Methyl 2-Cyano-3,11-dioxo-18{beta}-olean-1,12-dien-30-oate Is a Peroxisome Proliferator-Activated Receptor-{gamma} Agonist That Induces Receptor-Independent Apoptosis in LNCaP Prostate Cancer Cells

doi:10.1124/mol.107.041285

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Molecular Pharmacology Fast Forward
First published on November 7, 2007; DOI: 10.1124/mol.107.041285

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Mol Pharmacol 73:553-565, 2008

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Methyl 2-Cyano-3,11-dioxo-18β-olean-1,12-dien-30-oate Is a Peroxisome Proliferator-Activated Receptor- ${gamma}$ Agonist That Induces Receptor-Independent Apoptosis in LNCaP Prostate Cancer Cells

Sabitha Papineni, Sudhakar Chintharlapalli, and Stephen Safe

Department of Veterinary Physiology and Pharmacology, Texas A&M University, College Station, Texas (S.P., S.S.); and Institute of Biosciences and Technology, Texas A&M Health Science Center, Houston, Texas (S.C., S.S.)

Received August 28, 2007; accepted November 7, 2007

Abstract

Top
Abstract
Materials and Methods
Results
Discussion
References

Methyl 2-cyano-3,11-dioxo-18β-olean-1,12-diene-30-oate(β-CDODA-Me) is a synthetic analog of the naturally occurringtriterpenoid glycyrrhetinic acid, which contains a 2-cyano substituentin the A-ring. β-CDODA-Me was a potent inhibitor of LNCaPprostate cancer cell growth (IC₅₀ $~$ 1 µM) and activatedperoxisome proliferator-activated receptor ${gamma}$ (PPAR ${gamma}$ ), whereasanalogs without the cyano group were weakly cytotoxic and didnot activate PPAR ${gamma}$ . β-CDODA-Me induced p21 and p27, down-regulatedcyclin D1 protein expression, and induced two other proapoptoticproteins, namely nonsteroidal anti-inflammatory drug-activatedgene-1 and activating transcription factor-3. However, inductionof these responses by β-CDODA-Me was PPAR ${gamma}$ -independent anddue to activation of phosphatidylinositol-3-kinase, mitogen-activatedprotein kinase, and jun N-terminal kinase pathways by this compound.In contrast, β-CDODA-Me also decreased androgen receptor(AR) and prostate-specific antigen (PSA) mRNA and protein levelsthrough kinase-independent pathways. β-CDODA-Me repressedAR mRNA transcription, whereas decreased PSA mRNA levels weredependent on protein synthesis and were reversed by cycloheximide.Thus, potent inhibition of LNCaP cell survival by β-CDODA-Meis due to PPAR ${gamma}$ -independent activation of multiple pathways thatselectively activate growth-inhibitory and proapoptotic responses.

Peroxisome proliferator-activated receptors (PPARs) are a subfamilyof the nuclear receptor superfamily of ligand-activated receptors(Mangelsdorf et al., 1995

). The three members of this family,PPAR ${alpha}$ , PPAR ${gamma}$ , and PPARβ/ ${sigma}$ , are lipid sensors and play a keyrole in regulating tissue-specific lipid homeostasis and metabolism(Lee et al., 2003

). PPARs also play an important role in manydiseases, particularly those related to obesity, metabolic disorders,cancer, and atherogenesis (Escher and Wahli, 2000

; Lee et al.,2003

). Endogenous ligands for PPARs include fatty acid-derivedcompounds and 15-deoxy- ${Delta}$ ^12,14-prostaglandin J2 (PGJ2), whichexhibits high affinity for PPAR ${gamma}$ ; however, PGJ2 may not be theendogenous ligand for this receptor because of the low cellularexpression of this metabolite. Synthetic PPAR ${gamma}$ agonists, suchas the thiazolidinediones rosiglitazone and pioglitazone, areinsulin-sensitizing drugs that are widely used for clinicaltreatment of type II diabetes.

Several different structural classes of PPAR ${gamma}$ agonists have beencharacterized, and these include flavones, various indole derivatives,and triterpenoids such as 2-cyano-3,12-dioxo-17 ${alpha}$ -olean-1,9-dien-28-oicacid (CDDO) and related compounds (Honda et al., 1998; Rieussetet al., 2002; Berger et al., 2003; Qin et al., 2004; Schopferet al., 2005). PPAR ${gamma}$ is overexpressed in many tumor types andcancer cell lines (Ikezoe et al., 2001), and PPAR ${gamma}$ agonists showpromise for the clinical treatment of various types of tumors(Kubota et al., 1998; Chang and Szabo, 2000; Gupta et al., 2003;Qin et al., 2004). Ligands for this receptor typically inhibitG₀/G₁-to S-phase progression, and this is accompanied by down-regulationof cyclin D1 expression and induction of the cyclin-dependentkinase inhibitors p27 or p21. Research from our laboratory hasidentified a series of 1,1-bis(3'-indolyl)-1-(p-substitutedphenyl)methanes [methylene-substituted diindolyl-methanes (C-DIMs)],which inhibit cancer cell and tumor growth (Chintharlapalliet al., 2004, 2005a, 2007b; Hong et al., 2004; Qin et al., 2004;Abdelrahim et al., 2006) through both receptor-dependent andindependent pathways, and similar observations have been reportedfor other PPAR ${gamma}$ agonists (Clay et al., 2002; Konopleva et al.,2004; Samudio et al., 2005; Yang et al., 2006).

