Chemical Composition, Antioxidant Activity, Cytoprotective and In Silico Study of Ethanolic Extracts of Bougainvillea × buttiana (Var. Orange and Rose)

Bougainvillea × buttiana is a plant widely used in traditional Mexican medicine and other parts of the world for the treatment of various health disorders. In this study, the antioxidant and cytoprotective activities of three ethanolic extracts of B. × buttiana (BxbO (Orange), BxbR1 (Rose1) and BxbR2 (Rose2)) were investigated. Antioxidant activities were determined by the oxygen radical absorbance capacity (ORAC), DPPH free radicals scavenging activity, and radical scavenging effects on nitric oxide (NO). The in vitro cytoprotective effect of the extracts against oxidative stress induced by hydrogen peroxide-(H2O2) in a model of L929 cells was also determined as well as NO uptake with or without H2O2 through the MTT assay. The results revealed that there was a difference between the compounds present in each of the extracts, with the 2-Hydroxycinnamic acid compound being observed in all the extracts. The 2-Hydroxycinnamic acid compound was tested in silico to predict its biological (PASSonline) and toxicological (Osiris Property Explorer) activity. All extracts with 1 to 4 mg/mL inhibited the activity of the NO radical. In cells exposed to 1 mg/mL of extracts followed by H2O2 exposure, cell protection ranged from 66.96 to 83.46%. The treatment of the cells with extracts prevented the morphological changes caused by H2O2. The 2-Hydroxycinnamic acid compound showed a probability of in silico antioxidant and cytoprotective activity greater than 0.5 and 0.6, respectively. Therefore, the results demonstrated that Bxb extracts exert antioxidant and protective activities against H2O2-induced oxidative stress in L929 cells.


Introduction
Oxidative stress is an imbalance between oxidative and antioxidant molecules and results in the induction of cellular damage by oxidants. This imbalance occurs when the mechanisms of protection against these species are impaired or when a high production of reactive oxygen species (ROS) and/or reactive nitrogen species (RNS) occurs [1]. With a slight oxidative stress, it can generate an increase in the enzymatic antioxidant protection; however, when a high production of reactive species occurs, it can cause damage and cell death [2]. Biomolecules oxidations are natural processes in aerobiotic beings from the cellular metabolism, in which reactive species are produced naturally or by a some biological dysfunction [3]. This is an integral part of the human metabolism to produce ROS and/or RNS, in which reactive species have important biological functions, such as phagocytosis, but when their production is exacerbated, the organism has an efficient antioxidant system in which it can control or restore the equilibrium [4]. An excess of reactive species is harmful to the organism, and it can cause, for example, the peroxidation of membrane lipids and the aggression of the macromolecules of the tissues. The literature indicates the possibility that chronic degenerative diseases, such as diabetes mellitus, cancer, early cell aging, atherosclerosis, Alzheimer's and Parkinson's, disease, are related to DNA damage caused by the species reactive as well as oxidative stress [5]. According The extraction method was reported in detail in the patent MX/a/ 2011/813522 [22]. For different extraction, 10 g of powered BxbO, BxbR1 and BxbR2 were individually mixed with 100 mL of ethanol + water (1:1) at 26 • C for 24 h. Liquids extracts obtained were separated from the solid residue by 60 • C using a rotary evaporator pressure (Heidolph). All samples were performed in triplicate. Extracts from each extraction process were collected in separate extraction vials and maintained at room temperature until the phytochemical assays.

Analysis of Total Phenolic Contents
The total phenolic contents present in the extracts of BxbO (Orange), BxbR1 (Rose1) and BxbR2 (Rose2) were determined by the Folin-Ciocalteu assay using a gallic acid standard curve [23]. The absorbance determination was at 760 nm using a UV-Vis spectrophotometer, and the results were expressed as mg gallic acid equivalents (GAE) per 100 g FW. The equation is shown below: where "C" indicates the total phenolic component in (mg g −1 ) plant extract in GAE, "c" indicates the gallic acid concentration (mg mL −1 ), "V" indicates the volume of extracts in microliters (µL), and "m" indicates the weight of crude plant in grams. The correlation coefficients (R 2 ) value was determined using the mean of three absorbance determinations for each concentration. The equation is shown below: where "Y" signifies extract absorbance, "m" signifies the slope of the calibration curve, "x" signifies extract concentration, and "c" is the intercept. Concentrations of extracts were calculated using this regression equation. The phenolic content was estimated using the value for each extract concentration.

GC-MS Analysis for Characterization
For the identification, the extracts of B. × buttiana (Var. Orange and Rose 1 and Rose 2) they were called BxbO and BxbR1 and BxbR2, respectively. The analyses of each extract were performed with a chromatography GC-MS method. The analyses were performed according to the method described by Abarca-Vargas et al. 2016 [24].

