Anti-Cancer Effects of Cordycepin on Oral Squamous Cell Carcinoma Proliferation and Apoptosis in Vitro ()
1. Introduction
Oral squamous cell carcinoma (OSCC) shows a poor prognosis; the 5-year survival rate is only 35% - 50% despite recent advances in radiation therapy, improvement of surgical techniques, and the advent of aggressive chemotherapy protocols [1]. Conventional cytotoxic therapies primarily target rapidly dividing cells including malignant cells as well as certain normal cells, leading to significant morbidity and limited clinical benefits of afflicted patients [2]. Therefore, it is urgently required to improve anti-cancer therapies that effectively and specifically target epithelial tumor cells while minimizing the toxic side effects on physiologically proliferating cells. In this regard, the major concern has been focused on identifying new chemotherapeutic agents with fewer side effects, and increasing attention has been paid to naturally acquired compounds for new candidates of chemotherapeutic agent.
Among naturally acquired agents explored and tested, cordycepin is a nucleoside analogue (3’-deoxyadenosine) and extracted from Cordyceps militaris that has long been used empirically as a folk medicine in Korea, Japan and China. Cordyceps militaris consists of cordycepin, nucleosides, and various polysaccharides, but most of the pharmacologic effects of Cordyceps are attributed to cordycepin [3]. Although cordycepin has been primarily used as a natural antibiotics, emerging evidence now supports multiplepharmacological effects such as 1) selective anti-bacterial effect [4]; 2) maturations of antigen-presenting dendritic cell (improvement of immunoregulatory function) [3]; 3) anti-fungal (Candida albicans) activity [5]; 4) anti-viral effect [6]; 5) inhibition of platelet aggregation [7]; 6) anti-inflammatory effect [8]; and 5) anti-cancer effect [9,10].
Earlier studies on cordycepin focused on the anticancer effects for leukemia [10,11]. Recently, it has been found that cordycepin has inhibitory effects on solid tumors such as melanoma, epithelioid cervix carcinoma, and breast cancer cells in vitro [10,12]. In addition, cordycepin showed inhibitory effect on the growth of melanoma in a mouse model [13]. However, only a few studies have been performed to study the anti-cancer effect of Cordycepin on oral squamous cell carcinoma. Recently, Wu et al. [14] reported the pro-apoptotic effects of cordycepin on OEC-M1, a human oral squamous cancer cell line. It was demonstrated that 100 μM cordycepin induced apoptosis and decreased cellular proliferation in vitro. Nevertheless, their report did not encompass in vivo data and mechanistic consideration of anti-cancer effect of cordycepin.
The biological mechanisms of anti-cancer effects of cordycepin are not completely understood yet but previous studies suggested that cordycepin effects are mediated through adenosine-adenosine receptors [8,10]. Adenosine is a physiological regulator of various cellular activities such as cell growth, differentiation, and cell death in wide variety of cell types [15]. There are four types of G-protein coupled surface receptors for adenosine; they are A1, A2A, A2B, and A3 adenosine receptors and the specific cellular response to adenosine is thought to be decided by the expression of the specific type of receptor on the cell surface [16]. Indeed, cordycepin was shown to exert anti-cancer effect through antagonizing A3 adenosine receptor (A3AR) [10] in melanoma and lung carcinoma. In addition, for some types of solid tumors, the mRNA expression of A3AR was verified using cell lines. Melanoma [17], prostate carcinoma [18], and some types of breast carcinoma [19,20] cells expressed A3AR whereas bladder carcinoma cells [21] and some types of breast carcinoma cells [8,19] did not express A3AR. Gessi et al. [22] reported that the expression of A3AR protein was higher in colon carcinomas than in normal mucosa originating from the same individuals. Madi et al. [23] also verified the expression of A3AR in the tissues from breast and colon carcinomas patients. The results indicated that tissues from both colon and breast carcinoma expressed more A3AR mRNA and protein than those from the adjacent non-neoplastic tissue or normal tissues.
In this study, we sought to evaluate the anti-proliferating effect of cordycepin in OSCC cell lines in vitro and also in OSCC xenografted mouse tumor models in vivo. In addition, we determined whether the anti-tumoral effects of Cordycepin is mediated by specific adenosine receptors, specifically A3AR to obtain the rationale for further research; enhancing the therapeutic efficacy of cordycepin in OSCC.
