Chlorogenic Acid Entrapped in Hybrid Materials with High PEG Content: A Strategy to Obtain Antioxidant Functionalized Biomaterials?

The formation of pro-oxidant species after implantation of biomaterials could be responsible for the failure of the implant itself, because of oxidative stress-induced damage. In this work, the SiO2/polyethylene glycol (PEG)/chlorogenic acid (CGA) hybrids synthesized by the sol–gel method with 50 wt% of the polymer and different amounts of CGA (5, 10, 15 and 20 wt%) were studied. The hybrids soaked in simulated body fluid (SBF) showed the formation of hydroxyapatite layers on their surface, suggesting that the hybrids are bioactive. Their radical scavenging capacity towards DPPH· and ABTS·+ (2,2′-Azino-bis(3-ethylbenzthiazoline-6-sulfonic acid), evaluated at three different doses (0.5, 1 and 2 mg), showed probe- and dose-dependent behavior. In addition, the antioxidant properties of CGA were not affected by the presence of high amounts of the polymer. The in vitro biocompatibility in three cell lines (NIH 3T3, HaCaT and SH-SY5Y) was assessed by using the 3-(4,5-dimethyl-2-thiazolyl)-2,5-diphenyl-2H-tetrazolium bromide (MTT) assay. Apart from SH-SY5Y, the cell viability—expressed as mitochondrial redox activity percentage of cells directly exposed to powders—and morphology was not affected, suggesting that the hybrids have the ability to interfere and act selectively against tumor cells. The antibacterial properties of the different materials against Escherichia coli and Enterococcus faecalis were affected by different amounts of the natural antioxidant component.


Introduction
Under physiological conditions within the human body, cells are able to counteract the production of free radicals thanks to various enzymes that manage the redox homeostasis. However, when the biological repairing mechanisms are not sufficient and/or pro-oxidant species are overproduced, the homeostatic processes fail and the pro-oxidative/antioxidative cellular balance is compromised. In this condition, called 'oxidative stress', reactive oxygen species (ROS), nitrogen species (RNS) and consequently lipid peroxidation (LPO) products promote cellular injury and tissue damage [1,2].
Oxidative stress represents one of the main factors that negatively affect the tissue response to implantation of biomaterials, in that they are able to stimulate the formation of pro-oxidant species,

UV-Vis Spectra
The UV-Vis spectra of extracts from hybrids were recorded. To this purpose, powders of synthesized materials (100.0 mg) underwent solid-liquid extraction through ultrasound-assisted maceration (Advantage Plus model ES, Darmstadt, Germany). The extraction was carried out for 1 h using a hydroalcoholic solution (EtOH:H2O, 1:1, v:v; 2.0 mL) as extractant. After centrifugation at 4500 rpm for 5 min, collected supernatants were dried by a rotary evaporator and reconstituted in pure EtOH (1.0 mg/mL). UV-Vis spectra were acquired in the range 200-600 nm by a Shimadzu UV-1700 double beam spectrophotometer (Kyoto, Japan).

Bioactivity Test
The bioactivity of the different materials was evaluated using the simulated body fluid (SBF) solution [15], in which the ion concentration is nearly equal to that in human blood plasma. The formation of hydroxyapatite on the material's surface was observed by Quanta 200 SEM (FEI, Eindhoven, the Netherlands), equipped with an energy-dispersive X-ray (EDX), after soaking in SBF for 21 days at 37 °C. The reaction of hydroxyapatite nucleation is affected by the total surface area of the material exposed to SBF and its volume; thus, a constant ratio was maintained, according to the literature [15][16][17]. Also, apatite layers on the hybrid materials were analyzed by XRD analysis using a Philips 139 diffractometer, equipped with a PW 1830 generator, a tungsten lamp and a Cu anode, where the source 140 of the X-ray is given by the Cu-Kα radiation (λ = 0.15418 nm).

