Chondroprotective effects of Salubrinal in a mouse model of osteoarthritis

Cell culture

Human primary chondrocytes (PC136121A1-C, Asterand Bioscience, Cambridge, Massachusetts) and human chondrocyte cell line, C28/I2, were cultured in DMEM/F12 and DMEM mediums, respectively, which were supplemented with 10% fetal bovine serum and antibiotics (Life Technologies, Grand Island, New York). Cells were maintained at 37°C and 5% CO2 in a humidified incubator. After ten hours of serum-free conditions, cells were incubated with 10 ng/ml TNFα (R& D Systems, Minneapolis, Minnesota) in the presence and absence of 5 µM Salubrinal or 5 µM Guanabenz (TOCRIS Bioscience, Ellisville, Missouri). One µM thapsigargin (Santa Cruz Biotechnology, Santa Cruz, California) was used as a positive control (PC) for phosphorylation of eIF2α.

A mouse model of OA and administration of Salubrinal or Guanabenz

OA was surgically induced in the left knees of 118 C57/BL6 female mice (approximately nine weeks old) by transecting the medial collateral ligament and removing the medial meniscus.²³ Animal groups included age-matched sham control (CN), OA placebo, and OA treated with Salubrinal (OA + Sal). The sham surgery consisted of incision and suture. We also employed additional age-matched sham control and two OA groups treated with Guanabenz and its solvent (placebo). A total of three days after the induction of OA, Salubrinal (1.5 mg/kg) or Guanabenz (2.0 mg/kg) was administered daily into an intra-articular space, while their solvents (49.5% PEG 400 and 0.5% Tween 80 in PBS for Salubrinal; and distilled water including 5% glucose for Guanabenz) were used in the placebo groups. Mice were anaesthetised, after which injection was conducted to the intercondylar fossa from the patellar tendon in a sagittal plane to avoid potential damage to the load-bearing cartilage surface.

Western blot analysis

Human primary chondrocytes (15 minutes after addition of TNFα) and tibia cartilage (three weeks after the induction of OA) were lysed in a radioimmunoprecipitation assay buffer.²² We chose a tibia sample as they were able to be harvested with fewer potential contaminations with subchondral bone or bone marrow than femur samples. Isolated proteins were gel-fractionated and electro-transferred to Immobilon-P membranes (Millipore, Billerica, Massachusetts). The antibodies used were phosphorylated NFκB p65, NFκB p65 (Cell Signaling, Beverly, Masachusetts) and β-actin (Sigma, St Louis, Missouri). Images were taken with a luminescent image analyser (LAS-3000, Fuji Film, Tokyo, Japan), and signal intensities were quantified with Image J software (National Institute of Health, Bethesda, Maryland). Data were presented with reference to control intensities of β-actin.

Safranin O staining

Knee samples were decalcified in 10% ethylenediaminetetraacetic acid (EDTA) for two weeks, embedded in paraffin and sectioned at 4 µm thickness. After deparaffinisation and rehydration, slides were stained with Weigert’s iron haematoxyline solution for five minutes. They were differentiated in 1% acid–alcohol, and stained with 0.02% fast green solution. They were then rinsed in 1% acetic acid, stained in 1% Safranin O solution for 30 minutes and treated with graded ethyl alcohol and xylene.²⁵

Histological score for symptoms of osteoarthritis

Tissue sections (approximately 50 sections per mouse) were graded using the scoring system described by Glasson et al.²⁴ Because of the specific procedure taken for OA induction, we focused on the histological evaluation of the medial side that exhibited more severe symptoms than the lateral side. Accordingly, the grade was assigned by two independent scorers blinded to treatment allocation (KH, AN) as follows: “0” = normal; “0.5” = loss of Safranin O without structural changes; “1” = small fibrillations without loss of cartilage; “2” = vertical clefts down to the layer immediately below the superficial layer and some loss of surface lamina; and “3” to “6” = vertical clefts/erosion to the calcified cartilage extending to < 25%, 25% to 50%, 50% to 75%, and > 75% of the articular surface, respectively.

Determination of thickness of subchondral bone and synovial score

To evaluate the effects of OA induction on subchondral bone, its average thickness was determined using the procedure described previously.²⁶ In brief, the area of subchondral bone was measured using Image J software. The average thickness was then determined as a ratio of subchondral bone area to its weight-bearing width. We also determined synovial scores for evaluating inflammation of the synovium using the procedure described previously.²⁷

Statistical analysis

For in vitro experiments, three or four independent experiments were conducted and the Student’s t-test was employed. For the evaluation of histological scores, thickness of subchondral bone, and synovial scores, non-parametric statistical analysis (Kruskal–Wallis test and Mann–Whitney U test) was conducted. For the interpretation of in vivo protein samples, one-way analysis of variance followed by Dunnett’s post hoc test, was conducted. Data were expressed as mean and standard deviation (sd), and statistical significance was evaluated at p < 0.05. The single and double asterisks indicate p < 0.05 and p < 0.01, respectively.