2. Materials and Methods
2.1. Cell Culture
Two human OSCC cell lines, HSC3 (Japanese Cell Resources Bank, Osaka, Japan) and KB (American Type Culture Collection, Rockville, MD, USA), were used in this study. Cells were maintained at 37˚C in a humidified atmosphere of 5% CO2. In RPMI medium 1640 (Gibco, Rockville, MD, USA) supplemented with 10% fetal bovine serum (Gibco), 100 U/ml penicillin, and 100 μg/ml streptomycin (Gibco).
2.2. Western Blot Analysis
Cells were homogenized by Ultraturax (Polytron, Kinematica) in ice-cold lysis buffer [TNN buffer, 50 mM Tris buffer (pH 7.5), 150 mM NaCl, and NP40 0.5% for 20 min]. Cell debris was removed by centrifugation for 10 minutes at 14,000 rpm. The supernatants were used for Western blot analysis. Protein concentrations were determined using the Bio-Rad protein assay dye reagent. Equal amounts of the sample (50 μg) were separated by 10% SDS-PAGE. The resolved proteins were then electroblotted onto nitrocellulose membranes. Membranes were blocked with 1% BSA and incubated with the desired primary antibody-A1AR (sc28995), A2aAR (sc70321), A2bAR (sc28996), A3AR (sc7508) All antibodies were purchased (SantaCruz, Santa Cruz, CA, USA) and were used under the same reaction condition (dilution rate 1: 1000 and for 1 hour at room temperature). Blots were then washed and incubated with each type of secondary antibody for 1 hour at room temperature. Bands were recorded using ECL solution. The expression level of each receptor was measured by densitometric analysis using the BioRad scanning densitometer.
2.3. Proliferation Assay and Morphological Analysis
To verify the inhibitory effect of cordycepin (Sigma, St Louis, MO, USA) on the proliferation of cells, sulforhodamine B (SRB) method was used. HSC3 and KB cells (1 × 105 cells/well in 12 well plates) were incubated for 24 hours. Subsequently, the cells were treated with various concentrations of cordycepin (0 μM, 5 μM, 10 μM, 30 μM, 50 μM, 100 μM, 150 μM, and 200 μM) for 48 hours. The cells were fixed by incubation in 50 μl cold 50% TCA (trichloroacetic acid, Sigma) for 1 hour at 4˚C in the dark. The media and TCA were removed and the plates were rinsed with water five times and then air-dried. The cells were stained by addition of 100 μl of 0.4% sulforhodamine B (Sigma) in 1% acetic acid for 30 minutes. The stain was removed and the cells were washed five times with 1% acetic acid, air-dried, and 100 μl of 10 mM unbuffered Tris was then added to each well to dissolve the dye. The plates were shaken for 5 min until the dye was uniformly distributed and then read on a plate reader (Molecular Devices, Sunnyvale, CA) at 540 nm. SRB assays under various cordycepin concentrations were applied 10 times. For observation of morphologic changes of cells, KB cells and HSC3 cells (1 × 105 cells/ml in 12 well plate) were treated with cordycepin (0 μM, 25 μM, 50 μM, 100 μM, 200 μM, 500 μM) for 48 hours. Then, cells in plates were observed under light microscope and photographed.
To confirm whether cordycepin acts via adenosine receptor, antagonist for each adenosine receptor was applied to cells with cordycepin and SRB proliferation assays were performed. The following antagonists to adenosine receptors were used: 8-cyclopentyl-1, 3-dipropylxanthine (CPX), an A1AR antagonist; 8-(3-Chlorostyryl)-caffeine, an A2AAR antagonist; Alloxazine, an A2BAR antagonist; 3-ethyl 5-benzyl 2-methyl-6-phenyl-4-phenylethyl-1, 4-(±)- dihydropyridine-3,5-dicarboxylate (MRS-1191), an A3AR antagonist. In this assay, 50 μM of cordycepin and 1 μM of each antagonist were applied to 4 × 104 cells in 24-well plate and cells were remained for 48 hours. This assay was repeated 10 times for each antagonist.
