Primary Peripheral T Cells Become Susceptible to 2,3,7,8-Tetrachlorodibenzo-p-Dioxin-Mediated Apoptosis in Vitro upon Activation and in the Presence of Dendritic Cells

Narendra P. Singh, Mitzi Nagarkatti, and Prakash Nagarkatti

Department of Pathology, Microbiology, and Immunology, University of South Carolina School of Medicine, Columbia, South Carolina

Received November 10, 2007; accepted March 7, 2008

Abstract

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Abstract
Materials and Methods
Results
Discussion
References

Although the toxic effects of 2,3,7,8-tetrachlorodibenzo-p-dioxin(TCDD) on T cells in vivo have been well characterized, attemptsto reproduce these findings in vitro have not been successful.In the current study, we examined whether activation or thepresence of dendritic cells (DCs) would make primary naive Tcells from C57BL/6 mice susceptible to TCDD-induced apoptosisin vitro. Although nonactivated primary T cells cultured with10 to 1000 nM TCDD were relatively resistant to apoptosis, theybecame sensitive to apoptosis upon activation with concanavalinA (ConA). Moreover, ConA-activated T cells cultured in the presenceof DCs showed highest levels of TCDD-induced apoptosis. Likewise,primary T cells from OT.II.2a mice cultured with specific ovalbuminpeptide and syngeneic DCs showed higher levels of apoptosiscompared with similar nonactivated T cells. T-cell activationled to up-regulation of aryl hydrocarbon receptor (AhR), Fas,and Fas-ligand (FasL) expression. In addition, DC maturationand culture with TCDD caused significant induction of FasL.TCDD-mediated apoptosis in activated peripheral T cells wasAhR-dependent. Analysis of why nonactivated T cells are moreresistant, whereas activated T cells are sensitive to TCDD-inducedapoptosis revealed that TCDD treatment of activated but notnonactivated T cells led to down-regulation of cellular FLICEinhibitory protein (c-FLIP), an inhibitor of apoptosis. Moreover,down-regulation of c-FLIP using small interfering RNA in nonactivatedT cells made them sensitive to TCDD-induced apoptosis. The currentstudy demonstrates for the first time that TCDD can induce apoptosisin vitro in peripheral T cells upon activation and in the presenceof DCs and that this may be mediated by down-regulation of c-FLIP.

2,3,7,8-Tetrachlorodibenzo-p-dioxin (TCDD) is an environmentalpollutant that mediates toxicity through activation of the arylhydrocarbon receptor (AhR), a ligand-dependent transcriptionfactor and member of the basic helix-loop-helix-Per/Arnt/Sim(periodicity/aryl hydrocarbon receptor nuclear translocator/simple-minded)gene family (Marlowe and Puga, 2005

; Bock and Kohle, 2006

; Harperet al., 2006

). TCDD binds and activates cytosolic AhR attachedto 90-kDa heat shock protein; and upon activation, AhR dissociatesfrom 90-kDa heat shock protein, migrates to the nucleus, dimerizeswith AhR nuclear translocator (ARNT), and forms AhR/ARNT heterodimer.This in turn binds to dioxin-response elements (DRE), presentas cis-acting elements in the regulatory regions of dioxin-responsivegenes, and it up-regulates a large set of genes that directlyor indirectly participate in TCDD-induced toxicity (Schmidtand Bradfield, 1996

; Gonzalez and Fernandez-Salguero, 1998

;Tian et al., 1999

; Whitlock, 1999

; Sulentic et al., 2000

; Dertingeret al., 2001

; Matikainen et al., 2001

; Nazarenko et al., 2001

;Mimura and Fujii-Kuriyama, 2003

). Targeted disruption of theAhR in mice prevents induction of CYP1A1 and most forms of TCDDtoxicity (Marlowe and Puga, 2005

; Bock and Kohle, 2006

; Harperet al., 2006

Extensive previous studies have shown that the immune systemis very sensitive to the toxic effects of TCDD (Kerkvliet, 2002).It is noteworthy that although TCDD triggers thymic atrophyin all species tested, it is less toxic to naive secondary lymphoidorgans, including the spleen and lymph nodes. However, uponimmunization of animals with an antigen, TCDD is known to suppressthe antigen-specific T-cell response in secondary lymphoid organs(Kerkvliet, 2002). Yet another interesting feature about TCDD-inducedimmunotoxicity is that although TCDD has been shown to readilysuppress antigen-specific T-cell responses as well as triggerthymic atrophy in vivo, attempts to demonstrate the direct toxiceffects of TCDD in vitro against thymocytes and naive T cellshave not been successful (Kerkvliet, 2002). Moreover, previousstudies from our laboratory and elsewhere suggested that TCDDaltered the functions of T cells activated through antigen primingin vivo, but it failed to affect resting T cells (Lundberg etal., 1992; Rhile et al., 1996; Pryputniewicz et al., 1998).Recent studies from our laboratory demonstrated that TCDD up-regulatesFasL expression on thymic stromal cells and Fas on thymic Tcells and that when such cells come in contact with each other,the latter cells undergo apoptosis (Camacho et al., 2005). Inthe current study, we speculated that a similar mechanism maybe operative in the induction of apoptosis in antigen-activatedprimary T cells. Thus, we hypothesized that TCDD may act onantigen-presenting cells such as the DCs and increase FasL expressionin such a way that when they come in contact with Fas+ antigen-specificT cells during antigen presentation, the T cells would undergoapoptosis. We also analyzed why activated peripheral T cellsbecome susceptible to TCDD, and we noted that c-FLIP may playa crucial role in regulating apoptosis. The current study hasidentified certain key cells and molecules that regulate TCDD-inducedapoptosis in activated peripheral T cells.

