CTS was added to an acetic acid solution (No. A6283, 0.1 M, Sigma) under mild stirring for complete dissolution. The supernatant was collected and purified by passing through 0.22-μm filters. Its pH was adjusted to 7.0 using NaOH solution (No. S5881, 1 M, Sigma). Afterward, the final concentration of the CTS solution was adjusted to 5 w/v% using centrifugal filters (3 kDa MWCO). Subsequently, β-GP (G9422, Sigma) was used as a physical crosslinker. β-GP was first dissolved in Milli-Q water to achieve 12 wt%. Then, it was added to the CTS solution to prepare a thermosensitive CTS hydrogel precursor solution.

In addition, ICA (No. I1286, purity ≥94%, Sigma) was dissolved in dimethylsulfoxide (No. 472301, Sigma) at 20 mM, and the derived solution was added to the prepared CTS (hydrogel precursor solution) till a final concentration of 10 μg/ml was achieved. Finally, a thermosensitive ICA/CTS hydrogels precursor solution was formed. Both CTS and ICA/CTS hydrogel precursor solutions were incubated at 37°C for complete gelation if necessary.

The pristine ICA and CTS, as well as the gelated ICA/CTS hydrogel, were analyzed using an ATR–FTIR (model-Alpha, Bruker, Germany) spectrometer with a scanning range from 1000 to 4,000 cm⁻¹ at ambient temperature.

To test the in vitro release of ICA from the ICA/CTS hydrogel, gelated ICA/CTS hydrogel was immersed in 10 ml of high-glucose Dulbecco’s Modified Eagle Medium (DMEM, No. D5030, Sigma) supplemented with 10% fetal bovine serum (FBS, No. 12103C, Sigma) and incubated under 5% CO₂ at 37°C for 6 weeks. The medium was refreshed weekly. Samples were collected from the medium every week and dried. The dried samples were immersed in 10 ml of ethanol, exposed to ultrasonic vibration for 1 h, and incubated for two more days. The ICA/ethanol concentration was measured at 270 nm.

The initial weight of the lyophilized CTS and ICA/CTS hydrogels was considered as M₀. The gel was immersed in PBS (pH = 7.4) and incubated in an environment with 5% CO₂ at 37°C for 6 weeks. The samples were taken out of PBS every week, dried, and weighed again as M_n. The degradation rate was calculated as (M₀—M_n)/M₀ × 100%.

The rheological properties of the ICA/CTS and CTS hydrogels were evaluated using a controlled stress rheometer (HAAKE Rheo Stress 6000, Thermo Scientific, Germany) with parallel-plate (25 mm diameter) geometry at room temperature. The rheometer was further connected with a temperature-controlled water bath to test the dynamic storage modulus (G′) of hydrogels.

The initial gelated CTS and ICA/CTS hydrogels were fabricated in a cubic shape (1×1×1 cm³), and their volume was considered to be V₀. Thereafter, the hydrogels were immersed in PBS (pH = 7.4) and incubated in an environment with 5% CO₂ at 37°C for 60 h. The samples were taken out of PBS every 20 h, and their volumes were measured and denoted as V_n. The swelling ratio was calculated as follows: V_n/V₀ × 100%.

RAW264.7 macrophages (Saimofei, China) were pre-treated with 1 μg/ml lipopolysaccharide (LPS, No. SMB00610, Sigma) for 24 h. The pre-treated RAW264.7 macrophages were inoculated into ICA alone, and ICA/CTS and CTS hydrogel precursor solutions at a density of 5.0 × 10⁴ cells/mL. Thereafter, 2 ml of macrophage-loaded hydrogel was incubated at 37°C for complete gelation and cultured in high-glucose DMEM supplemented with 5% FBS at 37°C in 5% CO₂. After 24 h, samples from the two groups were collected for western blot (WB) analysis and real-time polymerase chain reaction (RT-PCR).

For WB examination, total protein extracts were prepared from samples using RIPA buffer (KeyGen, China). Protein samples were separated by SDS-PAGE, transferred to PVDF membranes, and blocked with 5% bovine serum albumin. Subsequently, PVDF membranes were covered with primary antibodies as probes against inflammation-related proteins, including interleukin 6 (IL-6) (1:1000, No. sc-57315, Santa Cruz Biotechnology, Inc.), tumor necrosis factor alpha (TNF-α) (1:1000, No. sc-12744, Santa Cruz Biotechnology, Inc.), and GAPDH antibodies (1:10,000, No. ab8245, Abcam). After the HRP-conjugated goat anti-rabbit/mouse IgG antibody (1:10,000, No. AS1110, Aspen Biotech, Shanghai, China) was applied, the bands formed were visualized using an ECL kit (No. AS1059-3, Aspen Biotech, Shanghai, China), and their intensity was analyzed using the Band-Scan software. The acquired images were further analyzed using the ImageJ software to quantify relative expression levels.

