Plumbagin quantification in roots of Plumbago scandens L. obtained by different extraction techniques

Paiva, Selma R. de; Lima, Lucilene A.; Figueiredo, Maria Raquel; Kaplan, Maria Auxiliadora C.

doi:10.1590/S0001-37652004000300004

Abstracts

The Plumbago genus belongs to the Plumbaginaceae family and it is known due to its variety of biological uses, most of them attributed to the presence of naphthoquinones. Plumbagin is a naturally occurring naphthoquinone that can be obtained from roots of Plumbago scandens L. In order to find out the better technique for plumbagin extraction, were applied: static maceration, dynamic maceration, with assistance of ultrasonic waves and in Soxhlet apparatus. Four compounds were qualitatively detected in all extracts: the naphthoquinones plumbagin and epi-isoshinanolone, palmitic acid and sitosterol. Plumbagin was always the major component in all analyzed extracts and it was quantitatively determined by gas chromatograph coupled with mass spectrometer. Soxhlet was the most efficient extraction technique however, prolonged heating time promoted plumbagin degradation.

Plumbaginaceae; Plumbago scandens L.; plumbagin; extraction techniques

O gênero Plumbago pertence à família Plumbaginaceae e apresenta uma variedade de atividades biológicas, a maioria atribuída à presença de naftoquinonas. Plumbagina é uma naftoquinona natural que pode ser obtida a partir de raízes de Plumbago scandens L. Na tentativa de descobrir a melhor técnica de extração dessa substância foram usadas, maceração estática, maceração dinâmica, extração com auxílio de ultrassom e extração em Soxhlet. Quatro substâncias foram detectadas qualitativamente: as naftoquinonas plumbagina e epi-isoshinanolona, o ácido palmítico e o sitosterol. Plumbagina foi sempre o componente majoritário em todos os extratos analisados e sua determinação quantitativa foi realizada através de cromatografia com fase gasosa acoplada à espectrometria de massas. A extração em Soxhlet foi a técnica mais eficiente para obtenção de plumbagina, entretanto a longa exposição a temperaturas elevadas favoreceu a degradação da plumbagina.

Plumbaginaceae; Plumbago scandens L.; plumbagina; técnicas de extração

CHEMICAL SCIENCES

Plumbagin quantification in roots of Plumbago scandens L. obtained by different extraction techniques

Selma R. de Paiva^{I, II}; Lucilene A. Lima^I; Maria Raquel Figueiredo^I; Maria Auxiliadora C. Kaplan^III

^ILaboratório de Química de Produtos Naturais, Far-Manguinhos, Fiocruz, Rua Sizenando Nabuco 100, 21041-250 Rio de Janeiro, RJ, Brasil

^IIPrograma de Pós-Graduação em Biotecnologia Vegetal, UFRJ, 21941-900 Rio de Janeiro, RJ, Brasil

^IIINúcleo de Pesquisas de Produtos Naturais, UFRJ, 21941-900 Rio de Janeiro, RJ, Brasil

^{Correspondence} Correspondence to Selma Ribeiro de Paiva E-mail: s_paiva@far.fiocruz.br

ABSTRACT

The Plumbago genus belongs to the Plumbaginaceae family and it is known due to its variety of biological uses, most of them attributed to the presence of naphthoquinones. Plumbagin is a naturally occurring naphthoquinone that can be obtained from roots of Plumbago scandens L. In order to find out the better technique for plumbagin extraction, were applied: static maceration, dynamic maceration, with assistance of ultrasonic waves and in Soxhlet apparatus. Four compounds were qualitatively detected in all extracts: the naphthoquinones plumbagin and epi-isoshinanolone, palmitic acid and sitosterol. Plumbagin was always the major component in all analyzed extracts and it was quantitatively determined by gas chromatograph coupled with mass spectrometer. Soxhlet was the most efficient extraction technique however, prolonged heating time promoted plumbagin degradation.

Key words: Plumbaginaceae, Plumbago scandens L., plumbagin, extraction techniques.

RESUMO

O gênero Plumbago pertence à família Plumbaginaceae e apresenta uma variedade de atividades biológicas, a maioria atribuída à presença de naftoquinonas. Plumbagina é uma naftoquinona natural que pode ser obtida a partir de raízes de Plumbago scandens L. Na tentativa de descobrir a melhor técnica de extração dessa substância foram usadas, maceração estática, maceração dinâmica, extração com auxílio de ultrassom e extração em Soxhlet. Quatro substâncias foram detectadas qualitativamente: as naftoquinonas plumbagina e epi-isoshinanolona, o ácido palmítico e o sitosterol. Plumbagina foi sempre o componente majoritário em todos os extratos analisados e sua determinação quantitativa foi realizada através de cromatografia com fase gasosa acoplada à espectrometria de massas. A extração em Soxhlet foi a técnica mais eficiente para obtenção de plumbagina, entretanto a longa exposição a temperaturas elevadas favoreceu a degradação da plumbagina.

