Fig. 3l). Importantly, the mRNA expression of PGRN in the ERN1-deficient chondrocytes was significantly downregulated under IL-1β-induced inflammatory conditions (Fig. 3m–o). The above data reveal that IRE1α and PGRN can bind to each other, and their expression profiles affect each other and change due to the influence of inflammatory factors. Additionally, the expression of PGRN in osteoarthritic cartilage tissue was significantly increased compared with that in normal cartilage tissue, consistent with the changes in the expression profiles of IRE1α, p-IRE1α, and XBP1s in the articular cartilage of OA patients, suggesting that PGRN and IRE1α are the key proteins involved in the progression of OA (Supplementary Figs. 1 and 8).
To further determine whether and how PGRN participates in the mechanism by which AdERN1 protects articular cartilage, we studied the treatment effect of AdERN1 in the ACLT-induced OA model in C57 wild-type mice and GRN-/- knockout (PGRN KO) mice. AdERN1 and AdERN1+siPGRN were injected into the knee joint cavity of WT C57 mice, while AdERN1 and AdERN1+rhPGRN were injected into the knee joint cavity of GRN-/- KO mice after ACLT (Fig. 4a, f). The results showed that local delivery of AdERN1 protected articular cartilage, while knockdown of PGRN inhibited the protective effect of AdERN1 on cartilage to a certain extent in the WT ACLT mouse model (Fig. 4b, c), and AdERN1 had no obvious chondroprotective effect in the GRN-/- KO mouse model. The OARSI score showed that there was no significant difference between the arthritis score of the AdERN1 group and that of the AdGFP group in the GRN-/- KO mouse ACLT model, indicating that PGRN deficiency inhibited the chondroprotective effect of AdERN1 on cartilage. The local delivery of AdERN1+rhPGRN restored the chondroprotective effect on articular cartilage in the GRN-/- KO mouse ACLT model (Fig. 4g, h).
IHC showed that in the WT ACLT mouse model, the number of aggrecan-positive cells on the cartilage surface of the AdERN1 group was significantly higher than that of the control group. After PGRN knockdown, the number of aggrecan-positive cells decreased. In contrast, the number of MMP13-positive cells in the AdERN1 group was significantly lower than that in the control group, while after knockdown of PGRN, the number of MMP13-positive cells increased (Fig. 4d). Moreover, in the GRN-/- KO mouse ACLT model, AdERN1 did not upregulate the expression of aggrecan and Col2 or downregulate that of MMP13, whereas rhPGRN recovered the above effects of AdERN1 in the AdERN1+rhPGRN group (Fig. 4i). Furthermore, Western blot analysis showed that the protein levels of aggrecan, Col2, PGRN, XBP1s, and IRE1α/p-IRE1α were increased in the AdERN1 group compared to the control group, whereas the expression of the above proteins was reduced after PGRN knockdown (Fig. 4e). Collectively, PGRN is involved in the protective effect of AdERN1 on cartilage in mice, and the chondroprotective effect of IRE1α is dependent on PGRN.
