Bacterial Stress and Osteoblast Responses on Graphene Oxide-Hydroxyapatite Electrodeposited on Titanium Dioxide Nanotube Arrays

To develop bone implant material with excellent antibacterial and biocompatible properties, nanotubular titanium surface was coated with hydroxyapatite (HA) and graphene oxide (GO). Layer-by-layer deposition was achieved by coating HA on an anodic-grown titanium dioxide nanotube array (ATi) with electrolytic deposition, followed by coating with GO using anodic-electrophoretic deposition. The antibacterial activity against both Gram-negative (Escherichia coli) and Gram-positive (Staphylococcus aureus) bacteria was determined based on the percentage of surviving bacteria and the amount of ribonucleic acid (RNA) leakage and correlated with membrane disruption. The oxidative stress induced in both strains of bacteria by GO was determined by cyclic voltammetry and is discussed. Importantly, the antibacterial GO coatings on HA-ATi were not cytotoxic to preosteoblasts and promoted osteoblast proliferation after 5 days and calcium deposition after 21 days in standard cell culture conditions.


Introduction
Hydroxyapatite (HA, Ca 10 (PO 4 ) 6 (OH) 2 ) is a mineralogic component of natural bone with a molar calcium to phosphate ratio of 1.67 [1].Several methods for coating HA onto biomaterial surfaces include plasma spray, microarc oxidation, and electrodeposition.Electrodeposition is an easy method that allows for adjustment of the thickness and porosity of the HA coating, increased corrosion protection, and reduced release of metal ions by changing systemic parameters.HA may be electrodeposited on an anodic-grown titanium dioxide (TiO 2 ) nanotube array on titanium (Ti), which is widely used in orthopedic implants to form a direct bone-to-metal interface, referred to as osseointegration [2,3].TiO 2 nanotubes fabricated by anodization are highly ordered and highly adhesive to the substrate due to the intrinsic chemical bonds between the nanotubes and Ti.
Bioactive HA has been widely used as a coating material for dental and orthopedic implants for many years, but by itself, it does not prevent bacterial infection after implantation.Infections associated with surgical implants are generally difficult to be suppressed and may require a longer period of antibiotic therapy and repeated surgical procedures [4].Antibacterial property of HA coating could be improved by adding other nanomaterials such as graphene oxide.
Graphene oxide (GO) has antibacterial activity that can reduce the risk of bacterial infection.GO nanosheets inhibit bacterial growth [5,6].GO coatings also promote osteoblast function and the antibacterial properties of implant materials [3,[6][7][8].A hydrothermal synthesized nanocomposite of HA nanorods on GO sheets showed faster adsorption of bovine serum albumin in adsorption-desorption process on its surface [9].Such nanocomposite was suitable for drug delivery due to its biocompatibility, high drug loading efficiency, and biodegradability.The nanocomposite of HA on reduced GO was also used as enzymatic electrochemical glucose biosensors which exhibited a superior detection limit and higher sensitivity [10].Graphene cytotoxicity in neural cells is due to the production of reactive oxygen species (ROS) in a concentration-and time-dependent manner [11,12].The antibacterial mechanism of another carbon-based nanomaterial, carbon nanotubes (CNTs), is induced by oxidizing a cellular structure or component of bacteria with CNTs [13].For example, the increased cytotoxicity of single-walled CNTs might be due to an increase of in cellular oxidative stress and a loss of cell membrane integrity [14].It remains unclear, however, whether intracellular ROS are most likely induced by external ROS produced by GO outside of the bacteria or whether intracellular ROS are directly produced by the GO surface.
Oxidative stress (or ROS formation) generated from other carbon nanomaterials, such as graphene [12], fullerene [15], and CNTs [16], is a key antibacterial mechanism.Many studies have measured oxidative stress and its relationship to disease, such as in acute pancreatitis and hemorrhagic shock syndrome [17,18].In the present study, electrochemical method was used to indirectly detect ROS in bacteria on the electrodeposited GO coatings.Once ROS react with an electron-acceptor protein at the cell membrane, an electrical signal is detected from the bacteria-seeded electrode in an electrochemical cell.Here, oxidative stress in both Gram-positive (Staphylococcus aureus) and Gram-negative (Escherichia coli) bacteria was studied after they colonized on GO coatings after 24 h.In addition, preosteoblast (MC3T3-E1) cell proliferation and calcium deposition under standard cell culture condition were examined to determine the early osteoblast response to electrodeposited GO coatings in vitro.