2.4. Apoptosis Assay
Apoptotic cells were detected in situ using terminal transferase dUTP nick end labeling (TUNEL) assay. HSC3 and KB cells (2 × 105 cells/well in 6 well plate) were cultured and treated with cordycepin (50 μM) alone or combined with 1 μM of each antagonist for 48 hours. Cells were fixed in 4% paraformaldehyde in PBS (pH 7.4) for 15 - 30 minutes at room temperature and permeabilized for 2 - 5 minutes. Subsequently, apoptotic cells were detected by the commercially available in situ apoptosis detection kit (Takara, Japan). After applying anti-FITC HRP Conjugate at 37˚C for 30 minutes, DAB (diaminobenzidine) was applied to generate an insoluble colored substrate at the site of DNA fragmentation for 10 - 15 minutes. The DAB-labeled, fragmented DNAs were stained as dark brown indicating apoptotic cells. The apoptosis index was defined as the percentage of positive cells in 1000 cells.
2.5. In Vivo Anti-Tumorigenesis and in Situ Apoptosis Assay
Ten 6-week old male BALB/c nude mice (Orient Co., Suwon, Korea), weighing about 20 g, were obtained and kept in an environment complying with the NIH guidelines for the care and use of laboratory animals. KB and HSC3 cells were suspended in regular culture media (1 × 106 cells in 0.5 ml), and inoculated subcutaneously into the right flank of mice. Cordycepin (30 mg/kg) was administered when the volume of the ensuing mass reached 75 - 100 mm3 to 10 mice of each group by intraperitoneal injection for 30 days [13]. Ten mice were used as controls and only diluent (RPMI medium 1640) was injected for them. All were scarified 24 hours after the last injection of cordycepin. Each mouse was weighed every day to evaluate side effects of administrations. To evaluate tumor growth, the length and width of tumor mass were measured with a slide caliper every three days. Tumor volume (in cubic millimeters) was calculated using the following equation; Volume (mm3) = Length × Width2 × 1/2. The relative tumor volume (RTV) was calculated as RTV = Vi /Vo, where Vi is the tumor volume at sacrifice and Vo is the volume at the time of initial treatment. After sacrifice, the tumors were excised, fixed in formalin, embedded in paraffin, and sectioned. Apoptosis of the cancer cells in vivo was detected using TUNEL assay with in situ apoptosis detection kit (Takara, Japan). The apoptosis index was defined as the percentage of positive cells in 1000 cells.
2.6. Statistical Analyses
The OD values under various cordycepin concentrations were compared with that of 0 μM with Wilcoxon signed rank test. OD values of cultured cells with and without each adenosine receptor antagonist and apoptosis index were compared by Mann-Whitney U test. Relative tumor volumes of control and experimental mice were also compared by Mann-Whitney U test. For all analyses, p < 0.05 was regarded as significant.
3. Results
3.1. Expression of Adenosine Receptor
We determined whether OSCC cells express adenosine receptors. All types of adenosine receptors were stably expressed in both OSCC cell lines. Three types of adenosine receptor were also expressed in normal oral keratinocytes but A2AAR was not detected in normal oral gingival keratinocytes (Figure 1(a)). When the protein expressions of adenosine receptors of OSCC cell lines were compared with normal oral keratinocytes, A1AR, A2BAR, and A3AR proteins were expressed significantly stronger than normal oral keratinocytes (Figure 1(b), p < 0.05).
3.2. Effects of Cordycepin and Adenosine Receptor Antagonists on Cell Proliferation in Vitro
We determined whether cordycepin suppress proliferation of oral squamous cell carcinoma cells. After 48 hours of
(a) (b)
Figure 1. (a) Protein expression of adenosine receptors in normal oral keratinocytes, KB and HSC3. Four types of adenosine receptor are strongly expressed in both OSCC cells while the expressions of adenosine receptors are weaker or not expressed in normal oral keratinocytes. (b) In both OSCC cells, expression levels of A1AR, A2BAR, and A3AR are stronger than each adenosine receptor of normal oral keratinocytes (*: statistically significant in mean difference of expression of each adenosine receptor between OSCC cells and normal oral keratinocytes, p < 0.05).
treatment with cordycepin in various concentrations, both KB cells and HSC3 cells showed a dose-dependent decrease in the number of surviving cells (Figure 2(a)), suggesting cordycepin suppressed tumor cell proliferation. The statistically significant changes in OD values appeared from the concentration of 50 μM in KB cell line and 30 μM in HSC3 cell line (p < 0.05). As illustrated in Figure 2(b), morphological changes were observed in both cells treated with cordycepin (50 μM). Both KB and HSC3 cells showed loss of their distinct morphologic characteristics and low cellular density. In addition, such a morphological change increased in a dose-dependent manner.
