Abstract
We investigated whether different doses of undenatured type II collagen (undenatured collagen, UC-II) help improve monosodium iodoacetate (MIA)-induced (osteoarthritis) OA in young and old rats. A total of 70 rats were divided into five groups: (1) control; (2) MIA (a single intra-articular injection of MIA); (3)–(5) MIA+ Undenatured Collagen with various oral doses (0.66, 1.33, and 2 mg/kg). The results showed that all doses of undenatured collagen in both age groups reduced knee diameter, while the two higher doses (1.33 mg/kg and 2 mg/kg) reduced the Mankin score and increased most gait measurements as early as day 14 compared to the MIA rats. However, the 2 mg/kg dose showed the best efficacy in improving Mankin score and gait measurements by 28 days post-OA induction. In young but not old rats, all doses of undenatured collagen reduced the Kellgren-Lawrence score compared to the MIA group. Undenatured collagen reduced the levels of most inflammatory and cartilage breakdown markers in serum and knee joint cartilage in both age groups. In conclusion, this data suggests that while all doses of undenatured collagen supplementation may ameliorate MIA-induced OA symptoms, the higher doses showed faster improvement in gait measurements and were more efficacious for overall joint health in rats.
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Introduction
Osteoarthritis (OA) affects over 500 million people worldwide and is considered one of the main reasons for disability. Globally, the proportion of people affected by OA has notably increased by 48% from 1990 to 20191. While many assume that OA is most prevalent in older individuals, previous studies have shown that more than half of patients diagnosed with symptomatic knee OA are under the age of 652. The increasing number of sports injuries, joint trauma, occupational exposure, and obesity have resulted in an increase in OA incidence among younger individuals3, 4. Inflammatory arthritis, which comprises inflammatory cell recruitment, synovial joint inflammation, and articular cartilage degeneration, is an age-related joint disease5. In parallel with the aging process, the systemic inflammatory status gradually intensifies due to an increase in age-related inflammation markers; thus, the risk of OA progression increases in older individuals6. Excessive activation of the nuclear factor kappa B (NF-κB) pathway may stimulate the production of inflammatory cytokines [such as interleukin 1-β (IL-1β), interleukin 6 (IL-6), and tumor necrosis factor α (TNF-α)] in chondrocytes, leading to the destruction of the joint structure and the onset of OA7. IL-1 plays a central role in immune disorders by activating intracellular T-cell interactions. IL-1β and TNFα are essential triggers of OA development, whereas IL-4, transforming growth factor β (TGF-β), and interferon-gamma (IFNγ) are categorized as anti-inflammatory cytokines in OA8. The increase in inflammatory cytokines and reactive oxygen species (ROS) with aging also stimulate matrix metalloproteinases (MMPs) that drive cartilage degradation in OA9, 10. Additionally, gut microbiota dysbiosis may contribute to OA progression due to a chronic systemic inflammatory process that may lead to cartilage degeneration11. Aging also exacerbates intestinal dysbiosis, increases proinflammatory symbionts, and reduces antigen-presenting T-cell activation12. It has been shown previously that modulating gut microbiota with dietary supplements, such as chondroitin sulfate and probiotics can alleviate OA symptoms in OA-induced rats11. In addition to aging-related factors, mechanical factors may also trigger the formation of OA earlier in life. Overloading the joint may stimulate ROS formation and inhibit proteoglycan production. This process exacerbates inflammatory cytokine production13 and chondrocyte senescence, similar to aging14. The MIA-induced OA model, extensively used in experimental studies, mimics these phases of OA progression, including initial inflammatory and pain behavior in young and old rats15,16,17.
