Cervical cancer is one of the most common malignant gynecological tumors in women worldwide. It is the third leading cause of cancer death among females in less developed countries (1). Concurrent radiotherapy with cisplatin-based chemotherapy plays a major role in treatment for early stage cervical cancerpatients (2). However, patients who experience radiotherapy and concurrent chemoradiotherapy may also suffer from very strong adverse effects such as bowel obstruction, bleeding, urinary hematuria, or vaginal atrophy (3,4). Therefore, it is necessary to develop new drugs with less adverse effects for the treatment of cervical cancer.Taraxerol is a triterpenoid compound, which has potent anti-inflammatory and anti-cancer activities. Taraxerol has effectively inhibited NADPH oxidase (NOS) activity in murine microglial cells (5). Our previous study found that taraxerol significantly inhibited lipopolysaccharide (LPS)- induced production of interleukin-1 (IL-1β), IL- 6, and tumor necrosis factor-alpha (TNF-α) by interfering with the activation of TAK1 and Akt, thus preventing NF-κB activation (6). It remarkably inhibited TPA-induced tumor promotion on mouse spontaneous mammary tumors (7). Taraxerol has shown in vitro cytotoxic activity against HepG2 and A431humancancer cell lines and potent inhibition of topoisomerase II (8). Taraxerol are also known to augment the inhibitory effects of cyclooxygenases-1 and -2 by measuring prostaglandin E2 (PGE2) production, and induce quinone reductase in cultured Hepa1c1c7 mousehepatoma cells (9). Many triterpenoids exhibit potent anti-cancer effects via the induction of apoptosis in tumor cells, including HeLa (10,12). Recently, it has been reported that taraxerol acetate induced apoptosis, autophagy, cell cycle arrest, and cell migration in humanglioblastoma cells and a mouse xenograft model (13). However, whether taraxerol induced apoptosis and its underlying mechanisms of action is not clear. In this study, we have used a humancervical cancer cell line (HeLa) to assess the effects of taraxerol on a mitochondrial apoptotic pathway and determined the release of cytochrome c to the cytosol, and the activation of caspases and anti-poly (ADP-ribose) polymerase (PARP).
Materials and Methods
Antibodies and reagents
3-(4,5-Dimethyl-2-thiazolyl)-2,5-diphenyl-2H- tetrazolium bromide (MTT), dimethyl sulfoxide (DMSO), anti-Cox IV, anti-Bcl-2, anti-Bax, anti-cleaved caspase 3, anti-cleaved caspase 9, anti-cleaved caspase 8, PARP, anti-phospho-Akt (Ser473), anti-Akt antibodies and anti-cytochrome c were purchased from Cell Signaling Technology (Beverly, MA, USA). Anti-phospho-PI3K p85α (Tyr467), and anti-PI3K p85α antibodies were obtained from Santa Cruz Biotechnology (Santa Cruz, CA, USA). GAPDH was purchased from Bioworld Biotechnology. DAPI was obtained from Invitrogen (Grand Island, NY, USA). DMEM cell cultures and fetal bovine serum (FBS) were purchased from Gibco (Gaithersburg, MD, USA). Taraxerol was obtained from Sigma (St. Louis, MO, USA).
Cell culture and taraxerol treatment
We purchased humancervical cancer cells
(HeLa) from the National Cell Bank of China,
and maintained in DMEM medium supplemented
with 10% FBS, 100 U/mL penicillin and 100 μg/
mL streptomycin. These cells were kept at 37˚C in
a humidified atmosphere that contained 5% CO2.
The taraxerol was dissolved in DMSO to make
a stock of 100 mM and further diluted to final
concentrations of 10-100 μM with a serum-free
culture medium. The amount of DMSO added to
the cell culture was less than 0.1% in all cases.
This experimental study was approved by the
Ethical Committee of Bengbu University.
Cell viability assay
Cell viability was determined using the MTT
assay. Briefly, cells were seeded in 96-well plates
at 37˚C with 5% CO2 for overnight incubation
and treated with appropriate concentrations of
taraxerol for the indicated times. The cells were
then incubated with a serum-free medium that
contained MTT at a final concentration of 0.5 mg/
mL for 4 hours. The crystals formed in intact cells
were solubilized in DMSO, and the absorbance
was measured at 570 nm. Results were expressed
as the percentages of reduced MTT, assuming the
absorbance of control cells as 100%.