Antiradical Capacity Assessment
DPPH and ABTS direct contact tests were used to evaluate the radical scavenging capacity of synthesized materials (0.5, 1.0, and 2.0 mg). Briefly, a methanolic solution of DPPH (9.4 × 10 −5 M; 1.0 mL final volume) was added directly to the powders of hybrid materials. The samples were thoroughly stirred and allowed to react for 30 min at 25 °C. Then, absorbance at 515 nm was measured in reference to a blank, using a Perkin-Elmer Victor3 multi-label reader. Analogously, an ABTS radical cation solution in PBS (pH 7.4; 1.0 mL final volume) was in direct contact with the materials for 6 min, after which the absorbance at 734 nm was measured, versus a blank. The results were

UV-Vis Spectra
The UV-Vis spectra of extracts from hybrids were recorded. To this purpose, powders of synthesized materials (100.0 mg) underwent solid-liquid extraction through ultrasound-assisted maceration (Advantage Plus model ES, Darmstadt, Germany). The extraction was carried out for 1 h using a hydroalcoholic solution (EtOH:H 2 O, 1:1, v:v; 2.0 mL) as extractant. After centrifugation at 4500 rpm for 5 min, collected supernatants were dried by a rotary evaporator and reconstituted in pure EtOH (1.0 mg/mL). UV-Vis spectra were acquired in the range 200-600 nm by a Shimadzu UV-1700 double beam spectrophotometer (Kyoto, Japan).

Bioactivity Test
The bioactivity of the different materials was evaluated using the simulated body fluid (SBF) solution [15], in which the ion concentration is nearly equal to that in human blood plasma. The formation of hydroxyapatite on the material's surface was observed by Quanta 200 SEM (FEI, Eindhoven, the Netherlands), equipped with an energy-dispersive X-ray (EDX), after soaking in SBF for 21 days at 37 • C. The reaction of hydroxyapatite nucleation is affected by the total surface area of the material exposed to SBF and its volume; thus, a constant ratio was maintained, according to the literature [15][16][17]. Also, apatite layers on the hybrid materials were analyzed by XRD analysis using a Philips 139 diffractometer, equipped with a PW 1830 generator, a tungsten lamp and a Cu anode, where the source 140 of the X-ray is given by the Cu-Kα radiation (λ = 0.15418 nm).

Antiradical Capacity Assessment
DPPH and ABTS direct contact tests were used to evaluate the radical scavenging capacity of synthesized materials (0.5, 1.0, and 2.0 mg). Briefly, a methanolic solution of DPPH (9.4 × 10 −5 M; 1.0 mL final volume) was added directly to the powders of hybrid materials. The samples were thoroughly stirred and allowed to react for 30 min at 25 • C. Then, absorbance at 515 nm was measured in reference to a blank, using a Perkin-Elmer Victor3 multi-label reader. Analogously, an ABTS radical cation solution in PBS (pH 7.4; 1.0 mL final volume) was in direct contact with the materials for 6 min, after which the absorbance at 734 nm was measured, versus a blank. The results were expressed in terms of the percentage decrease of the initial DPPH or ABTS + absorption by the test samples [8].

Cell Culture and Cytotoxicity Assessment
Cytotoxicity was measured via the MTT cell viability assay using the HaCat human keratinocyte, NIH-3T3 murine fibroblast and SH-SY5Y human neuroblastoma cell lines. All the cell lines were grown in Dulbecco's Modified Eagle Medium supplemented with 10% fetal bovine serum, 50.0 U/mL penicillin, and 100.0 µg/mL streptomycin, at 37 • C in a humidified atmosphere containing 5% CO 2 . The powders of each synthesized material (0.5, 1.0 and 2.0 mg) were placed in 12-well plates and the cells were seeded (3.5 × 10 5 cells/well). After 48 h of incubation, cells were treated with MTT (500 µL; 0.50 mg/mL), previously dissolved in culture media, for 2 h at 37 • C in a 5% CO 2 humidified atmosphere. The MTT solution was then removed and DMSO was added to dissolve the original formazan. Finally, the absorbance at 570 nm of each well was determined using a Victor3 Perkin Elmer fluorescence and absorbance reader. The cell viability was expressed as a percentage of mitochondrial redox activity of the cells directly exposed to powders, compared to an unexposed control [10].
The bacterial culture was diluted in distilled water to produce a bacterial cell suspension of 10×10 5 CFU/mL. E. coli was inoculated in TBX Medium (Tryptone Bile X-Gluc) (Liofilchem, Roseto degli Abruzzi (Te), Italy), while, E. faecalis was inoculated in Slanetz Bartley Agar Base (Liofilchem, Italy) in presence of 100 mg of the hybrid powders. Afterward, the bacteria were incubated with the materials for 24 h at 44 • C and 48 h at 36 • C, respectively. The microbial growth was evaluated by observing the diameter of the inhibition halo (ID). The obtained values are the mean standard (SD) deviation of the measurements carried out on samples analyzed three times.

