Abstract
Various beneficial biological activities have been reported for passion fruit (Passiflora edulis), grown in tropical and subtropical regions. However, no study has yet demonstrated its action against the Zika virus (ZIKV) infection. The present study aimed to investigate the anti-ZIKV of the ethanolic passion fruit seed extract (PFSE), from which, liquid chromatography tandem mass spectrometry (LC-MS/MS) analysis allowed to putatively annotate the occurrence of piceatannol, astringin, scirpusin A, scirpusin B, isookanin-7-O-glucoside and naringenin-7-O-glucoside, two quadranguloside derivatives, tyrosine, and phenylalanine. PFSE is well tolerated by cell lines (Vero E6 and HTR-8/SVneo) and tissue explants from the human placenta. With 1- and 24-h treatments, PFSE consistently reduced the viral load and NS1 protein expression of the two strains of ZIKV (MR766 and PE243) in placental explants and cell lines. Thus, PFSE has a promising potential for developing anti-ZIKV treatments, protecting the placenta against infection caused by ZIKV, along with relevant antioxidant potential, represented by ferric reducing antioxidant power (FRAP) of 390.5 Trolox eq per g dry extract and half maximal inhibitory concentration (IC50) for 2,2-diphenyl-1-picrylhydrazyl radical (DPPH•) of 12.1 µg mL-1, and more than 90% protection from lipid peroxidation. Although further studies need to be conducted, PFSE treatment was safe and effective in trophoblast cells and placental explants, thus representing a promising class of all-accessible products based on the reuse of industrial by-products.
Keywords:
passion fruit seeds; placenta protection; antiviral activity; piceatannol; agroindustrial waste
Introduction
Brazil is the largest producer of yellow passion fruit (Passiflora edulis f. flavicarpa) in the world, with approximately 60% of the global production.11 Oliveira, D. A.; Angonese, M.; Ferreira, S. R. S.; Gomes, C. L.; Food Bioprod. Process. 2017, 104, 137.,22 Corrêa, R. C. G.; Peralta, R. M.; Haminiuk, C. W. I.; Maciel, G. M.; Bracht, A.; Ferreira, I. C. F. R.; Trends Food Sci. Technol. 2016, 58, 79. Passion fruit is widely planted in tropical and subtropical regions in several parts of the world, especially in South America, the Caribbean, South Florida, South Africa, and Asia.33 He, X.; Luan, F.; Yang, Y.; Wang, Z.; Zhao, Z.; Fang, J.; Wang, M.; Zuo, M.; Li, Y.; Front. Pharmacol. 2020, 11, 617; Duarte, I. A. E.; Milenkovic, D.; Borges, T. K.; de Oliveira, L. L.; Costa, A. M.; Food Funct. 2021, 12, 11106; Zeraik, M. L.; Pereira, C. A. M.; Zuin, V. G.; Yariwake, J. H.; Rev. Bras. Farmacogn. 2010, 20, 459; Zeraik, M. L.; Serteyn, D.; Deby-Dupont, G.; Wauters, J.-N.; Tits, M.; Yariwake, J. H.; Angenot, L.; Franck, T.; Food Chem. 2011, 128, 259. Passion fruit has a yellowish peel in maturity, and contains multiple seeds (dark in color) surrounded by yellow gelatinous pulp with an acid-sweet flavor and intense aroma.22 Corrêa, R. C. G.; Peralta, R. M.; Haminiuk, C. W. I.; Maciel, G. M.; Bracht, A.; Ferreira, I. C. F. R.; Trends Food Sci. Technol. 2016, 58, 79. The seeds are widely used for the extraction of oil, which serves as raw material, mainly for cosmetic and nutritional purposes.44 Kiefer, J.; Lampe, A. I.; Nicoli, S. F.; Lucarini, M.; Durazzo, A.; Molecules 2019, 24, 3219. After extracting the oil from the seeds, a residual cake is obtained, which is generally underutilized. However, it is rich in bioactive compounds such as the stilbenes piceatannol and scirpusin B, phenolic compounds and flavonoids.55 Gadioli, I. L.; da Cunha, M. S. B.; de Carvalho, M. V. O.; Costa, A. M.; Pineli, L. L. O.; Crit. Rev. Food Sci. Nutr. 2018, 58, 785; Barbosa Santos, T.; de Araujo, F. P.; Neto, A. F.; de Freitas, S. T.; de Souza Araújo, J.; de Oliveira Vilar, S. B.; Brito Araújo, A. J.; Lima, M. S.; Int. J. Fruit Sci. 2021, 21, 255.
Beneficial biological activities have been reported for the Passiflora edulis species, from different parts of the plant,33 He, X.; Luan, F.; Yang, Y.; Wang, Z.; Zhao, Z.; Fang, J.; Wang, M.; Zuo, M.; Li, Y.; Front. Pharmacol. 2020, 11, 617; Duarte, I. A. E.; Milenkovic, D.; Borges, T. K.; de Oliveira, L. L.; Costa, A. M.; Food Funct. 2021, 12, 11106; Zeraik, M. L.; Pereira, C. A. M.; Zuin, V. G.; Yariwake, J. H.; Rev. Bras. Farmacogn. 2010, 20, 459; Zeraik, M. L.; Serteyn, D.; Deby-Dupont, G.; Wauters, J.-N.; Tits, M.; Yariwake, J. H.; Angenot, L.; Franck, T.; Food Chem. 2011, 128, 259. including anti-inflammatory,66 Montanher, A. B.; Zucolotto, S. M.; Schenkel, E. P.; Fröde, T. S.; J. Ethnopharmacol. 2007, 109, 281. neuropharmacological and antidepressant effects,77 Sena, L. M.; Zucolotto, S. M.; Reginatto, F. H.; Schenkel, E. P.; de Lima, T. C. M.; Exp. Biol. Med. 2009, 234, 967.,88 Alves, J. S. F.; Silva, A. M. S.; da Silva, R. M.; Tiago, P. R. F.; de Carvalho, T. G.; de Araújo Jr., R. F.; de Azevedo, E. P.; Lopes, N. P.; Ferreira, L. D. S.; Gavioli, E. C.; da Silva-Júnior, A. A.; Zucolotto, S. M.; Pharmaceutics 2020, 12, 383. anti-aging,99 Yepes, A.; Ochoa-Bautista, D.; Murillo-Arango, W.; Quintero-Saumeth, J.; Bravo, K.; Osorio, E.; Arabian J. Chem. 2021, 14, 102905. and antiproliferative effects on cancer cells via glyoxalase I (GLO I), the cellular enzyme that participates in the detoxification of methylglyoxal;1010 Yamamoto, T.; Sato, A.; Takai, Y.; Yoshimori, A.; Umehara, M.; Ogino, Y.; Inada, M.; Shimada, N.; Nishida, A.; Ichida, R.; Takasawa, R.; Maruki-Uchida, H.; Mori, S.; Sai, M.; Morita, M.; Tanuma, S.-i; Biochem. Biophys. Rep. 2019, 20, 100684. these effects also have been observed for its constituents, piceatannol and scirpusin B,1010 Yamamoto, T.; Sato, A.; Takai, Y.; Yoshimori, A.; Umehara, M.; Ogino, Y.; Inada, M.; Shimada, N.; Nishida, A.; Ichida, R.; Takasawa, R.; Maruki-Uchida, H.; Mori, S.; Sai, M.; Morita, M.; Tanuma, S.-i; Biochem. Biophys. Rep. 2019, 20, 100684. which prevent lipid oxidation in dairy beverages,1111 Rotta, E. M.; Giroux, H. J.; Lamothe, S.; Bélanger, D.; Sabik, H.; Visentainer, J. V.; Britten, M.; LWT- Food Sci. Technol. 