In vitro suppression of TNFα-induced NFκB phosphorylation and MMP13 activity by Salubrinal

In response to 10 ng/ml of TNFα, primary chondrocytes (PC136121A1-C) elevated the level of phosphorylated NFκB (p-NFκB) without altering the total level of NFκB (Fig. 1a) elevated the level of phosphorylated NFκB (p-NFκB) without altering the total level of NFκB (Fig. 1a) without altering the total level of NFκB (Fig. 1a). Their incubation with TNFα also increased MMP13 activity (Fig. 1b). However, simultaneous application of 5 µM of Salubrinal with TNFα significantly reduced the level of p-NFκB as well as MMP13 activity (Figs 1a and 1b). Although both Salubrinal and Guanabenz elevate the phosphorylation level of eIF2α, Guanabenz did not alter the level of p-NFκB (Fig. 1c). Although both Salubrinal and Guanabenz elevate the phosphorylation level of eIF2α, Guanabenz did not alter the level of p-NFκB (Fig. 1c) or MMP13 activity (Fig. 1d).

Figs. 1a - 1d

Graphs and staining showing the response of human primary chondrocytes to tumour necrosis factor alpha (TNFα) in the presence and absence of Salubrinal (Sal) or Guanabenz (Gu), with a) activation of nuclear factor kappa B (NFκB) by TNFα for 15 minutes and partial deactivation by Salubrinal, b) matrix metalloproteinase (MMP)13 activity induced by TNFα and suppressed by 5 µM Salubrinal, c) no detectable effect of Guanabenz on the level of p-NFκB and d) no detectable change of MMP13 activity by Guanabenz shown. CN, vehicle.

Reduced cartilage degradation by Salubrinal into the intra-articular space

In the mouse model of osteoarthritis, the sagittal sections stained with Safranin O indicated degradation of articular cartilage on the tibial and femoral surfaces in the knee joint (Fig. 2). The intensity of Safranin O staining decreased in the samples harvested three and six weeks after the induction of OA. However, daily administration of Salubrinal at a dose of 1.5 mg/kg from three days after the induction of OA partially restored Safranin O staining.

Figs. 2a - 2b

Images of safranin O staining of the sagittal knee joint section, with a) samples three weeks after induction of osteoarthritis (OA, placebo sample; OA + Sal, Salubrinal-treated OA sample; CN, sham control sample) and b) samples six weeks after induction of OA shown. The three panels in the top row show an entire knee section (bar = 200 µm), while the three panels in the bottom row depict their enlarged images (bar = 100 µm). The top section in each panel is the femur, and the bottom section is the tibia.

The histological score (0 for normal, and 6 for worst OA) revealed that Salubrinal significantly reduced OA-linked tissue degeneration (Fig. 3) revealed that Salubrinal significantly reduced OA-linked tissue degeneration (Fig. 3). In week three samples, the histological mean scores for the medial femoral condyle (MFC) were 0.8, sd 0.3 (control; CN), 3.8, sd 1.2 (OA placebo; OA), and 2.5, sd 0.5 (OA Salubrinal; OA + Sal) (CN vs OA, p < 0.01; and OA vs OA + Sal, p = 0.045), while the scores for the medial tibial plateau (MTP) were 0.3, sd 0.5 (CN), 2.8, sd 1.0 (OA), and 2.2, sd 0.8 (OA + Sal) (CN vs OA, p < 0.01; and OA vs OA + Sal, p = 0.530). In week six samples, the scores for MFC were 0.6, sd 0.2 (CN), 5.1, sd 0.8 (OA), and 4.0, sd 1.9 (OA + Sal) (CN vs OA, p < 0.01; and OA vs OA + Sal, p = 0.163), while the scores for MTP were 0.6, sd 0.4 (CN), 5.3, sd 0.7 (OA), and 3.7, sd 1.8 (OA + Sal) (CN vs OA, p < 0.01; and OA vs OA + Sal, p = 0.027).

Figs. 3a - 3b

Graphs showing histological scores for progression of osteoarthritis (OA), for a) medial femoral condyle (MFC) (left) and medial tibial plateau (MTP) (right) three-week samples (n = 6) and b) for MFC (left) and MTP (right) six-week samples (n = 5 sham control, CN, 8 OA + placebo, and 7 OA + Salubrinal (Sal)) are shown; *p < 0.05; **p < 0.01.

Increased subchondral bone formation and marginal osteophyte development are part of the joint pathology in OA. In the mouse model of OA in this study, the thickness of subchondral bone was not altered in week three samples, but it was significantly increased in MFC and MTP in week six samples (Fig. 4a). Administration of Salubrinal did not alter the thickness of MFC and MTP at either time points. Regarding synovial inflammation, induction of OA worsened the synovial score in week three and week six samples (Fig. 4b). Salubrinal reduced the score in both samples, although statistically significant reduction was observed only in week three samples.

Figs. 4a - 4b

Graphs showing the effects of Salubrinal on subchondral bone and synovium, with a) thickness of subchondral bone in the medial femoral condyle (MFC) (left) and medial tibial plateau (MTP) (right) (three weeks top row, six weeks bottom row) and b) synovial score for three-week (left) and six-week (right) samples. *p < 0.05; **p < 0.01.