A new class of synthetic PPAR ${gamma}$ agonists has been derived fromglycyrrhetinic acid (GA), a major triterpenoid acid found inlicorice extracts. Methyl 2-cyano-3,11-dioxo-18β-olean-1,12-dien-30-oate(β-CDODA-Me) is a 2-cyano derivative of GA and has thesame oleanolic acid pentacyclic triterpene backbone structureas CDDO, which is also a 2-cyano derivative of oleanolic acid(Honda et al., 1998). However, there are major structural differencesbetween CDODA and CDDO with respect to the position of the carboxylicacid group in the E-ring, the position of the double bonds andketo group in the C-ring. We reported recently that the 18 ${alpha}$ and18β isomers of CDODA-Me activate PPAR ${gamma}$ in colon cancer cellsand induced both caveolin-1 and Krüppel-like Factor-4 throughreceptor-dependent pathways (Chintharlapalli et al., 2007a).In this study, we investigated the effects of β-CDODA-Meon the proliferation of LNCaP prostate cancer cells, and theIC₅₀ value for growth inhibition was approximately 1 µM.In contrast to studies in colon cancer cells, β-CDODA-Mehad minimal effects on caveolin-1 or Krüppel-like Factor-4expression in LNCaP cells. The proapoptotic and growth-inhibitoryeffects of β-CDODA-Me in LNCaP cells were associated withthe induction of p21 and p27 expression, down-regulation ofcyclin D1, and induction of nonsteroidal anti-inflammatory drug-activatedgene 1 (NAG-1). β-CDODA-Me also decreased androgen receptor(AR) and prostate-specific antigen (PSA) protein and RNA expression,and all of these responses were PPAR ${gamma}$ -independent. Thus, β-CDODA-Me,a PPAR ${gamma}$ agonist, inhibited growth and induced apoptosis in LNCaPcells through activation of multiple receptor-independent pathways,including ablation of AR gene expression.

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
References

Cell Lines. LNCaP, PC3, and DU145 human prostate carcinoma cellswere obtained from American Type Culture Collection (Manassas,VA). Fetal bovine serum was obtained from JRH Biosciences (Lenexa,KS). LNCaP, PC3, and DU145 cells were maintained in RPMI 1640medium (Sigma Chemical, St. Louis, MO) supplemented with 0.22%sodium bicarbonate, 0.011% sodium pyruvate, 0.45% glucose, 0.24%HEPES, 10% FBS, and 10 ml/l 100x antibiotic/antimycotic solution(Sigma). Cells were maintained at 37°C in the presence of5% CO₂.

Antibodies and Reagents. Antibodies for poly(ADP-ribose) polymerase,cyclin D1, p27, FKBP51, AR, ATF3, Akt, and caveolin-1 were purchasedfrom Santa Cruz Biotechnology, Inc. (Santa Cruz, CA). PSA wasobtained from Dako Denmark A/S (Glostrup, Denmark); NAG-1 waspurchased from Upstate Biotechnology (Charlottesville, VA);and EGR-1, pAKT, phosphorylated extracellular signal-regulatedkinase, extracellular signal-regulated kinase, pJNK, and JNKwere obtained from Cell Signaling Technology Inc. (Danvers,MA). Monoclonal β-actin antibody and dihydrotesterone werepurchased from Sigma-Aldrich. Reporter lysis buffer and luciferasereagent for luciferase studies were purchased from Promega (Madison,WI). β-Galactosidase reagent was obtained from Tropix (Bedford,MA), and Lipofectamine reagents were supplied by Invitrogen(Carlsbad, CA). Western blotting chemiluminescence reagentswere from PerkinElmer Life and Analytical Sciences (Waltham,MA). The PPAR ${gamma}$ antagonist T007 was prepared in this laboratory,and the synthesis of the GA derivatives has been described previously(Chintharlapalli et al., 2007a).

Cell Proliferation and DNA Fragmentation Assays. LNCaP prostatecancer cells (2 x 10⁴/well) were added to 12-well plates andallowed to attach for 24 h. The medium was then changed to DMEM/Ham'sF-12 media containing 2.5% charcoal-stripped FBS, and eithervehicle (DMSO) or the indicated compounds were added. Freshmedium and indicated compounds were added every 48 h, and cellswere then trypsinized and counted after 2, 4, and 6 days usinga Coulter Z1 cell counter (Beckman Coulter, Fullerton, CA).Each experiment was done in triplicate, and results are expressedas means ± S.E. for each set of three experiments. TheDNA fragmentation assay was performed using an Apoptotic DNAladder extraction kit (BioVision, Mountain View, CA) accordingto the manufacturer's protocol.

Transfections. The Gal4 reporter construct containing 5x Gal4response elements (pGal4) was kindly provided by Dr. Marty Mayo(University of North Carolina, Chapel Hill, NC). The Gal4DBD-PPAR ${gamma}$ construct was a gift of Dr. Jennifer L. Oberfield (Glaxo SmithKline,Research Triangle Park, NC). The PPRE-luc construct containsthree tandem PPREs with a minimal TATA sequence linked to theluciferase gene in pGL2. The AR-luc construct containing the-5400 to +580 region of the androgen receptor promoter was providedby Dr. Donald J. Tindall (Mayo Clinic, Rochester, MN), and thePSA-luc construct containing the 5.8-kilobase region of thePSA promoter was provided by Dr. Hong-Wu Cheng (University ofCalifornia, Davis, CA). LNCaP cells (1 x 10⁵) were seeded in12-well plates in DMEM/Ham's F-12 media supplemented with 2.5%charcoal-stripped FBS and grown overnight. Transient transfectionswere performed using Lipofectamine reagent (Invitrogen) accordingto the protocol provided by the manufacturer. Transfection studieswere performed using 0.4 µg of Gal4Luc, 0.04 µgof β-galactosidase, 0.04 µg of Gal4DBD-PPAR ${gamma}$ , 0.4µg of AR-luc, and 0.3 µg of PSA-luc. Six hours aftertransfection, the transfection mix was replaced with completemedia containing either vehicle (DMSO) or the indicated ligandfor 20 to 22 h. Cells were then lysed with 100 µl of 1xreporter lysis buffer, and 30 µl of cell extract was usedfor luciferase and β-galactosidase assays. A Lumicountluminometer (PerkinElmer Life and Analytical Sciences) was usedto quantify luciferase and β-galactosidase activities,and the luciferase activities were normalized to β-galactosidaseactivity.

Fluorescence-Activated Cell Sorting Analysis. LNCaP cells weretreated with either the vehicle (DMSO) or the compound for 24h. Cells were trypsinized, centrifuged, and resuspended in stainingsolution containing 50 µg/ml propidium iodide, 4 mM sodiumcitrate, and 30 U/ml RNase. After incubation at room temperaturefor 1 h, cells were analyzed on a FACSVantage SE DiVa (BD Biosciences,San Jose, CA), using BD FACSDiva software, version 4.1.1. Propidiumiodide (PI) fluorescence was collected through a 610SP bandpassfilter, and list mode data were acquired on a minimum of 50,000single cells defined by a dot plot of PI width versus PI area.Data analysis was performed in BD FACSDiva software version4.1.1 using PI width versus PI area to exclude cell aggregates.

