Preparation of Cholesterol-Modified Hyaluronic Acid Nanogel-Based Hydrogel and the Inflammatory Evaluation Using Macrophage-like Cells

Nanogels are candidate biomaterials for tissue engineering and drug delivery. In the present study, a cholesterol–hyaluronic acid hydrogel was developed, and the pro-inflammatory response of macrophages to the hydrogel was investigated to determine its use in biomedical applications. Hyaluronic acid modified with cholesterol (modification rate: 0–15%) and maleimide (Chol-HA) was synthesized. The Chol-HA nanogel was formed through self-assembly via hydrophobic cholesterol interactions in aqueous solution. The Chol-HA hydrogel was formed through chemical crosslinking of the Chol-HA nanogel via a Michael addition reaction between the maleimide and thiol groups of 4arm−PEGSH. We found that the Chol-HA hydrogels with 5, 10, and 15% cholesterol inhibited the pro-inflammatory response of HiBiT−THP−1 cells, suggesting that the cholesterol contributed to the macrophage response. Furthermore, Interleukin 4 (IL−4) encapsulated in the hydrogel of the Chol-HA nanogel enhanced the inhibition of the inflammatory response in HiBiT-THP-1 cells. These results provide useful insights into the biomedical applications of hydrogels.

Nanogels are three-dimensional hydrogel materials in the nanoscale size range formed via the chemical and physical crosslinking of polymer chains.Akiyoshi et al. first reported the preparation of cholesterol-modified pullulan (CHP) nano gels via self-assembly via hydrophobic cholesterol moieties [15].Owing to their ability to encapsulate proteins and Gels 2023, 9, 866 2 of 13 nucleic acids, CHP nanogels have been applied in drug delivery [16].Numerous substrates and methods have been employed in nanogel preparation [17,18].
Recently, nanogels with reactive moieties, such as acryloyl, carbonyl, amino, and thiol groups, have been synthesized, and nanogel-based hydrogels have been prepared by crosslinking reactive moieties [17].Moreover, the presence of nanogel domains in hydrogels makes them useful scaffolds for tissue engineering because the nanogels are expected to function in a chaperone-like manner [19]; that is, the proteins are trapped in the nanogel without aggregation and released in their native form [15].These scaffolds have been applied in bone and muscle regeneration [17].Bone morphogenetic protein-2 (BMP-2), incorporated into CHP-crosslinked hydrogels, promotes new bone formation in mice with bone defects, through BMP-2 stimulation.Also, HA-based nanogels have been prepared by introducing cholesterol moieties [20].In contrast to pullulan, the physical properties of HA-based nanogels can be modulated by increasing the degree of cholesterol substitution on the HA polysaccharide chain.By maintaining the cholesterol modifications within a specific range, the nanogels precipitate under physiological salt conditions, suggesting that they can serve as effective sustained DDS materials.Conversely, within a different range, stable nanoparticles are formed under physiological salt conditions, suggesting that they could be used in targeted delivery applications.Furthermore, they can improve the loading capacity of protein pharmaceuticals [20].
The temporal regulation of M1-like and M2-like macrophages is crucial for tissue regeneration.When using HA-based hydrogels, during early-and late-stage skeletal muscle injury in mice, M1-like macrophage depletion completely inhibited muscle regeneration, and M2-like macrophage depletion reduced the effect of tissue remodeling, respectively [21,22].However, the immune response and temporal macrophage polarization in response to nanogels and its hydrogels have not been fully investigated.Also, high-molecular-weight HA is highly viscous with poor injectability, rendering its application in in situ regeneration difficult.Furthermore, a limited number of drug delivery substrates are known to gel in situ while stably retaining cytokines.In this study, we synthesized HA derivatives modified with cholesterol and a maleimide moiety (Chol-HA) and prepared the hydrogel via chemical crosslinking of the Chol-HA nanogel.The physicochemical and biological properties of the Chol-HA hydrogels were investigated.
In particular, we focused on the macrophage response to the Chol-HA hydrogels in order to understand the immune response to the Chol-HA hydrogel and design the Chol-HA hydrogel for the wide application of HA-based hydrogels to DDS and tissue engineering.In addition, the effect of cholesterol derivative substitution on THP-1 cells, an immune cell type, adhesion to the hydrogel and secreted inflammatory cytokines was determined at a constant hyaluronan main-chain molecular weight.

