silver bimetallic nanoencapsulated in PVP

Artificial Cells, Nanomedicine, and Biotechnology An International Journal

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Zinc oxide/silver bimetallic nanoencapsulated in PVP/PCL nanofibres for improved antibacterial activity Min Hu, Chenwen Li, Xin Li, Min Zhou, Jianbin Sun, Fangfang Sheng, Sanjun Shi & Laichun Lu To cite this article: Min Hu, Chenwen Li, Xin Li, Min Zhou, Jianbin Sun, Fangfang Sheng, Sanjun Shi & Laichun Lu (2017): Zinc oxide/silver bimetallic nanoencapsulated in PVP/PCL nanofibres for improved antibacterial activity, Artificial Cells, Nanomedicine, and Biotechnology, DOI: 10.1080/21691401.2017.1366339 To link to this article: http://dx.doi.org/10.1080/21691401.2017.1366339

Published online: 21 Aug 2017.

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Date: 22 August 2017, At: 08:12

ARTIFICIAL CELLS, NANOMEDICINE, AND BIOTECHNOLOGY, 2017 https://doi.org/10.1080/21691401.2017.1366339

Zinc oxide/silver bimetallic nanoencapsulated in PVP/PCL nanofibres for improved antibacterial activity Min Hua,b, Chenwen Lia,b, Xin Lia,b, Min Zhoua, Jianbin Suna, Fangfang Shenga, Sanjun Shib and Laichun Lua

Downloaded by [Australian Catholic University] at 08:12 22 August 2017

a Teaching Experimental Center, College of Pharmacy, Third Military Medical University, Chongqing, China; bDepartment of Pharmacy, Institute of Surgery Research, Daping Hospital, Third Military Medical University, Chongqing, China

ABSTRACT

ARTICLE HISTORY

The anti-infection ability and skin regeneration are important aspects on the progress of wound healing, which needs an ideal wound dressing that not only resists bacteria but also promotes skin regeneration. In this study, zinc oxide/silver/polyvinylpyrrolidone/polycaprolactone (ZnO/Ag/PVP/PCL) nanofibres were prepared through electrospinning. Firstly, zinc oxide nanoparticles (ZnONPs) and silver nanoparticle (AgNPs) were synthesized respectively. Secondly, the two nanoparticles were mixed with polyvinylpyrrolidone (PVP) and polycaprolactone (PCL) to obtain the nanofibres. The results of scanning electron microscopy (SEM) showed that ZnONPs and AgNPs were 40.07 ± 9.70 nm and 37.46 ± 12.02 nm, respectively. After electrospinning, the nanofibres were 368.22 ± 123.96 nm in diameter. Infrared spectroscopy revealed that ZnONPs/AgNPs bimetallic nanomaterials were physically embedded in the nanofibres. The antibacterial effects against Staphylococcus aureus and Escherichia coli of ZnO/Ag/PVP/PCL nanofibres were significantly better than these of the single metal material-loaded nanofibres. More importantly, the combination of ZnO and Ag reduced the cytotoxicity of ZnO/Ag/PVP/PCL bimetallic nanofibres toward fibroblasts. These findings demonstrated that ZnO/Ag/PVP/PCL bimetallic nanofibres should be of greater interest than the single metal nanomaterial-loaded nanofibres in inhibiting growth of bacteria.

Received 8 July 2017 Revised 2 August 2017 Accepted 7 August 2017

Introduction More recently, metal nanomaterials had attracted the scientists’ attention in the field of anti-infection because of their ability to overcome existing drug resistance at suitable doses, which can increase cellular uptake and reduce efflux of drugs from the microbial cell [1]. Zinc oxide nanoparticles (ZnONPs), which possess both antibacterial and anti-inflammatory properties and accelerate the healing of both acute and chronic wounds, are an ideal material for using in inhibiting growth of bacteria [2–6]. In addition, zinc is necessary for the human body as a trace element [7]. However, a lower concentration of zinc oxide inhibits but does not kill microbes and is likely to allow some microbial cells to live and therefore develop resistance when exposed to drug [1,8,9]. It is a contradiction that high concentrations of zinc oxide nanoparticles used would induce intolerance in the body. Therefore, a reliable drug delivery technology that can maintain the superiority of ZnONPs for anti-infection and reduce the dose of administration for drug while not reducing its efficacy on killing bacteria is highly desired. Silver nanoparticles (AgNPs), another metal materials investigated for a long time, are an alternative antibacterial agent to inhibit/kill bacteria and show a significantly better antibacterial capacity than many antibiotics [10–13]. Similar to ZnO, high amount of Ag used would result in resistance and serious side effects. More importantly, high amount of

