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| Original Article | ||||||||||
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Title |
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Yue Ying Zhanga,
Li Cun Wub, Zhao Peng Wanga, Zhao Xia Wanga,
Qing Jiaa, Guo Sheng Jianga, Wei Dong Zhanga,
c Manuscript received November 24, 2008; accepted January 6, 2009 Short Title: Scorpion Venom on Prostate Cancer Cells |
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| Abstract | ||||||||||
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Methods: Results: Conclusions:
Key words: |
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| Introduction | ||||||||||
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Apoptosis is regulated by several protein families, including the upstream Bcl-2 family (e.g., the anti-apoptotic Bcl-2 and pro-apoptotic Bax) and the downstream caspase family (e.g., caspase-3). The activation of apoptosis is controlled at multiple checkpoints within the cell. Upstream, the pro-apoptotic Bax and anti-apoptotic Bcl-2 are membrane-bound pore-forming proteins that interact through heterodimerization. Together they regulate the mitochondrial transmembrane passage of cytochrome c, which in turn activates caspase proteins. The Bax/Bcl-2 ratio appears more important than the individual Bax or Bcl-2 level in determining a cells vulnerability to apoptosis; high Bax/Bcl-2 ratios lead to greater apoptotic activity [36]. |
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Materials and Methods |
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DU145 cells, derived from a brain metastasis of a prostate cancer patient, were purchased from the Institute of Pharmacy, Chinese Academy of Medical Sciences (Beijing, China) and maintained in medium RPMI 1640 supplemented with 10% fetus bovine serum (FBS) in a humidified atmosphere of 5% CO2 at 37C. Cells were harvested when they were approximately 70% - 80% confluent. Cells were treated with serial concentrations of PESV in the following experiments. Untreated cells were used as controls. Cytotoxicity test of PESV using MTT colorimetric assay The effect of PESV on the viability of DU145 cells was determined by 3-(4, 5-dimethylthiazol-2-yl)-2, 5-diphenyl tetrazolium bromide (MTT) assay. The cells were plated at 2x105 cells per well in 200 L RPMI 1640 containing 0, 10, 20, 40, 80, 100, and 200 mg/mL PESV in a 96-well microtiter plate. Each concentration of PESV was repeated in 10 wells. The cells were incubated for 48 hours at 37C in an incubator. Following 24 hours of incubation, MTT reagent (4 L, 5 mg/mL in PBS) was added to each well and incubated for 2 hours. The microtiter plate containing the cells was centrifuged at 1,800 rpm for 5 minutes at 4C. The MTT solution was removed from the wells by aspiration and the formazan crystals were dissolved in DMSO (150 L). Absorbance was recorded on a microplate reader at 540 nm wavelength. Detection of apoptosis by TUNEL assay Coverslips with adherent cells treated with PESV (40mg/mL) for 48 hours were fixed in 4% paraformaldehyde for 15 minutes at room temperature. Then rinsed in distilled water and incubated with 0.2% Triton X-100 in phosphate buffered saline solution (PBS)-Tween 20 for 30 minutes. DNA fragments were labeled with TUNEL-Enzyme (Boehringer Mannheim). The kit was used according to the manufacturer's instructions, with the addition of incubation in TdT Reaction Buffer for 10 minutes before TUNEL reaction. The coverslips were then incubated in TdT Reaction Mixture for 2 hours at 40-45 C in humidified chamber, rinsed in stop wash buffer for 10 minutes and PBS-Tween 20 for 3 x 2 min. The reaction was detected by incubating coverslips with Streptavidin-HRP in PBS for 20 minutes at room temperature. Then rinse in PBS-Tween 20 for 3 x 2 min, and incubate sections with DAB solution for 5-10 minutes. Cells were counterstained with hematoxylin. Assessment of the apoptotic index Positive signal was defined as the presence of a dark brown staining on nuclei of the neoplastic cells or on apoptotic bodies as morphologically defined. Cells were defined as apoptotic if the