Diversity of the diterpenes in the leaves of <i>Xylopia laevigata</i> (Annonaceae) and their cytotoxicities

Costa, Emmanoel V.; Sampaio, Marília F. C.; Menezes, Leociley R. A.; Dutra, Lívia M.; Costa, Cinara O. S.; Pinheiro, Maria Lúcia B.; Silva, Felipe M. A. da; Soares, Milena B. P.; Bezerra, Daniel P.; Barison, Andersson; Koolen, Hector H. F.

doi:10.21577/0100-4042.20170504

Abstract

The phytochemical investigation of the hexane extract which was obtained from the leaves of Xylopia laevigata (Annonaceae) produced six terpenes. Among these, five diterpenes named abieta-7,13-dien-3-one, ent-7β-acetoxy-16β-hydroxy-kaurane, 4-epi-cupressic acid, powerol, and labdorffianic acid B, and one oxygenated sesquiterpene, spathulenol. This is the first time these isolated diterpenes from X. laevigata have been described. The different structures belong to the abietane, kaurane, and labdane diterpenoids, and are indicative of the chemical diversity found in X. laevigata. Moreover, the diterpene ent-7β-acetoxy-16β-hydroxy-kaurane is reported herein for the first time as a natural product, and 4-epi-cupressic acid, powerol, and labdorffianic acid B are reported for the first time in the Annonaceae family. The structures of the isolated compounds were established by extensive analyses using 1D and 2D NMR spectroscopy in combination with MS. The cytotoxic activities of compounds abieta-7,13-dien-3-one, spathulenol, 4-epi-cupressic acid, and powerol were evaluated against tumor and non-tumor cell lines, in which spathulenol was found to be the most active, mainly against K562 with an IC₅₀ value of 17.20 μmol L^-1.

Keywords:
Annonaceae, Xylopia laevigata; diterpenes; cytotoxic activity

INTRODUCTION

The genus Xylopia belongs to the Annonaceae family and comprises approximately 160 species of aromatic shrubs and trees, from which 40 can be found in South America, mainly in the Brazilian cerrado.¹1 Chatrou, L. W.; Pirie, M. D.; Erkens, R. H. J.; Couvreur, T. L. P.; Neubig, K. M.; Abbott, J. R.; Mols, J. B.; Mass, J. W.; Saunders, R. M. K.; Chase, M. W.; Bot. J. Linn. Soc. 2012, 169, 5; Maas, P. J. M.; Kamer, H. M.; Junikka, L.; Mello-Silva, R.; Rainer, H.; Rodriguésia 2001, 52, 61.^,²2 Moreira, I. C.; Roque, N. F.; Vilegas, W.; Zalewski, C. A.; Lago, J. H. G.; Funasaki, M.; Chem. Biodivers. 2013, 10, 1921. Several species are used as spices, and as natural medicines for the treatment of skin infections and fever, and also as antiemetic, digestive, and appetite enhancing agents.³3 Corrêa, M. P.; Dicionário das plantas úteis do Brasil e das exóticas cultivadas, IBDF: Rio de Janeiro, 1984.^,⁴4 Karioti, A.; Hadjipavlou-Litina, D.; Mensah, M. L. K.; Fleischer, T. C.; Skaltsa, H.; J. Agric. Food. Chem. 2004, 52, 8094. Previous phytochemical investigations of Xylopia spp. highlighted the presence of terpenoids,⁵5 Quintans, J. S. S.; Soares, B. M.; Ferraz, R. P. C.; Oliveira, A. C. A.; Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Prata, A. P. N.; Moraes, M. O.; Pessoa, C.; Antoniolli, A. R.; Costa, E. V.; Bezerra, D. P.; Planta Med. 2013, 79, 123; Queiroz, J. C.; Antoniolli, A. R.; Quintans-Júnior, L. J.; Brito, R. G.; Barreto, R. S. S.; Costa, E. V.; Silva, T. B.; Prata, A. P. N.; Lucca Jr., W.; Almeida, J. R. G. S.; Lima, J. T.; Quintans, J. S. S.; Sci. World J. 2014, 2014, ID 816450.^,⁶6 Silva, D. M.; Costa, E. V.; Nogueira, P. C. L.; Moraes, V. R. S.; Cavalcanti, S. C. H.; Salvador, M. J.; Ribeiro, L. H. G.; Gadelha, F. R.; Barison, A.; Ferreira, A. G.; Quim. Nova 2012, 35, 1570. flavonoids,⁵5 Quintans, J. S. S.; Soares, B. M.; Ferraz, R. P. C.; Oliveira, A. C. A.; Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Prata, A. P. N.; Moraes, M. O.; Pessoa, C.; Antoniolli, A. R.; Costa, E. V.; Bezerra, D. P.; Planta Med. 2013, 79, 123; Queiroz, J. C.; Antoniolli, A. R.; Quintans-Júnior, L. J.; Brito, R. G.; Barreto, R. S. S.; Costa, E. V.; Silva, T. B.; Prata, A. P. N.; Lucca Jr., W.; Almeida, J. R. G. S.; Lima, J. T.; Quintans, J. S. S.; Sci. World J. 2014, 2014, ID 816450.^,⁷7 Maia, J. G. S.; Andrade, E. H. A.; Da Silva, A. C. M.; Oliveira, J.; Carreira, L. M. M.; Araújo, J. S.; Flavour Fragance J. 2005, 20, 474; Moreira, I. C.; Lago, J. H. G.; Young, M. C. M.; Roque, N. F.; J. Braz. Chem. Soc. 2003, 14, 828. and alkaloids.⁸8 Da Silva, M. S.; Tavares, J. F.; Queiroga, K. F.; Agra, M. F.; Barbosa-Filho, J. M.; Almeida, J. R. G. S.; Da Silva, S. A. S.; Quim. Nova 2009, 32, 1566; Puvanendran, S.; Wickramasinghe, A.; Karunaratne, D. N.; Carr, G.; Wijesundara, D. S. A.; Andersen, R.; Karunaratne, V.; Pharm. Biol. 2008, 46, 352. Some of the isolated compounds from this genus exhibit pharmacological activities, such as antifungal,⁶6 Silva, D. M.; Costa, E. V.; Nogueira, P. C. L.; Moraes, V. R. S.; Cavalcanti, S. C. H.; Salvador, M. J.; Ribeiro, L. H. G.; Gadelha, F. R.; Barison, A.; Ferreira, A. G.; Quim. Nova 2012, 35, 1570.^,⁷7 Maia, J. G. S.; Andrade, E. H. A.; Da Silva, A. C. M.; Oliveira, J.; Carreira, L. M. M.; Araújo, J. S.; Flavour Fragance J. 2005, 20, 474; Moreira, I. C.; Lago, J. H. G.; Young, M. C. M.; Roque, N. F.; J. Braz. Chem. Soc. 2003, 14, 828. antioxidant,³3 Corrêa, M. P.; Dicionário das plantas úteis do Brasil e das exóticas cultivadas, IBDF: Rio de Janeiro, 1984.^,⁸8 Da Silva, M. S.; Tavares, J. F.; Queiroga, K. F.; Agra, M. F.; Barbosa-Filho, J. M.; Almeida, J. R. G. S.; Da Silva, S. A. S.; Quim. Nova 2009, 32, 1566; Puvanendran, S.; Wickramasinghe, A.; Karunaratne, D. N.; Carr, G.; Wijesundara, D. S. A.; Andersen, R.; Karunaratne, V.; Pharm. Biol. 2008, 46, 352. antileishmanial,⁹9 López, R.; Cuca, L. E.; Delgado G.; Parasite Immunol. 2009, 31, 623. cytotoxic,⁵5 Quintans, J. S. S.; Soares, B. M.; Ferraz, R. P. C.; Oliveira, A. C. A.; Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Prata, A. P. N.; Moraes, M. O.; Pessoa, C.; Antoniolli, A. R.; Costa, E. V.; Bezerra, D. P.; Planta Med. 2013, 79, 123; Queiroz, J. C.; Antoniolli, A. R.; Quintans-Júnior, L. J.; Brito, R. G.; Barreto, R. S. S.; Costa, E. V.; Silva, T. B.; Prata, A. P. N.; Lucca Jr., W.; Almeida, J. R. G. S.; Lima, J. T.; Quintans, J. S. S.; Sci. World J. 2014, 2014, ID 816450.^,¹⁰10 Castelo-Branco, M. V. S.; Tavares, J. F.; Silva, M. S.; Barbosa Filho, J. M.; Anazetti, M. C.; Frungillo, L.; Haun, M.; Diniz, M. F. F. M.; Melo, P. S.; Rev. Bras. Farmacogn. 2011, 21, 1035. anti-inflammatory,⁵5 Quintans, J. S. S.; Soares, B. M.; Ferraz, R. P. C.; Oliveira, A. C. A.; Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Prata, A. P. N.; Moraes, M. O.; Pessoa, C.; Antoniolli, A. R.; Costa, E. V.; Bezerra, D. P.; Planta Med. 2013, 79, 123; Queiroz, J. C.; Antoniolli, A. R.; Quintans-Júnior, L. J.; Brito, R. G.; Barreto, R. S. S.; Costa, E. V.; Silva, T. B.; Prata, A. P. N.; Lucca Jr., W.; Almeida, J. R. G. S.; Lima, J. T.; Quintans, J. S. S.; Sci. World J. 2014, 2014, ID 816450.^,¹¹11 Nishiyama, Y.; Moriyasu, M.; Ichimaru, M.; Iwasa, K.; Kato, A.; Mathenge, S. G.; Mutiso, P. B. C.; Juma, F. D.; J. Nat. Med. 2010, 64, 9. antinociceptive,⁵5 Quintans, J. S. S.; Soares, B. M.; Ferraz, R. P. C.; Oliveira, A. C. A.; Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Prata, A. P. N.; Moraes, M. O.; Pessoa, C.; Antoniolli, A. R.; Costa, E. V.; Bezerra, D. P.; Planta Med. 2013, 79, 123; Queiroz, J. C.; Antoniolli, A. R.; Quintans-Júnior, L. J.; Brito, R. G.; Barreto, R. S. S.; Costa, E. V.; Silva, T. B.; Prata, A. P. N.; Lucca Jr., W.; Almeida, J. R. G. S.; Lima, J. T.; Quintans, J. S. S.; Sci. World J. 2014, 2014, ID 816450.^,¹¹11 Nishiyama, Y.; Moriyasu, M.; Ichimaru, M.; Iwasa, K.; Kato, A.; Mathenge, S. G.; Mutiso, P. B. C.; Juma, F. D.; J. Nat. Med. 2010, 64, 9. acaricidal,¹²12 Pontes, W. J. T.; Oliveira, J. C. S.; Câmara, C. A. G.; Gondim Jr., M. G. C.; Oliveira, J. V.; Schwartz, M. O. E.; Quim. Nova 2007, 30, 838. and insecticidal activities.⁶6 Silva, D. M.; Costa, E. V.; Nogueira, P. C. L.; Moraes, V. R. S.; Cavalcanti, S. C. H.; Salvador, M. J.; Ribeiro, L. H. G.; Gadelha, F. R.; Barison, A.; Ferreira, A. G.; Quim. Nova 2012, 35, 1570.^,¹³13 Nguemtchouin, M. M. G.; Ngassoum, M. B.; Ngamo, L. S. T.; Gaudu, X.; Cretin, C.; Crop Prot. 2010, 29, 985.