KEYWORDS

Zinc oxide; silver; nanoparticles; electrospinning nanofibres; antibacterial activity

Ag nanoparticles used trend to aggregate resulting in decreased stability, which in turn reduce the antibacterial efficacy. Although attempts on the development of ZnO or Ag formulations have been made, the optimal antibacterial efficacy and the reduced toxicity still remain challenges [14–16]. Alternatively, Ag materials, especially Ag ions, can enhance the antimicrobial activity of ZnO [17]. In combination, therapy-based ZnO and Ag, both amount of ZnO and Ag could be reduced without reducing the therapeutic efficacy. Furthermore, the ZnO/Ag bimetallic nanomaterials would centralize all advantages of both drugs and provide a general means to maximize therapeutic efficacy, overcome treatment resistance and reduce adverse effects [14]. Consequently, this combination therapy based on ZnO/Ag bimetallic nanomaterials will be a better method to overcome the limitations of metal materials encountered in antimicrobial therapy. In practical use, polyvinylpyrrolidone (PVP)/polycaprolactone (PCL)-based electrospun nanofibres were performed subsequently to encapsulate ZnO/Ag bimetallic nanomaterials (ZnO/Ag/PVP/PCL). Therefore, in the study, we aim to fabricate ZnO/Ag/PVP/PCL nanofibres with superior antibacterial activity and good biocompatibility by electrospinning technology. After acquisition of ZnONPs and AgNPs, respectively, ZnO/Ag/PVP/PCL nanofibres were prepared by electrospinning. The products were characterized by scanning electron microscopy (SEM), Fourier transform infrared spectroscopy

CONTACT Sanjun Shi [email protected] Department of Pharmacy, Institute of Surgery Research, Daping Hospital, Third Military Medical University, [email protected] Teaching Experimental Center, College of Pharmacy, Third Military Medical University, Chongqing, China Chongqing, China; Laichun Lu ß 2017 Informa UK Limited, trading as Taylor & Francis Group

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(FT-IR) and differential scanning calorimetry (DSC). Cytotoxicity to human skin fibroblasts (HSFs) and antimicrobial activity against Staphylococcus aureus and Escherichia coli of the prepared nanofibres were studied.

Materials and methods


Materials Silver nitrate was supplied by the Guanghua Sci-Tech Co, Ltd. (Guangzhou, China), and zinc acetate and trifluoroethanol were supplied by Aladdin (Shanghai, China). Oxalate and polyvinylpyrrolidone K30 were purchased from the Sinopharm Chemical Reagent Co, Ltd. (Shanghai, China). Polyvinylpyrrolidone K90 was purchased from Tokyo chemical industry Co, Ltd. (Tokyo, Japan). Polycaprolactoneand dimethyl sulphoxide was obtained from Sigma-Aldrich (St. Louis., MO). 3–(4,5-Methylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) was procured from Solon (OH). Mueller–Hinton agar and Mueller–Hinton broth were supplied by the Solarbio (Bejijing, China).

Synthesis and characterization of ZnONPs and AgNPs Synthesis of ZnONPs ZnO nanoparticles were synthesized via an oxalate decomposition method [18]. In brief, 1.36 g of anhydrous zinc acetate was added to a round-bottomed flask with 25 ml of ethanol. The reaction system was stirred for 1 h until it formed white solution. The reaction mixture was elevated to 50 C and stirred for another 30 min. Afterwards, 1.0 g of oxalic acid dihydrate was rapidly added to the reaction vessel under reflux for 3 h. The precipitate was separated from the mixture followed by drying at 75 C for a whole night. After cooled down, the dried product was ground and calcined at 550 C for 2 h. The reaction equations are as follows: Zn ðCH3 COOÞ2 þ C2 H2 O4 2H2 O ! ZnC2 O4 þ 2CH3 COOH þ 2H2 O ZnC2O4 ! ZnOþCO2 " þ CO "