whole nuclear area of cells labeled positively. Apoptotic bodies were defined as small, positively labeled, globular bodies in the cytoplasm of the tumor cells that could be found either singly or in groups. The apoptotic index was determined by the percentage of apoptotic cells divided by the number of tumor cells in 400x magnification. A total of at least 1000 neoplastic nuclei were counted based on 10 randomly chosen fields at 400x magnification [37]. Apoptotic cells were identified by TUNEL in conjunction with characteristic morphological changes, such as cell shrinkage, membrane blebbing, and chromatin condensation. DNA cell cycle analysis The DU145 cells treated with PESV (40 mg/mL) in complete medium for 48 hours. The cells were trypsinized thereafter, washed twice with cold PBS, and centrifuged. The cell pellet was resuspended in 50 L cold PBS to which cold methanol (450 L) was added and the cells were incubated for 1 hour at 4C. The cells were centrifuged at 1,100 rpm for 5 minutes, washed twice with cold PBS, suspended in 500 L PBS, and incubated with 5 L RNase (20 g/mL final concentration) for 30 minutes. The cells were chilled over ice for 10 minutes and incubated with propidium iodide (50 g/mL final concentration) for an additional 30 min in the dark. Cells were then analysed for DNA content using a Becton-Dickinson flow cytometor to determine cell cycle phase.
Immunohistochemical stainings Coverslips with adherent cells treated with PESV (40mg/mL) for 48 hours were fixed in 4% paraformaldehyde for 15 minutes at room temperature. DU145 cells were subjected to immunohistochemical staining, with standard streptavidinbiotin- peroxidase techniques, with diaminobenzidine as the chromogen. In brief, DU145 cells were quenched for 10 minutes with 3% hydrogen peroxide, preincubated with blocking serum at 1:20 in 2% bovine serum albumin (BSA)/PBS for 15 minutes at room temperature. After incubation with the primary antibodies, slides were rinsed with PBS, and the secondary antibody was applied at 1:500 in PBS for 30 minutes at room temperature. After rinses with PBS for 30 seconds, slides were incubated with streptavidin/peroxidase at 1:500 in PBS for 30 minutes at room temperature, then rinsed with PBS and incubated for 15 minutes in 0.06% diaminobenzidine and counter-stained with hematoxylin. The following antibodies were used for immunohistochemical staining: Bcl-2 (clone: 124,1:40 dilution, incubation for 2 hours; Dako Corp, Carpinteria, CA), Bax (clone: H62, 1:100 dilution, incubation overnight; Santa Cruz Biotechnology, Inc, Santa Cruz, CA), P27/kip1(clone:M197,1:100 dilution, incubation overnight; Santa Cruz Biotechnology, Inc, Santa Cruz, CA ), Cyclin E (clone:M-20,1:50 dilution, incubation overnight; Santa Cruz Biotechnology, Inc, Santa Cruz, CA ). Replacing the primary antibody by PBS/5%BSA included negative controls. Assessment of protein immunoreactivity by Leica QWin V3 software Immunoreactivity was quantified within 5 random fields at 100x magnification with a Leica DM4000 B system and Leica QWin V3 software was applied to evaluate grey scale intensity variations. In computing, a grayscale or greyscale digital image is an image in which the value of each pixel is a single sample. Displayed images of this sort are typically composed of shades of gray, varying from black at the weakest intensity to white at the strongest. The grey scale intensity and protein expression have inverse relation. Statistical analysis All data are expressed as the mean SE. A t test for unpaired or paired data, as appropriate, was used to compare continuous variables between groups. P < 0.05 was considered to indicate statistical significance. All calculations were performed using the SPSS 10.0 statistical package. |
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| Results | ||||||||||
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We evaluated whether PESV treatment imparts antiproliferative effects in human prostate cancer cells. Employing the MTT assay, we observed that PESV (10- 200 mg/L) treatment on DU145 cells resulted in dose-dependent decrease in the cell growth (Fig. 1).
Figure 1.