UC-II undenatured type II collagen (undenatured collagen) is a patented form of collagen derived from chicken sternum cartilage18. Undenatured collagen provides > 3% undenatured (native) type II collagen for joint health support, and is produced using a gentle process designed to retain its native triple helix structure19 and preserve its biological activity. A small amount of undenatured collagen (40 mg/day) has been shown to induce a process known as oral tolerance that engages the immune system in repairing joint cartilage and reducing arthritis symptoms20. Undenatured collagen preserves glycosylated antigenic regions, which are recognized by the T-cells18. When undenatured collagen is administered orally, it interacts with Peyer’s patches in the gut and activates immune cells, transforming naive T-cells into T regulatory (Treg) cells that specifically recognize type II collagen18, 20, 21. Although many animal22,23,24,25 and human18, 26, 27 studies have demonstrated the beneficial effect and possible molecular mechanism of low-dose undenatured collagen administration on OA, the dose–response effect of undenatured collagen in different age groups is still unclear. Understanding the effect of different doses of undenatured collagen on OA may contribute to treatment recommendations for age- or injury-related OA in humans and provide supportive information for animals prone to joint disorders.
The data on the use of different doses of undenatured collagen in the treatment of OA is limited. It has been reported that different amounts of undenatured collagen may have differing pharmacological effects, especially on oral tolerance mechanisms19, 28. It has previously been shown that high doses of undenatured collagen (daily 480 and 640 mg) are more effective than lower doses (daily 80 mg) in eliminating clinical arthritis symptoms in horses29. However, these studies lacked systemic and molecular evaluation of various low doses of undenatured collagen within different age groups for OA. Therefore, we aimed to compare the efficacy of different doses of undenatured collagen in MIA-induced knee OA in young and old rats.
Materials and methods
Animals
All procedures were conducted in compliance with the ARRIVE guidelinesThey were conducted in strict compliance with the relevant laws, the Animal Welfare Act, the Public Health Services Policy, and guidelines established by the Institutional Animal Care and Use Committee of the Institute and the European Union guidelines (No. 2010/63/EU) for the protection of the laboratory animals used for scientific purposes. The experimental procedures were approved by the Animal Experiments Local Ethics Committee of Bingol University (20-04/01-02). All efforts were made to minimize animal suffering and the number of animals used. Rats were maintained under standard environmental conditions (a temperature of 22 ± 2 °C, 12 h light-12 h dark cycle, and 55% ± 3% humidity) in propylene cages (47 × 37 × 19 cm, three or four rats per cage) with ad libitum water and food.
A total of 70 female Wistar albino rats (35 young rats, eight weeks old, weighing 170 ± 20 g; 35 old rats, eighteen months old, weighing 340 ± 20 g) were obtained from the Bingol University Experimental Research Center. We chose female rats for this model because humoral and cellular immune responses to antigenic stimulation are more pronounced in females, and testosterone has an anti-inflammatory effect on arthritis. Therefore, the susceptibility of female rats to experimental arthritis is higher than male rats30.
Experimental design
After a week of acclimatization period, both young and old animals were divided into five groups, with seven animals in each group (Fig. 1): (1) control (saline-treated); (2) MIA (a single intra-articular injection of MIA); (3) MIA + UC 0.66 (0.66 mg/kg undenatured collagen-treated); (4) MIA + UC 1.33 (1.33 mg/kg undenatured collagen-treated); (5) MIA + UC 2 (2 mg/kg undenatured collagen-treated). Undenatured collagen doses were determined based on the human equivalent dose (HED) used in previous clinical studies31. HED doses (40, 80, and 120 mg/day) were converted to rat doses (0.66, 1.33, and 2 mg/kg), according to Shin et al.32. The UC-II undenatured type II collagen was obtained from Lonza Greenwood LLC. It is a powdered, glycosylated, and shelf-resistant component (Batch no:20GW246506). The product contains > 3% undenaturated type 2 collagen and > 25% total collagen. Normal saline (1 mL) was used as a vehicle for three undenatured collagen doses. Also, MIA rats received 1 mL of normal saline daily. Rats were dosed once daily with undenatured collagen by gastric gavage for 37 days, and OA was induced on the seventh day after initiation of undenatured collagen supplementation. Initially, rats were anesthetized using xylazine (10 mg/kg) and ketamine hydrochloride (50 mg/kg). Then the right knee of all rats was shaved for injection and disinfected with 70% alcohol. 1 mg of MIA (Sigma, St. Louis, USA) was dissolved in 50 μL sterile saline and injected into the right knee joint cavity through the infrapatellar ligament with a 29-G needle to induce knee OA33. In addition, 50 μL saline was injected into the right knee joint of the control rats.