Results
Recent advances in the synthetic methodologies of materials used in the biomedical field see the polymers as main actors, because of their great proficiency to adapt to several specific applications, due to a wide range of physical, chemical and biological properties [19]. Among synthetic polymers used for many decades in the design of biomaterials with controlled structure and dynamic functionality, PEG plays a prominent role. It is known as a versatile, biocompatible polymer, mainly used in polymer-based materials for drug delivery, and is responsible for the improvement of a number of biological properties of drugs [20]. With this in mind and with the aim to propose a new biomaterial with antioxidant activity, able to counteract oxidative stress involved in the pathogenesis of several diseases, we synthesized SiO 2 /PEG/CGA organic-inorganic hybrids, in which the polymer constituted 50 wt% and the natural antioxidant compound was embedded at four different percentages (5, 10, 15 and 20 wt%).

UV-Vis Spectra
In order to evaluate the incorporation of CGA in the SiO 2 /PEG-based matrix, the synthesized hybrids were subjected to ultrasound-assisted extraction in a hydroalcoholic solution, and the obtained extracts were investigated by UV-Vis spectroscopy. All the UV-Vis spectra showed a hypsochromic shift of the characteristic bands of CGA, probably due to the occurrence of structural modifications. These results allowed us to deduce that CGA was securely trapped inside the matrix ( Figure 2). Materials 2019, 12, x FOR PEER REVIEW 5 of 12 The formation of the hydroxyapatite layer on the surfaces of all the hybrid materials was evaluated by SEM images, after soaking for 21 days in simulated body fluid (SBF).
Comparing the surface materials in which different percentages of CGA were incorporated, no difference was observed in the distribution and amount of hydroxyapatite. Figure 3A shows a representative SEM micrograph of the hybrid with a high percentage of CGA, before soaking in SBF. Homogeneousness and absence of phase separation were visible as well, as in the other materials. Instead, the surface of the materials were covered when the hybrids were soaked in SBF, covered by a precipitate with a globular shape typical of hydroxyapatite ( Figure 3B) [15]. In fact, when the materials were soaked in SBF, the interaction between the OH-groups of the silica matrix and the Ca 2+ ions present in the fluid occurred, leading to the increase of positive surface charge. The Ca 2+ ions combined with the negative charge of the phosphate ions to form an amorphous phosphate, which spontaneously transformed into hydroxyapatite [Ca10(PO4)6(OH)2] [21].
In the energy-dispersive X-ray (EDX) microanalysis of the hybrids after exposure to SBF, the atomic ratio between Ca and P is equal to 1.67, depending on the number of days of exposure. While the EDX of the same samples without exposure to SBF were observed only in the peaks of the elements that formed the hybrids. Furthermore, the crystalline hydroxyapatite was confirmed by the intense peaks in the XRD spectrum ( Figure 4). In addition, the XRD results suggested that the hydroxyapatite layer on the material's surface was very thick. The formation of the hydroxyapatite layer on the surfaces of all the hybrid materials was evaluated by SEM images, after soaking for 21 days in simulated body fluid (SBF).
Comparing the surface materials in which different percentages of CGA were incorporated, no difference was observed in the distribution and amount of hydroxyapatite. Figure 3A shows a representative SEM micrograph of the hybrid with a high percentage of CGA, before soaking in SBF. Homogeneousness and absence of phase separation were visible as well, as in the other materials. Instead, the surface of the materials were covered when the hybrids were soaked in SBF, covered by a precipitate with a globular shape typical of hydroxyapatite ( Figure 3B) [15]. In fact, when the materials were soaked in SBF, the interaction between the OH-groups of the silica matrix and the Ca 2+ ions present in the fluid occurred, leading to the increase of positive surface charge. The Ca 2+ ions combined with the negative charge of the phosphate ions to form an amorphous phosphate, which spontaneously transformed into hydroxyapatite [Ca 10 (PO 4 ) 6 (OH) 2 ] [21].
In the energy-dispersive X-ray (EDX) microanalysis of the hybrids after exposure to SBF, the atomic ratio between Ca and P is equal to 1.67, depending on the number of days of exposure. While the EDX of the same samples without exposure to SBF were observed only in the peaks of the elements that formed the hybrids. The formation of the hydroxyapatite layer on the surfaces of all the hybrid materials was evaluated by SEM images, after soaking for 21 days in simulated body fluid (SBF).
Comparing the surface materials in which different percentages of CGA were incorporated, no difference was observed in the distribution and amount of hydroxyapatite. Figure 3A shows a representative SEM micrograph of the hybrid with a high percentage of CGA, before soaking in SBF. Homogeneousness and absence of phase separation were visible as well, as in the other materials. Instead, the surface of the materials were covered when the hybrids were soaked in SBF, covered by a precipitate with a globular shape typical of hydroxyapatite ( Figure 3B) [15]. In fact, when the materials were soaked in SBF, the interaction between the OH-groups of the silica matrix and the Ca 2+ ions present in the fluid occurred, leading to the increase of positive surface charge. The Ca 2+ ions combined with the negative charge of the phosphate ions to form an amorphous phosphate, which spontaneously transformed into hydroxyapatite [Ca10(PO4)6(OH)2] [21].
In the energy-dispersive X-ray (EDX) microanalysis of the hybrids after exposure to SBF, the atomic ratio between Ca and P is equal to 1.67, depending on the number of days of exposure. While the EDX of the same samples without exposure to SBF were observed only in the peaks of the elements that formed the hybrids. Furthermore, the crystalline hydroxyapatite was confirmed by the intense peaks in the XRD spectrum ( Figure 4). In addition, the XRD results suggested that the hydroxyapatite layer on the material's surface was very thick. Furthermore, the crystalline hydroxyapatite was confirmed by the intense peaks in the XRD spectrum ( Figure 4). In addition, the XRD results suggested that the hydroxyapatite layer on the material's surface was very thick.

