<i>Hibiscus acetosella</i> extract protects against alkylating agent-induced DNA damage in mice

VILELA, THAIS C.; LEFFA, DANIELA D.; DAMIANI, ADRIANI P.; DAMAZIO, DAIANE DAL COL; MANENTI, ALINE V.; CARVALHO, TIAGO JOSÉ G.; RAMLOV, FERNANDA; AMARAL, PATRICIA A.; ANDRADE, VANESSA M. DE

doi:10.1590/0001-3765201820180144

Abstract

Hibiscus acetosella was shown to exert beneficial effects in humans and animal models however, the effects of this plant on DNA are unknown. The aim of this study was to determine the antigenotoxic and antimutagenic effects of H. acetosella extracts on alkylating agent methyl methanesulfonate (MMS) in vivo in mice. Initially, we performed analysis of phenolic compounds in extracts of H. acetosella by high-performance liquid chromatography (HPLC). Next, mice were divided into 8 groups and treated with distilled water or plant extract (0.1 ml/10 g) by gavage for 15 days, followed by intraperitoneal (ip) administration of saline solution or MMS (40 mg/Kg b.w) on day 16. Caffeic acid, following by gallic acid, gallocatechin, coumaric acid, and 3,4-dihydroxybenzoic acid were found to be present in extracts of H. acetosella leaves. In peripheral blood analysis of groups receiving pretreatment with H. acetosella at doses of 50 or 100 mg/kg plus MMS decreased DNA damage as evidenced by comet assay and Micronucleus assays relative to MMS alone. These results suggested that H. acetosella extracts exerted protective effects dose dependent against genotoxicity and mutagenicity induced by alkylating agents.

Key words
Hibiscus acetosella; antigenotoxicity; comet assay; antimutagenicity; micronucleus test

INTRODUCTION

The low availability of currently available drugs have driven research in herbal medicine, with the goal of identifying new pharmacotherapeutic agents (Ouédraogo et al. 2012OUÉDRAOGO M, KONATÉ K, LEPENGUÉ AN, SOUZA A, M ’BATCHI B and SAWADOGO LL. 2012. Free radical scavenging capacity, anticandicidal effect of bioactive compounds from Sida cordifolia L., in combination with nystatin and clotrimazole and their effect on specific immune response in rats. Ann Clin Microbiol Antimicrob 11: 33., Venancio et al. 2016VENANCIO VP, MARQUES MC, ALMEIDA , MR , MARIUTTI LR, SOUZA VC, BARBOSA FJR, PIRES BIANCHI ML, MARZOCCHI - MACHADO CM, MERCADANTE AZ and ANTUNES LM. 2016. Chrysobalanus icaco L. fruits inhibit NADPH oxidase complex and protect DNA against doxorubicin-induced damage in Wistar male rats. J Toxicol Environ Health A 79(20): 885-893., Ferreira et al. 2016FERREIRA NH, DE ANDRADE KJ, LEANDRO LF, ACÉSIO NO, MENDES SA, CINTRA LS, JANUÁRIO AH and TAVARES DC. 2016. Testing of Schefflera vinosa extract in mammalian cells in vitro and in vivo for potential toxicity, genetic damage, and role of oxidation. J Toxicol Environ Health A 79(24): 1201-1210., Trindade et al. 2016TRINDADE C et al. 2016. Antimutagenic and antioxidant properties of the aqueous extracts of organic and conventional grapevine Vitis labrusca cv. Isabella leaves in V79 cells. J Toxicol Environ Health A 79(18): 825-836.). In this context, medicinal plants are often used for either prevention or treatment of several human diseases (Gemelli et al. 2015GEMELLI TF, PRADO LS, SANTOS FS, DE SOUZA AP, GUECHEVA TN, HENRIQUES JA, FERRAZ ADE B, CORRÊA DS, DIHL RR and PICADA JN. 2015. Evaluation of Safety of Arrabidaea chica Verlot (Bignoniaceae), a Plant with Healing Properties. J Toxicol Environ Health A 78(18): 1170-1180., dos Santos et al. 2016DOS SANTOS RL et al. 2016. The cardioprotective power of leaves. Arch. Med. Sci. 11, 819-39. Pomegranate peel extract attenuates oxidative stress by decreasing coronary angiotensin-converting enzyme (ACE) activity in hypertensive female rats . J Toxicol Environ Health A 79(21): 998-1007., Niwa et al. 2016NIWA AM, DE PAULA NA, VESENICK DC, SARTORI D, MAISTRO EL, RIBEIRO LR and MANTOVANI MS. 2016. Evaluation of lignan (-)-cubebin extracted from Piper cubeba on human colon adenocarcinoma cells (HT29). J Toxicol Environ Health A 79(2): 92-100.). The efficacy of these medicinal plants is often attributed to their antioxidant activities (Gülçin et al. 2006GÜLÇIN I, MSHVILDADZE V, GEPDIREMEN A and ELIAS R. 2006. Screening of antiradical and antioxidant activity of monodesmosides and crude extract from Leontice smirnowii tuber. Phytomedicine 13: 343-351., Trindade et al. 2016TRINDADE C et al. 2016. Antimutagenic and antioxidant properties of the aqueous extracts of organic and conventional grapevine Vitis labrusca cv. Isabella leaves in V79 cells. J Toxicol Environ Health A 79(18): 825-836., Ferreira et al. 2016FERREIRA NH, DE ANDRADE KJ, LEANDRO LF, ACÉSIO NO, MENDES SA, CINTRA LS, JANUÁRIO AH and TAVARES DC. 2016. Testing of Schefflera vinosa extract in mammalian cells in vitro and in vivo for potential toxicity, genetic damage, and role of oxidation. J Toxicol Environ Health A 79(24): 1201-1210.). Thus, plants used in traditional medicine may constitute an important source of new biologically active compounds (Da-Costa-Rocha et al. 2014DA-COSTA-ROCHA I, BONNLAENDER B, SIEVERS H, PISCHEL I and HEINRICH M. 2014. Hibiscus sabdariffa L. - a phytochemical and pharmacological review. Food Chem 165: 424-443.).

In Latin America, biodiversity is extensive; 40% of the countries in Latin America, including Brazil, have more plant species than most other nations worldwide (Michán and Llorente-Bousquets 2009MICHÁN L and LLORENTE-BOUSQUETS J. 2009. Bibliometría de la sistemática biológica sobre América Latina durante el siglo XX en tres bases de datos mundiales. Rev Biol Trop 58(2): 531-545.). In this context, natural plant extracts of the Malvaceae family were examined as potential sources of biologically active compounds (Kiessoun et al. 2012KIESSOUN K, SOUZA A, THÉRÈSE KY, DIBALA IC, BARRO N, MILLOGO - RASOLODIMBY J and NACOULMA OG. 2012. Phytochemical composition, antioxidant and anti-inflammatory potential of bioactive fractions from extracts of three medicinal plants traditionally used to treat liver diseases in Burkina Faso. Int J Phytomedicine 3: 406-415.). The Malvaceae family consists of 75 genera and 1500 species, which are widely distributed and found primarily in tropical and subtropical regions (Wang et al. 2012WANG ML, MORRIS B, TONNIS B, DAVIS J and PEDERSON GA. 2012. Assessment of oil content and fatty acid composition variability in two economically important Hibiscus species. J Agric Food Chem 60: 6620-6626.).