The expression levels of inflammation-related genes were further analyzed by RT-PCR. Total RNA extraction was performed using TRIzol™ reagent (No. 46301, Invitrogen). cDNA synthesis was performed using Moloney murine leukemia virus reverse transcriptase (No. QR0100, Invitrogen). Quantification was performed using RT-PCR with the primers (listed in Table 1) and a Fast Synergy Brands Green Master Kit and Light Cycler 480 System (Roche) according to the manufacturer’s instructions. The comparative threshold cycle method was used to analyze the results, and the expression of the endogenous reference gene GAPDH was used for their normalization.

The ethical approval required for this study was obtained from the Xuchang Central Hospital Ethics Committee. A 2–3-month-old goat was purchased from Shanghai Jiagan Experimental Animal Raising Farm (Shanghai, China). The auricular cartilage of the goat was collected and fragmented into 1 × 1 mm² pieces. Following this, the cartilage was digested with 0.2% collagenase NB4 (No.17454, SERVA, Germany) for 8 h at 37°C on a shaker. Singularized chondrocytes were collected and cultured in high-glucose DMEM supplemented with 10% FBS and 1% antibiotic–antimycotic (AA). Cells were passaged at >80% confluence. Finally, cells at their second passage (P2) were harvested for further application.

To determine the biocompatibility of ICA/CTS and CTS hydrogels, chondrocytes were evenly mixed with ICA, and the ICA/CTS and CTS precursor solutions. The final concentration was adjusted to 5.0 × 10⁵ cells/mL. This cell concentration was suitable for complete gelation after temperature enhancement to 37°C. Thereafter, the chondrocyte-loaded hydrogels were cultured in vitro in DMEM supplemented with 10% FBS/1% AA for 7 days. After 1, 4, and 7 days, the cell viability in the hydrogels was measured using a live/dead cell viability assay (No. 34862, Invitrogen) and measured using a confocal microscope (Nikon, Japan). ImageJ was used to quantitatively analyze the number of live cells from the acquired images. The cell proliferation levels in the samples were evaluated by measuring the absorbance of a cell counting kit-8 reagent (CCK-8, No. C0040, Beyotime, Shanghai, China) at 450 nm.

Chondrocytes were homogenously mixed within ICA/CTS and CTS hydrogel precursor solutions (1 × 10⁷ cells/mL) and gelated at 37°C. The cell suspensions were cultured in DMEM supplemented with 10% FBS/1% AA at 37°C in 5% CO₂. After 2 weeks of cultivation, samples from the ICA/CTS and CTS groups were retrieved for histological and biochemical evaluations.

For histological assessment, the specimens were fixed, decalcified, paraffin-embedded, and cut into sections of 5 μm thickness. Samples were stained with hematoxylin-eosin (HE) for morphological evaluation. Safranin-O staining was used for assessing glycosaminoglycan (GAG) distribution. Finally, the cartilage-specific ECM was analyzed by immunohistochemical staining for collagen II.

In addition, cartilage-related biochemical components of the retrieved samples from the ICA/CTS and CTS groups were further estimated. Samples (n = 3) were collected and minced to quantify DNA, GAG, and type II collagen using the PicoGreen dsDNA assay (No. 10225ES84, Invitrogen), dimethyl methylene blue assay (Sigma), and Collagen II Detection Kit (No. 6009, Chondrex Inc. Redmond, WA, United States), respectively. The DNA, GAG, and collagen II contents were normalized to the tissue wet weight. In addition, GAG/DNA and collagen II/DNA data were also calculated.

After 2 weeks, the in vitro engineered cartilage from both ICA/CTS and CTS groups was subcutaneously implanted into the dorsal area of the autologous goat. At three- and 6-week post-implantation, samples were harvested for cartilage-related evaluation and inflammatory assessment.