The relevant literature indicates 160 known species of this genus,¹⁴14 Barbosa, L. T. C.; Vega, M. R. G.; Rev. Virtual Quim. 2017, 9, 1712. and, approximately 20% (~30 species) have had previous chemical/pharmacological studies carried out, which reinforces the importance of new studies regarding the species of Xylopia. In this sense, Xylopia laevigata (Mart.) R.E. Fries is a small tree which is endemic to Brazil, popularly known as ‘meiú’ and ‘pindaíba’, and is found in the Northeastern and Southeastern regions.¹1 Chatrou, L. W.; Pirie, M. D.; Erkens, R. H. J.; Couvreur, T. L. P.; Neubig, K. M.; Abbott, J. R.; Mols, J. B.; Mass, J. W.; Saunders, R. M. K.; Chase, M. W.; Bot. J. Linn. Soc. 2012, 169, 5; Maas, P. J. M.; Kamer, H. M.; Junikka, L.; Mello-Silva, R.; Rainer, H.; Rodriguésia 2001, 52, 61.^,¹⁵15 Pontes, A. F.; Barbosa, M. R. V.; Maas, P. J. M.; Acta Bot. Bras. 2004, 18, 281. In the state of Sergipe, it is found in the last remaining fragments of the Atlantic forest near the coast.¹⁵15 Pontes, A. F.; Barbosa, M. R. V.; Maas, P. J. M.; Acta Bot. Bras. 2004, 18, 281. In local folk medicine, leaves and flowers are used in the treatment of painful disorders, inflammatory conditions and, in some cases, heart disease.⁴4 Karioti, A.; Hadjipavlou-Litina, D.; Mensah, M. L. K.; Fleischer, T. C.; Skaltsa, H.; J. Agric. Food. Chem. 2004, 52, 8094.

The essential oils of the leaves of X. laevigata are composed mainly of bicyclogermacrene, α-cadinene, (E)-caryophyllene, δ-copaene, germacrene D, and γ-muurolene.⁵5 Quintans, J. S. S.; Soares, B. M.; Ferraz, R. P. C.; Oliveira, A. C. A.; Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Prata, A. P. N.; Moraes, M. O.; Pessoa, C.; Antoniolli, A. R.; Costa, E. V.; Bezerra, D. P.; Planta Med. 2013, 79, 123; Queiroz, J. C.; Antoniolli, A. R.; Quintans-Júnior, L. J.; Brito, R. G.; Barreto, R. S. S.; Costa, E. V.; Silva, T. B.; Prata, A. P. N.; Lucca Jr., W.; Almeida, J. R. G. S.; Lima, J. T.; Quintans, J. S. S.; Sci. World J. 2014, 2014, ID 816450.^,¹⁶16 Costa, E. V.; Silva, T. B.; Menezes, L. R. A.; Ribeiro, L. H. G.; Gadelha, F. R.; Carvalho, J. E.; Souza, L. M. B.; Silva, M. A. N.; Siqueira, C. A. T.; Salvador, M. J.; J. Essent. Oil Res. 2013, 25, 179.