The Hibiscus genus is the largest of the Malvaceae family, consisting of approximately 300 species of annual or perennial herbs, shrubs, and trees (Wang et al. 2012WANG ML, MORRIS B, TONNIS B, DAVIS J and PEDERSON GA. 2012. Assessment of oil content and fatty acid composition variability in two economically important Hibiscus species. J Agric Food Chem 60: 6620-6626.). Some investigators suggested that plants of this genus possess antioxidant properties (Farombi and Fakoya 2005FAROMBI EO and FAKOYA A. 2005. Free radical scavenging and antigenotoxic activities of natural phenolic compounds in dried flowers of Hibiscus sabdariffa L. Mol Nutr Food Res 49: 1120-1128., Rosa et al. 2006ROSA RM, MELECCHI MIS, DA COSTA HALMENSCHLAGER R, ABAD FC, SIMONI CR, CARAMÃO EB, HENRIQUES JAP, SAFFI J and DE PAULA RAMOS ALL. 2006. Antioxidant and antimutagenic properties of Hibiscus tiliaceus L. methanolic extract. J Agric Food Chem 54: 7324-7330., Olalye and Rocha 2007OLALYE MT and ROCHA JBT. 2007. Commonly used tropical medicinal plants exhibit distinct in vitro antioxidant activities against hepatotoxins in rat liver. Exp Toxicol Pathol 58: 433-438., Mohamed et al. 2013MOHAMED J, SHING SW, IDRIS MHM, BUDIN SB and ZAINALABIDIN S. 2013. The protective effect of aqueous extracts of roselle (Hibiscus sabdariffa L. UKMR-2) against red blood cell membrane oxidative stress in rats with streptozotocin-induced diabetes. Clinics (Sao Paulo) 68: 1358-1363., Ehsan et al. 2015EHSAN Z, MAHMOUD M, SHOTT SR, AMIN RS and ISHMAN SL. 2015. The effects of anesthesia and opioids on the upper airway: a systematic review. Laryngoscope 126(1): 270-284., Kapelula et al. 2017KAPEPULA PM et al. 2017. Comparison of metabolic profiles and bioactivities of the leaves of three edible Congolese Hibiscus species. Nat Prod Res 21: 1-8.) owing to their potent scavenging effects on reactive oxygen species (ROS) and free radicals such as hydrogen peroxide (H₂O₂). Components of this genus including flavonoids and polyphenolic compounds are often active dietary constituents that contribute to these protective effects by exerting antioxidant actions. Indeed, Kapepula et al. (2017)KAPEPULA PM et al. 2017. Comparison of metabolic profiles and bioactivities of the leaves of three edible Congolese Hibiscus species. Nat Prod Res 21: 1-8. observed that although the species present different compositions, H. acetosella, H. cannabinus and H. sabdariffa displayed high cellular antioxidant activity with IC50 values ranging from 0.5 to 3 μg mL−1.

Pharmacological investigations of the Hibiscus genus reported that species of this genus displayed biological activities, including anti-inflammatory, antimicrobial, antidiabetic, hepatoprotective, and anticancer activities (Adetutu et al. 2004ADETUTU A, ODUNOLA OA, OWOADE OA, ADELEKE AO and AMUDA OS. 2004. Anticlastogenic effects of Hibiscus sabdariffa fruits against sodium arsenite-induced micronuclei formation in erythrocytes in mouse bone marrow. Phytother Res 18: 862-864., Farombi and Fakoya 2005FAROMBI EO and FAKOYA A. 2005. Free radical scavenging and antigenotoxic activities of natural phenolic compounds in dried flowers of Hibiscus sabdariffa L. Mol Nutr Food Res 49: 1120-1128., Olalye and Rocha 2007OLALYE MT and ROCHA JBT. 2007. Commonly used tropical medicinal plants exhibit distinct in vitro antioxidant activities against hepatotoxins in rat liver. Exp Toxicol Pathol 58: 433-438., Rosa et al. 2006ROSA RM, MELECCHI MIS, DA COSTA HALMENSCHLAGER R, ABAD FC, SIMONI CR, CARAMÃO EB, HENRIQUES JAP, SAFFI J and DE PAULA RAMOS ALL. 2006. Antioxidant and antimutagenic properties of Hibiscus tiliaceus L. methanolic extract. J Agric Food Chem 54: 7324-7330.). Therefore, the aim of this study was to determine whether Hibiscus acetosella extracts exerted antigenotoxic and antimutagenic capacities in vivo in a mouse model by using alkylating agents to induce DNA damage.

MATERIALS AND METHODS

PLANT COLLECTION AND EXTRACT PREPARATION

H. acetosella WeLw ex Hiern leaves were obtained from the Pe. Dr. Raulino Reitz Herbarium of University of Southern Santa Catarina (UNESC), City of Criciúma, Santa Catarina State, Brazil. The plant material used in the experiment was collected in a single time of the year (September), in order to avoid the possible change of chemical compounds in different seasons. An exsicta of the plant was previously identified by the botanic Dra. Vanilde Citadini Zanette and kept in the herbarium (register no: CRI:8551). Preparation of the extract was carried out as previously described (Carvajal-Zarrabal et al. 2009CARVAJAL-ZARRABAL O, HAYWARD - JONES PM, ORTA - FLORES Z, NOLASCO - HIPÓLITO C, BARRADAS - DERMITZ DM, AGUILAR - USCANGA MG and PEDROZA - HERNÁNDEZ M. 2009. Effect of Hibiscus sabdariffa L. dried calyx ethanol extract on fat absorption-excretion, and body weight implication in rats. J Biomed Biotechnol 2009: 394592.). The specimens were dried in an oven at 40°C for 40 hr. Subsequently dried leaves were crushed, to yield a powder, and 196.7 g of the material was subjected to maceration in 1 L ethanol at 70% (proportion of 1:5) for 15 days. Then the mixture was filtered, and solvent was eliminated using a rotary evaporator, yielding 57 g sample. The extract was diluted with distilled water for administration to animals by gavage.

ANALYSIS OF PHENOLIC COMPOUNDS BY HIGH-PERFORMANCE LIQUID CHROMATOGRAPHY (HPLC)

Aliquots (10 μl) of ethanolic extract (10 mg/ml dry weight) were analyzed using a liquid chromatograph (Shimzadu LC-10A) equipped with a C18 reverse-phase column (Vydac 218TP54; 250 mm × 4.6 mm Ø, 5 μm, 30 °C) and a UV-Vis spectrophotometric detector operating at 280 nm. Elution was carried out using water: acetic acid: n-butanol (350:1:10, v/v/v) as the mobile phase, with a flow rate of 0.8 ml/min. Detection of the compounds of interest was performed using co-chromatography and comparisons of retention times with standard compounds (gallocatechin, gallic acid, protocatechuic acid, coumaric acid, and caffeic acid; Sigma, St. Louis, MO, USA), under the same experimental conditions. Quantification of the phenolic compounds was carried out using an external standard curve for gallic acid (5–300 μg/ml, r² = 0.9958; y = 35158x), considering the peak areas of interest to calculate concentration. The presented values correspond to means of three injections per sample. The concentrations of phenolic compounds are expressed as μg/g dry mass.

ANIMALS

In the present study, 48 male Swiss albino mice (weighing approximately: 25 g; age: 7–8 weeks) were obtained from the Animal Center of the University of Southern Santa Catarina (UNESC, Brazil). All procedures involving animals and their care were performed in accordance with national and international laws and guidelines for the use of animals in biomedical research. The experimental procedures were approved by the local ethics committee for animal use (CEUA – UNESC; approval no.: 130/2011). Mice were randomized by weight and housed in polycarbonate cages with steel wire tops (6 animals per cage). Mice were housed under conditions of controlled room temperature (22 ± 2°C) and humidity (55% ± 10%) and exposed to alternating 12 hr light/dark cycle. On the last day of the experiment, the animals were acclimated in the laboratory for 30 minutes with controlled temperature of 22 ± 1ºC. Care was taken to minimize suffering and reduce external sources of stress, pain, and discomfort for the animals. Only the minimum number of animals necessary to produce reliable scientiﬁc data was used.