At the end of the undenatured collagen supplementation period (37th day), rats were weighed and sacrificed by decapitation under anesthesia (10 mg/kg xylazine and 50 mg/kg ketamine hydrochloride). Blood and articular cartilage samples were quickly removed. The right knee joints of animals were removed from the muscle tissue. Blood samples were centrifuged (2000 g for 10 min), and serum samples were collected into microtubes. Serum and articular cartilage samples were stored at − 80 °C for further analysis.
Gait test
The ink print method was used for the gait test23. The hind paws of each rat were dipped in black ink briefly, and then rats walked on a sheet of white paper (60 cm × 7 cm). The gait test was performed for each rat on the 3rd, 7th, 14th, and 28th days after the MIA injection. The white paper was scanned and transferred to a computer. Paw area (cm2), stride length (cm), and pad width (cm) were measured with Image J software (National Institutes of Health, USA). The size of the area around the right hind paw was defined as the paw area (cm2), the distance of the same right hind paw between two steps as stride length (cm), and the distance between the first and fifth toes of the right hind paw as pad width (cm). The arithmetic means of at least three measurements of paw areas, stride length, and pad width were considered for each rat.
Radiographic assessment and knee diameter measurement
For assessing the knee joint osteoarthritic deterioration, X-ray radiography of each animal’s right knee joint was taken immediately after dissection (37th day), and the Kellgren-Lawrence scoring system (grade 0: none, grade 1: doubtful, grade 2: minimal, grade 3: moderate, and grade 4: severe joint deformation) was used for radiographic assessment34. Radiographs were examined by a radiologist blinded to the groups during the entire study period. The mediolateral diameter (mm) of the right knee joint was measured at least three times with a digital caliper (Mitutoyo, Kawasaki, Japan) to assess joint swelling before dissection (37th day).
Histopathological analysis and Mankin classification
First, a portion of the right knee joint of the rats was stored in a formalin solution (10%) for several days. Next, joint cartilage samples were stored in a nitric acid solution (10%) for 30 days to decalcify the inorganic matter. Then, joint cartilage samples were blocked in paraffin and sectioned as 4-µm thick. Finally, the slides were stained with hematoxylin–eosin (H.E.), and the Mankin scoring system (Structure; score 0: smooth intact surface, score 1: slight surface irregularities, score 2: pannus/surface fibrillation, score 3: clefts into the transitional zone, score 4: clefts into the radial zone, score 5: clefts into the calcified zone, and score 6: total disorganization. Cells; score 0: uniform cell distribution, score 1: diffuse cell proliferation, score 2: cell clustering, and score 3: cell loss. Tidemark integrity; score 0: intact and score 1: vascularity) was used for the histopathological assessment of knee joint cartilage35. Tissue sections were assessed under a light microscope (LM) for the pathological features of LM by an experienced histopathologist blinded to the study groups during the entire study period.
Analyses of serum markers
A microplate reader (Elx-800, Bio-Tek Instruments Inc, Vermont, USA) was used to determine serum levels of IL-1β (catalog no: MBS2023030, intra- and inter CV was < 10% and < 12%), IL-6 (catalog no: MBS2701082, intra- and inter CV was < 10% and < 12%), TNF-α (catalog no: MBS2088120, intra- and inter CV was < 10% and < 12%), cartilage oligomeric matrix protein (COMP, catalog no: MBS267386, intra- and inter CV was < 8% and < 12%), c-reactive protein (CRP, catalog no: MBS2702539, intra- and inter CV was < 10% and < 12%), and prostaglandin E2 (PGE2, catalog no: MBS262150, intra- and inter CV was < 8% and < 12%) with rat specific enzyme-linked immunosorbent assay (ELISA) kits according to the manufacturer's procedure (MyBioSource, Inc. San Diego, CA, USA). The lower limit of variation of IL-1β, IL-6, TNF-α, COMP, CRP, and PGE2 was 15.6 pg/mL, 7.8 pg/mL, 15.6 pg/ml, 3.12 ng/mL, 0.78 ng/mL, and 15.6 pg/mL, respectively.