Effect of PESV on the growth of prostate cancer cells DU145. Cells
were treated with PESV (10, 20, 40, 80, 100, and 200mg/L), and the
percentage inhibition of cell growth was determined by MTT assay in
a 96-well microtiter plate as detailed in Materials and Methods.
Columns, mean of three separate experiments wherein each treatment
was repeated in 10 wells; bars, SE. Induction of cell apoptosis of DU145 cells and apoptosis index DU145 cells after exposure to PESV were stained by TUNEL. As shown in Fig. 2, apoptotic nuclei and fragmented DNA were stained dark brown in treated cells (Fig. 2b) but not in the untreated controls (Fig. 2a). The apoptotic index is significantly higher in the PESV-treated cells than in the control (Table 1). Figure 2. Detection of PESV-induced apoptosis on DU145 cells by DNA fragment TUNEL staining. Apoptotic nuclei and fragmented DNA were stained dark brown in treated cells (2b) but not in untreated controls (2a) in DU145 cells. Original magnification x400.
Apoptosis-related protein expression Grey Scale Intensity variants of Bax and Bcl-2 immunoreactivity were evaluated by Leica QWin V3 software in DU145 cells treated with PESV and control group. Fig. 3 indicated the inverse relation between the grey scale intensity and protein expression. Higher grey scale intensity stands for weaker protein expression, and lower intensity stands for stronger protein expression. Treatment with PESV resulted in overexpression of Bax in DU145 cells, whereas Bcl-2 expression reduced. In each comparison, there was a significant difference (P < 0.05).
Figure 3.
Grey Scale Intensity variants evaluated by Leica
QWin V3 software of Bax and Bcl-2 immunoreactivity in DU145 cells
treated with PESV and control group. Higher grey scale intensity
standing for weaker protein expression,and lower ,sronger protein
expression. Columns, mean of three separate experiments conducted in
triplicate with DU145 cells; bars, SE. Cell cycle analysis and cell cycle-related protein expression We determined the cell cycle phenotype of DU145 cell line by flow cytometry. As shown in Fig. 4, DU145 cells exhibited PESV-associated G1/S arrest occurring at 48 h after exposure to PESV (40 mg/mL). Cells showed a lack of proliferation at 48 h in comparison with untreated controls (not shown), indicating that the PESV (40 mg/mL) caused proliferation arrest. We further detected the expression of cycle-related protein cyclin E and p27 by immunohistochemical staining. Immunoreactivity was quantified within 5 random fields at 100x magnification. As shown in Fig. 5 and Fig. 6, cyclin E and p27(Kip1) immunostaining pattern was nuclear. DU145 cells exhibited lower expression of cyclin E protein and higher expression of p27(Kip1) protein after exposure to PESV (40mg/mL) compared with untreated control.
Figure
4. Representative DNA
histograms and percentage of cells in different cell cycle phases
after incubated with 40mg/L of PESV
(B) for 48 h in human DU145 cells by flow cytometry. The
growing cells (
Figure 5. Representative image of cell cycle-related protein expression. P27kip1 (5a, 5b) and Cyclin E (5c, 5d). p27 expressed in the nuclei in DU145 cells treated with PESV (5b) is stonger than the control (5a); But Cyclin E expressed in the nuclei in DU145 cells treated with PESV (5d) is weaker than the control (5c).