Quantification of apoptotic cells by flow cytometry
The extent of apoptosis was measured by an annexin V-FITC/PI apoptosis detection kit (Invitrogen, CA, USA) according to the manufacturer’s instructions. Cells treated with taraxerol for 24 hours were harvested, washed twice with phosphate-buffered saline (PBS, Beyotime, China), gently re-suspended in binding buffer, and incubated with annexin-V-FITC and PI in the dark for 10 minutes, then detected by flow cytometry (BD Accuri C6). The data were analyzed with BD Accuri C6 Software.
DAPI staining assay
In this assay, HeLa cells were fixed with 4% paraformaldehyde for 10 minutes and stained with 1 μg/mL DAPI for 5 minutes, followed by observation under fluorescence microscope.
Mitochondrial membrane potential
Cells were pretreated different concentration of taraxerol for 8 hours, then the cells were stained with 10 μM of JC-1 (Beyotime) for 25 minutes at 37˚C.The cells were subsequently centrifuged and the staining solution removed. The cells were washed twice with JC-1 staining buffer. Fluorescence was monitored with an ELx 800 Universal Microplate Reader (Bio-Tek, Inc.) using 490/530 nm for the monomeric form and 525/590 nm for the aggregate of JC-1. We calculated the fluorescence intensity ratio of aggregates to monomers as an indicator of mitochondrial membrane potential (MMP).
Isolation of mitochondrial and cytosolic fractions
HeLa cells were suspended in a solution
including (10 mM 4-(2-Hydroxyethyl)piperazine-
1-ethanesulfonic acid (HEPES, Beyotime, China),
10 mM KCl, 1 mM EDTA, 1 mM ethylene glycolbis(2-aminoethylether) tetraacetic acid (EGTA,
Sigma, USA), 68 mM sucrose, 220 mM mannitol,
0.1% bovine serum albumin (BSA, Beyotime,
China), and 1 mM phenylmethanesulfonyl fluoride
(PMSF, Sigma, USA), 2 μg/mL aprotinin, and 0.1
mM leupeptin) for 30 minutes in ice to incubate.
Cells were triturated and centrifuged at 200 x g for 2
minutes. We transferred the supernatant phase (500
μL) to a new tube, which was centrifuged at 7000
x g for 15 minutes to pellet all of the mitochondria.
The supernatants were centrifuged at 16000 x g
for 30 minutes and collected as cytosolic fractions.
The mitochondrial fraction was subsequently
solubilized in TBSTDS that consisted of 10 mM
Tris (pH=7.5), 150 mM NaCl, 1 mM EDTA,
1% Triton X-100, 0.5% sodium deoxycholate
(SDS), 0.02% NaN3, 0.0004% NaF and protease
inhibitors. The above steps were carried out at 4˚C
and then the fractions of mitochondria and cytosol
were kept at -75˚C before use.
Western blot analysis
After treatment with selected doses of taraxerol for the indicated times, HeLa cells were rinsed twice with ice-cold PBS, and lysed with the RIPA lysis buffer for 30 minutes on ice. Lysates were centrifuged (12000 x g) at 4˚C for 15 minutes. Total cell lysates (20 μg protein) were separated by SDS-polyacrylamide gel electrophoresis (PAGE) and transferred to nitrocellulose membranes or polyvinylidene difluoride membranes. Membranes were blocked for 60 minutes at room temperature. Membranes were probed with specific primary antibodies overnight at 4˚C and subsequently incubated with IRDye 800CW secondary antibodies for 1 hour. Membranes were visualized using an Odyssey Infrared Imaging Scanner. The fluorescence intensities were analyzed using Image Studio Software (Li-Cor Biosciences).
Statistical analysis
Data are presented as means ± SD from triplicate experiments. Statistical analyses were performed using an unpaired, two-tailed student’s t test. P<0.05 was considered significant.
Results
Taraxerol reduced cell viability in HeLa cells
We investigated the effect of taraxerol on HeLa cell viability. Cells were treated with different concentrations of taraxerol for 24 or 48 hours. Cell viability was examined by the MTT assay. Cells treated with increasing concentrations of taraxerol for 24 hours had significantly reduced cell viability to 95% (20 μM), 89.8% (40 μM), 82.6% (60 μM), 72.9% (80 μM), and 63.6% (100 μM). Cells treated with taraxerol for 48 hours had cell viability of 90.7% at a concentration of 20 μM and 53.6% at the 100 μM concentration (Fig .1A,B). The effects of taraxerol on cell morphology were determined. The cells exposed to different dosages of taraxerol (0 to 80 μM) for 24 hours underwent significant morphological changes. As shown in Figure 1C, taraxerol treatment resulted in obvious cell loss and shrinkage, rounding and partial detachment. These results indicated that taraxerol could inhibit the growth of HeLa cells.
