Abstract
Phenethyl isothiocyanate (PEITC) is a candidate anticancer compound found in certain cruciferous vegetables. In our tumor cell xenograft model, dietary administration of PEITC (100–150 mg/kg body weight/d) inhibited androgen-responsive LNCaP human prostate cancer cell tumor growth. We found that dietary treatment with PEITC significantly inhibited tumor platelet/endothelial cell adhesion molecule (PECAM-1/CD31) expression, a marker of angiogenesis. By contrast, we did not find the inhibitory effects of PEITC on tumor growth to be associated with alteration of specific markers for apoptosis, cell proliferation or androgen receptor-mediated pathways. Consistent with in vivo results, PEITC exerted little effects on cell proliferation, cell cycle and androgen-dependent pathways. Interestingly, PEITC significantly attenuated LNCaP cell plating efficiency that correlated with inhibition of integrin family proteins integrin β1, α2 and α6 mRNA expression. Thus, PEITC may be a dietary factor that inhibits androgen-responsive prostate tumor growth indirectly by selectively targeting factors involved in the tumor microenvironment.
Keywords: angiogenesis, phenethyl isothiocyanate, prevention, prostate cancer, xenograft
Introduction
Prostate cancer is one of the most insidious diseases in men in the Western hemisphere. Moreover, the incidence and mortality among men in industrialized Western countries is higher than in Asian men (1). The critical factor may be lifestyle and diet, specifically low consumption of the fruits and vegetables that contain many phytochemical agents (2–7). In addition to the high incidence and mortality, there remains a lack of satisfactory treatment options for metastatic prostate cancer. Therefore, prostate cancer is an ideal candidate disease for chemoprevention. Accordingly, there is intense effort to identify potential naturally occurring and synthetic agents with anticancer and anti-angiogenic activity (8,9).
Isothiocyanates (ITC), which are abundant in foods derived from cruciferous vegetables, are one of the most studied classes of chemopreventive agents (10). ITCs are released from glucosinolate precursors after hydrolysis by the enzyme myrosinase, which is activated during injury of the plant (11). There are over one hundred naturally occurring ITCs, and, of these, phenethyl isothiocyanate (PEITC) has received the most attention because of its ability to inhibit CYP enzymes, decrease cell survival, induce apoptosis in vitro, and attenuate tumor burden. For instance, in human HeLa cells, PEITC, as well as other isothiocyanates, has been shown to induce apoptosis through a capase-3-dependent mechanism (12). Additionally, cysteine protease (i.e., caspase-3 and -8) activity increases in human leukemia cells during PEITC-induced apoptosis (13). Most importantly, it has been reported that PEITC inhibits metastatic prostate cancer cell growth. In the androgen-independent PC-3 metastatic prostate cancer cell line, PEITC inhibits cell survival and increases apoptosis, effects that are mediated by activation of extracellular signal-regulated kinases (ERK1/2) (14). In addition, PEITC significantly inhibits phosphorylation of both IKKα and IKKβ in PC-3 cells (15). Moreover, PEITC treatment has been shown to inhibit the growth and migration of endothelial cells and the formation of new blood vessels (16). However, the effects of PEITC on the early prostate carcinogenesis process, as represented by androgen-responsive tumors, are not known. From a preventive perspective it is important to delineate the effects on this earlier stage.
In this study, we tested the effects of PEITC on cell proliferation, apoptosis, angiogenesis, and androgen-dependent signaling pathways in androgen-responsive LNCaP human prostate cancer cell xenografts in order to elucidate mechanisms that may help explain the prostate cancer preventive effects of PEITC. We also utilize cell culture model to examine potential mechanisms of action of PEITC. We found that PEITC may inhibit androgen-dependent prostate tumor growth by targeting angiogenesis and cell attachment.
Materials and methods
Chemicals and diets
PEITC (indicated purity 99%), dimethylsulfoxide (DMSO), and propidium iodide were purchased from Sigma-Aldrich Chemical Co. (Milwaukee, WI). Powdered AIN-93M diets with or without PEITC [3 μmol/g diet (17)] were prepared by Research Diets (New Brunswick, NJ) and stored at −20°C until weekly feedings.
Cells and cell culture
LNCaP human prostate cancer cells were obtained from the American Type Culture Collection (Manassas, VA) and grown in RPMI-1640 supplemented with 2 mM L-glutamine, 10% fetal bovine serum (FBS), 100 U/ml penicillin, and 100 μg/ml streptomycin (Invitrogen, Carlsbad, CA) at 37°C in a 5% CO2 atmosphere.