Measurement of Antioxidant Activity 2.3.1. ORAC Oxygen Radical Absorbance Capacity
The antioxidant activity was determined using Oxygen Radical Absorbance Capacity (ORAC) assay, as described by Dávalos et al., 2004 [25]. In brief, twenty-five microliters of Trolox standards (ranging from 3.125 to 100 µM), blank and sample of extracts were prepared in phosphate buffer 10 mM and pH 7.4. The reaction mixture containing extracts or Trolox and fluorescein at a final concentration of 70 nM was incubated for 10 min at 37 • C. Then, 12 mM of 2,2 azobis(2-amidno-propane) dihydrochloride was added to the mixture. The fluorescence was read every 56 s for 98 min by using FLUOstar Optima (BMG Labtech) fluorometer. The Area Under the Curve (AUC) was determined for each sample and compared with AUC corresponding Trolox. The data were expressed as an ORAC value (µmol Trolox equivalent (TE)/g extract).

DPPH Radicals Scavenging Activity
The antioxidant activity was determined using DPPH radical scavenging assay as adapted by Akkari et al., 2016 [26]. In brief, the volume of 1.4 mL solution of DPPH in methanol (0.1 mM) was added to 0.1 mL of each extract with different concentrations (10,20,40, and 80 × dilutions of each extract). Then, the tubes were incubated in a dark room for 30 min, and the absorbance was determined at 517 nm.

Antioxidant Activity NO (Nitric Oxide) Assay
The nitric oxide capture assay was performed according to the method described by Maia & Moura, 2015 [27]. The assay was performed in PBS (10 mM phosphate buffer, pH 7.3, 136 mM NaCl, and 2.7 mM KCl) and 5 mM sodium nitroprusside. Amounts from each extract (0, 0.001, 0.01, 0.1, 1 and 2 mg/mL) were added in a nitroprusside solution and incubated in a shaker at 25 • C with constant shaking at 70 rpm for 180 min. Gallic acid was used as standard in the concentration range of 0-160 µg/mL to construct a calibration curve. The control used for these assays presented a 100% nitrite formation. After incubation, an aliquot was removed and transferred to a 96-well plate and incubated with Griess's reagent (1% sulfanilamide solution in 3% phosphoric acid and 1% N-1 (1-naphthylethylenediamine) solution). The microplates containing the assays were maintained for 5 min at room temperature, and the absorbance was evaluated on a microplate reader at 540 nm. A calibration curve of sodium nitrite at concentrations of 0.0265 to 1 mM was performed to determine the nitrite concentrations present in the assays. The results were expressed as the mean standard deviation in percent inhibition relative to the control assay. All tests were run in sets of three plus the standard. The results were expressed by the percentage of antioxidant activity and were calculated using the following formula: where A sample represents absorbance of the plant extract sample and A control represents absorbance of the DPPH solution as a control.

Cell Proliferation and Viability Assay
Mouse fibroblast cells (ATCC clone L929) were grown in Dulbecco's Minimum Essential Medium (DMEM) containing 10% Fetal Bovine Serum (FBS), 100 U/mL penicillin, 100 mg/L streptomycin and 500 mg/L neomycin. Confluent cells were tripsinized, centrifuged and sub-cultured in the same medium, in a humidified 5% CO 2 atmosphere at 37 • C. For the experiments, a cell suspension was seeded at a density of 5 × 10 3 cells/well in DMEM culture medium supplemented with 10% FBS and dispensed in a 96 well microplate and incubated at 37 • C in a humidified 5% CO 2 atmosphere for 18 h. Afterwards, the culture medium was discarded and replaced with fresh medium containing 10% FBS for the control cultures, and amounts between 0 and 400 µg/mL of dry weight of each extract were dis-tributed to each well. All cultures, including the controls and those treated with the extracts, were incubated for 24 h and 48 h at 37 • C under 5% CO 2 atmosphere. Then, the culture medium was discarded and finally restored with 100 µL of fresh medium combined with 10 µg of MTT solution 3-(4,5-dimethylthiazol-2-yl) 2, 5-diphenyltetrazolium bromide and keep within dark conditions at 37 • C in a 5% CO 2 atmosphere for 3 h. After that time, 85 µL of the culture medium was removed, and then, a 50% solution of DMSO was added and incubated under the same conditions for 10 min; after formazan crystals' homogenization, the absorbance at 540 nm was assessed using a microplate reader. The percentage of cell proliferation/viability was calculated and compared to the control (100% viability).

