Introduction
Cancer metastasis consists of a complex cascade of events, which ultimately allow for tumor cell escape and seeding of ectopic environments [28]. Metastasis is a sequential process in which tumor cells detach from the primary growth, invade through the surrounding host tissue into the circulation and subsequently disseminate to distant organs, where they arrest, extravasate and proliferate to form metastatic foci [1]. Melanoma is the most aggressive form of skin cancer with high metastatic potential and extraordinary resistance to cytotoxic agents [24, 26]. Despite recent advances, the results of chemotherapy for patients with metastatic melanoma remain inadequate because of the relative drug resistance of metastatic cells.
Garlic (Allium sativum) has been used as a spice and an ingredient in folk medicine since ancient times [22, 25]. There have been many literature reports of epidemiological studies indicating that a garlic-rich diet decreases risk of some cancers such as gastric, stomach, and colon in vitro [6, 29] and the growth of transitional cell carcinoma xenografts [14, 19]. Recent studies in our team have revealed that a garlic-extracts or derived compounds are effective in suppressing metastasis [9, 16, 20], proliferation of cancer cells [8, 10, 21], sepsis [13] and inflammation [11, 12, 17]. Several individual compounds have been isolated from garlic and two major groups of compounds that show active anticancer effects have been identified [5, 8, 24]. One group is the lipid-soluble allyl sulfur compounds, and the other one is the water-soluble compounds [5, 24]. It is still unclear which compounds in garlic has positive role in the prevention of cancers.
Despite the abundant in vitro evidence for anti-cancer and anti-metastatic effect of garlic extract or its compounds is not well studied. In this study, we provide novel anti-metastatic activity from hexane fractions of dried garlic.
Materials and Methods
Animals
C57BL/6 female mice, 6-7 weeks old were purchased from Samtako (Osan-shi, Kyunggi-do, South Korea) and housed in polycarbonate cages under laboratory conditions with a 12 hr day-night cycle, room temperature of 22±2℃ and humidity of 50-60%. They were fed standard pelleted rats chow and had free access to water during the experiment. The animal experiments were approved by the Pusan National University, Institutional Animal Care and Use Committee (PNU-2010-000102).
Tumor cell line
B16F10 cells were obtained from Korean Cell Line Bank in Seoul, South Korea, maintained in RPMI-1640 medium supplemented with 10% FBS, antibiotics (100 U/ml penicillin G, 100 μg/ml streptomycin), in an incubator at 37℃ with a humidified atmosphere at 5% CO2 concentration. When needed for experiments the cells were harvested with trypsin:EDTA (0.05:0.03[w/v]) solution, and then washed in phosphate-buffered saline (PBS, pH 7.4). For the animal experiments, the recovered cells were adjusted to 1×106 cells/ml in PBS and then 100 μl of the suspension was injected into the tail-vein.
Anti-metastasis study of GHE in B16F10 cell implanted C57BL/6 mice
GHE was suspended in olive oil to the desired concentration (50, 100, 200 mg/kg body weight/2 interval day). For the studies, the GHE was administered orally (OA) starting on the day the B16F10 tumor cells were injected (1×106cells in 0.1 ml) by tail vein and there after the GHE was given for 21 days by OA.
Experimental groups for metastasis
C57BL/6 mice were divided into 6 groups of 10 mice each to carry out the level of GHE present in lung tumor bearing mice model. B16F10 cell line was injected (1×106 cells in 0.1 ml) by tail vein to groups III, IV, V and VI. GHE was given for respective group at a dose of 50, 100 and 200 mg/kg/body weight/day for 21 days after cell line implantation.
Group I : Controls animal (Olive oil alone administrated orally for 10 alternative days). Group II: Drug control (GHE-200 mg/Kg in olive oil administrated orally for 10 alternative days). Group III: Tumor alone (Olive oil alone administrated orally for 10 alternative days). Group IV: Tumor induced+GHE-50 mg/Kg in olive oil administrated orally for 10 alternative days. Group V: Tumor induced+GHE-100 mg/Kg in olive oil administrated orally for 10 alternative days. Group VI: Tumor induced+GHE-200 mg/Kg in olive oil administrated orally for 10 alternative days.
Pulmonary colonization assay
For in vivo experimental pulmonary metastasis assays, mice were injected with 1×106 B16F10 melanoma cells through the lateral tail vein. One day after tumor induction, GHE in olive oil at different concentrations were orally administrated for 10 alternative days. Whereas the tumor control mice were treated with the vehicle olive oil. The animals were sacrificed after 21 days of tumor induction, lungs were excised and metastatic colonies in lung were counted. Percentage of inhibition was calculated by the formula [(Control -Treated)/Control] ×100.
Statistical analysis
Results were provided as mean ± SE for each condition and statistically analyzed by the Student - Newman - Keuls test. p<0.05 was considered statistically significant.