Western blot analysis
The levels of IL-1β, IL-6, IL-10, TNF-α, cyclooxygenase-2 (COX2), NF-κB, collagen type 2, matrix metalloproteinase-3 (MMP3), COMP, and TGF-β in joint cartilage were determined by Western Blot method23. Joint cartilage tissues of each group were pooled and homogenized with a lysis buffer containing a protease inhibitor cocktail. The protein density of homogenates was measured by Qubit 2.0 Fluorometer (Invitrogen, Life Technologies Corporation, Carlsbad, CA, USA). A total of 20 µg of protein for each group was separated by sodium dodecyl sulfate–polyacrylamide gel electrophoresis (SDS-PAGE) and then transferred into a 0.45 µm nitrocellulose membrane (GVS, Bologna, Italy). The membrane was blocked for 1 h with 5% bovine serum albumin. Next, the membranes were incubated overnight at 4 °C with diluted (1:1000) primary antibodies (Santa Cruz Bio., IL-1β; sc-52012, IL-6; sc-57315, IL-10; sc-365858, TNF-α; sc-52746, NF- κB; sc-8008, MMP3; sc-21732, COMP; sc-374660, and Abcam COX2; ab283593, collagen type 2; ab34712, TGF-β; ab215715). Then, the membranes were treated with goat anti-mouse (Santa Cruz Bio., sc-2005) and goat anti-rabbit secondary antibodies (Abcam, ab205718). Diaminobenzidine substrate was used to visualize the interaction between primary and secondary antibodies. Bands were analyzed densitometrically using the Image J software (National Institute of Health, Bethesda, USA). β-actin (Sigma Aldrich, MA1-140) was used to check protein loading. Blots were repeated three times to confirm the reliability of the results.
Statistical analysis
A power analysis was performed using G*Power (Version 3.1.9.4) software to determine the sample size. For both age groups, the sample size was computed as seven rats per treatment group (0.05 type I error, 0.8 effect size, and a power of 90%). Data were presented as the mean ± standard error of the mean or box‐and‐whisker plots (with min and max values). SPSS software version 22.0 (IBM Corp., Armonk, NY, USA) was used for all statistical analyses. Shapiro–Wilk and Levene's tests were performed to analyze the normality of the data and the homogeneity of the variances, respectively. One-way ANOVA and Tukey post hoc tests were used for the parametric data, while the Kruskal–Wallis and Mann–Whitney tests were used for non-parametric data. p < 0.05 level was considered statistically significant.
Ethical statement
The experimental procedures were approved by The Animal Experiments Local Ethics Committee of Bingol University (2020/04-04/01-02). The animal experiment was designed and reported according to the ARRIVE guidelines.
