Silver Ions Incorporation into Nanoﬁbers for Enhanced hMSC Viability

: Antimicrobial properties of silver have been known for a long time, but there is also cytotoxicity of high concentrations of silver. Therefore, it is important to select the concentration and shape of silver depending on the goals. The ideal wound dressing should ensure that the wound remains optimally moist, protected from infections, has no toxic compounds, and stimulates regeneration. In the present work, we obtained a series of polycaprolactone-based nanomaterials fabricated by electrospinning and incorporated with silver ions (up to 0.6 at.%). By adjusting the magnetron current (0.3 A) and implanter voltage (5 kV), the deposition of TiO 2 and Ag + implantation into PCL/PEO nanoﬁbers was optimized to achieve implantation of Ag + without damaging the nanoﬁbrous structure of the biodegradable nanoﬁbers. The obtained results allow us to predict signiﬁcant protection properties of the developed material not only from mechanical inﬂuence but also thanks to the antimicrobial effect due to silver ions, which is important for chronic wounds and injuries with a large area of damage and can activate host cells proliferation. and allow us to predict signiﬁcant protection properties for the developed from to an antimicrobial effect to silver ions, and with area cell


Introduction
Currently, wound healing materials with protective and regenerative properties are in great demand, the development of which is actively being carried out all over the world [1]. To date, active research is underway on regenerative materials with an antibacterial effect. Silver is actively studied as an antibacterial component and is used in various creams, substances and nanomaterials for regenerative medicine [2][3][4][5]. In addition to the antibacterial effect, silver has a regenerative effect, provided by stimulating the proliferation of cells involved in regeneration. The antimicrobial properties of silver have been known for a long time, but there is also cytotoxicity of high concentrations of silver [6].
Silver-ion-releasing polylactide (PLA) nanofibrous scaffolds were developed using a silver-ion-releasing solution, Silvadur ET. This solution comprised AgNO 3 , a polymer binder, water, and ethanol. Nanofibers coated with solutions having different concentrations of silver ranging from 31.25 to 250 µg/mL have exhibited excellent antimicrobial properties toward both Gram-positive and Gram-negative bacteria while having no effect on silver-resistant bacteria [7]. Nanofibrous scaffolds coated with Silvadur ET solution containing silver less than 62.5 µg/mL maintained the viability and proliferation of both human dermal fibroblasts and human epidermal keratinocytes, although some decrease of the cell viability was evident even for lower concentrations [8].
The cytotoxicity effect of silver ions and silver nanoparticles is mainly due to oxidative stress and is independent of silver ions, while the generation of reactive oxygen species (ROS) on the surface of silver nanoparticles may additionally affect the viability of cells. Indeed, free silver ions play a considerable role in the toxicity of silver nanoparticle suspensions [9]. The Ag + strongly increases the production of reactive oxygen species, including Chemistry 2022, 4 932 superoxide anion radicals. These effects correspond to a strong decrease in intracellular reduced glutathione and to an increased susceptibility to H 2 O 2 -induced cell death [10]. Therefore, it is important to select the concentration and shape of silver depending on the goals. In the very specific range of silver ions concentration (from 5 to 20 µM) a positive effect on the MSC cell viability was previously shown [11]. Various factors may affect the cytotoxicity of silver ions including type of cell media, the presence of chloride ions, glucose, the form of silver, etc. [12]. The implantation of silver ions instead of incorporation of the Ag nanoparticles may reduce the cytotoxicity of produced materials. Recently, nanofibers coated with TiO 2 [13,14] and Cu films [15] were prepared by magnetron sputtering deposition onto biodegradable nanofibrous foils. The most critical issue for this process would be the prevention of structural damage to the nanofibrous scaffold during the deposition process [16].
In this work, we obtained a series of polycaprolactone/polyethyleneoxide PCL/PEObased nanomaterials fabricated by electrospinning, and incorporated with silver ions (up to 0.6 at.%). By adjusting the magnetron current and implanter voltage, the deposition of TiO 2 and Ag + implantation into PCL/PEO nanofibers was optimized to achieve the implantation of Ag + without damaging the nanofibrous structure of the PCL/PEO. It was shown that the maximum amount of silver was released from the PCL-Ti0.3-Ag-5 kV sample, and in the first hours there was a rapid release, then a smoother one, and for 7 days it continued to be released more slowly. The aim of this work was to determine the effect of the obtained samples on the viability and proliferative potential of mesenchymal stromal cells.