Synthesis of AgNPs In the study, 1.0 g of polyvinylpyrrolidone (PVP K30) was added to a 50 ml round-bottomed flask with 10 ml of ethanol followed by stirred and heated to 50 C. 10 ml of AgNO3 solution containing ethanol was quickly added into the round-bottomed flask. The concentration of AgNO3 in the final solution was 1.2%. The mixture was kept stirring at 50 C for another 4 h until the colour of solution did not change. In order to obtain a higher yield of AgNPs, the reaction solution was subjected to centrifugation at 14,000 rpm for 30 min. The lower layer liquid containing the precipitate was separated and then steamed at 40 C under vacuum. Characterization of ZnONPs and AgNPs The morphology of ZnONPs and AgNPs was examined by an S-3000 N SEM equipment (Hitachi, Japan). Briefly, specimens

of ZnONPs were uniformly blown on the conductive adhesive followed by placing under SEM to observe their morphology. Similarly, 3 5 drops of synthesized AgNPs solution were placed in the conductive adhesive followed by drying. The average particle sizes of ZnONPs and AgNPs were calculated by randomly selecting 50 nanoparticles from the image, respectively. 3 5 mg of ZnONPs and AgNPs were, respectively, dissolved in 10 ml of double-distilled water followed by ultrasonic. Then, the samples were characterized by an ultraviolent spectrometer (TU-1810, Beijing Purkinje General Instrument Co., Ltd. China). The quantity of ZnO and Ag present in the products was determined as follows: 25 mg of the prepared ZnONPs and AgNPs were added to different volumetric flasks, respectively. The samples were dissolved with the dilute nitric acid aqueous solution, which were measured by an atomic absorption spectrophotometer (Z5000, Hitachi).

Preparation of ZnO/ag/PVP/PCL nanofibres A total mixture of 12% of PVP K90 and PCL was dissolved in 2,2,2-trifluoroethanol in various proportions (PVP, PVP/ PCL ¼ 3/1, PVP/PCL ¼ 1, PVP/PCL ¼ 1/3, PCL) to prepare PVP/ PCL nanofibres. The polymer solutions were stirred for at least 24 h at room temperature and filled into a syringe with a needle (inter diameter 0.8 mm). Electrospinning was performed in a high-voltage power source. The prepared nanofibres were collected on a 15 15 cm aluminium foil, which was electrically grounded. The applied voltages, working distance and velocity were optimized. After acquisition of the optimal PVP/PCL nanofibres (PVP/ PCL ¼ 1/3), the drugs including ZnONPs and AgNPs were loaded into the PVP/PCL nanofibres at different concentrations (1% of ZnONPs (w/v), 1% of AgNPs, 0.25% of ZnONPs þ 0.75% of AgNPs, 0.5% of ZnONPs þ 0.5% of AgNPs). All the parameters were the same as mentioned earlier. As a result, ZnO/PVP/PCL nanofibres, Ag/PVP/PCL nanofibres, ZnO/Ag/ PVP/PCL nanofibres (ZnO/Ag ¼ 1) and ZnO/Ag/PVP/PCL nanofibres (ZnO/Ag ¼ 1/3) were obtained followed by drying under vacuum at 40 C for 2 h, respectively.

Characterization of the prepared nanofibres Fabrication and physicochemical characteristics of the nanofibres The morphology and diameter of the prepared nanofibres were determined via SEM. The diameter of nanofibres was recorded and calculated by randomly selecting 50 nanofibres from the image through Image J software (National Institutes of Health, Bethesda, MD). Fourier transformation infrared spectroscopy (Frontier, PerkinElmer, Waltham, MA) was used to study the structure and chemical bond of the polymer and nanoparticles. The infrared spectra of PVP/PCL (1/3) nanofibres, Ag/PVP/PCL nanofibres, ZnO/PVP/PCL nanofibres and ZnO/Ag/PVP/PCL nanofibres were measured from 4000 cm1 to 650 cm1. Thermodynamic properties of the prepared nanofibres were also studied using a differential scanning

ARTIFICIAL CELLS, NANOMEDICINE, AND BIOTECHNOLOGY


calorimeter instrument (1100LF, METTLER, Switzerland). The prepared nanofibres were placed in pans and heated from 20 to 450 C. The heating rate of the instrument was 10 C per minute.