17 Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Meira, C. S.; Guimarães, E. T.; Soares, M. B. P.; Prata, A. P. N.; Nogueira, P. C. L.; Costa, E. V.; Nat. Prod. Commun. 2013, 8, 403.^-¹⁸18 Nascimento, A. M. D.; Maia, T. D. S.; Soares, T. E. S.; Menezes, L. R. A.; Scher, R.; Costa, E. V.; Cavalcanti, S. C. H.; La Corte, R.; Neotrop. Entomol. 2017, 46, 223. On the other hand, the essential oil composition of the fresh fruits included α-pinene, β-pinene and limonene as major compounds.¹⁹19 Costa, E. V.; da Silva, T. B.; Costa, C. O.; Soares, M. B.; Bezerra, D. P.; Nat. Prod. Commun. 2016, 11, 417. Besides, the existing chemical knowledge, biological activities have been recorded for this essential oil; these being antioxidant,⁴4 Karioti, A.; Hadjipavlou-Litina, D.; Mensah, M. L. K.; Fleischer, T. C.; Skaltsa, H.; J. Agric. Food. Chem. 2004, 52, 8094. antibacterial,¹⁶16 Costa, E. V.; Silva, T. B.; Menezes, L. R. A.; Ribeiro, L. H. G.; Gadelha, F. R.; Carvalho, J. E.; Souza, L. M. B.; Silva, M. A. N.; Siqueira, C. A. T.; Salvador, M. J.; J. Essent. Oil Res. 2013, 25, 179. antifungal,¹⁶16 Costa, E. V.; Silva, T. B.; Menezes, L. R. A.; Ribeiro, L. H. G.; Gadelha, F. R.; Carvalho, J. E.; Souza, L. M. B.; Silva, M. A. N.; Siqueira, C. A. T.; Salvador, M. J.; J. Essent. Oil Res. 2013, 25, 179. antinociceptive,¹⁶16 Costa, E. V.; Silva, T. B.; Menezes, L. R. A.; Ribeiro, L. H. G.; Gadelha, F. R.; Carvalho, J. E.; Souza, L. M. B.; Silva, M. A. N.; Siqueira, C. A. T.; Salvador, M. J.; J. Essent. Oil Res. 2013, 25, 179. anti-inflammatory,¹⁶16 Costa, E. V.; Silva, T. B.; Menezes, L. R. A.; Ribeiro, L. H. G.; Gadelha, F. R.; Carvalho, J. E.; Souza, L. M. B.; Silva, M. A. N.; Siqueira, C. A. T.; Salvador, M. J.; J. Essent. Oil Res. 2013, 25, 179. cytotoxic,⁴4 Karioti, A.; Hadjipavlou-Litina, D.; Mensah, M. L. K.; Fleischer, T. C.; Skaltsa, H.; J. Agric. Food. Chem. 2004, 52, 8094.^,²⁰20 Pereira, T. S.; Esquissato, G. N. E.; Costa, E.V.; Nogueira, P. C. L.; Castro-Prado, M. A. A.; Nat. Prod. Res. 2019, doi:10.1080/14786419.2019.1624956.
https://doi.org/10.1080/14786419.2019.16... larvicidal,¹⁶16 Costa, E. V.; Silva, T. B.; Menezes, L. R. A.; Ribeiro, L. H. G.; Gadelha, F. R.; Carvalho, J. E.; Souza, L. M. B.; Silva, M. A. N.; Siqueira, C. A. T.; Salvador, M. J.; J. Essent. Oil Res. 2013, 25, 179. trypanocidal,¹⁷17 Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Meira, C. S.; Guimarães, E. T.; Soares, M. B. P.; Prata, A. P. N.; Nogueira, P. C. L.; Costa, E. V.; Nat. Prod. Commun. 2013, 8, 403. and mutagenic²⁰20 Pereira, T. S.; Esquissato, G. N. E.; Costa, E.V.; Nogueira, P. C. L.; Castro-Prado, M. A. A.; Nat. Prod. Res. 2019, doi:10.1080/14786419.2019.1624956.
https://doi.org/10.1080/14786419.2019.16... activities.

Furthermore, previous investigations regarding this species have described the identification of ent-kaurane diterpenes,⁶6 Silva, D. M.; Costa, E. V.; Nogueira, P. C. L.; Moraes, V. R. S.; Cavalcanti, S. C. H.; Salvador, M. J.; Ribeiro, L. H. G.; Gadelha, F. R.; Barison, A.; Ferreira, A. G.; Quim. Nova 2012, 35, 1570. such as ent-kaur-16-en-19-oic acid, 4-epi-kaurenic acid, ent-16β-hydroxy-17-acetoxy-kauran-19-al, ent-3β-hydroxykaur-16-en-19-oic acid, and ent-16β,17-dihydroxy- kauran-19-oic acid, as well as spathulenol and a mixture of β-sitosterol, stigmasterol, and campesterol.⁶6 Silva, D. M.; Costa, E. V.; Nogueira, P. C. L.; Moraes, V. R. S.; Cavalcanti, S. C. H.; Salvador, M. J.; Ribeiro, L. H. G.; Gadelha, F. R.; Barison, A.; Ferreira, A. G.; Quim. Nova 2012, 35, 1570. Among them, ent-3β-hydroxykaur-16-en-19-oic acid demonstrated potent larvicidal activity against Aedes aegypti larvae and antifungal activity against Candida glabrata and Candida dubliniensis.⁶6 Silva, D. M.; Costa, E. V.; Nogueira, P. C. L.; Moraes, V. R. S.; Cavalcanti, S. C. H.; Salvador, M. J.; Ribeiro, L. H. G.; Gadelha, F. R.; Barison, A.; Ferreira, A. G.; Quim. Nova 2012, 35, 1570. Moreover, alkaloids have been identified from leaf and stem extracts of this plant, and were mainly aporphines, oxoaporphines, tetrahydroprotoberberines, and benzylisoquinolines.²¹21 Costa, E. V.; Dutra, L. M.; Nepel, A.; Barison, A.; Biochem. Syst. Ecol. 2013, 51, 331.^,²²22 Menezes, L. R. A.; Costa, C. O. D.; Rodrigues, A. C. B. C.; Santo, F. R. E.; Nepel, A.; Dutra, L. M.; Silva, F. M. A.; Soares, M. B. P.; Barison, A.; Costa, E. V.; Bezerra, D. P.; Molecules 2016, 21, 890. Among them, lanuginosine, (+)-xylopine, and (+)-norglaucine displayed high cytotoxic activities.²²22 Menezes, L. R. A.; Costa, C. O. D.; Rodrigues, A. C. B. C.; Santo, F. R. E.; Nepel, A.; Dutra, L. M.; Silva, F. M. A.; Soares, M. B. P.; Barison, A.; Costa, E. V.; Bezerra, D. P.; Molecules 2016, 21, 890.^,²³23 Santos, L. S.; Silva, V. R. S.; Menezes, L. R. A. M.; Soares, M. B. P. S.; Costa, E. V.; Bezerra, D. P.; Oxid. Med. Cell. Longevity 2017, 2017, ID 7126872, doi: 10.1155/2017/7126872.
https://doi.org/10.1155/2017/7126872....

In our continuous search for new bioactive natural products from Annonaceae that possess cytotoxic potential, this study aimed to investigate the phytochemical and pharmacological properties of the leaves of X. laevigata. In this report six compounds were isolated and identified. These were five diterpenes and one sesquiterpene, all from the leaf hexane extract of X. laevigata. In addition, the cytotoxicity of the isolated compounds was assessed against B16-F10, HepG2, K562, and HL-60 tumor cell lines by the Alamar blue assay.

EXPERIMENTAL

General experimental procedures

Optical rotations in CHCl₃ were recorded with a Jasco P-2000 polarimeter at 589 nm. GC−MS analyses were performed with a Shimadzu QP5050A GC−MS system fitted with a J & W Scientific DB-5MS (5%-phenyl-95%-methylpolysiloxane) fused capillary column (30 m × 0.25 mm × 0.25 μm of film thickness). MS analyses from the GC−MS were recorded at 70 eV with a scan interval of 0.5 s and the fragments were detected in the m/z 40-500 Da range. Low-Resolution Mass Spectra (LRMS) analyses were performed on an Waters TQD mass spectrometer equipped with an ESI source which was operating in the negative ion mode. High-Resolution Electrospray Ionization Mass Spectrometry (HRESIMS) were performed using a Bruker UltrOTOF-Q mass spectrometer. 1D and 2D NMR data were acquired at 303 K in CDCl₃ on a Bruker Avance III 600 NMR spectrometer, operating at 14.1 Tesla, and ¹H and ¹³C at 600.13 and 150.61 MHz were observed, respectively. The spectrometer was equipped with a 5 mm, inverse detection, four channel (¹H, ¹³C, ¹⁵N, and ³¹P) probe with z-gradient. One-bond and long-range ¹H-¹³C correlations from HSQC and HMBC NMR experiments were optimized for average coupling constants ¹J_(H,C) and ^LRJ_(H,C) of 140 and 8 Hz, respectively. ¹H and ¹³C NMR chemical shifts were given in ppm related to the TMS signal at 0.00 ppm as the internal reference, and the coupling constants (J) expressed in Hz. Silica gel 60 (70-230 mesh) was used for column chromatography, while silica gel 60 F₂₅₄ was used for analytical (0.25 mm), and preparative (1.00 mm) TLC. Compounds were visualized by exposure to UV_254/365 light, spraying of p-anisaldehyde reagent, and followed by heating on a hot plate.