Antiradical Capacity Assessment
The widespread and easy to use DPPH · and ABTS ·+ methods are useful to evaluate the radical scavenging capacity of a tested sample, providing valid, accurate and reliable data strictly related to the sample chemical features. The adopted methods, which are based on the neutralization reaction induced by the transfer of an electron (ET) and/or a hydrogen atom (HAT), are commonly used in structure-antioxidant activity relationships, which chemically depends on the presence and/or the position of active groups in investigated samples. As CGA easily reacts with both the probes in a dose-dependent manner, their use was also used to verify the CGA preservation during hybrid synthesis (supporting data acquired through characterization techniques)-or at least the maintenance of the CGA antioxidant efficacy by the conservation of those functional groups-which are commonly held responsible for the activity of the natural substance. [22]. Indeed, the synthesized hybrid materials exerted a dissimilar radical scavenging effect towards the two considered probes, but depended on the percentage of CGA ( Figure 5). In fact, except for the sample containing the lowest percentage of CGA (SiO2/PEG50wt%/CGA5wt%), which did not show any activity towards both radicals, the other hybrids exerted a more pronounced antiradical capacity versus the radical cation ABTS. Furthermore, for each considered material, the increasing activity appeared directly correlated with the increase in the tested dose (0.5, 1 and 2 mg). An exception to this general trend was represented by the sample having the highest content of CGA (SiO2/PEG50wt%/CGA20wt%). The effectiveness towards ABTS + , in this case, reached a maximum-even at the 0.5 mg exposure doseand remained constant. This showed that the effectiveness in reducing the radical probe of this hybrid is a function of the high percentage of CGA contained therein. The mechanism of chlorogenic acid in exerting free radical scavenging activity, and in particular against DPPH, has been studied by López-Giraldo et al. [23]. The authors demonstrated that the global mechanism of DPPH stabilization likely proceeded ET and involved the dissociation of the phenolic hydroxyl group, the electron transfer from the phenolate anion to DPPH, and finally the stabilization of the DPPH anion by a proton present in the medium.