EXPERIMENTAL DESIGN

Animals were divided into 8 groups of 6 mice per group. The animals were treated as described in Table I. Mice in different groups were treated with distilled water or plant extracts (50, 100, or 200 mg/kg; 0.1 ml /10 g body weight) by daily gavage for 15 days, followed by intraperitoneal (ip) administration of saline solution, MMS (40 mg/Kg b.w).

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TABLE I
Experimental design to evaluate antigenotoxicity and antimutagenicity of Hibiscus acetosella extracts.

The doses of H. acetosella extracts used in this study were selected based on previous studies using other species of Hibiscus with biological activities in animal models (Adetutu et al. 2004ADETUTU A, ODUNOLA OA, OWOADE OA, ADELEKE AO and AMUDA OS. 2004. Anticlastogenic effects of Hibiscus sabdariffa fruits against sodium arsenite-induced micronuclei formation in erythrocytes in mouse bone marrow. Phytother Res 18: 862-864., Liu et al. 2010LIU LC, WANG CJ, LEE CC, SU SC, CHEN HL, HSU JD and LEE HJ. 2010. Aqueous extract of Hibiscus sabdariffa L. decelerates acetaminophen-induced acute liver damage by reducing cell death and oxidative stress in mouse experimental models. J Sci Food Agri 90: 329-337., Olalye and Rocha 2007OLALYE MT and ROCHA JBT. 2007. Commonly used tropical medicinal plants exhibit distinct in vitro antioxidant activities against hepatotoxins in rat liver. Exp Toxicol Pathol 58: 433-438.).

All treatments were made at the same time each day. Four hr after administration, peripheral blood was collected by tail vein without anesthesia. Twenty-four hr later, animals were killed by cervical dislocation, and bone marrow removed immediately. The samples were then processed for comet assays and micronucleus (MN) tests.

COMET ASSAY

Comet assays were carried out under alkaline conditions, as previously described by Tice et al. DC, March 25-26, 1999TICE RR, AGURELL E, ANDERSON D, BURLINSON B, HARTMANN A, KOBAYASHI H, MIYAMAE Y, ROJAS E, RYU JC and SASAKI YF. 2000. Single cell gel/comet assay: guidelines for in vitro and in vivo genetic toxicology testing . Environ Mol Mutagen 35: 206-321., an expert panel met to develop guidelines for the use of the single-cell gel (SCG(2000), and visual scores were classified according to the method of Collins et al. (1997)COLLINS A, DUSINSKÁ M, FRANKLIN M, SOMOROVSKÁ M, PETROVSKÁ H, DUTHIE S, FILLION L, PANAYIOTIDIS M, RASLOVÁ K and VAUGHAN N. 1997. Comet assay in human biomonitoring studies: Reliability, validation, and applications. Environ Mol Mutagen 30: 139-146.. Peripheral blood samples were collected in heparinized tubes and kept on ice. Blood cell aliquots (5 µl) were embedded in low melting agarose (0.75%, w/v; 95 or 80 µl, respectively). These mixtures were then placed onto microscope slides, which were precoated with normal melting point agarose (1.5%, w/v) and furnished with cover slips (two slides per sample). The slides were briefly placed on ice, and cover slips removed. The base slides were immersed in freshly prepared lysis solution (2.5 M NaCl, 100 mM ethylenediaminetetraacetic acid [EDTA], 10 mM Tris, pH 10.0–10.5) and then incubated for 20 min in freshly prepared alkaline buffer (300 mM NaOH, 1 mM EDTA, pH > 13). Electrophoresis (15 min/300 mA; 25 V; 0.7 V/cm) was then performed using the same buffer. All of these steps were carried out in minimal indirect light. Following electrophoresis, slides were neutralized with 400 mM Tris (pH 7.5) and stained with ethidium bromide solution (10 mg/ml). The images of 100 randomly selected cells (50 cells from each of the two replicate slides) were analyzed for each individual mice. DNA damage index (DI) were calculated by visually separating cells into 5 classes according to tail size (0 = no tails to 4 = maximum-length tails). An individual DI was thus obtained for each sample and consequently for each group studied. The group DI ranged between 0 (completely undamaged = 100 cells × 0) and 400 (maximum damage = 100 cells × 4). Visual scores of comet assays are considered a reliable evaluation method and are typically consistent with computer-based image analysis methods. All slides were coded for blind analysis.

PERCENTAGE OF DAMAGE REDUCTION (DR%)

The MMS DR% upon Hibiscus acetosella extracts administration was calculated as follows: [MMS mean-the mean of a plant extracts]/ (MMS mean-control group mean). Results were multiplied by 100 to obtain DR%. This procedure was performed to evaluate DR% in the comet assay according to Mauro et al. (2013)MAURO MO, MONREAL MT, SILVA MT, PESARINI JR, MANTOVANI MS, RIBEIRO LR, DICHI JB, CARREIRA CM and OLIVEIRA RJ. 2013. Evaluation of the antimutagenic and anticarcinogenic effects of inulin in vivo. Genet Mol Res 12: 2281-2293..

MICRONUCLEUS (MN) TESTS

MN tests were performed and analyzed according to the guidelines of the Gene-Tox program described by Mavournin et al. (1990)MAVOURNIN KH, BLAKEY DH, CIMINO MC, SALAMONE MF and HEDDLE JA. 1990. The in vivo micronucleus assay in mammalian bone marrow and peripheral blood. A report of the U.S. Environmental Protection Agency Gene-Tox Program. Mutat Res 239: 29-80.. Bone marrow was extracted from mice femurs, and smears were placed directly onto microscope slide using a drop of fetal calf serum (FCS). Slides were stained with Giemsa (5%), air-dried, and coded for blind analysis. To avoid false-negative results and as a toxicity measure, the ratio between polychromatic and normochromatic erythrocytes (PCE: NCE) was determined for 200 erythrocytes per animal. The presence of micronuclei (MN) was measured for 2000 erythrocytes for each animal (1000 from each of the two slides), using bright-field microscopy (1000× magnification). For individual animals, mean values of micronucleated polychromatic erythrocytes (MnPCE) and micronucleated normochromatic erythrocytes (MnNCE) were used as the experimental unit. The variation was based upon differences between mice of different groups.

STATISTICAL ANALYSIS

Statistical analyses were carried out using the Bioestat 5.8.4 software package. Results are expressed as mean values ± standard deviations. The normality of variables was evaluated using the Kolmogorov-Smirnov test. Statistical analyses for all groups were carried out using one-way analysis of variance (ANOVA). When ANOVA showed significant differences (p < 0.05), post-hoc analysis was performed with Tukey’s test.

RESULTS

QUANTITATIVE AND QUALITATIVE ANALYSIS OF PHENOLIC COMPOUNDS BY HPLC

Chromatographic analyses showed higher levels of caffeic acid, following by gallic acid, gallocatechin, coumaric acid, and 3,4-dihydroxybenzoic acid, in extracts of H. acetosella (Figure 1 and Table II).

Figure 1
Chromatographic profiles of phenolic compounds of H. acetosella extracts (HPLC, 280 nm). Peak 1: gallocatechin; 2: unidentified compound; 3: gallic acid; 4: 3,4-dihydroxybenzoic acid; 5: unidentified compound; 6: unidentified compound; 7: caffeic acid; 8: coumaric acid.

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TABLE II
HPLC analysis of phenolic compounds (µg/mL, dry weight) in ethanolic extracts of Hibiscus acetosella. Values are expressed as means ± standard deviations.

