Copaifera multijuga ethanolic extracts, oil-resin, and its derivatives display larvicidal activity against Anopheles darlingi and Aedes aegypti (Diptera: Culicidae)

Trindade, Frances Tatiane Tavares; Stabeli, Rodrigo Guerino; Pereira, Antônio Almeida; Facundo, Valdir Alves; Silva, Alexandre de Almeida e

doi:10.1590/S0102-695X2013005000038

Abstract

Copaifera spp. is a common tree species found in the tropical region of Latin America, popularly known as copaiba or pau-d'alho. Oil-resin from different Copaifera species and its components present several biological activities such as antimicrobial, anti-inflammatory, antioxidant and insecticidal, including larvicidal activity against mosquitoes. Thus, bark and leaf ethanolic extracts, oil-resin, essential oil and alepterolic acid from Copaifera multijuga Hayne, Fabaceae, were tested as larvicides against the main malaria vector in the north of Brazil, Anopheles darlingi and also Aedes aegypti, the dengue vector. A. darlingi larval mortality was significantly higher than A. aegypti for most tested compounds. Bark and leaf extracts resulted in lower Lethal Concentrations (LC50) values for A. darlingi, 3 and 13 ppm, respectively, while the essential oil provided the lowest LC50 value for A. aegypti, 18 ppm. Despite of that, the lowest LC values were from the alepterolic acid for both species, i.e. 0.9 and 0.7 ppm for A. darlingi and A. aegypti, respectively.

Copaifera multijuga; Anopheles darlingi; Aedes aegypti; vector control

Copaifera multijuga ethanolic extracts, oil-resin, and its derivatives display larvicidal activity against Anopheles darlingi and Aedes aegypti (Diptera: Culicidae)

Frances Tatiane Tavares Trindade^I,IV; Rodrigo Guerino Stabeli^II,IV; Antônio Almeida Pereira^III; Valdir Alves Facundo^III; Alexandre de Almeida e Silva^I,IV

^ILaboratório de Bioecologia de Insetos, Departamento de Biologia, Universidade Federal de Rondônia, Brazil

^IICentro de Estudos de Biomoléculas Aplicadas a Medicina, Departamento de Medicina, Universidade Federal de Rondônia, Brazil

^IIILaboratório de Pesquisas Químicas em Produtos Naturais, Departamento de Química, Universidade Federal de Rondônia, Brazil

^IVFiocruz-Rondonia, Brazil

^{Correspondence} Correspondence Alexandre de Almeida e Silva Laboratório de Bioecologia de Insetos, Departamento de Biologia, Universidade Federal de Rondônia BR 364, km 9,5 (sentido Acre) 78900-000 Porto Velho-RO, Brazil

ABSTRACT

Copaifera spp. is a common tree species found in the tropical region of Latin America, popularly known as copaiba or pau-d'alho. Oil-resin from different Copaifera species and its components present several biological activities such as antimicrobial, anti-inflammatory, antioxidant and insecticidal, including larvicidal activity against mosquitoes. Thus, bark and leaf ethanolic extracts, oil-resin, essential oil and alepterolic acid from Copaifera multijuga Hayne, Fabaceae, were tested as larvicides against the main malaria vector in the north of Brazil, Anopheles darlingi and also Aedes aegypti, the dengue vector. A. darlingi larval mortality was significantly higher than A. aegypti for most tested compounds. Bark and leaf extracts resulted in lower Lethal Concentrations (LC50) values for A. darlingi, 3 and 13 ppm, respectively, while the essential oil provided the lowest LC50 value for A. aegypti, 18 ppm. Despite of that, the lowest LC values were from the alepterolic acid for both species, i.e. 0.9 and 0.7 ppm for A. darlingi and A. aegypti, respectively.