Botanical material

Leaves of X. laevigata (SISGEN Register ACAAA36) were collected in Serra de Itabaiana (coordinates: 10º 44’ 53’’ S, 37º 20’ 21’’ W), Itabaiana, Sergipe state, Brazil, in March, 2010. The identification was confirmed by Dr. A. P. do N. Prata from the Departamento de Biologia from Universidade Federal de Sergipe. A specimen voucher (#15440) was deposited in the herbarium of the institution. The Chico Mendes Institute for Biodiversity Conservation, which belongs to the Brazilian Ministry of the Environment, provided an authorization for the sample collection (#25637-1). This study was also performed according to the special authorization given for access to genetic resources in Brazil #010240/2013-6, which was issued by CNPq/MCTI.

Extraction and isolation

Leaves of X. laevigata were dried in an air circulating oven at approximately 40 ºC for 72 h, and subsequently pulverized in a four-knife mill grinder (Marconi) to obtain the powdered material (750.0 g). Then, an exhaustive maceration with hexane (5 × 3L, 25 ºC) followed by MeOH (5 × 3L, 25 ºC). The extractive solutions obtained were concentrated in a rotary evaporator (Fisatom) at reduced pressure (40-50 ºC) in order to yield the hexane (54.3 g) and MeOH (191.1 g) extracts. The hexane extract presented a crystalline appearance after being dried. Subsequently, part (5.0 g) of the hexane extract was subjected to silica gel column chromatography (CC) which was eluted with gradients constituted of hexane, CH₂Cl₂, EtOAc, and MeOH mixtures in ascending order of polarity, which yielded 230 fractions. After TLC evaluation using a mixture of hexane-EtOAc in the proportions of 95:05, 90:10, 80:20, and 70:30 as the eluent system, the similar samples were pooled to give 20 groups (G1 to G20).

Group G7 (319.0 mg) from CC eluted with hexane-CH₂Cl₂ (10:90 v/v) and CH₂Cl₂ (100%) was submitted to a new silica gel CC eluted with hexane-EtOAc (100:0 to 50:50, v/v) and yielded 17 subfractions pooled into 8 subgroups (G7.1 to G7.8). Subgroup G7.2 (87.6 mg) from CC eluted with hexane-EtOAc (97:03, v/v) was submitted to a preparative TLC eluted with hexane-EtOAc (95:05, v/v, three elutions) and yielded 1 (45.1 mg).

Group G9 (562.0 mg) from CC eluted with CH₂Cl₂-EtOAc (95:05 and 90:10, v/v, respectively) was subjected to a silica gel CC eluted with hexane-EtOAc (100:0 to 30:70, v/v) and EtOAc-MeOH (100:0 to 20:80, v/v) and yielded 28 subfractions (25 mL each) that were subsequently pooled into 14 groups (G9.1 to G9.14), according to TLC analysis. G9.6 (37.4 mg) from CC eluted with hexane-EtOAc (95:05, v/v) was submitted to a preparative TLC eluted with hexane-EtOAc (90:10, v/v, four elutions) and yielded 2 (16.1 mg).

Group G12 (700.0 mg) from CC eluted with CH₂Cl₂-EtOAc (90:10, v/v) was submitted to another new silica gel CC eluted with hexane-EtOAc (100:0 to 50:50, v/v) followed by EtOAc-MeOH (100:0 to 20:80, v/v) and yielded 44 subfractions (25 mL each) that were pooled into 11 subgroups (G12.1 to G12.11) according to TLC analysis. Subgroup G12.7 (60.0 mg) from CC eluted with hexane-EtOAc 70:30 v/v was submitted to a preparative TLC eluted with hexane-EtOAc (80:20, v/v, four elutions) and yielded 3 (4.4 mg).

Group G14 (282.0 mg) from CC eluted with CH₂Cl₂-EtOAc (90:10; 80:20 and 70:30, v/v, respectively) was submitted to silica gel CC eluted with hexane-EtOAc (100:0 to 50:50, v/v) and EtOAc-MeOH (100:0 to 20:80, v/v) affording 34 subfractions (25 mL each), which were pooled into 10 subgroups (G14.1 to G14.10). Subgroup G14.7 (31.6 mg) from CC eluted with hexane-EtOAc (80:20, v/v) was submitted to a preparative TLC eluted with hexane-EtOAc (80:20, v/v, two elutions) and yielded 4 (11.4 mg).

Group G15 (299.0 mg), from CC eluted with CH₂Cl₂-EtOAc (50:50 and 30:70, v/v, respectively, and EtOAc 100%) was submitted to silica gel CC eluted with hexane-EtOAc (100:0 to 50:50, v/v), followed by EtOAc-MeOH (100:0 to 20:80, v/v) and yielded 39 subfractions (25 mL each) that were subsequently pooled into 8 groups (G15.1 to G15.8). Subgroup G15.4 (108.9 mg) from CC eluted with hexane-EtOAc (50:50 and 40:60, v/v, respectively) was obtained as crystalline white solid that showed high purity by GC−MS analysis and yielded 5 (108.9 mg).

Group G19 (70.0 mg) from CC eluted with EtOAc-MeOH (70:30 and 50:50, v/v, respectively) was submitted to a preparative TLC eluted with hexane-EtOAc (70:30, v/v, four elutions), and yielded 6 (5.3 mg).

Abieta-7,13-dien-3-one (1): Yellow oil (CHCl₃); [α]_D²⁵ + 30.81º (c 1.0, CHCl₃); ¹H and ¹³C NMR data see Table 2; EI-MS m/z 286 [M]^+•.

Thumbnail

Table 1
NMR data for ent-7β-acetoxy-16β-hydroxy-kaurane (3) and powerol (5) (CDCl₃, 600 MHz)

Thumbnail

Table 2
NMR data for abieta-7,13-dien-3-one (1), 4-epi-cupressic acid (4) and labdorffianic acid B (6) (CDCl₃, 600 MHz)
Spathulenol (2): Colorless oil (CHCl₃); [α]_D²⁵ +4.20º (c 1.2, CHCl₃); The ¹H and ¹³C NMR data were in agreement with those from the literature;²⁴24 Ragasa, C.Y.; Ganzon, J.; Hofileña, J.; Tamboong, B.; Rideout, J. A.; Chem. Pharm. Bull. 2003, 51, 1208. EI-MS m/z 220 [M]^+•.
ent-7β-Acetoxy-16β-hydroxy-kaurane (3): Amorphous white solid (CHCl₃); [α]_D²⁵−1.00º (c 0.4, CHCl₃); ¹H and ¹³C NMR data see Table 1; HR-ESIMS 371.2558 [M+Na]⁺ (C₂₂H₃₆O₃ + Na; calc. 371.2562); EI-MS m/z 270 [M−H₂O−C₂H₃O₂]^+•.
4-epi-Cupressic acid [13-Hydroxy-ent-labda-8,14-dien-18-oic acid] (4): Crystalline white solid (CHCl₃); [α]_D²⁵−57.12º (c 0.06, CHCl₃); ¹H and ¹³C NMR data see Table 2; HR-ESIMS 319.2262 [M−H]⁻ (C₂₀H₃₂O₃ − H; calc. 319.2273).
Powerol [(−)Kaurane-7β,16α-diol] (5): Crystalline white solid (CH₂Cl₂); [α]_D²⁵−2.70º (c 0.5, CHCl₃); ¹H and ¹³C NMR data see Table 1; HR-ESIMS 305.2129 [M−H]⁻(C₂₀H₃₄O₂ − H; calc. 305.2480); HR-ESIMS 329.2453 [M+Na]⁺ (C₂₀H₃₄O₂ + Na; calc. 329.2456); EI-MS m/z 306 [M]^+•.
Labdorffianic acid B [8,20-Epoxy-13-hydroxy-ent-labda-14-en-18-oic acid] (6): Colorless oil (CHCl₃); [α]_D²⁵ −36.1º (c 0.2, CHCl₃); ¹H and ¹³C NMR data see Table 2; LR-ESIMS [M−H]⁻ m/z 335.

