A New Diterpene Extracted from Daphne Mucronata, Effects on Human K562 and CCRF-CEM Cell Lines ()
1. Introduction
Various Daphne species (Tymelaeaceae) have been used to treat cancer since 200 AD [1-4]. There are so many reports on effects of Tymelaeaceae family in different parts of body, for example their; anti leukemia [5], emergency abortion [6], anti tumor [7], anti gout [8], anti microbial [9] and anti inflammatory [10] effects of Tymelaeaceae family [11,12].We reported inhibition of nucleic acid synthesis [13], inhibition of cell adhesion [14], and anti rat breast adenocarcinoma effect [15] of Daphne mucronata and Dendrostellera lessertii [16] in Iranian folk medicine. Therefore, as part of our studies on plants for new anticancer agents with emphasis on Tymelaeaceae family, we examined the cytotoxicity and anti-tumor activity of an alcohol: water (1:1, v/v) extract of Daphne mucronata leaves and one of its purified diterpene (Gnidilatimonoein) against two types of human leukemia cell lines. After exploring the high anti-tumor activity of plant extract, and its purified compound on human leukemia cell lines, we evaluated the mode of action of this anti-cancer plant. In that respect, we investigated the effects of the plant extract, and the purified component, and Taxol (an antineoplastic natural agent from the bark of the Pacific yew tree and with established mechanism of action) on the TNF-α secretion by the isolated human monocytes in the absence or the presence of LPS. Based on the literature data, Taxol inhibits cell growth by two mechanisms of cell cycle dependent and independent pathways. In cell cycle independent pathway, it rapidly down-regulates TNF-α receptors and stimulates TNF-α release by the isolated human monocytes in a similar way to LPS [17-20]. Leukemia treatment is an important medical problem. So in this study we investigated the Daphne mucronata extract and its purified diterpene (Gnidilatimonoein) effects on the isolated healthy human monocytes and the co-culture of human monocytes and two, chronic and acute, leukemia cell lines in the presence and absence of LPS as monocytes stimulant.
2. Materials & Methods
Human tumor necrosis factor alpha (TNF-α), Salmonella typhimurium LPS, RPMI 1640, Neomycin, Penicillin and other chemicals was purchased from Sigma Chemical Co. (Sigma-Aldrich Chime GmbH, Germany). Radioactive NaI125 was obtained from Atomic Energy Agency of Iran. Human leukopakes of normal donors were obtained from Blood Transfer Institute of Iran. Human leukemia cell lines, K562 (Chronic Mylocytic Leukemia), CCRF-CEM (Acute Lymphocytic Leukemia) were obtained from Iranian Cell Bank.
2.1. Plant Material
Aerial parts of Daphne mucronata (Magnoliopsida, Malvales, Thymelaeaceae, Daphne, mucronata) were collected from suburb of Kermanshah province at the end of spring. A voucher specimen was deposited in the herbarium of the faculty of Science, Tehran University (7658 THE). The plant material was dried, in the absence of direct light. The dried leaves were separated from the stems and powdered. The powder was kept in a closed container in a cold room.
2.2. Extraction
Extract solution was made with 500 g of powder in 7.5 liter of the solvent mixture and finally was concentrated to 500 mL. Briefly, each 100 gram of the powder extracted with 3 × 500 mL of EtOH-H2O (50:50, v/v), placed under agitation during 24 h. After filtration, the extracts are concentrated with a rotary evaporator, under reduced pressure, finally kept at freezer (–20˚C) for further investigation [21-23].
2.3. Purification
On the basis of Yazdanparast and her coworkers’ method, its active diterpene (Gnidilatimonoein) extracted and purified [24].
2.4. LC50 Estimation
The biological potency of plant extract was established through using brine shrimp (Artemia Solina) test as described by Mclaughlin and coworker [25]. Different amount of extract were transferred to sample vials containing 10 shrimps, 5 mL with sea water and a drop of dry yeast suspension (3 mg/mL). The vials were kept under the light and in the room temperature. After 24 hours the survivors were counted and their death percentage were determined at each dose. In the case of death in the controlled vials, the data were corrected by using the following formula: % death = [(test –control)]/ control 100 The LC50 were determined for each dose by using the probity analysis method which described by Finney [26].
2.5. Monocytes Isolation
Human monocytes were isolated from leukopakes by Cell adherence separation method. Briefly, cells were washed twice with Phosphate Buffer Saline (PBS), counted and suspended in the culture media at a final concentration of 5 × 106 cells/mL. After two hours of incubation at 37˚C in an incubator with 5% CO2 atmosphere, the non adherent cells were removed aseptically followed by 3-4 times of washing with cold PBS. The adherent cells were gently scraped with a rubber policeman in the presence of PBS/EDTA solution. The cells were finally re-suspended in the culture media at a concentration of 5 × 105 cells/mL [27].
2.6. Cell Cultures and Treatments with Stimuli
A total of 106 cells were incubated in duplicate, in 24- well plate. Each well contained the medium (RPMI 1640 containing 10% BCF, 100 IU penicillin, plus 100 μg/mL of streptomycin). After 20 hours incubation the cells in incubator at 37˚C in a 5% CO2 atmosphere, various concentrations of Daphne mucronata extract and its purified diterpene were added to each well up to a final volume of 1mL. The cultures were incubated with the extract and purified diterpene for 24 hours at 37˚C in a 5% CO2 atmosphere. The stimuli (crude extract and purified diterpene) were: plant extract (0 mg/ml, 10 mg/ml, 20 mg/ml, 40 mg/ml, 80 mg/ml, and 160 mg/ml of a 1:100 dilution of the original plant extract with a concentration corresponding to 1 g plant leaves powder per mL), and its purified diterpene (0.94 nM), in the presence and absence of LPS (100 ng/mL). The effect was compared with Taxol (0, 5 μM, 10 μM, 20 μM and 40 μM) as a positive control.