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
References

Mice. C57BL/6 (H-2^b) mice were purchased from the National Institutesof Health (Bethesda, MD). AhR knockout (KO) (Chris Bradfield;on C57BL/6J background) mice were purchased from The JacksonLaboratory (Bar Harbor, ME). OT.II.2a (C57BL/6-TgN(OT-II.2a)-RAG1^tm1Mom)mice were purchased from Taconic Farms (Hudson, NY). All animalswere housed in University of South Carolina Animal facility(Columbia, South Carolina). Care and maintenance of animalswere carried out in accordance with the guide for the care anduse of laboratory animals as adopted by Institutional and NationalInstitutes of Health guidelines.

Reagents and Antibodies. TCDD was a generous gift from Dr. K.Chae (National Institute of Environmental Health Sciences (ResearchTriangle Park, NC). TCDD dissolved in DMSO was used in the invitro studies.

L-Glutamine, HEPES, gentamicin, RPMI 1640 medium, Dulbecco'smodified Eagle's medium, PBS, and fetal bovine serum were purchasedfrom Invitrogen (Carlsbad, CA). ConA was purchased from Sigma-Aldrich(St. Louis, MO). The following monoclonal antibodies were purchasedfrom BD Biosciences Pharmingen (San Diego, CA): anti-mouse IgG-PE,FcBlock, CD3-PE (chain)-purified anti-FasL (k-10), anti-FasL-PE(Kay-10), and anti-Fas-PE (Jo2). The following inhibitors againstcaspase-3 (Z-DEVD), caspase-8 (Z-IETD-FMK), and caspase-9 (Z-LEHD-FMK)were purchased from R&D Systems (Minneapolis, MN). The followingprimary antibodies for Western blots were used: c-FLIP (CellSignaling Technology Inc., Danvers, MA) and β-actin (Sigma-Aldrich).HRP-conjugated secondary Abs was purchased from Cell SignalingTechnology Inc. RNeasy Mini kit and iScript cDNA synthesis kitwere purchased from QIAGEN (Valencia, CA). Epicenter's PCR premixF and Platinum Taq Polymerase kits were purchased from Invitrogen.TUNEL kits were purchased from Roche Diagnostics (Indianapolis,IN). ${alpha}$ -Naphthoflavone (ANF), an antagonist for AhR, was purchasedfrom Sigma-Aldrich.

Assessment of TCDD-Induced Apoptosis in Primary T Cells. Todetermine TCDD-induced apoptosis in primary T cells, T cellsfrom the spleens of three C57BL/6 mice were purified using nylonwool column (Polysciences, Warrington, PA), and the purity asdetermined by expression of CD3 and analysis by flow cytometry(Cytomics FC 500; Beckman Coulter, Fullerton, CA) was foundto be >90%. Because ConA activation of T cells requires accessorycells such as macrophages or DCs, we did not attempt to purifyT cells any further. Next, T cells were cultured with 2.5 µg/mlConA for 24 h (referred to as activated) or without ConA (referredto as nonactivated), and then they were harvested, washed, andsubsequently treated with different concentrations (10-1000nM) of TCDD for an additional 24 h. Apoptosis in naive or activatedT cells with or without DCs after TCDD or vehicle exposure wasdetermined by performing TUNEL assays (FITC-dUTP nick-end labeling)using In Situ Cell-Death Detection kit (Roche Diagnostics) asdescribed previously (Kamath et al., 1997, 1999). In brief,T cells were harvested after TCDD or vehicle treatment, andthen they were washed twice with ice-cold PBS. Cells were thenfixed in 4% paraformaldehyde for 30 to 45 min at room temperature.The cells were washed twice with ice-cold PBS, and then theywere permeabilized using freshly prepared permeabilization solutionand incubated at 4°C for 2 min. The cells were washed oncewith PBS, and then they were resuspended in 50 µl/tubeTUNEL reaction mixture and incubated for 60 min at 37°Cin a humidified atmosphere in the dark. The cells were washedtwice with PBS, and finally they were suspended in 200 to 500µl of ice-cold PBS and analyzed using flow cytometry (CytomicsFC 500; Beckman Coulter) and software.

Effect of DCs on TCDD-Induced Apoptosis in Nonactivated or ActivatedT Cells. In some experiments, purified T cells were culturedin the absence or presence of ConA for 24 h as described above.Next, mature syngeneic DCs, generated from bone marrow of C57BL/6mice, were added to these cultures along with TCDD or vehicle,and the cultures were incubated for an additional 24 h. Apoptosisin T cells was determined by staining the cells with PE-anti-CD3Abs and FITC-dUTP. DCs were generated from the bone marrowsof C57BL/6 mice by culturing the bone marrow cells with granulocytemacrophage-colony-stimulating factor and interleukin-14 (immature)followed by additional incubation with LPS (mature) as describedin our previous work (Do et al., 2004a,b). We also examinedTCDD-induced apoptosis in antigen-specific activated T cells.To this end, we used purified T cells from OT.II.2a mice, andwe cultured them in the absence or presence of mature syngeneicDCs pulsed with agonist ovalbumin peptide (Ova323-339: ISQAVHAAHAEINEAGR)for 3 days followed by addition of vehicle or TCDD to the cultures.Twenty-four hours later, the T-cell proliferation and apoptosiswere studied as described previously.