Hydrogen Peroxide-Induced Oxidative Stress in L929 Cells and Evaluation of Survival
To evaluate the cytoprotective effect of extracts, hydrogen peroxide was used to induce oxidative stress assay in accordance with the methods previously described by Balekar et al. 2012, [28]. Briefly, the L929 cells were cultivated at a density of 5 × 10 3 cells/well in DMEM supplemented with 10% FBS and incubated at 37 • C with 5% CO 2 for 18 h. To establish the H 2 O 2 concentration that provided cell damage, amounts of 0 to 1.0 mM were used for the hydrogen peroxide curve to evaluate the dose of H 2 O 2 , which caused a decrease of 50-80% in the cell viability after 24 h of exposure using the MTT method. The concentration chosen was 1.0 mM H 2 O 2 . For the assays, the L929 cells were cultured at a density of 5 × 10 3 cells/well containing DMEM medium supplemented with 10% FBS and incubated at 37 • C with 5% CO 2 . After 18 h of incubation, the medium was replaced with fresh medium containing 0 to 400 µg/mL dry weight of B. × buttiana extracts (Var. Orange and Rose), which were used to treat the cells at the different time periods.

In Silico Analysis of the Compounds
All chemical compounds identified in this study were represented by using their chemical structure, which was obtained using the ChemAxon program [29]. Predictions of all compounds were determined using the chemical structure. PASSonline software (Way2Drug.com, 2011-2022, version 2.0, accessed 1 August 2022) [30] was used to predict antioxidant and cytoprotective activity. This program calculates the structural and physicochemical properties necessary to make a comparison with its database. These results are expressed as a probability (P) ranging from 0 to 1, where 0 indicates that it is unlikely and 1 that it is very likely.
The in silico toxicological properties were also determined using the OSIRIS Property Explorer program [31]. This software allows calculating the properties without risk of unwanted effects and is shown in green, while those with medium risk are indicated in yellow, and in the case of high risk, they are represented in red.

Statistical Analyses
The data were obtained for each sample and summarized, which was followed by statistical analysis using one-way ANOVA and Tukey's test. Values of p lower than 0.05 were considered to be statistically significant. The values were expressed as the mean ± SD. Pairwise comparison of the control and each sample was carried out using a t-test. Significant statistical differences were considered at p < 0.01 compared to the untreated control.

Phytocompounds
Each plant was extracted in 50% ethanol (v/v) under the same conditions. GC-MS analyses of these extracts showed several peaks for BxbO (nine compounds), BxbR1 (seven compounds) and BxbR2 (eight compounds). Table 1 summarizes the compounds present and analyzed by chromatography GC-MS [32][33][34]. They were quantified by integration of the peaks areas, and the results are exhibited in Table 1. Between the compounds obtained, the 2-Hydroxycinnamic acid and 3-O-methyl-D-glucose were present in all extract studies.
The chemical structure of the compound 2-Hydroxycinnamic acid (Figure 1) was made with the ChemAxon version 22.13.0, (Budapest, Hungary) program [29]. pounds obtained, the 2-Hydroxycinnamic acid and 3-O-methyl-D-glucose in all extract studies. The chemical structure of the compound 2-Hydroxy ( Figure 1) was made with the ChemAxon version 22.13.0, (Budapest, Hun [29].

Total Phenolic Contents in Bougainvillea Extracts
The Total Phenolic Contents (TPC) in B. xbuttiana ethanolic extracts ar Table 2. The highest amounts of TPC were obtained in BxbR2 extract. Th from 27.43, 29.55 and 32.48 mgGA/g dry extract for BxbO, BxbR1 and BxbR2

Total Phenolic Contents in Bougainvillea Extracts
The Total Phenolic Contents (TPC) in B. × buttiana ethanolic extracts are presented in Table 2. The highest amounts of TPC were obtained in BxbR2 extract. The TPC ranged from 27.43, 29.55 and 32.48 mgGA/g dry extract for BxbO, BxbR1 and BxbR2, respectively.

Comparative Antioxidant Activity
The antioxidant activity of different extracts was evaluated by measuring their ability to scavenge DPPH and by ORAC assay. As shown in Table 3, the DPPH radical scavenging activities of three extracts followed the order of BxBR2 > BxbR1 > BxbO. Regarding the ORAC assay, BxbR1 and BxbR2 improve the ORAC values to 8100. 45 and 8105.38 µmol Trolox/mg gallic acid, respectively. The lowest ORAC value was obtained in the BxbO extract. Results of antioxidant capacities were also correlated to phenolic compound concentration determined by the Folin-Ciocalteu method. Results were obtained with DPPH and ORAC assay.

