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Journal of the Mexican Chemical Society
versión impresa ISSN 1870-249X
J. Mex. Chem. Soc vol.56 no.2 Ciudad de México abr./jun. 2012
Article
Antigiardial Activity of Cupania dentata Bark and its Constituents
Ignacio HernándezChávez,a Luis W. TorresTapia,a Paulino SimáPolanco,a Roberto CedilloRivera,b Rosa MooPuc,b and Sergio R. PerazaSáncheza*
a Unidad de Biotecnología, Centro de Investigación Científica de Yucatán, Calle 43 No. 130, Col. Chuburná de Hidalgo, Mérida 97200, Yucatán, México. *speraza@cicy.mx
b Unidad de Investigación Médica Yucatán, Unidad Médica de Alta Especialidad, Centro Médico Ignacio García Téllez, Instituto Mexicano del Seguro Social (IMSS), Calle 41 No. 439, Col. Industrial, Mérida 97150, Yucatán, México.
Received August 1, 2011.
Accepted November 29, 2011.
Abstract
The MeOH extract of Cupania dentata bark (Sapindaceae) as well as its hexane, CH2Cl2, EtOAc, and BuOH fractions showed high activity against Giardia lamblia trophozoites (IC50 = 2.129.52 μg/mL). The phytochemical study of fractions resulted in the isolation of taraxerone (1), taraxerol (2), scopoletin (3), and two mixtures of steroidal compounds. Taraxerone was the metabolite with the highest giardicidal activity (IC50 = 11.33 μg/mL).
Key words: Cupania dentata, Sapindaceae, giardicidal activity, taraxerone, taraxerol, scopoletin, sterols.
Resumen
El extracto MeOH de Cupania dentata corteza (Sapindaceae) así como sus fracciones de hexano, CH2C12, AcOEt y BuOH mostraron gran actividad contra los trofozoítos de Giardia lamblia (CI50 = 2.129.52 μg/mL). El estudio fitoquímico de estas fracciones resultó en el aislamiento de taraxerona (1), taraxerol (2), escopoletina (3) y dos mezclas esteroidales. Taraxerona tuvo la más alta actividad giardicida (CI50 = 11.33 μg/mL).
Palabras clave: Cupania dentata, Sapindaceae, actividad giardicida, taraxerona, taraxerol, escopoletina, esteroles.
Introduction
The protozoo Giardia lamblia is the most frequently isolated intestinal protozoan parasite around the world and it is the causal agent of the disease known as giardiasis [1]. In Latin America the prevalence of giardiasis is 3.722.3% [2] and a recent seroepidemiologic study in Mexico found an seroprevalence of 55.3%, with no significant differences among geographic regions according to their economic development [3]. The pharmacological treatment of giardiasis is based mainly in the use of nitroimidazoles, benzimidazoles, and nitrofurans; nevertheless, these drugs produce severe side effects and their indiscriminate use has generated a selection of resistant strains to these drugs [4, 5]. Due to this situation, the search for new drugs becomes necessary.
The Cupania L. genus comprises 45 species growing around warm places of the American continent [6]. C. belizensis is useful in treating diarrhea [7], C. americana leaves and seeds are used to treat pain and diarrhea, respectively [8], while C. vernalis leaves show antileishmanial activity [9]. Chemical compounds have been reported from some species, such as vernanolide, a glycosyl diterpene isolated from C. vernalis [9], a longchain fatty alcohol glycoside named cupanioside from C. glabra [7], and a polyprenol named cupaniol from C. latifolia [8].
Taking advantage of the ancestral knowledge on the medical use of some plant species growing in the Yucatan peninsula and the giardicidal activity described for the MeOH extract of Cupania dentata bark [10], we studied the hexane, CH2Cl2, EtOAc, and BuOH fractions of the MeOH extract of C. dentata bark in order to obtain those metabolites responsible of the giardicidal activity of the plant. Not any phytochemical or biological study has been reported for this species.
Results and Discussion
The methanol extract as well as the hexane, CH2Cl2, EtOAc, and BuOH fractions obtained by chromatographic partitioning were all evaluated against G. lamblia trophozoites (Table 1). The biological activity of the MeOH extract (IC50 = 8.17 μg/mL) was similar to that obtained previously (IC50 = 7.59 μg/mL) [10] and can be considered highly active according to the criteria established by Amaral et al. [11], who established extracts with IC50 ≤ 100 μg/mL as highly actives. The biological activity of C. dentata fractions remained similar to that of the crude MeOH extract (Table 1), in some cases stronger, such as the hexane and CH2Cl2 fractions (IC50 = 4.43 and 2.12 μg/mL, respectively).
