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(American Journal of Pathology. 2007;170:722-732.)
© 2007 American Society for Investigative Pathology
DOI: 10.2353/ajpath.2007.060651

Activation of Peroxisome Proliferator-Activated Receptor Contributes to the Survival of T Lymphoma Cells by Affecting Cellular Metabolism

From the Department of Pathology and Laboratory Medicine, Weill Medical College of Cornell University, New York, New York

	Abstract

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Peroxisome proliferator-activated receptor (PPAR) is a metabolic regulator involved in maintaining glucose and fatty acid homeostasis. Besides its metabolic functions, the receptor has also been implicated in tumorigenesis. Ligands of PPAR induce apoptosis in several types of tumor cells, leading to the proposal that these ligands may be used as antineoplastic agents. However, apoptosis induction requires high doses of ligands, suggesting the effect may not be receptor-dependent. In this report, we show that PPAR is expressed in human primary T-cell lymphoma tissues and activation of PPAR with low doses of ligands protects lymphoma cells from serum starvation-induced apoptosis. The prosurvival effect of PPAR was linked to its actions on cellular metabolic activities. In serum-deprived cells, PPAR attenuated the decline in ATP, reduced mitochondrial hyperpolarization, and limited the amount of reactive oxygen species (ROS) in favor of cell survival. Moreover, PPAR regulated ROS through coordinated transcriptional control of a set of proteins and enzymes involved in ROS metabolism. Our study identified cell survival promotion as a novel activity of PPAR. These findings highlight the need for further investigation into the role of PPAR in cancer before widespread use of its agonists as anticancer therapeutics.

Most studies of PPAR function focus on its role as a metabolic regulator. The receptor helps maintain lipid and glucose homeostasis in animals and humans.^3,4 Whereas systemic knockout of PPAR causes embryonic lethality,^5,6 disruption of the receptor in insulin target tissues such as fat, liver, or skeletal muscle results in insulin resistance.^7,8 Potential physiological ligands for PPAR are lipophilic molecules that are derived from nutrition or metabolic pathways, including 15-deoxy-^12,14-prostaglandin J₂ (15d-PGJ₂), polyunsaturated fatty acids and their oxidized forms, oxidized phospholipids, and triterpenoids. Thiazolidinediones (TZD, glitazones), potent synthetic ligands of PPAR, are currently a mainstay therapy for type 2 diabetes. The drugs, by activating the receptor, increase tissue sensitivity to insulin and alleviate hyperglycemia. PPAR regulates whole body lipid and glucose metabolism by its actions on the transcription of many metabolic genes at the cellular level. In adipose tissue, where it is most abundantly expressed, the receptor regulates genes of enzymes and transporters that increase uptake and reduce release of free fatty acid and glucose from cells to circulation.⁴

In addition to its role in metabolism, PPAR has also been implicated in the development of cancer. Despite active research in the past few years, it remains debatable whether PPAR is pro- or antineoplastic. PPAR is highly expressed in several cancers, including carcinomas of the colon,^9,10 breast,¹¹ and prostate¹² and liposarcoma.¹³ In addition, PAX8-PPAR1 fusion has been identified in cases of human follicular thyroid carcinomas.¹⁴ Functionally, most of the in vitro and xenograft studies have shown that synthetic ligands of PPAR inhibit proliferation and induce differentiation and apoptosis in tumor cells, suggesting that PPAR is antineoplastic.^15,16 However, in animals that are genetically predisposed to colon and mammary gland cancer, activation of PPAR exacerbates tumor formation and growth.^17-19 In humans, the receptor itself and several of its target genes are up-regulated in PAX8-PPAR1-positive follicular thyroid carcinomas in comparison to the tumors lacking the fusion, demonstrating that increased PPAR transcriptional activity contributes to carcinogenesis.²⁰

It is unclear whether the observed in vitro effects of PPAR ligands are mediated through the receptor or result from nonspecific activities of the drugs.¹⁶ To induce apoptosis of tumor cells, high concentrations of ligands are often required. In addition, antagonists that inhibit PPAR’s activities also show antineoplastic properties by inducing apoptosis, suggesting that the effect may not act through the receptor.^21,22 In a previous report, we found that PPAR promotes survival under the condition of growth factor deprivation.²³ Using cells containing or lacking PPAR, we showed that the survival-enhancing effect occurs via a receptor-dependent mechanism. Furthermore, we demonstrated that PPAR promotes cell survival by enhancing the ability of cells to maintain mitochondrial membrane potential.

