Affiliations of authors: K. Nishimura, N. Nonomura, E. Satoh, Y. Harada, M. Nakayama, T. Tokizane, T. Fukui, Y. Ono, H. Inoue, A. Okuyama (Department of Urology), M. Shin, Y. Tsujimoto, H. Takayama, K. Aozasa (Department of Pathology), Graduate School of Medicine, Osaka University, Suita-City, Japan.
Correspondence and reprint requests to: Kazuo Nishimura, M.D., Department of Urology, Graduate School of Medicine, Osaka University, 22 Yamadaoka, Suita-City 5650871 Japan (e-mail: kazu{at}uro.med.osaka-u.ac.jp).
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ABSTRACT |
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INTRODUCTION |
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Clinical use of glucocorticoids for the treatment of lymphoproliferative disorders and solid tumors (810) was prompted by the in vitro observations that glucocorticoids inhibit the proliferation of several cell types. There are at least two potential mechanisms by which glucocorticoids can inhibit proliferation: the induction of growth-inhibitory cytokines or the inhibition of growth-stimulatory cytokines. For example, in the androgen-independent prostate cancer cell line PC-3, dexamethasone inhibited cell growth through the induction of transforming growth factor-1 (11), whereas in human monocytes, dexamethasone inhibited the production of proinflammatory cytokines, such as interleukin (IL) 1
(IL-1
) and tumor necrosis factor-
(TNF-
) (12).
The biologic actions of glucocorticoids occur in cells that express glucocorticoid receptors (GRs). GRs belong to the family of nuclear hormone receptors that can function as transcription factors once the ligand has bound. Glucocorticoids have been shown to interfere with the transcriptional activity of several transcription factors, including nuclear factor-B (NF-
B) (13), that are important for the induction of several growth-stimulatory cytokines. Thus, glucocorticoids may inhibit growth-stimulatory cytokines by inhibiting NF-
B activity.
To understand the mechanism by which glucocorticoids have clinical benefit for patients with HRPC, we hypothesized that glucocorticoids act directly through GRs in prostate cancer cells and exert an antitumor effect, in addition to any effects that result from the in vivo suppression of adrenal androgen production. Furthermore, we hypothesized that, because androgen-independent prostate cancer cells are growth dependent on the cytokine IL-6 (14,15), whose transcription is partially dependent on NF-B (13), glucocorticoids exert their antitumor effect by inhibiting NF-
B activation and the production of NF-
B-dependent cytokines. Here, we tested this hypothesis in vitro with established human prostate cancer cell lines (LNCaP, DU145, and PC-3). Because high-dose (25 µg/mouse per day) dexamethasone may decrease expression of GRs (1618), we used a low-dose dexamethasone regimen that is considered to be desirable for maintaining sufficient inhibitory effects and for minimizing adverse effects in vivo in a xenograft model of androgen-independent prostate cancer. We also assessed GR expression in prostate cancers from patients, some of whom had received androgen ablation therapy (AAT).
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METHODS |
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DU145, PC-3, and HeLa cells were maintained in Dulbecco's modified Eagle medium (DMEM) supplemented with 10% heat-inactivated fetal calf serum (FCS). LNCaP cells were maintained in RPMI-1640 medium with 10% heat-inactivated FCS. All cell lines were obtained from the American Type Culture Collection (Manassas, VA).
Tumors and Patients
All patients signed consent forms approved by our institution. Prostate cancer tissue was obtained from a total of 16 patients treated with surgery alone (five patients) or surgery plus preoperative total AAT (11 patients), which consisted of luteinizing hormone-releasing hormone analogue plus antiandrogens for 312 months before surgery. Slides of tissue sections stained with hematoxylineosin were reviewed by a pathologist (K. Aozasa), who staged the cancers according to the tumornodemetastasis system of the American Joint Committee on Cancer in 1997 (19).