IRE1α accelerates XBP1s splicing and PGRN promotes the chondroprotective role of AdXBP1s through ERK1/2 signaling
Next, Pearson correlation analysis showed that the mRNA level of XBP1s was positively associated with the mRNA levels of ERN1 and PGRN in mouse cartilage tissues (Fig. 5a). Western blot analysis showed that overexpression of AdERN1 promoted the production of phosphorylated IRE1α and XBP1s in a dose-dependent manner. Overexpression of AdXBP1s also increased the protein level of PGRN, whereas siXBP1s inhibited the expression of PGRN (Fig. 5b, c). Notably, PGRN modulates the expression profile of IRE1α and XBP1s with positive feedback. We next explored whether and how PGRN affects the function of XBP1s. As shown in Fig. 5d and e, AdXBP1s and AdXBP1s+rhPGRN were injected into the knee joint cavity of WT C57 mice after ACLT. The results showed that compared with that of the AdGFP control group, the arthritis score of the AdXBP1s group was significantly lower, and the arthritis score of the AdXBP1s+rhPGRN group was significantly lower than that of the AdXBP1s group. IHC results also showed that XBP1s upregulates the expression of PGRN, the number of aggrecan-positive cells on the cartilage surface of the AdXBP1s group was higher than that of the AdGFP control group, and the value of the AdXBP1s+rhPGRN group was significantly higher than that of the AdXBP1s group; the number of MMP13-positive cells on the cartilage surface of the AdXBP1s group was reduced compared with that of the AdGFP control group, and the value of the AdXBP1s+rhPGRN group was significantly decreased compared with that of the AdXBP1s group (Fig. 5f, g). These data indicate that overexpression of AdXBP1s can protect articular cartilage and that rhPGRN can promote the chondroprotective effect of AdXBP1s in vivo. Moreover, overexpression of XBP1s increased the mRNA levels of Aggrecan and Col2 and decreased the mRNA levels of ADAMTS5 and MMP13 in cartilage tissue explants from OA patients. Then, rhPGRN promoted the upregulation of Aggrecan and Col2 by AdXBP1s and improved the downregulation of ADAMTS5 and MMP13 by AdXBP1s in the AdXBP1s+rhPGRN group under IL-1β-induced inflammatory conditions (Fig. 5h). As reported in the literature, PGRN activation of extracellular signal-regulated kinases (ERK1/2) is involved in the regulation of numerous processes, and ERK1/2 is known to protect chondrocytes from OA19,20,21. We then found that overexpression of XBP1s can activate the phosphorylation of the ERK1/2 signaling pathway in cartilage and chondrocytes with or without TNFα-induced inflammatory conditions (Fig. 6a, b). In addition, XBP1s can activate ERK1/2 signaling phosphorylation when the TNF-α effect is blocked or partially blocked by the TNFR1/2 antibody (Fig. 6c, d). Moreover, PGRN increased the phosphorylation of ERK1/2 activated by XBP1s, and this promoting effect was more obvious under TNFα-induced inflammatory conditions (Fig. 6e, f). Importantly, ERK1/2 phosphorylation activated by AdXBP1s and AdXBP1s+rhPGRN was blocked after U0126 treatment in chondrocytes. Furthermore, after inhibition of ERK1/2 phosphorylation in chondrocytes by U0126, the upregulation of Aggrecan and Col2 by AdXBP1s and AdXBP1s+rhPGRN and the downregulation of ADAMTS5 and MMP13 by AdXBP1s and AdXBP1s+rhPGRN were blocked. The protective articular cartilage roles of AdXBP1s and AdXBP1s+rhPGRN were dependent on ERK1/2 signaling (Fig. 6g, h). Collectively, XBP1s and XBP1s+PGRN exerted chondroprotective effects by activating ERK1/2 signaling.
ERN1 regulates collagen homeostasis by controlling collagen II expression through XBP1s
Previous studies have confirmed that XBP1s, a transcription factor with multiple regulatory functions, enters the nucleus to regulate the transcription and expression of related genes after splicing by phosphorylated IRE1α22,23. As shown in Fig. 7a, overexpression of AdERN1 increased the phosphorylation level of IRE1α and the spliced protein XBP1s in the nucleus under ER stress but had no significant effect on the protein level of XBP1s or phosphorylated IRE1α in the cytoplasm. Importantly, after the knockdown of PGRN with siRNA, overexpression of AdERN1 did not enhance the phosphorylation of IRE1α or the spliced protein level of XBP1s in the nucleus. In addition, in PGRN knockout chondrocytes constructed with the CRISPR‒Cas9 technique, the protein levels of IRE1α and XBP1u were obviously reduced compared to those of wild-type chondrocytes, whereas XBP1s, resulting from XBP1u splicing, was only clearly detectable under ER stress (Fig. 7b). During IL-1β-induced ER stress, the transcription factor XBP1s, spliced by phosphorylated IRE1α, undergoes nuclear translocation and regulates the transcription of related genes in the nucleus. As shown by cellular immunofluorescence, AdERN1 increased the expression of XBP1s in the nucleus after IL-1β treatment. However, siPGRN suppressed the nuclear translocation of XBP1s (Fig. 7c). Moreover, the nuclear translocation of XBP1s increased after rhPGRN treatment (Supplementary Fig. 9). Thus, the splicing and nuclear translocation of XBP1s are dependent on PGRN.