Growth factor-independent survival is characteristic of tumor cells. Under normal conditions, growth factor withdrawal induces a series of metabolic changes leading to apoptotic cell death, such as decreased glucose uptake, impaired glycolysis, depolarization of mitochondrial potential, ATP depletion, hyperpolarization of mitochondrial inner membrane, matrix swelling, rupture of mitochondrial outer membrane, and release of cytochrome c and other proteins from the intermembrane space. These are then followed by caspase activation and eventually cell death. One of the strategies tumor cells use to resist death under growth factor or nutrient limitation is through up-regulation of the expression or activity of antiapoptotic proteins such as BCL-x_L and AKT, which suppress apoptosis through their effects on cellular metabolic activities. One of the key functions of BCL-x_L is to promote efficient mitochondrial ATP/ADP exchange through voltage-dependent anion channel/adenine nucleotide translocase (VDAC/ANT) complex to sustain coupled respiration in the face of decreased mitochondrial membrane potential,²⁴ whereas AKT promotes glucose uptake and glycolysis that provide fuel to maintain mitochondrial potential and ATP production.

Reactive oxygen species (ROS) generation is one of the early events in several forms of cell death. Although it is still controversial whether ROS production during apoptosis precedes or follows mitochondrial damage,^25,26 scavenging of ROS blocks or attenuates apoptosis in several systems,²⁷ and BCL2 has been shown to inhibit apoptosis by preventing ROS generation.^28,29

As a known factor affecting metabolism, PPAR may impact tumor cell survival through its regulation of cellular metabolism similar to other antiapoptotic proteins. In the current study, we investigated the role of PPAR in the survival of tumor cells using anaplastic large cell lymphoma (ALCL) as a model. ALCL is a type of non-Hodgkin’s T-cell lymphoma characterized by large malignant cells with pleomorphic nuclei and abundant cytoplasm. It represents 2% of all types of lymphoma, 10% of pediatric lymphomas, and 50% of large cell lymphomas in the pediatric population. At the molecular level, ALCL is not a homogeneous entity; about 40 to 60% of cases carry a characteristic chromosomal translocation t(2;5), which generates a fusion between anaplastic lymphoma kinase (ALK) and nucleophosmin (NPM) gene.

We found that PPAR is highly expressed in several primary tissues of ALCL cases. Under the condition of serum starvation, PPAR agonists promote survival of an ALCL cell line that highly expresses the receptor but not of an ALCL line that lacks PPAR. Moreover, decreasing the amount of PPAR by RNA interference reduces the rate of cell survival. Given the role of PPAR in metabolism, we investigated whether its prosurvival effects are linked to its regulation of cellular metabolic activities. We demonstrated that PPAR activation leads to higher ATP and lower ROS levels that favor survival in serum-deprived cells. Moreover, PPAR limits amount of ROS through concerted transcriptional regulation of several proteins and enzymes that control cellular ROS. Last, transfection of PPAR into the PPAR-null T-cell lymphoma cell line imparts increased survival and reduced ROS accumulation. The finding that PPAR promotes survival is compatible with the observations that expression of PPAR is increased in many cancers and suggests that PPAR may confer a survival advantage on the malignant cells, allowing them to survive in an adverse environment.

	Materials and Methods

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Reagents and Tissues

15d-PGJ₂, rosiglitazone, and WY14643 were purchased from Cayman Chemical (Ann Arbor, MI). Paraffin-embedded tissues from nine cases of ALCL were obtained from the archives of the Department of Pathology and Laboratory Medicine at Weill Cornell Medical College and studied following Institutional Review Board review and approval.

Cell Lines and Culture

The anaplastic large cell lymphoma lines Karpas 299 and SUP-M2 have been described previously^30-32 and were maintained at 37°C in RPMI 1640 supplemented with 10% fetal bovine serum and penicillin/streptomycin. SUP-M2 cells were transfected with pcDNA3.1-hPPAR1 with TransFectin lipid reagent from Bio-Rad Laboratories (Hercules, CA) according to the manufacturer’s instructions.

Serum Starvation and Cell Viability Determination

To perform serum withdrawal, cells were washed three times with RPMI 1640, resuspended, and cultured in serum-free media. Cell viability was determined by cellular exclusion of 2 µg/ml propidium iodide followed by flow cytometric analysis of 10,000 events as described previously.²³ Various drug treatments of the cells are described in detail in figure legends.

Caspase-3 Activity

Caspase-3 activity was assayed using CaspGLOW fluorescein active caspase-3 staining kit (BioVision, Mountain View, CA). Serum-starved cells (3 x 10⁵ in 0.3 ml) were treated with 1 µl of caspase-3 substrates and incubated for 45 minutes in a 37°C incubator with 5% CO₂. Cells were then washed with the wash buffer, and 10,000 events were analyzed by flow cytometry using FL-1.