Determination of Fas and FasL Expression in Dendritic Cells.Expression of Fas and FasL in immature and mature dendriticcells was analyzed by using flow cytometry and reverse transcriptase-polymerasechain reaction (RT-PCR). In brief, dendritic cells from C57BL/6mice were generated as described previously (Do et al., 2004a,b).Immature DCs (without LPS) or mature DCs (pulsed with 100 nMLPS) for 48 h were cultured in the presence of vehicle or variousconcentrations (10-1000 nM) of TCDD for 24 h. Immature and matureDCs were harvested 24 h after vehicle or TCDD treatment, andthen they were analyzed for Fas and FasL expression using flowcytometry or RT-PCR as described previously (Singh et al., 2007).For flow cytometry, FITC-labeled anti-mouse Fas and PE-labeledanti-mouse FasL antibodies were used to stain DCs. For RT-PCR,total RNA from immature and mature DCs was isolated using RNeasyMini kit and following the protocol of the company (QIAGEN).First-strand cDNA synthesis was performed in a 20-µl reactionmix containing 2 µg of total RNA using iScript kit andfollowing the protocol of the manufacturer (Bio-Rad Laboratories,Hercules, CA). PCR was performed using mouse FasL or Fas-specificsets of forward and reverse primers. To detect mouse FasL expression(435 bp), forward (5'-CGG TGG TAT TTT TCA TGG TTC TGG-3') andreverse (5'-CTT GTG GTT TAG GGG CTG GTT GTT-3') primers wereused. Likewise, to detect the expression of mouse Fas (486 bp),forward (5'-TCT GGT GCT TGC TGG CTC AC-3') and reverse (5' CCATAG GCG ATT TCT GGG AC-3') primers were used. PCRs for bothFas and FasL were performed for 30 cycles using the followingconditions: 30 s at 95°C (denaturing temperature), 40 sat 60°C (annealing temperature), and 60 s at 72°C (extensiontemperature), with a final incubation of 10 min at 72°C.The PCR products, generated from mouse Fas and FasL primer pairs,were normalized against PCR products generated from mouse 18S-specificforward 5'-GCC CGA GCC GCC TGG ATA C-3' and reverse 5'-CCG GCGGGT CAT GGG AAT AAC-3' primers after electrophoresis on 1.5%agarose gel and visualization with UV light. The band intensityof PCR products was determined using Chemi-Doc, a Bio-Rad Laboratoriesimage analysis system.

RT-PCR to Determine the Expression of Fas and FasL in T Cells.For detection of mouse FasL (435-bp) and Fas (486-bp) expression,sets of forward and reverse primers specific to mouse Fas/FasLwere used (as described above). The PCR products, generatedfrom mouse Fas and FasL primer pairs, were normalized againstPCR products generated from β-actin (427-bp) forward (5'-AAGGCC AAC CGT GAA AAG ATG ACC-3') and reverse (5'-ACC GCT CGTTGC CAA TAG TGA TGA-3') primers after electrophoresis on 1.5%agarose gel and visualization with UV light. In some experiments,we used 18S as a control. The band intensity of PCR productswas determined using Chemi-Doc.

Blocking Assays to Determine the Role of FasL in TCDD-MediatedT-Cell Apoptosis. To investigate the role and participationof FasL in TCDD-mediated apoptosis in primary T cells, we usedConA-activated T cells as described above, and we cultured themin the absence or presence of antibody against mouse FasL (1-5µg/ml) 1 h before 100 nM TCDD treatment. Apoptosis inT cells 24 h after TCDD treatment was determined as describedpreviously. Data from three to four independent experimentswere pooled, and they are depicted as mean fluorescence units± S.E.M.

RT-PCR to Determine the Expression of AhR in T Cells. To detectthe expression of AhR in nonactivated or ConA-activated primaryT cells treated with vehicle (DMSO) or TCDD (482-bp), forward(5'-GCG GCC GCA GGA AGT GAG G-3') and reverse (5'-GTG CCG TTGATT TGC GTG TGCT-3') primers specific to mouse AhR were used.PCR was performed for 30 cycles using the following conditions:30 s at 95°C (denaturing temperature), 40 s at 60°C(annealing temperature), and 60 s at 72°C (extension temperature),with a final incubation of 10 min at 72°C. The PCR products,generated from mouse AhR primer pairs, were normalized againstPCR products generated from β-actin as described abovefor Fas and FasL. The band intensity of PCR products was determinedusing ChemiDoc image analysis system (Bio-Rad Laboratories).