Fig.1
Effects of taraxerol on cell viability and morphological change in HeLa cells. A, B. HeLa cells were treated with different
concentrations of taraxerol for 24 or 48 hours. Cell viability was examined by the MTT assay, and C. Morphological changes in HeLa cells
after treatment with taraxerol for 24 hours as examined by phase-contrast microscopy. All images shown are representative of three
independent experiments with similar results.
*; P<0.05 and **; P<0.01 vs. control.
Taraxerol induced apoptosis in HeLa cells
We sought to determine the occurrence of apoptotic cell death cause by taraxerol treatment. Cell morphological changes were examined by DAPI. We observed that, in a dose dependent manner, the chromatin became condensed and marginalized by pretreatment with different concentrations of taraxerol (Fig .2A). We further investigated apoptosis of cells by annexin V/ PI double staining. After incubation with 80 μM taraxerol for 24 hours, we observed a significant increase in both the early (24.2%) and late (16.2%) stages of apoptotic cells compared with the control group at the early (6.5%) and late (0.5%) stages (Fig .2B). These results demonstrated the ability of taraxerol to induce apoptosis in HeLa cells.
Fig.2
Taraxerol induced cell death in HeLa cells. The cells were treated with taraxerol at the indicated concentrations for 24 hours. A.
DAPI stained cells were observed and photographed by fluorescence microscopy (magnification: ×200) and B. Percentage of apoptotic
cells after treatment with various concentrations of taraxerol. Apoptosis was assessed by annexin V/PI double staining.
Effects of taraxerol on cell viability and morphological change in HeLa cells. A, B. HeLa cells were treated with different
concentrations of taraxerol for 24 or 48 hours. Cell viability was examined by the MTT assay, and C. Morphological changes in HeLa cells
after treatment with taraxerol for 24 hours as examined by phase-contrast microscopy. All images shown are representative of three
independent experiments with similar results.*; P<0.05 and **; P<0.01 vs. control.Taraxerol induced cell death in HeLa cells. The cells were treated with taraxerol at the indicated concentrations for 24 hours. A.
DAPI stained cells were observed and photographed by fluorescence microscopy (magnification: ×200) and B. Percentage of apoptotic
cells after treatment with various concentrations of taraxerol. Apoptosis was assessed by annexin V/PI double staining.
Taraxerol enhanced reactive oxygen species levels and attenuated the mitochondrial membrane potential in HeLa cells
Intracellular reactive oxygen species (ROS) were detected using a DCFH-DA fluorescent probe. ROS production increased 33.4% with 40 μM of taraxerol and 60.2% with 80 μM of taraxerol compared to the control (Fig .3A). Δψm was analyzed by JC-1 fluorescence. Taraxerol-treated cells displayed a loss of MMP (69%, Fig .3B). Taraxerol promoted the breakdown of MMP by preservation of the red JC-1 fluorescence.
Fig.3
Effect of taraxerol on oxidative stress. Cells were incubated with or without taraxerol (20, 40, 80 μM) for 8 hours. A. Reactive oxygen species (ROS) were detected with DCFH2-DA and we calculated the fluorescence intensity and B. Mitochondrial membrane potential (MMP, Δψm) was evaluated by staining with JC-1 and analysis by a microplate reader. The quantitative Δψm from each group is expressed as the ratio of red (JC-1 aggregates)/green (JC-1 monomers). Data was expressed as a percentage of untreated controls. All experiments were repeated three times. The data are expressed as mean ± SD (n=3).
*; P<0.05 and **; P<0.01 vs. control.
Effect of taraxerol on oxidative stress. Cells were incubated with or without taraxerol (20, 40, 80 μM) for 8 hours. A. Reactive oxygen species (ROS) were detected with DCFH2-DA and we calculated the fluorescence intensity and B. Mitochondrial membrane potential (MMP, Δψm) was evaluated by staining with JC-1 and analysis by a microplate reader. The quantitative Δψm from each group is expressed as the ratio of red (JC-1 aggregates)/green (JC-1 monomers). Data was expressed as a percentage of untreated controls. All experiments were repeated three times. The data are expressed as mean ± SD (n=3).*; P<0.05 and **; P<0.01 vs. control.