Reverse TranscriptionPolymerase Chain Reaction
Complementary DNA (cDNA) was synthesized by use of a reverse transcriptionpolymerase chain reaction (RTPCR) kit (Perkin-Elmer Corp., Foster City, CA) from 300 ng of total RNA from each of the prostate cancer cell lines (LNCaP, DU145, and PC-3). PCR was then performed with GR-specific primers (sense 5'-TCCCTTTCTCAACAGCAGGAT-3' and antisense 5'-CAATCATTCCTTCCAGCACAT-3') by a 40-cycle stepdown amplification program that consisted of five cycles of 94 °C for 30 seconds, 69 °C for 45 seconds, and 72 °C for 60 seconds, five cycles of 94 °C for 30 seconds, 64 °C for 45 seconds, and 72 °C for 60 seconds, five cycles of 94 °C for 30 seconds, 59 °C for 45 seconds, and 72 °C for 60 seconds, and 25 cycles of 94 °C for 30 seconds, 54 °C for 45 seconds, and 72 °C for 60 seconds. The primers were designed to span introns (from exons 2 to 4), such that any genomic DNA product would be distinguishable from the 371-base-pair cDNA product by a size difference after the PCR products were separated on a 2% agarose gel and visualized by staining with ethidium bromide. cDNA from HeLa cells was used as a positive control for GR messenger RNA (mRNA) expression. Distilled water was substituted for reverse transcriptase to serve as a negative control. -Actin primers (sense 5'-GTGGGGCGCCCCAGGCACCA-3' and antisense 5'-GTCCTTAATGTCACGCACGATTTC-3') were used to ensure the integrity of the cDNA samples.
Preparation of Cellular Protein and Western Blots
PC-3 and DU145 cells (5 x 105 cells) were seeded on 100-mm tissue culture dishes. The next day, the medium was changed to DMEM with hormone-depleted 5% charcoal-stripped FCS containing each specific dose of dexamethasone or an equivalent volume of ethanol (final concentration = 0.1%). After 48 hours, the cells were washed twice with phosphate-buffered saline (PBS), collected by scraping, suspended in lysis buffer (i.e., 50 mM TrisHCl [pH 7.4], 1% Nonidet P-40, 0.5% sodium deoxycholate, 150 mM NaCl, 1 mM phenylmethyl sulfonylfluoride, 1 µg/mL aprotinin, 1 µg/mL leupeptin, 1 µg/mL pepstatin, and 1 mM sodium orthovanadate), incubated for 1 hour on ice, and centrifuged at 10 000g for 10 minutes at 4 °C. For GR expression of LNCaP cells, 5 x 105 cells were seeded on 100-mm tissue culture dishes with RPMI-1640 medium with 10% charcoal-stripped FCS and incubated for 3 days, and the lysate was prepared by the same procedure. After the determination of the protein concentration of the supernatants, the samples were diluted in electrophoresis sample buffer (i.e., 100 mM TrisHCl, 25% glycerol, 2% sodium dodecyl sulfate, 0.01% bromphenol blue [pH 6.8], and 5% -mercaptoethanol) and boiled for 3 minutes. An aliquot (10 µg of total protein) of each sample was loaded on a 7.5% polyacrylamide gel, separated by electrophoresis, and transferred to polyvinylidenefluoride by standard electroblotting techniques. A standard protein marker (Kaleidoscope Prestained Standards; Bio-Rad Laboratories, Hercules, CA) was used to determine the molecular weights of the separated proteins. After blotting, the membrane was blocked with 5% nonfat milk in PBS containing 0.1% Tween-20 (PBS-T) for 12 hours at 4 °C, washed with PBS-T, and incubated with a specific primary antibody (i.e., rabbit polyclonal anti-GR [Santa Cruz Biotechnology, Inc., Santa Cruz, CA] diluted 1 : 1000 in PBS-T; rabbit polyclonal anti-NF-
B p65 [Santa Cruz Biotechnology, Inc.] diluted 1 : 1000 in PBS-T; rabbit polyclonal I
B
[Santa Cruz Biotechnology, Inc.] diluted 1 : 1000 in PBS-T; or mouse monoclonal anti-
-actin [Sigma Chemical Co., St. Louis, MO] diluted 1 : 5000 in PBS-T) for 1 hour at room temperature. The membrane was washed in PBS-T and then incubated with the appropriate alkaline phosphatase-conjugated or horseradish peroxidase-conjugated secondary antibody (Santa Cruz Biotechnology, Inc.) diluted in 1 : 1000 PBS-T for 4560 minutes. The membrane was washed in PBS-T, and then the immunoreactive bands were visualized by exposing the membrane to 5-bromo-4-chloro-3-indolylphosphate-nitro blue tetrazolium phosphatase substrate (Bio-Rad Laboratories, Hercules, CA) (for detection of alkaline phosphatase-conjugated antibodies) or to the enhanced chemiluminescence (ECL) substrate per instructions of the manufacturer (Amersham Pharmacia Biotech, Tokyo, Japan) (for the detection of horseradish peroxidase-conjugated antibodies). Membranes incubated with the ECL reagents were stripped and reprobed for additional proteins as described in the manufacturer's instructions. An isotype-specific rabbit or mouse immunoglobulin was substituted in place of each primary antibody to serve as a negative control. The relative level of each protein was measured by densitometry and compared with that of
-actin. The ratio of the level of each protein to
-actin in ethanol-treated control cells was arbitrarily given a value of 1.0.