Experimental Materials and Methods
2.1.Anodic-Electrophoretic Deposition of Graphene.GO solutions were prepared by dispersing GO in isopropyl alcohol (Ajax Finechem, New Zealand) at concentrations of 50, 100, 150, and 200 g ml −1 , named GO1, GO2, GO3, and GO4, respectively.GO was deposited by anodic-electrophoretic deposition on HA-ATi samples prepared as described previously [3,19].A direct current of 10 V was applied at room temperature for 10 min during anodic-electrophoretic deposition.HA-ATi layers without GO (GO0) were used as a control.

Physical and Chemical
Characterizations.The surface morphology of the coatings was characterized by scanning electron microscopy (SEM, CamScanMX2600, UK) with a 10 keV electron beam.The amount of GO was indirectly analyzed using image analysis software (ImageJ version 1.32, Montgomery, National Institutes of Health, Maryland).The crystal structures of the coating were examined using an Xray diffractometer with CuK1 radiation (Shimadzu Model: XRD 6000, Japan) at a scanning rate of 1 ∘ /min.

Bacterial
Responses.All samples were tested against S. aureus and E. coli bacteria as Gram-positive and Gramnegative models, respectively.The bacteria were cultured in Mueller-Hinton broth (Thailand Science Park, Thailand) at 37 ∘ C for 24 h with shaking at 200 rpm.The bacteria were then centrifuged at 5000 rpm for 5 min.The bacteria pellet was added to 10 ml sterilized saline solution to reach a concentration of bacteria of 10 6 colony forming units (CFU) per milliliter.

Antibacterial Drop Test.
Each sample was placed into a sterilized 24-well plate.Then, 100 l of diluted bacterial suspension was spread on the surface of the sample.After sonication of the sample at 37 ∘ C for 60 min, the bacteria were washed from the surface of the sample with 1.5 ml sterilized phosphate-buffered saline (PBS) in the sterilized 24-well plate.Then, 50 l of each bacterial suspension was added to Mueller-Hinton broth and incubated at 37 ∘ C for 24 h to measure bacterial absorbance using a spectrophotometer, and percent of relative bacterial cell survival was calculated (1).The reported data are the mean value of three independent experiments.

Measurement of Ribonucleic Acid (RNA)
Efflux.First, the media remaining from oxidative stress measurement of each sample were centrifuged at 13,000 rpm for 2 min.The supernatant of the solution was then used to measure the RNA efflux of the bacteria.RNA was separated using a RNA purification kit (RBC Bioscience, Taiwan) in which singlestranded RNA and double-stranded RNA of more than 200 to 1000 of base pairs in length were efficiently purified.Elution solutions of RNA were measured to determine the RNA concentration with a microplate reader (Infinite5 200 PRO NanoQuant, Switzerland).

Determination of Bacterial Oxidative Stress Using the Electrochemical Method
(1) Preparation of Samples for Electrochemical Measurements.
Oxidative stress was studied electrochemically using cyclic voltammetry (CV) technique.CV analysis was selected as a reliable and effective method to measure oxidative stress without pretreating the sample surface or using any specific chemical before analysis.Effects of various GO concentrations and initial-seeding cell concentrations on oxidative stress in bacterial cells were studied.The oxidation measurement area, 0.25 cm 2 , was controlled by coating with corrosion-protective paint (Jotun, Thailand), as shown in Figure 1.Prior to testing with bacteria, sterilized samples were exposed to 30,000 WS cm −2 of 254 nm UV energy (JKL, USA) for 4 h on each side.
(2) Culture of Bacterial Cells for Electrochemical Measurements.The samples (Figure 1) were placed in a sterilized 24-well plate.Then, 1 ml of the diluted bacterial suspension (10 6 CFU ml −1 ) was spread onto the sample surface.The bacteria were cultured in Mueller-Hinton broth at 37 ∘ C for 24 h at an angular velocity of 200 rpm.The samples were placed in a three-electrode electrochemical system to measure oxidative stress.Bacteria absorbance in the medium of each sample was measured using a microplate reader (Infinite5 200 PRO NanoQuant, Switzerland).Relative bacterial cell survival was calculated using (2).The mean percent of relative cell survival was determined from three independent experiments.