COMET ASSAYS: GENOTOXICITY AND ANTIGENOTOXICITY

Data demonstrated that MMS alone (group 2) significantly increased DNA damage using comet assays (DI) in peripheral blood (P < 0.05) (Figure 2a and 2b). Also, the figure 2a show the genotoxic effects of different doses of H. acetosella, constituting groups 3–5 (50 mg/kg,100 mg/kg and 200 mg/kg, respectively). In this way, we can see that peripheral blood of groups treated with H. acetosella extracts at doses of 100 and 200 mg/kg showed increased DNA damage in relation to control group (P < 0.05).

Figure 2
Genotoxic (a) and Antigenotoxic (b) effects of different doses of H. acetosella in the blood cells of mice. *p < 0.05 compared with saline; #p < 0.05, compared with saline plus MMS, using ANOVA and Tukey test.

Next, we evaluated the antigenotoxic effects of different doses of H. acetosella, constituting groups 6–8 (50 mg/kg plus MMS, 100 mg/kg plus MMS, and 200 mg/kg plus MMS, respectively) in relation to the DNA damage induced in groups 2 (positive control MMS) (Figure 2b). Peripheral blood of groups pretreated with H. acetosella extracts at doses of 50 or 100 mg/kg plus MMS showed decreased DNA damage in relation to those treated with MMS alone (P < 0.05) (Figure 2b). For the percentages of peripheral cells, mice that received extracts at doses of 50 and 100 mg/kg showed reductions of 78.8% and 57.2% for DI, respectively, compared with those of the positive control group (MMS). In animals treated with the higher dose of 200 mg/kg, damage caused by MMS could not be prevented (P > 0.05) (Figure 2b).

MN tests: mutagenicity and antimutagenicity

Animals treated only with the MMS showed high levels of MnPCEs in the bone marrow compared with that in control animals (Table III). Next, we evaluated the mutagenic effects of different doses of H. acetosella, constituting groups 3–5 (50 mg/kg, 100 mg/kg, and 200 mg/kg, respectively). No significant differences in MnPCE levels were observed between the negative control and the groups treated with H. acetosella extracts (Table III).

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TABLE III
Values obtained using MN tests in bone marrow at different doses of Hibiscus acetosella.

Table IV shows antimutagenic effects of different doses of H. acetosella, constituting groups 6–8 (50 mg/kg plus MMS, 100 mg/kg plus MMS, and 200 mg/kg plus MMS, respectively). Oral administration of extracts at low and intermediate doses (50 and 100 mg/kg) significantly decreased MnPCE levels compared with that in the MMS group (Table IV). The inhibition percentages were 88.2% and 85.4%, respectively. No significant differences in MnPCE levels were observed between the MMS and 200 mg/kg plus MMS groups (Table IV).

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TABLE IV
Values obtained using MN tests in bone marrow at different doses of Hibiscus acetosella after administration of MMS.

DISCUSSION

Medicinal plants are widely used and may have critical applications as nutraceuticals and phytomedicine. A literature review revealed that plants of genus Hibiscus are rich in phenolics, flavonoids, and tannins (Ramirez-Rodrigues et al. 2011RAMIREZ-RODRIGUES MM, PLAZA ML, AZEREDO A, BALABAN MO and MARSHALL MR. 2011. Physicochemical and phytochemical properties of cold and hot water extraction from Hibiscus sabdariffa. J Food Sci 76: C428-35.). In our experiments, we show that administration of H. acetosella extracts at low dose (50 mg/kg) was not genotoxic or mutagenic and still protected DNA from damage caused by the alkylating agent (MMS). Besides, our results suggest that the protective effect of H. acetosella extracts appears to be dose dependent. Collectively, our results offer new insight into the H. acetosella extracts impacts in the in the DNA damage index.

In the present study, caffeic acid, following by gallic acid, gallocatechin, coumaric acid, and 3,4-dihydroxybenzoic acid were found to be present in extracts of H. acetosella leaves, as previously reported (Tsumbu et al. 2012TSUMBU CN, DEBY - DUPONT G, TITS M, ANGENO , L , FREDERICH M, KOHNEN S and MOUITHYS - MICKALAD A. 2012. Polyphenol content and modulatory activities of some tropical dietary plant extracts on the oxidant activities of neutrophils and myeloperoxidase. Int J Mol Sci 13: 628-650., Kapelula et al. 2017KAPEPULA PM et al. 2017. Comparison of metabolic profiles and bioactivities of the leaves of three edible Congolese Hibiscus species. Nat Prod Res 21: 1-8.). These compounds have been of particular interest for their potential bioactive properties and promising role as alternative treatment in several illnesses. In this sense, Li et al. (2015)LI Y, CHEN LJ, JIANG F, YANG Y, WANG XX, ZHANG Z, LI Z and LI L. 2015. Caffeic acid improves cell viability and protects against DNA damage: involvement of reactive oxygen species and extracellular signal-regulated kinase. Braz J Med Biol Res 48(6): 502-508. in study in vitro showed that caffeic acid-treated cells generated lower levels of ROS that induced signal-regulated kinase (ERK) signaling pathway. Inhibition of ERK signaling blocked the caffeic acid -induced improvement of cell viability and protection against DNA damage caused by H₂O₂ treatment. Similarly, studies in human and animal models suggest that gallic acid reduces oxidatively damaged DNA in lymphocytes, liver, colon and lungs and protects these organs against γ-irradiation-induced strand breaks and formation of oxidatively damaged DNA-bases (Chakraborty et al. 2009CHAKRABORTY A, FERK F, SIMIC T, BRANTNER A, DUSINSKA M, KUNDI M, HOELZL C, NERSESYAN A and KNASMULLER S. 2009. DNA-protective effects of sumach (Rhus coriaria L.) a common spice: Results of human and animal studies. Mutat Res 661: 10-17., Nair and Nair 2013NAIR GG and NAIR CKK. 2013. Radioprotective Effects of Gallic Acid in Mice. BioMed Research International 2013: 953079.). Thus, these findings of phytochemicals reflected the important potential applications of these extracts.

The genotoxicity of H. acetosella extracts were evaluated and the dose of 100 and 200 mg/kg utilized presented effect genotoxic, suggesting that the protective effect of H. acetosella extracts appears to be dose dependent. However, mice that received 50 and 100 mg/kg of the extract plus MMS showed reduced DNA damage compared with MMS group, attenuating the genotoxic activity of the alkylating agent. The similar findings were previously reported by Rosa et al.ROSA RM, MOURA DJ, MELECCHI MIS, DOS SANTOS RS, RICHTER MF CAMARÃO EB, HENRIQUES JAP, DE PAULA RAMOS ALL and SAFFI J. 2007. Protective effects of Hibiscus tiliaceus L. methanolic extract to V79 cells against cytotoxicity and genotoxicity induced by hydrogen peroxide and tert-butyl-hydroperoxide. Toxicol In Vitro 21: 1442-1452. as test media, it has been shown that HME strongly inhibited the mutagenic action of H(2(2006, 2007) that observe both antigenotoxic and antimutagenic effects against oxidative DNA damage of other species of Hibiscus (Hibiscus tiliaceus). Furthermore, the treatment with a dose of 200 mg/kg was genotoxic and not able to prevent DNA damage caused by MMS. However, the comet assay is a sensitive test that can detect small changes in the number of strand breaks within a nucleus, which can be repair (Collins et al. 1997COLLINS A, DUSINSKÁ M, FRANKLIN M, SOMOROVSKÁ M, PETROVSKÁ H, DUTHIE S, FILLION L, PANAYIOTIDIS M, RASLOVÁ K and VAUGHAN N. 1997. Comet assay in human biomonitoring studies: Reliability, validation, and applications. Environ Mol Mutagen 30: 139-146.). Thinking about that, we also performed MN test and observe that no dose of H. acetosella extracts was mutagenic. Also, the half-maximal lethal dose (LD₅₀) of Hibiscus extracts in rodents was found to be more than 5000 mg/kg, suggesting that the extract was virtually nontoxic (Ali et al. 2005ALI BH, AL WABEL N and BLUNDEN G. 2005. Phytochemical, pharmacological and toxicological aspects of Hibiscus sabdariffa L.: A review. Phytother Res 19: 369-375.).