Effect of Extracts on Nitric Oxide Capture
The antioxidant activity of ethanolic extracts of B. × buttiana was determined using a NO scavenging assay. Figure 2 shows the nitrite concentration values and the percentage of inhibition of the formation of this anion by increasing the concentrations of the Bougainvillea extracts. The concentration of nitrite in the absence of the extract was approximately 26.2 µM. The formation of nitrite occurs spontaneously in the reaction medium from NO and O 2 , being an indirect method of determination of NO generated by the decomposition of sodium nitroprusside [27]. The extracts of BxbO, BxbR1 and BxbR2 at the concentrations used (0.001 and 0.01 mg/mL) were shown to be able to decrease the formation of nitrite, differentiating significantly in relation to the control but without a significant difference between them. The inhibition of NO increased with the use of extract concentrations of 0.1 mg/mL, reaching the maximum with 1 mg/mL concentration of the extracts. At concentrations of 1 mg/mL, the inhibition NO percentages was 62.97, 63.75 and 64.85% for BxbO, BxbR1 and BxbR2, respectively. In contrast, when concentrations of 2 to 4 mg/mL were used, the NO inhibition was significantly reduced (p < 0.001). These results suggest that extracts of BxbO, BxbR1 and BxbR2 act as antioxidants against NO ( Figure 2). The kinetics of antioxidant activity is described in Figure 3. For the positive control for nitrite inhibition, gallic acid was used, reaching the highest percentage of antioxidant The kinetics of antioxidant activity is described in Figure 3. For the positive control for nitrite inhibition, gallic acid was used, reaching the highest percentage of antioxidant activity (48.84%) with 80 µg/mL incubated for 180 min (data not shown). The formation of nitrite decreased with increased exposure time to the extracts. The maximum antioxidant activity percentages reached by the extracts at 1 mg/mL were 62.70, 63.75 and 64.85% for BxbO, BxbR1 and BxbR2, respectively ( Figure 3). With increasing concentrations at 2 to 4 mg/mL of extracts, the percentages of antioxidant activity were significantly reduced.

Effect of Extracts on Cell Viability and Proliferation
The effect of the extracts from B. × buttiana using Var. Orange and Rose on the viability was evaluated in L929 cells in different concentrations after 24 and 48 h using the MTT method ( Figure 4). Cultures of cells were treated with 0.1, 1 and 10 µg/mL extracts, and the extracts did not prove to be toxic to the cells. For cultures treated for 24 h at 100 µg/mL, the percentages of cell viability were 96.4, 95 and 120% for the extracts BxbO, BxbR1 and BxbR2, respectively. Whereas, in cultures treated for 48 h at 100 µg/mL, the percentages of cell viability were 91.6, 90.8 and 100% for the extracts BxbO, BxbR1 and BxbR2, respectively ( Figure 4). The concentrations of 200 to 400 µg/mL in all extracts for both times of exposure significantly decreased the cell viability (p < 0.01). At the concentration of 100 µg/mL of BxbR2 extract, it was possible to observe proliferation in both the intervals: 24 and 48 h. In contrast, in cell cultures treated with 300 and 400 µg/mL of this extract, the percentages of viability were significantly lower for both 24 and 48 h ( Figure 4). This data allowed selecting the optimal non-cytotoxic concentrations of the extracts as 100 µg/mL, which was used in further experiments. of cell viability were 91.6, 90.8 and 100% for the extracts BxbO, BxbR1 and BxbR2, respectively ( Figure 4). The concentrations of 200 to 400 µg/mL in all extracts for both times of exposure significantly decreased the cell viability (p < 0.01). At the concentration of 100 µg/mL of BxbR2 extract, it was possible to observe proliferation in both the intervals: 24 and 48 h. In contrast, in cell cultures treated with 300 and 400 µg/mL of this extract, the percentages of viability were significantly lower for both 24 and 48 h (Figure 4).