Antiradical Capacity Assessment
The widespread and easy to use DPPH · and ABTS ·+ methods are useful to evaluate the radical scavenging capacity of a tested sample, providing valid, accurate and reliable data strictly related to the sample chemical features. The adopted methods, which are based on the neutralization reaction induced by the transfer of an electron (ET) and/or a hydrogen atom (HAT), are commonly used in structure-antioxidant activity relationships, which chemically depends on the presence and/or the position of active groups in investigated samples. As CGA easily reacts with both the probes in a dose-dependent manner, their use was also used to verify the CGA preservation during hybrid synthesis (supporting data acquired through characterization techniques)-or at least the maintenance of the CGA antioxidant efficacy by the conservation of those functional groups-which are commonly held responsible for the activity of the natural substance. [22]. Indeed, the synthesized hybrid materials exerted a dissimilar radical scavenging effect towards the two considered probes, but depended on the percentage of CGA ( Figure 5). In fact, except for the sample containing the lowest percentage of CGA (SiO 2 /PEG 50wt% /CGA 5wt% ), which did not show any activity towards both radicals, the other hybrids exerted a more pronounced antiradical capacity versus the radical cation ABTS. Furthermore, for each considered material, the increasing activity appeared directly correlated with the increase in the tested dose (0.5, 1 and 2 mg). An exception to this general trend was represented by the sample having the highest content of CGA (SiO 2 /PEG 50wt% /CGA 20wt% ). The effectiveness towards ABTS + , in this case, reached a maximum-even at the 0.5 mg exposure dose-and remained constant. This showed that the effectiveness in reducing the radical probe of this hybrid is a function of the high percentage of CGA contained therein. The mechanism of chlorogenic acid in exerting free radical scavenging activity, and in particular against DPPH, has been studied by López-Giraldo et al. [23]. The authors demonstrated that the global mechanism of DPPH stabilization likely proceeded ET and involved the dissociation of the phenolic hydroxyl group, the electron transfer from the phenolate anion to DPPH, and finally the stabilization of the DPPH anion by a proton present in the medium.

Cell Culture and Cytotoxicity Assessment
The MTT test was applied to evaluate if the synthesized materials had effects on cell proliferation or showed direct cytotoxic effects, thus affecting biocompatibility. This test determines the activity levels of mitochondrial dehydrogenases toward 3-(4,5-dimethyl-2-thiazolyl)-2,5-diphenyl-2Htetrazolium bromide (MTT), which is converted to formazan crystals only by living cells [24]. Cell viability was expressed as the mitochondrial redox activity percentage of cells directly exposed to powders, compared to an unexposed control.
NIH-3T3 murine fibroblast, HaCat human keratinocyte and SH-SY5Y human neuroblastoma cell lines were screened. Fibroblasts and keratinocytes are suitable for the use in biocompatibility tests; fibroblasts are representative of the predominant tissue in the body and, in particular, the NIH/3T3 cell line is one of the most frequently used lines in material/cell interaction research [25]. Furthermore, the SH-SY5Y cell line was chosen for their particular sensitivity to oxidative stress onset, making them a model cell system for studying the mechanisms involved in oxidative stress-mediated apoptosis [26].
These data obtained highlight that the different hybrids do not induce morphological changes and cytotoxic effects on the murine fibroblast and human keratinocyte cell lines tested. In particular, the sample containing a CGA amount equal to 15 wt% induced a slight increase in the percentage of HaCat viable cells, compared to other hybrids ( Figure 6), whereas the NIH-3T3 cell viability did not change in response to the different materials used (Figure 7).

Cell Culture and Cytotoxicity Assessment
The MTT test was applied to evaluate if the synthesized materials had effects on cell proliferation or showed direct cytotoxic effects, thus affecting biocompatibility. This test determines the activity levels of mitochondrial dehydrogenases toward 3-(4,5-dimethyl-2-thiazolyl)-2,5-diphenyl-2Htetrazolium bromide (MTT), which is converted to formazan crystals only by living cells [24]. Cell viability was expressed as the mitochondrial redox activity percentage of cells directly exposed to powders, compared to an unexposed control.
NIH-3T3 murine fibroblast, HaCat human keratinocyte and SH-SY5Y human neuroblastoma cell lines were screened. Fibroblasts and keratinocytes are suitable for the use in biocompatibility tests; fibroblasts are representative of the predominant tissue in the body and, in particular, the NIH/3T3 cell line is one of the most frequently used lines in material/cell interaction research [25]. Furthermore, the SH-SY5Y cell line was chosen for their particular sensitivity to oxidative stress onset, making them a model cell system for studying the mechanisms involved in oxidative stress-mediated apoptosis [26].
These data obtained highlight that the different hybrids do not induce morphological changes and cytotoxic effects on the murine fibroblast and human keratinocyte cell lines tested. In particular, the sample containing a CGA amount equal to 15 wt% induced a slight increase in the percentage of HaCat viable cells, compared to other hybrids ( Figure 6), whereas the NIH-3T3 cell viability did not change in response to the different materials used (Figure 7).