For cartilage evaluation, samples were histologically stained using HE, Safranin-O, and immunohistochemical collagen II reagents. Additionally, GAG and collagen II were further evaluated as cartilage-related biochemical components, in which the GAG and collagen II contents were normalized to the tissue wet weight. Briefly, total GAG was precipitated using guanidinium chloride solution (0.98 mol/L). The OD values were determined at 595 nm after the GAG precipitate was dissolved. A standard curve was prepared using chondroitin-4-sulfate, and the total GAG content was measured from the OD value correlating to the corresponding GAG content in the standard curve. The total collagen content was quantified in the hydroxyproline assay. Samples were prepared by alkaline hydrolysis, and free hydroxyproline hydrolyzates were assayed. The hydroxyproline content was converted to the total collagen content according to a collagen to hydroxyproline mass ratio of 7.25.

The expression levels of the inflammatory cytokines interleukin 1β (IL-1β), IL-6, and TNF-α and an apoptosis-related marker (TUNEL) in the samples were analyzed by immunofluorescence staining. Samples were treated overnight with primary antibodies against collagen type II, IL-1β, IL-6, TNF-α, and TUNEL (No. ab188570, ab254360, ab303458, ab183218, and ab66108, Abcam) at 4°C. After rinsing, the samples were treated with goat anti-rabbit secondary antibody (1:1000, ab150077, Abcam) in dark. Finally, coverslips were mounted with 4′,6-diamidino-2-phenylindole (No. 10236276001, DAPI, Sigma) mounting solution, visualized using a fluorescent imaging system, and analyzed by a fluorescence microscope (Olympus). The acquired images were analyzed with ImageJ software to calculated the relative intensity as follows: M/N × 100%, where M is the occupied area of the positive expressed marker and N is the area of the total image.

Data were reported as mean value ±standard deviation (SD) and analyzed using SPSS version 17.0 software. Inter-group differences were analyzed by Student’s t-test. All experiments were performed in triplicate. p < 0.05 denoted a statistically significant difference.

To endow the CTS hydrogel with concurrent chondrogenesis and anti-inflammatory effect, ICA was loaded into the CTS hydrogel to prepare a composite ICA/CTS hydrogel. FTIR spectral data were used to confirm the chemical stability of ICA in the ICA/CTS hydrogel (Figure 1A). For pristine CTS samples, the characteristic peaks at 2872 and 1650 cm⁻¹ were attributed to the -C-H and carbonyl (-C-O) stretching vibrations of the secondary amide (amide I band), respectively. The characteristic peaks of ICA appeared at 2923, 1595, and 1259 cm⁻¹, corresponding to methylene (CH₂), benzene ring, and methoxyl (O–CH₃), respectively. Both the characteristic peaks of pristine CTS and ICA samples were observed in the ICA/CTS sample, indicating the successful preparation of the ICA/CTS hydrogel. Notably, the characteristic peak of ICA at 2921 cm⁻¹ appeared in the ICA/CTS hydrogel with no change, suggesting zero chemical change in ICA during ICA/CTS hydrogel production, which could have helped retain the original bioactivity of ICA.

We further conducted in vitro experiment to illustrate the release kinetics of ICA from the ICA/CTS hydrogel. Our data indicated that ICA presents sustained release kinetics from the ICA/CTS hydrogel when immersed in chondrocyte co-culture medium. Almost 100% percent of ICA was completely released from the ICA/CTS hydrogel at 6 weeks (Figure 1B). In addition, our data revealed that the degradation rate of CTS and ICA/CTS hydrogels exhibited a similar trend with the release kinetics of ICA (Figure 1C), suggesting that the addition of ICA did not affect the rate of CTS hydrogel degradation. Thus, the release kinetics of ICA could be governed by the degradation of CTS.

In addition, both ICA/CTS and CTS hydrogels exhibited similar shear-thinning, storage modulus (G′), and swelling ratio behaviors (Figures 1D–F), suggesting that the addition of ICA did not affect the rheological, gelation, and swelling properties of the CTS hydrogel. These results indicated that the ICA/CTS hydrogel retained the properties of original CTS hydrogel for use in cartilage regeneration.

To test the anti-inflammatory properties of the ICA/CTS hydrogel, RAW264.7 macrophages were pre-induced with LPS and incubated with ICA, ICA/CTS, and CTS hydrogels for 24 h. WB examination indicated a significant attenuation in the protein expression of all inflammatory cytokines (including IL-6 and TNF-α) in the ICA/CTS group compared to that in the CTS group (Figures 2A–D). RT-PCR examination further confirmed that all inflammatory protein-encoding genes (including IL-6 and TNF-α) were expressed at lower levels in the ICA/CTS group than in the CTS group (Figures 2E,F). Thus, the addition of ICA endowed the ICA/CTS hydrogel with pronounced anti-inflammatory properties. In addition, our data revealed that the expressions of both IL-6 and TNF-α in the ICA group was similar to that in the ICA/CTS group, suggesting that CTS fabrication does not affect the anti-inflammatory potential of ICA.