Compounds 1 and 2 were isolated from the hexane fraction and were identified as taraxerone and taraxerol, respectively, by comparison of their spectroscopic data with those reported in the literature [1214]. Both compounds are ubiquitous metabolites found in a large number of plants. Compounds 1 and 2 have been reported with different biological activities, such as allelopathic and antifungal [15, 16]; taraxerol has been reported with analgesic and antiinflammatory activities [17, 18].
Also, from the hexane fraction a mixture (A) of stigmasterol and βsitosterol in a ratio 2:1 was obtained. The sterols were identified by comparison their MS data with the database of the equipment and to those reported in the literature [19]. The ratio was determined by inspection of the gas chromatogram. Both are ubiquitous compounds of plants. βSitosterol possesses different activities, such as antibacterial, antimicotic, and as an inhibitor of the carcinogenesis [20], while stigmasterol was found to inhibit tumor promotion in twostage carcinogenesis in mice [21]. The mixture of both sterols has shown antiinflammatory activity in topical applications [22].
Compound 3 was isolated from the CH2Cl2 fraction and was identified as scopoletin, a 6,7dioxygenated coumarin, by comparison of its spectroscopic data with those reported in the literature [23, 24]. Scopoletin exhibited a potent inhibitory effect on rabbit platelet aggregation [25] and showed activity as inhibitor of eicosanoidrelease from ionophorestimulated mouse peritoneal macrophages [26].
The mixture B was isolated from the BuOH fraction and was identified as a combination of βsitosterol3OβDglucopyranoside and stigmasterol3OβDglucopyranoside (1:1.5). The ratio was determined by inspection of the 1H NMR spectrum. The components of this mixture were identified by comparison of their spectroscopic data, mainly 13C NMR, with those reported in the literature [27].
None of the metabolites mentioned above has been reported in the literature as having antigiardial activity, except for two reports on βsitosterol and its glucoside [28, 29] with an IC50 = 71.1 and 61.5 μ/mL, respectively, but the mixture of stigmasterolβsitosterol (2:1) has not been reported with this activity. In the present work, the two triterpenes taraxerone (1) and taraxerol (2) showed an IC50 = 11.33 and 16.11 μg/mL, respectively, while the coumarin scopoletin (3) had an IC50 = 33.60 μg/mL in the growth inhibition bioassay. In the literature there are 31 metabolites reported as having antigiardial activity with an IC50 ≤ 25.0 μg/mL [11], then the antigiardial activity of 1 and 2, in comparison, is considered outstanding on this aspect, but moderate with respect to the drug of election, metronidazole, which showed an IC50 = 0.2 μg/mL. Taraxerol acetate did not show antigiardial activity in the same model. Scopoletin (3) showed only a week activity against G. lamblia, but this is the first report of scopoletin as having this activity. The mixture of sterols (A) showed a stronger activity, with an IC50 = 5.23 μg/mL, which, perhaps, depends on the synergism that there might be within stigmasterol and βsitosterol together, but more studies are necessary to confirme this hypothesis. The mixture (B) of stigmasterol and βsitosterol glucosides showed less activity (IC50 = 26.77 μ/mL) than the mixture (A). In other bioassay models, some works have demonstrated activity of various mixtures, such as that formed of the stilbene pinosylvin and the flavonoid galangin that worked in concert to provide antifeedant activity, while they were not active individually [30].
General Experimental Procedures
EIMS data were determined on an Agilent Technologies 6890N chromatograph connected to a mass detector 5975B. The 1H and 13C NMR data were obtained on a Bruker Avance 400 instrument (400 MHz). Chemical shifts were referred to TMS (δ 0) as internal standard. Vacuum liquid chromatography (VLC) separations were carried out using TLCgrade silica gel (Merck); opencolumn chromatography separations were run using silica gel 60 (70230 mesh, Merck); and flash columns were run using silica gel 60 (230400 mesh, Merck). Sephadex LH20 (GE Healthcare) was used for gel permeation column chromatography. Preparative TLC (PTLC) separations were performed on glasscoated (1 mm thickness) 20 x 20 cm plates (Aldrich). TLC analyses were carried out using aluminumbacked silica gel 60 F254 plates (0.20 mm thickness, Merck); spots on TLC plates were first visualized under a UV lamp (254 and 365 nm) and then by spraying with 4% phosphomolibdic acid containing a trace of ceric sulfate in 5% H2SO4, followed by heating at 100 °C.