In vivo xenograft bioassay
All experimental protocols were in accordance with the National Institutes of Health guidelines and were approved by the USDA Animal Research Advisory Committee. Male athymic nude mice (BALB/c nu/nu, 20–22 g, 5–6 weeks old; Charles River, Frederick, MD) were individually housed in filter-top cages at the USDA BHNRC animal facility and consumed food and fresh tap water ad libitum. Food consumption and body weights were recorded weekly. After an acclimation period of 1 week, during which mice were fed control AIN-93M diet, the mice were randomized into 2 experimental groups, with 19 animals in the control group and 22 animals in the PEITC treatment group. Two weeks later, LNCaP human prostate cancer cell xenografts were established in the mice by injection s.c. in the flank with LNCaP cells (2×106 cells) in 50 μl of phosphate-buffered saline (PBS) plus 50 μl Matrigel (BD Biosciences, Mansfield, MA). This produced palpable tumors within 4–5 days. Cancer preventive efficacy of the treatments was assessed once a week by measuring tumor volume (cm3) = 0.523 × [length (cm) × width2 (cm2)] (18). Mice remained on their respective diets for 7 weeks after cell injection, until tumors reached 2–3 cm3 in volume, and the animals were then sacrificed. A portion of tumor tissue was fixed in 10% neutral buffered formalin for in situ immunohistochemical analysis and quantitation of proliferation, apoptosis, and angiogenesis as previously described (19). A portion of tumor tissue was quickly frozen in liquid nitrogen and stored at −70°C for mRNA and protein analysis as described below.
Cell proliferation and cell attachment assay
LNCaP cells (1–5×105 cells/well) were plated in 24-well plates (Corning Life Sciences, Corning, NY) and 24 h later were treated with 0 (vehicle, DMSO), 0.1, 1, or 5 μM PEITC for 0–75 h, with the medium replaced every 24 h. Cell growth was analyzed using the sulforhodamine B (SRB) assay as described previously (22). Results are expressed as mean absorbance plus or minus standard error of the mean (mean ± SE). For cell attachment assays, LNCaP cell were harvested by trypsinization and re-suspend in media containing 0, 0.5, 1, 2.5 or 5 μM of PEITC at 1×105 cells/ml. Cells were immediately plated in 24-well-plates (1×105 cell/well). After overnight incubation, media were removed from the wells and the wells were wash once with PBS, fixed with 10% trichloroacetic acid. Cells attached to culture plate surface were determined by SRB method (22).
FACS analysis of cultured cells
LNCaP cells were plated in duplicate at a density of 1×105 cells/well in 6-well plates (Corning), which were incubated for 24 h and subsequently synchronized by culturing without serum for 24 h; results are from two independent experiments. Based on the results from the cell growth assays, the cells were then treated with PEITC at 5 or 10 μM for 24, 48, and 72 h. The cells were fixed and stained with propidium iodide for analysis by flow cytometry (FACSCalibur, Mansfield, MA), and the results were evaluated using FlowJo software (BD Biosciences, San Jose, CA).
RNA isolation and reverse transcription (RT)-PCR in cultured cells and tumors
LNCaP prostate cancer cells were plated in 6-well plates (1×106 cells/well) and 24 h after plating were switched to Media B [RPMI-1640 medium without phenol red (Invitrogen), 2 mM L-glutamine, 100 U/ml penicillin, 100 μg/ml streptomycin, and 10% charcoal dextran-treated FBS (Hyclone, Logan, UT)] to minimize the effect of serum hormones. Twenty-four hours later, the medium was replaced with fresh medium containing 1 nM dihydrotestosterone (DHT) with or without 0–5 μM PEITC. The medium was changed daily to fresh medium with test compounds, and after 48 h cells were harvested for total RNA isolation using the TRIzol method (Invitrogen) as described previously (22). For determination of mRNA expression in tumor samples, tumor total RNA was isolated using the TRIzol (Invitrogen) method following the manufacturer's protocol. Gene expression was quantified by the TaqMan real-time RT-PCR method as described previously (22). TaqMan gene expression assay primers and probes for human prostate specific antigen (PSA) and glyceraldehydes-3-phosphate dehydrogenase (G3PDH), proliferating cell nuclear antigen (PCNA), Ki-67, integrin β1 (ITGB1), integrin α2 (ITGA2), integrin α5 (ITGA5), integrin α6 (ITGA6), mouse and human vascular endothelial growth factor (VEGF) A, mouse PECAM-1 and mouse and human TATA binding protein were purchased from Applied Biosystems (Foster City, CA). G3PDH was used as a housekeeping gene for calculation of relative expression levels in vitro and mouse or human TATA binding protein was used for tumor samples.