Synthesis of Chol-HA
HA, with a molecular weight of 120 kDa, was used to synthesize Chol-HA from tetrabutylammonium hyaluronan (which was prepared as previously described [20]).Specifically, synthesis was achieved through the condensation of the cholesteryl-6-aminohexylcarbamate amine group with the HA carboxylic acid moiety, using DMT-MM.The structures of the synthesized maleimide-modified HA derivatives at different degrees of cholesterol derivative (1, 5, 10, and 15%) were confirmed via 1H NMR (Figure S1).A maleimidecharacteristic peak was also identified at 6.9 ppm, and the resulting degree of substitution was determined as 15 maleimide groups per 100 HA units.

Characterization of the Chol-HA Nanogel Using Dynamic Light Scattering (DLS)
The particle size associated with aggregation in solution was measured using DLS (Table 1).When dissolved in a phosphate-buffered solution (2 mg/mL, pH 7.4), Chol-HA self-aggregated into nanoparticles in water.The particle size decreased with an increase in Chol.The smallest particle size was observed at a Cholesterol moiety of 15%.Normally, Gels 2023, 9, 866 3 of 13 HA does not form nanoparticles; however, when modified with 15% maleimide, particles as small as 180 nm were formed.

Preparation of the Chol-HA Hydrogel
To prepare the hydrogels, Chol-HA nanogel and 4arm-PEGSH solutions were poured into a disk-shaped silicone rubber mold with a diameter of 6 mm and a depth of 3 mm, and then, incubated at 37 • C for 24 h. Figure 1 shows the formation of Chol-HA hydrogels at various cholesterol levels.Transparent hydrogels were obtained from all the Chol-HA samples.For the Chol-HA hydrogels with 0, 1, 5, 10% cholesterol, the gel shape was maintained when the silicone mold was removed.However, the Chol-HA hydrogel with 15% cholesterol deformed upon removal from the silicone mold.Figure 2 verifies the formation process of Chol-HA hydrogels using ATR-FTIR spectroscopy.A decrease in the peak at 1695 cm −1 derived from maleimide, and the disappearance of the peak at 690 cm −1 , were observed.
HA does not form nanoparticles; however, when modified with 15% maleimide, particles as small as 180 nm were formed.To prepare the hydrogels, Chol−HA nanogel and 4arm-PEGSH solutions were poured into a disk-shaped silicone rubber mold with a diameter of 6 mm and a depth of 3 mm, and then, incubated at 37 °C for 24 h. Figure 1 shows the formation of Chol−HA hydrogels at various cholesterol levels.Transparent hydrogels were obtained from all the Chol−HA samples.For the Chol−HA hydrogels with 0, 1, 5, 10% cholesterol, the gel shape was maintained when the silicone mold was removed.However, the Chol−HA hydrogel with 15% cholesterol deformed upon removal from the silicone mold.Figure 2 verifies the formation process of Chol−HA hydrogels using ATR-FTIR spectroscopy.A decrease in the peak at 1695 cm −1 derived from maleimide, and the disappearance of the peak at 690 cm −1 , were observed.
Figure 3 shows SEM images of the Chol−HA hydrogel surfaces after freeze-drying.The 0.1% Chol−HA hydrogel exhibited a rough surface without pores.The 5, 10, and 15% Chol−HA hydrogels exhibited pores of approximately 700 µm 2 on their surfaces (Figure 3, upper images).In addition, for all samples, dots were observed on the hydrogel (Figure 3, lower images).Figure 3 shows SEM images of the Chol-HA hydrogel surfaces after freeze-drying.The 0.1% Chol-HA hydrogel exhibited a rough surface without pores.The 5, 10, and 15% Chol-HA hydrogels exhibited pores of approximately 700 µm 2 on their surfaces (Figure 3, upper images).In addition, for all samples, dots were observed on the hydrogel (Figure 3, lower images).