As reported by Cameron et al., cartilage-specific deficiency of XBP1 in mice causes chondrodysplasia characterized by reduced chondrocyte proliferation and delayed cartilage maturation and mineralization24. We constructed six mRNA libraries between XBP1 KO cartilage and normal cartilage and then identified the different mRNAs through whole transcriptome RNA-seq18. We compared some differentially expressed collagen-related proteins, including Col2a1, Col9a2, and Col16a1. The FPKM (fragments per kilobase of transcript sequence per million base pairs sequenced) expression of Col2a1 was the most significantly different in the XBP1-deficient chondrocytes, and its expression was significantly reduced compared with that of the control (p = 0.009). In addition, the FPKM expression of PGRN was significantly decreased compared with that of the control (p = 0.026) (Fig. 7d, e). We next predicted the binding site of the transcription factor XBP1s to the Col2a1 promoter, and chromatin immunoprecipitation (ChIP) analysis confirmed that XBP1s could bind to the Col2a1 (−1267 to +285) promoter regions. Furthermore, overexpression of the transcription factor XBP1s significantly upregulated the transcriptional activity of the Col2a1 reporter gene (pGL3-Col2) (Fig. 7f–h). Similarly, IHC data showed that the expression of Col2 was significantly higher than that in the control group in the articular cartilage of mice after XBP1s was overexpressed by injection of AdXBP1s into the articular cavity (Fig. 7i, j). Additionally, in ERN1-null chondrocytes, ERN1 deficiency led to reduced XBP1s expression in chondrocytes, and the expression of Col2 was also significantly suppressed (Fig. 7k). Immunofluorescence analysis of primary chondrocytes revealed that the expression of Col2 in the ERN1 cKO group was lower than that in the control group with or without IL-1β treatment, and Col2 expression in the ERN1 cKO group decreased more significantly than that in the control group (Fig. 7l). This finding further shows that IRE1α/ERN1 promotes the expression of Col2 through the XBP1s signaling axis to protect cartilage. Moreover, the sGAG assay showed that the level of sGAG in the ERN1 cKO group was lower than that in the control group, and there was no significant difference between the control and cKO sham groups; however, after ACLT surgery, the level of sGAG in the ERN1 cKO group was reduced more significantly than that in the control group. Proteoglycans constituting the extracellular matrix (ECM) and articular cartilage were significantly reduced and degraded in the ACLT-induced model of ERN1-deficient mice compared to control mice (Fig. 7m). We next observed the ultrastructure of collagen in cartilage and chondrocytes using TEM and SEM. TEM data revealed that the organelles of chondrocytes were destroyed when ERN1 was deficient, including nuclear condensation and marginalized nuclear chromatin, increased vacuolization in the cytoplasm, disrupted ER, and disordered collagen arrangement around chondrocytes (Fig. 7n). The SEM results were consistent with the TEM data, showing that the cartilage collagen fibers were discontinuous, had a rough surface, and had a disordered arrangement in the cartilage of the ERN1-deficient mice compared with that in the control mice (Fig. 7o). Collectively, we found that in ERN1-deficient chondrocytes, collagen homeostasis is imbalanced and that the ultrastructure is abnormal. We further show that ERN1 maintains collagen homeostasis by regulating Col2 transcription and expression through the transcription factor XBP1s.
Discussion
Osteoarthritis is primarily characterized by progressive breakdown, loss of extracellular matrix proteins and collagen fibers, and articular cartilage damage caused by various factors, including aging and injury25,26. ER stress has been confirmed to be related to the occurrence and development of many diseases, including OA27,28, RA16,29, and other inflammatory diseases30,31. IRE1α is a classic sensor of the UPR, which is involved in the folding of secreted proteins in the ER, including collagens II, IX, and X, proteoglycans and other proteins that make up the ECM. According to the heterogeneity and complexity of OA, the expression profiles of several UPR genes, including IRE1α and XBP1s/u, presented obvious differences with different OA patients and disease courses. This finding is also confirmed by the high expression of IRE1α and its phosphorylation we observed (Supplementary Fig. 1) and the differential expression profiles reported in the literature16,32. The highly conserved UPR molecules present a complex and variable expression profile with the course of OA, suggesting the importance of individualized and precise treatment of OA.