Palavras-chave: Plumbaginaceae, Plumbago scandens L., plumbagina, técnicas de extração.

INTRODUCTION

The plant kingdom represents an extraordinary resource of organic compounds. However, only few plants have been investigated chemically. The rapid disappearance of tropical forests has meant that it is essential to have access to methods which lead to the rapid isolation and identification of bioactive natural products and also minimize the amount of plant material used in a phytochemical study (Hostettmann et al. 1997).

Plumbago scandens L. (Plumbaginaceae) is a scandent subshrub distributed in America, native from Brazil. The chemical profile of the genus is marked by the presence of naphthoquinones, flavonoids and terpenoids (Paiva et al. 1995).

Quinones structurally encompass pigments, antibiotics, vitamin K and coenzymes. The last ones function in metabolism as one-electron transfer agents by virtue of their property to form reversible rather stable semiquinone radicals on reduction. Quinones biosynthesis is diversified, some types come from polyketide pathway, while others derived from shikimic acid route (Torssel 1983). These compounds represent a chemical defense for plants and have many known biological properties.

Plumbagin (2-methyl-5-hydroxy-1,4-naphthoquinone) (Figure 1) is a naturally occurring yellow pigment, produced by members of Plumbaginaceae, accumulated mostly in roots (Van der Vijver 1972).

Biological activities of crude plant extracts from different Plumbago species as well as of plumbagin have been studied exhaustively. Plumbagin showed anticancer (Melo et al. 1974), leishmanicidal (Chan-Bacab and Peña-Rodriguez 2001) and bactericidal (Durga et al. 1990) activities, being also effective against insects (Kubo et al. 1980, Ghosh et al. 1994).

Secondary metabolites concentration in plant organs can vary along the year and different extraction techniques may interfere quantitatively and qualitatively in the extract composition.

Conventional extraction methods with organic solvents, as maceration or hot extraction in Soxhlet apparatus, are widely used to obtain plant extracts. The amount of dried plant extract depends on the analytical technique that will be employed (Sargenti and Vichnewski 2000). Other parameters should be considered such as: type of solvent, the organic solvent volume, the temperature and the extractive process duration.

The objective of the present work was to find out the better extraction technique of the naphthoquinone plumbagin, in terms of efficiency.

MATERIALS AND METHODS

SOLVENTS

The solvents used (chloroform and ethyl acetate) were PA grade.

PLANT MATERIAL

Roots of Plumbago scandens L. were collected at Fundação Oswaldo Cruz campus, Rio de Janeiro State, Brazil. A voucher of this plant was deposited at Rio de Janeiro Botanical Garden Herbarium (RB) under the number 340.340.

EXTRACTS PREPARAT ION

Roots of P. scandens were oven dried at 40^°C and powdered (5 mm of particle diameter). The plant (9.5 g) was extracted with 300 ml of chloroform by different extraction techniques: static maceration (24h), dynamic maceration (10h + 14h of static maceration), extraction with aid of ultrasonic waves (2h) and extraction in the Soxhlet apparatus at different process duration (2h, 5h, 10h). Chloroform was employed as solvent for these extractions, once it was reported in literature for nafthoquinones extraction (Sidhu and Sankaram 1971, Zhong et al. 1984, Pakulski and Budzianowski 1996). All the solutions were evaporated to dryness under reduced pressure. The extraction efficiency was defined as follows:

INSTRUMENTS

Instrumentation consisted of an Agillent Technologies gas chromatograph model 6890N equipped with a mass selective detector, model 5973 and an automatic injector model 5683. Capilar column HP-5MS (5% phenyl, 95% methyl syloxan), 30 m × 0.25 mm × 0.25 mm. The data acquisition was performed by HP Chemistation Data Acquisition Software.

SAMPLE PREPARATION

A portion of the crude chloroform extracts (2 g each) was dissolved in ethyl acetate (1 ml), and injected into a gas chromatograph coupled with a mass spectrometer.

CHROMATOGRAPHIC CONDITIONS

The following conditions were used: helium as carrier gas, mass detector, detector temperature = 280^°C, injector temperature 270^°C, flow rate 1.0 ml/min, split of 1:20, injection volume = 1.0 ml, initial temperature = 120^°C and oven program from 5^°C/min to 290^°C followed by an isoterm period of 20 min.