However, contrary to our expectation, none of adenosine receptor antagonist rescued the effects of cordycepin on tumor cell proliferation (Figure 3(a), p > 0.05). In addition, morphological observation confirmed the result of proliferation assay. As shown in Figure 3(b), the shape and density of cultured cells treated with both cordycepin and one type of cordycepin receptor antagonist (A1AR, A2AAR, A2BAR, or A3AR antagonist) were not morphologically different from those of cells treated with cordycepin alone.
3.3. Apoptosis Assay in vitro
Under light microscope, the number of dark brown stained cells indicating apoptosis were increased in cordycepin treated group (Figures 4(a), (b), (d) and (e)). However, treatment of 1 μM of adenosine receptor antagonist did not reverse cordycepin induced apoptosis in both cell lines. For example, A3AR antagonist treatment did not cause any change in both cells which had been treated with 50 μM Cordycepin (Figures 4(c) and (f)). Evaluation of apoptotic index confirmed this phenomenon statistically (Figure 4(g)). There were significant differences in apoptosis index between the control group and the Cordycepin treated group. While the apoptosis index of KB and HSC3 cells were 9.2 (± 3.2) and 5.2 (± 2.9) respectively, those of cells which were treated with cordycepin (50 μM, 48 h) increased to 18.4 (± 2.1) for KB and 21.8 (± 3.5) for HSC3 (p < 0 .05). However, there is no significant difference in apoptosis index between the groups treated with cordycepin alone and the group treated with cordycepin and additional each type of adenosine receptor antagonist (p > 0.05, Figure 4(g)).
3.4. Tumor Growth and Degree of Apoptosis in Vivo Model
Next, we determined the effects of cordycepin on human OSCC implanted nude mice. The tumor volume of OSCCs in the nude mice continuously increased during whole experimental period. The relative tumor volumes (RTVs) of the KB and HSC3 tumors in the cordycepin-treated group on sacrifice were 17.6 and 8.96 respectively, which means that the tumor volume increased up to 17.6 and 8.96 times during treatment period. Meanwhile, the RTVs of KB and HSC3 tumors in the control group were 18.4 and 9.20 at sacrifice (Figure 5(a)(b)). However, no significant difference was found between the experimental group and the control group in tumor volume change (p > 0.05). Histological observation of the tumor showed that there was no difference in the degree of in situ apoptosis (stained as dark brown) between the experimental group which was administered with cordycepin (30 mg/kg, 14 days) and the control
Figure 2. (a) Proliferation (OD) of KB and HSC-3 cells under various concentrations of cordycepin for 48 hours. Both cells show decreases in proliferation in a dose-dependent manner. Statistically significant decreases (*) appear from 50 μM in KB cells and 30 μM in HSC3 cells. (b) Morphological changes in KB and HSC3 cells treated with cordycepin are observed under the light microscope and photographed. As concentration of cordycepin is higher, cells become pleomorphic in shape and show low cellular density (magnification, × 100).
Figure 3. (a) Effect of adenosine receptor antagonists on the anti-proliferating effect of cordycepin. No adenosine receptor antagonist reverses the anti-proliferating effect of cordycepin. (b) Morphological changes in KB and HSC3 cells treated with cordycepin (50 μM) alone or cordycepin with each adenosine receptor antagonist (1 μM) for 48 hours. In each cell line treated with cordycepin, the addition of each adenosine receptor could not induce significant reversal of cellular density or cell morphology (magnification, × 40).