Hydrogen Peroxide-Induced Oxidative Stress and Survival
H 2 O 2 as a precursor of various ROS was chosen as the oxidant reagent in this study. Various concentrations of H 2 O 2 were used to determine the appropriate dose. L929 cells were treated with 1 mM hydrogen peroxide as a model of oxidative stress, and this caused a decrease in the cell viability by around 75% after 24 h of exposure. In Figure 5, the potential antioxidant effect of the extracts was tested before and after exposure to H 2 O 2 for 3 h and combined with H 2 O 2 for 24 h. In comparison, the extracts were effective in the cellular protection against oxidative stress before exposure to H 2 O 2 , resulting in a protection of 83.46, 66.96 and 77.21% for the extracts BxbO, BxbR1 and BxbR2, respectively. However, when the cells were exposed to extracts after or combined with H 2 O 2 for 3 h, they did not protect the cells against the oxidative stress caused by H 2 O 2 ( Figure 5). In the BxbO and BxbR2 extracts, the best cell protection, expressed as cell viability values, was observed for treatment with 10 and 100 µg/mL before H 2 O 2 . In contrast, for the BxbR1 extract with the best cell protection, the viability values for the treatments of 10 and 100 µg/mL were combined and after H 2 O 2 ( Figure 5).  Once the mode and amount of extract with the highest percentage of cell viability was established, we also compared the level of protection with the compounds present in the  Table 1 show that of all the different compounds found in the extracts BxbO, BxbR1 and BxbR2, where one of them was the phenolic compound, we found 2-Hydroxycinnamic acid. Another new test was carried out to verify which of these compounds could be responsible for the protection of the oxidative stress of the extracts ( Figure 6). The treatment of L929 cells with 2-Hydroxycinnamic acid was shown to be effective in cell protection under the three different conditions. In the cultures of cells treated with 100 µg/mL of this compound before H 2 O 2 , the viability was significantly higher in relation to the control, with a percentage of 42.73% ( Figure 6). In contrast, with the decrease in the concentration from 50 to 1.56 µg/mL, the viability was significantly increased ( Figure 6). In cultures treated with 100 µg/mL of 2-Hydroxycinnamic acid combined or after H 2 O 2 , the viability percentages were 44.24 and 46.05%, respectively ( Figure 6). Decreasing the compound dose from 50 to 6.25 µg/mL increased the cell viability ( Figure 6). Under the conditions performed in this study, treatment with concentrations of 0.78 to 3.125 µg/mL, the viability percentages were greater than 100% ( Figure 6). Once the mode and amount of extract with the highest percentage of cell viability was established, we also compared the level of protection with the compounds present in the extracts. The results presented in Table 1 show that of all the different compounds found in the extracts BxbO, BxbR1 and BxbR2, where one of them was the phenolic compound, we found 2-Hydroxycinnamic acid. Another new test was carried out to verify which of these compounds could be responsible for the protection of the oxidative stress of the extracts ( Figure 6). The treatment of L929 cells with 2-Hydroxycinnamic acid was shown to be effective in cell protection under the three different conditions. In the cultures of cells treated with 100 µg/mL of this compound before H2O2, the viability was significantly higher in relation to the control, with a percentage of 42.73% ( Figure 6). In contrast, with the decrease in the concentration from 50 to 1.56 µg/mL, the viability was significantly increased ( Figure 6). In cultures treated with 100 µg/mL of 2-Hydroxycinnamic acid combined or after H2O2, the viability percentages were 44.24 and 46.05%, respectively (Figure 6). Decreasing the compound dose from 50 to 6.25 µg/mL increased the cell viability ( Figure 6). Under the conditions performed in this study, treatment with concentrations of 0.78 to 3.125 µg/mL, the viability percentages were greater than 100% ( Figure 6). The groups of cells treated with 1 mg of Bougainvillea extracts contained 2-Hydroxycinnamic acid in the concentrations of 11.24, 1.90 and 8.21 µg for BxbO, BxbR1 and BxbR2, respectively. The different concentrations present in each extract were used to compare their effects with the total extract in cell cultures treated before, combined, or after H2O2 (Figure 7). The results obtained in cell cultures treated before H2O2 showed that 2-Hydroxycinnamic acid was not significant for the cytoprotective effect achieved for whole extracts. These results suggest that this treatment effect may be due to the action of other compounds. The groups of cells treated with 1 mg of Bougainvillea extracts contained 2-Hydroxycinnamic acid in the concentrations of 11.24, 1.90 and 8.21 µg for BxbO, BxbR1 and BxbR2, respectively. The different concentrations present in each extract were used to compare their effects with the total extract in cell cultures treated before, combined, or after H 2 O 2 ( Figure 7). The results obtained in cell cultures treated before H 2 O 2 showed that 2-Hydroxycinnamic acid was not significant for the cytoprotective effect achieved for whole extracts. These results suggest that this treatment effect may be due to the action of other compounds.

In Silico Analysis of the Compounds
The results of the analysis on the biological effects of the compounds present in the extracts were obtained from PASSonline (Table 4). It was observed that the phenolic compounds and fatty acids presented a greater probability of acting as cytoprotective; however, the compound 2-Hydroxycinnamic acid was present in all three extracts and presented a higher probability of antioxidant and cytoprotective activity.

In Silico Analysis of the Compounds
The results of the analysis on the biological effects of the compounds present in the extracts were obtained from PASSonline (Table 4). It was observed that the phenolic compounds and fatty acids presented a greater probability of acting as cytoprotective; however, the compound 2-Hydroxycinnamic acid was present in all three extracts and presented a higher probability of antioxidant and cytoprotective activity.  Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. Pa-probability of being active, Pi-probability of being inactive., BxbO (Orange), BxbR1 (Rose1) and BxbR2 (Rose2).
Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Pa-probability of being active, Pi-probability of being inact and BxbR2 (Rose2).
Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation.