Electrospinning of PCL and PCL/PEO Nanofibers
The overall scheme for preparing functionalized nanofibers is depicted in Figure 1. The electrospun PCL nanofibers were prepared by electrospinning a 9 wt.% solution of polycaprolactone PCL (80,000 g/mol). The processing of the sample can be found elsewhere [17]. Briefly, the granulated PCL was dissolved in a mixture of acetic acid (99%) and formic acid (98%) [15]. All compounds were purchased from Sigma Aldrich (Darmstadt, Germany). The weight ratio of acetic acid (AA) to formic acid (FA) was 2:1. The PCL solutions in AA and FA were stirred at 25 • C for 24 h.
Chemistry 2022, 4, FOR PEER REVIEW 2 cells. Indeed, free silver ions play a considerable role in the toxicity of silver nanoparticle suspensions [9]. The Ag+ strongly increases the production of reactive oxygen species, including superoxide anion radicals. These effects correspond to a strong decrease in intracellular reduced glutathione and to an increased susceptibility to H2O2-induced cell death [10]. Therefore, it is important to select the concentration and shape of silver depending on the goals. In the very specific range of silver ions concentration (from 5 to 20 µM) a positive effect on the MSC cell viability was previously shown [11]. Various factors may affect the cytotoxicity of silver ions including type of cell media, the presence of chloride ions, glucose, the form of silver, etc. [12]. The implantation of silver ions instead of incorporation of the Ag nanoparticles may reduce the cytotoxicity of produced materials.
Recently, nanofibers coated with TiO2 [13,14] and Cu films [15] were prepared by magnetron sputtering deposition onto biodegradable nanofibrous foils. The most critical issue for this process would be the prevention of structural damage to the nanofibrous scaffold during the deposition process [16].
In this work, we obtained a series of polycaprolactone/polyethyleneoxide PCL/PEObased nanomaterials fabricated by electrospinning, and incorporated with silver ions (up to 0.6 at.%). By adjusting the magnetron current and implanter voltage, the deposition of TiO2 and Ag+ implantation into PCL/PEO nanofibers was optimized to achieve the implantation of Ag+ without damaging the nanofibrous structure of the PCL/PEO. It was shown that the maximum amount of silver was released from the PCL-Ti0.3-Ag-5 kV sample, and in the first hours there was a rapid release, then a smoother one, and for 7 days it continued to be released more slowly. The aim of this work was to determine the effect of the obtained samples on the viability and proliferative potential of mesenchymal stromal cells.

Electrospinning of PCL and PCL/PEO Nanofibers
The overall scheme for preparing functionalized nanofibers is depicted in Figure 1. The electrospun PCL nanofibers were prepared by electrospinning a 9 wt.% solution of polycaprolactone PCL (80,000 g/mol). The processing of the sample can be found elsewhere [17]. Briefly, the granulated PCL was dissolved in a mixture of acetic acid (99%) and formic acid (98%) [15]. All compounds were purchased from Sigma Aldrich (Darmstadt, Germany). The weight ratio of acetic acid (AA) to formic acid (FA) was 2:1. The PCL solutions in AA and FA were stirred at 25 °C for 24 h. According to our methodology reported elsewhere [18], PCL/PEO nanofibers with a ratio 3:1 PEO prepared by electrospinning of the 9 wt.% solutions containing 75% PCL and 25% PEO (Mw = 100,000, Sigma-Aldrich, Steinheim am Albuch, Germany).
The solutions were electrospun with a 20 cm long wired electrode using a Nanospider™ NSLAB 500 machine (ELMARCO, Liberec, Czech Republic). The applied voltage was 50 kV. The distance between the electrodes was set to 100 mm. The as-prepared and non-treated PCL nanofibers are referred to as PCL-ref throughout the text.

Deposition of TiO 2 Coating and Ag Ion Implantation
The deposition experiments were performed using a vacuum set-up with a magnetron sputtering unit equipped with the MEVVA-type ion implanter [19]. The titania films (~20 nm thick) were deposited by magnetron sputtering of a composite TiC-CaO-Ti 3 PO x target in a gaseous mixture of Ar and 15% N 2 . The applied magnetron current was 0.5 or 0.3 A, the magnetron voltage was~450 V, and the bias voltage was kept at −50 V (samples denoted as PCL/PEO-Ti). The target to substrate distance was fixed to 120 mm.