Relative cell survival (%) =
Absorbance of sample × 100% Absorbance of control (polystyrene plate) . ( (3) Cyclic Voltammetry.A three-electrode electrochemical system was used in this study.France) and 1 vol% penicillin/streptomycin (Invitrogen Corporation).Cells were cultured at 37 ∘ C in a humidified atmosphere of 5% CO 2 in air and media were replaced every 3 days.

Cell Viability.
Cells were subcultured through trypsinization (0.25% trypsin and 0.53 M EDTA; Invitrogen Corporation) and then seeded onto plastic polystyrene (control) at a density of 4 × 10 4 cells cm −2 in 24-well culture plates.Cell viability was tested using a commercial MTT assay (Sigma-Aldrich, Thailand).The 10 vol% solution of MTT in 1x phosphate buffer saline was mixed with alpha-MEM without phenol red to form a yellowish solution before being added to the cell-seeded samples at day 5 of the culture.Mitochondrial dehydrogenases of viable cells cleave the tetrazolium ring, yielding purple formazan crystals on cell-seeded samples after incubation for 1 h.The blue formazan crystals trapped in the cells were dissolved in sterile DMSO (100 l) by incubating at 37 ∘ C for 30 min.Absorbance of the purple solution was measured at 550 nm using a spectrophotometer (Synergy Mx Multi-Mode Reader, US).A concomitant change in the amount of formazan formed correlates to the change in the number of viable cells in the samples.Therefore, the percentages of viable cells in the samples are calculated as shown in Cell viability (%) = Absorbance of colored solution incubated with samples × 100% Absorbance of colored solution incubated with control (polystyrene plate) . (3)
(2) Cell Lysis and Calcium Content Analysis.After removing the culture media and washing the samples with PBS, 200 l SDS lysis buffer was added to each sample.The samples were shaken using an orbital shaker at an angular velocity of 200 rpm for 5 min and then incubated in a CO 2 incubator at 37 ∘ C for 1 h.Incubated samples were placed into a mixture of 5 N HCl solution (Ajax Finechem, New Zealand) and the cell lysate, with a fixed ratio as 250 l of 5 N HCl per 1 ml of cell lysate.The solution was mixed with the samples using an orbital shaker at 200 rpm for 5 min.The samples were then incubated at 4 ∘ C for 4 h.Calcium quantification was performed after cell lysates were incubated more than 4 h.The cell lysates were then mixed with ethanolamine buffer as 10 l per 1000 l in autoclaved microcentrifuge tubes, and 100 l ortho-cresolphthalein (0.63 mM; Sigma-Aldrich) was added to the ethanolamine and cell lysate solution in microcentrifuge tubes to obtain a purplish red color of solution.The light absorbance of calcium in the supernatant was measured using a microplate reader at a wavelength of 570 nm.The calcium concentration was calculated according to a standard curve generated from a serial dilution of standard calcium solutions.Calcium content was reported as micrograms of calcium per square centimeter of the sample area (g cm −2 ).Nine samples in each group were tested at culture day 21.The experiment was repeated three times.

Statistical Analysis.
Analysis of variance (ANOVA) and independent-samples t-test were used with Minitab5 16 (Minitab Inc., USA).A probability of 0.05 was considered statistically significant.