Real-Time PCR. Total RNA was isolated using the RNeasy ProtectMini kit (QIAGEN, Valencia, CA) according to the manufacturer'sprotocol. RNA was eluted with 30 µl of RNase-free waterand stored at -80°C. RNA was reverse-transcribed using SuperscriptII reverse transcriptase (Invitrogen) according to the manufacturer'sprotocol. cDNA was prepared from the LNCaP cell line using acombination of oligodeoxythymidylic acid and dNTP mix (AppliedBiosystems, Foster City, CA) and Superscript II (Invitrogen).Each PCR was carried out in triplicate in a 25-µl volumeusing SYBR Green Master mix (Applied Biosystems) for 15 minat 95°C for initial denaturing, followed by 40 cycles of95°C for 30 s and 60°C for 1 min in the ABI Prism 7700sequence detection system (Applied Biosystems). The ABI DissociationCurves software was used after a brief thermal protocol (95°Cfor 15 s and 60°C for 20 s, followed by a slow ramp to 95°C)to control for multiple species in each PCR amplification. Thecomparative CT method was used for relative quantitation ofsamples. Values for each gene were normalized to expressionlevels of TATA-binding protein. Primers were purchased fromIntegrated DNA Technologies (Coralville, IA). The sequencesof the primers used for reverse transcription-PCR were as follows:AR: forward, 5'-GTA CCC TGG CGG CAT GGT-3', and reverse, 5'-CCCATT TCG CTT TTG ACA CA-3'; PSA: forward, 5'-GCA TTG AAC CAGAGG AGT TCT TG-3', and reverse, 5'-TTG CGC ACA CAC GTC ATT G-3';and TATA-binding protein: forward, 5'-TGC ACA GGA GCC AAG AGTGAA-3', and reverse, 5'-CAC ATC ACA GCT CCC CAC CA-3'.

Western Blot Analysis. Cells were seeded in DMEM/Ham's F-12media containing 2.5% charcoal-stripped FBS for 24 h and thentreated with either the vehicle (DMSO) or the indicated compounds.Cells were collected by scraping in 150 µl of high-saltlysis buffer [50 mM HEPES, 0.5 M NaCl, 1.5 mM MgCl₂, 1 mM EGTA,10% (v/v) glycerol, 1% (v/v) Triton X-100, and 5 µl/mlProtease Inhibitor Cocktail (Sigma)]. The lysates were incubatedon ice for 1 h with intermittent vortexing followed by centrifugationat 20,000g for 10 min at 4°C. Before electrophoresis, sampleswere boiled for 3 min at 100°C; the amount of protein wasdetermined, and 60 µg of protein was applied per lane.Samples were subjected to SDS-polyacrylamide gel electrophoresison 10% gel at 120 V for 3 to 4 h. Proteins were transferredon to polyvinylidene difluoride membrane (Bio-Rad Laboratories,Hercules, CA) at 0.9 V for 90 min at 4°C in 1x transferbuffer (48 mM Tris-HCl, 39 mM glycine, and 0.025% SDS). Themembranes were blocked for 30 min with 5% TBST-Blotto (10 mMTris-HCl, 150 mM NaCl, pH 8.0, 0.05% Triton X-100, and 5% nonfatdry milk) and incubated in fresh 5% TBST-Blotto with primaryantibody overnight with gentle shaking at 4°C. After washingwith TBST for 10 min, the polyvinylidene difluoride membranewas incubated with secondary antibody (1:5000) in 5% TBST-Blottofor 2 to 3 h. The membrane was washed with TBST for 10 min andincubated with 10 ml of chemiluminescence substrate (PerkinElmerLife Sciences) for 1.0 min and exposed to ImageTeK-H medicalimaging film (Eastman American X-Ray Supply, Inc., Rochester,NY).

Statistical Analysis. Statistical differences between differentgroups were determined by analysis of variance and Scheffe'stest for significance. The data are presented as mean ±S.E. for at least three separate determinations for each treatmentgroup.

Results

Top
Abstract
Materials and Methods
Results
Discussion
References

Cytotoxicity of β-CDODA-Me and Activation of PPAR ${gamma}$ . β-DODAor 1,2-dehydro-GA exhibited minimal inhibition of LNCaP cellgrowth with an IC₅₀ value >15 µM, whereas the IC₅₀value for the corresponding methyl ester derivative was between10 and 15 µM (Fig. 1A). Introduction of a 2-cyano groupto give β-CDODA-Me increased the cytotoxicity by at leastan order of magnitude, and the IC₅₀ value was approximately1 µM in LNCaP cells (Fig. 1A). These results were similarto those observed in colon cancer cells (Chintharlapalli etal., 2007a) and demonstrate the importance of 2-cyano substituentsin mediating the cytotoxicity of GA derivatives. Figure 1B showsthat decreased LNCaP cell survival induced by β-CDODA-Mewas not affected after cotreatment with the PPAR ${gamma}$ antagonistT007, suggesting that the cytotoxicity of this compound wasreceptor-independent. β-CDODA-Me was also cytotoxic toandrogen-insensitive PC3 and DU145 prostate cancer cells (Fig. 1C).The induction of PPAR ${gamma}$ -dependent transactivation by β-CDODA-Mewas also investigated in LNCaP cells transfected with PPAR ${gamma}$ -GAL4/GAL4-Lucor PPRE₃-Luc constructs and treated with 1 to 5 µM concentrations.β-CDODA-Me significantly induced luciferase activity (Fig. 1D),and in cells cotreated with β-CDODA-Me plus 10 µMT007 (a PPAR ${gamma}$ antagonist), there was significant inhibition ofinduced transactivation. In contrast, β-DODA-Me did notactivate PPAR ${gamma}$ (data not shown), demonstrating the requirementfor the 2-cyano substituent to confer PPAR ${gamma}$ agonist activityon the GA derivative.