Role of AhR in TCDD-Induced Regulation of Fas and FasL Expressionin T Cells. To determine the role of AhR in TCDD-induced up-regulationof Fas and FasL expression in T cells, we performed series ofin vitro assays using nonactivated and ConA-activated T cellsfrom wild-type (C57BL/6) and AhR KO mice. In brief, nonactivatedand ConA-activated (2.5 µg/ml/24 h) purified T cells fromwild-type or AhR KO mice were treated with vehicle (DMSO) or10 to 1000 nM TCDD for 24 h. Cells were harvested 24 h aftervehicle or TCDD treatment, and then they were stained usingFITC-labeled anti-mouse Fas- and PE-labeled anti-mouse FasLantibodies. Cells were analyzed for Fas and FasL expressionin T cells using flow cytometry (Cytomics FC 500; Beckman Coulter).

Role of AhR in TCDD-Induced T-Cell Apoptosis. To determine therole of AhR in TCDD-induced apoptosis, we performed a seriesof in vitro assays using T cells from wild-type (C57BL/6) andAhR KO mice. In brief, purified T cells from wild-type or AhRKO mice were activated with ConA (2.5 µg/ml) for 24 h,and then they were treated with vehicle (DMSO) or 100 to 1000nM TCDD. Apoptosis in T cells 24 h after TCDD treatments wasdetermined by performing TUNEL assays and using flow cytometry(Cytomics FC 500; Beckman Coulter) as described above. Furthermore,1 µM ANF, an antagonist for AhR, was added in the cultureof wild-type T cells 1 h before TCDD treatment, and apoptosiswas determined. Data from three to four independent experimentswere pooled, and they are depicted as mean fluorescence units± S.E.M.

Analysis of Caspase-3/7, Caspase-8, and Caspase-9 Activity.Activities of caspase-3/7, -8, and -9 were measured in T cellsexposed to TCDD using the Apo-ONE homogeneous caspase-3/7, caspase-8,and caspase-9 assays according to manufacturer's instructions(Promega, Madison, WI). In brief, ConA-activated T cells weretreated with various concentrations (1-1000 nM) of TCDD or vehicle(DMSO) for 24 h at 37°C, 5% CO₂. The following day, thecells were collected and used for caspase assays. A Wallac 1420multilabel counter, Victor² (PerkinElmer Life and AnalyticalSciences, Boston, MA) was used to measure the relative fluorescenceunits of each sample at an excitation wavelength of 485 nm andat an emission wavelength of 535 nm. Luminescence of caspase-8and caspase-9 was also measured using Wallac 1420 multilabelcounter, Victor² (PerkinElmer Life and Analytical Sciences).Data from three to four independent experiments were pooled,and they are depicted as mean fluorescence units ± S.E.M.

Caspase Blocking Assays to Determine the Role of Various Caspasesin TCDD-Induced T-Cell Apoptosis. To investigate the role andparticipation of various caspases in TCDD-mediated apoptosisin primary T cells, we performed in vitro assays as describedabove, and inhibitors specific to mouse caspase-3 (Z-DEVD),caspase-8 (Z-IETD-FMK), and caspase-9 (Z-LEHD-FMK) at a concentrationof 20 µM were added in the culture. The cells were incubatedwith caspase inhibitor for at least 1 h before TCDD treatment.These inhibitors were purchased from R&D Systems. The cellswere harvested 24 h after vehicle or TCDD treatment, and TUNELassays were performed for apoptosis as described previously.At least three independent experiments were performed, and thedata are shown represent one of the experiments.

Analysis of Mitochondrial Membrane Potential. Mitochondrialmembrane potential ( ${Delta}$ ${Psi}$ _m) of T cells after vehicle or TCDD exposurewas determined using 3,3'-dihexyloxacarboeczyme (DiOC₆; Sigma-Aldrich)as described previously (Singh et al., 2007). In brief, ConA-activatedT cells were treated with TCDD or vehicle for 24 h at 37°C,5% CO₂. The cells were harvested, washed twice with ice-coldPBS, and then they were incubated in the presence of 40 nM DiOC₆for 30 min at 4°C. After washing several times with ice-coldPBS, the cells were suspended in 200 to 500 µl of PBS,and then they were analyzed using flow cytometry (Cytomics FC500; Beckman Coulter) and software. Propidium iodide was usedto differentiate the dead cells. At least three independentexperiments were performed.

RT-PCR to Detect Expression of c-FLIP in T Cells after TCDDTreatment. To detect the expression of c-FLIP in T cells aftervehicle or TCDD treatment, total RNA from various experimentalsamples was isolated, and cDNAs were synthesized as describedabove. To detect the expression of c-FLIP (518-bp), forward(5'-GTCCTGCTGATGGAGATTG-3') and reverse (5'-GCTCCTTGGCTGGACTGGG-3') primers specific to mouse c-FLIP were used. PCR wasperformed for 30 cycles using the following conditions: 30 sat 95°C (denaturing temperature), 40 s at 58°C (annealingtemperature), and 60 s at 72°C (extension temperature),with a final incubation for 10 min at 72°C. The PCR products,generated from experimental samples of mouse T cells were normalizedagainst PCR products, generated from β-actin (427 bp) forward(5'-AAG GCC AAC CGT GAA AAG ATG ACC-3') and reverse (5'-ACCGCT CGT TGC CAA TAG TGA TGA-3') primers after electrophoresison 1.5% agarose gel and visualization of the PCR products withUV light. The band intensity of PCR products was determinedusing Chemi-Doc.