Results
Gait test
The gait test was performed on the 3rd, 7th, 14th, and 28th day post-MIA injection. As demonstrated in Fig. 2, intra-articular MIA injection impaired gait patterns compared to healthy controls in both young and old rats (Fig. 2a–f). At day seven, the gait patterns were reduced in young rats (p < 0.05 for paw area,p < 0.01 for stride length, and p < 0.0001 for pad width), whereas no statistical difference was detected in old rats (p > 0.05). At days 14 and 28 after OA-induction, gait patterns were reduced compared to the control group in young and old rats (p < 0.0001, for all). In young and old rats, 1.33 mg/kg and 2 mg/kg of undenatured collagen supplementation increased paw area and stride length as early as 14 days post-OA induction. In addition, while the 0.66 mg/kg dose improved paw area and pad width in old rats, the younger group also showed an increase, but it was not statistically significant. At day 14 in both age groups, stride length alone did not improve with 0.66 mg/kg undenatured collagen supplementation compared to MIA rats (p > 0.05). At the same time point, supplementation of 2 mg/kg of undenatured collagen increased paw area compared to 0.66 mg/kg in young and old rats (p < 0.01). Also, stride length (p < 0.05) and pad width (p < 0.01) was markedly improved by 2 mg/kg undenatured collagen compared to 0.66 mg/kg in old rats. At day 28, all doses of undenatured collagen supplementation improved all gait measurements in old rats; however, this improvement was not statistically signficant with the lower dose (0.66 mg/kg) in young rats (p > 0.05). The 2 mg/kg undenatured collagen supplementation was more effective than the 0.66 mg/kg dose in improving gait measurements in both age groups (young rats: p < 0.01 for paw area, p < 0.0001 for stride length; old rats: p < 0.001 for paw area and stride length, p < 0.01 for pad width).
Kellgren-Lawrence score and knee diameter
At the end of the study (37th day), Kellgren-Lawrence scoring system was used to assess the severity of knee OA. MIA injection led to structural joint changes by increasing the Kellgren-Lawrence score and the joint diameter in both young and old rats, as seen in Fig. 3 (p < 0.0001). In young rats, all doses of undenatured collagen reduced the Kellgren-Lawrence score compared with MIA rats (p < 0.05 for 0.66 mg/kg and p < 0.01 for 1.33 mg/kg and 2 mg/kg). In old rats, compared with MIA rats, a significant improvement in the Kellgren-Lawrence score was achieved with the 1.66 mg/kg and 2 mg/kg doses (p < 0.01), however the lower dose of 0.66 mg/kg could not significantly reduce the score (p > 0.05).
As expected, joint diameter was higher in MIA rats compared with control rats (Fig. 3d , p < 0.0001). All doses of undenatured collagen reduced joint swelling in young and old rats compared with MIA rats (p < 0.0001). For young rats, 2 mg/kg undenatured collagen supplementation was more effective in reducing joint swelling than 0.66 mg/kg (p < 0.01). In contrast, no significant difference between undenatured collagen groups was found in older rats (p > 0.05).
Histopathological analysis and Mankin score
The articular cartilage surface was smooth, and the chondrocyte distribution was uniform in the control group in both age groups (Fig. 4a and c, respectively). As predicted, intra-articular MIA injection altered the histological structure of joint cartilage by damaging the cartilage surfaces and reducing the number of chondrocytes in the cartilage tissue. In both age groups, as shown in Fig. 4, higher doses of undenatured collagen (1.33 and 2 mg/kg) attenuated the histopathological manifestations and decreased the Mankin score compared with the MIA rats (p < 0.05 for 1.33 mg/kg; p < 0.01 for 2 mg/kg; for both age groups). Young rats administered 2 mg/kg undenatured collagen had lower Mankin scores than young rats administered 0.66 mg/kg undenatured collagen dose (p < 0.01). Old rats administered 2 mg/kg undenatured collagen had lower Mankin scores than old rats administered 0.66 (p < 0.01) and 1.33 mg/kg (p < 0.05) undenatured collagen doses.
Serum markers
To explore the anti-inflammatory function of undenatured collagen supplementation and its effect on cartilage markers, serum levels of IL-1β, IL-6, TNF-α, COMP, CRP, and PGE2 were measured. MIA-induced OA increased all measured inflammatory markers in young and old rats (p < 0.0001, Fig. 5a–f). In young rats, all doses of undenatured collagen markedly suppressed the serum levels of IL-1β, IL-6, CRP, PGE2 (p < 0.0001, for all), TNF-α (p < 0.001 for MIA vs. MIA + UC 0.66, and p < 0.0001 for other comparisons), and COMP (p < 0.05 for MIA vs. MIA + UC 0.66 mg/kg, and p < 0.0001 for other comparisons) compared with the MIA group. The results also indicated a dose–response effect for CRP and IL-6 levels. In old rats, undenatured collagen markedly suppressed the serum IL-1β, IL-6, PGE2, TNF-α, and COMP levels in a dose-dependent manner (Fig. 5). Overall, 2 mg/kg of undenatured collagen was more effective than 0.66 mg/kg in reducing all inflammatory markers in both age groups.