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Fig. 1. Effects of β-CDODA-Me and related compounds on LNCaP cell survival and activation of PPAR ${gamma}$ . Cell survival of LNCaP (A and B), PC3, and DU145 (C) cells. Prostate cancer cells were treated with different concentrations of β-DODA, β-DODA-Me, or β-CDODA-Me alone or in combination with 5 µM T007 (C) for 96 h, and the percentage of cell survival relative to DMSO (solvent control set at 100%) was determined as described under Materials and Methods. Results are expressed as means ± S.E. for three separate determinations for each treatment group, and significantly (p < 0.05) decreased survival is indicated (^*). D, β-CDODA-Me activates PPAR ${gamma}$ . LNCaP cells were treated with β-CDODA, T007, or their combination, transfected with PPAR ${gamma}$ -GAL4/pGAL4 or PPRE-luc, and luciferase activity determined as described under Materials and Methods. Results are expressed as means ± S.E. for three replicate determinations for each treatment group, and significant (p < 0.05) induction by β-CDODA-Me (^*) and inhibition after cotreatment with T007 (^**) are indicated.

PPAR ${gamma}$ agonists typically modulate the expression of one or moreof the cell cycle proteins p27, p21, and cyclin D1, and Fig. 2Aillustrates the effects of 1 to 5 µM β-CDODA-Me onthe expression of these proteins in LNCaP cells. There was aconcentration-dependent induction of p27 and p21 and a decreasein cyclin D1 proteins and retinoblastoma protein phosphorylationin cells treated with β-CDODA-Me alone, and similar resultswere observed in cells cotreated with the PPAR ${gamma}$ antagonist T007and β-CDODA-Me (Fig. 2B), suggesting that these responseswere PPAR ${gamma}$ -independent. FACS analysis of LNCaP cells treatedwith different concentrations of β-CDODA-Me indicated that1 µM β-CDODA-Me did not affect the percentage ofcells in G₀/G₁, S, or G₂/M, whereas at higher concentrations,the percentage of cells in these phases of the cell cycle decreased(Fig. 2C). β-CDODA-Me induced a concentration-dependentincrease in the percentage of apoptotic sub-G₁ LNCaP cells,and the proapoptotic effects of this compound were also observedin PC3 and DU145 cells (Fig. 2D), in which β-CDODA-Me inducedcaspase-dependent PARP cleavage. Thus, the overall cytotoxicityof β-CDODA-Me in prostate cancer cells was associated withboth inhibition of growth and induction of apoptosis.

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Fig. 2. β-CDODA-Me modulates the cell cycle and cell cycle genes and induces apoptosis in prostate cancer cells. Modulation of cell cycle genes by β-CDODA-Me alone (A) and in combination with T007 (B). Cells were treated as indicated for 24 h, and whole-cell lysates were analyzed by Western blot analysis as described under Materials and Methods. C, cell cycle progression. LNCaP cells were treated with DMSO and different concentrations of β-CDODA-Me for 24 h and analyzed for the percentage of distribution of cells in different phases of the cell cycle by FACS analysis as described under Materials and Methods. Results are expressed at means ± S.E. for three replicate determinations, and significant (p < 0.05) changes (compared with DMSO group) are indicated by an asterisk. D, induction of PARP cleavage. PC3 and DU145 cells were treated for 24 h with different concentrations of β-CDODA-Me, and whole-cell lysates were analyzed by Western blots as described under Materials and Methods.

Induction of Proapoptotic Responses by β-CDODA-Me. NAG-1and ATF-3 are proapoptotic proteins induced by PPAR ${gamma}$ agonists,and results in Fig. 3A show that 1 to 5 µM β-CDODA-Meinduced NAG-1 and ATF-3, which are often coinduced, and thiswas accompanied by caspase-dependent PARP cleavage, DNA fragmentation,and decreased bcl2 expression in LNCaP cells. In addition, theDNA laddering response was not affected after cotreatment withthe PPAR ${gamma}$ antagonist T007 (Fig. 3B). In LNCaP cells cotreatedwith β-CDODA-Me plus T007 (Fig. 3C), the induced responseswere not inhibited by the PPAR ${gamma}$ antagonist, indicating that inductionof these proapoptotic responses was receptor-independent. Previousstudies show that different structural classes of PPAR ${gamma}$ agonistsdown-regulate AR expression in LNCaP cells, and this responsecan also result in the activation of apoptosis (Yang et al.,2006; Chintharlapalli et al., 2007b). Figure 3D summarizes theeffects of β-CDODA-Me on AR expression in the presenceor absence of 10 nM DHT and on the expression of FKBP51 andPSA, two androgen-responsive genes in LNCaP cells. DHT increasesexpression of AR as a result of stabilization of the receptorand induces both androgen-responsive FKBP51 and PSA genes; incells treated with 1 to 5 µM β-CDODA-Me, there wasa concentration-dependent decrease in AR, PSA, and FKBP51 expressionin the presence or absence of DHT. In addition, down-regulationof AR, PSA, and FKBP51 proteins in LNCaP cells treated withβ-CDODA-Me was not affected by cotreatment with the PPAR ${gamma}$ antagonist T007 or the proteasome inhibitor MG132 (Fig. 3E).In contrast, β-CDODA-Me-dependent degradation of cyclinD1 was inhibited after cotreatment with MG132, and these observationsare similar to those reported for other PPAR ${gamma}$ agonists that induceproteasome-dependent degradation of cyclin D1 (Chintharlapalliet al., 2004, 2005a,b). These results clearly show that β-CDODA-Medecreases expression of androgen-responsive genes and AR throughPPAR ${gamma}$ -independent pathways. The down-regulation of AR in cellstreated with β-CDODA-Me is consistent with the inductionof apoptosis by this compound because decreased AR expressionby small inhibitory RNAs in LNCaP cells also induces apoptosis(Liao et al., 2005).

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Fig. 3. β-CDODA induces apoptotic pathways and decreases androgen-responsiveness in LNCaP cells. β-CDODA-Me alone (A) and in combination with T007 (B and C) induces proapoptotic pathways. LNCaP cells were treated as indicated for 24 h, and whole-cell lysates were analyzed by Western blot analysis as described under Materials and Methods. β-CDODA-Me-induced DNA fragmentation (A and B) was also determined as described. Effects of β-CDODA-Me alone and in combination with DHT or T007 (D) or MG132 (E) on AR and androgen-responsive proteins. LNCaP cells were treated with DMSO or the various compounds for 24 h, and whole-cell lysates were analyzed by Western blot analysis as described under Materials and Methods.