Keywords:Copaifera multijuga; Anopheles darlingi; Aedes aegypti; vector control

Introduction

Mosquitoes (Diptera: Culicidae) are important vectors of several human diseases including malaria and dengue. Anopheles darlingi is the principal vector of malaria in Rondonia and other Amazonian states; it is captured in high densities and frequency in anthropized environments (Gil et al., 2003). The dengue vector, Aedes aegypti, is a domestic and highly endophilous mosquito species (Consoli & Lorenço-de-Oliveira, 1994). Among many variables, the use of insecticides in vector control plays an important role in preventing transmission of these diseases. However, since chemical control often results in insect resistance to synthetic insecticides (Hemingway & Ranson, 2000), identifying new molecules with insecticidal properties remains a priority in the biotechnology field.

Copaifera spp. (commonly know as copaiba or pau-d'alho) is a tree species found throughout the tropics of Latin America that exudes oil-resin from the trunks (Leandro et al., 2012). Although many Copaifera species exists in the Amazon region, Copaifera multijuga Hayne, Fabaceae, provides a considerable amount of oil-resin commercialized (≈5%) (Lawrence, 1980), that peaks during the rainy season, especially ones growing in clay soils (Alencar, 1982). Up to 60% of the oil-resin composition comprises diterpene acids and volatile substances, such as sesquiterpene hydrocarbons. Plant nutrition, insect herbivory and light conditions greatly influences the concentration and composition of copaiba's oil-resin (Veiga Jr. et al., 2005; Langenheim, 1990).

The medicinal properties of Copaifera oil-resin have been described since the sixteenth century (see Veiga Jr et al., 2005 for a review). Oil-resin and other substances derived from different Copaifera species displayed antimicrobial, anti-inflammatory, antioxidant, and insecticidal activities (Leandro et al., 2012). Regarding insecticides, previous studies reported that oil-resin effectively killed mosquito larvae (Prophiro et al., 2012; Silva et al., 2003). Therefore, we evaluated the larvicidal activity of copaiba extracts, oil-resin, essential oil and alepterolic acid from C. multijuga against the malaria and dengue vectors, A. darlingi and A. aegypti.

Material and Methods

Processing the plant material

Oil-resin, bark, and leaves from Copaifera multijuga Hayne, Fabaceae, were collected in March 2008 from a tree located in Candeias do Jamari, Rondonia State, Brazil. Taxonomists from the Instituto Nacional de Pesquisas da Amazônia performed plant identification and the voucher specimen was deposited in the herbarium with identification number 223.353.

Dried and grounded C. multijuga trunk bark (1.6 kg) and leaves (1.9 kg) were extracted with 99% ethanol (2.0 L and 2.5 L, respectively) at room temperature over the course of five days. The solvent was evaporated under reduced pressure, leaving 36.0 g of bark ethanolic extract and 29.6 g of leaves ethanolic extract.

Extracting and analyzing the essential oil

Ten milliliters of oil-resin was distillated in a 500 mL round-bottom flask fitted with a 40 cm distillation column and a serpentine condenser coupled with an oil separator. The distillation process took 4 h and yielded 4 mL of essential oil.

The essential oil was analyzed by GC/MS (determination of Kovats Indices) with a HP-5971 apparatus, using a 25 m x 0.25 mm fused silica capillary SP-2100 column, helium as carrier gas 1 mL/min flow rate, and temperature programmed from 50-250 ºC at 4 ºC/min. Compound identification was initially done using a MS library search with Kovats indices as a pre-selection routine (Alencar et al. 1984; 1990) followed by visual confirmation to the standard MS obtained from literature (Adams, 2007).

Isolating and characterizing the components from the remaining oil-resin

After extracting the volatile compounds from the oil-resin, the remaining oil was separated from the aqueous phase using a separation funnel. This fraction was dried using anhydrous sodium sulphate and submitted to silica gel column chromatography eluted with n-hexane and chloroform in increasing polarity. The resulting white amorphous solid was subjected to IR, RMN ¹H and ¹³C spectroscopic analysis.