STANDARD SOLUTIONS

For system calibration, individual stock solution of plumbagin (previously isolated from roots of P. scandens and identified by spectrometrical techniques) was prepared with ethyl acetate in volumetric flask. Known concentration aliquots of plumbagin (0.10; 0.50; 1.00; 1.50; 2.00; to 2.50 mg/ml) were used in order to have a standard curve (Figure 2).

RESULTS AND DISCUSSION

The efficiencies of plumbagin extraction by different techniques were compared. As expected, Soxhlet extraction was the most efficient technique (Figure 3). Its efficiency is due to the employment of a small volume of solvent which is continuously renewed in contact with the plant material, promoting more interactions between them.

Extractions in Soxhlet apparatus for 5 hours demonstrated a high efficiency, yielding almost 50% over the extract obtained in 2 hours of extraction. Comparatively 10 hours of extraction yielded approximately 8.5% more than the obtained in 5 hours.

A sample of each extract solution in ethyl acetate (2 mg/ml) was submitted to a gas chromatograph coupled with a mass spectrometer. The samples were submitted to a chromatographic fractionation twice in order to guarantee the fidelity of the experiment. None of the used extraction techniques showed qualitative change of the chemical composition, since the same compounds were identified in all extracts by GC/MS retention time and molecular fragmentation. The chromatograms and the spectral analysis demonstrated the presence of four main compounds identified as the naphthoquinone plumbagin, the naphthoquinone epi-isoshinanolone, palmitic acid and sitosterol (Figure 4). Plumbagin was always the major component, independent of the extraction technique. The variation profile of these compounds in different extraction techniques can be observed in Figure 5.

Plumbagin was isolated from roots of P. scandens and identified by comparison of its spectral data to those reported in the literature (Carvalho 1986). This compound can be dissolved in solvents with low and medium polarity and its melting point is at 74^°C. Its quantitative determination was carried out in all extracts. The results are described in Table I. The lowest level of this substance was observed in the extract obtained by static maceration (6.47%), while the highest content was verified in the Soxhlet extraction for 2, 5 and 10 hours (35.78; 57.65 and 50.27, respectively). However, the process duration of 10 hours demonstrated a decrease of 12.8% in the plumbagin content, suggesting its degradation under long exposition time to high temperature. It is interesting to point out the 30h time hot extraction reported by former researchers studying Plumbago species (Sankaram et al. 1976).

Thumbnail

The naphthoquinone plumbagin is a compound of great interest due to its biological properties. This work aimed to investigate the better extraction technique for this compound from plant material. Plumbagin can be isolated in large amounts, especially from roots of Plumbago species and represents an important target for new pharmacological tests. It could be concluded that the extraction in Soxhlet apparatus was optimal to reach high percentage extraction of plumbagin, however the process duration should not be so long over 5h, in order to maintain the better yield of plumbagin.

ACKNOWLEDGMENTS

The authors wish to thank the Analytical Center of Far-Manguinhos, Maria Beatriz S. Almeida, André Luis Zanela and Sergio Monteiro and the Brazilian Research National Council for Scientific and Technological Development (CNPq).

Manuscript received on February 2, 2003; accepted for publication on February 23, 2004;