Mechanical Properties of the Chol-HA Hydrogel
The mechanical properties of the Chol-HA hydrogels were evaluated using a compression test.There was no significant difference in the elastic moduli of the Chol-HA hydrogels with 0, 1, 5, and 10% cholesterol (Figure 4).However, the elasticity of the Chol-HA hydrogel with 15% cholesterol was lower than that of the Chol-HA nanogel with 0% cholesterol.

Mechanical Properties of the Chol−HA Hydrogel
The mechanical properties of the Chol−HA hydrogels were evaluated using a co pression test.There was no significant difference in the elastic moduli of the Chol−H hydrogels with 0, 1, 5, and 10% cholesterol (Figure 4).However, the elasticity of t Chol−HA hydrogel with 15% cholesterol was lower than that of the Chol−HA nano with 0% cholesterol.

Mechanical Properties of the Chol−HA Hydrogel
The mechanical properties of the Chol−HA hydrogels were evaluated using a compression test.There was no significant difference in the elastic moduli of the Chol−HA hydrogels with 0, 1, 5, and 10% cholesterol (Figure 4).However, the elasticity of the Chol−HA hydrogel with 15% cholesterol was lower than that of the Chol−HA nanogel with 0% cholesterol.

Mechanical Properties of the Chol−HA Hydrogel
The mechanical properties of the Chol−HA hydrogels were evaluated using a compression test.There was no significant difference in the elastic moduli of the Chol−HA hydrogels with 0, 1, 5, and 10% cholesterol (Figure 4).However, the elasticity of the Chol−HA hydrogel with 15% cholesterol was lower than that of the Chol−HA nanogel with 0% cholesterol.

Cell Adhesion on the Chol-HA Hydrogel
First, we investigated whether NIH3T3 cells, which are fibroblasts without CD44, adhered to the Chol-HA hydrogels.NIH3T3 cells were seeded on the hydrogels and observed using fluorescence microscopy following calcein-AM staining, which stained Gels 2023, 9, 866 5 of 13 viable cells.Spherical cells without elongation were observed on the hydrogels, irrespective of cholesterol introduction (Figure 5A).Several cells were aggregated.The number and area of adhered cells were calculated using fluorescence images (Figure 5B).There was no significant difference in the number and area of adherent cells between the Chol-HA hydrogels, irrespective of cholesterol addition.The area of cells divided by the number of cells was investigated as an index of cell aggregation.There was no significant difference in cell aggregation between Chol-HA hydrogels with various cholesterol moieties.

Cell Adhesion on the Chol−HA Hydrogel
First, we investigated whether NIH3T3 cells, which are fibroblasts without CD44, adhered to the Chol−HA hydrogels.NIH3T3 cells were seeded on the hydrogels and observed using fluorescence microscopy following calcein-AM staining, which stained viable cells.Spherical cells without elongation were observed on the hydrogels, irrespective of cholesterol introduction (Figure 5A).Several cells were aggregated.The number and area of adhered cells were calculated using fluorescence images (Figure 5B).There was no significant difference in the number and area of adherent cells between the Chol−HA hydrogels, irrespective of cholesterol addition.The area of cells divided by the number of cells was investigated as an index of cell aggregation.There was no significant difference in cell aggregation between Chol−HA hydrogels with various cholesterol moieties.Second, HiBiT-THP-1 cells' adhesion to Chol−HA hydrogels was investigated.THP-1 is a monocyte CD44-positive cell line used to explore macrophage-like differentiation upon PMA stimulation.HiBiT-THP-1 cells are genetically modified with the HiBiT peptide, which is a short peptide of 11 amino acids that can bind to LgBiT and shows luminescent activity [23].PMA-stimulated HiBiT-THP-1 cells were seeded on the hydrogels and observed using fluorescence microscopy after cultivation for 6 days and calcein-AM staining (Figure 6A).Spherical cells without elongation and aggregated cells were observed for all Chol−HA hydrogels.The cell numbers and areas of Chol−HA hydrogels with various cholesterol moieties were measured (Figure 6B).The cell numbers and area of adherent cells increased with an increase in the amount of cholesterol moiety, and higher adhesion was achieved for the hydrogels of Chol−HA with cholesterol levels of of 5 and 10%.The cell adhesion decreased in the Chol−HA hydrogels with 15% cholesterol.Second, HiBiT-THP-1 cells' adhesion to Chol-HA hydrogels was investigated.THP-1 is a monocyte CD44-positive cell line used to explore macrophage-like differentiation upon PMA stimulation.HiBiT-THP-1 cells are genetically modified with the HiBiT peptide, which is a short peptide of 11 amino acids that can bind to LgBiT and shows luminescent activity [23].PMA-stimulated HiBiT-THP-1 cells were seeded on the hydrogels and observed using fluorescence microscopy after cultivation for 6 days and calcein-AM staining (Figure 6A).Spherical cells without elongation and aggregated cells were observed for all Chol-HA hydrogels.The cell numbers and areas of Chol-HA hydrogels with various cholesterol moieties were measured (Figure 6B).The cell numbers and area of adherent cells increased with an increase in the amount of cholesterol moiety, and higher adhesion was achieved for the hydrogels of Chol-HA with cholesterol levels of of 5 and 10%.The cell adhesion decreased in the Chol-HA hydrogels with 15% cholesterol.