The cytocompatibility of ICA/CTS was evaluated in vitro by co-culture with chondrocytes for 7 days. Live/dead staining revealed an increasing trend of cell number with increased incubation time from 1 to 7 days in the ICA, ICA/CTS, and CTS groups (Figures 3A,B). Scarcely dead cells were observed in both groups, indicated by the negligible number of red-stained cells. Notably, cell number were greater in the ICA and ICA/CTS groups than in the CTS group. In addition, phalloidin staining revealed that the ICA group had greater F-actin expression and stretching than both ICA/CTS and CTS groups, suggesting that the chondrocytes changed their morphology in response to hydrogel treatment (c). Consistent with the above results, the OD values determined from the CCK-8 assay were elevated with the increase in culture duration, and the OD values in the ICA and ICA/CTS groups were greater than those in the CTS hydrogel (Figure 3D). The results indicated that both the ICA/CTS and CTS hydrogels were highly cytocompatible, and that the addition of ICA significantly promoted chondrocyte proliferation.

Both ICA/CTS and CTS hydrogels colonized with chondrocytes and were subjected to culture for 2 weeks to verify the in vitro chondrogenesis potential. According to our positive results from safranin-O and immunohistochemical collagen II staining methods, samples in both ICA/CTS and CTS hydrogels displayed apparent cartilage-specific ECM deposition (Figure 4A). Of note, both safranin-O and collagen II staining test results indicated more intensive staining in ICA/CTS hydrogel samples than in CTS hydrogel samples. In addition, the quantitative analyses of cartilage-related biochemical components, including DNA, GAG, GAG/DNA, collagen II, and collagen II/DNA, showed an obvious increasing trend in the ICA/CTS hydrogel than in the CTS hydrogel (Figures 4B–F). Notably, the higher GAG/DNA and collagen II/DNA levels in the ICA/CTS group than in the CTS group suggested that the ICA/CTS hydrogel contributed to greater chondrogenic ECM production but not owing to a larger chondrocyte population. The results suggested that both ICA/CTS and CTS hydrogels can be used for cartilage regeneration in vitro and ICA addition can promote significant chondrogenesis.

The in vitro regenerated cartilage samples from both ICA/CTS and CTS hydrogels were subcutaneously implanted in an autologous goat model and subject to in vivo incubation for 3 and 6 weeks to confirm the feasibility of cartilage formation in an immunocompetent large animal. Compared to CTS hydrogels, ICA/CTS hydrogel samples had more markable cartilage-specific ECM secretion and a typical lacuna-like structure at both weeks three and six post-implantation. This result was confirmed by both HE staining and the more intense safranin-O and collagen II staining methods (Figures 5A,B). Additionally, cartilage-specific ECM showed a declining trend, and a typical lacuna structure was observed for a long duration in samples from both ICA/CTS and CTS hydrogels. The above results were further confirmed by the quantitative analysis results of cartilage-related biochemical components. In these analyses, higher levels of GAG and collagen II were observed in the ICA/CTS group than in the CTS group, and lower levels were observed after a considerable duration (Figures 5C,D). The results indicated that the ICA/CTS hydrogel exhibited potential for subcutaneous cartilage regeneration in a goat, and the addition of ICA significantly promoted cartilage regeneration in an immunocompetent large animal model.

The cartilage tissue generated from ICA/CTS and CTS hydrogels was evaluated for inflammatory reactions to elucidate the mechanism of action of ICA in promoting cartilage regeneration in an immunocompetent large animal. More intensive immunofluorescence staining of all inflammation-related factors (IL-1β, IL-6, and TNF-α) and apoptosis-related marker (TUNEL) was observed with time over 3–6 weeks in both ICA/CTS and CTS hydrogels (Figures 6A–D). The immunofluorescence of IL-1β, IL-6, TNF-α, and TUNEL was attenuated in the ICA/CTS hydrogel compared to that in CTS hydrogel. Quantitative analyses further confirmed that the relative intensity of IL-1β, IL-6, TNF-α, and TUNEL was elevated with time over 3–6 weeks, and lower levels were observed in ICA/CTS hydrogels than in the CTS hydrogel (Figures 6E–H). Collectively, these results demonstrated that the addition of ICA endowed the ICA/CTS hydrogel with a pronounced anti-inflammatory property.