2020, 123, 109088. have a suppressive effect on IgE production revealing their antiallergic potential,1212 Mizusaki, A.; Nishi, K.; Nishiwaki, H.; Ishida, M.; Tamamoto, T.; Sugahara, T.; J. Funct. Foods 2017, 32, 176. attenuate oxidative stress1313 Kandandapani, S.; Balaraman, A. K.; Ahamed, H. N.; Chin. J. Nat. Med. 2015, 13, 680. and have antidiabetic and antiplatelet effects,1414 Salles, B. C. C.; Silva, M. A.; Taniguthi, L.; Ferreira, J. N.; Rocha, C. Q.; Vilegas, W.; Dias, P. H.; Pennacchi, P. C.; Duarte, S. M. S.; Rodrigues, M. R.; Brigagão, M. R. P. L.; Paula, F. B. A.; Biol. Pharm. Bull. 2020, 43, 169. among others. To our knowledge, there are still no reports on the protective effect against Zika virus (ZIKV) infection, and dereplication strategies have played a central role in various strategies to define possible new biological activities for natural products.1515 Pilon, A. C.; Selegato, D. M.; Fernandes, R. P.; Bueno, P. C. P.; Pinho, D. R.; Carnevale Neto, F.; Freire, R. T.; Castro-Gamboa, I.; Bolzani, V. S.; Lopes, N. P.; Quim. Nova 2020, 43, 329; Brunetti, A. E.; Carnevale Neto, F.; Vera, M. C.; Taboada, C.; Pavarini, D. P.; Bauermeister, A.; Lopes, N. P.; Chem. Soc. Rev. 2018, 47, 1574. In this way, the determination of the chemical composition of complex mixtures like ethanol passion fruit seed extract (PFSE) can be a challenge. Mass spectrometry is one of the possible analytical methods for metabolomics analyses in natural products, looking for or not for specific chemical signals.1515 Pilon, A. C.; Selegato, D. M.; Fernandes, R. P.; Bueno, P. C. P.; Pinho, D. R.; Carnevale Neto, F.; Freire, R. T.; Castro-Gamboa, I.; Bolzani, V. S.; Lopes, N. P.; Quim. Nova 2020, 43, 329; Brunetti, A. E.; Carnevale Neto, F.; Vera, M. C.; Taboada, C.; Pavarini, D. P.; Bauermeister, A.; Lopes, N. P.; Chem. Soc. Rev. 2018, 47, 1574. In a recent study,88 Alves, J. S. F.; Silva, A. M. S.; da Silva, R. M.; Tiago, P. R. F.; de Carvalho, T. G.; de Araújo Jr., R. F.; de Azevedo, E. P.; Lopes, N. P.; Ferreira, L. D. S.; Gavioli, E. C.; da Silva-Júnior, A. A.; Zucolotto, S. M.; Pharmaceutics 2020, 12, 383. the chemical profile of Passiflora edulis leaves, cultivated in the Rio Grande do Norte, was published, where liquid chromatography tandem mass spectrometry (LC-MS/MS) had shown a predominant accumulation of C-flavonoids in this cultivar. All structures were proposed based on the gas phase decomposition chemistry. Later, the injection of standards confirmed all the proposals,88 Alves, J. S. F.; Silva, A. M. S.; da Silva, R. M.; Tiago, P. R. F.; de Carvalho, T. G.; de Araújo Jr., R. F.; de Azevedo, E. P.; Lopes, N. P.; Ferreira, L. D. S.; Gavioli, E. C.; da Silva-Júnior, A. A.; Zucolotto, S. M.; Pharmaceutics 2020, 12, 383. opening the perspective to use the same strategy for seeds extracts analysis.
In recent years, several arboviruses, a high proportion seen in tropical and subtropical regions, have been responsible for numerous outbreaks worldwide.1616 Goh, V. S. L.; Mok, C. K.; Chu, J. J. H.; Molecules 2020, 25, 2796. Among arboviruses, ZIKV has attracted worldwide attention since the appearance of the infection in Brazil in 2015,1717 Gurung, S.; Nadeau, H.; Maxted, M.; Peregrine, J.; Reuter, D.; Norris, A.; Edwards, R.; Hyatt, K.; Singleton, K.; Papin, J. F.; Myers, D. A.; J. Virol. 2020, 94, e00058-20. where it caused a worrying number of newborns with brain malformations.1818 Rodriguez-Morales, A. J.; Cardona-Ospina, J. A.; Ramirez-Jaramillo, V.; Gaviria, J. A.; González-Moreno, G. M.; Castrillón-Spitia, J. D.; López-Villegas, A.; Morales-Jiménez, E.; Ramírez-Zapata, V.; Rueda-Merchán, G. E.; Trujillo, A. M.; Tabares-Villa, F. A.; Henao-SanMartin, V.; Murillo-Garcia, D. R.; Herrera-Soto, J. A.; Buitrago-Cañas, M. L.; Collins, M. H.; Sepúlveda-Arias, J. C.; Londoño, J. J.; Bedoya-Rendón, H. D.; de Jesús Cárdenas-Pérez, J.; Olaya, S. X.; Lagos-Grisales, G. J.; Travel Med. Infect. Dis. 2018, 25, 20. ZIKV infection during pregnancy can also lead to infection of the fetus by vertical transmission, which can result in spontaneous abortion, microcephaly, and other neurological damages, in addition to congenital anomalies collectively addressed as ZIKV congenital syndrome.1717 Gurung, S.; Nadeau, H.; Maxted, M.; Peregrine, J.; Reuter, D.; Norris, A.; Edwards, R.; Hyatt, K.; Singleton, K.; Papin, J. F.; Myers, D. A.; J. Virol. 2020, 94, e00058-20.,1919 Rasmussen, S. A.; Jamieson, D. J.; Birth Defects Res. 2020, 112, 1139. Therefore, the impact of ZIKV infection on human health reflects devastating fetal and neonatal outcomes, including long-term infection.2020 Cao, B.; Diamond, M. S.; Mysorekar, I. U.; J. Interferon Cytokine Res. 2017, 37, 287. In this context, preventing placental infection by ZIKV is important in order to protect the fetus; however, existing antiviral drugs may be harmful to the pregnancy.
As such, natural products such as the presently reported PFSE could be an alternative to protect fetuses from the harmful effects of ZIKV infection during pregnancy, which is cited by the World Health Organization (WHO) as a priority in the research and development plans for neglected diseases.2121 http://who.int/blueprint/priority-diseases/en/, accessed in December 2021.
http://who.int/blueprint/priority-diseas...
Experimental
Chemicals
The analytical grade compounds were purchased from Sigma-Aldrich (Steinheim, Germany): DPPH• (α,α diphenyl-picrylhydrazyl radical), TPTZ (2,4,6-tripyridyl-s-triazine), AAPH (2,2-azobis(2 amidinopropane)di-hydrochloride), soy phosphatidylcholine, Trolox®, methylglyoxal, hemoglobin, fluorescein, formic acid and acetonitrile, F12 culture medium, L-15 medium. Hank’s balanced salt solution (HBSS), phosphate-buffered saline (PBS) and trypsin-ethylenediamine tetraacetic acid (EDTA), fetal bovine serum (FBS) and L-glutamine were purchased from Thermo Fisher Scientific (Waltham, MA, USA). Chloroquine was provided by Farmanguinhos (Fundação Oswaldo Cruz, Rio de Janeiro, Brazil). 4,4-Difluoro-5 (4 phenyl-1,3 butadienyl)-4-bora-3a,4a-diaza-S indacene-3 undecanoic acid (C11 BODIPY581/591) was obtained from Molecular Probes (Ontario, Canada). All reagents were of analytical grade, and the stock solutions and buffers were prepared with Milli-Q purified water.
Preparation of the ethanol extracts of passion fruit seeds
Passiflora edulis seeds were separated from the pulp, washed with distilled water, and dried in an oven at 50 °C for 48 h. The seeds were then ground in a blade mill and stored in amber glass vials. Firstly, 12 g of dry seeds was weighed and degreased using hexane (250 mL) in a Soxhlet apparatus for a period of 6 h and extraction performed in ethanol (250 mL) for 6 h. The extract was concentrated in a rotary evaporator, stored in amber glass under refrigeration at 4 ºC, and identified as PFSE. SisGen access number: A9493F8.