Pro-Inflammation Response of HiBiT-THP-1 to the Chol-HA Hydrogel
IL-1β is an inflammatory cytokine.The HiBiT gene was genetically inserted under the IL-1β gene for HiBiT-THP-1.Therefore, IL-1β secretion was measured via luminescence.HiBiT-THP-1 was seeded on the hydrogels, and the IL-1β secretion from HiBiT-THP-1 was measured using a HiBiT assay (Figure 7).For the Chol-HA hydrogels with 0 and 1% cholesterol, the luminescence increased over time.For the Chol-HA hydrogels with 5% cholesterol, the luminescence increased on Day 6. Constant luminescence was observed for the Chol-HA hydrogels with 10% and 15% cholesterol (Figure 7A).The luminescence of the Chol-HA hydrogels with 5%, 10%, and 15% cholesterol was lower than those with 0% and 1% (Figure 7B).

Pro-Inflammation Response of HiBiT-THP-1 to the Chol−HA Hydrogel
IL-1β is an inflammatory cytokine.The HiBiT gene was genetically inserted under the IL-1β gene for HiBiT-THP-1.Therefore, IL-1β secretion was measured via luminescence.HiBiT-THP-1 was seeded on the hydrogels, and the IL-1β secretion from HiBiT-THP-1 was measured using a HiBiT assay (Figure 7).For the Chol−HA hydrogels with 0 and 1% cholesterol, the luminescence increased over time.For the Chol−HA hydrogels with 5% cholesterol, the luminescence increased on Day 6. Constant luminescence was observed for the Chol−HA hydrogels with 10% and 15% cholesterol (Figure 7A).The luminescence of the Chol−HA hydrogels with 5%, 10%, and 15% cholesterol was lower than those with 0% and 1% (Figure 7B).
The effects of IL-4 encapsulation on the Chol−HA hydrogels were determined.The Chol−HA hydrogel with 5% cholesterol that exhibited a pro-inflammatory HiBiT-THP-1 cell response was investigated using the hydrogels encapsulating IL-4 before and after gelation (Figure 8).In both cases, the luminescence increased on Day 4, and then, decreased on Day 6 (Figure 8A), whereas the luminescence of the Chol−HA hydrogel with 5% and without IL-4 expression increased over time.The luminescence of the hydrogel expressing IL-4 was lower than that of the hydrogel without IL-4.Also, there was a difference in the luminescence of the hydrogel encapsulating IL-4 after and before gelation, the hydrogel encapsulating IL-4 after gelation was lower than that of the hydrogel encapsulating IL-4 before gelation (Figure 8B).The effects of IL-4 encapsulation on the Chol-HA hydrogels were determined.The Chol-HA hydrogel with 5% cholesterol that exhibited a pro-inflammatory HiBiT-THP-1 cell response was investigated using the hydrogels encapsulating IL-4 before and after gelation (Figure 8).In both cases, the luminescence increased on Day 4, and then, decreased on Day 6 (Figure 8A), whereas the luminescence of the Chol-HA hydrogel with 5% and without IL-4 expression increased over time.The luminescence of the hydrogel expressing IL-4 was lower than that of the hydrogel without IL-4.Also, there was a difference in the luminescence of the hydrogel encapsulating IL-4 after and before gelation, the hydrogel encapsulating IL-4 after gelation was lower than that of the hydrogel encapsulating IL-4 before gelation (Figure 8B).