Western blot analysis of tumor samples
Tumor tissue from 4 mice in each dietary treatment group was lysed with T-PER Tissue Protein Extraction Reagent (Pierce, Rockford, IL) supplemented with protease inhibitors (Complete Mini Protease Inhibitor Cocktail Tablets (Roche Applied Science, Indianapolis, IN), 50 mmol/l sodium fluoride, and 1 mmol/l sodium orthovanadate) and homogenized. Total cell lysate proteins (30 μg) were separated using 4–20% or 8–16% pre-cast denaturing polyacrylamide Tris-glycine gels (Invitrogen) and transferred by iBlot machine (Invitrogen) onto PVDF membranes (Invitrogen). The membrane was probed or with antibodies (all from Santa Cruz Biotechnology, Santa Cruz, CA) against human caspase-3 (clone H-277), human VEGF (clone 147), diluted 1:200 overnight at 4°C, and developed using the WesternBreeze Chemiluminescent Immunodetection Kit (Invitrogen) according to the manufacturer's instructions. Two blots were run for each antibody. Blots were stripped and re-probed with anti-β-actin (Chemicon International, Inc., Temecula, CA) as a loading control. Immunoreactive bands were visualized by X-ray film (Kodak X-Omat MR-1) and digitized using a flatbed scanner (Hewlett-Packard model 4850, Hewlett-Packard, Palo Alto, CA) according to the manufacturer's protocol. The intensity of the band was determined using ImageJ software (http://rsb.info.nih.gov/ij/).
Statistical analysis
In our in vivo experiments StatView (SAS Institute, Cary, NC) software was used for statistical analysis. Repeated measures multivariate analysis of variance with Wilks' λ as the test statistic was used to compare differences between control and PEITC groups in time-to-appearance of palpable tumor and rate of tumor growth between control and PEITC groups over time. The 19–22 animals used per group gave >97% power to detect effects and provided ≥85% power to detect differences as small as 35%. For our in vitro experiments, the GraphPad PRISM 4 (GraphPad Software Inc. San Diego, CA) was used. The unpaired Student's t-test was used to compare experiments with two groups. ANOVA followed by Bonferroni's multiple comparison post hoc test was used to examine differences in PSA mRNA levels between DHT-treated and DHT-non-treated groups.
Results
PEITC inhibits tumor growth in an LNCaP prostate cancer cell xenograft model
Dietary administration of PEITC (3 μmol/g diet) did not significantly affect body weight or food consumption of treated mice compared to control mice (Fig. 1). However, during the final weeks of the experiment mice in both the control and treated groups experienced a slight decrease in body weight and food consumption as the LNCaP prostate cancer cell xenografts grew in size in both the control and treated groups. Each mouse in the treatment group consumed ~100–150 mg/kg body weight/day of PEITC. Four mice from each group died prior to study termination. Overall, administration of PEITC to athymic nude mice did not present any observable toxicity as determined by pathological analysis of kidney and liver from the mice (data not shown).
Fig. 2 illustrates the temporal effects of dietary PEITC on tumor growth in mice fed either control or PEITC diet. We observed a significant delay in tumor growth in mice consuming PEITC compared to control diet. The difference was observed at 6 and 7 weeks after injection of LNCaP prostate tumor cells.
PEITC does not affect apoptosis, cellular proliferation, or androgen-dependent pathways in vivo
We evaluated whether the reduced rate of tumor growth with PEITC treatment was due to induction of apoptosis or a decrease in proliferation in the tumor. As illustrated in Fig. 3A, dietary treatment of mice with PEITC did not lead to changes in apoptosis index in the tumor as determined by TUNEL assay, nor did it affect the intensity of cellular proliferation marker PCNA (Fig. 3B). In addition to cell proliferation and apoptosis, we examined the effects of PEITC on androgen-dependent pathways, as androgen is a known risk factor for prostate cancer and is associated with increased proliferation and decreased apoptosis. We found the androgen responsive gene PSA protein levels in the tumor were not affected by PEITC as determined by immunohistochemistry (Fig. 4A). Additional analyses using real-time PCR and Western blot analyses were performed on tumor samples to confirm the results of immunohistochemical analysis. We also observed no differences in mRNA levels of PSA (Fig 4B), the proliferation markers PCNA (Fig. 5A) or Ki-67 (Fig. 5B) between control (n=4) and PEITC-treated (n=4) tumor samples. We found no change in pro-apoptosis protein Bax mRNA levels (Fig. 5C). We detected pro, but not processed (cleaved) caspase-3 in the tumor samples by Western blot analysis, and densitometric quantitation of the bands revealed no significant differences between control and PEITC-treated mice (Fig. 6A).
