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Cytotoxic activity of marine algae against cancerous cells

Abstract

This paper presents an investigation on the cytotoxic activity in human tumor cell from dichloromethane, chloroform, methanol, ethanol, water extracts, and hexane and chloroform fractions from green, brown and red algae collected at Riacho Doce Beach, north coast of Alagoas, Brazil, against the cancer cells K562 (chronic myelocytic leukemia), HEp-2 (laryngeal epidermoid carcinoma) and NCI-H292 (human lung mucoepidermoid carcinoma) through the MTT colorimetric method. The dichloromethane extract and chloroform fraction of Hypnea musciformis showed the best cytotoxic activity against K562 (3.8±0.2 µg.mL-1 and 6.4±0.4 µg.mL-1, respectively). Dichloromethane extracts of Dictyota dichotoma (16.3±0.3 µg.mL-1) and the chloroform fraction of H. musciformis (6.0±0.03 µg.mL-1) and chloroform fraction of P. gymnospora (8.2±0.4) were more active against HEp-2 as well as ethanol extracts of P. gymnospora (15.9±2.8 µg.mL-1) and chloroform fraction of H. musciformis (15.0±1.3 µg.mL-1) against the cell NCI-H292. The constituents with higher anticancer action are present in the extracts of dichloromethane and chloroform and in the chloroform fraction of H. musciformis, Digenea simplex, P. gymnospora, and D.dichotoma. In the case of the seaweed S. vulgare, the anticancer constituents are present in the aqueous extract.

seaweed; cancerous cells; cytotoxicity; algae extract


Cytotoxic activity of marine algae against cancerous cells

Élica A. C. GuedesI; Teresinha G. da SilvaII; Jaciana S. AguiarII; Lurdiana D. de BarrosI; Laura M. Pinotti* * Correspondence: Laura Marina Pinotti. Departamento de Engenharias e Tecnologia, Universidade Federal do Espírito Santo. Rodovia BR 101 Norte, km 60, Bairro Litorâneo, 29.932-540. Tel.: 27 3312 1592, 27 3312 1510. laurapinotti@ceunes.ufes.br , III; Antonio E. G. Sant'AnaIV

IInstituto de Ciências Biológicas e da Saúde, Universidade Federal de Alagoas, Brazil,

IIDepartamento de Antibióticos, Universidade Federal de Pernambuco, Brazil,

IIIDepartamento de Engenharias e Tecnologia, Universidade Federal do Espírito Santo, Brazil

IVInstituto de Química e Biotecnologia, Universidade Federal de Alagoas, Brazil

ABSTRACT

This paper presents an investigation on the cytotoxic activity in human tumor cell from dichloromethane, chloroform, methanol, ethanol, water extracts, and hexane and chloroform fractions from green, brown and red algae collected at Riacho Doce Beach, north coast of Alagoas, Brazil, against the cancer cells K562 (chronic myelocytic leukemia), HEp-2 (laryngeal epidermoid carcinoma) and NCI-H292 (human lung mucoepidermoid carcinoma) through the MTT colorimetric method. The dichloromethane extract and chloroform fraction of Hypnea musciformis showed the best cytotoxic activity against K562 (3.8±0.2 µg.mL-1 and 6.4±0.4 µg.mL-1, respectively). Dichloromethane extracts of Dictyota dichotoma (16.3±0.3 µg.mL-1) and the chloroform fraction of H. musciformis (6.0±0.03 µg.mL-1) and chloroform fraction of P. gymnospora (8.2±0.4) were more active against HEp-2 as well as ethanol extracts of P. gymnospora (15.9±2.8 µg.mL-1) and chloroform fraction of H. musciformis (15.0±1.3 µg.mL-1) against the cell NCI-H292. The constituents with higher anticancer action are present in the extracts of dichloromethane and chloroform and in the chloroform fraction of H. musciformis, Digenea simplex, P. gymnospora, and D.dichotoma. In the case of the seaweed S. vulgare, the anticancer constituents are present in the aqueous extract.