Discussion
In this study, we prepared a novel HA hydrogel through Chol−HA nanogel crosslinking and investigated its biological properties.Hyaluronic acid with cholesterol (modification rate: 0-15%) and maleimide (Chol−HA) was synthesized.The hydrodynamic diameter of the Chol−HA nanogel in 10 mM phosphate buffer was measured via DLS.The average particle sizes of the Chol−HA nanogels tended to decrease with an increasing degree of substitution of the cholesterol moiety.These results suggest that Chol−HA, which has 15 maleimide groups per 100 HA units, was physically crosslinked via hydrophobic interactions between the cholesteryl groups of Chol−HA to form Chol−HA nanogels [20].
The Chol−HA nanogel could crosslink with 4arm-PEGSH via Michael addition, and the hydrogel of Chol−HA nanogel was obtained.Transparent Chol−HA hydrogels were prepared with different cholesterol incorporation ratios.With the exception of the Chol−HA hydrogel with 15% cholesterol, the Chol−HA hydrogel shape was maintained upon mold removal.The elastic modulus of the Chol−HA hydrogel with 15% cholesterol was lower than that of the other hydrogels, indicating that crosslinking in the Chol−HA

Discussion
In this study, we prepared a novel HA hydrogel through Chol-HA nanogel crosslinking and investigated its biological properties.Hyaluronic acid modified with cholesterol (modification rate: 0-15%) and maleimide (Chol-HA) was synthesized.The hydrodynamic diameter of the Chol-HA nanogel in 10 mM phosphate buffer was measured via DLS.The average particle sizes of the Chol-HA nanogels tended to decrease with an increasing degree of substitution of the cholesterol moiety.These results suggest that Chol-HA, which has 15 maleimide groups per 100 HA units, was physically crosslinked via hydrophobic interactions between the cholesteryl groups of Chol-HA to form Chol-HA nanogels [20].
The Chol-HA nanogel could crosslink with 4arm-PEGSH via Michael addition, and the hydrogel of Chol-HA nanogel was obtained.Transparent Chol-HA hydrogels were prepared with different cholesterol incorporation ratios.With the exception of the Chol-HA hydrogel with 15% cholesterol, the Chol-HA hydrogel shape was maintained upon mold removal.The elastic modulus of the Chol-HA hydrogel with 15% cholesterol was lower than that of the other hydrogels, indicating that crosslinking in the Chol-HA hydrogel did not occur sufficiently.Although we do not have a clear answer as to the mechanism, we believe that it is due to the large molecular weight between crosslinking points.Dynamic light scattering (DLS) analysis showed that the number of associations was highest and particle size was smallest at 15% Chol incorporation, suggesting that the distance between crosslinks of nanogels was larger at Chol 15%, or that the distance between crosslinking points was larger and the elastic modulus was low because the crosslinking groups were unreacted.
Pore sizes were observed on the hydrogel surfaces using SEM.For Chol-HA hydrogels with 5, 10, and 15% cholesterol, pores were observed on the gel surface.Pores are formed during the freezing process.The hydration of Chol-HA with 0 and 1% cholesterol was different to that of hydrogels with 5, 10 and 15% cholesterol.In addition, dots were observed on the Chol-HA hydrogel, irrespective of the cholesterol incorporation ratio.The size of the dots decreased with increasing cholesterol, and the size of the Chol-HA nanogel before gelation, as measured using DLS, decreased with increasing cholesterol.From these results, it is presumed that the Chol-HA nanogels were observed as dots in the SEM images, indicating that the hydrogel was formed due to the Chol-HA nanogels crosslinking.