Cell Culture and Cytotoxicity Assessment
The MTT test was applied to evaluate if the synthesized materials had effects on cell proliferation or showed direct cytotoxic effects, thus affecting biocompatibility. This test determines the activity levels of mitochondrial dehydrogenases toward 3-(4,5-dimethyl-2-thiazolyl)-2,5-diphenyl-2Htetrazolium bromide (MTT), which is converted to formazan crystals only by living cells [24]. Cell viability was expressed as the mitochondrial redox activity percentage of cells directly exposed to powders, compared to an unexposed control.
NIH-3T3 murine fibroblast, HaCat human keratinocyte and SH-SY5Y human neuroblastoma cell lines were screened. Fibroblasts and keratinocytes are suitable for the use in biocompatibility tests; fibroblasts are representative of the predominant tissue in the body and, in particular, the NIH/3T3 cell line is one of the most frequently used lines in material/cell interaction research [25]. Furthermore, the SH-SY5Y cell line was chosen for their particular sensitivity to oxidative stress onset, making them a model cell system for studying the mechanisms involved in oxidative stress-mediated apoptosis [26].
These data obtained highlight that the different hybrids do not induce morphological changes and cytotoxic effects on the murine fibroblast and human keratinocyte cell lines tested. In particular, the sample containing a CGA amount equal to 15 wt% induced a slight increase in the percentage of HaCat viable cells, compared to other hybrids ( Figure 6), whereas the NIH-3T3 cell viability did not change in response to the different materials used (Figure 7).  On the contrary, cytotoxic effects were observed for all neuroblastoma cell samples, even when the lowest dose of chlorogenic acid (5 wt%) was entrapped. The cytotoxicity becomes more pronounced with the increase of the CGA amount, reaching about 90% of cell proliferation inhibition at the highest weight percentage (Figure 8). This could be explained taking into account the so-called double-edged sword behavior of phenols and polyphenols [27], meaning that they can be used as antioxidant compounds against oxidative stress at lower doses and as pro-oxidant agents at higher doses. This is in line with our previous findings, which explored the growth inhibitory effect of SiO2/PEG/CGA hybrids-with lower amounts of the polymer-against breast cancer and osteosarcoma cell lines [28]. In this context, these encouraging data suggested the ability of the investigated hybrids to induce a consistent variation of protein levels, such as cyclin-dependent kinase inhibitor p21 and caspase-3. Furthermore, the herein observed pro-oxidant effects could depend also on environmental conditions, such as the pH and the presence of transition metals, particularly copper. A viable hypothesis reported in the literature concerns the reduction of Cu(II) to Cu(I), which becomes available in Fenton-like reactions, i.e., promoting the formation of reactive oxygen species [29]. The relationship between phenols and copper was previously investigated in SH-SY5Y cells, treated with oleuropein. The authors demonstrated that depleting cells of copper by treatment with the copper chelator triethylenetetramine, which binds copper with higher affinity than oleuropein, was less toxic than oleuropein with copper-adequate cells [30]. On the contrary, cytotoxic effects were observed for all neuroblastoma cell samples, even when the lowest dose of chlorogenic acid (5 wt%) was entrapped. The cytotoxicity becomes more pronounced with the increase of the CGA amount, reaching about 90% of cell proliferation inhibition at the highest weight percentage (Figure 8). This could be explained taking into account the so-called double-edged sword behavior of phenols and polyphenols [27], meaning that they can be used as antioxidant compounds against oxidative stress at lower doses and as pro-oxidant agents at higher doses. This is in line with our previous findings, which explored the growth inhibitory effect of SiO 2 /PEG/CGA hybrids-with lower amounts of the polymer-against breast cancer and osteosarcoma cell lines [28]. In this context, these encouraging data suggested the ability of the investigated hybrids to induce a consistent variation of protein levels, such as cyclin-dependent kinase inhibitor p21 and caspase-3. Furthermore, the herein observed pro-oxidant effects could depend also on environmental conditions, such as the pH and the presence of transition metals, particularly copper. A viable hypothesis reported in the literature concerns the reduction of Cu(II) to Cu(I), which becomes available in Fenton-like reactions, i.e., promoting the formation of reactive oxygen species [29]. The relationship between phenols and copper was previously investigated in SH-SY5Y cells, treated with oleuropein. The authors demonstrated that depleting cells of copper by treatment with the copper chelator triethylenetetramine, which binds copper with higher affinity than oleuropein, was less toxic than oleuropein with copper-adequate cells [30]. The obtained results allowed us to state that synthesized materials containing different percentages of CGA determined dissimilar responses, based on the considered cell line, and in particular, hybrids are able to interfere and act selectively against tumor cells.  The obtained results allowed us to state that synthesized materials containing different percentages of CGA determined dissimilar responses, based on the considered cell line, and in particular, hybrids are able to interfere and act selectively against tumor cells.