Keywords: seaweed; cancerous cells; cytotoxicity; algae extract

Introduction

The quest for promising substances through rational selection of natural products as anticancer drugs source is an alternative subsidy to cancer treatment and have guided numerous research for new medicines (Magalhães, 2005). Algae, fungi, lichens, fungi and vascular plants are major sources for the research of new bioactive molecules through the direct use of secondary metabolites or biosynthesis-derived compounds produced in order to increase effectiveness and absorption or to decrease toxicity (Hostettman et al., 1997).

Extensive researches on the cellular and molecular basis of the carcinogenesis cascade provides a targeted approach for cancer chemoprevention, which aims to halt or reverse the development and progression of precancerous cells through use of non cytotoxic doses of nutrients and/or pharmacological agents (Theisen, 2001; Gamal-Eldeen et al., 2009). The HEp-2 cell (American Type Culture Collection CCL-23), a tumor cell strain derived from human larynx carcinoma grown in monolayers on glass slides, has proved to be an excellent medium for self-antigens provision in the IIF-ANAtest (antinuclear antibody-immunofluorescence) since 1980. This HEp-2 cell virtually replaced cuts or rodents' liver imprint in clinical laboratories throughout the world due to its excellent visibility and easy handling for cell culture compared to the maintenance of animal facilities suitable for laboratory breeding routine (Dellavance & Andrade, 2011). NCI-H292 cells correspond to a continuous strain of mucoepidermoid cells obtained from human lung carcinoma, which has been used for isolation and propagation of Paramyxo virus humano (Morier et al., 1996). The K562 strain is Ph+erythroleukemic, widely used as a model for studying drugs with anti-proliferative capacity and/or inductors of fetal hemoglobin synthesis (Lozzio & Lozzio 1975).

Anti-tumor cytotoxic substances from marine organisms have been reported over the past 40 years (Ibrahim et al., 2005). Marine organisms are important and promising resources in cancer research and a number of compounds from these organisms have undergone clinical trials as antitumor agents. Shoeib et al. (2004) screened for in-vitro cytotoxic activities using DLD-1 cells of methanolic extracts of 33 species of British marine algae. The methanolic extract of Polysiphonia lanosa was the only one found to have an IC50 value of less than 50 µg.mL-1, and its chloroform fraction was found to be significantly more active than the parent methanolic extract. P. lanosa is rich in brominated phenolic compounds.

Harada & Kamei (1997) selected, among 306 seaweed species, those with in vitro cytotoxic potential against L1210 leukemic cells, observing that only seventeen were active. The methanol extract of Amphiroa zonata (IC50 20 µg.mL-1) was more efficient against strains of human leukemic cells (L1210 and K562). Testing eight alga species in China with potential antitumor activity, Xu et al (2004) found that chloroform and ethanol extracts from Polysiphonia urcedata, the ethanolic from Scytosiphon lomentarius and hexane from Dictyopteris divaricata showed cytotoxic activity against human oral epidermoid carcinoma (KB). Substances isolated from algae, such as fucoidan, laminaran and terpenoids have activity against cancer cell strains (Gerwick & Bernart 1993; Synytsya et al., 2010) and the search for new drugs from these organisms is crescent. In order to be considered effective in treating cancer, it is necessary to a drug have a selective antitumor activity without side effects (Xu et al., 2004). Jolles et al. (1963) were the first researchers to report the influence of a sulphated degraded laminarin obtained from seaweed extract in inhibiting the growth of tumor cells.

The use of cells as a tool of biological processes has been stimulated, since several research lines can be addressed such as: gene expression, proliferation, cell-cell interaction, adhesion and carcinogenesis (Perez & Curi, 2005).

This paper presents a study on the screening of some green, brown and red alga species from Riacho Doce beach, Alagoas, Brazil, by evaluating the in vitro cytotoxic potential of extracts and fractions of these organisms on three cancer cell strains: NCI-H292 (human lung cancer), Hep-2 (human larynx epidermoid carcinoma) and K562 (chronic myelocytic leukemia).