Anodic-Electrophoretic Deposition of a Graphene Oxide and Hydroxyapatite
Coating.SEM images of GO coatings on HA-ATi by anodic-electrophoretic deposition are shown in Figures 2(a)-2(e).The SEM images show thin layers of GO coatings on top of HA layers.Our previous study confirmed the presence of the carbon content of the GO on the coatings after electrodeposition by energy-dispersive X-ray and Fourier transform infrared spectroscopy [10].In the present study, quantitative analysis of the carbon content was conducted by indirectly measuring HA intensity using ImageJ.The results in Figure 2 suggest that the HA content decreases when the electrodeposited GO content increases, and the highest GO content was found on the GO4 sample (200 g ml −1 ) compared to the other coatings.This implies that a thick GO coating is obtained when using a high concentration of GO in the electrolyte during the electrophoretic deposition process.The crystal structures of the samples in the present study were analyzed using XRD, as shown in Figure 3.The results of XRD spectra confirmed that the layers of HA (Ca 10 (PO 4 ) 6 (OH) 2 ) and TiO 2 (anatase phase) existed on all surfaces; however, the intensity of their peaks was lower on the GO-coated samples.In our previous work, XRD spectrum of GO powder (before electrodeposition) showed a peak at two Theta = 10.16 ∘ [21].However, the XRD patterns of GO1, GO2, GO3, and GO4 samples (Figure 3) did not show the peaks at two Theta range of 10-12 ∘ .The previous study reported that the absence of the peak at two Theta approximately to 10-12 ∘ was found in reduced GO [22].It is possible that reduced GO coating is formed after the electrophoretic deposition in the present study.In addition, if GO content in coating is less than 5 wt%, its peak would not show due to limitation of the technique.Although the GO peaks did not appear, it may be implied from XRD patterns that GO existed on the surface due to reduction of apatite and anatase peaks with an increase of GO content used in the anodic-electrophoretic deposition.The reduction of the peaks may be resulted from an increase of GO concentration on the coatings.

Measurements of Bacterial Survival and RNA Leakage.
GO0 samples had weak antibacterial activity.The GO-coated samples, however, exhibited considerable antibacterial activity.Specifically, after 1 h of culture, 98% (GO1), 49% (GO2), 34% (GO2), and 37% (GO4) of the E. coli survived on the surface of the GO-coated samples.Figure 4 shows similar results for S. aureus.Similar to E. coli, the GO was toxic to S. aureus.The GO exhibited stronger antibacterial activities against S. aureus than against E. coli.In fact, only 86% (GO1), 57% (GO2), 23% (GO3), and 26% (GO4) of the S. aureus survived on the GO surface after 1 h of culture.Although electrodeposited GO on HA-ATi was toxic to both types of bacteria, it was more toxic to the Gram-positive (S. aureus) bacteria.
The results confirmed that the GO-coated samples reduced bacterial survival.The mechanisms to kill the bacteria were likely oxidation and membrane disruption.Therefore, the toxicity of the samples to bacteria through membrane damage can be investigated by measuring intracellular materials such as RNA in the supernatant surrounding the bacteria exposed to the GO-coated samples [9].Thus, the efflux of the cytoplasmic materials of the bacteria was examined by measuring the concentration of RNA in the solution (Figure 4).The RNA concentrations in the solutions of bacteria exposed to GO-coated samples at each concentration were significantly higher than that of the control samples (GO0), except that for GO1 against E. coli bacteria.This is due to direct contact between GO and bacteria causing RNA leakage.Because GO has extremely sharp edges, it could damage the bacterial membrane [23].In the present study, when the GO concentrations increased, RNA leakage also increased.
The RNA effluxes from S. aureus exposed to GO were significantly higher than those of E. coli under the same culture conditions.This may be due to the greater resistance of E. coli in direct contact with the edge of the GO compared with S. aureus.Although S. aureus is a Gram-positive bacteria whose peptidoglycan layer provides additional strength to the cell wall, which is also thicker (20-80 nm) than that of E. coli (Gram-negative) bacteria (7-8 nm) [9,24,25], the S. aureus was less resistant than E. coli.Gram-negative E. coli has a much thinner layer of peptidoglycan, but it also has a layer of lipopolysaccharides that might protect the cell.A previous report indicated that E. coli exhibited more resistance to direct contact interaction induced by an atomic force microscopy tip than S. aureus due to the outer membrane of the Gram-negative E. coli bacteria [26].Moreover, comparison between the stiffness of Grampositive and Gram-negative bacterial cells suggested that, for these particular strains of bacteria, the stiffness of S. aureus (95 MPa) was lower than that of the E. coli (220 MPa) [27].
Therefore, E. coli should be more resistant to membrane damage than S. aureus.