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Fig. 4. β-CDODA-Me induces proapoptotic proteins and kinases. Induction of NAG-1, ATF3, and Egr-1 (A) and kinases (B) by β-CDODA-Me. LNCaP cells were treated with 2.5 µM β-CDODA-Me, and whole-cell lysates isolated at different times after treatment were analyzed by Western blot analysis as described under Materials and Methods. Effects of kinase inhibitors on proapoptotic responses (C) and quantitation of NAG-1 and ATF3 expression (D). LNCaP cells were treated with 2.5 µM β-CDODA alone or in combination with various kinase inhibitors, and after 24 h, whole-cell lysates were analyzed by Western blot analysis. Levels of NAG-1 and ATF3 proteins (normalized to β-actin) (D) are means ± S.E. for three separate determinations for each treatment group, and significantly (p < 0.05) decreased levels after cotreatment with a kinase inhibitor are indicated (^**).

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Fig. 5. β-CDODA-Me induction of p21 is MAPK-dependent. A, effects of kinase inhibitors on induction of p21. LNCaP cells were treated with DMSO, 2.5 µM β-CDODA-Me alone or in combination with kinase inhibitors for 24 h, and whole-cell lysates were analyzed by Western blot analysis as described under Materials and Methods. B, β-CDODA-Me activates p21 promoter constructs. LNCaP cells were transfected with p21 promoter constructs, treated with DMSO or different concentrations of β-CDODA-Me, and luciferase activity was determined as described under Materials and Methods. Results are means ± S.E. for three separate determinations for each treatment group, and significant (p < 0.05) induction of activity is indicated (^*). C, inhibition by PD98059. Cells were transfected with p21-luc(101), treated with DMSO or β-CDODA-Me alone or in combination with 10 µM PD98059. Results are expressed as means ± S.E. for three separate determinations for each treatment group, and significant (p < 0.05) induction by β-CDODA-Me (^*) and inhibition after cotreatment with PD98059 (^**) are indicated.

β-CDODA-Me Induced Kinase-Dependent Activation of Proapoptotic/GrowthInhibitory Pathways. Previous studies show that NAG-1 is inducedby some PPAR ${gamma}$ agonists and other cytotoxic compounds in coloncancer cells (Baek et al., 2003

, 2005

; Chintharlapalli et al.,2005a

) through PI3K-dependent activation of EGR-1, which actsas a transacting factor to induce NAG-1 expression. Figure 4Asummarizes the time-dependent induction of EGR-1, ATF-3, andNAG-1 by 2.5 µM β-CDODA-Me, and the induction responsesfollowed a similar time course, whereas EGR-1-dependent inductionof NAG-1 in colon cancer cells is associated with the increasedexpression of EGR-1 before induction of NAG-1 (Baek et al.,2005

; Chintharlapalli et al., 2005a

). Previous studies showthat NAG-1 induction is kinase-dependent (Baek et al., 2005

;Chintharlapalli et al., 2005a

), and results in Fig. 4B showthat 2.5 µM β-CDODA-Me induces activation of theJNK (pJNK), PI3K (pAkt), and MAPK (pErk) pathways. Maximal activationof JNK and PI3K was observed after 8 and 8 to 12 h, respectively,whereas pErk activation remained elevated for 24 h. The effectsof inhibitors of MAPK (PD98059), PI3K (LY294002), protein kinaseC (GF109203X), and JNK (SP600125) on induction of NAG-1 andATF3, and decreased expression of AR, PSA, and FKBP51 was alsoinvestigated in LNCaP cells treated with 2.5 µM β-CDODA-Me(Fig. 4C). Both PD98059 and LY294002 inhibited the inductionof NAG-1 by β-CDODA-Me. However, the JNK inhibitor SP600125was the most potent inhibitor of ATF-3 induction (Fig. 4, C and D).In contrast, decreased expression of AR, PSA, and FKBP51 inLNCaP cells treated with β-CDODA-Me was unaffected by kinaseinhibitors. CDDO and related compounds also induce activationof JNK in leukemia cells through increased reactive oxygen species(Ikeda et al., 2003

), and Fig. 4E illustrates the effects ofβ-CDODA-Me on activation of JNK and ATF3 after cotreatmentwith the antioxidant NAC. Induction of JNK phosphorylation andATF3 by β-CDODA-Me was inhibited after cotreatment withNAC, demonstrating that like CDDO (Ikeda et al., 2003

), β-CDODA-Meactivates JNK through increased oxidative stress.

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Fig. 6. β-CDODA-Me decreases AR gene expression. Effects of T007 (A) and cycloheximide (B) on β-CDODA-Me-dependent effects on AR gene expression. LNCaP cells were treated with β-CDODA-Me alone or in combination with T007 or cycloheximide for 18 h, and AR mRNA levels were determined by real-time PCR as described under Materials and Methods. Similar results were observed after treatment for 12 h (data not shown). C, β-CDODA-Me decreases AR promoter activity. LNCaP cells were transfected with AR-luc, treated with DMSO or β-CDODA-Me, and luciferase activity was determined as described under Materials and Methods. Results are means ± S.E. for three separate experiments for each treatment group, and a significant (p < 0.05) decrease in activity is indicated (^*). D, time-dependent effects of β-CDODA-Me on AR, Sp1, and PARP (cleaved). LNCaP cells were treated with DMSO or β-CDODA-Me for up to 24 h, and whole-cell lysates were analyzed by Western blot analysis as described under Materials and Methods.

These results suggest that the underlying pathways associatedwith the growth-inhibitory/proapoptotic pathways induced byβ-CDODA-Me in LNCaP cells are due in part to activationof kinases. Therefore, the effects of kinase inhibitors on modulationof cell cycle proteins by β-CDODA-Me were also investigated,and the down-regulation of cyclin D1 and induction of p21 werepartially blocked in cells cotreated with the MAPK inhibitorPD98059 (Fig. 5A); MAPK-dependent activation of p21 has beenobserved previously (De Siervi et al., 2004

). Results in Fig. 5Bshow that the 1 to 5 µM β-CDODA-Me also induces luciferaseactivity in LNCaP cells transfected with constructs containing-2325 to +8 [p21-Luc (Fl)], -124 to +8 [p21-Luc (-124)], -101to +8 [p21-Luc (-101)], and -60 to +8 [p21-Luc (-60)] p21 promoterinserts. The latter three constructs contain the six proximalGC-rich sites (VI-I), and the results of the transfection studiessuggest that these GC-rich sites are necessary for β-CDODA-Me-inducedtransactivation. Deletion analysis of the p21 promoter indicatesthat loss of inducibility [i.e., p21-luc(60)] is associatedwith loss of GC-rich sites IV and III, which are essential forMAPK-dependent activation of p21 by β-CDODA-Me. The roleof MAPK in activation of the p21 promoter was confirmed in LNCaPcells transfected with p21-luc(101); β-CDODA-Me inducedluciferase activity, and cotreatment with the MAPK inhibitorPD98059 inhibited this response (Fig. 5C). These results showthat the induction of p21 and the proapoptotic NAG-1 proteinby β-CDODA-Me were related to the activation of MAPK andPI3K but were independent of PPAR ${gamma}$ (Fig. 2, B and C).