Characterization of the ethanolic extract
The PFSE was analyzed by high-performance liquid chromatography (HPLC) with a diode array detector coupled to a mass spectrometer with electrospray ionization source (ESI) and time of flight analyzer (HPLC-ESI-MS/MS, micrOTOF-QII, Bruker Daltonics®, Billerica, MA, USA). For chromatographic analysis, 5 mg of the PFSE was mixed with 2 mL of a methanol-water solution (75:25). The chromatographic parameters used were: Kinetex XB C18 column (100 × 2.1 mm, 2.6 μm, 100 Å), temperature 40 °C, injection volume 2 μL, and flow rate 0.4 mL min-1. The mobile phase was composed of 0.1% formic acid in water (v/v; solvent A) and 0.1% formic acid in acetonitrile (v/v; solvent B). The elution gradient started with a ramp 5 to 35% B for 23 min, 35 to 100% B for 17 min, maintaining 100% B for 8 min and then 100 to 5% B in 2 min, remaining at 5% B for 10 min and ending the run in a total time of 60 min.
The detection system consisted of a mass spectrometer operated in positive and negative ionization modes. In the first ionization mode, a capillary voltage of 4.5 kV and a cone voltage of 500 V were used as instrumental parameters. For the negative ionization mode, a capillary voltage of 3.2 kV and a cone voltage of 400 V were used. In both measurement modes, a temperature of 200 °C and a mass detection range of m/z 50-1500 were used. The parameters of MS/MS were Auto MS/MS with the selection of precursor ions in cycles of 3.0 s, excluding the selection after detection of two spectra of the same ion or after 0.60 min, reconsidering its selection if the ion intensity precursor was twice the previous. For the fragmentation of precursor ions a collision energy ramp of 20 to 50 eV was used.
Radical scavenging ability toward DPPH• (RSA-DPPH•)
The antioxidant capacity of the PFSE was determined by radical scavenging using the DPPH• method.2222 Sánchez-Moreno, C.; A. Larrauri, J.; Saura-Calixto, F.; Food Res. Int. 1999, 32, 407. Aliquots of 0.30 mL of the extract dissolved in ethanol (5-25 μg mL-1) were mixed with 2.70 mL of DPPH• solution (40 μg mL-1 in methanol). The mixture was then homogenized and stored in the dark for 30 min and the measurements performed at 516 nm, using a UV-Vis spectrophotometer (Agilent 8453, Burlington, MA, United States). The analyses were performed in triplicate (n = 3) and the percentage inhibition or the IC50 (half maximal inhibitory concentration) was calculated graphically, using an analytical curve in the linear range, by plotting the extract concentration versus the corresponding scavenging effect (I%, inhibition percentage) at 30 min.
Ferric reducing antioxidant power (FRAP) assay
The FRAP assay was performed according to the method described previously with some modifications.2323 Benzie, I. F.; Strain, J. J.; Anal. Biochem. 1996, 239, 70. Briefly, the FRAP reagent was prepared by mixing a solution of TPTZ (10 mM) in 40 mM HCl, FeCl3 (20 mM), and acetate buffer (pH 3.6, 0.30 M). 90 μL of sample (25 μg mL-1) were mixed with 2.7 mL of FRAP reagent and then incubated at 37 °C for 30 min. The absorbance of the reaction mixture was measured at 595 nm and an analytical curve prepared with Trolox® (0.04 to 7.50 μg mL-1). The analyses were performed in triplicate (n = 3) and the results expressed as Trolox equivalent antioxidant capacities (TEAC) in mg Trolox eq per g dry extract.
Lipid peroxidation measurements
Unilamellar vesicles of soy phosphatidylcholine (1 mM) were prepared by extrusion (100 nm pore diameter membrane, at 25 °C),2424 MacDonald, R. C.; MacDonald, R. I.; Menco, B. P. M.; Takeshita, K.; Subbarao, N. K.; Hu, L. R.; Biochim. Biophys. Acta, Biomembr. 1991, 1061, 297. in 10 mL of phosphate buffer (50 mM) at pH 7.4 with the additional incorporation of 0.1 μM of the peroxyl-sensitive fluorescent probe C11 BODIPY581/591.2525 Drummen, G. P.; van Liebergen, L. C.; den Kamp, J. A. O.; Post, J. A.; Free Radical Biol. Med. 2002, 33, 473. The particle size was measured by Nanotrac-Zetatrac, model NPA151-31 A-0000-D30-10 M (Microtrac, Burlington, MA, United States), at around 100 nm.
Fluorescence measurements were carried out at 37 °C, using an RF-5301PC spectrofluorophotometer (Shimadzu, Minato, Japan). In a 1-mL quartz cuvette, adequate amounts of unilamellar vesicle suspension, phosphate buffer pH 7.4, and the PFSE (5, 25, and 50 μg mL-1) or positive control (Trolox, 100 μg mL-1) were mixed. Ethanol was used as negative controls. The reaction was initiated by the addition of 100 μL of AAPH (100 mM). The fluorescence decay of fluorescent probe (λex = 580 nm, λem = 600 nm) was monitored continuously for 30 min. The analyses were performed in triplicate (n = 3).
HTR-8/SVneo cell line culture
The HTR-8/SVneo (ATCC® CRL-3271™) was kindly donated by Prof Estela Bevilacqua from the University of São Paulo. It was a placental cell line derived from first trimester extravillous trophoblast cells, routinely cultured in DMEM/F12 medium, supplemented with 10% (v/v) FBS and 2 mM L-glutamine and kept in a humid incubator at 37 ºC and 5% CO2. Cells were subcultured every 5 days with 80% confluence for HTR-8/SVneo cells and the medium replenished every 2 days.
Ethical issues
The ethical committee approved the use of placentas from the Federal University of Alagoas through the national Plataforma Brasil unified system (CAEE 57828616.3.0000.5013), with signed informed consent from all patients according to Brazilian Health Ministry guidelines.
Placenta collection and chorionic villi explant culture
Placentas derived from term pregnancies (37-40 weeks of pregnancy) were obtained from the Obstetrics Service of Prof Alberto Antunes University Hospital of the Federal University of Alagoas, Brazil (HUPAA/UFAL) by elective cesarean section. Five-term placentas from healthy pregnant women were collected from women with no detectable infections, hypertensive disorders, chronic diseases, or other conditions. After placenta collection, fresh samples from the chorionic villi were washed extensively in 0.1 M PBS and HBSS, followed by the separation of terminal chorionic villi for explant culture in 24-well plates with DMEM/F12-supplemented medium, and kept in a humid incubator at 37 ºC and 5% CO2 where they could be cultured for 12 days without losing significant viability, as described previously,2626 Miller, R. K.; Genbacev, O.; Turner, M. A.; Aplin, J. D.; Caniggia, I.; Huppertz, B.; Placenta 2005, 26, 439. and used routinely worldwide.
The 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) cell viability assay
The MTT assay was used to verify the possible cytotoxicity of the PFSE on both placental cell lines and placental explant cultures. As such, placental explants were weighed and plated in equal proportions in each well, and Vero E6 cells or HTR-8/SVneo cells were plated at 2.5 × 105 cells per well and treated with the extract diluted in DMEM/F12 medium in different concentrations (0.01, 0.1, 1, 10, and 100 μg mL-1), and cultured for a further 24 h. Since chloroquine (CQ) has been described as a potent in vitro anti-ZIKV agent,2727 Delvecchio, R.; Higa, L. M.; Pezzuto, P.; Valadão, A. L.; Garcez, P. P.; Monteiro, F. L.; Loiola, E. C.; Dias, A. A.; Silva, F. J. M.; Aliota, M. T.; Caine, E. A.; Osorio, J. E.; Bellio, M.; O’Connor, D. H.; Rehen, S.; de Aguiar, R. S.; Savarino, A.; Campanati, L.; Tanuri, A.; Viruses 2016, 8, 322.