Figure 4. Apoptosis assays on KB cells and HSC3 cells. Cordycepin induced apoptosis in both OSCC cell lines and apoptotic cells are represented as dark brown stain. Note more apoptotic bodies are observed in cordycepin treated KB (b) and HSC3 (e) cells than in respective control cells (a and d, magnification × 100). Meanwhile, cordycepin induced apoptosis are not morphologically reversed by adenosine receptor antagonist (A3AR in this figure) treatment in KB (c) and HSC3 (f). Apoptosis index (g) demonstrates that there is a significant difference in apoptosis between the cordycepin treated group and the control group (*, p < 0.05) while no significance is detected in apoptosis index between the group of cordycepin treatment alone and the each group of adenosine receptor antagonist combined with cordycepin (**, p > 0.05).
Figure 5. Tumorigenesis assay and in situ apoptosis assays on tissues obtained from the xenografted mice. Relative tumor volume (RTV) increased through experimental period in KB (a) and HSC3 (b). Note that RTV of the cordycepin treated group is lower than that of the control group in some experimental period, but is not statistically significant (p > 0.05) There is no difference in the density of apoptotic cell and histo-morphological characteristics between control mice (c) and cordycepin treated mice (d) (apoptotic cell stained as dark brown, magnification, × 100). (e) Apoptotic index is not significantly different between in the control (injection of diluent) and the experimental (30 mg/kg of cordycepin) groups (**: p > 0.05).
(administration of diluent only) group (Figures 5(c) and (d)). While the apoptosis index of KB and HSC3 cells were 53.2 (± 15.4) and 67.9 (± 11.9) respectively, those of cordycepin treated cells increased to 59.2 (± 9.4) for KB and 78.3 (± 10.3) for HSC3. Difference of apoptotic index was not statistically significant between the control group and the experimental group (Figure 5(e); p < 0.05).
4. Discussion
In the present study, the results of in vitro anti-proliferating assay showed significant and dose dependent anti-proliferating activity of cordycepin on OSCC. The statistically significant decreases of the cellular proliferation appeared from the concentration of 50 μM in KB cell and 30 μM in HSC3 cell. The inhibitory concentrations of this study were much lower than those of Wu’s study14 but inhibitory effect was weaker than those of melanoma case. Cordycepin at 100 μM for 48 hours could reduce the cell number of mouse melanoma cell (B16-BL6) by 83% [10] whereas OD values of KB cells and HSC3 cells decreased only 21.7% and 17.32% in this study. Even though the major advantage of cordycepin is its wide safety margin, relatively weaker anti-proliferating activity of cordycepin may be a definite limitation in practical application of cordycepin as a novel chemotherapeutic drug. Thus, it is recommended that further studies to enhance anti-proliferating activity of cordycepin are needed.
Among four types of adenosine receptor, A3AR and inhibitory effect of its agonist on many cancer cell types were mainly inspected and it is now generally accepted that A3AR agonists exert their anti-cancer effects on solid tumors, such as melanoma, breast carcinoma, prostate carcinoma, and colon carcinoma [8,18,19,24-26]. Accordingly, cordycepin has been also studied based on the relationship with A3AR. Recently, Nakamura et al.10 revealed the structural similarity between adenosine and cordycepin and they tested cordycepin as an A3AR agonist. According to their in vitro experiment, the inhibitory effect of cordycepin on tumor growth was exclusively antagonized by only a selective A3AR antagonist among all adenosine receptor antagonists. With this result, they concluded that cordycepin exerts inhibitory effects on the growth of mouse melanoma and lung carcinoma cells by stimulating A3AR on tumor cells. Moreover, the concentration of A3AR agonist is thought to be a major factor to determine the inhibitory mechanism in case of lymphoma and leukemia [27,28]. However, in solid tumors, the existence or expression level of A3AR is also thought be an additional important factor because A3AR is not expressed consistently in all types of solid tumors [8]. In an attempt to reveal the relationships with adenosine receptor in OSCC, we evaluated the expression of all types of adenosine receptor using OSCC cell lines. Our Western blotting data clearly demonstrated that two tested cell lines, KB and HSC3 showed stronger expression of all types of adenosine receptors than primary cultured oral gingival keratinocytes. From these results, adenosine-adenosine receptor mechanism was also thought be a critical tumorigenic process in case of OSCC. However, when each adenosine receptor antagonist was applied to cordycepin treated cancer cells in the current study, none of adenosine receptor antagonists significantly reversed the anti-proliferating effect of cordycepin on OSCC cell. These results could be reconfirmed by observing cancer cells with light microscope. Thus, we concluded that cordycepin seemed to have anti-proliferating effect not mediated by any type of adenosine receptor in OSCC cell lines despite strong expression of all types of adenosine receptors.