Determination of Bacterial Oxidative Stress
Using the Electrochemical Method.Bacterial survival percentages of S. aureus and E. coli were presented in Figure 5(a).GO0 samples exhibited weak antibacterial activity for both bacteria strains.In contrast, GO-coated samples exhibited considerable antibacterial activity based on a toxicity test.The number of both bacterial species was significantly reduced with an increase in the GO concentration.Relative survival of bacteria on the GO3 sample, however, did not differ significantly from that on the GO4 sample ( > 0.05).Antibacterial activities against S. aureus of the GO-coated samples were stronger than those against E. coli.Importantly, GO on HA-ATi samples was more toxic to Gram-positive S. aureus than Gramnegative E. coli.The exact mechanism of damage to the bacteria remains unclear.There are other models, however, suggesting that bacterial adhesion is influenced by some force factors such as electrostatic forces, van der Waals forces, hydrophobic forces, hydrogen bonding, and covalent bonding of bacterial cells and substrates [28,29].Mafu et al. reported that the first and the most important such force was the electrostatic force of charges between the surface substrate and bacterial membrane [29].They show that GO being negatively charged due to the presence of carboxyl, hydroxyl, and epoxy groups is less repulsive to Gram-positive bacteria than Gram-negative bacteria [25].
CV is fundamental electrochemical method, applied for many electrochemical characterizations.This technique can be used to analyze oxidation/reduction behaviors or antioxidants without requiring any pretreatment, catalysts, or use of specific reagents [30].CV was used in this study to demonstrate the oxidation signals of both S. aureus and E. coli after treatment with different GO concentrations on HA-ATi (Figures 5(b [31].The other controls were samples without an oxidation reaction in PBS solution.There was no oxidation peak but there was a reduction peak, which may be due to the reduction of some of the C-C bonds of GO detected in PBS (Figure 6(b)).Such behavior was previously by Kamyabi Shafiee [32].
Furthermore, a shift in the higher oxidation current with an increase in GO concentration was observed (Figures 5(b)-5(c)).For a better understanding of the induced oxidative stress, voltammograms were replotted to compare peak currents, which are representatives of the oxidative power of the materials on each bacterial species, with the GO concentrations (Figure 7).An increase in the GO concentration increased the oxidative current peaks in S. which can explained in two ways.First, it is possible that a high GO concentration causes high oxidative stress, resulting in high oxidation peak [8].Second, the increase of GO concentration increased an electrical conduction between bacteria and electrode when GO was used as the mediator of the sensor system [34].The effect of GO concentration on peak current for E. coli, however, was much lower.As discussed previously, the cell membrane of each bacterium affects adhesion to the substrate.For S. aureus, there was a higher potential to adhere on the surface, as shown in the cyclic voltammograms (Figure 7).
To better understand the oxidative stress mechanism, more studies of this bacterial process are needed.Moreover, these GO-coated samples show the potential to be used as sensors to detect biological matter [12].In situ diagnosis using this GO-coated material will be a new trend for an implantable label-free sensor.Biocompatibility testing will be required to develop this new potential use of this novel material.

Preosteoblast Proliferation (MTT Assay).
To evaluate the biological responses to biomaterials, the osteoblast cell density of 4 × 10 4 cells cm −2 was seeded on samples in each well.An MTT test was performed to evaluate cell viability.Cell viability was higher in GO3 than in the other samples (Figure 8).Although MTT activity on HA-ATi (GO0) was high, it was still lower than those on the other GO-coated samples.Thus, the GO did not exert any cytotoxic effects on the cells and actually promoted osteoblast cell attachment and proliferation.Several previous reports focused primarily on the biocompatibility of GO films [14,35,36].The results of the previous studies are generally consistent with those of the present study with regard to the finding that GO film enhances mammalian cell proliferation.Taken together, these findings indicate that GO supports osteoblast growth and proliferation.GO effects on cellular inhibition are dosedependent, as reported by Chang et al. [14].They found that the GO did not enter A549 (adenocarcinoma human alveolar Percentages of cell viability were analyzed using absorbance at 550 nm.The  value was calculated using an independent-samples t-test;  = 3;  = 3; *  < 0.05. basal epithelial cells) and had no obvious cytotoxicity.GO causes dose-dependent oxidative stress in the cell and high concentrations of GO induce a slight loss of cell viability.Moreover, Wojtoniszak et al. reported that GO at concentrations ranging from 3.125 to 25 g ml −1 exhibited the best biocompatibility with mouse L929 fibroblast cells [37].
The osteoblast cell membrane has the same negative charge as bacterial cell membranes.The negative charge is due to phosphate groups on the bilayers.The charge of the membrane protein does differs, however, from that of the extracellular matrix.To adhere onto negatively charged surfaces, Gongadze et al. reported that the mechanism was established in two steps [38].The cell membrane makes nonspecific contact caused by electrostatic forces.Positively charged proteins then attach to the negatively charged surface, followed by specific binding involving an integrin assembly [39].A number of questions arise regarding the protective mechanism that preosteoblast cells use to protect themselves from GO. Almeida reported that, to prevent oxidative stress, cells utilized diverse mechanisms involving both enzymatic reactions and altered gene transcription [40].These mechanisms are superior to those of bacteria with respect to stability and high reducing power.In another study, glutathione reductases from Saccharomyces cerevisiae and E. coli were rapidly inactivated following aerobic incubation with NADPH, NADH, and several reductants in a time-and temperature-dependent manner [41].Therefore, to eliminate the effect of ROS inside the cells, ROS reduction in mammalian cells must be easier than that in bacteria.The toxicity of GO nanomaterials, however, is concentration dependent for both bacterial and mammalian cells.