Materials and Methods

Biological material

Algae were manually collected from the Riacho Doce beach, (9° 34 '0 "S and 35 ° 39' 0" W) during low tide period between October 2007 to July 2009. The collected samples were immediately transported to the Phycology Laboratory of the Biological Sciences Institute, Universidade Federal de Alagoas. Nine species of algae from three divisions were used for this study: Chlorophyta-Ulva lactuca Linnaeus-MAC51238, Phaeophyta- Dictyota dichotoma (Hudson) J.V.Lamouroux-MAC51230; Padina gymnospora (Kutzing) Sonder-MAC51235 Sargassum vulgare C. Agardh- MAC 51236 and Rhodophyta- Gracilaria caudata J. Agardh - MAC51232, Hypnea musciformis (Wulfen) J.V. Lamouroux-MAC51234, Galaxaura rugosa (J. Ellis & Solander) J.V. Lamouroux-MAC51239; Gellidium pusillum (J.Stackhouse) Le Jolis-MAC51233, Digena simplex (Wulfen) C. Agardh-MAC51231). The voucher of respected species were deposited in the MAC Herbarium, Environment Institute of the city of Maceió, Alagoas, as internal reference material.

Extracts obtainment

Algae were washed with distilled water, dried in air-circulating ovens (Blue Mod1401440SC, USA) at 45 °C for 5 h and crushed in industrial blender (type TA-2 METVISA model, Brazil). The dried and ground material from each collection and each alga was mixed in equal amounts to dilute any possible seasonal difference in chemical extracts to be obtained. To obtain crude extracts, 500 g samples of dried seaweed were suspended in 1000 mL dichloromethane, chloroform, methanol, ethanol and water and macerated for 72 h with three repetitions. Organic extracts were filtered and roto-evaporated (Rotevaporator Buchii Heating Bath-B490, Switzerland) at 25 and 40 °C, except for the aqueous extract that was lyophilized (Edwards High Vacuum Lyophilizer, ModE2MB, Brazil). The mass from these extracts was measured and stored under refrigeration for subsequent cytotoxicity assays. Dichloromethane extracts from H. musciformis and P. gymnospora were selected for fractionation by having higher yields: 11.86 g (2.58%) and 13.96 g (3.04%), respectively. For fractionation by liquid-liquid partition, crude extracts of H. musciformis (2.73 g) and P. gymnospora (1.90 g) were suspended in methanol:water (3:1) and extracted with hexane and chloroform respectively, resulting in hexane and chloroform fractions to test for cytotoxic activities. All solvents used were VETEC-Quimica Fina (RJ-Brazil).

Cytotoxic activity in vitro

Cell strains K562 (Human chronic myelocytic leukemia), NCI-H292 (Human lungmucoepidermoid carcinoma), HEp-2 (Human larynx epidermoid carcinoma) were all obtained from Cell Bank in Rio de Janeiro (Rio de Janeiro, Brazil). Cells were maintained in DMEM GIBCO® supplemented with 10% fetal bovine serum, 2mM glutamine, 100 U.mL-1 penicillin, 100 µg.mL-1 streptomycin at 37 °C with 5% CO2 (Eagle, 1955).

Cells suspension of 1x105 cells/mL (HEp-2 e NCI-H292) and 0.3x106 cells/mL (K562) were distributed in 96-well plates and incubated at 37 °C in a wet atmosphere (5% CO2) for 24 h. After 24 h, extracts (6.25, 12.50, 25.0 and 50 µg.mL-1) dissolved in DMSO were added to each well and incubated for 72 h. Control groups received DMSO. Etoposide (1.25 - 20 µg.mL-1) was used as positive control. The growth of tumor cells was quantified by the ability of living cells to reduce yellow tetrazolium MTT (3-(4, 5-dimethylthiazolyl-2)-2, 5-diphenyltetrazolium bromide) to a blue formazan product (Mosmann 1983; Alley et al 1988). At the end of 72 h incubation, the plate was added with MTT (5.0 mg.mL-1). Three hours later, for suspended cells and two for adherent cells, the formazan product of MTT reduction was dissolved in DMSO and absorbance was measured using a multi-plate reader. The drug effect was quantified as percentage of control absorbance of reduced dye at 450 nm (Multiplate Reader Thermoplate-Mod TP_Reader). Results were expressed as mean percentage of growth inhibition in 50% of cell population (IC50 growth inhibition) (GI)%±SD).