Luciferase Assay

Five micrograms of acylCoAx3-TK-LUC, a Firefly luciferase reporter construct containing three copies of PPRE, and 0.5 µg of Renilla expression plasmid were cotransfected into 5 x 10⁶ Karpas 299 cells using the Amaxa Nucleofector instrument (Amaxa Biosystems, BioCampus, Cologne, Germany) in 100 µl of solution V using the A30 program. Rosiglitazone (2 µmol/L) or DMSO vehicle control was added 16 hours after transfection. Cells were then harvested 24 hours after drug addition. Firefly and Renilla luciferase activities were measured using a dual-luciferase reporter assay system (Promega, Madison, WI) according to the manufacturer’s instructions. Luminescence was measured using MLX microplate luminometer (Dynex Technologies Inc., Chantilly, VA). PPAR transcriptional activity was expressed as firefly luciferase activity normalized to Renilla luciferase activity.

Immunohistochemical Assays

Immunohistochemical staining for PPAR (E-8; Santa Cruz Biotechnology Inc., Santa Cruz, CA) and CD30 (clone BerH2; DakoCytomation, Carpinteria, CA) was performed on formalin-fixed, paraffin-embedded tissue sections using the TechMate 500 automated immunostainer (Ventana Medical Systems Inc., Tucson, AZ). Immunostaining for PPAR was performed following antigen retrieval in an autoclave using Target Retrieval Solution, High pH (DakoCytomation). Immunoreactivity for PPAR was identified using HRP-labeled mouse Envision Plus detection system (DakoCytomation) and DAB liquid chromogen (DakoCytomation). The sections were then retrieved in the autoclave with Target Retrieval Solution, Citrate pH 6 (DakoCytomation), and immunostained for CD30 using ChemMate alkaline phosphatase detection system (Ventana Medical Systems). The alkaline phosphatase reaction was developed by BT Red reagent substrate provided in the kit. Sections were counterstained with hematoxylin, dehydrated, and mounted in Cytoseal-XYL (Richard-Allan Scientific, Kalamazoo, MI).

RNA Interference and Nucleofection

Small interfering RNA (siRNA) against PPAR and scrambled double-stranded RNA controls were purchased from Dharmacon Inc. (Boulder, CO) in the form of SMART pool. The delivery of siRNA pools into Karpas 299 cells was performed using nucleofection technology with the Nucleofector instrument (Amaxa Biosystems). A total of 3 µg of the siRNA pools were delivered into 2 x 10⁶ cells suspended in 100 µl of solution V using the A30 nucleofection program. Two micrograms of pmaxGFP vector were cotransfected to monitor transfection efficiency.

Measurement of Cellular ATP Levels

Intracellular ATP levels were determined using the ATP bioluminescence assay kit HS II (Roche Applied Science, Indianapolis, IN) following the manufacturer’s instructions. In brief, 25 µl of lysis reagent was added to 25 µl of cells (1 x 10⁵ cells/ml), incubated for 5 minutes at room temperature, and 50 µl of luciferase reagent was then added. Luminescence was quantified using a MLX microtiter plate luminometer (Dynex Technologies).

Measurement of Mitochondrial Membrane Potential

At various time points following serum withdrawal, 2 x 10⁵ to 4 x 10⁵ cells were stained with 20 nmol/L tetramethylrhodamine ethyl ester in a 37°C CO₂ incubator for 30 minutes. Cells were then analyzed by flow cytometry using FL-2.

Measurement of Intracellular ROS

Intracellular ROS were detected with carboxy-H₂DCFDA (DCF; Molecular Probes, Eugene, OR). Three hundred thousand cells were washed once, resuspended in 500 µl of PBS, and loaded with 10 µmol/L carboxy-H₂DCFDA for 30 minutes at 37°C. DCF fluorescence of 10,000 events was measured by flow cytometry using FL-1.

RNA Preparation, Reverse Transcription, and Real-Time PCR

Total RNA was isolated from cells using RNeasy Kit (Qiagen, Valencia, CA) according to the manufacturer’s instructions. The amounts of total RNA were quantified using spectrophotometric measurements. RNA was reverse-transcribed into cDNA using a reverse transcription system (Promega) according to the manufacturer’s protocol. Real-time PCR was conducted in an ABI PRISM 7000 Sequence Detection System [Applied Biosystems (ABI), Foster City, CA]. cDNA made from 100 ng of total RNA was added to a 20 µl 1x Taqman Universal Master Mix (ABI). The PCR reactions were conducted at 50°C for 2 minutes, 95°C for 10 minutes, followed by 50 cycles of 95°C for 15 se-conds and 60°C for 60 seconds. Primers and probe were purchased from ABI for detection of PPAR (Hs00234592_m1), catalase (Hs00156308_m1), Cu, Zn superoxide dismutase (CuZn-SOD, Hs00166575_m1), p67 (Hs00166416_m1), and UCP2 (Hs00163349_m1); sequences are not provided by the manufacturer. Manganese SOD (Mn-SOD) was detected using SYBR Green method. Primer sequences are: forward, 5'-AGCATGTTGAGCCGGGCAGT-3' and reverse 5'-AGGTTGTTCACGTAGGCCGC-3'. Real-time PCR results were analyzed with ABI PRISM 7000 SDS software. Autothresholds and autobaselines determined by the software were applied to generate values of corresponding threshold cycles (Ct). Ct values of various genes were normalized to human ß-actin that was purchased from ABI (Hs 99999903_m1).