PEITC attenuated microvessel density in tumor xenografts
In addition to cellular proliferation and apoptosis, the tumor microenvironment may also affect prostate tumor growth. Therefore, we examined the effects of PEITC on microvessel density. As illustrated in Fig. 7, treatment with PEITC resulted in significantly lower microvessel density, as indicated by PECAM-1/CD31 staining intensity in the tumor. We were not able to detect the mouse PECAM-1 using Western blot analysis. However, real-time PCR analysis showed no difference in mouse PECAM-1 mRNA expression between control (n=4) and PEITC-treated (n=4) tumor samples (Fig. 5D). We also found no difference in mouse or human VEGF mRNA expression between control (n=4) and PEITC-treated (n=4) tumor samples (Fig. 5E and F) or in mouse or human VEGF expression using immunohistochemical detection (data not shown). There were no differences in human VEGF protein expression between control and PEITC-treated tumor samples as determined by Western blot analyses (Fig. 6B).
PEITC affects cell attachment, but not proliferation in vitro
Given the small response of PEITC on angiogenesis we further asked what other pathways may account for inhibition of tumor growth using LNCaP cell culture model. Consistent with the lack of effects on cell proliferation and apoptosis in vivo, PEITC exerted minimal effects on LNCaP cells in culture. Concentrations of PEITC ≤5 μM had no effect on the growth of the LNCaP cells in vitro (Fig. 8A). In addition, cell cycle analysis showed no effect of PEITC on cell cycle progression or appearance of sub-G0 DNA, an indicator of apoptosis. Also consistent with in vivo results, PEITC did not affect DHT-induced increase in PSA mRNA levels in vitro (Fig. 8B). Interestingly, we found as illustrated in Fig. 9A, in the presence of PEITC there was a significant inhibition of LNCaP cell plating efficiency. This effect occurred at relatively low (0.5 μM) PEITC concentration. The integrin family proteins are known to play important roles in cell adhesion/attachment and prostate cancer development (23). We therefore asked whether alteration in integrins may correlate with a decreased in LNCaP cell plating efficiency. We found mRNA expression of integrins ITGB1, ITGA2 and ITGA6 was significantly inhibited in the PEITC (5 μM) treated LNCaP that attached to cell culture plate as compared to vehicle control (Fig. 9B). By contrast, ITGA5 mRNA expression was not affected by PEITC treatment (Fig. 9B).
Discussion
The present study examined the anti-tumor effects of PEITC on androgen-responsive LNCaP human prostate cancer cells in vitro and in vivo. Three important pieces of information were revealed in this study: i) PEITC suppression of tumor growth is associated with diminished microvessel density in vivo. ii) PEITC at the dose and concentrations used in our study demonstrated no direct effects on LNCaP cancer cell growth in vitro and in vivo. iii) Cell attachment, but not proliferation was significantly affected by PEITC in vitro. The level of consumption of PEITC in the diet by nude mice was approximately 100–150 mg/kg body weight/day. At this level of PEITC consumption, a significantly lower tumor volume than in mice fed control diet was observed (Fig. 2). This growth inhibition was observed as early as 6 weeks after tumor cell injection (Fig. 2). The anti-tumor effect of PEITC on LNCaP cells is similar to observations by others in the androgen non-responsive PC-3 human prostate cancer cell line (14–16,24,25). However, the more interesting aspect of our study is the absence of direct effects of PEITC on cell proliferation and apoptosis in tumor in vivo. There were no differences in levels of PCNA, a proliferation marker, or DNA fragmentation (ApoTag), consistent with the lack of effects on LNCaP cell growth (Fig. 8A) and cell cycle (data not shown) we observed in vitro. Further supporting the immunohistochemical data, there were no significant differences in mRNA expression of PCNA (Fig. 5A) or another proliferation marker Ki-67 (Fig. 5B) and pro-apoptosis protein Bax (Fig. 5C), in tumor samples from control and PEITC-treated mice. The growth inhibitory and anti-apoptotic effects of PEITC in vitro reported by others in LNCaP cells (26,27) might arise from different culture conditions than ours. The differential effect of PEITC on apoptosis in PC-3 cell tumors and LNCaP cell tumors in vivo could be due to differences between an androgen non-responsive human prostate cancer model (PC-3 cells) and an androgen- responsive model (LNCaP cells). However, in addition to the cell proliferation end-point, PEITC also had no effect on PSA expression in LNCaP prostate tumors (Fig. 5B and C), corroborating the lack of PEITC effects on androgen-mediated pathways in vitro (Fig. 5A). These results support the notion that the inhibitory effect of PEITC on LNCaP cell tumor xenograft lay elsewhere.