2.7. Determination of hTNF-α
The hTNF-α level in the supernatant of each culture monocytes sample was achieved by our developed biotin-streptavidin enzyme immunoassay system [28]. Each sample supernatant (or the diluted sample 1:10) was added to a well of a 96 well plate (100 μL/well). The plate was incubated at room temperature for one hour on a plate shaker. After washing, 100 μL of biotinylated antibody was added to each well, incubated at room temperature for one hour on a plate shaker and rinsed with the wash buffer (PBS with 0.05% TWEEN 20). Then 100 μl of streptavidin-HRP conjugate was added to each well followed by 30 minutes of incubation at room temperature while shaking on the plate shaker. Finally the plate was washed and the color was developed by adding the substrate buffer solution containing TMB and H2O2 (100 μL/well). The reaction was stopped after 30 minutes by the addition of 100 μl of 1.8 M sulfuric acid. The optical density of each well was recorded at 450 nm in an ELISA plate reader (Spectra, Tecan, Austria). The levels of the TNF-α in each sample were established via the use of the corresponding calibration graph.
3. Results
Based on experiments carried out on shrimp test, biological potency of Daphne mucronata extract LC50 was 0.062 mg/ml plant leave and 0.3 mg mg/ml plant stem. The effects of Daphne mucronata extract and its purified diterpene (Gnidilatimonoein, MW 663) on acute and chronic leukemia cell lines are shown in Figure 1. These data clearly show that the purified component is biologically active. In the presence of the human monocytes, and under all identical conditions, cell viability decreased almost by a factor of four (Figure 2). In other words, the concentration of the plant extract or the purified component required a half reduction in cell number, decreased considerably and statistically significant for the crude extract and also for the purified component (Figure 2). Determination of TNF-α in the cell culture media of the co-culture revealed that under the effect of the plant extract and its purified active component (Figure 3) the concentration of TNF-α increase in a dose dependent way. It is interesting to note that the effects of the purified compound and LPS on TNF-α secretion by the monocytes are neither addition nor synergistic.
The results are presented as the mean ± SD of three independent experiments in duplicate.
Comparison between two groups was done with t-test and between groups according ANOVA test, (the significance consider for P ≤ 0.05).
4. Discussion
Tymelaeaceae family has been used to treat diseases from many years ago [2]. Daphne is the most important genus in the Tymelaeaceae family. There are many reports about Daphne therapeutic effects [5-8]. Daphne mucronata is specific to Iranian folk medicine. At first we reported the effects of its alcohol: water inhibition on nucleic acid synthesis and cell adhesion [13,14]. Our investigations showed that Daphne Mucronata extract has a decreasing effect on the size of breast adenocarcinoma in rats and stimulate TNF-α releasing from monocytes [15]. Taxol is an antineoplastic natural agent which extracted from the bark of the Pacific yew tree and established as an effective drug for many types of cancers [16-18]. Based on the literature data, Taxol inhibits cell growth by cell cycle independent pathway through mo-
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Figure 1. Daphne mucronata diluted (1:100) extract (a) and its diterpene (b) effect on leukemia cell viability, k562 (■), CCRF-CEM (▲).
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Figure 2. Daphne mucronata diluted (1:100) extract (a) and its diterpene (b) effect on leukemia cell viability, k562 (white), CCRF-CEM (black) in co culture with human monocytes.
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Figure 3. Daphne mucronata extract (a) and its diterpene (b) effect on TNF-a secretion in co culture of human monocytes and leukemia cell lines.
nocytes/macrophage TNF-α release stimulation [16,18]. On the basis of our reported data, alcohol: water extract of Daphne mucronata and its purified component showed similar effects on the isolated healthy human monocytes activation [15,29]. In this study after exploring the high anti-tumor activity of plant extract, and its purified diterpene (Gnidilatimonoein) on human leukemia cell lines, we evaluated the mode of action of this anticancer plant. In that respect, we investigated the effects of the plant extract, and the purified component, on TNF-α secretion by the isolated human monocytes in the absence or the presence of LPS. The co-culture of human monocytes and two, chronic and acute leukemia cell lines showed non additive and non synergistic properties between the plant extract and LPS. Based on these observations, it may be concluded that the higher sensitivity of K562 and CCRF-CEM cells to Daphne mucronata, in the co-culture samples, is most probably due to the secretion of TNF-α by the monocytes. We hope this diterpene, after evaluating its side effects; become an effective drug against human leukemia.
5. Acknowledgment
We are thankful to Endocrine Research Center of Shahid Beheshti University of Medical Sciences for providing the financial support of this investigation. The authors also wish to thank Prof. David L. Smith for providing the FAB/MS of the purified active components of D. mucronata.
Abbreviation List
Enzyme Linked Immunosorbent Assay (ELISA), Ethylene Diamine Tetra Acetic acid (EDTA), Lipopolysaccharide (LPS), Phosphate Buffer Saline (PBS), Roswell Park Memorial Institute (RPMI), Tumor Necrosis Factor alpha (TNF-a)