Western Blot Analyses

The analyses were conducted as described previously.²³ Antibodies against PPAR, UCP2, and p67 were purchased from Santa Cruz Biotechnology, Alpha Diagnostic International (San Antonio, TX), and BD Biosciences (Franklin Lakes, NJ), respectively.

Assay for Manganese Superoxide Dismutase Activity

The activity of the enzyme was assayed in whole-cell extracts using a superoxide dismutase assay kit purchased from Cayman Chemical. The assays were performed according to the manufacturer’s instructions. To determine selectively the activity of Mn-SOD, cell lysates were treated with 3 mmol/L KCN to inactivate CuZn-SOD before performing the assay.

Statistical Analysis

Student’s t-test was used to perform the statistical analyses. P values are indicated in each figure.

	Results

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PPAR Is Highly Expressed in Human T-Cell Lymphoma and Low Doses of Rosiglitazone Attenuate Serum Withdrawal-Induced Lymphoma Cell Death

Although expression of PPAR has been found in mouse and human lymphoma cell lines, expression of PPAR in human primary lymphoma tissues has not been demonstrated. We examined nine cases of ALCL for PPAR expression by immunohistochemistry. To ensure that PPAR is expressed in the malignant cells, we performed staining for PPAR as well as CD30, which specifically marks the malignant large cells in ALCL tissues. Positive PPAR staining was found in six of nine cases, and a pair of positive and negative cases is shown in Figure 1A . In a typical positive case, the malignant anaplastic large cells that are marked with cytoplasmic CD30 (pink) were stained positive for PPAR (brown) in nuclei (Figure 1A , left panel), whereas a typical negative case lacks PPAR staining in CD30-marked tumor cells (Figure 1A , right panel). The admixed positive and negative results among nine cases are not unexpected, because ALCL cases are not homogeneous at the molecular level.

View larger version (77K): [in this window] [in a new window]   Figure 1. Expression of PPAR in human T-cell lymphoma and effects of rosiglitazone on serum withdrawal-induced cell death. A: Medium power views of PPAR-positive and -negative ALCL cases. Red, CD30 cytoplasmic staining; brown, PPAR nuclear staining. B: PPAR protein expression in Karpas 299 and SUP-M2 lymphoma cell lines. Immunohistochemical assay was performed on cell blocks made from the two cell lines. Nuclear staining is shown in brown. C: Survival of serum-deprived Karpas 299 and SUP-M2 cells in the presence or absence of rosiglitazone. Serum-deprived cells were cultured for various periods as indicated in the presence of 2 µmol/L rosiglitazone or DMSO. Cell survival was determined by propidium iodide exclusion with flow cytometric analysis. Data shown are mean ± SE of three independent experiments. D: Caspase-3 activity in serum-deprived Karpas 299 cells. Serum-deprived cells were cultured for 18 hours in the presence of 2 µmol/L rosiglitazone or DMSO. E: Dose titration of rosiglitazone. Serum-deprived Karpas 299 and SUP-M2 cells were cultured in the presence or absence of rosiglitazone at various concentrations as indicated and survival was determined at 48 hours after serum withdrawal. Data shown are mean ± SE of three independent experiments. F: Relative luciferase activity in Karpas 299 cells treated with DMSO or 2 µmol/L rosiglitazone. Firefly luciferase activity was normalized to that of Renilla luciferase that was cotransfected into the cells. Luciferase activity of DMSO-treated cells was set as 1.

Next, we examined whether high levels of PPAR confer a survival advantage on the lymphoma cells under stress conditions. Serum starvation was performed with Karpas 299 and SUP-M2 cells treated with PPAR ligand rosiglitazone or drug vehicle, and survival of the cells was determined by propidium iodide exclusion. Although survival of both Karpas 299 and SUP-M2 cells decreased with time, death of Karpas 299 cells was attenuated by rosiglitazone treatment, whereas survival of SUP-M2 cells was not influenced (Figure 1C) . The cell death is apoptotic in nature, since caspase-3 was activated in serum-starved Karpas 299 cells (Figure 1D , DMSO). In addition, rosiglitazone treatment of the cells suppressed caspase-3 activation, supporting that the PPAR agonist is prosurvival in serum-starved cells (Figure 1D , Rosi versus DMSO).