Preosteoblast Differentiation (Calcium Deposition).
Proliferation of osteoblasts on material surfaces alone, however, is not sufficient to achieve long-term osseointegration for orthopedic implants.order of days to weeks) functions of osteoblasts on the GOcoated HA-ATi materials were investigated using a calcium deposition assay.The mineralization process of preosteoblasts in in vitro culture was used as a model to test the effects of biomaterial surfaces on bone cell differentiation and bone formation.Calcium deposition is an indicator of successful in vitro bone formation and can be measured specifically by calcium deposition assay [1].
A calcium deposition assay was performed to evaluate different GO-coated HA-ATi surfaces.For any test period, there were barely detectable amounts of calcium deposited on the polystyrene substrates (Figure 9).The calcium content in the extracellular matrix in all samples in this study was significantly ( < 0.05) greater than that on polystyrene substrate formulations after 21 d of culture.The GO3 surface had the highest ability to support the mineralization of preosteoblast cells after 21 d.Moreover, compared with GO0, the calcium content in the extracellular matrix for GO3 was significantly ( < 0.05) greater after culture for 21 d.
The findings of the present study supported previous cell proliferation studies indicating that GO3 exhibited the highest potential to support cell growth compared with the other concentrations of GO.Proliferation and differentiation showed similar trends.At the beginning, cell-biomaterial interactions during the first period (such as cell adhesion and proliferation) could affect long-term cell function, such as synthesis of extracellular matrix proteins or calcium deposition [42,43].
The effect of GO-coated HA-ATi on bacterial behavior and the response of preosteoblast cells are summarized in Table 1.The cytotoxic effects of the materials on cell survival were classified as medium if cell survival was lower than 70% according to the ISO 10993-5 standard [44].In the cases of GO0 and GO1, there was no sign for toxicity toward MC3T3-E1, S. aureus, and E. coli.High GO concentrations (GO2, GO3, and GO4) exhibited slightly toxic effects on both types of bacteria (S. aureus and E. coli.), but not for MC3T3-E1.These findings indicated that biomaterials coated with GO2, GO3, and GO4 had antibacterial properties.Moreover, they were cytocompatible with preosteoblast cells and promoted cell proliferation and calcium deposition.
Importantly, the highest cell viability and calcium deposition were observed for GO3.Thus, this novel material has the potential to promote osseointegration of surrounding bone cells.The results of the in vitro study revealed that GOcoated HA-ATi enhanced long-term functions (specifically, concentration of calcium deposition) of preosteoblasts when the GO concentration in electrolyte was 150 g ml −1 .More studies of long-term osteoblast cultures are needed to ensure differentiation on GO-HA-ATi.The cytotoxicity of GO is expected to differ significantly from that of widely studied three-dimensional CNTs [45].The two materials have a similar crystalline structure, however, but a different shape (flat atomic sheets for GO and tubular for nanotubes).Zhang et al. studied GO interactions with neuron-like cells (PC12) in vitro and found that GO cytotoxicity in PC12 cells was relatively low compared with CNT; both GO and CNT induced concentration-and shapedependent cytotoxic effects [11].Zhang et al. [11] also suggested that fibroblast adhesion and proliferation should be studied in addition to preosteoblasts to examine the integration between implants with the surrounding soft tissues.Moreover, the solubility of GO composite in stimulated body fluid solution should be tested to confirm the stability of this composite material in the host [46].