Collecting mosquitoes and breeding larvae

Adult A. darlingi mosquitoes were captured using a modified BG sentinel trap in peri-urban regions of Porto Velho, Rondonia. A. aegypti eggs were obtained from the Laboratório de Ecologia Química de Insetos Vetores, UFMG, Brazil and colonized under laboratory conditions (25-28 ºC, 12 h photoperiod and 80% humidity). Adult mosquitoes fed on blood from rabbits for 15 min to stimulate egg production and then were transferred to plastic cups covered with fine netting, where they fed on 20% sucrose. Three days after a meal, oviposition was induced in female mosquitoes by removing one wing from A. darlingi or introducing beakers containing distilled water to A. aegypti. The resulting larvae were fed with TetraMin Tropical Flakes fish food ad libitum until the 3^rd or 4^th instar stage.

Larvicidal bioassays

Larvicidal tests were performed in two sets. Set 1 was a dose response test with nine concentrations for extracts and oils (ppm: 5, 10, 25, 50, 125, 250, 500, 750, 1000) in order to determine the concentrations for the lethal concentration (LC50 and LC90) assay (Set 2) using five different concentrations and four replicates (WHO, 2005). Set 2 tests were repeated three times. Larval mortality was recorded from 24 to 48 h for LC calculation and interrupted after 96 h. Plant extracts or oils were diluted in DMSO and pipetted under the water surface of plastic cups (150 mL) containing 100 mL of distillated water and larvae (10 for Set 1 or 25 for Set 2) were introduced in the cups 30 min after pipetting. Lethal concentrations (LC) were calculated using Probit analysis and Weibull distribution (Minitab, Minitab Inc).

Statistical analysis

The effects of extract oils and isolated substance concentration on larval mortality were analyzed by TwoWay Anova or by non-parametric analysis, i.e., Kruskal-Wallis or Rank sum test (SigmaStat 2.0, 1992-1997) when data transformation for normalization failed.

Results

The essential oil extracted from the oil-resin was comprised of sequiterpene hydrocarbons with β-caryophyllene (57.1%) and α-humulene (10.2%) making up the principal compounds (Table 1).

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The IR, RMN ¹H and ¹³C spectroscopic analysis of the white amorphous solid isolated from the remaining oil-resin (after essential oil extraction) was identified as alepterolic acid or 3-hydroxy-copalic acid. Comparison of the RMN ¹H e ¹³C data with published data (Geris et al., 2008) confirmed the proposed structure.

The mortality rate of A. darlingi and A. aegypti larvae was significantly affected by different concentrations of extracts, oils, and alepterolic acid, often showing, an increasing number of deaths from 24 to 96 h. The larval mortality of A. aegypti and A. darlingi in most assays increased up to 48 and 72 h, accordingly (Figure 2 and 3). However, A. aegypti larval mortality was significantly lower than A. darlingi's when fed with bark (T=5.68; p<0.001) or leaf extract (T=8700.0; p<0.001), or oil-resin (T=7323.5; p=0.003), but not for essential oil (T=6593.0; p=0.603) even at high concentrations (Figure 1 and 2, respectively).

The C. multijuga bark extract affected of A. aegypti and A. darlingi larval mortality significantly in most of the extract concentrations tested (F=294,81; p<0,001 and F=29.36; p<0.001, respectively). At 200 ppm, bark extracts killed 86% of A. aegypti larvae after 48 h, while 83% of the A. darlingi larvae were dead within the same period at 125 ppm. A. darlingi larvae mortality reached 93% after 96 h (Figure 1A and 2A).

Larvicidal leaf extract caused larval mortality of both species in a similar temporal pattern described above, but with weaker effects compared to bark extract. For example, larval mortality at 200 ppm after 48 h reached 57% for A. aegypti (F=102.2; p<0.001) and 72% for A. darlingi (F=13.17; p<0.001) (Figure 1B and 2B).

Oil-resin from C. multijuga was tested at different concentrations for A. aegypti and A. darlingi. Oil-resin caused A. darlingi larval mortality only at higher concentrations (100-75 ppm) (F=30,1; p<0,001). For all other concentrations tested, A. aegypti larval mortality differed significantly (F=282.2; p<0.001). Although the larval mortality caused by the oil-resin was generally significantly higher for A. darlingi than A. aegypti (T=7325.5; p=0.003), the larval mortality of A. aegypti reached 90% after 96 h at 200 ppm, while for A. darlingi, 90% larval mortality was reached with 100 ppm (Figure 1D).