A dose titration of rosiglitazone revealed that the survival effect in Karpas 299 cells could be observed at a concentration as low as 0.5 µmol/L and reached maximum at 2 µmol/L (Figure 1E) . These concentrations largely overlap with pharmacologically achievable serum concentrations of rosiglitazone in diabetic patients (0.16 to 1.26 µmol/L) (Rosiglitazone Maleate, http://home.mdconsult.com, 2006). In comparison, in the same dose range, rosiglitazone did not show any effects on the survival of SUP-M2 cells (Figure 1E) . Two micromolar was chosen for the subsequent experiments. At this concentration, PPAR was activated as a transcriptional factor as shown by a luciferase reporter assay (Figure 1F) .

Low Doses of Other PPAR but Not PPAR Agonists Promote Survival in Serum-Deprived Lymphoma Cells

To ensure that the survival effect is mediated via PPAR rather than a special property of rosiglitazone, other PPAR agonists were tested for their activities in serum withdrawal-induced apoptosis. GW7845, a tyrosine analogue that is chemically distinct from glitazones,³⁴ promoted survival of the Karpas 299 cells in the dose range of 0.5 to 5 µmol/L but reduced survival at higher concentrations (Figure 2A) . 15d-PGJ₂, a potential physiological ligand of PPAR, increased cell survival in the dose range of 0.1 to 1 µmol/L but killed cells at concentrations above and equal to 5 µmol/L (Figure 2B) . Last, WY14643, a PPAR agonist, did not influence cell survival under this condition (Figure 2C) . Taken together, these data demonstrate that low doses of PPAR agonists attenuated serum withdrawal-induced lymphoma cell apoptosis, whereas high doses promoted cell death.

View larger version (18K): [in this window] [in a new window]   Figure 2. Other PPAR but not PPAR agonists promote cell survival. A: Survival of serum-deprived Karpas 299 cells in the presence of GW7845 at concentrations indicated. B: Survival of serum-deprived Karpas 299 cells in the presence of 15d-PGJ2 at concentrations indicated. C: Survival of serum-deprived Karpas 299 cells in the presence of WY14643 at concentrations indicated. Cell survival was determined at 42 hours after serum withdrawal and data shown are mean ± SE of three independent experiments.

Reducing the Amount of PPAR with siRNA Decreases Survival in Serum-Deprived T Lymphoma Cells

To determine whether the prosurvival effect of the PPAR agonists acts through the receptor, PPAR in Karpas 299 cells was specifically inhibited using siRNA. A pool of four PPAR siRNA was transfected into cells with an efficiency of 65% as assessed by the cotransfection of a green fluorescent protein-containing plasmid. The level of PPAR transcripts was knocked down to 45% of the level in control cells transfected with scrambled double-stranded RNA (Figure 3A) . Reduction of PPAR protein was confirmed with Western blot analysis, and the effect on cell survival was then determined (Figure 3B) . siRNA transfection decreased the survival of Karpas 299 cells in the presence or absence of rosiglitazone, confirming that prosurvival activity is dependent on PPAR (Figure 3C) .

View larger version (20K): [in this window] [in a new window]   Figure 3. Reducing PPAR attenuates survival in Karpas 299 cells. A: PPAR mRNA levels in Karpas 299 cells transfected with PPAR siRNA or control scrambled RNA. mRNA was measured by real-time RT-PCR at 48 hours after transfection. The level of PPAR mRNA in control RNA-transfected cells was arbitrarily set as 100%. B: PPAR protein levels were determined by Western blot analysis in whole-cell lysates at 48 hours after transfection. C: Cell viability was determined at 48 hours after serum starvation in the presence of DMSO or 2 µmol/L rosiglitazone. Results shown are mean ± SE of three independent experiments.

The Prosurvival Effect of PPAR Is Accompanied by Increased Cellular ATP and Decreased Mitochondrial Hyperpolarization

ATP depletion is one of the early events during apoptotic death induced by growth factor withdrawal.²⁴ In the next experiment, we investigated whether total cellular ATP level is affected by PPAR activation following serum starvation. We compared ATP levels of Karpas 299 and SUP-M2 cells treated with or without rosiglitazone. As shown in Figure 4A , following serum withdrawal, cellular ATP in the Karpas 299 cells treated with rosiglitazone was significantly higher than those cells treated with DMSO, whereas rosiglitazone had no effect on the total ATP level in the SUP-M2 cells.