Water vapour transmission rate The water vapour transmission rate of the prepared nanofibres was determined by an ASTEM E 96 desiccant method [19]. In brief, the samples were divided into nine groups: PVP nanofibres, PCL nanofibres, PVP/PCL nanofibres (1/3), PVP/PCL nanofibres (1/1), PVP/PCL nanofibres (3/1), Ag/PVP/PCL nanofibres, ZnO/PVP/PCL nanofibres, ZnO/Ag/PVP/PCL nanofibres and non-woven fabrics (used as the control group) [20]. Some allochroic silica gel was put into small cups accompanied with the nanofibres and non-woven fabrics followed by sealing. These cups were placed in a test chamber at 37 C with a humidity of 75%. The weight change was recorded at a predetermined time and the water vapour transmission rate was calculated by the following formulas. RWVP ¼W=ðA DPÞ P ¼ RWVP d

(1) (2)

RWVP represents water vapour transmission rate (gh1 cm2mmHg1); W represents the quantity of water permeating the nanofibres (gh1); A represents the area of the small cup mouth (cm2); DP represents the pressure difference on both sides of nanofibres (mmHg); d represents the thickness of nanofibres (cm); and P means the permeability of nanofibres.

Swelling degree and weight loss The prepared nanofibres and non-woven fabrics were immersed in phosphate buffer solution (PBS, pH ¼ 7.4) at 37 C for 24 h. The swelling degree and weight loss of the nanofibres were calculated based on the weight change by the following formulas. Swelling degree ð%Þ ¼ ðWt Wo Þ=Wo 100 Weight loss ð%Þ ¼ ðWo Wd Þ=Wo 100

(3) (4)

Among the two equations, Wt means wet weight of the nanofibres after immersed in PBS, while Wd means dry weight of the nanofibres after immersed in PBS. Wo represents the initial weight of the nanofibres.

Antibacterial study Antibacterial activity of the nanofibre formulations was studied using a disc diffusion method and an antibacterial kinetic test with bacterial strains of Staphylococcus aureus and Escherichia coli. The bacterial suspensions in Mueller–Hinton broth with a concentration of 0.5 McFarland were prepared (1.5 108 cfu/mL). Then, the suspension was diluted several times to achieve a bacteria concentration at 105 cfu/mL. Firstly, the nanofibre formulations were cut into circular sheet mat (15 mg; 14.00 mm in diameter) by a circular punch. 100 lL of the diluted bacterial suspension (105 cfu/mL) were coated on the surface of Mueller–Hinton agar (MHA) medium

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and spread evenly with a triangular glass rod. The discshaped nanofibres were adhered to the surface of the medium and the culture dishes were incubated at 37 C for 24 h. Bactericidal kinetic study was tested by measuring the OD value of cultured bacterial suspension. Thirty milligrams of cropped nanofibre formulations were added to the sterilized culture tubes containing 10 mL of bacterial suspension (105 cfu/mL), which was cultured at 37 C for 20 h. At desired time intervals, 150 lL of bacterial suspension were collected for absorbance measurement at 600 nm (Molecular Devices, Sunnyvale, CA).

Cytotoxicity measurement of ZnONPs/AgNPs and the nanofibre formulations In this study, the potential cytotoxicity of the nanoparticles and nanofibres was evaluated against the human skin fibroblasts (HSFs). Four types of drug-containing medium, including ZnONPs, AgNPs, ZnO/Ag nanoparticles (1/1) and ZnO/Ag nanoparticles (1/3), were prepared at a concentration of 125 ng/mL (ZnO/Ag equivalent), respectively. Then, the original medium in the 96-well plates was replaced by the drugcontaining medium followed by incubation at 37 C for 2 days. Simultaneously, the sterilized nanofibre formulations were added to another 96-well plate before 100 lL of fresh medium was added. At 2- and 4-d post-treatment, the cytotoxicity of ZnONPs/AgNPs and the nanofibres was evaluated via a MTT test. The adherent fibroblasts were purged twice with PBS after the culture medium was sucked away. Another 180 lL of fresh medium was added into the wells before 20 lL of MTT regent (5 mg/mL) was added. The fibroblasts were incubated for another 4 h at 37 C. Then, 200 lL of dimethyl sulphoxide (DMSO) was added to the wells after the medium was sucked away. The absorbance was measured by a Spectra max plus microplate reader (Molecular Devices) at 490 nm.