Characterization of Samples
The sample's morphology was examined by scanning electron microscopy (SEM), which was carried out with a JSMF 7600 microscope (JEOL Ltd., Tokyo, Japan) equipped with an energy-dispersive X-ray spectrometer. To compensate for surface charge, the samples were coated with a~5 nm thick Pt layer.
The sample chemical characterization was performed by X-ray photoelectron spectroscopy (XPS), energy-dispersive X-ray spectroscopy (EDXS) and Fourier-transformed infrared (FTIR) spectroscopy. The XPS analysis was carried out using a PHI5500VersaProbeII instrument (PHI) equipped with a monochromatic Al Kα X-ray source (hν = 1486.6 eV) at a pass energy of 23.5 eV and X-ray power of 50 W. The data processing was performed using CASAXPS software as reported elsewhere [20][21][22].
The sample wettability was assessed by measuring the water contact angle (WCA). The measurements were carried out on an Easy Drop Kruss (KR¨ŪSS, Hamburg, Germany) device. For each sample, at least five WCA measurements were performed.

Cell Tests
Human MSCs 4-6 were taken from the culture bank of RICEL-branch ICG SB RAS, which had been extracted from bone marrow using standard methods [23]. Cells were cultured in DMEM/F12 Medium (Sigma Aldrich, Paisley PA4 9RF, UK) that was supplemented with 10% foetal bovine serum (FBS, Gibco, Carlsbad, CA, USA) under standard culture conditions (humidified atmosphere, 5% CO 2 and 95% air, at 37 • C).
Nanofibrous samples were cut into pieces with 0.5 diameter and used in set of experiments. The MTT test was conducted to test the cytotoxicity of used Ag concentrations. 5 × 10 3 hMSC were seeded in 96-wells plate, Ag-PCL membrane samples were soaked in culture medium for 24 h, then this medium was transferred to cells for incubation for 3 days. Results were measured by optical density by using Multiscan FC spectrophotometer. To test the proliferation rate, human mesenchymal stromal cells were seeded on Ag-PCL membranes 5 × 10 3 per sample and incubated for 3 days in standard conditions (95% humidity, 5% CO 2 ). To further evaluate the total amount, cells were dyed with Hoechst reagent to visualize cell nuclei and with EdU Click iT-reagent to count the number of proliferating cells.

Statistical Analysis
All experimental data were analysed by Statistica 8.0 software with nonparametric Mann-Whitney U test. The results presented as mean ± standard deviation with statistical significance p < 0.05.

Morphology of Nanofibrous Samples
The SEM micrographs of PCL/PEO-Ti-Ag nanofibers are presented in Figure 1. The Ag + implantation at 15 kV (Figure 1b) Figure 2. It is evident that the nanofibers are not damaged, but their surface after Ag + implantation is smoother as compared to PCL/PEO-ref.
Chemistry 2022, 4, FOR PEER REVIEW 4 reagent to visualize cell nuclei and with EdU Click iT-reagent to count the number of proliferating cells.

Statistical Analysis
All experimental data were analysed by Statistica 8.0 software with nonparametric Mann-Whitney U test. The results presented as mean ± standard deviation with statistical significance p < 0.05.

Morphology of Nanofibrous Samples
The SEM micrographs of PCL/PEO-Ti-Ag nanofibers are presented in Figure 1. The Ag + implantation at 15 kV (Figure 1b) led to a significant destruction of nanofibrous material as compared to PCL/PEO-ref. The damage of the PCL nanofibrous structure at the high current and high implanting voltage conditions was caused by the highly energetic ions as well as "nanodroplets" of the silver nanomaterials approaching the surface. At higher current and higher voltage, stronger thermal heating of the substrate (PCL nanofibers) led to significant damage of the nanostructure. The samples prepared at 5

Chemical Characterization of Biodegradable Nanohybrid Materials
The PCL and PCL/PEO polymers are well known and their compositions were reported elsewhere [18]. The modified nanofibers are of much higher interest, and the compositions of all samples evaluated by XPS are summarized in Table 1. The incorporation of TiO 2 and Ag in PCL/PEO-Ti-Ag samples was evident from the surface's overall atomic composition. The analysis of Ti2p and Ag3d (not reported here) revealed that titanium and silver were both the oxidized states: TiO 2 and Ag 2 O, respectively. The WCA analysis revealed that the unmodified nanofibers exhibited a hydrophobic nature and the implantation of Ag + ions led to significant decrease of WCA and, thus, the surface of all modified samples was hydrophilic (see Table 1).