Extracts
Compounds Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Derived from the previous analysis, an in silico analysis of the toxicological ac was performed in the OSIRIS Property Explorer program of the different compounds sent in the three extracts. The results are coded in colors, as shown in Table 5. The p erties without risk are represented in green color, those of moderate risk are represe in yellow color and those with high risk are represented in red color for undesirable e such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. T Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being sent in the three extracts was decisive for its antioxidant and cytoprotective evaluati

Extracts
Compounds Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation.

Extracts
Compounds Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective  Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective  Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective  Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective  Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop
Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Table 5. Toxicity risk by OSIRIS Property Explorer.

Extracts Compounds
BxbR2 3,5-Dihydroxy-6-methyl-2,3-dihydro-4H-pyran-4-on BxbO, BxbR1, BxbR2 2-Hydroxycinnamic acid BxbR2 2,3-Dihydro-1-benzofuran BxbR1, BxbR2 Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation Pa-probability of being active, Pi-probability of being inactive., BxbO (Orange), B and BxbR2 (Rose2).
Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective  Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop Table 5. Toxicity risk by OSIRIS Property Explorer.
Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant Table 5. Toxicity risk by OSIRIS Property Explorer.

Extracts Compounds
BxbR2 3,5-Dihydroxy-6-methyl-2,3-dihydro-4H-pyran-4-on BxbO, BxbR1, BxbR2 2-Hydroxycinnamic acid BxbR2 2,3-Dihydro-1-benzofuran BxbR1, BxbR2 Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant  Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation.  Derived from the previous analysis, an in silico analysis of the toxicological activit was performed in the OSIRIS Property Explorer program of the different compounds pre sent in the three extracts. The results are coded in colors, as shown in Table 5. The prop erties without risk are represented in green color, those of moderate risk are represente in yellow color and those with high risk are represented in red color for undesirable effect such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2 Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being pre sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation.  Derived from the previous analysis, an in silico analysis of the toxicologi was performed in the OSIRIS Property Explorer program of the different comp sent in the three extracts. The results are coded in colors, as shown in Table 5 erties without risk are represented in green color, those of moderate risk are r in yellow color and those with high risk are represented in red color for undesir such as mutagenicity, teratogenicity, irritability, and effects on the reproduct Hydroxycinnamic acid compound shows zero risk of undesirable effects, and sent in the three extracts was decisive for its antioxidant and cytoprotective ev  Derived from the previous analysis, an in silico analysis of the toxicological ac was performed in the OSIRIS Property Explorer program of the different compounds sent in the three extracts. The results are coded in colors, as shown in Table 5. The p erties without risk are represented in green color, those of moderate risk are represe in yellow color and those with high risk are represented in red color for undesirable e such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. T Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being sent in the three extracts was decisive for its antioxidant and cytoprotective evaluati  Derived from the previous analysis, an in silico analysis of the toxicological activ was performed in the OSIRIS Property Explorer program of the different compounds p sent in the three extracts. The results are coded in colors, as shown in Table 5. The pr erties without risk are represented in green color, those of moderate risk are represen in yellow color and those with high risk are represented in red color for undesirable eff such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. Th Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being p sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation  Derived from the previous analysis, an in silico analysis of the toxicolo was performed in the OSIRIS Property Explorer program of the different com sent in the three extracts. The results are coded in colors, as shown in Table  erties without risk are represented in green color, those of moderate risk ar in yellow color and those with high risk are represented in red color for unde such as mutagenicity, teratogenicity, irritability, and effects on the reprodu Hydroxycinnamic acid compound shows zero risk of undesirable effects, a sent in the three extracts was decisive for its antioxidant and cytoprotective   Derived from the previous analysis, an in silico analysis of th was performed in the OSIRIS Property Explorer program of the di sent in the three extracts. The results are coded in colors, as show erties without risk are represented in green color, those of moder in yellow color and those with high risk are represented in red colo such as mutagenicity, teratogenicity, irritability, and effects on th Hydroxycinnamic acid compound shows zero risk of undesirable sent in the three extracts was decisive for its antioxidant and cytop  Derived from the previous analysis, an in silico an was performed in the OSIRIS Property Explorer program sent in the three extracts. The results are coded in color erties without risk are represented in green color, those in yellow color and those with high risk are represented such as mutagenicity, teratogenicity, irritability, and ef Hydroxycinnamic acid compound shows zero risk of u sent in the three extracts was decisive for its antioxidant  Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds pre-sent in the three extracts. The results are coded in colors, as shown in Table 5. The prop-erties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being pre-sent in the three extracts was decisive for its antioxidant and cytoprotective evaluation.  Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation.  Derived from the previous analysis, an in silico analysis of the toxicological activity was performed in the OSIRIS Property Explorer program of the different compounds present in the three extracts. The results are coded in colors, as shown in Table 5. The properties without risk are represented in green color, those of moderate risk are represented in yellow color and those with high risk are represented in red color for undesirable effects such as mutagenicity, teratogenicity, irritability, and effects on the reproduction. The 2-Hydroxycinnamic acid compound shows zero risk of undesirable effects, and being present in the three extracts was decisive for its antioxidant and cytoprotective evaluation. : High risk., BxbO (Orange), BxbR1 (Rose1) and BxbR2 (Rose2)