Results and Discussion

The cytotoxic activity of 48 samples of crude algae extracts and its fractions on human cancer cell strains is presented in table 1. The evaluation was conducted in accordance with the Protocol of the American Cancer Institute (NCI), which recommends that IC50 values < 30µg.mL-1 should be considered significant for crude extracts of plant origin as well as IC50 values < 4µg.mL-1 for pure substances (Geran et al., 1972). This paper presents the preliminary studies on the effect of crude extracts and fractions of different algal species from the coast of Alagoas on different cancer cell strains, emphasizing that 55.17% of species showed cytotoxic activity, when utilized the method MTT.

Ethanol extracts of H. musciformis (22.0±3.5 µg.mL-1), P. gymnospora (15.9±2.8 µg.mL-1), D. dichotoma (22.7±4.2 µg.mL-1) and chloroform extracts of D. dichotoma (25.2±1.1 µg.mL-1) showed selectivity towards NCI-H292 cells. Regarding HEp-2 cells, the dichloromethane extract (16.3±0.3 µg.mL-1), chloroform extract (18.2±0.3) and extract methanolic (20.6±0.7 µgmL-1) of D. dichotoma were active against these cells. Cytotoxicity showed by Dictyota may be due to the presence of diterpenes common to Dictyotaceae family, which shows activity against tumor cells (Gedara et al., 2003).