Effect of taraxerol on cytochrome c, Bcl-2 and Bax expression in HeLa cells
Next, we assessed the potential involvement of inhibition of cytochrome c release. We found that the cytochrome c levels markedly decreased in the cytosolic fraction and increased in the mitochondrial fraction with the taraxerol-treated group (Fig .4A). Furthermore, Bcl-2 and Bax were determined. The data demonstrated that taraxerol could induce downregulation of the anti-apoptotic protein Bcl-2 and upregulation of the pro-apoptotic protein Bax. The decreased ratio of Bcl-2/Bax could exacerbate cytochrome c release, thereby increasing apoptosis (Fig .4B,C).
Fig.4
Effect of taraxerol on cytochrome c release, Bax, and Bcl-2.
A. Cells were incubated with taraxerol (0, 20, 40, 80 μM) for 12
hours. Expression of mitochondrial cytochrome c (Mito-cyto c),
cytosolic cytochrome c (Cyto-cyto c). Cox IV and GAPDH were as
control in the mitochondrial and cytosolic fractions, respectively,
B. Expressions of Bax and Bcl-2 as measured by Western blot,
and C. The ratio of Bcl-2/Bax. All experiments were repeated
three times. The data are expressed as mean ± SD (n=3). **;
P<0.01 vs. control.
Effect of taraxerol on cytochrome c release, Bax, and Bcl-2.
A. Cells were incubated with taraxerol (0, 20, 40, 80 μM) for 12
hours. Expression of mitochondrial cytochrome c (Mito-cyto c),
cytosolic cytochrome c (Cyto-cyto c). Cox IV and GAPDH were as
control in the mitochondrial and cytosolic fractions, respectively,
B. Expressions of Bax and Bcl-2 as measured by Western blot,
and C. The ratio of Bcl-2/Bax. All experiments were repeated
three times. The data are expressed as mean ± SD (n=3). **;
P<0.01 vs. control.
Effect of taraxerol on caspases 8, 9, and 3, and anti-poly (ADP-ribose) polymerase expression in HeLa cells
We assessed caspases 8 and 9 to understand the mechanism of taraxerol-induced apoptosis. The results demonstrated that caspase 9 activity obviously increased, while caspase 8 was unchanged in the HeLa cells (Fig .5A). Our data also showed that taraxerol increased the levels of activated caspase 3 and cleaved PARP in a concentration-dependent manner in these cells. spase 3 and PARP, as the main cleavage targets of effector caspases 8 and 9, suggested that taraxerol induced apoptosis via the mitochondrial pathway including the release of cytochrome c to the cytosol and the activation of caspases 9, caspases 3 and PARP (Fig .5B).
Fig.5
Taraxerol alters the expression of caspases 8, 9, and 3, and
cleavage of anti-poly (ADP-ribose) polymerase (PARP). Cells were
incubated with taraxerol (0, 20, 40, 80 μM) for 12 hours. A. The
expressions of caspase 8 and 9 as assessed by immunoblotting
and B. Expressions of Bax and Bcl-2, cleaved caspase 8 and
cleaved caspase 9 as measured by Western Blot. GAPDH was
used as the loading control. The results were expressed as mean
± SD of three independent experiments.
Taraxerol alters the expression of caspases 8, 9, and 3, and
cleavage of anti-poly (ADP-ribose) polymerase (PARP). Cells were
incubated with taraxerol (0, 20, 40, 80 μM) for 12 hours. A. The
expressions of caspase 8 and 9 as assessed by immunoblotting
and B. Expressions of Bax and Bcl-2, cleaved caspase 8 and
cleaved caspase 9 as measured by Western Blot. GAPDH was
used as the loading control. The results were expressed as mean
± SD of three independent experiments.
Taraxerol decreased the PI3K/Akt signaling pathway
In our previous study, taraxerol reduced Akt activation in LPS-induced RAW264.7 cells (6). We explored the roles of these signaling pathways in taraxerol-induced apoptosis by determining the total and phosphorylated levels of Akt and PI3K. Western blot analysis showed that the protein levels of p-PI3K and p-Akt both reduced in a dose-dependent manner. Total Akt and PI3K levels remained unchanged (Fig .6). Collectively, these results demonstrated that taraxerol might induce cell apoptosis via decreased PI3K/Akt signaling.