β-CDODA-Me Differentially Decreased AR and PSA Gene Expressionin LNCaP Cells. β-CDODA-Me decreases expression of AR,PSA, and FKBP51 protein levels through proteasome and PPAR ${gamma}$ -independentpathways (Fig. 3, D and E), and these responses are also notmodulated by kinase inhibitors (Fig. 4C). The results in Fig. 6Ashow that β-CDODA-Me also decreases AR mRNA levels aftertreatment for 18 h, and cotreatment with the PPAR ${gamma}$ antagonistT007 did not affect mRNA levels confirming the β-CDODA-Me-induceddown-regulation of AR mRNA levels was also PPAR ${gamma}$ -independent.Similar results were obtained in LNCaP cells treated with β-CDODA-Mealone or in the presence of the protein synthesis inhibitorcycloheximide (10 µg/ml) (Fig. 6B); cycloheximide didnot modulate the effects of β-CDODA-Me, suggesting thatan induced inhibitory protein(s) does not mediate the effectsof β-CDODA-Me on AR mRNA expression. β-CDODA-Me alsodecreased luciferase activity in LNCaP cells transfected withthe AR-Luc construct that contains the -5400 to +580 regionof the AR promoter linked to the luciferase gene (Fig. 6C).The results indicate that β-CDODA-Me inhibits AR transcriptionwithout the parallel induction of inhibitory transacting factors.Recent studies suggest that AR down-regulation of a PPAR ${gamma}$ -inactivethiazolidinedione analog was due to down-regulation of Sp1 protein(Yang et al., 2007). Results in Fig. 6D show that β-CDODA-Meinduces a time-dependent induction of PARP cleavage and a decreaseof both AR and Sp1.

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Fig. 7. β-CDODA-Me decreases PSA expression. Effects of T007 (A) and cycloheximide (B) on β-CDODA-Me-dependent effects on PSA gene expression. LNCaP cells were treated with β-CDODA-Me alone or in combination with T007 or cycloheximide for 18 h, and PSA mRNA levels were determined by real-time PCR as described under Materials and Methods. Similar results were observed after treatment for 12 h (data not shown). β-CDODA-Me decreases PSA promoter (C) and DHT-induced (D) PSA promoter activity. LNCaP cells were transfected with PSA-luc, treated with DMSO, β-CDODA-Me, DHT, and β-CDODA-Me plus DHT (combined), and luciferase activity determined as described under Materials and Methods. Results are means ± S.E. for three replicate determinations for each treatment group, and significantly (p < 0.05) decreased basal or DHT-induced luciferase activity by β-CDODA-Me is indicated (^*).

PSA protein expression is also decreased in LNCaP cells treatedwith β-CDODA-Me (Fig. 3D), and similar effects were observedfor PSA mRNA levels after treatment for 18 h; these responseswere not inhibited after cotreatment with the PPAR ${gamma}$ antagonistT007 (Fig. 7A). However, β-CDODA-Me-induced down-regulationof PSA mRNA levels after treatment for 18 h was significantlyinhibited after cotreatment with cycloheximide (Fig. 7B). Inaddition, β-CDODA-Me inhibited transactivation in LNCaPcells transfected with the PSA-Luc construct (contains 5.85kilobases of the PSA promoter insert) (Fig. 7C), and similarresults were obtained for DHT-induced luciferase activity (Fig. 7D).Thus, in contrast to results obtained for AR, β-CDODA-Meinhibits PSA expression through induction of inhibitory transactingfactors, and the mechanisms associated with the decreased PSAexpression and the cis-elements important for this responseare currently being investigated.

Discussion

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Abstract
Materials and Methods
Results
Discussion
References

PPAR ${gamma}$ agonists have been investigated extensively in both invitro and in vivo cancer models for their potential applicationsin cancer chemotherapy (Honda et al., 1998; Escher and Wahli,2000; Berger et al., 2003; Qin et al., 2004). PPAR ${gamma}$ agonistsinhibit prostate cancer cell and tumor growth (Kubota et al.,1998; Moretti et al., 2001; Segawa et al., 2002; Chintharlapalliet al., 2007b), and the fact that approximately 40% of patientswith prostate cancer carry hemizygous deletions of PPAR ${gamma}$ (Muelleret al., 2000) suggests that this receptor may serve as a tumorsuppressor gene for prostate cancer. However, in animal studiesusing the transgenic adenocarcinoma mouse prostate model withhemizygous deletion in PPAR ${gamma}$ , it was shown that the loss of receptorexpression did not enhance or inhibit prostate tumor developmentin these animals (Saez et al., 2003). Thus, at least in thetransgenic adenocarcinoma mouse prostate mouse model, PPAR ${gamma}$ doesnot seem to act as a tumor suppressor gene.

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Fig. 8. β-CDODA-Me-dependent activation of kinases and kinase-dependent genes and repression of AR and PSA.

One of the perplexing problems with PPAR ${gamma}$ agonists is that althoughthese compounds inhibit cancer cell and tumor growth, theirmechanisms of action are both receptor-dependent and -independentin different cancer cell lines. For example, PGJ2, troglitazone,and PPAR ${gamma}$ -active C-DIMs induce NAG-1 in HCT-116 colon cancercells; however, only induction by PGJ2 is inhibited by a PPAR ${gamma}$ antagonist (Baek et al., 2003

; Chintharlapalli et al., 2005a

).Caveolin-1 is induced by C-DIM compounds and CDDO in colon cancercell lines, and this response is inhibited after cotreatmentwith PPAR ${gamma}$ antagonists (Chintharlapalli et al., 2004

, 2005b

).In contrast, C-DIMs decreased caveolin-1 expression in LNCaPcells, and this response was PPAR ${gamma}$ -independent (Chintharlapalliet al., 2007b

β-CDODA-Me is a triterpenoid acid that contains an oleanolicacid backbone structure similar to that of CDDO and CDDO-Me(methyl ester) (Honda et al., 1998), but there are importantstructural differences in the C-, D-, and E-rings that differentiatebetween these compounds. However, for both compounds, the 2-cyanogroup was necessary for the activation of PPAR ${gamma}$ .