View larger version (22K): [in this window] [in a new window]   Figure 4. PPAR attenuates decline in ATP level and reduces mitochondrial hyperpolarization in serum-deprived cells. A: Relative ATP levels in Karpas 299 and SUP-M2 cells withdrawn from serum. Cells were cultured with or without 2 µmol/L rosiglitazone as indicated. Total cellular ATP levels were determined in lysates from a million cells at 40 hours after serum withdrawal. The amount of ATP in DMSO-treated Karpas 299 cells was arbitrarily set as 100%. Data shown are mean ± SE of three independent experiments. B: Mitochondrial membrane potential measured by tetramethylrhodamine ethyl ester incorporation. Karpas 299 cells were cultured in the presence or absence of serum for 37 hours with or without rosiglitazone as indicated.

PPAR Suppresses Accumulation of Reactive Oxygen Species in Serum-Deprived T Lymphoma Cells

ROS are generated following application of many apoptotic stimuli,²⁵ and scavenge of ROS has been shown to prevent or delay cell death.²⁷ We compared the levels of intracellular oxidants of the T lymphoma cells in the presence or absence of serum. Serum deprivation caused an increase in intracellular ROS in both Karpas 299 and SUP-M2 cells (Figure 5 , thick solid and dotted lines versus thin solid and dotted lines). In serum-deprived Karpas 299 cells, rosiglitazone treatment led to a reduction in the ROS level (Figure 5 , left panel, thick solid versus thick dotted line) whereas rosiglitazone did not influence the ROS level in serum-deprived SUP-M2 cells (Figure 5 , right panel, thick solid versus thick dotted line). This result suggests that activation of PPAR suppresses accumulation of ROS, thus leading to improved survival.

View larger version (12K): [in this window] [in a new window]   Figure 5. ROS is suppressed in serum-deprived Karpas 299 cells by PPAR activation but not in SUP-M2 cells. Karpas 299 and SUP-M2 cells were cultured with or without serum in the presence of DMSO or 2 µmol/L rosiglitazone as indicated. Cells were harvested at 48 hours after serum withdrawal and incubated with 10 µmol/L DCF at 37°C for 30 minutes. Ten thousand events in live cell gate were analyzed by flow cytometry.

PPAR Regulates a Set of Enzymes and Proteins That Controls Cellular ROS Level

PPAR is known as a nuclear hormone receptor that acts as a transcription factor. The receptor may affect the cellular ROS through its transcriptional regulation of proteins and enzymes responsible for ROS generation and scavenge. Activation of NADPH oxidase produces many species of free radical oxidants. Recently, it has been shown that NADPH oxidase is expressed in the T lymphocytes,³⁵ and expression of several subunits of NADPH oxidase, including p67, p22, and p47, is regulated by pioglitazone treatment of endothelial cells.³⁶ Because the p67 subunit plays an important role in regulating the enzymatic activity of NADPH oxidase, we analyzed expression of p67 in serum-deprived T lymphoma cell lines. Real-time RT-PCR revealed that p67 mRNA expression was reduced by rosiglitazone treatment in Karpas 299 cells but not in SUP-M2 cells (Figure 6A , left panel). This observation was confirmed at the protein level by Western blot analysis (Figure 6A , right panel).

View larger version (26K): [in this window] [in a new window]   Figure 6. A set of ROS regulating enzymes is coordinately controlled by PPAR activation. Karpas 299 and SUP-M2 cells treated with 2 µmol/L rosiglitazone or DMSO were harvested at 42 hours after serum withdrawal. A: p67 mRNA was measured by real-time RT-PCR (left). The amount of p67 mRNA in DMSO-treated Karpas 299 cells was arbitrarily set as 100%. p67 protein levels were determined by Western blot analysis in whole-cell lysates (right). D, DMSO; R, rosiglitazone. B: UCP2 mRNA was measured by real-time RT-PCR (left). The amount of UCP2 mRNA in DMSO-treated Karpas 299 cells was arbitrarily set as 100%. UCP2 protein levels were determined by Western blot analysis in whole cell lysates (right). D, DMSO; R, rosiglitazone. C: Mn-SOD mRNA was measured by real-time RT-PCR (left). The amount of Mn-SOD mRNA in DMSO-treated Karpas 299 cells was arbitrarily set as 100%. Mn-SOD activity was determined in whole-cell lysates. D: CuZn-SOD and catalase mRNA levels were determined by real-time RT-PCR. The amount of mRNA in DMSO-treated Karpas 299 cells was arbitrarily set as 100%. Data shown in A–D are mean ± SE of at least three independent experiments.