Western blot analysis
MIA-induced knee OA caused inflammation as indicated by elevated expression levels of IL-1β, IL-6, IL-10, TNF-α (Fig. 6a–d), COX-2, NF-κB, MMP-3, and COMP (Fig. 7a–e) proteins in the knee joint cartilage of both young and old rats (p < 0.0001). Additionally, knee joint CTX-II and TGF-β levels were lowered in the MIA rats of both age groups (p < 0.0001). We found that undenatured collagen treatment ameliorated the expression of most inflammatory cytokines in a dose-dependent manner in both young and old rats (Fig. 6 and Fig. 7, p < 0.001). More specifically, the protein level of NF-κB, MMP3, and COMP in the knee joint was reduced in a dose-dependent manner by undenatured collagen compared with the MIA group (Fig. 7b, d and e, p< 0.001). In young rats, knee joint CTXII and TGF-β proteins were significantly improved with the 2 mg/kg dose vs. The 0.66 mg/kg dose (p < 0.001). On the other hand, in the old age group, there was a dose-dependent effect of undenatured collagen for these markers (p < 0.0001 for Collagen type 2 and p < 0.01 for TGF-β). We also found that 1.33 and 2 mg/kg undenatured collagen similarly reduced knee joint protein levels of IL-10, IL-6, TNF-α, and COX2 in young rats (p > 0.05), while in the old age group, we observed a dose-dependent effect for most of these markers.
Discussion
Many animal22,23,24,25 and human18, 26, 27 studies have demonstrated a beneficial effect of undenatured collagen administration on OA; however, the effects of undenatured collagen in different doses and age groups have not been investigated. The present study is the first to compare the efficacy of different doses of undenatured collagen on MIA-induced OA in young and old rats. MIA injection has been shown to inhibit glyceraldehyde-3-phosphatase and lead to chondrocyte deaths36, 37, causing cartilage degeneration, joint space narrowing, and subchondral bone deformation in joint cartilage38. Radiographic and histopathological findings in response to MIA injection in both age groups agree with that reported by Orhan et al.39. Our data also show that intra-articular MIA injection exacerbates inflammatory status regardless of age in rats, as indicated by Ogbonna et al.40 and Ro et al.17. In addition, we demonstrated for the first time that in young and old rats, undenatured collagen (particularly 1.33 and 2 mg/kg) prevented the progression of OA by reducing markers of joint cartilage breakdown and knee swelling, improving most gait measurements, and reducing the production of inflammatory cytokines. It should be noted that previous studies have reported an oral tolerance mechanism for undenatured collagen during arthritic cartilage destruction18,20,22,23,24,,23,41, and acute inflammatory events, in healthy subjects. For this study, we chose to focus on the effect of undenatured collagen in MIA-induced OA rats.
Based on the Kellgren-Lawrence score, MIA-injected rats had moderate OA (approximately up to grade 3), and undenatured collagen reduced OA severity (approximately to grade 1) in young rats at all doses and in old rats at 1.33 and 2 mg/kg This effect was probably linked to preventing inflammation-related subchondral bone deformation by undenatured collagen23. The collagen type 2-specific oral tolerance mechanism mediated by undenatured collagen can increase anti-inflammatory cytokines in joint tissue, thereby promoting the production of the articular cartilage matrix by chondrocytes42. Also, undenatured collagen contains cartilage matrix amino acids necessary for synthesizing and repairing connective tissue42. Because aging exacerbates the inflammatory state43 and potentially suppresses oral tolerance44, higher doses of undenatured collagen may be required to show better efficacy in arthritic old rats. On the other hand, inflammatory responses43, oral tolerance44, and cartilage-repairing activities can be more active in early life45. Therefore, in young rats, undenatured collagen administration prevented joint deformities, as reported in our previous study23, probably through the stimulation of oral tolerance.