Cell Growth Assay
To assess cell growth, we seeded DU145 and PC-3 cells (1.5 x 103 cells per well) in a 96-well culture plate in DMEM with 5% charcoal-stripped FCS. The medium was changed to DMEM with 5% charcoal-stripped FCS containing dexamethasone (109 to 106 M) or an equivalent volume of ethanol (0.1%) the next day (day 1) and 2 days later (day 3). The same procedure was followed for LNCaP cells, with the exception that 3 x 103 cells per well were seeded in a 96-well culture plate in RPMI-1640 medium with 10% charcoal-stripped FCS. On day 6, cell growth was measured with the cell viability MTT [i.e., 3-(4,5-dimethylthiazol-2-yl)-2, 5-diphenyl tetrazolium bromide] assay kit (Chemicon International, Temecula, CA) according to instructions of the manufacturer. Each data point indicates the mean of six determinations from a representative experiment. At least three separate experiments were performed to confirm the results.
Transfection Studies
The pMMTV-Luc reporter, driven by the mouse mammary tumor virus (MMTV) long terminal repeat promoter, was provided by B. O'Malley at Baylor University (Houston, TX). The pRL-CMV Vector (Promega Corp., Madison, WI) was used as an internal control reporter. PC-3, DU145, and LNCaP cells (1 x 105 cells) were seeded in 60-mm dishes 24 hours before transfection. Cells were transfected with 6 µg of DNA (4 µg of pMMTV-Luc and 2 µg of pRL-CMV) according to the "SuperFect Transfection" instructions (Qiagen KK, Tokyo, Japan). After 2 hours, cells were treated with medium supplemented with charcoal-stripped FCS containing either 107 M dexamethasone or 0.1% ethanol (equivalent volume of dexamethasone). Cells were further incubated at 37 °C for 48 hours, washed with PBS, and harvested. Cell lysates were prepared and used in luciferase assays according to the manufacture's recommendations (Promega Corp.). Luciferase activity was calculated relative to the internal control luciferase activity. Dexamethasone-treated samples were compared with ethanol-treated control samples to determine glucocorticoid-dependent MMTV promoter transactivation. Four sets of experiments were performed.
Immunolocalization of NF-B
Forty-eight hours after treatment with 107 M dexamethasone or 0.1% ethanol control, DU145 cells (2 x 104 cells) grown on a two-well culture slide (Becton Dickinson, Franklin Lakes, NJ) were washed in PBS, then fixed in 3.7% formalin in PBS for 15 minutes at room temperature. The cells were permeabilized with 0.2% Triton X-100 in PBS for 15 minutes at room temperature and blocked with 10% FCS in PBS for 1 hour at room temperature. Immunoreactivity of the p65 subunit of NF-B was detected with a specific antibody against p65 (Santa Cruz Biotechnology, Inc.) diluted 1 : 100 in PBS for 1 hour at room temperature. The cells were washed in PBS and then incubated with a rhodamine-labeled goat anti-rabbit secondary antibody (Santa Cruz Biotechnology, Inc.) diluted 1 : 100 in PBS for 45 minutes at room temperature in the dark. Immunofluorescent cells were photographed with a Nikon Microphot-FXA photomicroscope (Nikon Corp., Tokyo, Japan). As a negative control, blocking peptide (Santa Cruz Biotechnology, Inc.) for anti-NF-
B p65 was preincubated with anti-NF-
B p65 according to the instructions of the manufacturer. Negative control cells showed low background immunofluorescence. Only cells showing more intense immunofluorescence than any of the negative control cells were determined to be positive. To show size and nuclei of the cells, we fixed ethanol-treated control cells by the same procedure and stained them with hematoxylin for 5 minutes at room temperature.