28 Li, C.; Zhu, X.; Ji, X.; Quanquin, N.; Deng, Y. Q.; Tian, M.; Aliyari, R.; Zuo, X.; Yuan, L.; Afridi, S. K.; Li, X. F.; Jung, J. U.; Nielsen-Saines, K.; Qin, F. X. F.; Qin, C. F.; Xu, Z.; Cheng, G.; EBioMedicine 2017, 24, 189.-2929 Shiryaev, S. A.; Mesci, P.; Pinto, A.; Fernandes, I.; Sheets, N.; Shresta, S.; Farhy, C.; Huang, C. T.; Strongin, A. Y.; Muotri, A. R.; Terskikh, A. V.; Sci. Rep. 2017, 7, 15771. we tested whether it would affect cell lines or placental explants viability at 50 μg mL-1, in order to use it as a positive control added 1 h after ZIKV incubation. The control group had no addition of extracts. The medium was replaced with a fresh culture medium containing 5 μg mL-1 of MTT and the supernatant discarded after a 4-h incubation period at 37 °C, followed by the addition of 150 μL of DMSO. The absorbance of the dissolved MTT formazan product was measured spectrophotometrically at 540 nm. The percentage viability was determined in relation to the controls [(absorbance of treated cells/absorbance of untreated cells) × 100].
Zika virus propagation and titration
Two stock strains of ZIKV were kindly donated by Dr Juliano Bordignon from the Instituto Carlos Chagas of Fundação Oswaldo Cruz (ICC/FIOCRUZ-PR): the MR766 strain (isolated in Uganda in 1947, third passage, stock titer of 6.25 × 107 fluorescent focus units (FFU) mL1, GenBank accession KX421193), and the PE243 strain (isolated in Pernambuco, Brazil in 2016, third passage, stock titulation of 1 × 108 FFU mL-1, GenBank accession MF352141.1). To perform viral propagation, both strains were cultured, in separate, in Aedes albopictus derived C6/36 cells with L-15 medium supplemented with 10% (v/v) FBS, 10% (v/v) tryptose and 1% PSA until 80% confluence. Cell-free supernatants were harvested 5 days post-infection (dpi), aliquoted, and stored at -80 °C. Titration was performed after viral infection using green monkey kidney-derived Vero E6 cells cultured with supplemented DMEM for 1 h under gentle agitation. The media was changed and cells were incubated with 1.5% (m/v) carboxymethylcellulose (CMC) in DMEM with 2% FBS at 1:1 (v/v). Plaque formation was observed at 5 dpi after 10% (v/v) formalin fixation and 2% (v/v) violet crystal staining. Viral titration of MR766 strain was stocked at 5 × 105 plaque-forming units (PFU) mL-1 and PE243 at 3 × 105 PFU mL-1.
ZIKV infection of HTR-8/SVneo cells and treatment
Cells were plated at 3 × 105 cells per well in 24-well plates for 24 h, with DMEM/F12 medium supplemented with 2% FBS and received 100 μg mL-1 of the PFSE for 1 h. Afterward, cells were infected with one multiplicity of infection (MOI) of MR766 or PE243 ZIKV strains for 1 h. The supernatant was removed and the cells washed thoroughly with PBS. A new culture medium was added and the cells cultured for 24 h. Positive controls were performed with addition of 100 μg mL-1 of chloroquine diphosphate to the cultures after ZIKV incubation and culture medium change. As such, cultures after the medium change were nominated as 0 h and all time-points afterward showed only the effects derived from the 1-h ZIKV incubation. The ZIKV infection efficiency was accessed by flow cytometry, quantitative reverse transcription polymerase chain reaction (RT-qPCR) and immunofluorescence.3030 Oliveira, M. B. S.; Valentim, I. B.; Rocha, T. S.; Santos, J. C.; Pires, K. S. N.; Tanabe, E. L. L.; Borbely, K. S. C.; Borbely, A. U.; Goulart, M. O. F.; Ind. Crops Prod. 2020, 152, 112503.
Flow cytometry analysis of ZIKV infection
To access the percentage of cells infected by ZIKV, cells were detached with 2.5% trypsin-EDTA, and fixation and permeabilization were performed using commercial flow cytometry kits (e-Bioscience, San Diego, CA, USA). A monoclonal primary mouse antibody anti-ZIKV NS1 (1:100, E107, MA5-24585, Invitrogen, Carlsbad, CA, USA) was incubated with Zenon Alexa 488-conjugated secondary anti-mouse antibody (1:250; Thermo Fisher Scientific Burlington, MA, USA) for 5 min to form an immunocomplex with further addition of Zenon Blocking Reagent for further 5 min. The immunocomplex was later incubated with cells for 1 h at 37 °C. The percentage of ZIKV infected cells was analyzed with FACS CantoTM® II flow cytometer (BD Biosciences, San Jose, CA, USA), using FlowJo software (BD Biosciences).
Quantitative reverse transcription polymerase chain reaction (RT-qPCR)
The ribonucleic acid (RNA) viral load from the cellular supernatants was extracted using PureLink™ Viral RNA/DNA Mini Kit (Invitrogen, Carlsbad, CA, USA), following the manufacturer’s instructions. The complementary DNA was synthesized and amplified using M-MLV reverse transcriptase (Invitrogen, Carlsbad, CA, USA). Next, ZIKV RNA copies were quantified using StepOnePlus™ Real-Time PCR System (Applied Biosystems, Life Technologies, Foster City, CA, USA). For each single-well amplification reaction, a threshold cycle (Ct) was evaluated in the exponential phase. The primers used were ZIKV 1086 and ZIKV 1162c.3131 Lanciotti, R. S.; Kosoy, O. L.; Laven, J. J.; Velez, J. O.; Lambert, A. J.; Johnson, A. J.; Stanfield, S. M.; Duffy, M. R.; Emerging Infect. Dis. 2008, 14, 1232.
Immunofluorescence for ZIKV NS1
The HTR-8/SVneo cells were fixed with 4% (v/v) paraformaldehyde in PBS and permeabilized with 0.1% Triton X-100 in PBS (v/v). Then, unspecific antigens blockade was performed with 0.05% fish-skin gelatin in PBS (m/v) (Merck/Sigma-Aldrich, Burlington, MA, USA) for 1 h, followed by monoclonal primary mouse antibody anti-ZIKV NS1 (1:100, E107, MA5-24585, Invitrogen, Carlsbad, CA, USA) incubation with Zenon Alexa 488 conjugated secondary anti-mouse antibody (1:250; Thermo Fisher Scientific, Waltham, MA, USA) for 5 min to form an immunocomplex, which was later incubated with Zenon Blocking Reagent (1:250; Thermo Fisher Scientific, Waltham, MA, USA) for a further 5 min at room temperature. The immunocomplex mixture was added to cells for 1 h at 37 °C. Nuclei were stained with 4’,6-diamidino-2-phenylindole (DAPI; 1:1000 in PBS; Merck/Sigma-Aldrich, Burlington, MA, USA), and mounting was performed with PBS/glycerol (1:9, v/v) under glass slides. The results were visualized with a fluorescence microscope (Nikon DS-Ri1, Minato, Japan) and images acquired using DP2-BSW software (Nikon).
Statistical analyses
The results for the antioxidant tests were expressed as mean ± standard deviation (SD), and statistical evaluation was determined by analysis of variance (ANOVA) followed by Tukey’s post-test. The results for the antiviral tests were expressed as mean ± standard error of the mean (SEM), and the statistical evaluation was determined by ANOVA with Geisser-Greenhouse correction followed by Tukey’s post-test, at the level of significance of 95%, using Graphpad Prism 8.3.0 software.3232 GraphPad Prism, 8.3.0 software; GraphPad Software, San Diego, CA, USA, 2016.