Our MN test of mutagenicity in bone marrow were different of the findings of comet assays. We show that no dose of H. acetosella extracts was mutagenic. Also, pretreatment with H. acetosella decreased the damage caused by alkylating agent (MMS), primarily when used at a dose of 50 and 100 mg/kg of the extract. Notably, comet assays detect strand breaks, whereas MN tests provide a measure of both chromosome breakage and chromosome loss and have been shown to be a sensitive indicator of chromosome damage (Mavournin et al. 1990MAVOURNIN KH, BLAKEY DH, CIMINO MC, SALAMONE MF and HEDDLE JA. 1990. The in vivo micronucleus assay in mammalian bone marrow and peripheral blood. A report of the U.S. Environmental Protection Agency Gene-Tox Program. Mutat Res 239: 29-80.). In accordance with our results, Olvera-García et al. (2008)OLVERA-GARCÍA V, CASTAÑO - TOSTADO E, REZENDIZ - LOPEZ RI, REYNOSO - CAMACHO R, GONZÁLEZ DE MEJÍA E, ELIZONDO G and LOARCA - PIÑA G. 2008. Hibiscus sabdariffa L. extracts inhibit the mutagenicity in microsuspension assay and the proliferation of HeLa cells. J Food Sci 73: T75-81. and Farombi and Fakoya (2005) showed strong in vitro and in vivo antimutagenic activity of phenolic compounds in H. sabdariffa extracts. The antioxidant activity of phenolic compounds has been shown to inhibit mutations because they can scavenge free radicals or induce antioxidant enzymes (Hochstein and Atallah 1988HOCHSTEIN P and ATALLAH AS. 1988. The nature of oxidants and antioxidant systems in the inhibition of mutation and cancer. Mutat Res 202: 363-375.). Thus, the present results suggest that the genoprotective assignments of H. acetosella may be similar as others antioxidants components, such vitamin C, that have the ability to compete with DNA alkylation targets, reducing the activity of alkylating agents, also having an important role in the regulation of DNA repair enzymes (Cooke et al. 1998COOKE MS, EVANS MD, PODMORE ID, HERBERT KE, MISTRY N, MISTRY P, HICKENBOTHAM PT, HUSSIENI A, GRIFFITHS HR and LUNEC J. 1998. Novel repair action of vitamin C upon in vivo oxidative DNA damage. FEBS Lett 439: 363-367.).

On the other hand, has been proposed that other mechanisms than the antioxidant activities could be involved in the protective effect of these phenolic compounds. In this way, evidences suggest an ability of phenolic compounds to interact with signaling pathways that modulate apoptosis (Spencer 2007SPENCER JP. 2007. The interactions of flavonoids within neuronal signalling pathways. Genes Nutr 2007 2(3): 257-273.), including the nuclear factor-ĸB or mitogen-activated protein kinase (MAPK) pathways (Ramassamy 2006RAMASSAMY C. 2006. Emerging role of polyphenolic compounds in the treatment of neurodegenerative diseases: a review of their intracellular targets. Eur J Pharmacol 545(1): 51-64.). Furthermore, phenolic acids have exhibited anti-inflammatory and anti-cancer properties (Ambriz-Pérez et al. 2016AMBRIZ-PÉREZ DL, LEYVA - LÓPEZ N, GUTIERREZ - GRIJALVA EP and HEREDIA JB. 2016. Phenolic compounds: Natural alternative in inflammation treatment. A review. Cogent Food Agric 2: 1131412.). Therefore, others biological mechanisms associated to antigenotoxic and antimutagenic action of H. acetosella extracts on alkylating agent can be involved.

In conclusion, under the described experimental conditions, administration of H. acetosella extracts at dose of 50 and 100 mg/kg was shown to have protective effects against the genotoxicity and mutagenicity induced by alkylating agents, probably due to the antioxidant activities of phenolic compounds. Besides, this protective effect appears to be dose dependent. Additional biochemical investigations are necessary to elucidate the mechanisms of action of H. acetosella extracts, which were found to have a role in protection against DNA damage. Thus, the results supported the utilization of this plant may have potential therapeutic interest and could justify their use in traditional medicine and local nutraceutical resources.

ACKNOWLEGMENTS

We thank UNESC for financial support. The authors declare that they have no conflicts of interest.