contributed by MARIA AUXILIADORA C. KAPLAN^*

* Member of Academia Brasileira de Ciências

CARVALHO VR de. 1986. Epi-isoshinanolone from Plumbago scandens Phytochemistry 25: 764-765.
CHAN-BACAB MJ AND PEÑA-RODRIGUEZ LM. 2001. Plant natural products with leishmanicidal activity. Nat Prod Rep 18: 674-688.
DURGA R, SRIDHAR P AND POLASA H. 1990. Effects of plumbagin on antibiotic resistance in bacteria. Indian J Med Res 91: 18-20.
GHOSH D, SOM K, DINDA B AND CHEL G. 1994. Potentiality of plumbagin to Culex fatigans A growth inhibitor. J of Adv Zool 15: 112-115.
HOSTETTMANN K, WOLFENDER JL AND RODRIGUEZ S. 1997. Rapid detection and subsequent isolation of bioactive constituents of crude plant extracts. Planta Med 63: 2-10.
KUBO I, TANIGUCHI M, CHAPYA A AND TSUJIMOTO K. 1980. An insect antifeedant and anti-microbial agent from Plumbago capensis Planta Med (suppl.): 185-187.
MELO AM, JARDIM ML, SANTANA CF DE, LACET Y, FILHO JL, LIMA I AND LEONCIO OG. 1974. First observations on the topical use of primin, plumbagin and mayteni in patients with skin cancer. Rev Inst Antibiot 14: 9-16.
PAIVA SR DE, KAPLAN MAC AND GOTTLIEB OR. 1995. Systematic positioning of Plumbaginaceae. An Acad Bras Cienc 67: 461-466.
PAKULSKI G AND BUDZIANOWSKI J. 1996. Ellagic acid derivatives and naphthoquinones of Dionaea muscipula from in vitro cultures. Phytochemistry 4: 775-778.
SANKARAM AVB, SRIINIVASARAO A AND SIDHU GS. 1976. Chitranone - a new binaphthoquinone from Plumbago zeylanica Phytochemistry 15: 237-238.
SARGENTI SR AND VICHNEWSKI W. 2000. Sonication and Liquid Chromatography as a Rapid Technique for Extraction and Fractionation of Plant Material. Phytochem Anal 11: 69-73.
SIDHU GS AND SANKARAM AVB. 1971. New biplumbagin and 3-chloroplumbagin from Plumbago zeylanica Tetrahedron Lett 26: 2385-2388.
TORSSEL KBG. 1983. Natural Product Chemistry. A mechanistic and biosynthetic approach to secondary metabolism, London: John Wiley & Sons Ltd, 401p.
VAN DER VIJVER LM. 1972. Distribution of plumbagin in the Plumbaginaceae. Phytochemistry 11: 3247-3248.
ZHONG SM, WATERMAN PG AND JEFFREVS JAD. 1984. Naphthoquinones and triterpenes from african Diospyrus species. Phytochemistry 23: 1067-1072.

Correspondence to

Selma Ribeiro de Paiva

E-mail:

s_paiva@far.fiocruz.br

Publication Dates

Publication in this collection
23 Aug 2004
Date of issue
Sept 2004

History

Accepted
23 Feb 2004
Received
02 Feb 2003

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

[1] CARVALHO VR de. 1986. Epi-isoshinanolone from Plumbago scandens Phytochemistry 25: 764-765.

[2] CHAN-BACAB MJ AND PEÑA-RODRIGUEZ LM. 2001. Plant natural products with leishmanicidal activity. Nat Prod Rep 18: 674-688.

[3] DURGA R, SRIDHAR P AND POLASA H. 1990. Effects of plumbagin on antibiotic resistance in bacteria. Indian J Med Res 91: 18-20.

[4] GHOSH D, SOM K, DINDA B AND CHEL G. 1994. Potentiality of plumbagin to Culex fatigans A growth inhibitor. J of Adv Zool 15: 112-115.

[5] HOSTETTMANN K, WOLFENDER JL AND RODRIGUEZ S. 1997. Rapid detection and subsequent isolation of bioactive constituents of crude plant extracts. Planta Med 63: 2-10.

[6] KUBO I, TANIGUCHI M, CHAPYA A AND TSUJIMOTO K. 1980. An insect antifeedant and anti-microbial agent from Plumbago capensis Planta Med (suppl.): 185-187.

[7] MELO AM, JARDIM ML, SANTANA CF DE, LACET Y, FILHO JL, LIMA I AND LEONCIO OG. 1974. First observations on the topical use of primin, plumbagin and mayteni in patients with skin cancer. Rev Inst Antibiot 14: 9-16.

[8] PAIVA SR DE, KAPLAN MAC AND GOTTLIEB OR. 1995. Systematic positioning of Plumbaginaceae. An Acad Bras Cienc 67: 461-466.

[9] PAKULSKI G AND BUDZIANOWSKI J. 1996. Ellagic acid derivatives and naphthoquinones of Dionaea muscipula from in vitro cultures. Phytochemistry 4: 775-778.

[10] SANKARAM AVB, SRIINIVASARAO A AND SIDHU GS. 1976. Chitranone - a new binaphthoquinone from Plumbago zeylanica Phytochemistry 15: 237-238.

[11] SARGENTI SR AND VICHNEWSKI W. 2000. Sonication and Liquid Chromatography as a Rapid Technique for Extraction and Fractionation of Plant Material. Phytochem Anal 11: 69-73.

[12] SIDHU GS AND SANKARAM AVB. 1971. New biplumbagin and 3-chloroplumbagin from Plumbago zeylanica Tetrahedron Lett 26: 2385-2388.

[13] TORSSEL KBG. 1983. Natural Product Chemistry. A mechanistic and biosynthetic approach to secondary metabolism, London: John Wiley & Sons Ltd, 401p.

[14] VAN DER VIJVER LM. 1972. Distribution of plumbagin in the Plumbaginaceae. Phytochemistry 11: 3247-3248.

[15] ZHONG SM, WATERMAN PG AND JEFFREVS JAD. 1984. Naphthoquinones and triterpenes from african Diospyrus species. Phytochemistry 23: 1067-1072.