Statistical analysis The data are expressed as the mean plus or minus the standard deviation (mean ± SD). Statistical significance of differences among groups was evaluated using one-way analysis of variance (ANOVA). Differences were considered statistically significant at p < .05.

Results and discussion Characterization of ZnONPs and AgNPs As shown in Figure 1, it can be obviously observed that ZnONPs and AgNPs were successfully prepared. The morphology of both ZnONPs and AgNPs was spherical in shape and the average diameters of ZnONPs and AgNPs were 40.07 ± 9.70 and 37.46 ± 12.02 nm, respectively. The ultraviolent-visible spectroscopy of both two types of nanoparticles was also investigated and the results were showed in Figure 1. It can be concluded that the maximum absorption band of ZnONPs and AgNPs is 379 and 417 nm, respectively.


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Figure 1. Characterization of ZnONPs and AgNPs. (A) SEM image of ZnONPs. (B) Particle size distribution of ZnONPs (n ¼ 50); (C) Ultraviolent-visible spectroscopy of ZnONPs. (D) SEM image of AgNPs. (E) Particle size distribution of AgNPs (n ¼ 50). (F) Ultraviolent-visible spectroscopy of AgNPs.

Figure 2. Optimization of nanofibre formulations on the voltage, flow rate and collected distance. The prepared nanofibres were observed by a microscope (200).

Simultaneously, the mass concentration of ZnO and Ag included in the nanopartilces was 84% and 89%, respectively.

Optimization of nanofibre formulations The effects of voltage (10, 15 and 20 kV), flow rate (0.4, 0.8 and 1.2 mL/h) and distance from the nozzle to the receiving plate (10, 15 and 20 cm) on the morphologies of electrospun nanofibres were investigated. Obviously, the nanofibres exhibited the best morphology at the voltage of 15 kV, the

flow rate of 0.8 mL/h and the distance from the nozzle to the receiving plate of 15 cm (Figure 2). Due to the high hydrophobicity of PCL, hydrophilic PVP was involved into the nanofibres to improve the swelling degree and change other properties of the formulations. To optimize the PVP/PCL proportion, the morphology, water vapour permeability and swelling degree were performed. Figure 3(A) shows the micrographs of PVP/PCL nanofibres collected on the surface of a glass slide. When high concentration of PVP was used, many fibres collected were crooked. More orderly fibres were observed and the beaded fibres



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Figure 3. Influence of PVP/PCL proportion on nanofibre formulations. (A) Micrographs of PVP/PCL nanofibres at different mass ratios. (B) Influence of various proportion of PVP/PCL on the water vapour permeability. (C) Influence of various proportion of PVP/PCL on the swelling degree. (D) Influence of various proportion of PVP/ PCL on the weight loss. p < .05; p < .01; p < .001, compared with the control group (n ¼ 3).

were disappeared gradually as the concentration of PVP decreased. And the satisfactory results were obtained in PVP/ PCL (1/3) and PCL groups. The permeability of moisture and gases (water vapour permeability) is desired in wound dressings to keep the wound comfortable. As a result, water vapour permeability of the nanofibre formulations was determined by an ASTEM E 96 desiccant method. In the study, non-woven fabrics were set as the control group [20]. It can be seen from Figure 3(B) that the water vapour permeability of pure PVP nanofibres and PVP/PCL nanofibres (3/1) was weaker than non-woven fabrics (p < .05), while the other groups including PVP/PCL (PVP/PCL ¼ 1), PVP/PCL (PVP/PCL ¼ 1/3) and PCL nanofibres were superior to the non-woven fabrics (p< .05). The highest water vapour permeability was obtained in the PVP/PCL nanofibres (1/3) group. Swelling degree and weight loss are two important parameters to evaluate the preparation of the nanofibres. The swelling degree of PVP nanofibres could not be detected because PVP was almost completely soluble in water. The addition of PVP improved the swelling degree of the nanofibres (Figure 3(C)). When the PVP/PCL proportion was 1: 3, the swelling degree reached to 200% approximately. The weight loss of

the nanofibres had positive correlation with the amount of PVP (Figure 3(D)). Compared with non-woven fabrics, PVP/ PCL (1/3) and PCL group showed the obviously lower weight loss (p< .05). Following with these findings, PVP/PCL (1/3) was performed during the electrospinning process to prepare drug-loaded nanofibres.