Results and Discussion
Characterization of the ethanol extract
Initially, the yield of PFSE was 7.9%, calculated from the initial mass of seeds submitted to extraction with ethanol. HPLC-MS/MS analysis of the ethanolic extract was conducted to characterize the major secondary metabolites. The compounds’ annotation was supported by the fragmentation profile,3333 Crotti, A. E. M.; Lopes, J. L. C.; Lopes, N. P.; J. Mass Spectrom. 2005, 40, 1030. and individual analysis of the gas phase decomposition reactions.3434 Demarque, D. P.; Crotti, A. E. M.; Vessecchi, R.; Lopes, J. L. C.; Lopes, N. P.; Nat. Prod. Rep. 2016, 33, 432. Finally, spectroscopic data and literature comparison were used to support the proposals (Table 1). The dereplication strategies allowed the annotation of 10 compounds in total, of which five were identified in negative ionization mode and five in positive ionization mode. The detailed mass spectrometric analyses of the compounds are summarized in the Supplementary Information (SI)
Supplementary Information
Supplementary data are available free of charge at http://jbcs.sbq.org.br as PDF file.
section (Figures S1-S12). The results obtained by LC-MS/MS in a negative ionization allowed us to annotate the signals at 18.5, 17.4, 21.0, 22.4, and 17.2 min, referring to [M - H]- ions of m/z 243, 405, 485, 469 and 449, respectively, and presented a fragmentation profile consistent with the compounds piceatannol (m/z 243), astringin (m/z 405), scirpusin B (m/z 485) and scirpusin A (m/z 469) (Figure S11), along with isookanin-7 O glucoside (m/z 449).3535 Moss, R.; Mao, Q.; Taylor, D.; Saucier, C.; Rapid Commun. Mass Spectrom. 2013, 27, 1815.
36 Yu, J.; Qi, J.; Zhang, L.; Yu, X.; Kong, Q.; Ren, X.; J. Chromatogr. B: Anal. Technol. Biomed. Life Sci. 2018, 1096, 88.-3737 Sano, S.; Sugiyama, K.; Ito, T.; Katano, Y.; Ishihata, A.; J. Agric. Food Chem. 2011, 59, 6209. In the positive ionization mode, it was possible to observe the presence of naringenin-7-O-glucoside (m/z 435), tyrosine (m/z 182), phenylalanine (m/z 166), and two derivatives of quadranguloside saponin (m/z 621 and m/z 593; Figure S12). The absence of signals of C-flavonoids observed confirmed a significant difference of the chemical profiles of leaves and seeds. High resolution analysis, listed in Table 1, confirmed all molecular formulas with less than 10 ppm error, corroborating the correct number of C, H and O atoms.
To reinforce, all mass spectrometric annotations are based on high resolution and fragmentation patterns. As already described in the literature, stilbenes are found in passion fruit seeds.55 Gadioli, I. L.; da Cunha, M. S. B.; de Carvalho, M. V. O.; Costa, A. M.; Pineli, L. L. O.; Crit. Rev. Food Sci. Nutr. 2018, 58, 785; Barbosa Santos, T.; de Araujo, F. P.; Neto, A. F.; de Freitas, S. T.; de Souza Araújo, J.; de Oliveira Vilar, S. B.; Brito Araújo, A. J.; Lima, M. S.; Int. J. Fruit Sci. 2021, 21, 255.,1010 Yamamoto, T.; Sato, A.; Takai, Y.; Yoshimori, A.; Umehara, M.; Ogino, Y.; Inada, M.; Shimada, N.; Nishida, A.; Ichida, R.; Takasawa, R.; Maruki-Uchida, H.; Mori, S.; Sai, M.; Morita, M.; Tanuma, S.-i; Biochem. Biophys. Rep. 2019, 20, 100684.,3737 Sano, S.; Sugiyama, K.; Ito, T.; Katano, Y.; Ishihata, A.; J. Agric. Food Chem. 2011, 59, 6209.
38 Krambeck, K.; Oliveira, A.; Santos, D.; Pintado, M. M.; Silva, J. B.; Lobo, J. M. S.; Amaral, M. H.; Pharmaceuticals 2020, 13, 73.-3939 Pan, Z. H.; Ning, D. S.; Fu, Y. X.; Li, D. P.; Zou, Z. Q.; Xie, Y. C.; Yu, L. L.; Li, L. C.; J. Agric. Food Chem. 2020, 68, 1555. Astringin is the glycosylated piceatannol molecule; the compounds scirpusin B and scirpusin A are dimers of piceatannol. Of these compounds, piceatannol is the most studied and has shown important biological activities, with antidiabetic,4040 Uchida-Maruki, H.; Inagaki, H.; Ito, R.; Kurita, I.; Sai, M.; Ito, T.; Biol. Pharm. Bull. 2015, 38, 629.,4141 Jiang, L.; Wang, Z.; Wang, X.; Wang, S.; Cao, J.; Liu, Y.; RSC Adv. 2020, 10, 4529. antioxidant,4242 les Parellada, F.; Deleruyelle, S.; Cassagnes, L. E.; Boutin, J. A.; Balogh, B.; Arbones-Mainar, J. M.; Biron, S.; Marceau, P.; Richard, D.; Nepveu, F.; Mauriège, P.; Carpéné, C.; Chem.-Biol. Interact. 2016, 258, 115.
43 Costa, F. P. D.; Puty, B.; Nogueira, L. S.; Mitre, G. P.; dos Santos, S. M.; Teixeira, B. J. B.; Kataoka, M. S. S.; Martins, M. D.; Barboza, C. A. G.; Monteiro, M. C.; Rogez, H.; de Oliveira, E. H. C.; Lima, R. R.; Antioxidants 2020, 9, 16.-4444 Hosoda, R.; Hamada, H.; Uesugi, D.; Iwahara, N.; Nojima, I.; Horio, Y.; Kuno, A.; J. Pharmacol. Exp. Ther. 2021, 376, 385. anticancer4545 Banik, K.; Ranaware, A. M.; Harsha, C.; Nitesh, T.; Girisa, S.; Deshpande, V.; Fan, L.; Nalawade, S. P.; Sethi, G.; Kunnumakkara, A. B.; Pharmacol. Res. 2020, 153, 104635.,4646 Sáez, V.; Pastene, E.; Vergara, C.; Mardones, C.; Hermosín-Gutiérrez, I.; Gómez-Alonso, S.; Gómez, M. V.; Theoduloz, C.; Riquelme, S.; von Baer, D.; Food Chem. 2018, 265, 101. and anti-inflammatory1010 Yamamoto, T.; Sato, A.; Takai, Y.; Yoshimori, A.; Umehara, M.; Ogino, Y.; Inada, M.; Shimada, N.; Nishida, A.; Ichida, R.; Takasawa, R.; Maruki-Uchida, H.; Mori, S.; Sai, M.; Morita, M.; Tanuma, S.-i; Biochem. Biophys. Rep. 2019, 20, 100684.,4747 Son, Y.; Chung, H. T.; Pae, H. O.; BioFactors 2014, 40, 138. potential.
Scirpusins A and B showed in vitro anti-HIV-14848 Yang, C. X.; Zhou, J. T.; Li, Y. Z.; Hu, C. Q.; Planta Med. 2005, 71, 569. (IIIB strain) activity. Sano et al.3737 Sano, S.; Sugiyama, K.; Ito, T.; Katano, Y.; Ishihata, A.; J. Agric. Food Chem. 2011, 59, 6209. isolated piceatannol and scirpusin B from passion fruit seeds and demonstrated their antioxidant and vasorelaxing potential,3737 Sano, S.; Sugiyama, K.; Ito, T.; Katano, Y.; Ishihata, A.; J. Agric. Food Chem. 2011, 59, 6209. with scirpusin B showing better effects than piceatannol. Scirpusin B also showed hypoglycemic activity through an amylase inhibitory activity.3939 Pan, Z. H.; Ning, D. S.; Fu, Y. X.; Li, D. P.; Zou, Z. Q.; Xie, Y. C.; Yu, L. L.; Li, L. C.; J. Agric. Food Chem. 2020, 68, 1555. Scirpusin A showed strong inhibition of the β-amyloid peptide aggregation process,4949 Rivière, C.; Papastamoulis, Y.; Fortin, P. Y.; Delchier, N.; Andriamanarivo, S.; Waffo-Teguo, P.; Kapche, G. D. W. F.; Amira-Guebalia, H.; Delaunay, J. C.; Mérillon, J. M.; Richard, T.; Monti, J. P.; Bioorg. Med. Chem. Lett. 2010, 20, 3441. and inhibitory activity of arginase in mammals.5050 Arraki, K.; Totoson, P.; Decendit, A.; Zedet, A.; Maroilley, J.; Badoc, A.; Demougeot, C.; Girard, C.; Molecules 2021, 26, 1694.