In vivo suppression of OA-induced NFκB phosphorylation and MMP13 activity by Salubrinal

Protein samples harvested from the tibial cartilage, showed upregulation of p-NFκB as well as MMP13 activity compared with the age-matched sham control (Fig. 5). Consistent with the in vitro result, daily administration of Salubrinal significantly reduced p-NFκB (p-NFκB/β-actin CN vs OA, p = 0.001; OA vs OA + Sal, p = 0.023; and p-NFκB/NFκB CN vs OA, p = 0.285; OA vs OA + Sal, p = 0.042) as well as MMP13 activity (CN vs OA, p < 0.001; and OA vs OA + Sal, p < 0.001). Of note, TNFα in the in vitro assay did not alter the level of total NFκB, however, OA protein samples presented an elevated level of NFκB. We also evaluated the levels of p-eIF2α in the mouse cartilage samples as well as C28/I2 chondrocytes, in which 1 µM thapsigargin was employed as a positive control (PC) of elevation of p-eIF2α. In the cartilage samples, the significant elevation of p-eIF2α was not detected (Fig. 6a) of elevation of p-eIF2α. In the cartilage samples, the significant elevation of p-eIF2α was not detected (Fig. 6a). In vitro chondrocyte samples did not also present statistically significant elevation of p-eIF2α in response to TNFα with and without 5 µM Salubrinal (Fig. 6b). Collectively, the result showed that Salubrinal-driven suppression of p-NFκB was not directly linked to the regulation of p-eIF2α.

Figs. 5a - 5b

Graphs showing suppression of p-nuclear factor kappa B (p-NFκB) p65 and activity of matrix metalloproteinase 13 (MMP13) by Salubrinal in a mouse model of osteoarthritis; (n = 12 CN, sham control, 10 OA placebo, and 11 OA + Salubrinal (Sal)), with a) attenuation of the level of p-NFκB p65 by Sal and b) suppression of activity of MMP13 by Sal shown.

Figs. 6a - 6b

Graphs and staining showing evaluation of the phosphorylation level of eukaryotic translation initiation factor 2 alpha (eIF2α) in cartilage samples and C28/I2 chondrocytes, with a) levels of p-eIF2α in tibial cartilage samples (three weeks after the induction of osteoarthritis; OA); (n = 12 CN, sham control, 10 OA placebo, and 11 OA + Salubrinal (Sal)) and b) levels of p-eIF2α in C28/I2 chondrocytes treated with TNFα in the presence and absence of 5 µM Salubrinal for 15, 30, and 360 minutes shown. Thapsigargin at 1 µM was used as a positive control (PC) for p-eIF2α.

No suppressive effects to OA progression with Guanabenz

In response to Guanabenz, the progression of OA was not detectably changed in the femur (MFC) and the tibia (MTP) both in week three and week six samples (Fig. 7) and the tibia (MTP) both in week three and week six samples (Fig. 7) both in week three and week six samples (Fig. 7). In week six samples, for example, the histological score for MFC was 0.8, sd 0.3 (CN), 5.1, sd 0.8 (OA), and 5.2, sd 0.7 (OA + Gu) (CN vs OA, p < 0.01; and OA vs OA + Gu, p = 0.772), while the score for MTP was 0.6, sd 0.4 (CN), 4.8, sd 0.7 (OA), and 4.7, sd 0.5 (OA + Gu) (CN vs OA, p < 0.01; and OA vs OA + Gu, p = 0.758). Compared with the OA control samples, administration of Guanabenz did not alter the thickness of subchondral bone of MFC and MTP at either time points (Fig. 8a) (CN vs OA, p < 0.01; and OA vs OA + Gu, p = 0.758). Compared with the OA control samples, administration of Guanabenz did not alter the thickness of subchondral bone of MFC and MTP at either time points (Fig. 8a). Compared with the OA control samples, administration of Guanabenz did not alter the thickness of subchondral bone of MFC and MTP at either time points (Fig. 8a). Unlike Salubrinal, which significantly reduced the synovial score in week three samples, Guanabenz did not change the synovial score both in week three and week six samples (Fig. 8b).

Figs. 7a - 7b

Histological images and graphs showing no significant prevention of the progression of osteoarthritis (OA) by Guanabenz (Gu). Safranin O staining of the sagittal knee joint section and histological scores, with a) samples three weeks after induction of OA; (n = 6 CN, control sham, 9 OA placebo and OA + Gu) and b) samples six weeks after induction of OA; (n = 5 CN, and 9 OA, and OA + Gu) shown. OA, OA placebo sample; OA + Gu-treated OA sample.

Figs. 8a - 8b

Graphs showing the effects of Guanabenz on subchondral bone and synovium, with a) thickness of subchondral bone for three-week (top) and six-week (bottom) samples in the medial femoral condyle (MFC) (left) and medial tibial plateau (MTP) (right) and b) synovial score for three-week (left) and six-week (right) samples.*p < 0.05; **p < 0.01.

No significant effects on the contralateral knee

Examination of the contralateral knee, which did not receive surgery for OA induction or administration of Salubrinal or Guanabenz, revealed that no significant effects were detected on thickness of subchondral bone or histological scores.