It is reported that A3AR agonists exert inhibitory effects on cancer cells through two different mechanisms; cytostatic effect (cell-cycle arresting) via A3AR and cytotoxic effect (induction of apoptosis) via active transport [16,29]. A3AR agonists, at low concentration, resulted in cell cycle arrest but at high concentration, induced apoptosis of melanoma and leukemia cells [16,29]. Likewise, induction of apoptosis has been proposed as another mechanism of cordycepin for suppression of cancer cells [16]. Evidences showed apoptosis could be induced in cancer cells that do not have A3AR and this means that induction of apoptosis may not be directly mediated by A3AR [8,30,31]. This is evidenced by the facts that apoptosis of cells by A3AR agonists was not reversed by A3AR antagonists [32] but antagonized by the addition of adenosine transporter protein [30,31]. Thus, cancer cells that do not have A3AR or not respond to A3AR activation may be inhibited by cordycepin at higher concentration via induction of apoptosis. In our in vitro apoptosis assay demonstrated that the apoptosis index of both OSCC cell lines significantly increased by 50 μM of cordycepin, and apoptotic process was not reversed by adenosine receptor antagonist in both cell lines. In addition to the proliferation assay, these results confirmed that OSCC did not respond to adenosine receptor activation and suggested that anti-cancer effect of cordycepin may be mediated by induction of apoptosis. Thus, previous studies and the results of current study support that inducing apoptosis of OSCC cells is mediated by active transport, independent of adenosine receptor.
Although in vitro results of the current study showed that cordycepin exhibits effective anti-cancer activity via direct cellular apoptotic effect, a critical question about the practical value of cordycepin as a main anti-cancer agent for OSCC was raised because cordycepin treatment failed to inhibit tumor growth in vivo OSCC model in the present study. In a report, administration of cordycepin (15 mg/kg per day) for 2 weeks inhibited the tumor enlargement inoculated with mouse melanoma (B16-BL6) cells in mice [13]. However, in our study, even cordycepin administration of higher concentration (30 mg/kg per day for 4 weeks) could not suppress OSCC growth significantly in two types of xenotransplanted nude mice model. The tumor mass generated by inoculation with KB or HSC3 cells grew without any reduction in mass size throughout the experimental period. Moreover, in situ apoptosis assay showed that there was no difference of apoptotic index between the experimental group animals and the control group animals. We originally expected based on in vitro experiment that, at the very least, tumor mass growth of the tumor would be retarded with increased apoptosis. However, there was no evidence of growth inhibition of tumor mass and no increased apoptosis following cordycepin administration. The results of this preliminary in vivo study suggest some possibilities as followed, although more advanced experimental analyses should be performed in further study to prove them. First, originally sensitive OSCC cells in vitro state gained resistance against cordycepin by altering genetic characteristics during tumorigenic process. The second possibility is that plasma levels of cordycepin could not be achieved enough to induce direct apoptosis by presented administration method. Considering that in vitro study showed that anti-cancer effect of cordycepin on OSCC cells was not mediated with adenosine receptor activation but dependent on direct induction of apoptosis, higher concentration and longer application time of cordycepin might be a prerequisite for induction of apoptosis [29,32]. Therefore, pharmacokinetic evaluation and blood concentration monitoring of cordycepin will be needed in further study. In summary, this study highlighted the possibility of Cordycepin as a safe and a natural anti-cancer agent against OSCC in vitro but, there’s definite limitation to be used as sole anti-cancer drug in vivo.
5. Acknowledgements
“This research was supported by Basic Science Research Program through the National Research Foundation of Korea (NRF) funded by the Ministry of Education, Science and Technology (2010-0016443). Ju-Hyon Lee and Soon-Min Hong gave equal contribution on this paper as 1st author.”