Isoflavonoids like naringenin can be found mainly in citrus fruits,5151 Hartogh, D. J. D.; Tsiani, E.; Biomolecules 2019, 9, 99. and soybeans cultivars.5252 Bueno, P. C. P.; Lopes, N. P.; ACS Omega 2020, 5, 1752. Narigenin has several biological properties, such as attenuation of oxidative stress, and regulation of Nrf2 and its target genes,5353 Ramprasath, T.; Senthamizharasi, M.; Vasudevan, V.; Sasikumar, S.; Yuvaraj, S.; Selvam, G. S.; J. Physiol. Biochem. 2014, 70, 407. and levels of reduced glutathione (GSH) in cells,5454 Hernández-Aquino, E.; Muriel, P.; World J. Gastroenterol. 2018, 24, 1679. acting in the prevention of non-alcoholic fatty liver disease,5555 Wang, Q.; Ou, Y.; Hu, G.; Wen, C.; Yue, S.; Chen, C.; Xu, L.; Xie, J.; Dai, H.; Xiao, H.; Zhang, Y.; Qi, R.; Br. J. Pharmacol. 2020, 177, 1806. attenuating renal interstitial fibrosis and the expression of inflammatory factors,5656 Wang, R.; Wu, G.; Dai, T.; Lang, Y.; Chi, Z.; Yang, S.; Dong, D.; Exp. Ther. Med. 2020, 21, 66. and improving steatohepatitis induced by type 2 diabetes mellitus,5757 Syed, A. A.; Reza, M. I.; Shafiq, M.; Kumariya, S.; Singh, P.; Husain, A.; Hanif, K.; Gayen, J. R.; Life Sci. 2020, 257, 118118. among others. Flavonoids such as isookanin, with a catechol moiety, have one important structural requirement to inhibit the neutrophil superoxide anion generation,5858 Kanashiro, A.; Kabeya, L. M.; Polizello, A. C. M.; Lopes, N. P.; Lopes, J. L. C.; Lucisano-Valim, Y. M.; Phytother. Res. 2004, 18, 61. and demonstrate anti-inflammatory,5959 Xin, Y.-J.; Choi, S.; Roh, K.-B.; Cho, E.; Ji, H.; Weon, J. B.; Park, D.; Whang, W. K.; Jung, E.; Molecules 2021, 26, 255. and antidiabetic6060 Ahmed, D.; Kumar, V.; Sharma, M.; Verma, A.; BMC Complementary Altern. Med. 2014, 14, 243. activities.
Saponins are used as vaccine adjuvants. Cibulski et al.6161 Cibulski, S.; Teixeira, T. F.; Varela, A. P. M.; de Lima, M. F.; Casanova, G.; Nascimento, Y. M.; Tavares, J. F.; da Silva, M. S.; Sesterheim, P.; Souza, D. O.; Roehe, P. M.; Silveira, F.; Vaccine 2021, 39, 571. used a saponin-rich fraction of the Quillaja brasiliensis species and a nanoadjuvant with this fraction in experimental vaccines against ZIKV and observed stimulation of the immune response.6161 Cibulski, S.; Teixeira, T. F.; Varela, A. P. M.; de Lima, M. F.; Casanova, G.; Nascimento, Y. M.; Tavares, J. F.; da Silva, M. S.; Sesterheim, P.; Souza, D. O.; Roehe, P. M.; Silveira, F.; Vaccine 2021, 39, 571. The presence of saponins in the Passiflora genus has been previously described.6262 Reginatto, F. H.; Gosmann, G.; Schripsema, J.; Schenkel, E. P.; Phytochem. Anal. 2004, 15, 195.,6363 Gosmann, G.; Provensi, G.; Comunello, L. N.; Rates, S. M. K.; Rev. Bras. Biociências 2011, 9, 88.
In this work, through the fragmentation profile of the saponin quadranguloside, we found two possible derivatives. The derivative I (m/z 621) refers to the quadranguloside with one less gentiobiose moiety, and linked to a glucose molecule. According to Reginatto et al.,6464 Reginatto, F. H.; Kauffmann, C.; Schripsema, J.; Guillaume, D.; Gosmann, G.; Schenkef, E. P.; J. Braz. Chem. Soc. 2001, 12, 32. the quadranguloside C34H56O8 is known as 9,19-cyclolanost-24-Z-en-3b,21,26-trihydroxy-3,26 di O-gentiobiose.6464 Reginatto, F. H.; Kauffmann, C.; Schripsema, J.; Guillaume, D.; Gosmann, G.; Schenkef, E. P.; J. Braz. Chem. Soc. 2001, 12, 32. This generates the derivative II (m/z 593), through the loss of one of the gentibiose groups and one glucose molecule (Figure S13, SI section Supplementary Information Supplementary data are available free of charge at http://jbcs.sbq.org.br as PDF file. ). In both cases we are able only to characterize the signals by mass spectrometry, but our data open the perspective for an isolation guide by MS to characterize these metabolites and possible new analogues, as described in several metabolomics protocols.1515 Pilon, A. C.; Selegato, D. M.; Fernandes, R. P.; Bueno, P. C. P.; Pinho, D. R.; Carnevale Neto, F.; Freire, R. T.; Castro-Gamboa, I.; Bolzani, V. S.; Lopes, N. P.; Quim. Nova 2020, 43, 329; Brunetti, A. E.; Carnevale Neto, F.; Vera, M. C.; Taboada, C.; Pavarini, D. P.; Bauermeister, A.; Lopes, N. P.; Chem. Soc. Rev. 2018, 47, 1574.,5252 Bueno, P. C. P.; Lopes, N. P.; ACS Omega 2020, 5, 1752.
In vitro radical scavenging assays
Oxidative stress is directly related to numerous diseases, including those caused by viral infections, promoting virus replication in infected cells, decreasing cell proliferation and inducing cell apoptosis.6565 Fedoreyev, S.; Krylova, N.; Mishchenko, N.; Vasileva, E.; Pislyagin, E.; Iunikhina, O.; Lavrov, V.; Svitich, O.; Ebralidze, L.; Leonova, G.; Mar. Drugs 2018, 16, 509. Almeida et al.6666 Almeida, L. T.; Ferraz, A. C.; Caetano, C. C. S.; Menegatto, M. B. S.; Andrade, A. C. S. P.; Lima, R. L. S.; Camini, F. C.; Pereira, S. H.; Pereira, K. Y. S.; Silva, B. M.; Perucci, L. O.; Talvani, A.; de Magalhães, J. C.; de Brito Magalhães, C. L.; Virus Res. 2020, 286, 198084. investigated the role of oxidative stress in ZIKV infection and observed in infected cells a significant increase in ROS production, in the formation of lipid peroxidation products, in carbonyl protein levels, in addition to a decrease in the activities of the redox enzymes superoxide dismutase and catalase. In this context, the antioxidant potential was investigated using the methods of DPPH•, FRAP and lipid peroxidation.
PFSE exhibited an IC50 (DPPH) value of 12.1 ± 1.6 µg mL-1 and 390 ± 6 mg Trolox eq per g dry extract in the FRAP analysis. Yepes et al.99 Yepes, A.; Ochoa-Bautista, D.; Murillo-Arango, W.; Quintero-Saumeth, J.; Bravo, K.; Osorio, E.; Arabian J. Chem. 2021, 14, 102905. studied the ethanolic extract of purple passion fruit seeds and found an IC50 (DPPH) value of 132.6 µg mL-1, about 10-fold higher than the present study. Rotta et al.1111 Rotta, E. M.; Giroux, H. J.; Lamothe, S.; Bélanger, D.; Sabik, H.; Visentainer, J. V.; Britten, M.; LWT- Food Sci. Technol. 2020, 123, 109088. obtained an IC50 (DPPH) of 19 ± 3 µg mL-1 for the Passiflora edulis seed extract, similar to the present study.