Fabrication and characterization of drug-loaded nanofibres Electrospinning is a feasible, efficient and economy technique that was employed to obtain nanofibres for using in many fields. We selected a 1:3 mass ratio of PVP and PCL to prepare drug-loaded nanofibres, including Ag/PVP/PCL, ZnO/ PVP/PCL and ZnO/Ag/PVP/PCL nanofibres (ZnO/Ag ¼ 1/3). The morphology of nanofibre formulations was investigated by SEM and TEM. SEM images revealed that all the nanofibres were smooth in shape, but the irregular clumps exposed outside of the fibres in ZnO/PVP/PCL and Ag/PVP/ PCL groups (Figure 4(A)), which were considered as the inhomogeneous nanofibres. In the ZnO/Ag/PVP/PCL group, the nanoparticle masses disappeared and ZnO/Ag bimetallic nanoparticles were evenly distributed in the nanofibres


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Figure 4. Morphology and in vitro characteristics of ZnO/Ag/PVP/PCL composite nanofibres. (A) Drug-loaded nanofibre formulations visualized by scanning electron microscope (SEM), Scale bar: 1 lm; arrows represent nanoparticle mass. (B) The fibre diameter distribution of drug-loaded nanofibres.

Figure 5. FT-IR analysis of the nanofibre formulations.

(Figure 4(A)). The average diameters of the nanofibres in the PVP/PCL, Ag/PVP/PCL, ZnO/PVP/PCL and ZnO/Ag/PVP/PCL groups were 391.52 ± 157.70 nm, 357.34 ± 135.90 nm, 350.85 ± 126.15 nm and 368.22 ± 123.96 nm, respectively (Figure 4(B)). In addition, the ZnO/Ag bimetallic nanoparticles were encapsulated inside the nanofibres. These findings suggested that the single metal nanoparticles clustered easily when electrospinning, which could be overcome by the combination of ZnONPs and AgNPs. FT-IR is a reliable method for analysing molecular-specific interactions in polymer blends because it is especially sensitive to polymer microstructure. As shown in Figure 5, the absorption bands of PVP/PCL nanofibres were 2944 cm1 (C-H asymmetric stretching), 2868 cm1 (C-H symmetric stretching), 1652 cm1 (C ¼ O stretching in primary amide), 1464 cm1 and 1422 cm1 (C-H deformation), 1366 cm1 (C-O stretching symmetric) and 1238 cm1 (C-O-C stretching asymmetric), respectively. After drug entrapment, Ag/PVP/PCL, ZnO/PVP/PCL and ZnO/Ag/PVP/PCL did not change the

Figure 6. DSC analysis of the nanofibre formulations.

absorption bands, suggesting that ZnONPs and AgNPs were physically entrapped in the nanofibres through van der Waals forces [21,22]. In addition, differential scanning calorimetry (DSC) was also used to investigate the thermal and crystalline properties of the nanofibres formulations. It can be seen from Figure 5 that the tested materials show the low glass transition temperature (60 C, higher than the physiological human body temperature). The exothermic peaks of ZnO/PVP/PCL nanofibres and Ag/PVP/PCL nanofibres were 361.0 and 306.7 C (Figure 6), respectively, while the exothermic peak of ZnO/Ag/PVP/PCL nanofibres was 351.6 C. This would be attributed to the formation of bimetallic nanofibres based on ZnONPs and AgNPs. The results showed that the ZnO/Ag bimetallic nanopartilces were dispersed in the nanofibres without aggregation (Figure 4). Otherwise, the aggregation leaded to reduced antibacterial efficacy [23]. After loaded into the PVP/PCL nanofibres, ZnONPs or/and AgNPs did not influence the water vapour permeability of


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Figure 7. Physicochemical properties of the drug-loaded nanofibre formulations. (A) Water vapour permeability of drug-loaded nanofibres. (B) Swelling degree of drug-loaded nanofibres. (C) Weight loss of drug-loaded nanofibres. n.s., no significance (n ¼ 3).

relative drug-loaded formulations compared with PVP/PCL nanofibres (p> .05) (Figure 7(A)). In addition, except for a high permeability and hygroscopicity, an ideal wound dressing requires a high degree of swelling and little weight loss. Similarly, in swelling degree and weight loss tests, no significant differences between the drug-loaded nanofibres and PVP/PCL nanofibres were observed (p> .05) (Figure 7(B,C)). These findings suggested that the encapsulation of ZnONPs, AgNPs or ZnO/Ag bimetallic nanoparticles does not change the physicochemical properties of PVP/PCL nanofibres.