REFERENCES

ADETUTU A, ODUNOLA OA, OWOADE OA, ADELEKE AO and AMUDA OS. 2004. Anticlastogenic effects of Hibiscus sabdariffa fruits against sodium arsenite-induced micronuclei formation in erythrocytes in mouse bone marrow. Phytother Res 18: 862-864.
ALI BH, AL WABEL N and BLUNDEN G. 2005. Phytochemical, pharmacological and toxicological aspects of Hibiscus sabdariffa L.: A review. Phytother Res 19: 369-375.
AMBRIZ-PÉREZ DL, LEYVA - LÓPEZ N, GUTIERREZ - GRIJALVA EP and HEREDIA JB. 2016. Phenolic compounds: Natural alternative in inflammation treatment. A review. Cogent Food Agric 2: 1131412.
CARVAJAL-ZARRABAL O, HAYWARD - JONES PM, ORTA - FLORES Z, NOLASCO - HIPÓLITO C, BARRADAS - DERMITZ DM, AGUILAR - USCANGA MG and PEDROZA - HERNÁNDEZ M. 2009. Effect of Hibiscus sabdariffa L. dried calyx ethanol extract on fat absorption-excretion, and body weight implication in rats. J Biomed Biotechnol 2009: 394592.
CHAKRABORTY A, FERK F, SIMIC T, BRANTNER A, DUSINSKA M, KUNDI M, HOELZL C, NERSESYAN A and KNASMULLER S. 2009. DNA-protective effects of sumach (Rhus coriaria L.) a common spice: Results of human and animal studies. Mutat Res 661: 10-17.
COLLINS A, DUSINSKÁ M, FRANKLIN M, SOMOROVSKÁ M, PETROVSKÁ H, DUTHIE S, FILLION L, PANAYIOTIDIS M, RASLOVÁ K and VAUGHAN N. 1997. Comet assay in human biomonitoring studies: Reliability, validation, and applications. Environ Mol Mutagen 30: 139-146.
COOKE MS, EVANS MD, PODMORE ID, HERBERT KE, MISTRY N, MISTRY P, HICKENBOTHAM PT, HUSSIENI A, GRIFFITHS HR and LUNEC J. 1998. Novel repair action of vitamin C upon in vivo oxidative DNA damage. FEBS Lett 439: 363-367.
DA-COSTA-ROCHA I, BONNLAENDER B, SIEVERS H, PISCHEL I and HEINRICH M. 2014. Hibiscus sabdariffa L. - a phytochemical and pharmacological review. Food Chem 165: 424-443.
DOS SANTOS RL et al. 2016. The cardioprotective power of leaves. Arch. Med. Sci. 11, 819-39. Pomegranate peel extract attenuates oxidative stress by decreasing coronary angiotensin-converting enzyme (ACE) activity in hypertensive female rats . J Toxicol Environ Health A 79(21): 998-1007.
EHSAN Z, MAHMOUD M, SHOTT SR, AMIN RS and ISHMAN SL. 2015. The effects of anesthesia and opioids on the upper airway: a systematic review. Laryngoscope 126(1): 270-284.
FAROMBI EO and FAKOYA A. 2005. Free radical scavenging and antigenotoxic activities of natural phenolic compounds in dried flowers of Hibiscus sabdariffa L. Mol Nutr Food Res 49: 1120-1128.
FERREIRA NH, DE ANDRADE KJ, LEANDRO LF, ACÉSIO NO, MENDES SA, CINTRA LS, JANUÁRIO AH and TAVARES DC. 2016. Testing of Schefflera vinosa extract in mammalian cells in vitro and in vivo for potential toxicity, genetic damage, and role of oxidation. J Toxicol Environ Health A 79(24): 1201-1210.
GEMELLI TF, PRADO LS, SANTOS FS, DE SOUZA AP, GUECHEVA TN, HENRIQUES JA, FERRAZ ADE B, CORRÊA DS, DIHL RR and PICADA JN. 2015. Evaluation of Safety of Arrabidaea chica Verlot (Bignoniaceae), a Plant with Healing Properties. J Toxicol Environ Health A 78(18): 1170-1180.
GÜLÇIN I, MSHVILDADZE V, GEPDIREMEN A and ELIAS R. 2006. Screening of antiradical and antioxidant activity of monodesmosides and crude extract from Leontice smirnowii tuber. Phytomedicine 13: 343-351.
HOCHSTEIN P and ATALLAH AS. 1988. The nature of oxidants and antioxidant systems in the inhibition of mutation and cancer. Mutat Res 202: 363-375.
KAPEPULA PM et al. 2017. Comparison of metabolic profiles and bioactivities of the leaves of three edible Congolese Hibiscus species. Nat Prod Res 21: 1-8.
KIESSOUN K, SOUZA A, THÉRÈSE KY, DIBALA IC, BARRO N, MILLOGO - RASOLODIMBY J and NACOULMA OG. 2012. Phytochemical composition, antioxidant and anti-inflammatory potential of bioactive fractions from extracts of three medicinal plants traditionally used to treat liver diseases in Burkina Faso. Int J Phytomedicine 3: 406-415.
LI Y, CHEN LJ, JIANG F, YANG Y, WANG XX, ZHANG Z, LI Z and LI L. 2015. Caffeic acid improves cell viability and protects against DNA damage: involvement of reactive oxygen species and extracellular signal-regulated kinase. Braz J Med Biol Res 48(6): 502-508.
LIU LC, WANG CJ, LEE CC, SU SC, CHEN HL, HSU JD and LEE HJ. 2010. Aqueous extract of Hibiscus sabdariffa L. decelerates acetaminophen-induced acute liver damage by reducing cell death and oxidative stress in mouse experimental models. J Sci Food Agri 90: 329-337.
MAURO MO, MONREAL MT, SILVA MT, PESARINI JR, MANTOVANI MS, RIBEIRO LR, DICHI JB, CARREIRA CM and OLIVEIRA RJ. 2013. Evaluation of the antimutagenic and anticarcinogenic effects of inulin in vivo. Genet Mol Res 12: 2281-2293.
MAVOURNIN KH, BLAKEY DH, CIMINO MC, SALAMONE MF and HEDDLE JA. 1990. The in vivo micronucleus assay in mammalian bone marrow and peripheral blood. A report of the U.S. Environmental Protection Agency Gene-Tox Program. Mutat Res 239: 29-80.
MICHÁN L and LLORENTE-BOUSQUETS J. 2009. Bibliometría de la sistemática biológica sobre América Latina durante el siglo XX en tres bases de datos mundiales. Rev Biol Trop 58(2): 531-545.
MOHAMED J, SHING SW, IDRIS MHM, BUDIN SB and ZAINALABIDIN S. 2013. The protective effect of aqueous extracts of roselle (Hibiscus sabdariffa L. UKMR-2) against red blood cell membrane oxidative stress in rats with streptozotocin-induced diabetes. Clinics (Sao Paulo) 68: 1358-1363.
NAIR GG and NAIR CKK. 2013. Radioprotective Effects of Gallic Acid in Mice. BioMed Research International 2013: 953079.
NIWA AM, DE PAULA NA, VESENICK DC, SARTORI D, MAISTRO EL, RIBEIRO LR and MANTOVANI MS. 2016. Evaluation of lignan (-)-cubebin extracted from Piper cubeba on human colon adenocarcinoma cells (HT29). J Toxicol Environ Health A 79(2): 92-100.
OLALYE MT and ROCHA JBT. 2007. Commonly used tropical medicinal plants exhibit distinct in vitro antioxidant activities against hepatotoxins in rat liver. Exp Toxicol Pathol 58: 433-438.
OLVERA-GARCÍA V, CASTAÑO - TOSTADO E, REZENDIZ - LOPEZ RI, REYNOSO - CAMACHO R, GONZÁLEZ DE MEJÍA E, ELIZONDO G and LOARCA - PIÑA G. 2008. Hibiscus sabdariffa L. extracts inhibit the mutagenicity in microsuspension assay and the proliferation of HeLa cells. J Food Sci 73: T75-81.
OUÉDRAOGO M, KONATÉ K, LEPENGUÉ AN, SOUZA A, M ’BATCHI B and SAWADOGO LL. 2012. Free radical scavenging capacity, anticandicidal effect of bioactive compounds from Sida cordifolia L., in combination with nystatin and clotrimazole and their effect on specific immune response in rats. Ann Clin Microbiol Antimicrob 11: 33.
RAMASSAMY C. 2006. Emerging role of polyphenolic compounds in the treatment of neurodegenerative diseases: a review of their intracellular targets. Eur J Pharmacol 545(1): 51-64.
RAMIREZ-RODRIGUES MM, PLAZA ML, AZEREDO A, BALABAN MO and MARSHALL MR. 2011. Physicochemical and phytochemical properties of cold and hot water extraction from Hibiscus sabdariffa J Food Sci 76: C428-35.
ROSA RM, MELECCHI MIS, DA COSTA HALMENSCHLAGER R, ABAD FC, SIMONI CR, CARAMÃO EB, HENRIQUES JAP, SAFFI J and DE PAULA RAMOS ALL. 2006. Antioxidant and antimutagenic properties of Hibiscus tiliaceus L. methanolic extract. J Agric Food Chem 54: 7324-7330.
ROSA RM, MOURA DJ, MELECCHI MIS, DOS SANTOS RS, RICHTER MF CAMARÃO EB, HENRIQUES JAP, DE PAULA RAMOS ALL and SAFFI J. 2007. Protective effects of Hibiscus tiliaceus L. methanolic extract to V79 cells against cytotoxicity and genotoxicity induced by hydrogen peroxide and tert-butyl-hydroperoxide. Toxicol In Vitro 21: 1442-1452.
SPENCER JP. 2007. The interactions of flavonoids within neuronal signalling pathways. Genes Nutr 2007 2(3): 257-273.
TICE RR, AGURELL E, ANDERSON D, BURLINSON B, HARTMANN A, KOBAYASHI H, MIYAMAE Y, ROJAS E, RYU JC and SASAKI YF. 2000. Single cell gel/comet assay: guidelines for in vitro and in vivo genetic toxicology testing . Environ Mol Mutagen 35: 206-321.
TRINDADE C et al. 2016. Antimutagenic and antioxidant properties of the aqueous extracts of organic and conventional grapevine Vitis labrusca cv. Isabella leaves in V79 cells. J Toxicol Environ Health A 79(18): 825-836.
TSUMBU CN, DEBY - DUPONT G, TITS M, ANGENO , L , FREDERICH M, KOHNEN S and MOUITHYS - MICKALAD A. 2012. Polyphenol content and modulatory activities of some tropical dietary plant extracts on the oxidant activities of neutrophils and myeloperoxidase. Int J Mol Sci 13: 628-650.
VENANCIO VP, MARQUES MC, ALMEIDA , MR , MARIUTTI LR, SOUZA VC, BARBOSA FJR, PIRES BIANCHI ML, MARZOCCHI - MACHADO CM, MERCADANTE AZ and ANTUNES LM. 2016. Chrysobalanus icaco L. fruits inhibit NADPH oxidase complex and protect DNA against doxorubicin-induced damage in Wistar male rats. J Toxicol Environ Health A 79(20): 885-893.
WANG ML, MORRIS B, TONNIS B, DAVIS J and PEDERSON GA. 2012. Assessment of oil content and fatty acid composition variability in two economically important Hibiscus species. J Agric Food Chem 60: 6620-6626.