Cytotoxicity assay

Tumor cell lines: B16-F10 (mouse melanoma), HepG2 (human hepatocellular carcinoma), K562 (human chronic myelocytic leukemia) and HL-60 (human promyelocytic leukemia) were kindly provided by the A.C. Camargo Hospital, São Paulo, Brazil. Cells were maintained in Roswell Park Memorial Institute-1640 (RPMI-1640) medium with 10% fetal bovine serum, 2 mmol L^-1 glutamine, and 50 μg mL^-1 gentamycin. Adherent cells were collected by treatment with a 0.25% trypsin-EDTA solution. All cell lines were cultured in cell culture flasks at 37 ºC in 5% CO₂ and sub-cultured every 3-4 days to maintain exponential growth. All experiments were performed with cells in the exponential growth phase. All cell lines were evaluated for mycoplasma using on a Sigma-Aldrich Mycoplasma stain kit, and all cells were free from contamination. Heparinized blood (from 20-35-year-old, healthy, non-smokers who had not taken any drugs for at least 15 days prior to sampling) was collected, and peripheral blood mononuclear cells (PBMCs) were isolated using a standard protocol which used a Ficoll density gradient in a GE Ficoll-Paque Plus. PBMCs were washed and re-suspended at a concentration of 0.3 x 10⁶ cells mL^-1 in RPMI-1640 medium with 20% fetal bovine serum, 2 mmol glutamine, and 50 μg mL^-1 gentamycin at 37 ºC with 5% CO₂. Concanavalin A (ConA) was used as a mitogen to trigger cell division in T-lymphocytes. ConA (10 μg mL^-1) was added at the beginning of culture, and cells were treated with the compounds after 24 h. Over 90% of the cells were viable at the beginning of the culture, according to the Trypan blue exclusion assay. Cell growth was quantified using the Alamar blue assay. Cells were seeded in 96-well plates for all experiments (0.7 x 10⁵ cells mL^-1 for adherent cells or 0.3 x 10⁶ cells mL^-1 for suspended cells in 100 μL of medium).²⁵25 Ahmed, S. A.; Gogal, R. M.; Walsh, J. E.; J. Immunol. Methods 1994, 170, 211. After 24 h of incubation, the compounds (dissolved in DMSO at a concentration of 0.19 – 25 μg mL^-1) were added and incubated for 72 h. Doxorubicin was used as the positive control (0.08-5 μg mL^-1), while DMSO (0.5%) was used as negative control. Four hours (for tumor cell lines) and 24 h (for PBMCs) before the endo of incubation period, 20 μL of Alamar blue reagent were added to each well. Subsequently, absorbance was measured on a Spectra Max 190 multiplate reader at 570 nm and 600 nm. Half-inhibitory concentration (IC₅₀) was obtained by nonlinear regression with 95% confidence intervals (CI 95%).

RESULTS AND DISCUSSION

The phytochemical investigation of the hexane extract from the leaves of X. laevigata (Annonaceae) yielded six compounds (Figure 1), including one uncommon ent-kaurene diterpenoid ent-7β-acetoxy-16β-hydroxy-kaurane (3), in addition to other five isolated compounds, abieta-7,13-dien-3-one (1),²⁶26 Feliciano, A. S.; Del Corral, J. M. M.; Gordaliza, M.; Castro, M. A.; Phytochemistry 1991, 30, 695. spathulenol (2),²⁴24 Ragasa, C.Y.; Ganzon, J.; Hofileña, J.; Tamboong, B.; Rideout, J. A.; Chem. Pharm. Bull. 2003, 51, 1208. 13-hydroxy-ent-labda-8,14-dien-18-oic acid (4-epi-cupressic acid) (4),²⁷27 Hieda, T.; Mikami, Y.; Obi, Y.; Kisaki, T.; Agric. Biol. Chem. 1992, 46, 2477. (−)-kaurane-7β,16α-diol (powerol) (5),²⁸28 González, A. G.; Fraga, B. M.; Hernández, M. G.; Luis, J. G.; Tetrahedron 1973, 29, 561. and 8,20-epoxy-13-hydroxy-ent-labda-14-en-18-oic acid (labdorffianic acid B) (6).²⁹29 Dos Santos, P. F.; Duarte, M. C.; Bezerra, D. A. C.; Agra, M. de F.; Filho, J. M. B.; Da Silva, M. S.; Tavares, J. F.; Helv. Chim. Acta 2013, 96, 1085.

Figure 1
Chemical structures of the isolated compounds 1-6

Compound 3 was obtained as a white amorphous powder with the molecular formula C₂₂H₃₆O₃ as determined by HR-ESIMS (m/z 371.2558 [M+Na]⁺, calc. 371.2562) and NMR data. HR-ESIMS also showed a fragment at m/z 271.2440 [M−H₂O−C₂H₃O₂]⁺ (Figure 2), which is in agreement with the fragment at m/z 270 [M−H₂O−C₂H₃O₂]^+• observed using the GC−MS analysis. The ¹H NMR spectrum displayed the characteristic signals of four methyl groups, which are characteristic of diterpenes from the kaurane series, and typical for C-17, C-18_ax, C-19_eq and C-20_ax.²⁵25 Ahmed, S. A.; Gogal, R. M.; Walsh, J. E.; J. Immunol. Methods 1994, 170, 211. The signals at δ_H 2.05 (s, 3H) and δ_H 4.62 (dd, J = 2.8 and 2.9 Hz, 1H) revealed the presence of an acetoxy group and an oxygenated carbon in the structure, respectively. The ¹³C{¹H} and DEPT135 NMR spectra, as well as one-bond and long-range ¹H-¹³C correlations from HSQC and HMBC NMR experiments indicated a total of 22 carbon atoms, which comprised of five methyls, eight methylenes, four methines (one oxygenated at δ_C 76.2), four quaternary carbons (one oxygenated at δ_C 72.0), and one acetoxy group (Table 1). The hydrogen signal at δ_H 4.62 (H-7) showed direct ¹H-¹³C correlation with the carbon at δ_C 76.2 and long-range ¹H-¹³C correlations with the carbons at δ_C 46.8 (C-9), δ_C 48.1 (C-5) and δ_C 170.5, which supports the substitution pattern proposed with the acetoxy group placed at C-7 (Figure 3).

Figure 2
Proposed fragmentation pathway for compound 3

Figure 3
Main HMBC and NOESY correlations observed for ent-7β-acetoxy-16β-hydroxy-kaurane (3)

The relative configuration of this compound was determined via 1D NOESY NMR experiments. The selective irradiation of the NMR frequency of the methyl group at δ_H 2.05 (s) caused a NOE enhancement in the signals at δ_H 4.62 (dd, J = 2.9 and 2.8 Hz, H-7_eq), δ_H 1.66 (m, H-6_eq), δ_H 1.57 (m, H-9_ax), δ_H 1.31 (dd, J = 9.1 and 2.8 Hz, H-5_ax), δ_H 1.19 (d, J = 13.6 Hz, H-15_ax), and δ_H 0.78 (s, H-19_eq). Similarly, the selective irradiation of H-7 caused NOE intensification of the signals at δ_H 1.63 (m, H-6_ax), δ_H 1.66 (H-6_eq), δ_H 0.98 (H-14_eq), and δ_H 1.19 (H-15_pax), which confirmed the β-orientation of the acetoxy group at C-7 (i.e. acetoxy group is in axial position). On the other hand, the selective irradiation of NMR frequency of H-17 (methyl group) caused a NOE enhancement in the signals at δ_H 1.19 (H-15_ax) and δ_H 1.53 (m, H-13_eq), which confirms the presence of a hydroxyl group in β-orientation at the C-16 position (i.e. the hydroxyl group is in an axial position). Furthermore, the selective irradiation of H-18 at δ_H 0.80 caused a NOE enhancement of the signals at δ_H 0.78 (s, H-19_eq), δ_H 0.96 (s, H-20_ax), δ_H 1.41 (m, H-3_eq), and δ_H 1.60 (H-6_ax). The selective irradiation of a singlet at δ_H 0.78 (H-19) showed NOE intensifications at δ_H 1.17 (m, H-3_ax), δ_H 1.41 (m, H-3_eq), δ_H 1.31 (dd, H-5_ax), δ_H 1.66 (H-6_eq), δ_H 2.05 (s, CH₃COO), and some intensification of the signal at δ_H 0.96 (H-20_ax). These observations confirm the axial and equatorial orientations of the methyl groups at C-18 and C-19, respectively. Likewise, the selective irradiation of H-20 at δ_H 0.96 caused NOE intensifications at the signals at δ_H 0.80 (s, H-18_ax), δ_H 1.70 (m, H-14_ax), δ_H 1.59 (m, H-2_ax), and δ_H 1.60 (m, H-6_ax), this fact proves the β-orientation of the methyl group C-20 (Figure 3). The exhaustive analysis of 1D and 2D NMR data enabled the structure to be fully established, and ¹H and ¹³C NMR chemical shifts unequivocally assigned (Table 1). Therefore, compound 3 was identified as the known ent-kaurane diterpene called ent-7β-acetoxy-16β-hydroxy-kaurane (also known powerol 7β-acetate), which was a product of acetylation of (−)-kaurane-7β,16α-diol (powerol) (5) (Table 1). Therefore, this is the first report of compound 3 as a natural product, as well as its second report in the literature. According to previously published literature data,²⁸28 González, A. G.; Fraga, B. M.; Hernández, M. G.; Luis, J. G.; Tetrahedron 1973, 29, 561. only some ¹H NMR resonances were described for this compound, which enabled us to extensively revise 1D and 2D NMR data and unequivocally assign the chemical shifts of hydrogen and carbon atoms (Table 1), and its relative configuration.