The lipid peroxidation inhibition assay was also performed to evaluate the antioxidant potential of the PFSE; the effects against lipid peroxidation at concentrations of 5, 25 and 50 μg mL-1 are shown in Figure 1. The experiments with the blank (ethanol) in the absence of antioxidants showed that the liposomal lipid peroxidation induced by AAPH occurs, causing the loss of fluorescence. The positive control, Trolox® (100 µg mL-1), inhibited lipid peroxidation and offered approximately 95% protection at the end of the evaluation. The PFSE (25 μg mL-1) showed a percentage inhibition of lipid peroxidation similar to that of Trolox®. Even at the lowest concentration tested (5 μg mL-1) showed protection within 10 min, similar to that found for the other concentrations and at the end of 30 min monitoring, about 70% inhibition. de Oliveira et al.6767 de Oliveira, A. C.; Valentim, I. B.; Silva, C. A.; Bechara, E. J. H.; de Barros, M. P.; Mano, C. M.; Goulart, M. O. F.; Food Chem. 2009, 115, 469. studied the methanolic extract of passion fruit residue and observed a protection against lipid peroxidation higher than 90%, similar to that found in this study.
Potential inhibitor of lipid peroxidation of passion fruit seed extract (PFSE) in different concentrations (5, 25, and 50 µg mL-1) during the 30 min time interval.
The PFSE showed significant protection against lipid peroxidation, further highlighting the promising potential of this extract in inhibiting or delaying oxidative damage.
Analyses of aqueous extracts in Vero E6 and HTR-8/SVneo cells and placental explant viability
The PFSE was first dissolved in an aqueous solution and analyzed in the Vero E6 cell line. As a result, no decrease whatsoever in cell viability was observed, and at the highest concentration used (100 μg mL-1) a solid increase in viability was seen, which might be related to a possible increase in proliferation or mitochondrial activity (Figure 2a). Then, we tested cell viability of placental human HTR-8/SVneo cells in the presence of PFSE, also with no reduction in cell viability at any concentration used (Figure 2b). We further analyzed the PFSE toxicity on human placental tissue explant culture, and no reduction on placenta viability was observed at all the various concentrations analyzed (Figure 2c), indicating that the extract is well tolerated by cell lines and human placental tissue explants.
Cellular viability in Vero E6 cells (a), HTR-8/SVneo cells (b) and placental tissue explants viability (c) under different concentrations of passion fruit seed extracts (PFSE). Cells and explants were treated with DMEM/F12 solution (control), with 0.01, 0.1, 1, 10, and 100 μg mL-1 PFSE. The bar graphs represent the mean values ± SEM; n = 3, *p < 0.05.
Viral load RT-qPCR analysis from HTR-8/SVneo cells treated with PFSE and infected with ZIKV
HTR-8/SVneo cells were plated at 1 × 106 cells per well and treated, as described above, with 1 h of ZIKV incubation, culture medium removal and PBS washing with the addition of fresh medium. The supernatants were collected and analyzed by RT-qPCR to evaluate the concentration of eventual new viral copies released by infected cells. After 24 h, cells infected with the MR766 strain showed an average viral load of 4.772 ± 1.148 × 104 PFU μL-1, and both treatments, with 1 h or 24 h of PFSE exposure, significantly reduced the viral load to 0.927 ± 0.047 × 104 PFU μL-1 and 0.649 ± 0.292 × 104 PFU μL-1, respectively (both with p < 0.01 in comparison to ZIKV MR766 group; Figure 3a). Moreover, cells infected with the PE243 strain showed an average of 5.956 ± 2.089 × 105 PFU μL-1, and a remarkable reduction of viral load when the PFSE was added as a treatment for 1 h and 24 h, which ablated to 0.127 ± 0.002 × 105 PFU μL-1 and 0.161 ± 0.062 × 105 PFU μL-1, respectively (p < 0.05 and p < 0.01 in comparison to ZIKV PE243 group; Figure 3b). As such, 1 h of treatment with PFSE was enough to reduce the viral load from both ZIKV strains consistently, and the effect was the same with 24 h of treatment.
RT-qPCR analyzes of ZIKV viral load after HTR-8/SVneo cells or placental explants infection. After ZIKV MR766 strain (a) or ZIKV PE243 (b) infection in HTR-8/SVneo cells, and ZIKV PE243 (c) infection in placental explants. Treatments were made with DMEM/F12 solution (control), and with 100 μg mL-1 of passion fruit seed extract (PFSE) 1 h and 24 h prior viral incubation, and with 50 μg mL-1 of chloroquine (CQ) after 1 h of viral incubation. After culture medium renewal, cells were left for 24 h, and their supernatants were analyzed to observe ZIKV viral load. The bar graphs represent the mean values ± SEM; n = 4 for explants and n = 5 for cells. *p < 0.05; **p < 0.01; ***p < 0.001.
Regarding the placental explants, they were infected with PE243 ZIKV strain only, once the MR766 strain already was shown to not infect them.3030 Oliveira, M. B. S.; Valentim, I. B.; Rocha, T. S.; Santos, J. C.; Pires, K. S. N.; Tanabe, E. L. L.; Borbely, K. S. C.; Borbely, A. U.; Goulart, M. O. F.; Ind. Crops Prod. 2020, 152, 112503. The infected explants had an average of 2.769 ± 0.896 × 105 PFU μL-1, and a remarkable reduction of viral load when PFSE was added as a treatment for 24 h, which reduced the viral load to 0.041 ± 0.009 × 105 PFU μL-1 (p < 0.01 in comparison to ZIKV PE243 group; Figure 3c).
Flow cytometry and immunofluorescence analysis on ZIKV NS1 protein expression in HTR-8/SVneo cells
Since the extract was well tolerated by trophoblast cells and placental tissue explants and reduced ZIKV viral load remarkably for both strains, we aimed to verify ZIKV NS1 protein expression by flow cytometry analysis in HTR-8/SVneo cells. As such, the MR766 strain infected an average of 69.7 ± 9.68% of cells in the control group (Figures 4a and 4d), but the treatment was unable to reduce the number of cells with ZIKV positivity (59.27 ± 14.05%). As such, it seems that cells are infected but viruses are not released into the culture media, since the viral load was reduced after the treatment, as previously shown here. The PE243 strain infected an average of 64.47 ± 9.38% in the control group (Figures 4b and 4d), whereas the treatment was able to reduce consistently the ZIKV positivity to 13.55 ± 6.97% (p = 0.024), indicating that the PFSE was able to reduce both viral load in the culture medium and cellular infectivity of trophoblast cells. Immunofluorescence confirmed the results obtained by flow cytometry, showing that NS1 ZIKV protein was not found in control cells (Figure 5a), and cells infected with PE243 strain and treated with PFSE showed reduced immunolocalization of NS1 proteins in comparison to the PE243 group (Figures 5b and 5c).
Flow cytometry analysis on passion fruit seed extract treatment on ZIKV placenta infection. HTR-8/SVneo cells were pre-treated with 100 μg mL-1 of the extract for 1 h and further infected with MR766 (a and d) or PE243 (b and d) ZIKV strains. Cellular gate for size and granularity of HTR-8/SVneo cells is depicted in (c). In (d), negative control (C-), in the first line MR766 and second-line PE243 strain. The treatment was able to reduce remarkably PE243 NS1 protein in trophoblast cells, which indicated reduced infection (b and d). Experiments were performed in n = 3. *p < 0.05.