Fig.6
Effects of taraxerol on phosphorylation of PI3K/Akt in
HeLa cells. Cells were pretreated with 0, 20, 40, or 80 μM
of taraxerol for 6 hours. The cell lysates were collected and
analyzed by Western blot with anti-phosphorylated PI3K and
anti-phosphorylated Akt. The results were expressed as mean ±
SD of three independent experiments.
Effects of taraxerol on phosphorylation of PI3K/Akt in
HeLa cells. Cells were pretreated with 0, 20, 40, or 80 μM
of taraxerol for 6 hours. The cell lysates were collected and
analyzed by Western blot with anti-phosphorylated PI3K and
anti-phosphorylated Akt. The results were expressed as mean ±
SD of three independent experiments.
Discussion
In this study, taraxerol modulated apoptosis in HeLa cells via morphological changes, cell viability, activation of caspase, and PARP. DAPI staining and flow cytometry revealed that both apoptotic bodies and the percentage of apoptotic cells significantly increased in a dose-dependent manner. These results indicated that taraxerol exhibited anti-cancer activity through induction of apoptosis. It has been reported that mitochondrial outer membrane permeabilization (MOMP) mediated the release of cytochrome c from mitochondria in the mitochondrial pathway (the intrinsic pathway). Cytochrome c binds with Apaf- 1 and caspase 9 to form the apoptosome, which cleave and activate caspases 3 and 7, subsequently leading to cell apoptosis. Our data have indicated that taraxerol caused the release of cytochrome c and activation of caspases 9 and 3 in HeLa cells. Furthermore, mitochondrial damage plays an important role in the apoptosis process. The loss of MMP (Δψm) and an increase in ROS production are crucial parameters of mitochondrial damage. In this study, we have observed that taraxerol enhanced ROS levels and the MMP (Δψm) in HeLa cells.The ratio of Bcl-2 to Bax appears to be one of the critical factors of cell apoptosis (14). Thus, downregulation of the Bcl-2/Bax expression ratio could be a predominant mitochondria-mediated apoptosis mechanism. Our current results have demonstrated that taraxerol treatment led to a significant loss of MMP, downregulated Bcl-2 expression, and increased Bax levels in HeLa cells which suggested that Bcl-2 and Bax participated in controlling taraxerol-induced mitochondrial damage. However, we could not rule out the possibility that other Bcl-2 family proteins might be involved. PI3K/Akt signaling plays a critical role in prevention of apoptosis (15). The PI3K/ Akt pathway has been shown to inhibit Bax translocation from cytoplasm to the mitochondria and upregulate Bcl-2 expression (16,17). Consistent with our previous study, we showed that the protein level of p-Akt reduced in a dose- dependent manner. Recent studies demonstrated that natural or synthetic triterpenoids inhibited the Akt pathways, which decreased Bcl-2/Bax ratio in cells (18,19). Blockage of PI3K/Akt signaling promotes apoptosis in neoplastic cells. Thus, it is possible that suppression of PI3K and Akt activation is a critical target for inhibition of Bcl-2 by taraxerol.
Conclusion
The results demonstrated that taraxerol could significantly reduce HeLa cell survival and induce apoptosis mainly via the mitochondrial pathway which included the release of cytochrome c to the cytosol and activation of caspases. Taraxerol suppressed the PI3K/Akt signaling pathway. Thus, taraxerol might be a potential anticancer drug candidate.
Authors: Dae Sik Jang; Muriel Cuendet; Alison D Pawlus; Leonardus B S Kardono; Kazuko Kawanishi; Norman R Farnsworth; Harry H S Fong; John M Pezzuto; A Douglas Kinghorn Journal: Phytochemistry Date: 2004-02 Impact factor: 4.072
Authors: S Pugazhenthi; A Nesterova; C Sable; K A Heidenreich; L M Boxer; L E Heasley; J E Reusch Journal: J Biol Chem Date: 2000-04-14 Impact factor: 5.157
Authors: Lindsey A Torre; Freddie Bray; Rebecca L Siegel; Jacques Ferlay; Joannie Lortet-Tieulent; Ahmedin Jemal Journal: CA Cancer J Clin Date: 2015-02-04 Impact factor: 508.702
Fig.1
Fig.2
Fig.3
Fig.4
Fig.5
Fig.6