The isolated compounds: abieta-7,13-dien-3-one (1),²⁶26 Feliciano, A. S.; Del Corral, J. M. M.; Gordaliza, M.; Castro, M. A.; Phytochemistry 1991, 30, 695. spathulenol (2),²⁴24 Ragasa, C.Y.; Ganzon, J.; Hofileña, J.; Tamboong, B.; Rideout, J. A.; Chem. Pharm. Bull. 2003, 51, 1208. 13-hydroxy-ent-labda-8,14-dien-18-oic acid (4),²⁷27 Hieda, T.; Mikami, Y.; Obi, Y.; Kisaki, T.; Agric. Biol. Chem. 1992, 46, 2477. (−)-kaurane-7β,16α-diol (5),²⁸28 González, A. G.; Fraga, B. M.; Hernández, M. G.; Luis, J. G.; Tetrahedron 1973, 29, 561. and 8,20-epoxy-13-hydroxy-ent-labda-14-en-18-oic acid (6)²⁹29 Dos Santos, P. F.; Duarte, M. C.; Bezerra, D. A. C.; Agra, M. de F.; Filho, J. M. B.; Da Silva, M. S.; Tavares, J. F.; Helv. Chim. Acta 2013, 96, 1085. were identified by comparison of their NMR and MS data with those previously reported in the literature. Nevertheless, compounds 1, 4, and 6 have been described a long time ago and their published NMR data was incomplete (¹H and ¹³C NMR). As well as showing some ambiguities in the scalar coupling constants, most of them not been previously assigned.²⁶26 Feliciano, A. S.; Del Corral, J. M. M.; Gordaliza, M.; Castro, M. A.; Phytochemistry 1991, 30, 695.^,²⁷27 Hieda, T.; Mikami, Y.; Obi, Y.; Kisaki, T.; Agric. Biol. Chem. 1992, 46, 2477.

28 González, A. G.; Fraga, B. M.; Hernández, M. G.; Luis, J. G.; Tetrahedron 1973, 29, 561.^-²⁹29 Dos Santos, P. F.; Duarte, M. C.; Bezerra, D. A. C.; Agra, M. de F.; Filho, J. M. B.; Da Silva, M. S.; Tavares, J. F.; Helv. Chim. Acta 2013, 96, 1085. Therefore, the complete and unequivocal NMR data for these diterpenes were reviewed according to the 1D and 2D NMR experiments (Tables 1 and 2).

The absolute configurations of the diterpenoids from the ent and normal series can be established based on their specific rotations ([α]_D), since they can be correlated to similar diterpenes with well-defined absolute configurations.³⁰30 Velandia, J. R.; Carvalho, M. G.; Braz-Filho, R.; Quim. Nova 1998, 21, 397. Therefore, those that divert to the right (+) belong to the normal series, while those that divert the polarized light to the left (−) belong to the ent series.³⁰30 Velandia, J. R.; Carvalho, M. G.; Braz-Filho, R.; Quim. Nova 1998, 21, 397. Thus, it was established that the diterpenes 3 ([α]_D²⁵ −1.00º) and 5 ([α]_D²⁵ −2.70º) belong to the ent series.³⁰30 Velandia, J. R.; Carvalho, M. G.; Braz-Filho, R.; Quim. Nova 1998, 21, 397.

Diterpenes of ent-kaurane type are common in Annonnaceae, especially in the species of Annona and Xylopia.³¹31 Leboeuf, M.; Cavé, A.; Bhaumik, P. K.; Mukherjee, B.; Mukherjee, R.; Phytochemistry 1982, 21, 2783.

32 Takahashi, J. Á.; Boaventura, M. A. D.; Bayma, J. C.; Oliveira, A. B.; Phytochemistry 1995, 40, 607.

33 Takahashi, J. A.; Vieira, H. S.; Boaventura, M. A. D.; Hanson, J. R.; Hitchcock, P. B.; Oliveira, A. B.; Quim. Nova 2001, 24, 616.^-³⁴34 Chen, C. Y.; Chang, F. R.; Wu, Y. C.; J. Chin. Chem. Soc. 1997, 44, 313. The presence of other diterpene types in X. laevigata indicates that Xylopia species have a strong ability to produce different diterpenes (compounds 1, 4, and 6) and suggest the need for more investigation in order to confirm the presence of other compounds of these types in this species, as well as other Xylopia spp., such as 6, that has been only previously reported as occurring in Xylopia langsdorffiana.³⁰30 Velandia, J. R.; Carvalho, M. G.; Braz-Filho, R.; Quim. Nova 1998, 21, 397. On the other hand, diterpenes 1, 3, 4, and 5 have been reported for the first time in Annonaceae. The occurrence of diterpenes possessing the acetoxy function was described previously in Annonaceae.³¹31 Leboeuf, M.; Cavé, A.; Bhaumik, P. K.; Mukherjee, B.; Mukherjee, R.; Phytochemistry 1982, 21, 2783.

32 Takahashi, J. Á.; Boaventura, M. A. D.; Bayma, J. C.; Oliveira, A. B.; Phytochemistry 1995, 40, 607.

33 Takahashi, J. A.; Vieira, H. S.; Boaventura, M. A. D.; Hanson, J. R.; Hitchcock, P. B.; Oliveira, A. B.; Quim. Nova 2001, 24, 616.^-³⁴34 Chen, C. Y.; Chang, F. R.; Wu, Y. C.; J. Chin. Chem. Soc. 1997, 44, 313. Therefore, this study contributes to the chemotaxonomy of the genus Xylopia, as well as to the Annonaceae family.

The cytotoxic activity of the isolated compounds 1, 2, 4 and 5 was evaluated against tumor (B16-F10, HepG2, HL-60, and K562) and non-tumor (PBMC) cell lines (Table 3) with increasing concentrations under 72 h of incubation and analyzed using the Alamar blue assay. Compared to the positive control (doxorubicin), compound 2 exhibited a moderate cytotoxic effect by showing IC₅₀ from 17.20 to 50.78 μmol L^-1 for the tumor cell lines tested (Table 3). For K562, compound 2 showed a significant cytotoxic effect with an IC₅₀ value of 17.20 μmol L^-1. However, the cytotoxic activity against the normal cell PBMC (IC₅₀ = 70.75 μmol L^-1) was considered moderate, since it showed slow selectivity against K562. Furthermore, compound 5 also exhibited moderate cytotoxic effect against B16-F10, HL-60, and K562 tumor cell lines with an IC₅₀ of 80.36, 47.11, and 64.60 μmol L^-1, respectively, although, it was inactive against HepG2 cell line (IC₅₀ greater than 81.57 μmol L^-1) (Table 3). On the other hand, this compound was also considered not to be cytotoxic for normal cell lines of IC₅₀ (IC₅₀ > 81.57 μmol L^-1). Doxorubicin presented IC₅₀ values which ranged from 0.15 μmol L^-1 to 0.28 μmol L^-1 for the tumor cell lines evaluated (Table 3). In addition, doxorubicin also displayed cytotoxic activity against PBMC with IC₅₀ value of 4.54 μmol L^-1. However, it is important to mention that doxorubicin is the drug used in the treatment of cancer, though also responsible for serious collateral effects.