Extracts that showed cytotoxic activity against K562 cells were obtained with dichloromethane (3.8±0.2 µg.mL-1) and chloroform (17.4±1.1 µg.mL-1) of H. musciformis. Dichloromethane (14.9±0.7 µg.mL-1) and chloroform (15.5±0.7 µg.mL-1) extracts of P. gymnospora and dichloromethane extract of D. dichotoma (14.4±0.7 µg.mL-1) were also active for K562 cells. Ktari & Guyot (1999) evaluated the cytotoxic activity of dichloromethane extract of Padina pavonica against KB cells and the results showed significant activity (IC50 10µg.mL-1). In our study, chloroform fraction of the dichloromethane extract of P. gymnospora showed similar value to that found by these authors for K562 (IC50 11.0 µg.mL-1) and HEp-2 (IC50 8.2 µg.mL-1) cells. Abourriche et al. (1999) determined the cytotoxic activity (20 µg.mL-1) of dichloromethane extract of Cystoseira tamariscifolia collected in Morocco (Mexico) which inhibited 30% KB cells. Cytotoxicity results obtained with the chloroform fraction of dichloromethane extract of H. musciformis were significant for all three tested cell strains: NCI-H292 (IC50 15.0±1.3 µg.mL-1), HEp-2 (IC50 6.0±0.3 µg.mL-1) and K562 (IC50 6.4±0.4 µg.mL-1) suggesting the existence of specific secondary metabolites that can interfere with cellular mitosis (Moo-Puc et al., 2009). The chloroform fraction of P. gymnospora also showed significant values against NCI-H292 (IC50 20.9±1.1 µg.mL-1), HEp-2 (IC50 8.2±0.4 µg.mL-1) and K562 (IC50 11.0±0.6 µg.mL-1). Shoeib et al. (2004), evaluating the in vitro cytotoxic activity of the red alga Polysiphonia lanosa against DLD-1 and HCT-116 cells (human colon carcinoma) showed that the chloroform fraction yielded better results than the methanol extract, which was also observed in our study regarding chloroform fraction of H. musciformis against HEp-2 cells (IC50 6.0±0.3 µg.mL-1). Some evidence has suggested that phenolic compounds inhibit telomerase activity in tumor cells (Naasani et al., 1998; Chakraborty et al., 2006). In most tumors the maintenance of telomeres occurs with the telomerase expression (Akiyama et al., 2002). Moo-Puc et al. (2009) performed a test to evaluate the effect of aqueous and organic (dichloromethane:methanol-7:3) extracts of 27 algal species on three human cancer cell strains (Hep-2, KB and HeLa) and found that most of cytotoxic extracts were organic and from species belonging to Chlorophyta (Udotea flabellum 22.5 µg.mL-1±1.2 and ±1.4 U. conglutinate 22.2 µg.mL-1) and Rhopdophyta (Bryothamnion triquetrum 8.2±1.3µg.mL-1) divisions against Hep-2 cells and Phaeophyta division (Lobophora vairegata 26.2 µg.mL-1±1.3 ±1.2 and Dictyota caribaea 27.9 µg.mL-1) that showed cytotoxic activity against KB strains. Taskin et al. (2010) investigated the antitumor activity of Padina pavonica and H. musciformis against breast cancer cells (MCF-7) and several strains of prostate cancer (DU-145, LNCaP and PC3) by in vitro cytotoxicity assay with methanolic extract and found that crude extracts of H. musciformis at 100 µg.mL-1 had low toxicity against cell strains tested. In this study, methanolic extract of H. musciformis also showed no cytotoxic activity against cell strains tested; however, it showed promising cytotoxicity for dichloromethane, chloroform and ethanol extracts. Concerning to aqueous extracts, only S. vulgare showed activity (IC50 18.7±3.8 µg.mL-1) thus considering that organic extracts have different constituents in comparison with hydrophilic ones, which have permeability with respect to cell membrane, partly explaining the limited effects of aqueous extracts on cancer cells (Moo-Puc et al., 2009). Wang et al. (2008) tested for proliferative potential of aqueous extract of twelve algae species from Hong Kong in HL-60 cells (promyelocytic leukemia) and MCF-7 (breast cancer) and found that Hydroclathrus clathratus and Padina arborescens inhibited their growth being also less toxic to normal cells. The extract that showed increased cytotoxic activity in this study was dichloromethane of H. musciformis (IC50 3.8±0.2 µg.mL-1) against K562 cells which is higher than the etoposid control. H. musciformis, D. simplex, P. gymnospora, S. vulgare and D. dichotoma were among species considered promising by IC50 values <30 obtained from different extracts.

Although the metabolites responsible for the antiproliferative action of algae species studied have not been chemically characterized in this study, the data suggest the occurrence of several secondary compounds with low polarity which are spread more easily in cell membranes than the more polar (Moo-Puc et al., 2009; 2011) once the crude extracts of dichloromethane, ethanol and chloroform fraction concentrated the substances responsible for the most significant cytotoxic activity.

Authors' contributions

EACG and LDB contributed in collecting plant sample and identification, confection of herbarium, running the laboratory work, analysis of the data and drafted the paper. EACG, JSA (PhD student) and TGS contributed to biological studies. LMP contributed to analysis of the data, drafted the paper and to critical reading of the manuscript. AEGS'A designed the study, supervised the laboratory work and contributed to critical reading of the manuscript. All the authors have read the final manuscript and approved the submission.

Received 25 Jun 2013

Accepted 19 Aug 2013

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  • *
    Correspondence: Laura Marina Pinotti. Departamento de Engenharias e Tecnologia, Universidade Federal do Espírito Santo. Rodovia BR 101 Norte, km 60, Bairro Litorâneo, 29.932-540. Tel.: 27 3312 1592, 27 3312 1510.
  • Publication Dates

    • Publication in this collection
      13 Sept 2013
    • Date of issue
      Aug 2013

    History

    • Received
      25 June 2013
    • Accepted
      19 Aug 2013
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