Plant Material
The bark of Cupania dentata DC. (Sapindaceae) was collected 22 Km west of Bacalar on the road to Carrillo Puerto, Quintana Roo, Mexico, and identified by the experienced taxonomist Paulino Simá Polanco. A voucher specimen (PSimá 2587) was deposited on the herbarium of the Unidad de Recursos Naturales of the Centro de Investigación Científica de Yucatán.
Extraction and Isolation
Driedground bark (983 g) was extracted with methanol three times at room temperature, for 48 h each time. After filtration, the extracts were combined and the solvent was evaporated under reduced pressure to give 166.4 g of organic extract. The extract was suspended in a mixture of methanol/water (1:3, 500 mL) and the resulting aqueous suspension was successively partitioned between hexane (2:1, 3x), CH2Cl2 (2:1, 3x), EtOAc (2:1, 3x), and BuOH (2:1, 3x), to afford the hexane (6.1 g), CH2Cl2 (11.0 g), EtOAc (59.2 g), and BuOH (30.2 g) fractions.
The hexane fraction was purified by VLC using gradient elutions of hexane/ethyl acetate, ethyl acetate/acetone and acetone/methanol to produce nine fractions (3A3I) and a precipitate, which was washed with methanol and then recrystallized from chloroform to give 51.9 mg of the mixture (A) of stigmasterol and βsitosterol. The fractions 3B and 3C presented two different precipitates, both were washed with methanol and then recrystallized from chloroform, to give taraxerone (1, 16.0 mg), with m.p. = 241243 °C and [a]D = + 11.9° (CHCl3) [31], and taraxerol (2, 52.2 mg), with m.p. = 279280 °C and [α]D = + 2.9° (CHCl3) [31].
The CH2Cl2 fraction was purified by VLC, using gradient elutions of hexane/dichloromethane and dichloromethane/ methanol to produce seven fractions (4A4G). Opencolumn chromatography purification of fraction 4D (538.1 mg) eluting with dichloromethane and gradient mixtures of dichloromethane/methanol produced 11 fractions (5A5K). Further purification of fraction 5C (136.9 mg), using an open chromatography column with chloroform/methanol (98:2), afforded fractions 6D and 6E, which were washed with hexane and then recrystallized from methanol to give 37.7 mg of compound 3, with m.p. = 199201 °C [32].
The BuOH fraction was purified by a SephadexLH20 column using gradient elutions of methanol/butanol/water to produce nine fractions (7A7I). Fraction 7B was further purified using a SephadexLH20 column in methanol to obtained 58.7 mg of crystals of mixture (B), constituted by stigmasterol glucoside and βsitosterol glucoside.
Taraxerol acetate (4). A mixture of taraxerol (10 mg), acetic anhydride (1 mL) and pyridine (0.5 mL) was allowed to stir at room temperature for 72 h. After the usual work up 7.3 mg (66.4%) of crude acetylated product, identified as taraxerol acetate (4), were obtained, with m.p. = 296298 °C [31].
Taraxerone (1). White crystals: mp 241243 °C; [α]D +11.9 (c 0.360, CHCl3); 1H NMR (CDCl3, 400 MHz) δ 5.56 (1H, dd, J = 3.2, 8.2 Hz, H15), 2.58 (1H, m, H2a), 2.33 (1H, m, H2b), 2.07 (1H, dt, J = 3.3, 12.9 Hz, H7a), 1.92 (1H, dd, J = 3.1, 15.1 Hz, H16a), 1.88 (1H, m), 1.14 (3H, s, H25), 1.09 (3H, s, H26), 1.08 (3H, s, H23), 1.07 (3H, s, H24), 0.95 (3H, s, H29), 0.92 (3H, s, H27), 0.91 (3H, s, H30), 0.83 (3H, s, H28); 13C NMR (CDCl3, 100 MHz) δ 217.7 (C3), 157.6 (C14), 117.2 (C15), 55.8 (C5), 48.7 (C18), 48.7 (C9), 47.6 (C4), 40.6 (C19), 38.9 (C8), 38.3 (C1), 37.7 (C13), 37.7 (C17), 37.5 (C10), 36.7 (C16), 35.8 (C12), 35.1 (C7), 34.1 (C2), 33.5 (C21), 33.3 (C29), 33.1 (C22), 29.8 (C26), 29.9 (C28),28.8 (C20), 26.1 (C23), 25.6 (C27), 21.5 (C24), 21.3 (C30), 19.9 (C6), 17.4 (C11), 14.8 (C25); EIMS m/z (rel. int.): 424 [M]+ (25), 300 (87), 285 (70), 204 (100), 133 (67).