The adhesion of NIH3T3 and THP-1 cells to the Chol-HA hydrogels was also investigated.Few NIH3T3 cells adhered to all hydrogels, whereas the adhesion of HiBiT-THP-1 increased with an increase in cholesterol.CD44 is an HA receptor [24].NIH3T3 cells were CD44-negative, and HiBiT-THP-1 cells were CD44-positive cells; thus, HiBiT-THP-1 cells could adhere to the Chol-HA hydrogel [25].The shape of the HiBiT-THP-1-adherent cells was spherical; spread and elongation of the cells was not observed on the Chol-HA hydrogels.THP-1 cells are monocytes that differentiate into macrophage-like cells via PMA stimulation [26].In this study, HiBiT-THP-1 cells were seeded after PMA stimulation to investigate the macrophage response to Chol-HA hydrogels.For the control of TCPS, and elongated cells were observed, which are typical adhesion formations in integrin-adhesion protein interactions.Thus, the adhesion of HiBiT-THP-1 cells to the Chol-HA hydrogel, with a spherical formation, was probably mediated by the CD44-hyarulonic acid interaction.Because the interaction between CD44 and HA was weaker than that of the integrin-mediated cell adhesion, the ratio of adhered cells to seeded cells was approximately 1.2%.Interestingly, the adhesion of HiBiT-THP-1 cells increased with increasing cholesterol introduction into HA.The cells contacted and bonded via CD44-hyaluronic acid interaction and may have interacted with the cholesterol assembly in the nanogel, resulting in the maintenance of cellular adhesion on the hydrogels of Chol-HA.This mechanism remains unknown and should be investigated in detail in future studies.
The pro-inflammatory macrophage response to the Chol-HA hydrogels was investigated using HiBiT-THP-1; the HiBiT gene was genetically inserted under the IL-1b gene [23].For this system, the IL-1β secretion could be measured via luminescence.The luminescence was strongly dependent on cholesterol introduction and was inhibited at higher cholesterol levels in the hydrogels.As described above, HiBiT-THP-1 cells adhered to CD44.The binding of CD44 to macrophages stimulates pro-and anti-inflammatory responses in macrophages [2].In this case, the pro-inflammatory macrophage response bound through the CD44-hyaluronic acid interaction was inhibited on the hydrogels of Chol-HA because the luminescence decreased with increasing cell adhesion.However, for the hydrogel with 15% cholesterol, low luminescence was exhibited.However, the cell adhesion was low, and was similar to that on hydrogels with 0 and 1% cholesterol.Pro-and anti-inflammatory stimulation via the CD44-hyaluronic acid interaction was not sufficient because the Chol-HA binding site was decreased by cholesterol modification.Also, it may be considered that the lowest elastic modulus of the Chol-HA hydrogel with 15% cholesterol induced low inflammatory activation [27,28], or the cholesterol in the nanogel affected the inhibition of pro-inflammatory and enhancement of anti-inflammatory reactions, although the mechanism is still unknown.
Chol-HA hydrogels encapsulating IL-4, an anti-inflammatory cytokine, were prepared to induce an anti-inflammatory response in macrophages [29][30][31].Compared to the hydrogel of Chol-HA without IL-4, IL-1β secretion was inhibited and high inhibition of IL-1β secretion was achieved on Day 6.Interestingly, the Chol-HA hydrogel, in which IL-4 was encapsulated after gelation, inhibited the proinflammatory response of macrophages.It was suggested that IL-4 was released and affected macrophage response.Further investigation for the release profiles of the hydrogels before and after gelation is needed.

Conclusions
In the present study, we successfully synthesized an HA-modified hydrogel using cholesterol and maleimide.The Chol-HA hydrogel was obtained via chemical crosslinking of the Michael addition reaction (between the maleimide and thiol groups of 4arm-PEGSH).It was found that Chol-HA hydrogels with higher cholesterol modification inhibited IL-1β secretion, which is one pro-inflammatory response of macrophage-like THP-1 cells.Moreover, IL-4 encapsulated in the Chol-HA hydrogel enhanced the inhibition of inflammation Gels 2023, 9, 866 9 of 13 in THP-1 cells.These results provide useful insights into the biomedical applications of hydrogels.