Thumbnail

Table 3
In vitro cytotoxic activity

CONCLUSION

The phytochemical investigation of the hexane extract of the leaves of X. laevigata yielded six terpenoids, including an uncommon diterpene known as ent-7β-acetoxy-16β-hydroxy-kaurane (3), herein reported for the first time as a natural product. Compounds 1, 3, 4, and 5 are described here for the first time within the family Annonaceae. This work reinforces the fact that Xylopia is a rich, natural source for different types of diterpernes. Besides this, spathulenol (2) showed moderated cytotoxicity against all cell lines tested, while powerol (5) displayed weak activity.

SUPPLEMENTARY MATERIAL

Supplementary information containing 1D and 2D NMR, and MS data for isolated compounds is available free of charge at http://quimicanova.sbq.org.br as a PDF file.

ACKNOWLEDGEMENTS

The authors are grateful to Prof. Dr. Norberto P. Lopes and José Carlos Tomaz from Faculdade de Ciências Farmacêuticas de Ribeirão Preto, USP for the ESIMS analysis, Prof. Dr. A. P. do N. Prata of the DBI/UFS for the botanical identification, as well as to CNPq, CAPES, FAPITEC/SE, FINEP, UFPR, UFS and UFAM for financial support and research fellowships.

REFERENCES

¹
Chatrou, L. W.; Pirie, M. D.; Erkens, R. H. J.; Couvreur, T. L. P.; Neubig, K. M.; Abbott, J. R.; Mols, J. B.; Mass, J. W.; Saunders, R. M. K.; Chase, M. W.; Bot. J. Linn. Soc. 2012, 169, 5; Maas, P. J. M.; Kamer, H. M.; Junikka, L.; Mello-Silva, R.; Rainer, H.; Rodriguésia 2001, 52, 61.
²
Moreira, I. C.; Roque, N. F.; Vilegas, W.; Zalewski, C. A.; Lago, J. H. G.; Funasaki, M.; Chem. Biodivers. 2013, 10, 1921.
³
Corrêa, M. P.; Dicionário das plantas úteis do Brasil e das exóticas cultivadas, IBDF: Rio de Janeiro, 1984.
⁴
Karioti, A.; Hadjipavlou-Litina, D.; Mensah, M. L. K.; Fleischer, T. C.; Skaltsa, H.; J. Agric. Food. Chem. 2004, 52, 8094.
⁵
Quintans, J. S. S.; Soares, B. M.; Ferraz, R. P. C.; Oliveira, A. C. A.; Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Prata, A. P. N.; Moraes, M. O.; Pessoa, C.; Antoniolli, A. R.; Costa, E. V.; Bezerra, D. P.; Planta Med. 2013, 79, 123; Queiroz, J. C.; Antoniolli, A. R.; Quintans-Júnior, L. J.; Brito, R. G.; Barreto, R. S. S.; Costa, E. V.; Silva, T. B.; Prata, A. P. N.; Lucca Jr., W.; Almeida, J. R. G. S.; Lima, J. T.; Quintans, J. S. S.; Sci. World J. 2014, 2014, ID 816450.
⁶
Silva, D. M.; Costa, E. V.; Nogueira, P. C. L.; Moraes, V. R. S.; Cavalcanti, S. C. H.; Salvador, M. J.; Ribeiro, L. H. G.; Gadelha, F. R.; Barison, A.; Ferreira, A. G.; Quim. Nova 2012, 35, 1570.
⁷
Maia, J. G. S.; Andrade, E. H. A.; Da Silva, A. C. M.; Oliveira, J.; Carreira, L. M. M.; Araújo, J. S.; Flavour Fragance J. 2005, 20, 474; Moreira, I. C.; Lago, J. H. G.; Young, M. C. M.; Roque, N. F.; J. Braz. Chem. Soc. 2003, 14, 828.
⁸
Da Silva, M. S.; Tavares, J. F.; Queiroga, K. F.; Agra, M. F.; Barbosa-Filho, J. M.; Almeida, J. R. G. S.; Da Silva, S. A. S.; Quim. Nova 2009, 32, 1566; Puvanendran, S.; Wickramasinghe, A.; Karunaratne, D. N.; Carr, G.; Wijesundara, D. S. A.; Andersen, R.; Karunaratne, V.; Pharm. Biol. 2008, 46, 352.
⁹
López, R.; Cuca, L. E.; Delgado G.; Parasite Immunol. 2009, 31, 623.
¹⁰
Castelo-Branco, M. V. S.; Tavares, J. F.; Silva, M. S.; Barbosa Filho, J. M.; Anazetti, M. C.; Frungillo, L.; Haun, M.; Diniz, M. F. F. M.; Melo, P. S.; Rev. Bras. Farmacogn. 2011, 21, 1035.
¹¹
Nishiyama, Y.; Moriyasu, M.; Ichimaru, M.; Iwasa, K.; Kato, A.; Mathenge, S. G.; Mutiso, P. B. C.; Juma, F. D.; J. Nat. Med. 2010, 64, 9.
¹²
Pontes, W. J. T.; Oliveira, J. C. S.; Câmara, C. A. G.; Gondim Jr., M. G. C.; Oliveira, J. V.; Schwartz, M. O. E.; Quim. Nova 2007, 30, 838.
¹³
Nguemtchouin, M. M. G.; Ngassoum, M. B.; Ngamo, L. S. T.; Gaudu, X.; Cretin, C.; Crop Prot. 2010, 29, 985.
¹⁴
Barbosa, L. T. C.; Vega, M. R. G.; Rev. Virtual Quim. 2017, 9, 1712.
¹⁵
Pontes, A. F.; Barbosa, M. R. V.; Maas, P. J. M.; Acta Bot. Bras. 2004, 18, 281.
¹⁶
Costa, E. V.; Silva, T. B.; Menezes, L. R. A.; Ribeiro, L. H. G.; Gadelha, F. R.; Carvalho, J. E.; Souza, L. M. B.; Silva, M. A. N.; Siqueira, C. A. T.; Salvador, M. J.; J. Essent. Oil Res. 2013, 25, 179.
¹⁷
Silva, T. B.; Menezes, L. R. A.; Sampaio, M. F. C.; Meira, C. S.; Guimarães, E. T.; Soares, M. B. P.; Prata, A. P. N.; Nogueira, P. C. L.; Costa, E. V.; Nat. Prod. Commun. 2013, 8, 403.
¹⁸
Nascimento, A. M. D.; Maia, T. D. S.; Soares, T. E. S.; Menezes, L. R. A.; Scher, R.; Costa, E. V.; Cavalcanti, S. C. H.; La Corte, R.; Neotrop. Entomol. 2017, 46, 223.
¹⁹
Costa, E. V.; da Silva, T. B.; Costa, C. O.; Soares, M. B.; Bezerra, D. P.; Nat. Prod. Commun. 2016, 11, 417.
²⁰
Pereira, T. S.; Esquissato, G. N. E.; Costa, E.V.; Nogueira, P. C. L.; Castro-Prado, M. A. A.; Nat. Prod. Res. 2019, doi:10.1080/14786419.2019.1624956.
» https://doi.org/10.1080/14786419.2019.1624956
²¹
Costa, E. V.; Dutra, L. M.; Nepel, A.; Barison, A.; Biochem. Syst. Ecol. 2013, 51, 331.
²²
Menezes, L. R. A.; Costa, C. O. D.; Rodrigues, A. C. B. C.; Santo, F. R. E.; Nepel, A.; Dutra, L. M.; Silva, F. M. A.; Soares, M. B. P.; Barison, A.; Costa, E. V.; Bezerra, D. P.; Molecules 2016, 21, 890.
²³
Santos, L. S.; Silva, V. R. S.; Menezes, L. R. A. M.; Soares, M. B. P. S.; Costa, E. V.; Bezerra, D. P.; Oxid. Med. Cell. Longevity 2017, 2017, ID 7126872, doi: 10.1155/2017/7126872.
» https://doi.org/10.1155/2017/7126872.
²⁴
Ragasa, C.Y.; Ganzon, J.; Hofileña, J.; Tamboong, B.; Rideout, J. A.; Chem. Pharm. Bull. 2003, 51, 1208.
²⁵
Ahmed, S. A.; Gogal, R. M.; Walsh, J. E.; J. Immunol. Methods 1994, 170, 211.
²⁶
Feliciano, A. S.; Del Corral, J. M. M.; Gordaliza, M.; Castro, M. A.; Phytochemistry 1991, 30, 695.
²⁷
Hieda, T.; Mikami, Y.; Obi, Y.; Kisaki, T.; Agric. Biol. Chem. 1992, 46, 2477.
²⁸
González, A. G.; Fraga, B. M.; Hernández, M. G.; Luis, J. G.; Tetrahedron 1973, 29, 561.
²⁹
Dos Santos, P. F.; Duarte, M. C.; Bezerra, D. A. C.; Agra, M. de F.; Filho, J. M. B.; Da Silva, M. S.; Tavares, J. F.; Helv. Chim. Acta 2013, 96, 1085.
³⁰
Velandia, J. R.; Carvalho, M. G.; Braz-Filho, R.; Quim. Nova 1998, 21, 397.
³¹
Leboeuf, M.; Cavé, A.; Bhaumik, P. K.; Mukherjee, B.; Mukherjee, R.; Phytochemistry 1982, 21, 2783.
³²
Takahashi, J. Á.; Boaventura, M. A. D.; Bayma, J. C.; Oliveira, A. B.; Phytochemistry 1995, 40, 607.
³³
Takahashi, J. A.; Vieira, H. S.; Boaventura, M. A. D.; Hanson, J. R.; Hitchcock, P. B.; Oliveira, A. B.; Quim. Nova 2001, 24, 616.
³⁴
Chen, C. Y.; Chang, F. R.; Wu, Y. C.; J. Chin. Chem. Soc. 1997, 44, 313.