Intra-articular MIA injection can increase ROS levels that cause chondrocyte death and trigger cartilage deformation, and elevate articular IL-1β, IL-6, COX246, TNF-α, and NF-κB levels23, while reducing TGF-β levels in rats8. We found that undenatured collagen supplementation decreased most inflammatory cytokine activity, cartilage degradation markers (including MMP3 and COMP), and joint swelling used for joint inflammation monitoring in a dose-dependent manner. The dose-dependent functionality of undenatured collagen might have been linked to the oral tolerance mechanism that depends on age status44 and antigen dose47. The activity of oral tolerance is suppressed by aging due to the loss of functionality of Peyer’s patches and the reduction in regulatory cytokines and T-cells48. Consequently, the stimulability of oral tolerance may be reduced due to decreased susceptibility to oral antigen induction during aging48. On the other hand, a very high dose of oral antigen intake may deteriorate the oral tolerance mechanism by inactivating T-cells, while low doses stimulate the oral tolerance to produce Treg cells49. Our observed findings indicate that the higher doses of undenatured collagen used in this study (1.33 mg/kg and 2 mg/kg) were still below the level to deteriorate oral tolerance in both young and old rats.
COMP, a non-collagenous glycoprotein, is produced by articular chondrocytes to regulate matrix organization in cartilage50. The increased COMP levels in the serum and joint are considered diagnostic and prognostic OA biomarkers51. Similarly, MMP3, responsible for the degradation of the cartilage matrix by accelerating collagen type 2 degradation52, could be used as a biomarker for knee osteoarthritis53. The stimulation of NF-κB can exacerbate inflammatory processes and the production of joint MMP354 and elevate TNF-α related serum COMP levels55. We showed that MIA-induced inflammation increased joint COMP and MMP3 levels regardless of age stage. The present findings also showed that undenatured collagen administration reduced NF-κB in the joint cartilage, owing to its anti-inflammatory function23; thus, undenatured collagen may have contributed to suppressing NF-κB-related COMP and MMP3 activity.
TGF-β plays a crucial role in the oral tolerance response by stimulating CD4+ Treg cells56. Undenatured collagen drives collagen type 2 specific Treg cell production in Peyer’s patches20. Tregs secrete anti-inflammatory cytokines, particularly TGF-β57, and together prevent autoimmune cartilage destruction in joint cartilage via recognizing specific self-antigens such as type 2 collagen20. Our findings in young rats showed that the 0.66 mg/kg and 1.33 mg/kg undenatured collagen doses similarly affected the protein expression of joint TGF-β and collagen type 2, while the 2 mg/kg dose showed the best efficacy. This could be attributed to the oral tolerance mechanism being more active in early life58. TGF-β stimulatory activity of undenatured collagen-stimulated Treg cells may have partially contributed to chondrocytes survival for cartilage repair59. Aging decreases anabolic factors and stimulates catabolic and inflammatory activity in chondrocytes60. This age-related catabolic activity probably led to a dose-dependent alteration impacting TGF-β and collagen type 2 levels in old rats. TGF-β is a key regulator of collagen type 2 expression in chondrocytes, but aging may dampen this regulatory activity59 because chondrocytes become less sensitive to TGF-β-stimulated proliferative activity60. Taken together, we can assume that the efficiency of the same dose of undenatured collagen may decline with age due to the loss of oral tolerance functionality44.