Antibacterial Activity
E. coli and E. faecalis were inoculated in presence of 100 mg of the hybrid powders. Figure 9A shows a representative image of the zones of inhibition that are clearly visible when E. coli was incubated with high amounts of CGA, compared with the hybrids containing only PEG. The results of the diameter of the zone of inhibition ( Figure 9B) of all the hybrids, suggested that the materials exhibited strong activity against E. coli and E. faecalis in function of the CGA content, due to disruption the bacterial cell membrane, which lead to cell death [31][32][33]. This happened despite the different cell wall structures of either model bacteria (Gram-positive and Gram-negative).
The damage of the bacterial cell membrane could be caused by excessive generation of ROS in the cells. In fact, it is known that the equilibrium of levels of ROS is crucial in cells. In particular, it plays many roles in intracellular signaling in different organisms, from bacteria to mammalian cells [34]. Therefore, when ROS increases or depletion occurs, numerous signaling pathways are affected. This leads to malfunction and cellular dysfunction [35].
Lee et al. [36] suggested that CGA-induced bacterial apoptosis-like death is not associated with oxidative stress. Instead, it is possible to observe inhibition of bacterial growth due to ROS depletion by CGA, which is a strong antioxidant compound, as suggested by the ABTS and DPPH results above. Probably, the obtained results are due to CGA inducing ROS depletion in both bacteria, resulting in death from apoptosis.

Conclusions
The use of antioxidant biomaterials, able to control oxidant species formed in the implantation site, represents a valuable strategy to reduce all the pathological consequences derived from oxidative stress. As a part of a consolidated line of research from our group, in this work we evaluated the capability of new SiO2/PEG/CGA hybrids, synthesized by the sol-gel method, to neutralize free radicals, influence cell viability in vitro and inhibit bacterial growth. The radical scavenging effect seemed to be dependent on the amount of CGA and was more pronounced towards ABTS ·+ . The viabilities of the fibroblast and keratinocyte cell lines tested were not compromised. On the contrary, cytotoxicity of the neuroblastoma cell line was observed with increasing doses of CGA. The recorded UV-Vis spectra of all samples, compared with that of pure chlorogenic acid, suggested that there was no release of CGA, which was instead securely trapped inside the SiO2/PEG matrix. Finally, the bioactivity was not affected by the presence of CGA in the hybrids, which showed excellent antibacterial activity.

Conclusions
The use of antioxidant biomaterials, able to control oxidant species formed in the implantation site, represents a valuable strategy to reduce all the pathological consequences derived from oxidative stress. As a part of a consolidated line of research from our group, in this work we evaluated the capability of new SiO 2 /PEG/CGA hybrids, synthesized by the sol-gel method, to neutralize free radicals, influence cell viability in vitro and inhibit bacterial growth. The radical scavenging effect seemed to be dependent on the amount of CGA and was more pronounced towards ABTS ·+ . The viabilities of the fibroblast and keratinocyte cell lines tested were not compromised. On the contrary, cytotoxicity of the neuroblastoma cell line was observed with increasing doses of CGA. The recorded UV-Vis spectra of all samples, compared with that of pure chlorogenic acid, suggested that there was no release of CGA, which was instead securely trapped inside the SiO 2 /PEG matrix. Finally, the bioactivity was not affected by the presence of CGA in the hybrids, which showed excellent antibacterial activity.