Discussion
The antioxidant potentiality of plant extracts was also extensively proven by using various assays in vitro [35]. The radical-scavenging assay and chelate transition metals have gained acceptance among researchers for their capacity to rapidly screen materials of interest. The phenolics derived from plants are well known as beneficial for human health due to their antioxidant activity, and they can act in different ways to protect cells from oxidative damage. Research found that micromolar concentrations of vitamin E and many polyphenols are effective against oxidative stress through the direct scavenging of reactive oxygen species, as shown in the cell culture model for the study of different diseases. The mechanism of action includes the prevention of reactive species formation, scavenging radicals or repairing damage to target molecules [36]. The estimation of total phenolic content is an important parameter to determine the amounts of antioxidants [21,22,[32][33][34]. The amount of total phenolic contents in the extracts varied among extracts samples. These differences could be due to the different physicochemical properties of the phenolic components. In extracts of Bougainvillea, various phenolic compounds were obtained, and we investigated the antioxidant activity of extracts [21,22,33,34]. We have documented that Bougainvillea extracts have significant antioxidant capacity due to their phenolic compounds [22,[32][33][34]. In the present study, the ability to inhibit DPPH production appeared to be significantly potent in all Bougainvillea extracts. With respect to the ORAC assay based on the delay of oxidation, the ORAC values of different extracts obtained in this study ranged from 7114.43 to 8105.38 µmol Trolox/g of dry extract, suggesting the extraction system used in this study was efficient at extracting potent antioxidant compounds.
The antioxidant activity of Bxb extract is thought to be related to its content of phenolic compounds. However, these molecules are unstable and could easily suffer degradation. Therefore, some parameters such as temperature, exposure to O 2 , and the time of extraction should be monitored during the extraction process to avoid the loss of biological activity as a consequence of the phenolic compound degradation [36]. In this study, the scavenging properties of Bxb extracts were tested in vitro using the NO scavenging method. The NO is mediated by an antioxidant compound through nitrogen atom donation, forming a stable compound. Although the Bxb extracts revealed an interesting antioxidant activity at higher concentrations, they were harmful to L929 cells in culture. In L929 cells treated with 1 mg/mL extract concentrations, the viability percentages were around 80%. Concentrations of 2 to 4 mg/mL of Bxb extracts were cytotoxic to L929 cells by around 30% after 24 and 48 h of exposure. This effect could be explained by a possible pro-oxidant property exerted by high concentrations of antioxidants. The phenolics compounds were capable of converting iron and cooper ions into their reduction forms which react with hydrogen peroxide to produce the highly toxic hydroxyl radicals [37,38]]. Factors that contribute to turning antioxidants into pro-oxidants included the concentrations of the antioxidants, nature of the neighboring molecules and availability of transitions metals [39,40]. Nitrile oxide is a compound synthesized by living organisms from the moment that nitric oxide synthase (NOS) becomes catalytically active, converting the amino acid L-arginine to NO and L-citrulline. When stimulated, human phagocytes can also produce this radical in greater quantities. It is a free radical that acts on a variety of biological processes, such as muscle relaxation, transmission, and immune regulation. While diffusing rapidly between and within cells, it is not reactive enough to attack DNA directly; however, it can react with the superoxide anion radical O 2 , and when exposed to air, it reacts with oxygen, forming NO 2 [41,42].
Hydrogen peroxide alone is practically innocuous, and although it is not considered a free and important radical, it can easily diffuse through cell membranes and participate in reactions that produce the OH-radical in the presence of metals such as iron. H 2 O 2 in vivo is generated by the dismutation of O 2 − or by the β-oxidation of fatty acids [43]. All Bxb extracts at concentrations between 0.001 and 1 mg/mL were investigated regarding their protective effect using an in vitro oxidative stress model. For this, L929 cells were exposed to H 2 O 2 for 3 h, and the extracts were added to the culture medium before or after H 2 O 2 exposure. In addition, cells were also treated with a combination of Bxb extracts and H 2 O 2 for 24 h. Hydrogen peroxide-induced oxidative stress concomitantly or after the extracts was lethal for L929 cells. H 2 O 2 is a small uncharged molecule that could diffuse through cellular membranes easily [44]. This rapid transport to inside the cell could be responsible for the deleterious effect of H 2 O 2 that acted faster than the cytoprotective phytochemicals added to the culture medium. The mitochondria that are sources of O 2 are also rich in dismutase superoxide (SOD) that converts this anion radical into H 2 O 2 , and, thus, the hydrogen peroxide generated and partially eliminated by catalase, peroxidase glutathione and peroxidase linked to thioredoxin. However, this elimination has low efficiency, and a large part of the H 2 O 2 is released from other regions of the cell.
Extracts added before H 2 O 2 exposure were effective in protecting L929 cells from death, mainly with the BxbR2 extract. Preincubation with the extracts led to metabolic changes that resulted in cytoprotective effects against severe stress caused by H 2 O 2 . Phytochemicals can promote mild stress induction that elicits adaptative beneficial responses, thereby increasing protection against a further oxidative challenge. This process is known as hormesis and might contribute to explaining the results herein described [45,46].
Protection against oxidative stress occurs through two mechanisms [47]. First, the antioxidant functions through a direct antioxidant system, where the antioxidants are redox active with a lifespan and are sacrificed when they act on ROS. Due to this direct effect, antioxidants need to be regenerated so that they can curtail ROS levels. The second mechanism is an indirect antioxidant effect, which can trigger the self-defense mechanisms of the host cells to fight oxidative stress. Phenolic acids are divided into polyphenols, oligophenols and monophenols or simple phenolic compounds such as benzoic and cinnamic acids and their hydroxylated derivatives. Hydroxycinnamic acid derivatives are naturally occurring phenolic compounds that have an aromatic ring with a carbon chain, consisting of three carbons attached to the ring. These acids exist in plants, usually in the form of esters, such as chlorogenic acid or the ester of quinic acid. They are also found in the form of glycosides or linked to proteins and other cell wall polymers and, rarely, as free acids. Isomers of chlorogenic acid and caffeic acid are described with antioxidants [48,49]. These groups of phenolic acids have shown antioxidant properties. Although other characteristics also contribute to the antioxidant activity of phenolic acids and their esters, this is generally determined by the number of hydroxyls present in the molecule [50]. The presence of a second hydroxyl in the ortho or para position also increases the antioxidant activity. The sequestering effect of the hydroxyl radical appears to be directly related to the hydroxyl groups located in the para position in the aromatic ring.
In an in vivo model of the efficacy of 2-Hydroxycinnamic acid at a dose of 50 mg/kg body weight on oxidative stress in Winstar rats, a modest improvement in reactive oxygen species levels was demonstrated by induction with trichlorfon [51]. Therefore, it will be advisable to carry out studies in the future with other types of free radicals in an in vitro model in order to reduce the use of laboratory animals.
The in silico analysis was carried out through PASSonline, a platform that makes predictions about biological activities through the structure-activity relationship with an accuracy greater than 95% [30]. The chemical compounds 2-Hydroxycinnamic acid and 3-O-methyl-D-glucose are present in all three extracts; however, only 2-Hydroxycinnamic acid had high antioxidant and cytoprotective potential. The results obtained by the OSIRIS program on toxicity detected a greater number of molecules with a high risk of unwanted effects in the BxbO extract than in the other two extracts.