In this study, we investigated the growth-inhibitory and proapoptoticeffects of β-CDODA-Me in LNCaP cells and the role of PPAR ${gamma}$ in mediating these responses. β-CDODA-Me was a more potentinhibitor of LNCaP cell growth than analogs (β-DODA andβ-DODA-Me) that did not contain a 2-cyano substituent (Fig. 1A).Moreover, β-CDODA-Me decreased survival of androgen-insensitivePC3 and DU145 cells (Fig. 1C) and also induced apoptosis inthese cells (Fig. 2D). β-CDODA-Me activated PPAR ${gamma}$ -dependenttransactivation in transient transfection studies in LNCaP cells(Fig. 1D), and compounds without the CN-group were inactive(data not shown) as reported previously for these analogs incolon cancer cells (Chintharlapalli et al., 2007a). β-CDODA-Meinduced p27 expression and down-regulated levels of cyclin D1protein (Fig. 2, A and B). Similar effects were reported previouslyfor C-DIMs in LNCaP cells (Chintharlapalli et al., 2007b), andthe effects of both compounds were receptor-independent; however,β-CDODA-Me-induced responses were observed at lower concentrations(1-2.5 µM) than the C-DIM compounds (7.5-10 µM).C-DIMs did not induce p21 in LNCaP cells (Chintharlapalli etal., 2007b), whereas β-CDODA-Me induced p21 protein, andthis response was not inhibited after cotreatment with PPAR ${gamma}$ antagonist T007 (Fig. 2B). Differences between PPAR ${gamma}$ -active C-DIMsand β-CDODA-Me in their induction of p21 in LNCaP cellswas due to activation of MAPK signaling by the latter compound(Fig. 4B), which was required for the induction of p21 protein(Fig. 5A) and activation of the p21 promoter (Fig. 5C). Thisis a novel pathway for induction of p21 in LNCaP cells; however,previous studies in other cell lines have demonstrated MAPK-dependentinduction of p21 expression (De Siervi et al., 2004).

NAG-1 and ATF3 are growth-inhibitory and proapoptotic proteins(Hartman et al., 2004; Jang et al., 2006), and previous studieswith PPAR ${gamma}$ agonists report both receptor-dependent and -independentinduction of NAG-1 (Baek et al., 2003; Chintharlapalli et al.,2005a,b). Induction of NAG-1 and ATF3 by β-CDODA-Me inLNCaP cells was also PPAR ${gamma}$ -independent. Both PI3K and MAPK inhibitorsblocked the induction of NAG-1; however, the JNK inhibitor SP600125was the most potent inhibitor of ATF3 (but not NAG-1) induction.The inhibitory effects of SP600125 are consistent with previousstudies showing that homocysteine also induces ATF3 in vascularcells through activation of JNK, which activates c-jun and ATF3through an activator protein-1 site in the ATF3 promoter (Chenget al., 2006). The structurally related triterpenoid CDDO inducesoxidative stress in leukemia and pancreatic cancer cells (Ikedaet al., 2003; Samudio et al., 2005), and this is correlatedwith pro-oxidant-dependent induction of JNK phosphorylationand other responses that are inhibited by antioxidants suchas NAC (Ikeda et al., 2003). Similar results were observed inthis study where NAC also inhibits β-CDODA-Me-dependentactivation of JNK and induction of ATF3 (Fig. 4E). The kinase-dependentinduction of NAG-1 has been reported previously, and these effectsare both structure- and cell context-dependent. For example,troglitazone and PPAR ${gamma}$ -active C-DIMs induce NAG-1 in HCT116 coloncancer cells through rapid activation of Egr-1, which subsequentlyactivates NAG-1 through direct interaction with the proximalregion of the NAG-1 promoter (Chintharlapalli et al., 2005a).However, this induction response is MAPK-dependent for troglitazoneand PI3K-dependent for the C-DIM compound. In this study, thetime-dependent induction of both EGR-1 and NAG-1 are similarin LNCaP cells (Fig. 4A), and inhibition of NAG-1 expressionis observed with both PI3K and MAPK inhibitors (Fig. 4B). Thismay involve cooperative interactions of both kinase pathwaysfor the induction of NAG-1 by β-CDODA-Me in LNCaP cells,and mechanisms for these responses are currently being investigated.It is interesting that induction of NAG-1 by PPAR ${gamma}$ -active C-DIMsin LNCaP cells was inhibited only by the MAPK inhibitor PD98059(Chintharlapalli et al., 2007b), suggesting differences betweenβ-CDODA-Me and C-DIMs in the same cell line. Thus, inductionof both NAG-1 and ATF3 in LNCaP cells is differentially inducedby two PPAR ${gamma}$ agonists, C-DIMs and β-CDODA-Me, through receptor-independentactivation of different kinase pathways.