IL-6 Assay
DU145 or PC-3 cells (5 x 105 cells) were seeded on 100-mm tissue culture dishes. The next day, the medium was removed and replaced with DMEM containing 5% charcoal-stripped FCS and containing each specific dose of dexamethasone. Control cells were treated with 0.1% ethanol. After 48 hours, the chemiluminescent enzyme immunoassay kit (Fujirebio Inc., Tokyo, Japan) was used to assay for IL-6 in each culture medium. IL-6 levels from each treatment were evaluated as the mean ± 95% confidence interval (CI) of four separate samples. Two independent assays were performed. This IL-6 assay detects between 0.2 and 1000 pg/mL of human IL-6 and does not cross-react with human IL-1, IL-1
, IL-4, granulocyte colony-stimulating factor, macrophage colony-stimulating factor, epidermal growth factor, TNF-
, and soluble IL-6 receptor. Human recombinant IL-6 standards (0, 20, 400, and 1000 pg/mL) (Fujirebio Inc.) were used to generate a standard curve.
In Vivo Xenograft Model
Animal care was in accordance with the laboratory animal guidelines of the Institute of Experimental Animal Sciences in Osaka University Medical School. To establish DU145 tumors in mice, DU145 cells were detached with trypsin and resuspended in DMEM with 10% FCS. Six-week-old male athymic nude or severe combined immunodeficiency (SCID) mice were each given a single subcutaneous injection in the dorsal area of 0.5 x 107 cells (nude mice, n = 6) or 1 x 107 cells (SCID mice, n = 6) in 0.1 mL of DMEM. Three times a week, the six mice were each given a subcutaneous injection at peritumor site of dexamethasone (1 µg per mouse per injection), which had been dissolved in ethanol and diluted 1 : 2000 in sterile saline immediately before injection. The dexamethasone treatment was started at the time of cell inoculation. Six control mice were given an injection of ethanol, which had been diluted 1 : 2000 in sterile saline. The tumor volumes were measured weekly with a slide caliper and determined by the following formula: (length x width2)/2. At the completion of the experiments, the mice were killed, and tumors from the dexamethasone-treated or ethanol-treated SCID mice were removed for immunohistochemical studies.
Immunohistochemical Analysis
For the determination of GR expression in tissue sections, surgical specimens of human prostate cancers or DU145 xenograft tumors were fixed in 10% buffered formalin, processed, and embedded in paraffin. Serial tissue sections (5 µm thick) were obtained and mounted on slides that were then deparaffinized, rehydrated, and incubated with 3% (vol/vol) hydrogen peroxide in PBS for 15 minutes at room temperature to inhibit endogenous peroxidase activity. The sections were then blocked with 10% bovine serum albumin for 15 minutes at 37 °C and incubated for 4 hours at 37 °C with a rabbit polyclonal anti-GR (Santa Cruz Biotechnology, Inc.) at a dilution of 1 : 100 in PBS. The sections were then rinsed with PBS three times, incubated with a peroxidase-labeled anti-rabbit immunoglobulin antibody (Bio-Rad Laboratories, Richmond, CA) at a dilution of 1 : 1000 in PBS for 10 minutes at 37 °C, and exposed to avidinbiotinperoxidase complex (Dako kit; Dako Corp., Carpinteria, CA) according to the instructions of the manufacturer. The sections were reacted with 3,3'-diaminobenzidine as the color-developing reagent and counterstained with hematoxylin. An isotype-specific rabbit immunoglobulin was substituted in place of the primary anti-GR antibody to serve as a negative control.
The sections were scanned under a Nikon microscope (Nikon Corp.), at magnifications of x40, x100, x200, and x400, and the area containing the greatest number of positive cancer cells was selected for each sample. Only cancer cells that showed intense nuclear staining were scored as positive. The number of GR-positive cells per 500 cancer cells was counted and expressed as a percentage. The average percent GR-positive cells among normal epithelial cells in the cancer sections was used to determine the cut point between high and low GR expression. A high level of GR expression was defined as at least 30% GR-positive cells, and a low level was defined as less than 30% GR-positive cells. The intensity of the immunoreactivity was not considered in determining the level of GR expression.
Statistical Analysis
The statistical significance of the results was analyzed by unpaired Student's t test, and P<.05 was considered to be statistically significant. For multiple comparisons, the level of statistical significance assigned to the P value was adjusted for the total number of comparisons (n), such that P<.05/n. The level of statistical significance was confirmed by MannWhitney U test. All statistical analyses were performed by use of the StatView software (SAS Institute Inc., Cary, NC). All statistical tests were two-sided.