Analysis of Cell Viability and Proliferation
The cell images are depicted in Figure 3. The first row presents all cell nuclei on the membranes (on PCL/PEO-Ti0.3-Ag-8 kV and PCL/PEO-Ti0.3-Ag-5 kV samples, cells almost create a monolayer). The second row presents proliferating cells that incorporated EdU reagent. Based on the calculations of cells and the EdU+/Dapi ratio, we obtained that all variants of PCL membranes with Ag nanoparticles tend to increase proliferation, especially PCL/PEO-Ti0.3-Ag-8 kV made it significant.
The release of Ag + ions differed in samples depending on the initial Ag concentrations and was presented in the article [15]. Here, Ag concentrations in all samples had no toxicity on human mesenchymal cells, furthermore, Ag + ions released in culture medium from PCL/PEO-Ti0.5-Ag-15 kV and PCL/PEO-Ti0.3-Ag-5 kV resulted in an increased percentage of living cells compared to the control (Figure 4). The total cell count was significantly higher in PCL/PEO-Ti0.3-Ag-8 kV samples in comparison to PCL/PEO-ref membranes. However, the proliferation rate was higher in all samples in comparison to PCL/PEO-ref ( Figure 5).
The Ag modification of PCL/PEO nanofibers (PCL/PEO-Ti0.3-Ag-8 kV) with a 0.3 A current for TiO 2 deposition and Ag + implantation at 8kV induces proliferation of human mesenchymal cells. Besides that, fast Ag + ion release from these nanofibers in the first 24 h could have possibly reduced bacterial activity in wound dressings but is low enough for a longer period of time and did not cause cytotoxicity. The obtained results allow us to expect that the material can be applied for tissue engineering as it can provide effective protection not only from mechanical influence but also has an antimicrobial effect because of the Ag [5,15], which is important for chronic wounds and injuries with a large area of damage, and can activate host cell proliferation.        The Ag modification of PCL/PEO nanofibers (PCL/PEO-Ti0.3-Ag-8 kV) with a 0.3 A current for TiO2 deposition and Ag+ implantation at 8kV induces proliferation of human mesenchymal cells. Besides that, fast Ag+ ion release from these nanofibers in the first 24 h could have possibly reduced bacterial activity in wound dressings but is low enough for a longer period of time and did not cause cytotoxicity. The obtained results allow us to expect that the material can be applied for tissue engineering as it can provide effective protection not only from mechanical influence but also has an antimicrobial effect because of the Ag [5,15], which is important for chronic wounds and injuries with a large area of damage, and can activate host cell proliferation.

Conclusions
In this work, a series of polycaprolactone-based nanomaterials were fabricated by electrospinning and modified by deposition of a TiO2 layer and implantation of silver ions (up to 0.6 at.%). By adjusting the magnetron current (0.3 A) and implanter voltage (5 kV), the deposition of TiO2 and Ag+ implantation into the PCL/PEO nanofibers were optimized to achieve significant implantation of Ag + without damaging the nanofibrous structure of the biodegradable nanofibers. The nanofibers with the implanted silver ions exhibited enhanced cell viability and proliferation. The obtained results allow us to predict significant protection properties for the developed material not only from mechanical influence but also thanks to an antimicrobial effect due to silver ions, which is important for chronic wounds and injuries with a large area of damage and can activate host cell proliferation.

Conclusions
In this work, a series of polycaprolactone-based nanomaterials were fabricated by electrospinning and modified by deposition of a TiO 2 layer and implantation of silver ions (up to 0.6 at.%). By adjusting the magnetron current (0.3 A) and implanter voltage (5 kV), the deposition of TiO 2 and Ag + implantation into the PCL/PEO nanofibers were optimized to achieve significant implantation of Ag + without damaging the nanofibrous structure of the biodegradable nanofibers. The nanofibers with the implanted silver ions exhibited enhanced cell viability and proliferation. The obtained results allow us to predict significant protection properties for the developed material not only from mechanical influence but also thanks to an antimicrobial effect due to silver ions, which is important for chronic wounds and injuries with a large area of damage and can activate host cell proliferation.