Superoxide dismutase, an important ROS scavenger, is responsible for converting superoxide radicals into H₂O₂ and molecular oxygen. It has two cellular forms, a mitochondria-associated enzyme using Mn as a cofactor (Mn-SOD) and a cytosolic enzyme using copper and zinc as cofactors (CuZn-SOD). As shown in Figure 6C , PPAR activation regulated the mRNA expression and enzymatic activity of Mn-SOD specifically in serum-deprived Karpas 299 cells but not in SUP-M2 cells. In contrast, CuZn-SOD was not affected by PPAR activation in either cell line (Figure 6D , left panel). Expression of catalase, the enzyme that converts H₂O₂ to water and molecular O₂, did not respond to rosiglitazone treatment either (Figure 6D , right panel). Taken together, we found that activation of PPAR modulates expression of three ROS-controlling factors, p67 subunit of NADPH, UCP2, and Mn-SOD, thereby limiting the level of ROS and promoting cell survival.

Transfection of PPAR into PPAR-Deficient SUP-M2 Cells Improves Cell Survival and Suppresses ROS Accumulation

To provide more definitive evidence that PPAR promotes survival by suppressing ROS accumulation, PPAR was stably transfected into the SUP-M2 lymphoma cell line that lacks the receptor (Figure 7A) . Survival and ROS levels were then determined in these cells in comparison to SUP-M2 cells transfected with an empty vector. As shown in Figure 7B , during serum starvation, the survival of the PPAR-positive SUP-M2 clone was significantly higher than the vector-transfected cells in the presence of rosiglitazone (Figure 7B , left panel). To exclude the possibility that this effect was due to properties of a specific clone, a pool of PPAR-positive clones was then tested. Again, survival of the PPAR-positive pool was significantly improved over the survival of the control pool (Figure 7B , right panel).

View larger version (22K): [in this window] [in a new window]   Figure 7. Transfection of PPAR into SUP-M2 cells improves cell survival and suppresses ROS accumulation. A: PPAR or pcDNA3 vector was stably transfected into SUP-M2 cells. Western blot shows the presence or absence of the PPAR protein expression in stable cell lines containing PPAR expression vector or pcDNA3 vector. B: Cell survival in serum-deprived SUP-M2 cells with or without PPAR. Rosiglitazone (2 µmol/L) was added at the time of serum withdrawal. Individual stable clones are shown on the left and pools of stably transfected cells are shown on the right. C: ROS levels in serum-deprived SUP-M2 cells with or without PPAR. Rosiglitazone (2 µmol/L) was added at the time of serum withdrawal. Individual stable clones are shown on the left and pools of stably transfected cells are shown on the right.

	Discussion

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In this report, we provide several pieces of evidence showing that PPAR confers cell survival in malignant T cells under the condition of serum withdrawal. First, activation of the receptor is capable of enhancing survival in Karpas 299 cells that highly express PPAR but not in SUP-M2 cells that lack PPAR. Not only the glitazone type of PPAR agonists but also the other types of agonists (GW7845 and 15d-PGJ₂) act to increase cell survival, whereas a PPAR agonist shows no effects. Second, reducing the level of the receptor in Karpas 299 cells with siRNA decreased cell survival rate. Third, cellular metabolic activities, including ATP, mitochondrial membrane potential, and ROS, are changed in directions that are consistent with PPAR being a prosurvival factor. Fourth, several ROS controlling molecules are coordinately regulated by PPAR activation in the directions that lead to ROS limitation. Lastly and importantly, introduction of the receptor into PPAR-negative SUP-M2 cells results in increased cell survival and decreased ROS accumulation during serum starvation. Collectively, these observations support the notion that PPAR promotes T lymphoma cell survival through regulation of cellular metabolic activities.

In addition to our report, several groups have found that PPAR improves cell survival in other systems. Haraguchi et al³⁷ reported that several PPAR agonists inhibit serum starvation induced apoptosis in kidney cells. In addition, it has been shown that infusion of 15d-PGJ₂ and rosiglitazone resulted in reduction in size of brain infarct³⁸ as well as myocardial infarct in rats.³⁹ These findings are consistent with our results that PPAR attenuates cell death induced by nutrient/growth factor deprivation.