When mosquito larvae were exposed to the C. multijuga essential oil, the mortality rate did not differ between mosquito species. The number of deaths increased significantly after 24 h (F=6.84; p<0.001 - A. aegypti and F=5.52; p=0.002 - A. darlingi) and with increasing concentrations (F=175.34; p<0.001- A. aegypti and F=22.26; p<0.001 - A. darlingi) (Figure 1C and 2C).

The larvicidal activity of alepterolic acid did not differ significantly between species (T=6113.5; p=0.26) or change over the course of time (H=0.67; p=0.87 - A. aegypti and H=0.12; p=0.98 - A. darlingi) (i.e., highest mortality was reached after 24 h and did not increase afterwards) (Figure 3). However, larvae mortality increased significantly (H=77.3; p<0.001 - A. aegypti and H=77.5; p<0.001 - A. darlingi) with the concentration range tested, surpassing 50% for the lowest concentration evaluated at 1 ppm (Figure 3).

Bark and leaf extracts resulted in lower LC50 values for A. darlingi while the essential oil provided the lowest LC50 value for A. aegypti. Despite of that, the lowest LC values were from the alepterolic acid for both species (Table 2).

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Discussion

All the C. multijuga extracts tested affected larval mortality of the malaria vector A. darlingi and the dengue vector A. aegypti. However, the degree of larvicidal activity depended on concentration and duration of the assays.

The present data indicate that Copaifera ethanolic extracts from different organs have significant larvicidal activity against the mosquito species tested. Ribeiro et al. (2009) reported that fruit peel and leaf extracts of C. langsdorffii lead to greater reduction in food consumption and larvae weight of Spodoptera frugiperda compared to fruit pulp and seed extracts. The fungitoxicity of C. multijuga essential oil was higher than the oil-resin. Furthermore, the response of different fungus species to this species was variable (Deus et al., 2011). Such variation in biological activity probably arises from differences in qualitative and quantitative active chemical compounds from Copaifera. For example, Chen et al. (2009) showed that the concentration of individual sesquiterpenes of C. officinalis isolated from various plant organs (leaves, stems and roots) were different.

Thus, comparing biological activity using Copaifera extracts or mixtures was not a straightforward process even when using the same species due to different biological aspects, such as the chemical composition of extracts and compound mixtures and species variation. For example, Silva et al. (2007) and Kanis et al. (2011) evaluated the larvicidal activity of the oil-resin of C. reticulata on A. aegypti and acquired very different lethal concentration (LC) values.

Oliveira et al. (2006) studied the oil-resin production and composition of C. duckei, C. marttii, and C. reticulata in Moju, Para, Brazil for several months in 2003 and 2004 and related differences in oil-resin production and composition, even between individuals of the same species.

A. darlingi larvae were more susceptible to C. multijuga extracts compared to A. aegypti larvae. However, susceptibility to larvicides in Anophelinae and Culicinae species did not follow a pattern. Joseph et al. (2004) demonstrated that Culex quinquefasciatus larvae acquired a higher LC50 than A. gambiae when exposed to petroleum extracts of Neotatenia mitus. Other studies showed that A. stephensis larval mortality to pure oil of Dalbergia sissoo was much lower than A. aegypti and C. quinquefasciatus (Ansari et al., 2000). Bond et al. (2004) related a similar larvicidal activity of spinosad, a neurotoxin mixture produced by an actinomycete, against A. aegypti and A. albimanus.

The calculated LC for A. aegypti was generally greater than A. darlingi, except for when essential oil and isolated substance was applied. Bark extract had a LC50 ten times lower than oil-resin for A. darlingi, but most biological assays and chemical characterization comprise Copaifera oil-resin only. Silva et al. (2001; 2003) tested the susceptibility of A. aegypti and C. quinquefasciatus larvae to the oil-resin extracted from C. langsdorffii and C. reticulata, respectively, and observed a gradual decrease in susceptibility as the larvae progressed from 1st to 4th instar. The estimated LC50 ranged from 0.4 (1st instar) to 80 ppm (4th instar); Prophiro et al. (2012) related a LC50 of 47 and LC90 of 91 ppm for wild A. aegypti using Copaifera spp. oil.