Recent reports show that in LNCaP cells, AR knockdown by RNAinterference results in apoptosis (Liao et al., 2005), and stableknockdown using short hairpin RNAs for AR results in decreasedAR and PSA expression and inhibition of tumor growth in vivo(Cheng et al., 2006). Like β-CDODA-Me, AR and PSA expressionsare also decreased by C-DIMs and troglitazone in LNCaP cells,and 3,3'-diindolylmethane (DIM) also decreases expression ofboth genes and proteins (Bhuiyan et al., 2006; Li et al., 2007).Troglitazone differentially decreases PSA and AR expressionat relatively low (IC₅₀ $≤$ 10 µM) and high (IC₅₀ $~$ 40 µM)concentrations, respectively (Yang et al., 2006). In contrast,C-DIMs decreased AR and PSA mRNA, protein and reporter geneactivity in cells transfected with PSA-Luc and AR-Luc constructsover a narrow range of concentrations (7.5-10 µM) (Chintharlapalliet al., 2007b), and similar results were observed for β-CDODA-Me(1-2.5 µM) in this study (Figs. 6 and 7). Moreover, cycloheximidereversed the β-CDODA-Me- and C-DIM-dependent down-regulationof PSA but not AR mRNA levels, suggesting a similar mechanismof action for both compounds. One study reported that DIM inhibitednuclear uptake of AR in LNCaP cells (Le et al., 2003), and likeβ-CDODA-Me, DIM also decreased AR and PSA expression inLNCaP and androgen-insensitive C4-2B cells (Bhuiyan et al.,2006; Li et al., 2007). However, there are several differencesbetween the pathways associated with down-regulation of thesegenes by β-CDODA-Me and DIM, and this includes the pivotalrole for DIM as an inhibitor of phospho-Akt (Bhuiyan et al.,2006; Li et al., 2007), whereas β-CDODA-Me induces phospho-Akt(Fig. 4B), and the PI3K inhibitor LY294002 does not affect β-CDODA-dependentdown-regulation of AR, PSA, or FKBP51 (Fig. 4C) or inductionof p21 or p27 (Fig. 5A).

A recent report indicated that decreased AR expression in LNCaPcells treated with a PPAR ${gamma}$ -inactive thiazolidinedione derivativewas due to proteasome-dependent degradation of Sp1 (Yang etal., 2007). Our results also show a parallel decrease of ARand Sp1 in LNCaP cells treated with β-CDODA-Me (Fig. 6D);however, down-regulation of AR was not reversed by a proteasomeinhibitor (Fig. 3E), and the mechanism of this response is currentlybeing investigated. Loss of AR by RNA interference results inthe induction of apoptosis in LNCaP cells (Liao et al., 2005).In contrast, 2.5 µM β-CDODA-Me rapidly induces PARPcleavage and apoptosis in LNCaP cells before decreased AR expression(Fig. 6D) demonstrating that apoptotic pathways activated byβ-CDODA-Me in LNCaP cells are not associated with lossof AR, and the proapoptotic mechanisms are currently being investigated.

Results of this study demonstrate that β-CDODA-Me is apotent inhibitor of LNCaP cell growth and induces proapoptoticresponses through activation of kinases, which differentiallyactivate ATF3, NAG-1, and p21. In contrast, decreased expressionof AR and PSA are kinase-independent and occur through differentpathways (Fig. 8). β-CDODA-Me, C-DIMs, DIM, and troglitazoneexhibited both differences and similarities in their modes ofaction in LNCaP cells, although all of these compounds decreasedexpression of AR and PSA. The growth-inhibitory and proapoptoticeffects of β-CDODA-Me were primarily PPAR ${gamma}$ -independent inLNCaP cells (Figs. 1B and 3). β-CDODA-Me also decreasedsurvival and induced apoptosis in androgen-insensitive PC3 andDU145 prostate cancer cells (Figs. 1C and 2D), and similar resultshave been observed for other PPAR ${gamma}$ agonists. It is apparent thatβ-CDODA-Me decreases survival and induces apoptosis throughmultiple pathways, including its potent antiandrogenic activityin LNCaP cells. The successful applications of β-CDODA-Meand other such compounds for single or combined prostate cancerchemotherapies will require insights on their mechanisms ofaction and prostate cancer cell context-dependent similaritiesand differences in activating critical pathways such as thoseillustrated in Fig. 8.

Footnotes

This work was supported by the National Institutes of Health(ES09106) and the Texas Agricultural Experiment Station.

S.P. and S.C. contributed equally to this study.

ABBREVIATIONS: PPAR, peroxisome proliferator-activated receptor;PGJ2, 15-deoxy- ${Delta}$ ^12,14-prostaglandin J2; TZD, thiazolidinedione;CDDO, 2-cyano-3,12-dioxo-17 ${alpha}$ -olean-1,9-dien-28-oic acid; C-DIM,1,1-bis(3'-indolyl)-1-(p-substituted phenyl)methane; GA, glycyrrhetinicacid; β-CDODA-Me, methyl 2-cyano-3,11-dioxo-18β-olean-1,12-diene-30-oate;NAG-1, nonsteroidal anti-inflammatory drug-activated gene 1;AR, androgen receptor; PSA, prostate-specific antigen; T007,N-(4'-aminopyridyl)-2-chloro-5-nitrobenzamide; DIM, 3,3'-diindolylmethane;ATF3, activating transcription factor 3; MAPK, mitogen-activatedprotein kinase; JNK, c-Jun NH₂-terminal kinase; FBS, fetal bovineserum; DMEM, Dulbecco's modified Eagle's medium; DMSO, dimethylsulfoxide; FACS, fluorescence-activated cell sorting; PCR, polymerasechain reaction; TBST, Tris-buffered saline/Tween 20; EGR-1,early growth response-1; PARP, poly(ADP-ribose) polymerase;DHT, dihydrotestosterone; PI3K, phosphoinositol-3-kinase; NAC,N-acetyl cysteine; PI, propidium iodide; MG132, N-benzoyloxycarbonyl(Z)-Leu-Leu-leucinal; PD98059, 2'-amino-3'-methoxyflavone; LY294002,2-(4-morpholinyl)-8-phenyl-1(4H)-benzopyran-4-one hydrochloride;SP600125, 1,9-pyrazoloanthrone; GF109203X, 3-[1-[3-(dimethylaminopropyl]-1H-indol-3-yl]-4-(1H-indol-3-yl)-1H-pyrrole-2,5-dionemonohydrochloride.

Address correspondence to: Dr. Stephen Safe, Department of Veterinary Physiology and Pharmacology, Texas A&M University, 4466 TAMU, College Station, TX 77843-4466. E-mail: ssafe{at}cvm.tamu.edu

References

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Abstract
Materials and Methods
Results
Discussion
References

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Methyl 2-Cyano-3,11-dioxo-18β-olean-1,12-dien-30-oate Is a Peroxisome Proliferator-Activated Receptor- Agonist That Induces Receptor-Independent Apoptosis in LNCaP Prostate Cancer Cells

Methyl 2-Cyano-3,11-dioxo-18β-olean-1,12-dien-30-oate Is a Peroxisome Proliferator-Activated Receptor- ${gamma}$ Agonist That Induces Receptor-Independent Apoptosis in LNCaP Prostate Cancer Cells