Dynamic Light Scattering Measurement of Chol-HA Nanogel
The Chol-HA solution in 10 mM phosphate buffer (pH 7.4) was characterized via dynamic light scattering (DLS) analysis using an ELSZ-2000 instrument (Otsuka Electronics).Autocorrelation functions were calculated using the cumulant method.The hydrodynamic diameter of Chol-HA was analyzed using the Stokes-Einstein equation.

Preparation of Chol-HA Nanogel-Based Hydrogel (Chol-HA Hydrogel)
Chol-HA hydrogel was prepared through crosslinking, via a Michael addition reaction between the maleimide and thiol groups.Briefly, the Chol-HA (10 mg/mL) and 4arm-PEGSH (20 mg/mL) were dissolved separately in 10 mM phosphate buffer (pH 7.4).Subsequently, the two precursor solutions were poured into disk-shaped silicone rubber molds (mold diameter and depth: 8 mm and 1.5 mm, and 6 mm and 3 mm), which were placed on a polytetrafluoroethylene membrane and cooled to 5 • C. Next, a silicone coversheet was used to cover the mold, which was incubated at 37 • C for 30 min.After incubation, the samples were transferred into well plates.The molar ratio of the maleimide to thiol groups was 1.1:1.

Total Reflectance-Fourier Transform Infrared (ATR-FTIR) Spectroscopic Analysis
ATR-FTIR spectra were recorded using an ATR-FTIR spectrometer (Perkin Elmer, Waltham, MA, USA).The spectra were obtained in the range of 4000-400 cm −1 and at a 4 cm −1 resolution with 8 co-added scans per spectrum.The absorption intensities under the spectra were integrated at wavenumbers of 1800-1300 and 1000-400 cm −1 , which represent the regions of maleimide and alkene C-H, respectively.The freeze-dried samples of Chol-HA and Chol-HA hydrogel were subjected to IR measurements.

Encapsulation of IL-4 in the Chol-HA Hydrogel
Before and after gelation, IL-4 was encapsulated in the Chol-HA hydrogels.Before gelation, the Chol-HA (10 mg/mL) nanogel solution was mixed with the IL-4 (2 µg/mL) solution and incubated at 4 • C for 24 h, and then, gelatinized at 37 • C for 30 min.Next, IL-4 was added to the Chol-HA nanogel solution prior to gelation such that IL-4 was 20 ng/mL after gelation.After gelation, the Chol-HA nanogel solution was gelatinized at 37 • C for 30 min and the hydrogel was soaked in the IL-4 (20 ng/mL) solution at 4 • C for 24 h.

Cell Culture on the Chol-HA Hydrogel
Chol-HA hydrogels were added to 48-well plates.The NIH3T3 cell suspension was prepared in EMEM (containing 10% FBS and 1× penicillin/streptomycin) at 1.14 × 10 4 cells/mL.The cell suspension (0.5 mL) was seeded in each plate well and the plate was incubated at 37 • C and 5% CO 2 for 1, 3, and 5 days.The HiBiT-THP-1 cell suspension was prepared in RPMI-1640 (containing 10% FBS and PMA (320 µM)) and seeded (4.5 × 10 5 cells/mL) in each well, and the plate was incubated at 37 • C and 5% CO 2 for 1, 3, and 5 days.

Fluorescent Microscopic Observation of Cells on the Chol-HA Hydrogel
The cells on the hydrogels were washed with PBS and stained with Calcein-AM.The hydrogels were then transferred to another plate and observed under a fluorescence microscope (BZ-X710; Keyence Corp., Osaka, Japan).Using fluorescence images of cells stained with calcein-AM on the hydrogel, the cell number and area were measured using

Figure 1 .
Figure 1.Photographs of Chol−HA hydrogels modified with different cholesterol levels.Scale bar: 5 mm.

Figure 1 .
Figure 1.Photographs of Chol-HA hydrogels modified with different cholesterol levels.Scale bar: 5 mm.