Publication Dates

Publication in this collection
10 June 2020
Date of issue
Apr 2020

History

Received
02 Oct 2019
Accepted
14 Jan 2020
Published
31 Mar 2020

This is an Open Access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

[1] SUPPLEMENTARY MATERIAL

Supplementary information containing 1D and 2D NMR, and MS data for isolated compounds is available free of charge at http://quimicanova.sbq.org.br as a PDF file.

Position	ent-7β -acetoxy-16β -hydroxy-kaurane (3)		Powerol (5)
Position	δ_C	δ_H mult. (J in Hz)	δ_C	δ_H mult. (J in Hz)
1	39.1	ax 0.88 m eq 1.55 m	39.2	ax 0.88 m eq 1.53 m
2	18.1	ax 1.59 m eq 1.40 m	18.2	ax 1.59 m eq 1.40 m
3	42.0	ax 1.17 m eq 1.41 m	42.1	ax 1.20 m eq 1.41 m
4	32.5		32.6
5	48.1	ax 1.31 dd (9.1 and 2.8)	47.3	1.35 dd (12.3 and 2.8)
6	24.0	ax 1.60 m eq 1.66 m	26.9	ax 1.61 m eq 1.63 m
7	76.2	eq 4.62 dd (2.9 and 2.8)	73.9	eq 3.39 dd (2.9 and 2.8)
8	37.1		32.6
9	46.8	ax 1.57 m	46.1	ax 1.53 m
10	37.6		37.8
11	22.5	ax 1.18 m eq 1.99 m	23.6	ax 1.50 m eq 1.66 m
12	23.4	ax 1.24 m eq 1.52 m	22.5	ax 1.98 dddd (14.5, 11.7, 3.0 and 3.0) eq 1.17 m
13	37.8	eq 1.53 m	37.8	1.54 m
14	26.5	ax 1.70 m eq 0.98 m	26.8	ax 1.63 m eq 0.90 m
15	50.4	ax 1.19 d (13.6) eq 1.56 d (13.6)	51.4	ax 1.27 m eq 1.72 m
16	72.0		72.2
17	30.6	1.29 s	30.6	1.31 s
18	21.5	0.80 s	21.7	0.82 s
19	33.0	0.78 s	33.2	0.86 s
20	13.4	0.96 s	13.5	0.95 s
CH₃COO-7	170.5
CH₃COO-7	21.2	2.05 s

Position	abieta-7,13-dien-3-one (1)		4-epi-cupressic acid (4)		labdorffianic acid B (6)
Position	δ_C	δ_H mult. (J in Hz)	δ_C	δ_H mult. (J in Hz)	δ_C	δ_H mult. (J in Hz)
1	38.1	ax 1.51 ddd (14.5, 13.5 and 3.9) eq 2.17 ddd (13.5, 5.3 and 3.6)	38.0	ax 1.15 m eq 1.81 m	38.0	ax 1.15 m eq 1.78 m
2	34.8	ax 2.28 ddd (14.4, 3.9 and 3.6) eq 2.76 ddd (14.5, 14.4 and 5.3)	18.4	ax 1.60 m eq 1.78 m	17.6	ax 1.58 m eq 1.61 m
3	216.9		37.1	ax 1.63 m eq 1.79m	37.0	ax 1.63 m eq 1.77 m
4	47.6		47.5		47.2
5	51.4	1.66 dd (11.8 and 5.0)	49.6	1.95 dd (12.5 and 2.8)	49.2	1.88 dd (12.4 and 4.6)
6	24.2	ax 2.09 m eq 2.16 m	26.8	eq 1.35 dddd (12.8, 5.4, 2.8 and 2.3) ax 1.46 dddd (13.1, 12.8, 12.5 and 4.3)	24.3	ax 1.45 m eq 1.60 m
7	120.7	5.47 m	37.8	ax 2.04 ddd (13.1, 12.7 and 5.4) eq 2.34 ddd (12.7, 4.3 and 2.3)	36.2	eq 1.33 ddd (12.6, 4.4 and 2.5) ax 1.94 dddd (12.8, 12.6, 4.7 and 1.8)
8	135.3		148.0		59.2
9	50.0	1.89 m	57.2	1.65 m	54.2	1.52 m
10	34.8		39.1		39.7
11	22.7	ax 1.29 m eq 1.84 m	17.5	1.32 m 1.55 m	15.9	0.78 m 1.21 m
12	27.4	ax 2.10 m eq 2.11 m	41.2	1.34 m 1.71 m	43.6	1.51 m 1.65 m
13	145.8		73.7		73.5
14	122.1	5.81 m	145.0	5.90 dd (17.3 and 10.8)	145.4	5.88 dd (17.3 and 10.7)
15	34.9	2.24 m	111.7	5.07 dd (10.8 and 1.1) 5.21 dd (17.3 and 1.1)	111.4	5.02 dd (10.7 and 1.3) 5.19 dd (17.3 and 1.3)
16	21.4	1.01 d (6.7)	28.1	1.27 s	27.9	1.22 s
17	20.8	1.02 d (6.7)	107.1	4.50 d (1.2) 4.82 d (1.2)	50.7	2.48 d (4.3) 2.77 dd (4.3 and 1.8)
18	22.2	1.14 s	16.4	1.14 s	16.3	1.17 s
19	25.0	1.07 s	184.3		183.9
20	13.4	1.03 s	14.7	0.70 s	14.9	0.82 s

Compounds	IC₅₀ µmol L^-1
Compounds	B16-F10	HepG2	HL-60	K562	PBMC
1	>87.27	>87.27	>87.27	>87.27	>87.27
2	52.96 44.36 - 63.46	50.78 43.55 - 59.41	51.65 38.46 - 69.59	17.20 6.73 - 44.09	70.75 59.64 - 84.23
4	>78.01	>78.01	>78.01	>78.01	>78.01
5	80.36 73.37 - 88.30	>81.57	47.11 26.24 - 84.80	64.60 50.65 - 82.68	>81.57
Doxorubicin	0.15 0.09 - 0.26	0.15 0.11 - 0.18	0.17 0.11 - 0.22	0.28 0.15 - 0.57	4.54 3.31 - 6.24

Brasil