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RESULTS |
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We hypothesized that glucocorticoids act directly through GRs to inhibit tumor growth. To test this hypothesis, we first examined GR mRNA and protein expression in the human prostate cancer cell lines LNCaP, DU145, and PC-3 by RTPCR and western blot analysis, respectively. GR-specific mRNA and protein were detected in DU145 and PC-3 cells but not in LNCaP cells (Fig. 1, A and B). HeLa cells were used as a positive control for GR mRNA and protein expression (data not shown). We tested whether the cell lines expressed functional GRs with the use of the MMTV luciferase reporter gene assay. Glucocorticoid-dependent MMTV promoter transactivation was observed in DU145 and PC-3 cells but not in LNCaP cells (data not shown).
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To determine whether dexamethasone (109 to 106 M) affects the growth of prostate cancer cells in vitro, we performed 5-day cell growth assays. Compared with the growth of ethanol-treated control cells, the growth of DU145 cells was statistically significantly lower in those cultures treated with dexamethasone concentrations of greater than 108 M (108 M, P = .001; 107 M, P<.001; and 106 M, P<.001) (Fig. 1, D). The growth-inhibitory effect was dose dependent between 109 and 107 M, with a plateau effect seen at higher concentrations of dexamethasone. By contrast, compared with the growth of ethanol-treated control cells, the growth of PC-3 cells was statistically significantly lower only in those cultures treated with a dexamethasone concentration of 107 M (P = .009) (Fig. 1, D
). The growth of PC-3 cells was not statistically significantly inhibited by 106 M dexamethasone, presumably because GR levels were decreased by dexamethasone treatment (Fig. 1, C
). There was no statistically significant inhibition of growth in LNCaP cells treated with dexamethasone (Fig. 1, D
), which corresponded to the absence of GRs in these cells (Fig. 1, A and B
). Because of the growth-inhibitory effect in DU145 cells treated with a broad range of dexamethasone concentrations (108 to 106 M), we concentrated our efforts on this cell line for subsequent experiments.
Elucidating the Mechanism of Dexamethasone-Mediated Growth Inhibition: Importance of NF-B, I
, and IL-6
Glucocorticoids have been shown to cooperate with other transcription factors in modulating gene expression (20). One such transcription factor is NF-B (13). We assessed the effects of dexamethasone on members of the NF-
B transcription factor family to elucidate the mechanism by which dexamethasone may inhibit DU145 cell growth. DU145 cells were treated with dexamethasone (108 to 105 M) for 48 hours, and the protein levels of p65, one of the components of NF-
B, and I
B
, one of the natural cytoplasmic inhibitors of NF-
B, were analyzed by western blot analyses. There was a dose-dependent increase in I
levels but not in NF-
levels in dexamethasone-treated cells (Fig. 2, A
). To determine whether the increased levels of I
prevented nuclear translocation of NF-
B, we examined the subcellular localization of NF-
B in DU145 cells by indirect immunofluorescence. NF-
B localized to both the nuclear and cytoplasmic compartments in control ethanol-treated DU145 cells (Fig. 2, B
). However, NF-
B localized only to the cytoplasmic compartment, which was accompanied by a loss in localization to the nuclear compartment, in dexamethasone-treated DU145 cells (Fig. 2, B
).
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Effects of Dexamethasone on DU145 Xenograft Growth
We next determined whether dexamethasone could also inhibit the growth of androgen-independent prostate DU145 tumors in vivo. Because we previously demonstrated the clinical benefits of low-dose dexamethasone for patients with HRPC (7), we wanted to mimic a similar low-dose dexamethasone regimen in the xenograft model. We selected a dose of 1 µg per mouse three times per week because this low dose effectively inhibited the in vivo growth of another type of adenocarcinoma cells (22). Athymic nude mice, which lack T cells, were first given an injection subcutaneously of DU145 tumor cells. On the same day, the mice were started on the regimen of dexamethasone treatments. After 8 weeks, the mean tumor volume in the dexamethasone-treated mice was 333 mm3 (95% CI = 267 mm3 to 399 mm3), statistically significantly smaller (P = .006) than that in the ethanol-treated control mice (731 mm3; 95% CI = 651 mm3 to 811 mm3) (Fig. 3, A).