The role of PPAR in cancer is controversial. Although several genetic models suggest that PPAR promotes tumor formation when combined with other oncogenes, studies in vitro and using xenograft models have shown the antiproliferative and proapoptotic effects of PPAR agonists in a variety of tumor cells. Based on these studies, it has been proposed that PPAR ligands may be used as anticancer agents. However, a careful review of the literature reveals that many of these studies used PPAR ligands at concentrations much higher than their K_D for PPAR. In a study of PPAR in leukemia, 25 µmol/L rosiglitazone are required to induce 50% cell death in leukemic cell lines,⁴⁰ whereas a prosurvival effect can be seen at a concentration as low as 0.5 µmol/L. In patients taking rosiglitazone to control diabetes, maximum plasma concentration of the drug falls between 0.16 and 1.26 µmol/L following an oral dose of 1 to 8 mg. Likewise, micromolar doses of 15d-PGJ₂ were required to induce lymphoma cell death,^41,42 whereas physiological concentrations of the metabolite are in the range of picomolar to nanomolar. In our system, 15d-PGJ₂ generated a small but dose-dependent increase in cell survival in the range of 0.1 to 1 µmol/L but induced cell death when doses were above 5 µmol/L. Similar to our observations, Lin et al.³⁸ also found that high doses of PPAR agonists 15d-PGJ₂ (5 µmol/L) and rosiglitazone (10 µmol/L) cause cytotoxicity as indicated by lactate dehydrogenase release from cultured neurons, whereas low concentrations of the agonists (15d-PGJ₂, 1 µmol/L, and rosiglitazone, 0.5 µmol/L) suppress rat and human neuronal apoptosis and necrosis induced by H₂O₂ treatment. Requirements for high doses of ligands suggest the possibility that apoptosis induction is an off-target effect independent of the receptor. A more definitive piece of evidence for the prosurvival role of PPAR is derived from our study with genetic manipulation of the receptor. We showed that, on one hand, decreasing PPAR level with siRNA in Karpas 299 cells impaired cell survival and, on the other hand, transfection of the receptor into SUP-M2 cells results in increased survival in serum-deprived cells.

Setoguchi and colleagues⁴³ reported that proliferation and survival of B cells on LPS or IgM stimulation were increased in PPAR heterozygous mice compared with the wild-type mice, suggesting that the receptor suppresses B cell proliferation and survival under physiological conditions. In the meantime, the proliferative response of T cells was not affected by reduced level of PPAR in the haploinsufficient mice. So, B and T lymphocytes apparently responded differently to PPAR activation in this study in terms of proliferation. Survival of T cells was not determined; thus, a direct comparison to our study is not possible. Importantly, we have found that PPAR does not affect cell survival under normal conditions, it only does so when cells suffer from growth factor/nutrient deprivation.^23,33 These data led us to believe that cellular conditions are crucial in dictating how cells respond to PPAR activation.

As a metabolic regulator, how does PPAR cause metabolic changes at the cellular level to favor cell survival when cells are deprived of growth factors/nutrients? Our data show that PPAR attenuates the decline in ATP under conditions of serum withdrawal. In cells deprived of growth factor, a drop in cellular ATP reflects compromised mitochondrial function and is one of the steps leading to cell death. In this study, we showed that activation of PPAR with rosiglitazone results in a higher ATP level in serum-deprived cells (Figure 4A) . Moreover, hyperpolarization of mitochondrial membrane is alleviated by rosiglitazone treatment (Figure 4B) . These data suggest that PPAR helps maintain cellular ATP level in the face of nutrient deprivation leading to improved mitochondrial homeostasis and increased cell survival.

ROS generation is a necessary step during apoptosis as ROS scavengers block or delay apoptosis. We found that serum withdrawal-induced ROS production is attenuated by PPAR activation in Karpas 299 cells but not in SUP-M2 cells. Moreover, introduction of PPAR into SUP-M2 leads to ROS limitation in the transfected cells, providing strong evidence that PPAR plays a key role in the regulation of ROS metabolism. Our investigation has further identified that proteins and enzymes regulating ROS are coordinately controlled by PPAR. PPAR increases the amount of UCP2 and Mn-SOD and reduces the amount of the p67 subunit of NADPH oxidase at both the mRNA and protein levels, leading to decreased ROS accumulation and increased cell survival. Together with the information in the literature, we have proposed a model showing the molecular and metabolic mechanisms underlying the prosurvival function of PPAR (Figure 8) .

View larger version (18K): [in this window] [in a new window]   Figure 8. Proposed mechanisms underlying the prosurvival function of PPAR. The model was made based on findings in the current report and literature (see Discussion). Dashed arrow indicates that the effects may or may not be direct.

Our data also suggest cautionary use of TZD in diabetic patients with concurrent lymphomas or other types of cancers. Currently, over 1.6 million patients in the United States take TZD chronically to manage their diabetes. If PPAR promotes tumor survival, alternative therapy should be considered in the treatment of this subpopulation of diabetic patients.

	Acknowledgements

 
We thank Yuanyuan Zhang for technical assistance and Pin Lu, M.D., Ph.D., for critical reading of the manuscript.

	Footnotes

 
Address reprint requests to Y. Lynn Wang, Department of Pathology and Laboratory Medicine, Weill Medical College of Cornell University, New York, NY 10021. E-mail: lyw2001{at}med.cornell.edu

Supported by career award K08-HL068850 (to Y.L.W.) from the National Heart, Lung and Blood Institute.

Accepted for publication October 24, 2006.

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