Irregularity in the articular surface is one of the main findings of OA that originated from the degradation of the collagen matrix and cartilage damage19. The anti-inflammatory and collagen type 2 stimulating activity of undenatured collagen may help cartilage regeneration against MIA-induced OA22, 23. Bagi et al.24 demonstrated that a low dose of 40 mg HED of undenatured collagen for 8 weeks could prevent cartilage damage in rats in a different OA model induced by partial medial meniscectomy tear. In the present study, according to Mankin scores, only 1.33 and 2 mg/kg undenatured collagen (equivalent to 80 and 120 mg HED) administration attenuated cartilage degradation in young and old rats. The difference between Bagi et al.24 and our study may have stemmed from the OA induction method and the longer duration of undenatured collagen administration. Previously we reported that a 40 mg HED dose could not reduce the Mankin score in MIA rats23 as in the present study. This could be because higher doses of undenatured collagen were required to alleviate cartilage damage by regenerating the cartilage microstructure in rats.
Previous studies show that OA treatment using undenatured collagen alleviates joint pain and improves quality of life27. Although a low dose of undenatured collagen did not effectively attenuate joint cartilage damage in old rats, the present findings show that all doses of undenatured collagen supplementation reduced knee swelling and improved gait patterns, closely related to pressure pain thresholds. These results are probably related to decreased pain sensitivity and increased pain threshold parallel to ageig61.
Supplementation with the different doses of undenatured collagen used in this study appears to be safe. We did not observe any changes in body weight, serum glucose, BUN, creatine, ALT, and AST levels in young or old rats (Supplementary Table 1). The MIA-induced OA model is less severe regarding the pain phenotype and adverse effects on animal welfare62. Therefore, there was no worsening of body conditions due to the MIA injection, and knee joint swelling severity was not enough to affect the well-being of MIA rats. In addition, we did not detect any pathomorphological, hematological, or biochemical changes after different doses of undenatured collagen. Similar observations with 0.66 mg/kg of undenatured collagen have beenreported in previous studies22, 23, 63, 64.
This study presents several limitations. First, the influence of hormonal effect during aging needed to be considered, especially since estrogen levels regulate changes in OA by preventing degradation of the extracellular matrix65. In this study, we were unable to evaluate the difference in the development of osteoarthritis caused by varied estrogen levels in young and aged rats. In addition, the effect of anti-inflammatory and joint health-promoting activity of undenatured collagen on healthy animals should be clarified. Lastly, the exact mechanism of action of undenatured collagen in OA is still lacking, and additional mechanistic studies are needed to achieve greater understanding of the ingredient.
Conclusion
In the current study, we showed for the first time the activity of various doses of undenatured collagen in reducing OA symptoms in young and old rats. We concluded that while the lower dose of undenatured collagen (0.66 mg/kg) partially ameliorates MIA-induced OA symptoms, and protects the joint structure in rats, higher doses work faster and are more efficacious in improving overall joint health. Also, this preliminary data indicated that lower doses of undenatured collagen might help treat either injury- or age-related OA in different age categories in rats. However, there is a need for comprehensive clinical studies in humans or animals with OA to support our present findings.
Data availability
Correspondence and requests for materials should be addressed to K. Sahin.
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Acknowledgements
The authors would like to thank Vijaya Juturu for her contribution to the study design and management of the study.
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This project was funded by Lonza Greenwood LLC (SC, USA) and the Turkish Academy of Sciences (TUBA, KS) in part. The funders were not involved in the project design, collection, analysis, and interpretation of data, the writing of this article, or the decision to submit it for publication.
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K.S. and Z.S. supervised and conceived the study. K.S. and E.S. wrote the draft manuscript. C.O., E.S., and F.E. conducted formal analysis and investigation. E.S. and C.O. performed data curation, statistical analysis, and visualization. K.S., E.K.A., Z.S., S.D. reviewed and edited the manuscript. All the authors read and approved the final manuscript.
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Z.S., S.D., and E.K.A. are employees of Lonza Greenwood LLC (Greenwood, NC, USA). The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
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Sahin, E., Orhan, C., Erten, F. et al. The effect of oral administration of undenatured type II collagen on monosodium iodoacetate-induced osteoarthritis in young and old rats. Sci Rep 13, 6499 (2023). https://doi.org/10.1038/s41598-023-33763-2
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DOI: https://doi.org/10.1038/s41598-023-33763-2
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