Antibacterial activity Staphylococcus aureus (Gram positive) and Escherichia coli (Gram negative) were used to evaluate the antibacterial activity of the nanofibre formulations. Nanofibres with better antibacterial effect can promote wound healing more prominently. In order to assess the antibacterial effect, different mass ratios of ZnO/Ag in the nanofibres were performed to inhibit Staphylococcus aureus and Escherichia coli, which were used as the test organism. The results revealed that different antibacterial activities against both bacteria were obtained after treatment of ZnO- or/and Ag-loaded nanofibres (Figure 8(A)). At the same time, Ag could improve the antibacterial efficiency of ZnO based on the nanofibres. Compared with ZnO/Ag/PVP/PCL (ZnO/Ag ¼ 1/1), ZnO/Ag/ PVP/PCL (ZnO/Ag ¼ 1/3) nanofibres improved the antibacterial efficiency because of the addition of Ag. Among them, ZnO/ Ag/PVP/PCL (ZnO/Ag ¼ 1/3) group showed the best antibacterial activity for Escherichia coli. Simultaneously, ZnO/Ag/ PVP/PCL (ZnO/Ag ¼ 1/3) and Ag/PVP/PCL groups were the best two groups for Staphylococcus aureus. No antibacterial activity was observed in PVP/PCL group. The results of bactericidal kinetic study showed in Figure 8(B) and (C) reflected the growth of Staphylococcus aureus and Escherichia coli in the Mueller–Hinton broth medium. The absorbance value (OD value) increased as the bacteria grew. From the results, we could find that the growth of Staphylococcus aureus and Escherichia coli was inhibited by ZnO/Ag/PVP/PCL nanofibres (ZnO/Ag ¼ 1/3) and Ag/PVP/PCL nanofibres. ZnO/Ag/PVP/PCL nanofibres (ZnO/Ag ¼ 1/3) were superior to the single metal nanopaticles (ZnONPs or AgNPs)loaded nanofibres and ZnO/Ag/PVP/PCL nanofibres

(ZnO/Ag ¼ 1) in inhibiting bacteria. Especially for Escherichia coli, ZnO/Ag/PVP/PCL nanofibres (ZnO/Ag ¼ 1/3) showed the highest antibacterial activity. As reported, AgNPs can induce bacteria death by destroying cell wall or membrane, disturbing protein synthesis and processing, preventing DNA replication and disturbing the antioxidative system [11,12]. Ag þ ions released from AgNPs can attach directly onto cell surfaces and change the membrane permeability, resulting in induction and accumulation of intracellular ROS. On the other hand, ZnONPs are also a well-known antibacterial material that produces ROS to attack the bacterial cells. In our study, hybrid ZnO/Ag nanosystems were shown to be more efficient than single components (ZnONPs or AgNPs) due to synergistic effects of bimetallic combination [24]. Moreover, Ag ions can enhance the antimicrobial activity of ZnO by ROS production [11,17]. Therefore, the enhancement of antibacterial activity induced by the incorporated metal-loaded nanofibres may be caused by the increased oxidative stress followed by cell damage.

Cytotoxicity of ZnO/Ag/PVP/PCL nanofibres In the study, the MTT test was used to evaluate potential cytotoxicity of the prepared nanofibres, including PVP/PCL, ZnO/PVP/PCL, Ag/PVP/PCL, ZnO/Ag/PVP/PCL (ZnO/Ag ¼ 1) and ZnO/Ag/PVP/PCL nanofibres (ZnO/Ag ¼ 1/3). The ZnONPs alone showed slight cytotoxicity towards HSF cells at a concentration of 125 ng/mL (Figure 9(A)), while reducing the amount of ZnO (the mixed nanoparticles) could increase the cell viability (p