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GR Expression in DU145 Xenograft and Human Prostate Cancers
To determine whether in vivo administration of low-dose dexamethasone alters the level of GRs, after 7 weeks of low-dose dexamethasone treatment, we harvested the DU145 xenografts from the SCID mice and examined GR expression by immunohistochemistry. GRs were readily detected in xenograft tumors from the ethanol-treated control (Fig. 4, A) and low-dose dexamethasone-treated (Fig. 4, B
) groups, suggesting that GR levels in DU145 tumor cells were maintained under the long-term administration of low-dose dexamethasone.
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DISCUSSION |
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To our knowledge, only one previous study (24) addressed GR status in human prostate cancer. The investigators of that study reported that, in radical prostatectomy specimens from patients without preoperative AAT, GR expression was lower in tumor epithelial cells than in tumor stromal cells. In our study, we compared GR expression in the cancers of patients who did and did not receive preoperative AAT. Because the cancers of six of 11 patients treated with AAT had high GR levels, androgen-independent prostate cancer cells may be potential targets for glucocorticoid-based therapies, even if after ATT not all of the residual cancer cells are androgen independent.
The mechanism responsible for the antiproliferative effect of glucocorticoids is poorly understood. One mechanism is a direct effect on cell cycle regulatory proteins. The glucocorticoidGR complex mediates cell cycle arrest in several cell types, including human osteosarcoma cells, human cervical carcinoma cells, rat hepatoma cells, and human lymphocytes (2528). When we analyzed the cell cycle distribution of dexamethasone-treated DU145 cells, we found that cells accumulated in the G1 phase, which was associated with increased levels of the cell cycle regulatory protein p27 but not p21 (data not shown). Because GR-mediated growth arrest is cell type specific (25), further study is required to clarify the involvement of p27 and p21 in prostate cancer cells.
A second mechanism by which glucocorticoids may exert their antiproliferative effects is through the modulation of growth-related cytokines or their transcriptional regulators. The transcription factor NF-B is constitutively activated in DU145 cells (29), and its activation is implicated in the control of cell proliferation and apoptosis in many tumors (3032). Because glucocorticoids are potent inhibitors of NF-
B activation in cultured cells (33), inactivation of NF-
B may be an essential mechanism involved in GR-mediated growth inhibition of DU145 cells. Our data indicate that, in response to dexamethasone, NF-
B accumulates in the cytosol of treated cells. This accumulation is accompanied by an increase in I
B
protein levels and a decrease in secreted IL-6 levels, an NF-
B-inducible gene. Thus, because IL-6 has been implicated as an autocrine growth factor for androgen-independent prostate cancer cells (14,15), the antiproliferative effects of dexamethasone may be mediated through the inhibition of an NF-
BIL-6-dependent pathway. Consistent with previous reports (14,15), the addition of antibodies to IL-6 inhibited the growth of DU145 cells in vitro (data not shown). A recent study (34) showed that PC-3 xenograft tumors regressed after the in vivo administration of antibodies to IL-6. Moreover, patients with HRPC were reported to have elevated serum IL-6 levels (35). We measured IL-6 levels in serum from patients with HRPC who had been treated with low-dose dexamethasone therapy (7) and found that the mean IL-6 levels declined from 5.4 pg/mL (95% CI = 1.9 pg/mL to 8.9 pg/mL) to 1.2 pg/mL (95% CI = 0.9 pg/mL to 1.5 pg/mL). Taken together, these results and observations suggest that the inhibition of IL-6 production by the cancer cells may be a major mechanism responsible for dexamethasone-mediated antitumor activity against HRPC.
Although the growth-inhibitory effect of dexamethasone alone is not dramatic, combinations with other chemotherapeutic agents may enhance its antiproliferative activity. Because NF-B activation is implicated as a principal mechanism of inducible tumor chemoresistance (36), NF-
B inactivation by dexamethasone may substantially augment and prolong chemosensitivity. Therefore, our results may provide a basis for developing improved protocols for dexamethasone therapy alone or in combination with chemotherapy agents for treating patients with HRPC.
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NOTES |
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We thank Naoko Matsumoto, Kyoko Adachi, and Yukako Morioka (Osaka University) for technical assistance.
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Manuscript received February 15, 2001; revised August 28, 2001; accepted September 12, 2001.
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