Larvicidal activity of isolated substances or subfractions of Copaifera spp oil-resin components resulted in a much lower LC for A. aegypti. For example, the LC50 of methanolic subfractions of C. reticulata for mono, sesquiterpenes, and labdane diterpenes were 3.9, 7.5 and 0.8 ppm, respectively (Silva et al., 2007). The labdane diterpene 3-β-acetoxylabdan-8 (17)-13-dien-15-oic acid isolated from C. reticulata with LC50 0.8 ppm (Geris et al., 2008) caused several ultra-structural alterations in the A. aegypti midgut and killed the larvae after 22 h of exposure (Valotto et al., 2011). Geris et al. (2008) also evaluated the larvicidal effect of the alepterolic acid against A. aegypti but received LC values 100 times higher compared to the present work. This was not surprising since resistance to insectides (e.g., temephos) and detoxifying enzymes, such as GST and alfa esterases activity, may vary greatly within A. aegypti populations that are 10 km apart (Lima et al., 2011).

Finally, C. multijuga larvicidal activity against A. darlingi, the main malaria vector in Northern Brazil, is presented here for the first time. Chemical characterization of bark and leaf extract derived from C. multijuga and larvicidal evaluation of the isolated compounds against A. darlingi or the principal essential oil compounds against A. aegypti may provide insight into potential larvicidal compounds with a lower lethal concentration as demonstrated with alepterolic acid. The present data also show that A. darlingi are more susceptibility to Copaifera extracts compared to the dengue vector A. aegypti.

Acknowledgements

The authors thank Nanobiotec-CAPES 10; CNPq grants 575563/2008-7, 550854/2010-0 and 550934/2010-3 for financial support of this project; Mei Tong, UMass Medical School for the English revision of the manuscript, and Elizângela Melo, Isabel Lucena and Hilamani Torres for their assistance during the insect collection and experiment set up.

Authors' contributions

FTTT contributed in the larvicidal experiments, analysis of the data and drafted the paper. AAP contributed in the phytochemical analysis. VAF supervised the phytochemical analysis and critical reading of the manuscript. RGS contributed to critical reading of the manuscript. AAS designed the study, supervised the laboratory work, drafted the paper and contributed with data analysis. All the authors have read the final manuscript and approved the submission.

Fiocruz-Rondonia, Rua da Beira, 7671

76812-245 Lagoa, Porto Velho-RO, Brazil

Tel.: +55 69 3219-6010 Fax: +55 69 3219-6000

alealsil@unir.br

Received 13 Dec 2012

Accepted 3 Apr 2013

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Correspondence

Alexandre de Almeida e Silva

Laboratório de Bioecologia de Insetos, Departamento de Biologia, Universidade Federal de Rondônia

BR 364, km 9,5 (sentido Acre)

78900-000 Porto Velho-RO, Brazil

Publication Dates

Publication in this collection
14 May 2013
Date of issue
June 2013

History

Received
13 Dec 2012
Accepted
03 Apr 2013

This work is licensed under a Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International License.

[1] Adams RP 2007. Identification of Essential Oil Components by Gas Chromatography/Mass Spectroscopy. Allured Publishing Corporation: New York, NY, USA.

[2] Alencar JC 1982. Estudos silviculturais de uma população natural de Copaifera multijuga Hayne-Leguminosae, na Amazonia Central. Acta Amazonica 12:75-89.

[3] Alencar JW, Craveiro AA, Matos FJA, Machado MLL 1990. Kovats indices simulation in essential oil analysis. Quim Nova 13:282-284.

[4] Alencar JW, Craveiroand AA, Matos EJA 1984. Kovats indices preselection routine in mass spectra library searches of volatiles. J Nat Prod 47:890-892.

[5] Ansari MA, Razdan RK, Tandon M, Vasudevan P 2000. Larvicidal and repellent actions of Dalbergia sissoo Roxb. (F. Leguminosae) oil against mosquitoes. Bior Tech 73:207-211.