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Fig. 1. Effect of TCDD on induction of apoptosis in activated and nonactivated primary T cells in vitro. Purified primary T cells from C57BL/6 mice were cultured in the presence of ConA (activated) or absence (nonactivated) for 24 h followed by an additional culture for 24 h with TCDD. In some cultures, mature syngeneic DCs, generated from bone marrow of C57BL/6 mice, were added to these cultures along with 10 to 1000 nM TCDD or vehicle (DMSO), and the cultures were incubated for an additional 24 h. Apoptosis in T cells was determined by staining the cells with PE-anti-CD3 Abs and FITC-dUTP. The PE+ gated cells were analyzed for apoptosis using flow cytometry (Cytomics FC 500; Beckman Coulter). Data are depicted as viable cellularity (A) and apoptosis as determined by TUNEL assays (B and C). In A and C, the following comparisons made using ANOVA test and Tukey-Kramer multiple comparisons test between various groups were statistically significant (p < 0.05): vehicle versus TCDD-treated nonactivated T cells (a versus e, i, m, and q), vehicle versus TCDD-treated nonactivated T cells + DCs (b versus f, j, n, and r), vehicle versus TCDD-treated activated T cells (c versus g, k, o, and s), and vehicle versus TCDD-treated activated T cells + DCs (d versus h, l, p, and t). In addition, the following comparisons made using Student's t test between different groups after 10 to 1000 nM TCDD treatment were also statistically significant (p < 0.05): nonactivated T cells versus nonactivated T cells + DCs (e versus f, i versus j, m versus n, and q versus r), activated T cells versus activated T cells + DCs (g versus h, k versus l, o versus p, and s versus t), nonactivated versus activated T cells (e versus g, i versus k, m versus o, and q versus s), and nonactivated T cells + DCs versus activated T cells + DCs (f versus h, j versus l, n versus p, and r versus t). In B, the top percentage data represent the actual percentage of apoptosis obtained in each histogram, and the bottom percentage data represent the percentage of apoptosis seen after subtracting the background apoptosis in vehicle-treated cells. In A and C, data from five independent experiments were analyzed and depicted as mean ± S.E.M. B is a representative experiment showing the histograms.

Immunoblot Analysis. Immunoblotting was performed as describedpreviously (Singh et al., 2007

). Cell lysates were preparedby freezing and thawing, and the protein concentration was measuredusing standard Bradford assay (Bio-Rad Laboratories). The proteinswere fractionated in 12% SDS-polyacrylamide gel electrophoresisand transferred onto polyvinylidene difluoride membranes usinga DryBlot apparatus (Bio-Rad Laboratories). The membrane wasincubated in blocking buffer for 1 h at room temperature, followedby incubation in mouse-specific c-FLIP (1:1000; Cell SignalingTechnology Inc.) primary antibody, and β-actin (1:5000;Sigma-Aldrich) primary antibody at 4°C overnight. HRP-conjugatedsecondary Ab was used at 1:2000 dilutions (Cell Signaling TechnologyInc.). The membrane was then washed three times (10-15 min)with washing buffer (PBS + 0.2% Tween 20), and then it was incubatedfor 1 h in HRP-conjugated secondary antibody (Cell SignalingTechnology Inc.) in blocking buffer. The membrane was then washedseveral times and incubated in developing solution (equal volumeof solution A and B; enhanced chemiluminescence Western blottingdetection reagents; GE Healthcare, Chalfont St. Giles, Buckinghamshire,UK), and signal was detected using ChemiDoc System (Bio-RadLaboratories). Densitometric analyses of the Western blots wereperformed using ChemiDoc software (Bio-Rad Laboratories).

Transfection of Mouse Primary T Cells with Mouse c-FLIP siRNA.Primary T cells (5 x 10⁶) purified from C57BL/6 mice were transfectedwith 1.7 µM mouse siGenome ON-TARGETplus-SMART pool duplex(5-8) small interfering RNAs (siRNAs) (Dharmacon RNA Technologies,Lafayette, CO) using nucleofection of primary T cells with mouseT-cell Nucleofector transfection reagent kit and NucleofactorII electroporation system following the protocols of the company(Amaxa Biosystems, Gaithersburg, MD). As a control, 5 x 10⁶mouse T cells were transfected with mouse-specific control SiGLORISK-free siRNA (3 µg; designated control siRNA) unconjugatedor conjugated with Cy-3 (pool D-001206-13-05; Dharmacon RNATechnologies) and pmaxGFP plasmid (2 µg). TransfectedT cells were cultured for 48 h in complete medium at 37°Cand 5% CO₂.We observed >85% cell viability after transfection.To examine the efficiency of transfection, we observed pmaxGFPplasmid-transfected T cells under fluorescent microscope andobserved >60% cells expressing green fluorescent protein.We also examined the expression of fluorescent protein by performingflow cytometry (Cytomics FC 500; Beckman Coulter). T cells,untransfected (nonactivated and ConA-activated) or transfectedwith control siRNA or mouse-specific c-FLIP siRNAs, were treatedwith vehicle or 100 nM TCDD. T cells 24 h after treatment wereharvested and apoptosis was determined by performing TUNEL assayand using flow cytometry (Cytomics FC 500; Beckman Coulter).