Results
The effect of GHE on inhibition of lung cancer was assessed by counting the number of lung tumor colony formed in the respective groups as given in Table 1. The lungs of GHE-treated mice showed less number of tumor colonies (35.2±11.52) compared to those mice. Metastastic tumor bearing mouse treated with GHE showed significant reduction on tumor colony formation in a dose dependent manner (Fig. 1, Fig. 2). Untreated control animals developed a massive number of tumor colonies (97.4±30.2) in the lung. Lung metastasis frequency was significantly reduced by 6.93, 46.80 and 50.53% in mice treated with 50, 100 and 200 mg/kg of GHE, respectively (Fig. 3). In comparison with control, reduction of lung weight also noticed in mice treated with GHE at dose-dependent manner (Table 1).
Table 1.B16F10 melanoma cells (1×106 cells/mice) were injected to the lateral tail vein of mice. After GHE treatment for 10 alternative days animals were sacrifice and lung nodule were counted. Values are mean ± standard error, n=10.
FIG. 1.Effect of GHE on B16F10 lung metastasis. Mice injected with B16F10 cells were orally administrated either with GHE at different concentration and olive oil. After treatment of 10 alternative days lung were excised and tumor colonies were counted.
Fig. 2.Effect of GHE on formation of metastatic foci in lung of mice injected with B16F10 cells. B16F10 melanoma cells (1×106 cells/mice) were injected through the lateral tail vein of mice. After GHE treatment for 10 alternative days animals were sacrifice and lung nodule were counted. Values are mean ± standard deviation, n=10. Comparisons between control and treatment groups were performed by Student-Newman-Keuls test. p values **<0.01, *<0.05.
Fig. 3.Inhibitory effect of GHE on lung metastasis induced by B16F10 cells. Values are mean ± standard deviation, n=10. Comparisons between control and treatment groups were performed by Student-Newman-Keuls test. p values **<0.01, *<0.05.
Metastasis remains to be the major cause of death in cancer patients and it has critical importance in cancer therapy. Some drugs used for metastasis therapy have low efficiency, low response rate and it also produce a number of side effects. In the present study we investigate the anti-metastatic effect of garlic hexane extract on lung metastasis induced by B16F10 melanoma cell in experimental mice. GHE extracted from garlic showed that it could significantly abrogate the metastatic formation of nodules in lung by dose-dependent manner (Fig. 1, Fig. 2). More than 100 mg/kg garlic extract exert maximum anti-metastatic effect with 56% (Fig. 3). Though GHE showed inhibition of metastasis, this study opens ups further investigation on mode of action behind this effect.
Discussion
Melanoma is the most aggressive form of skin cancer with high metastatic potential and extraordinary resistance to cytotoxic agents. Despite recent advances, the results of chemotherapy for patients with metastatic melanoma remain inadequate because of the relative drug resistance of metastatic cells. Metastasis is a sequential process in which tumor cells detach from the primary growth, invade through the surrounding host tissue into the circulation and subsequently disseminate to distant organs, where they arrest, extravasate and proliferate to form metastatic foci [1]. Metastasis covers 90% of causality of cancer patients’ death [4] indicating that anti-metastatic agents are required for efficient cancer therapy. Consequently, identification of novel agents that are nontoxic but can delay onset and/or progression of cancer is highly desirable. Natural products have received increasing attention in recent years for the discovery of novel cancer preventive and therapeutic agents [15].
Many in vitro and animal studies have reported a relation between garlic intake supplementation and risk cancer prevention [18, 24]. Recent studies have provided evidence that sarcoma cell migration was inhibited by aged garlic extract [7] and different garlic extracts [9]. However, it is still ambiguous by which agents suppress metastasis of cancer cells from garlic extracts. In the present study, to screen the novel anti-metastasis compound from garlic, we prepared different extracts of garlic such as raw garlic and black garlic. During this process, hexane extract provide novel activity which suppresses the migration of cancer cells [9] and the proliferation of cancer cells [9], and garlic constituent sulfur [16], various solvent extracts were highly effective in suppressing growth of cancer cells in intro [10].
Several other research studies stated the establishment of the experimental lung metastasis model or pulmonary metastatic model by intravenously injected mouse melanoma B16F10 in C57BL/6 mice [3, 27]. The B16F10 mouse melanoma cell line was chosen on the basis of its high metastatic potential in this study. Specifically, the B16F10 line has been shown to metastasize to the lungs when injected into the lateral tail vein and the majority of cells find themselves in the pulmonary tissue, but some are also localized in other organs [2] and is accepted as useful model for the study of lung metastasis [23]. We showed that the mice received B16F10 cells only implanted, the melanoma cells quite well and the lungs of these hosts were visibly riddled with metastatic tumor nodules within 21 days (Fig. 1). Using C57BL/6 model mouse, we demonstrated that GHE could inhibit the colony forming rate of melanoma cells in dosedependent manners (Fig. 3). Moreover, GHE significantly inhibited the colony-forming ability of melanoma cells. In conclusion, the results of the present study indicate that oral administration of GHE prevents development of melanoma carcinoma and multiplicity of pulmonary metastatic lesions in C57BL/6 mice without causing weight loss.
참고문헌
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