We observed and found that older ERN1-specific knockout mice were more prone to spontaneously developing OA symptoms, such as severe proteoglycan loss, more obvious cartilage damage, joint pain, and abnormal gait, than control mice. In addition, degenerative biomarkers, including MMP13, were significantly elevated, whereas levels of the anabolic markers aggrecan and Col2 were critically decreased in the cartilage of the ERN1 cKO mice compared with that of the control group with aging (Fig. 1a–f, h)33. Type II collagen-positive (Col2+) progenitors are the major source of endochondral ossification, and they are major stem cells that control skeletal development and vascular formation34. Col2a1-Cre was shown to target chondrocytes and osteoblastic lineage cells, including osteocytes, osteoblasts, and their precursors/progenitors, in long bones35. Herein, we observed that the expression of some osteocyte marker genes, including DMP, OPG and Col1, was upregulated in the cartilage tissue of ERN1 CKO mice (Fig. 1g). These findings suggested that Col2Cre-specific chondrocyte lineage defects in the ERN1 gene may be involved in cartilage degeneration and damage by affecting endochondral ossification. In the ERN1 cKO ACLT mouse model, more severe loss of proteoglycan in safranin O staining, a significantly higher arthritis score, elevated expression of MMP13 and ADAMTS5, and reduced expression of aggrecan and Col2 were observed (Fig. 2). Combined with these data, the loss of IRE1α in chondrocytes may accelerate OA aging and degeneration. ERN1 plays a protective role in articular cartilage.
Through proteomics analysis, we identified that PGRN binds to IRE1α and participates in the regulation of IRE1α on chondrocyte metabolism. PGRN has been implicated in a variety of physiological processes and pathological states and has multiple functions36,37,38,39. The unique domains or motifs of PGRN determine the diversity of proteins that bind to it and thus the functional diversity of PGRN. Previous reports have shown that most PGRN-related proteins can be divided into the following three categories40: cell membrane receptors, ECM molecules, and intracellular chaperones and lysosomal hydrolases39,41,42,43,44,45,46,47,48,49. In this study, we detected and identified a novel PGRN-binding protein, IRE1α. PGRN, as an intracellular chaperone, binds to the kinase domain of IRE1α and assists in the phosphorylation of IRE1α to promote the splicing of XBP1u to generate XBP1s during ER stress (Fig. 3). Intriguingly, IRE1α achieves its chondroprotective effect by combining with PGRN and promoting XBP1s splicing. This chondroprotective effect of IRE1α is dependent on PGRN and is achieved through upregulation of ERK1/2 signaling (Figs. 4–6). Moreover, the expression profiles of PGRN, IRE1α and XBP1s are positively correlated and can influence each other. They can form a positive feedback regulatory loop. Intra-articular injection of rhPGRN protein has been reported to attenuate OA-like phenotypes and relieve OA progression in mice. This therapeutic effect of PGRN is mediated through interactions with the TNF-α and β-catenin signaling pathways50. Herein, PGRN is associated with IRE1α/XBP1s, the most conserved signaling pathway in ER stress, and plays a protective role in cartilage via positive feedback regulation with IRE1α/XBP1s during the process of OA. PGRN assists IRE1α in realizing the splicing and nuclear translocation of XBP1s. Activated XBP1s then translocates to the nucleus, where it functions as a multifunctional transcription factor. Cameron et al. reported that cartilage-specific XBP1-deficient mice exhibit chondrodysplasia, and the UPR pathway presents genetic redundancy in cartilage pathology, thereby mediating the XBP1-independent UPR signaling pathway10,24. Although the XBP1-independent UPR signaling pathway may compensate for some of the defects in XBP1s function due to ERN1 deficiency, the role and mechanism of how ERN1 deficiency and XBP1-dependent UPR signaling affect other downstream molecules to regulate cartilage metabolism in ERN1-deficient mice is unclear. Of note, we demonstrate that PGRN serves as a master regulator of cartilage metabolism in OA, compensating for some of the functions lost due to ERN1 deficiency by promoting and upregulating the biological effects of XBP1s. Moreover, the protective articular cartilage roles of XBP1s and XBP1s+PGRN were dependent on ERK1/2 signaling (Fig. 6), which is involved in the regulation of cell proliferation and survival. These results again confirm our previous findings15,51. Huang et al. also showed that deficiency of IRE1α in chondrocytes downregulates the prosurvival factors XBP1s and Bcl-2, which promotes the apoptosis of chondrocytes17. In addition to survival and apoptosis, collagen homeostasis imbalance and loss are major features of cartilage senescence, and aging is the main cause of OA. Intriguingly, we found that XBP1s can maintain collagen homeostasis by regulating the expression of type II collagen, thus participating in the protection against cartilage degeneration in OA (Fig. 7).