Statistical Analysis. Results presented here represent at leastfour to five independent experiments, and they are presentedas the mean ± S.E.M. Statistical analyses were performedusing Prism software (GraphPad Software Inc., San Diego, CA).Student's t test was used for paired observations if data followeda normal distribution to compare TCDD-induced apoptosis in Tcells, expression and quantification of Fas, FasL, and AhR inDCs or in T cells, caspase assays, and quantification of proteins.The multiple comparisons were made using one-way analysis ofvariance (ANOVA) test and Tukey-Kramer multiple comparisonstests. A p value of $≤$ 0.05 is considered to be statistically significant.

Results

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Abstract
Materials and Methods
Results
Discussion
References

TCDD-Mediated Apoptosis in Primary T Cells Required Their Activationand/or Their Interaction with Dendritic Cells. We first examinedTCDD-induced apoptosis in activated and nonactivated primaryperipheral T cells in vitro. To this end, T cells were purifiedfrom the spleens of C57BL/6 mice and cultured in the absenceor presence of ConA for 24 h. Next, the cultures were incubatedwith TCDD or vehicle for an additional 24 h, and cell viabilityand apoptosis were determined. In some experimental settings,mature syngeneic DCs were added in both nonactivated and activatedT cell cultures at the time of addition of TCDD. We observeda dose-dependent decrease in viability of T cells incubatedwith TCDD, and activated T cells were more sensitive comparedwith nonactivated T cells (Fig. 1A). Similar results were obtainedusing TUNEL assays in which we noted that activated primaryT cells were more sensitive to apoptosis compared with nonactivatedT cells. It is noteworthy that when we cultured the nonactivatedT cells in the presence of syngeneic DCs and TCDD, we notedapoptosis in T cells (Fig. 1, B and C). However, we noted highestlevels of apoptosis in T cells when activated T cells were culturedin the presence of syngeneic DCs and TCDD (Fig. 1, B and C).It should be noted that in these assays, the lowest concentrationat which TCDD triggered significant levels of apoptosis was10 nM. We did not observe apoptosis in nonactivated or activatedT cells with or without DCs when 1 nM TCDD was used in the culture(data not presented). These data demonstrated that primary peripheralT cells become more susceptible to TCDD in vitro when they areactivated with ConA and especially in the presence of maturesyngeneic DCs.

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Fig. 2. TCDD causes apoptosis in antigen-specific activated T cells in vitro. Purified primary T cells from OT.II.2a mice were activated with ovalbumin-specific peptide (ISQAVHAAHAEINEAGR) by coculturing T cells and peptide-pulsed mature DCs for 3 days, and then they were treated with various doses of TCDD (100-1000 nM; A-C). Proliferation of T cells was determined by [³H]thymidine incorporation (A) 24 h after TCDD exposure and apoptosis as determined by TUNEL assays (B and C). A represents mean of triplicate cultures ± S.E.M. The following comparisons made using ANOVA and Tukey-Kramer multiple comparisons test between various groups were statistically significant (p < 0.05): proliferation of vehicle versus TCDD-treated Ova-activated OT.II.2a T cells in the presence of DCs (b versus d, f, and h). No significant (p > 0.05) difference in proliferation was observed between vehicle and TCDD-treated nonactivated OT.II.2a T cells + DCs (a versus c, e, and g). B is representative of three independent TUNEL assays, and data are depicted as mean ± S.E.M. in C. Statistical analysis using ANOVA and Tukey-Kramer multiple comparisons test showed significant (p < 0.05) difference in apoptosis between the following groups: vehicle versus TCDD-treated nonactivated OT.II.2a T cells (a versus d, g, and j), vehicle versus TCDD-treated nonactivated OT.II.2a T cells + DCs (b versus e, h, and k), and vehicle versus TCDD-treated Ova-activated OT.II.2a T cells + DCs (c versus f, i, and l).

TCDD Caused Apoptosis in Antigen-Specific Activated T Cells.Normally, professional antigen-presenting cells (APCs) suchas DCs present the processed antigens to T cells during an antigen-specificT-cell response. We therefore addressed whether during suchT-cell DC interaction, presence of TCDD would promote apoptosisin T cells. To this end, we used purified T cells from OT.II.2amice, and we cultured them in the presence of mature syngeneicDCs in the absence or presence of specific agonist ovalbuminpeptide (Ova323-339: ISQAVHAAHAEINEAGR) for 3 days, and thenwe treated them with different concentrations (100-1000 nM)of TCDD for 24 h. In these experiments, we also included culturesin which nonactivated T cells from OT.II.2a mice were incubatedwith TCDD for an additional 24 h. The T-cell proliferation wasmeasured by [³H]thymidine incorporation, and apoptosis in Tcells was determined by gating CD3-positive T cells and detectingTUNEL-positive cells. We noted a dose-dependent decrease inthe proliferative response of T cells to Ova323-339, upon TCDDtreatment (Fig. 2A). We observed low levels of TCDD-inducedapoptosis in nonactivated primary T cells (Fig. 2, B and C).It is noteworthy that Ova-specific T cells cultured with DCsin the absence of specific peptide also showed significant sensitivityto TCDD-induced apoptosis. However, highest levels of apoptosiswere detected in T cells cultured with DCs + Ova peptide (Fig. 2, B and C).Together, these data demonstrated that DCs play a critical rolein inducing apoptosis in T cells in the presence of TCDD.