The mechanisms underlying the inhibitory effects of PEITC on LNCaP cell-derived tumor growth may in part through altered angiogenesis (28,29). Microvessel density was significantly lower in tumors in mice consuming PEITC compared to control, as indicated by immunohistochemical staining for PECAM-1/CD31 (30), a marker for microvessel density (Fig. 7). However, this is different from a recent study that showed in PC-3 cells that PEITC at pharmacologically achievable concentrations inhibits angiogenesis in vitro and ex vivo by targeting VEGF (16). We did not detect changes in VEGF protein by immunohistochemistry, Western blot analysis or mRNA by real-time PCR (Fig. 5E and F). Alternatively, we propose that the effects of PEITC may occur right after tumor cell injection. In our experiment, animals were fed PEITC for two weeks before injection. This may create an environment where sufficient PEITC in circulation may already exist to prevent tumor cells to attach. Our cell culture results support this hypothesis. As illustrated in Fig. 9A, cell plating efficiency after overnight exposure to PEITC was significantly reduced in a concentration-dependent fashion that occurred at concentration as low as 0.5 μM. Furthermore, in those cells that attached to cell culture plate, we found a significantly lower mRNA expression of integrin family proteins ITGB1, ITGA2, ITGA6 in cells exposed to PEITC (Fig. 9B). ITGB1 is a common subunit for fibronectin, laminin and collagen receptors (31–33). ITGA2 is a subunit for collagen receptor (32) and ITGA6 is a subunit for laminin receptor (33). These integrins are known to play an important role in cell adhesion/attachment and prostate cancer development (23,31–33). Therefore, it is possible that this inhibition of cell adhesion/attachment-related protein may decrease initial number of cells established at the injection site and lead to smaller tumor size in PEITC-fed animals. Thus, the tumor growth inhibitory effects of PEITC in our system may be indirect. The effect of PEITC on integrins appeared to be specific as ITGA5 mRNA levels did not alter (Fig. 9B). Additional studies are warranted to further support this hypothesis.
Cruciferous vegetables are unique among the foods consumed in the diet in that they have been consistently shown to have beneficial effects in the prevention of various forms of cancers, including prostate (10,34–37). These effects may be due to modulation of multiple pathways by various ITCs present in these vegetables. In addition to the inhibition of angiogenesis by PEITC observed in this study, indoles, another family of phytochemicals found in cruciferous vegetables, are known to modulate androgen-responsive pathways (38). Moreover, sulforaphane, also found in cruciferous vegetables, may offer protection against carcinogens through activation of xenobiotic metabolism pathways (39). It would be of interest to examine combinations of compounds, as well as temporal effects during carcinogenesis, to further elucidate the benefits of cruciferous vegetables.
In conclusion, the effects of PEITC on androgen-responsive LNCaP human prostate cancer cells in the present study appeared to differ from those seen in androgen-non-responsive PC-3 human prostate cancer cells (16,25). The mechanisms underlying the inhibitory effects of PEITC on growth of LNCaP xenografts appeared to be independent of cell proliferation or apoptosis and may be through modulation of the tumor microenvironment by regulation of attachment and/or angiogenesis.
Acknowledgements
This work was supported by US appropriated funding to USDA, project no. 1235-51530-052-00 (T.T.Y.W., T.-C.W.) and the National Cancer Institute (T.S.H., S.D.H., S.N.P.), Grant no. P30ES007784 from the National Institute of Environmental Health Sciences (SDH, SNP) and by U54 Howard-Hopkins partnership grant (U54CA091431, TSH). T.S.H. was supported by a National Cancer Institute Cancer Prevention Fellowship when the work was performed. The authors would like to thank Dr Diana Haines, Maureen Kennedy, and Scott Lawrence of the Pathology/Histotechnology Laboratory, SAIC-Frederick, for their assistance in immunohistochemical analysis.
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