Publication Dates

Publication in this collection
Jul-Sep 2018

History

Received
15 Feb 2018
Accepted
11 May 2018

This is an open-access article distributed under the terms of the Creative Commons Attribution License

[1] ADETUTU A, ODUNOLA OA, OWOADE OA, ADELEKE AO and AMUDA OS. 2004. Anticlastogenic effects of Hibiscus sabdariffa fruits against sodium arsenite-induced micronuclei formation in erythrocytes in mouse bone marrow. Phytother Res 18: 862-864.

[2] ALI BH, AL WABEL N and BLUNDEN G. 2005. Phytochemical, pharmacological and toxicological aspects of Hibiscus sabdariffa L.: A review. Phytother Res 19: 369-375.

[3] AMBRIZ-PÉREZ DL, LEYVA - LÓPEZ N, GUTIERREZ - GRIJALVA EP and HEREDIA JB. 2016. Phenolic compounds: Natural alternative in inflammation treatment. A review. Cogent Food Agric 2: 1131412.

[4] CARVAJAL-ZARRABAL O, HAYWARD - JONES PM, ORTA - FLORES Z, NOLASCO - HIPÓLITO C, BARRADAS - DERMITZ DM, AGUILAR - USCANGA MG and PEDROZA - HERNÁNDEZ M. 2009. Effect of Hibiscus sabdariffa L. dried calyx ethanol extract on fat absorption-excretion, and body weight implication in rats. J Biomed Biotechnol 2009: 394592.

[5] CHAKRABORTY A, FERK F, SIMIC T, BRANTNER A, DUSINSKA M, KUNDI M, HOELZL C, NERSESYAN A and KNASMULLER S. 2009. DNA-protective effects of sumach (Rhus coriaria L.) a common spice: Results of human and animal studies. Mutat Res 661: 10-17.

[6] COLLINS A, DUSINSKÁ M, FRANKLIN M, SOMOROVSKÁ M, PETROVSKÁ H, DUTHIE S, FILLION L, PANAYIOTIDIS M, RASLOVÁ K and VAUGHAN N. 1997. Comet assay in human biomonitoring studies: Reliability, validation, and applications. Environ Mol Mutagen 30: 139-146.

[7] COOKE MS, EVANS MD, PODMORE ID, HERBERT KE, MISTRY N, MISTRY P, HICKENBOTHAM PT, HUSSIENI A, GRIFFITHS HR and LUNEC J. 1998. Novel repair action of vitamin C upon in vivo oxidative DNA damage. FEBS Lett 439: 363-367.

[8] DA-COSTA-ROCHA I, BONNLAENDER B, SIEVERS H, PISCHEL I and HEINRICH M. 2014. Hibiscus sabdariffa L. - a phytochemical and pharmacological review. Food Chem 165: 424-443.

[9] DOS SANTOS RL et al. 2016. The cardioprotective power of leaves. Arch. Med. Sci. 11, 819-39. Pomegranate peel extract attenuates oxidative stress by decreasing coronary angiotensin-converting enzyme (ACE) activity in hypertensive female rats . J Toxicol Environ Health A 79(21): 998-1007.

[10] EHSAN Z, MAHMOUD M, SHOTT SR, AMIN RS and ISHMAN SL. 2015. The effects of anesthesia and opioids on the upper airway: a systematic review. Laryngoscope 126(1): 270-284.

[11] FAROMBI EO and FAKOYA A. 2005. Free radical scavenging and antigenotoxic activities of natural phenolic compounds in dried flowers of Hibiscus sabdariffa L. Mol Nutr Food Res 49: 1120-1128.

[12] FERREIRA NH, DE ANDRADE KJ, LEANDRO LF, ACÉSIO NO, MENDES SA, CINTRA LS, JANUÁRIO AH and TAVARES DC. 2016. Testing of Schefflera vinosa extract in mammalian cells in vitro and in vivo for potential toxicity, genetic damage, and role of oxidation. J Toxicol Environ Health A 79(24): 1201-1210.

[13] GEMELLI TF, PRADO LS, SANTOS FS, DE SOUZA AP, GUECHEVA TN, HENRIQUES JA, FERRAZ ADE B, CORRÊA DS, DIHL RR and PICADA JN. 2015. Evaluation of Safety of Arrabidaea chica Verlot (Bignoniaceae), a Plant with Healing Properties. J Toxicol Environ Health A 78(18): 1170-1180.

[14] GÜLÇIN I, MSHVILDADZE V, GEPDIREMEN A and ELIAS R. 2006. Screening of antiradical and antioxidant activity of monodesmosides and crude extract from Leontice smirnowii tuber. Phytomedicine 13: 343-351.

[15] HOCHSTEIN P and ATALLAH AS. 1988. The nature of oxidants and antioxidant systems in the inhibition of mutation and cancer. Mutat Res 202: 363-375.

[16] KAPEPULA PM et al. 2017. Comparison of metabolic profiles and bioactivities of the leaves of three edible Congolese Hibiscus species. Nat Prod Res 21: 1-8.

[17] KIESSOUN K, SOUZA A, THÉRÈSE KY, DIBALA IC, BARRO N, MILLOGO - RASOLODIMBY J and NACOULMA OG. 2012. Phytochemical composition, antioxidant and anti-inflammatory potential of bioactive fractions from extracts of three medicinal plants traditionally used to treat liver diseases in Burkina Faso. Int J Phytomedicine 3: 406-415.

[18] LI Y, CHEN LJ, JIANG F, YANG Y, WANG XX, ZHANG Z, LI Z and LI L. 2015. Caffeic acid improves cell viability and protects against DNA damage: involvement of reactive oxygen species and extracellular signal-regulated kinase. Braz J Med Biol Res 48(6): 502-508.

[19] LIU LC, WANG CJ, LEE CC, SU SC, CHEN HL, HSU JD and LEE HJ. 2010. Aqueous extract of Hibiscus sabdariffa L. decelerates acetaminophen-induced acute liver damage by reducing cell death and oxidative stress in mouse experimental models. J Sci Food Agri 90: 329-337.

[20] MAURO MO, MONREAL MT, SILVA MT, PESARINI JR, MANTOVANI MS, RIBEIRO LR, DICHI JB, CARREIRA CM and OLIVEIRA RJ. 2013. Evaluation of the antimutagenic and anticarcinogenic effects of inulin in vivo. Genet Mol Res 12: 2281-2293.

[21] MAVOURNIN KH, BLAKEY DH, CIMINO MC, SALAMONE MF and HEDDLE JA. 1990. The in vivo micronucleus assay in mammalian bone marrow and peripheral blood. A report of the U.S. Environmental Protection Agency Gene-Tox Program. Mutat Res 239: 29-80.

[22] MICHÁN L and LLORENTE-BOUSQUETS J. 2009. Bibliometría de la sistemática biológica sobre América Latina durante el siglo XX en tres bases de datos mundiales. Rev Biol Trop 58(2): 531-545.

[23] MOHAMED J, SHING SW, IDRIS MHM, BUDIN SB and ZAINALABIDIN S. 2013. The protective effect of aqueous extracts of roselle (Hibiscus sabdariffa L. UKMR-2) against red blood cell membrane oxidative stress in rats with streptozotocin-induced diabetes. Clinics (Sao Paulo) 68: 1358-1363.