Figure 6. Grey Scale Intensity variants evaluated by Leica QWin V3 software of Cyclin E and p27 immunoreactivity in DU145 cells treated with PESV and control group. Higher grey scale intensity standing for weaker protein expression,and lower ,sronger protein expression. |
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| Discussion | ||||||||||
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The molecular studies reported here demonstrate that PESV strongly induces the protein expression of Kip1/p27, and decreases cyclin E expression, with an increased interaction/binding between CDKIs and CDK which possibly causes an inhibition in the kinase activity of CDKs. These mechanistic observations were in accordance with an overall efficacy of PESV in inducing a G1 arrest in the cell cycle followed by the inhibition of cell growth. Cell division depends on the activation of cyclin, which binds to CDKs to induce cell cycle progression towards S phase and later to initiate mitosis; uncontrolled CDK kinase activity is one of the major causes of cancer progression as their functions are tightly regulated by CDKIs such as the Cip1/p21 and Kip1/p27 proteins in normal cell cycle progression (38). Following anti-mitogenic signals or DNA damage, CDKIs (Cip1/p21 and Kip1/p27) bind to the cyclinCDK complexes to inhibit their catalytic activity and thus inhibit cell cycle progression [38]. The Rb protein, which is involved in the regulation of the transcription factor E2F [41], is a critical determinant for the restriction-point transition during G1 phase [38, 39], as it is phosphorylated during G1 phase initially by CDK4 or CDK6 and is subsequently maintained in this form by CDK2 [40,41]. The expression level of cyclins is also an important determinant in cell cycle progression particularly during G1/S and G2/M transitions [38]. D-type cyclins have been shown to be important for progression through the G1 phase, where cyclin E is expressed in late G1 that plays an important role in the G1 to S transition [42-45]. The increased protein expression of G1 cyclins in cancer cells has also been shown to be a major factor in driving uncontrolled growth because cancer cells either lack (with undetectable expression) CDKIs or they are non-functional [46]. The increased expression of CDKIs with decreased expression of cyclins and CDKs and decreased CDK kinase activity induced by PESV treatment in human prostate cancer cells suggest that PESV might be effective for the treatment or prevention of prostate cancer. Apoptosis is regulated by several protein families, including the upstream Bcl-2 family (e.g., the antiapoptotic Bcl-2 and proapoptotic Bax) and the downstream caspase family (e.g., caspase-3). The activation of apoptosis is controlled at multiple checkpoints within the cell. Bcl-2 family members are important regulators of apoptosis that include antiapoptotic (Bcl-2, Bcl-XL and Mcl-1), proapoptotic (Bax and Bak) and the BH3-domain-only (Bim, Bid and Bik) proteins [47]. Molecules belonging to the B-cell lymphoma leukaemia-2 (Bcl-2)/Bax system play a crucial role in the regulation of the apoptotic process. In particular, Bcl-2 is an intracellular protein that inhibits apoptosis while Bax counteracts the anti-apoptotic function of Bcl-2 by binding to this molecule [36]. Upstream, the proapoptotic Bax and antiapoptotic Bcl-2 are membrane-bound pore-forming proteins that interact through heterodimerization. Together, they regulate the mitochondrial transmembrane passage of cytochrome C, which in turn activates caspase proteins. The Bax/Bcl-2 ratio appears more important than the individual Bax or Bcl-2 level in determining a cells vulnerability to apoptosis; high Bax/Bcl-2 ratios lead to greater apoptotic activity [36]. This study has also shown that PESV induces cell apoptosis in DU145 prostate cancer cells. We conformed that the induction of apoptosis was mediated through Bax overexpression with bcl-2 down regulation. Cancer develops when the balance between cell proliferation and cell death is disturbed, and the aberrant cell proliferation leads to tumor growth. It is well known that apoptosis and its related signaling pathways have a profound effect on the progression of cancer [48-49], suggesting that agents inducing apoptotic death of human cancer cells may play a critical role in cancer prevention/intervention including prostate cancer. In this regard, whereas there are several classes of chemotherapy drugs causing apoptotic death of cancer cells, their non-selective efficacy (toxicity) in other tissues has been a limitation in their efficacy. Our data demonstrate significant apoptotic death induction by PESV only in prostate cancers, but not in normal prostate epithelial cells, suggesting the possibility of both selectivity and specificity in PESV efficacy against prostate cancer cells. More studies, however, are needed in the future to support this assumption, and to identify its mechanism of action in modulating mitogenic and survival signaling cascades in human prostate cancer. In addition, the significance of the observations made in the present study need to be established in a broader context by conducting further studies in a variety of cell lines and xenograft animal models of human prostate cancer. The encouraging data suggest that PESV might be a promising agent in adjuvant therapy for prostate cancer. |
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| Footnotes | ||||||||||
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