Conclusions
The production of phenolic compounds by plants is vast (about 8000 compounds have already been detected). These compounds are natural constituents that exert antioxidant action due to their chemical structure (a benzene ring with associated hydroxyls), and they can provide several biological benefits. Among all that has been discovered, research involving antioxidant agents in the B. × buttiana plant must continue, as they are of great importance for the pharmaceutical industry. With regard to the pharmaceutical field, the search continues for substances' functional aspects in the fight against free radicals and all the possible dangers they pose to human health. According to our results, we comparatively investigated the total phenolic contents of BxbO, BxbR1 and BxbR2 extracts and tested their antioxidant and cytoprotective activities. These extracts exerted scavenging activity on NO and DPPH radicals, with a higher inhibitory extend detected in the DPPH assay. Other potential antioxidant activity, determined using ORAC assay, showed that Bougainvillea extracts are active radical scavengers. In the present study, the results indicated that BxbO, BxbR1 and BxbR2 extracts exert antioxidant and protective activities against oxidative stress induced by H 2 O 2 on L929 cells. The results obtained showed that these extracts exert a protective action by decreasing cell death and by inhibiting around of 64% of NO radical activity, suggesting that these phenolic contents may be useful for those oxidative stress-related degenerative diseases. Follow-up studies that isolate and test individual constituents in the extracts and different combination studies may help to determine the specific health-protective effects of each constituent.