[24] NAIR GG and NAIR CKK. 2013. Radioprotective Effects of Gallic Acid in Mice. BioMed Research International 2013: 953079.

[25] NIWA AM, DE PAULA NA, VESENICK DC, SARTORI D, MAISTRO EL, RIBEIRO LR and MANTOVANI MS. 2016. Evaluation of lignan (-)-cubebin extracted from Piper cubeba on human colon adenocarcinoma cells (HT29). J Toxicol Environ Health A 79(2): 92-100.

[26] OLALYE MT and ROCHA JBT. 2007. Commonly used tropical medicinal plants exhibit distinct in vitro antioxidant activities against hepatotoxins in rat liver. Exp Toxicol Pathol 58: 433-438.

[27] OLVERA-GARCÍA V, CASTAÑO - TOSTADO E, REZENDIZ - LOPEZ RI, REYNOSO - CAMACHO R, GONZÁLEZ DE MEJÍA E, ELIZONDO G and LOARCA - PIÑA G. 2008. Hibiscus sabdariffa L. extracts inhibit the mutagenicity in microsuspension assay and the proliferation of HeLa cells. J Food Sci 73: T75-81.

[28] OUÉDRAOGO M, KONATÉ K, LEPENGUÉ AN, SOUZA A, M ’BATCHI B and SAWADOGO LL. 2012. Free radical scavenging capacity, anticandicidal effect of bioactive compounds from Sida cordifolia L., in combination with nystatin and clotrimazole and their effect on specific immune response in rats. Ann Clin Microbiol Antimicrob 11: 33.

[29] RAMASSAMY C. 2006. Emerging role of polyphenolic compounds in the treatment of neurodegenerative diseases: a review of their intracellular targets. Eur J Pharmacol 545(1): 51-64.

[30] RAMIREZ-RODRIGUES MM, PLAZA ML, AZEREDO A, BALABAN MO and MARSHALL MR. 2011. Physicochemical and phytochemical properties of cold and hot water extraction from Hibiscus sabdariffa J Food Sci 76: C428-35.

[31] ROSA RM, MELECCHI MIS, DA COSTA HALMENSCHLAGER R, ABAD FC, SIMONI CR, CARAMÃO EB, HENRIQUES JAP, SAFFI J and DE PAULA RAMOS ALL. 2006. Antioxidant and antimutagenic properties of Hibiscus tiliaceus L. methanolic extract. J Agric Food Chem 54: 7324-7330.

[32] ROSA RM, MOURA DJ, MELECCHI MIS, DOS SANTOS RS, RICHTER MF CAMARÃO EB, HENRIQUES JAP, DE PAULA RAMOS ALL and SAFFI J. 2007. Protective effects of Hibiscus tiliaceus L. methanolic extract to V79 cells against cytotoxicity and genotoxicity induced by hydrogen peroxide and tert-butyl-hydroperoxide. Toxicol In Vitro 21: 1442-1452.

[33] SPENCER JP. 2007. The interactions of flavonoids within neuronal signalling pathways. Genes Nutr 2007 2(3): 257-273.

[34] TICE RR, AGURELL E, ANDERSON D, BURLINSON B, HARTMANN A, KOBAYASHI H, MIYAMAE Y, ROJAS E, RYU JC and SASAKI YF. 2000. Single cell gel/comet assay: guidelines for in vitro and in vivo genetic toxicology testing . Environ Mol Mutagen 35: 206-321.

[35] TRINDADE C et al. 2016. Antimutagenic and antioxidant properties of the aqueous extracts of organic and conventional grapevine Vitis labrusca cv. Isabella leaves in V79 cells. J Toxicol Environ Health A 79(18): 825-836.

[36] TSUMBU CN, DEBY - DUPONT G, TITS M, ANGENO , L , FREDERICH M, KOHNEN S and MOUITHYS - MICKALAD A. 2012. Polyphenol content and modulatory activities of some tropical dietary plant extracts on the oxidant activities of neutrophils and myeloperoxidase. Int J Mol Sci 13: 628-650.

[37] VENANCIO VP, MARQUES MC, ALMEIDA , MR , MARIUTTI LR, SOUZA VC, BARBOSA FJR, PIRES BIANCHI ML, MARZOCCHI - MACHADO CM, MERCADANTE AZ and ANTUNES LM. 2016. Chrysobalanus icaco L. fruits inhibit NADPH oxidase complex and protect DNA against doxorubicin-induced damage in Wistar male rats. J Toxicol Environ Health A 79(20): 885-893.

[38] WANG ML, MORRIS B, TONNIS B, DAVIS J and PEDERSON GA. 2012. Assessment of oil content and fatty acid composition variability in two economically important Hibiscus species. J Agric Food Chem 60: 6620-6626.

Group	Dose	Period	Day 16	Day 16 (4 h)	Day 17 (24 h)
1 (Negative control)	Distillated water	15 days	Saline solution	Peripheral blood collection	Death and collection of bone marrow
2 (Positive control)	Distilled water	15 days	MMS
3	Extract (50 mg/kg)	15 days	Saline solution
4	Extract (100 mg/kg)	15 days	Saline solution
5	Extract (200 mg/kg)	15 days	Saline solution
6	Extract (50 mg/kg)	15 days	MMS
7	Extract (100 mg/kg)	15 days	MMS
8	Extract (200 mg/kg)	15 days	MMS

Compound	Concentration (μg/mL)
Caffeic acid	51.13 ± 2.60
Coumaric acid	3.72 ± 0.43
3,4 protocatechuic dihydroxybenzoic acid	3.46 ± 0.67
Gallocatechin	4.13 ± 1.06
Gallic acid	14.22 ± 3.71

Treatment	Number of animals	MnPCEs	PCE/NCE
Negative control	6	2.50 ± 1.05	0.53 ± 0.03
Positive control MMS	6	8.20 ± 3.83^*	0.54 ± 0.04
Extract 50 mg/kg	6	2.17 ± 1.17^#	0.55 ± 0.03
Extract 100 mg/kg	6	1.80 ± 1.30^#	0.55 ± 0.04
Extract 200 mg/kg	6	2.00 ± 1.67^#	0.54 ± 0.03

Treatment	Number of animals	MnPCEs	Reduction
Negative control	6	2.50 ± 1.05	-
Positive control MMS	6	8.20 ± 3.83*	-
Extract 50 mg/kg + MMS	6	3.17 ± 1.33#	88.2%
Extract 100 mg/kg + MMS	6	3.33 ± 0.82#	85.4%
Extract 200 mg/kg + MMS	6	5.50 ± 3.45	-

Brasil

Brasil

Hibiscus acetosella extract protects against alkylating agent-induced DNA damage in mice

Abstract

INTRODUCTION

MATERIALS AND METHODS

PLANT COLLECTION AND EXTRACT PREPARATION

ANALYSIS OF PHENOLIC COMPOUNDS BY HIGH-PERFORMANCE LIQUID CHROMATOGRAPHY (HPLC)

ANIMALS

EXPERIMENTAL DESIGN

COMET ASSAY

PERCENTAGE OF DAMAGE REDUCTION (DR%)

MICRONUCLEUS (MN) TESTS

STATISTICAL ANALYSIS

RESULTS

QUANTITATIVE AND QUALITATIVE ANALYSIS OF PHENOLIC COMPOUNDS BY HPLC

COMET ASSAYS: GENOTOXICITY AND ANTIGENOTOXICITY

MN tests: mutagenicity and antimutagenicity

DISCUSSION

ACKNOWLEGMENTS

REFERENCES

Publication Dates

History