Conclusions
The antibacterial properties and osteoblast response (proliferation and calcium deposition) of GO on HA-ATi samples were studied.The GO coatings on HA-ATi were prepared using anodic-electrophoretic deposition.Various GO concentrations in electrolytes were used to deposit GO nanowalls on HA-ATi.Based on the antibacterial drop test, GO reduced the growth of bacteria in both strain models: S. aureus and E. coli.The results of RNA leakage tests revealed that direct contact of the bacteria with GO causes membrane stress, leading to irreversible damage.The RNA efflux indicated greater damage to the cell membrane of S. aureus compared with the cell membrane of E. coli.The higher resistance of E. coli against interaction with the nanowalls compared with S. aureus might be due to the greater stiffness of E. coli.The increased current density of oxidative peaks in the CV tests in this study positively correlated with the number of surviving bacteria, suggesting that the increase in cytotoxicity was due to an increase in cellular oxidative stress (similar to the result of membrane stress causing RNA leakage).Therefore, the findings of the present study indicated that survival of bacteria, oxidative stress, and membrane stress were GO-concentration-dependent mechanisms.The results also suggested that GO-HA composite coatings decreased susceptibility to both S. aureus and E. coli and thus could be applied as effective antibacterial agents to suppress bacterial invasion in orthopedic implants.Moreover, the osteoblast responses demonstrated that the GO-HA composite coatings increased osteoblast proliferation after 5 d of cultures.The results from the calcium deposition assay after culture for 21 d confirmed that GO-HA composite coatings supported an early stage of osteoblast differentiation.Electrodeposited GO at concentrations of 150 g ml −1 and 200 g ml −1 was found to be optimal in this study because GO coatings at these concentrations induced cell death in both strains of bacteria but promoted high proliferation and calcium deposition of preosteoblasts.Therefore, GO electrodeposited on HA-ATi are very promising not only for antibacterial applications, but also for orthopedic applications.Further in vitro studies and in vivo studies are needed to examine long-term osteoblast differentiation, protein, and gene expression of osteoblasts.

Figure 1 :
Figure 1: Scheme of sample preparation for electrochemical measurements.

Figure 2 :Figure 3 :Figure 4 :
Figure 2: SEM micrographs of GO coated on HA-ATi in a layer-by-layer deposition method on (a) HA-ATi or GO0 and HA-ATi coated with various GO concentrations.(b) GO1; (c) GO2; (d) GO3; (e) GO4.Inset micrographs show ImageJ analysis of the figures; (f) a comparison of HA intensity, derived from ImageJ analysis.The  value was calculated using one-way ANOVA;  = 3, *  < 0.05.Scale bars are 5 m.

Figure 5 :
Figure 5: (a) Cytotoxicity of GO coating on HA-ATi to E. coli and S. aureus exposed to various concentrations of GO coating on HA-ATi samples, for 24 h.The  value was calculated using one-way ANOVA;  = 3; *  < 0.05.Cyclic voltammograms of detected (b) S. aureus and (c) E. coli ROS.The bacteria were incubated on GO-HA-ATi and CV was measured in PBS electrolyte at room temperature after 24 h.

Figure 6 :
Figure 6: (a) Cyclic voltammograms of the Fe(CN) 6 4−/3− redox system were used as a positive control and (b) samples without adhered cells in PBS solution were used as a negative control.

2 )Figure 7 :
Figure7: Plot of the samples with anodic peak current analysis.A  value was calculated using one-way ANOVA;  = 3; *  < 0.05 when compared with coating incubated with S. aureus.* * ,#  < 0.05 when compared with coating incubated with E. coli.

Figure 8 :
Figure 8: MTT test on osteoblast cultures 5 d after cell seeding.Percentages of cell viability were analyzed using absorbance at 550 nm.The  value was calculated using an independent-samples t-test;  = 3;  = 3; *  < 0.05.