Immunolocalization of ZIKV NS1 in HTR-8/SVneo cells. The ZIKV NS1 (green) was localized in control (a), cells infected with PE243 strain (b) and cells treated with PFSE for 24 h, then infected with ZIKV PE243 (c). Nuclei stained with DAP-I (blue). Cells infected with PE243 strain showed intense staining in the cytoplasm, whereas PFSE treated cells had lower amount and intensity in comparison. Images acquired with 100× magnification.
Since the WHO included ZIKV as a priority in the research and development plans for neglected diseases that represent potential global threats,2121 http://who.int/blueprint/priority-diseases/en/, accessed in December 2021.
http://who.int/blueprint/priority-diseas...
the world has been seeking new therapies and drugs that could be employed against ZIKV infection. In this context, the inhibition or prevention of ZIKV placental infection would also prevent harmful effects to the developing fetus. Nevertheless, existing drugs with antiviral effects against ZIKV are contraindicated in pregnancy, and only a few new compounds are in phase I or II clinical trials.6868 de Souza, A. A. A.; Torres, L. R.; Lima, L. R. P.; de Paula, V.; Barros, J. J.; Bonecini-Almeida, M. G.; Waghabi, M. C.; Gardel, M. A.; Meuser-Batista, M.; de Souza, E. M.; Braz. J. Infect. Dis. 2020, 24, 505. As such, natural products are thought to represent potential reservoirs of novel and safe antiviral drugs that could indeed advance the treatment of pregnant women.6969 Li, J. W.; Vederas, J. C.; Science 2009, 325, 161. Therefore, based on our results, PFSE seems to be a promising candidate to further studies on this behalf. PFSE clearly reduced the viral load in different models using tissue explants and cell cultures, as well as reducing NS1 expression in infected cells, which could indicate that PFSE somehow inhibits the viral entrance and should be further investigated to clarify the potential antiviral mechanism.
In addition to investigating the promise of PFSE, we used the antimalarial chloroquine diphosphate as a positive control of antiviral activity, as has been described by different sources.2626 Miller, R. K.; Genbacev, O.; Turner, M. A.; Aplin, J. D.; Caniggia, I.; Huppertz, B.; Placenta 2005, 26, 439.
27 Delvecchio, R.; Higa, L. M.; Pezzuto, P.; Valadão, A. L.; Garcez, P. P.; Monteiro, F. L.; Loiola, E. C.; Dias, A. A.; Silva, F. J. M.; Aliota, M. T.; Caine, E. A.; Osorio, J. E.; Bellio, M.; O’Connor, D. H.; Rehen, S.; de Aguiar, R. S.; Savarino, A.; Campanati, L.; Tanuri, A.; Viruses 2016, 8, 322.-2828 Li, C.; Zhu, X.; Ji, X.; Quanquin, N.; Deng, Y. Q.; Tian, M.; Aliyari, R.; Zuo, X.; Yuan, L.; Afridi, S. K.; Li, X. F.; Jung, J. U.; Nielsen-Saines, K.; Qin, F. X. F.; Qin, C. F.; Xu, Z.; Cheng, G.; EBioMedicine 2017, 24, 189.,7070 Kao, J.-C.; HuangFu, W.-C.; Tsai, T.-T.; Ho, M.-R.; Jhan, M.-K.; Shen, T.-J.; Tseng, P.-C.; Wang, Y.-T.; Lin, C.-F.; PLoS Neglected Trop. Dis. 2018, 12, e0006715.
Other active plants have been already described, such as extracts of Schinus terebinthifoliusRaddi, which showed similar effects on ZIKV entrance into placental cells,3030 Oliveira, M. B. S.; Valentim, I. B.; Rocha, T. S.; Santos, J. C.; Pires, K. S. N.; Tanabe, E. L. L.; Borbely, K. S. C.; Borbely, A. U.; Goulart, M. O. F.; Ind. Crops Prod. 2020, 152, 112503. Doratoxylon apetalum extract inhibited ZIKV infection in leukocytes,7171 Haddad, J. G.; Koishi, A. C.; Gaudry, A.; dos Santos, C. N. D.; Viranaicken, W.; Desprès, P.; El Kalamouni, C.; Int. J. Mol. Sci. 2019, 20, 2382. (-)-epigallocatechin gallate (EGCG) inhibited ZIKV entry in Vero E6 cells,7272 Carneiro, B. M.; Batista, M. N.; Braga, A. C. S.; Nogueira, M. L.; Rahal, P.; Virology 2016, 496, 215 and curcumin and suramin also inhibited ZIKV infection of different cells.7373 Tan, C. W.; Sam, I.-C.; Chong, W. L.; Lee, V. S.; Chan, Y. F.; Antiviral Res. 2017, 143, 186.,7474 Mounce, B. C.; Cesaro, T.; Carrau, L.; Vallet, T.; Vignuzzi, M.; Antiviral Res. 2017, 142, 148. Other compounds, such as GSK126, nanchangmycin, obatoclax, pentagalloylglucose, saliphenylhalamide (SaliPhe), and 25-hydroxycholesterol have also been described to inhibit ZIKV endocytosis or entry in different models.7575 da Silva, S.; Martins, D. O. S.; Jardim, A.; Viruses 2018, 10, 255. Additionally, of the compounds found in PFSE, it has already been shown that one of them, naringenin-7-O-glucoside, has anti-ZIKV activity in different cell lines and dendritic cells.7676 Cataneo, A. H. D.; Kuczera, D.; Koishi, A. C.; Zanluca, C.; Silveira, G. F.; de Arruda, T. B.; Suzukawa, A. A.; Bortot, L. O.; Dias-Baruffi, M.; Verri, W. A.; Robert, A. W.; Stimamiglio, M. A.; dos Santos, C. N. D.; Wowk, P. F.; Bordignon, J.; Sci. Rep. 2019, 9, 16348.
Conclusions
This work reported for the first time an extract of passion fruit seeds with antiviral potential against ZIKV, showing no toxicity in trophoblast cells and in explants of human placenta. The treatment consistently reduced both viral load in the culture medium and cellular NS1 expression of trophoblastic cells. The assembly of biologically active compounds in PFSE is relevant. These results show the promising potential of PFSE as an adjunct therapy in human health, especially maternal and child health, notably against ZIKV. Further studies are required, including in vivo tests to assess better the administration in pregnant women, to identify the constituent or constituents responsible for the antiviral activity and to define the mechanism of action to ensure safe and effective future clinical applications.
PFSE is a safe nutraceutical natural product. The use of natural products, in safe and effective doses, may show significant advantages over synthetic drugs: fewer side effects; lower price, making them accessible to patients from lower-income communities; and with additional advantage of being easily included in the diet, so avoiding the distress associated with drug administration.
The valorization of industrial by-products represents a fundamental strategy for a circular and sustainable bioeconomy, especially in the case of new natural therapeutic approaches.
Supplementary Information
Supplementary data are available free of charge at http://jbcs.sbq.org.br as PDF file.
Acknowledgments
The authors gratefully acknowledge the financial support of the Brazilian research funding agencies Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq) for financial support (435704/2018-4) and fellowships (NPL, JCCS and MOFG), Coordenação de Aperfeiçoamento de Pessoal de Nível Superior-Brazil (CAPES) - Finance Code 001, CAPES/RENORBIO/PROAP (23038.011373/2017-31), CAPES/PROCAD, INCT-Bioanalítica (process 465389/2014-7), and FAPEAL (PPSUS/Decit/MS/CNPq/SESAU-AL/FAPEAL No.06/2016:60030 000819/2016). The authors wish to thank Aldy dos Santos and Juliane Pereira da Silva for technical assistance to Dr Alessandra Borges for the donation of Vero E3 cells and C6/36 cells and Dr Ênio Bassi and the IMMUNOREG group for the help with viral growth and titration. We acknowledge Farmanguinhos (Fundação Oswaldo Cruz, Rio de Janeiro, Brazil) for providing chloroquine diphosphate.
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Publication Dates
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Publication in this collection
17 June 2022 -
Date of issue
2022
History
-
Received
08 Sept 2021 -
Published
05 Jan 2022