[6] Bond JG, Marina C F, Williams T 2004. The naturally derived insecticide spinosad is highly toxic to Aedes and Anopheles mosquito larvae. Med Vet Entomol 18:50-56.

[7] Chen F, Al-Ahmad H, Joyce B, Zhao N, Kollner TG, Degenhardt J, Stewart Jr. CN 2009 Within-plant distribution and emission of sesquiterpenes from Copaifera officinalis. Plant Physiol and Biochem 47:1017-1023.

[8] Consoli RAGB, Oliveira RL 1994. Principais mosquitos de importância sanitária no Brasil. Rio de Janeiro, RJ, Brasil.

[9] Deus RJA, Alves CN, Arruda MSP 2011. Avaliação do efeito antifúngico do óleo resina e do óleo essencial de copaíba (Copaifera multijuga Hayne). Rev Bras Pl Med 13:1-7.

[10] Geris R, Silva IG, Silva HHG, Barison A, Rodrigues-Filho E, Ferreira AG 2008. Diterpenoids from Copaifera reticulata Ducke with larvicidal activity against Aedes aegypti (L.) (Diptera, Culicidae). Rev Inst Med Trop S Paulo 50:25-28.

[11] Gil LHS, Alves FP, Zieler H, Salcedo JMV, Durlacher RR, Cunha RPA, Tada MS, Camargo LMA, Camargo EP, Pereira-Da-Silva LH 2003. Seasonal malaria transmission and variation of anopheline density in two distinct endemic areas in Brazilian Amazônia. J Med Entomol 40:636-641.

[12] Hemingway J, Ranson H 2000. Insecticide resistance in insect vectors of human disease. Annu Rev Entomol 45:371-391.

[13] Josepha CC, Ndoilea MM, Malimab RC, Nkunyaa MHH 2004. Larvicidal and mosquitocidal extracts, a coumarin, isoflavonoids and pterocarpans from Neorautanenia mitis. Trans of the Roy Soc Trop Med Hyg 98:451-455.

[14] Kanis LA, Prophiro JS, Vieira ES, Nascimento MP, Zepon KM, Kulkamp-Guerreiro IC, Silva OS 2011. Larvicidal activity of Copaifera sp. (Leguminosae) oleoresin microcapsules against Aedes aegypti (Diptera: Culicidae) larvae. Parasitol Res 110:1173-117.

[15] Langenheim JH 1990. Plant resins. Americ Scient 78:16-24.

[16] Lawrence BM 1980. Progress in essential oil: Natural Flavor and Fragance. Materials 5:32.

[17] Leandro LM, Vargas FS, Barbosa PCS, Neves JKO, Silva JA, Veiga-Junior VF 2012. Chemistry and biological activities of terpenoids from Copaiba (Copaifera spp.) oleoresins. Molecules 17:3866-3889.

[18] Lima EP, Paiva MHS, Araújo AP, Silva EVG, Silva UM, Oliveira LN, Santana AEG, Barbosa CN, Neto CCP, Goulart MOF, Wilding CS, Ayres CFJ, Santos MAVM 2011. Insecticide resistance in Aedes aegypti populations from Ceará, Brazil. Paras & Vectors 4:1-12.

[19] Oliveira ECP, Lameira AO, Zoghbi MGB 2006. Identificação da época de coleta do óleo-resina de copaíba (Copaifera spp.) no município de Moju, PA. Rev Bras Pl Med 8:14-23.

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[25] Valotto CFB, Silva HHG, Cavasin G, Geris R, Filho ER, Silva IG 2011. Alterações ultraestruturais em larvas de Aedes aegypti submetidas ao diterpeno labdano, isolado de Copaifera reticulata (Leguminosae), e a uma fração rica em taninos de Magonia pubescens (Sapindaceae). Rev Soc Bras de Med Trop 44:194-200.

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[27] WHO 2005. Guidelines for laboratory and field testing of mosquito larvicidas. World Health Organization Technical Report Series. Geneva.

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