TCDD Up-Regulated Fas and FasL Expression in Mature DCs. Bonemarrow-derived immature and mature DCs exposed to vehicle orvarious concentrations (10-1000 nM) of TCDD for 24 h were examinedfor expression of Fas and FasL by flow cytometry and RT-PCRusing mouse Fas/FasL-specific primers. More than 90% of allDC cultures tested expressed Fas (Fig. 3A). Furthermore, immatureDCs expressed low levels of Fas and upon maturation, they expressedsignificantly higher levels of Fas as indicated by an increasein mean fluorescent intensity (Fig. 3). Exposure of all DC culturesto TCDD did not cause a significant increase in Fas expression.Unlike Fas expression, only a small percentage of immature DCsexpressed FasL. DC maturation did not increase the density ofFasL but caused a significant increase in the percentage ofcells expressing FasL in vehicle-treated groups (Fig. 3, B and C).Addition of TCDD to DC cultures increased the percentage ofcells expressing FasL and the density of FasL particularly inmature DCs pulsed with the peptide (Fig. 3, B and C). RT-PCRdata further corroborated data generated by flow cytometry (Fig. 3, D and E).

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Fig. 3. Mature DCs express up-regulated Fas and FasL upon TCDD exposure. Immature, mature, and mature DCs pulsed with ova peptides (OvaPep), generated from C57BL/6 mice were cultured in the presence of vehicle (DMSO) or 10 to 1000 nM TCDD for 24 h. Expression of Fas and FasL in immature and mature DCs was determined by flow cytometry (A-C) or RT-PCR (D) 24 h after TCDD treatments. Data in A and B are representatives of three independent assays, which are plotted in C as mean ± S.E.M. As summarized in C, Fas expression was noted to be increased (p < 0.0001 using ANOVA and Tukey-Kramer multiple comparisons test in mature DCs or in mature DCs + Ova peptide groups compared with immature DCs (a versus i and q, b versus j and r, c versus k and s, and d versus l and t). In the above-mentioned three groups, exposure of DCs to TCDD failed to cause a significant increase of Fas (p > 0.05; a versus f, g, and h; i versus j, k, and l; and q versus r, s, and t) and FasL (p > 0.05) in immature and mature DCs groups (b versus f, n, and v and c versus l, o, and w), but it caused significant increase (p < 0.05) in FasL in mature DCs + OvaPep group (u versus v, w, and x). Data in E represent semiquantitative RT-PCR. Expressions of Fas and FasL are presented as percentage of 18S expression on the y-axis, and expression of 18S was considered to be 100% for each experiment. Data in E represent mean ± S.E.M. of three independent experiments. As summarized in E, Fas expression was noted to be increased (p < 0.0001) using ANOVA and Tukey-Kramer multiple comparisons test in mature DCs or in mature DCs + Ova peptide groups compared with immature DCs (1 versus 11 and 21, 2 versus 12 and 22, 3 versus 13 and 23, 4 versus 14 and 24, and 5 versus 15 and 25). In the above-mentioned three groups, TCDD exposure caused a significant increase in FasL (p < 0.005) in mature DCs + Ova peptide groups (26 versus 27, 28, 29, and 30), 7 versus 17 and 27, 8 versus 18 and 28, 9 versus 19 and 29, and 10 versus 20 and 30), but it did not significantly (p > 0.05) increase in immature (6 versus 7, 8, 9, and 10) or mature DCs (16 versus 17, 18, 19, and 20). MIF, mean fluorescent intensity.

TCDD Up-Regulated the Expression of Fas, FasL, and AhR in ConA-ActivatedT Cells. Previous studies from our laboratory have shown thatTCDD induces apoptosis in T cells involving Fas/FasL interactionsin vivo (Kamath et al., 1999

; Camacho et al., 2002

, 2005

). Inthe present study, therefore, we investigated whether the increasedsusceptibility of activated T cells to TCDD results from up-regulationof Fas, FasL, or AhR, in ConA-activated T cells. To this end,we determined the expression of Fas, FasL, and AhR in nonactivatedand ConA-activated T cells exposed to TCDD or vehicle, by performingRT-PCR using mouse Fas-, FasL-, and AhR-specific sets of primers.We observed significant increase in expression of Fas and FasLin TCDD-treated activated T cells compared with similar culturesof nonactivated T cells (Fig. 4, A and B).