As summarized in Fig. 8, IRE1α binds to PGRN and splices XBP1u to generate XBP1s, which undergoes nuclear translocation, subsequently upregulating the expression of Col2 to maintain collagen homeostasis and achieve a chondroprotective effect. Furthermore, the chondroprotective effect of IRE1α relies on PGRN. Moreover, XBP1s exerts a chondroprotective role by activating ERK1/2 signaling, and PGRN promotes this effect. Enhancement of XBP1s function by PGRN may play a compensatory role in the absence of ERN1/XBP1s function. ERN1 deficiency accelerates cartilage degeneration in OA by reducing PGRN expression and XBP1 splicing, which in turn decreases the expression of type II collagen, resulting in collagen structural abnormalities and an imbalance in collagen homeostasis. The exploration of the mechanisms underlying OA development and pathogenesis is important for the clinical individualized precision treatment of OA. This study provides the key role of IRE1α in the progression of OA and presents new insights into the role of IRE1α in the treatment of degenerative joint diseases.
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Acknowledgements
We are particularly grateful to Professor Chuanju Liu of New York University and Professor Lin Chen of Daping Hospital of Army Medical University for their strong support and help with this project. This work was supported by the National Natural Science Foundation of China (No. 82272550, No. 81871769), the Postdoctoral Science Foundation of China (No. 2021M700632), and the Special Postdoctoral Science Foundation of Chongqing (No. 2020-379-46). All experiments were completed on the experimental platform provided by the Core Facility of Development Biology of Basic Medical College (Chongqing Medical University).
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The manuscript was written through the contributions of all authors. All authors have given approval to the final version of the manuscript. F.J.G. and L.L. designed the experiments; L.L., F.M.Z. and N.B.F. completed the data collation and article writing; L.L., F.M.Z., N.B.F., B.K., M.T.F., Y.M.P., P.F.Z., N.N.G., X.Y.L., M.L.X., L.D., X.L.L., L.K., F.T.L., Q.Y.T. and Y.L.X. analyzed the data; C.C. provided the cartilage tissues of OA patients; F.J.G. designed the manuscript and had full access to all of the data in the study and takes responsibility for the integrity of the data and the accuracy of the data analysis. All authors approved the final manuscript prior to submission.
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The experimental procedures ensured the safety of practitioners in laboratory animal projects, conformed to human ethical standards and international practices and were approved by the Animal Experimental Ethics Committee of Chongqing Medical University. All animal experiments conformed to the guidelines of Directive 2010/63/EU of the European Parliament on the protection of animals used for scientific purposes. All experiments were completed on the experimental platform provided by the Core Facility of Development Biology of Basic Medical College (Chongqing Medical University).
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Liang, L., Zhang, F., Feng, N. et al. IRE1α protects against osteoarthritis by regulating progranulin-dependent XBP1 splicing and collagen homeostasis. Exp Mol Med 55, 2376–2389 (2023). https://doi.org/10.1038/s12276-023-01106-w
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DOI: https://doi.org/10.1038/s12276-023-01106-w