Taraxerol (2). White crystals: mp 279280 °C; [α]D +2.9 (c 0.490, CHCl3); 1H NMR (CDCl3, 400 MHz) δ 5.53 (1H, dd, J = 3.2, 8.2 Hz, H15), 3.24 (1H, dd, J = 4.7, 11.0 Hz, H3), 2.03 (1H, dt, J = 3.1, 12.6 Hz, H7a), 1.92 (1H, dd, J = 3.0, 14.6 Hz, H16a), 1.09 (3H, s, H26), 0.98 (3H, s, H23), 0.95 (3H, s, H29), 0.93 (3H, s, H25), 0.91 (3H, s, H27), 0.90 (3H, s, H30), 0.82 (3H, s, H28), 0.80 (3H, s, H24); 13C NMR (CDCl3, 100 MHz) δ 158.1 (C14), 116.9 (C15), 79.1 (C3), 55.5 (C5),49.2 (C18), 48.7 (C9), 41.3 (C19), 39.0 (C4), 38.7 (C8),38.0 (C1), 37.7 (C17), 37.6 (C13), 37.5 (C10), 36.6 (C16),35.8 (C12), 35.1 (C7), 33.7 (C21), 33.3 (C29), 33.1 (C22),29.9 (C28), 29.8 (C26), 28.8 (C20), 28.0 (C23), 27.1 (C2),25.9 (C27), 21.3 (C30), 18.8 (C6), 17.5 (C11), 15.4 (C24), 15.4 (C25); EIMS m/z (rel. int.): 426 [M]+ (9), 302 (25), 287(25), 204 (100), 133 (40).
Scopoletin (3). Yellow crystals: mp 199201 °C; 1H NMR (CD3OD, 400 MHz) δ 7.86 (1H, d, J = 9.5 Hz, H4), 7.13 (1H, s, H5), 6.78 (1H, s, H8), 6.21 (1H, d, J = 9.6 Hz, H3), 3.81 (3H, s, 6OCH3); 13C NMR (CD3OD, 100 MHz): δ 164.1 (C2), 152.9 (C7), 151.4 (C9), 147.1 (C6), 146.1 (C4), 112.6 (C3), 112.6 (C10), 109.9 (C5), 103.9 (C8), 56.8 (6OCH3); EIMS m/z (rel. int.): 192.1 [M]+ (100), 177 (64), 164 (29), 149 (60), 121 (27), 69 (43), 79 (21).
Biological evaluation
Giardia lamblia trophozoites
Giardia lamblia IMSS:0696:1 isolate, obtained from an individual with symptomatic giardiasis, was used [33]. Trophozoites were cultured in TYIS33 modified medium, supplemented with 10% calf serum, and subcultured twice a week; for the assay, trophozoites were tested in their log phase of growth [34].
Antiprotozoal assay
The assay has been described in the literature [3537]. Stock solutions of extracts, fractions, or pure compounds were prepared with DMSO (5 mg/mL), from which, by means of twofolded serial dilutions with TYIS33 modified medium, four final solutions in a range of 150 μ/mL were obtained. Each solution was inoculated with G. lamblia to achieve an inoculum of 5 x 104 trophozoites/mL. The test included metronidazole (SigmaAldrich) as the drug of reference, a control (culture medium with trophozoites and DMSO), and a blank (culture medium). After 48 h at 37 °C, parasites were detached by chilling, and 50 iL of each culture tube were subcultured in fresh medium without extracts or drug and incubated for 48 h at 37 °C. Cell proliferation was measured with a hemocytometer, and the percentage of trophozoite growth inhibition was calculated by comparison with the controls. The percentage of inhibition calculated for each concentration was transformed into Probit units. The plot of Probit against log concentration was made; the best straight line was determined by regression analysis, and the 50% inhibitory concentration (IC50) values were calculated. The experiments were done in duplicate and repeated at least three times.
Acknowledgements
This work was supported by the International Foundation for Science (IFS), Stockholm, Sweden, and the Organization for the Prohibition of Chemical Weapons (OPCW), The Hague, Netherlands, through a research grant to Dr. Sergio R. PerazaSánchez (Agreement No. F/32782F). Ignacio HernándezChávez thanks CONACYT for a thesis scholarship (170695).
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