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Fig. 4. Role of Fas and FasL in TCDD-mediated apoptosis in T cells. Expression of Fas and FasL in nonactivated or ConA-activated T cells was determined by performing RT-PCR. A, expression of Fas and FasL in nonactivated and activated T cells (RT-PCR). β-Actin was used as an internal control to normalize the expression of Fas and FasL. The band intensity of PCR products was determined using a Bio-Rad Laboratories image analysis system. The quantity of PCR products was determined using ChemiDoc image analysis software (Bio-Rad Laboratories). B, semiquantitative RT-PCR and expressions of Fas and FasL are presented as percentage of β-actin expression on the y-axis, and expression of β-actin was considered to be 100% for each experiment. Data in B are depicted as mean ± S.E.M. of three independent experiments. Significant increase in expression of Fas in TCDD-treated activated T cells was noted compared with similar cultures of nonactivated T cells (p < 0.05) by Student's t test (b versus f, c versus g, and d versus h). TCDD-treated activated T cells also showed an increase in FasL (p < 0.05) compared with nonactivated T cells (j versus n, k versus o, and l versus p). In C, ConA-activated T cells cultured with TCDD were incubated in the absence or presence of mouse-specific anti-FasL Ab, and apoptosis was studied by TUNEL assays. The data presented in C are representative of three independent experiments, and they are depicted as mean ± S.E.M. in D. Significant reduction in TCDD-mediated apoptosis of T cells cultured in the presence of anti-FasL Ab compared with T cells cultured in the absence of anti-FasL Ab (p < 0.0033 using ANOVA and Tukey-Kramer multiple comparisons test; d versus e and f, g versus h and i, and j versus k and l).

FasL Played a Significant Role in Initiating Death-ReceptorPathway during TCDD-Mediated T-Cell Apoptosis. To test whetherFasL initiates death-receptor pathway to cause TCDD-mediatedapoptosis in T cells, ConA-activated T cells were cultured inthe absence or presence of various concentrations (1-5 µg/ml)of anti-mouse FasL mAb. FasL mAb was added to the culture 1h before TCDD treatment. We observed significant (p < 0.0033)reduction in TCDD-mediated T-cell apoptosis when 1 to 5 µg/mlFasL mAb was added to the culture (Fig. 4, C and D). Additionof isotype control Abs failed to exhibit any significant effecton TCDD-mediated apoptosis (data not shown). The data obtaineddemonstrated that FasL plays a crucial role in TCDD-mediatedapoptosis in primary peripheral T cells.

Role of AhR in TCDD-Induced Up-Regulation of Fas and FasL Expressionin T Cells. Upon examination of TCDD-induced expression of AhRin T cells by RT-PCR, we observed significant (p < 0.05)increase in AhR expression in TCDD-treated nonactivated T cellscompared with vehicle-treated nonactivated T cells (Fig. 5, A and B).We also observed significant increase in AhR expression (p <0.05) in TCDD-treated activated T cells compared with vehicle-treatedactivated T cells (Fig. 5, A and B).

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Fig. 5. Role of AhR in TCDD-induced apoptosis in T cells. A, expression of AhR in nonactivated and ConA-activated T cells (RT-PCR). B, semiquantitative RT-PCR data and expressions of AhR are presented as percentage of β-actin expression on the y-axis, and expression of β-actin was considered to be 100% for each experiment. Data in B are depicted as mean ± S.E.M. of three independent experiments. TCDD, compared with the vehicle, increased the expression of AhR in both nonactivated T cells as determined by ANOVA test (p < 0.05; a versus b, c, and d) and activated T cells (p < 0.05; e versus f, g, and h), and in vehicle-treated activated T cells (p < 0.05; a versus e) compared with vehicle-treated nonactivated T cells. Data in C are summarized for three independent experiments, and they are represented as mean ± S.E.M. Significantly higher TCDD-induced expression of Fas as determined by Student's t test (p < 0.0034; c versus m, e versus o, g versus q, and i versus s) and FasL (p < 0.0001; f versus p; h versus r, and j versus t) was seen in wild-type T cells compared with AhR KO nonactivated T cells. D, expression of Fas and FasL in TCDD- or vehicle-treated activated T cells from wild-type and AhR KO mice. Data presented in D are summarized for three independent experiments and represented as mean ± S.E.M. Significantly higher TCDD-induced expression of Fas (p < 0.0036; c versus m, e versus o, g versus q, and i versus s) and FasL (p < 0.0001; f versus p, h versus r, and j versus t) as determined by Student's t test in wild-type T cells compared with AhR KO activated T cells. In E, ConA-activated T cells from wild-type and AhR KO mice were cultured with 100 and 1000 nM TCDD or vehicle (DMSO) for 24 h, and apoptosis in T cells was determined. Data presented in E represent one of three independent experiments, and vertical bars in F represent mean ± S.E.M. Significantly lower levels of apoptosis was noted in AhR KO mice compared with wild-type mice as determined by Student's t test (p < 0.0001; a versus e, b versus f, c versus g, and d versus h). In G, ConA-activated T cells from wild-type mice were cultured with 100 and 1000 nM TCDD or vehicle (DMSO) for 24 h in the absence or presence of ANF in the culture, and apoptosis in T cells was determined. Data presented in G represent one of three independent experiments, and vertical bars represent mean ± S.E.M. Significantly lower TCDD-induced apoptosis was seen in T cells when ANF was used in the culture as determined by Student's t test (p < 0.0001; c versus d, e versus f, and g versus h).

We performed a series of in vitro assays using nonactivatedor ConA-activated primary T cells from wild-type (C57BL/6) orAhR KO mice to test the role of AhR in TCDD-induced up-regulationof Fas and FasL in T cells. Upon examination of whether TCDD-inducedAhR participates in up-regulation of Fas and FasL in T cells,we observed significantly higher levels of Fas (p < 0.0034)and FasL (p < 0.0001) in wild-type T cells compared withAhR KO-nonactivated T cells (Fig. 5C); and similarly, significantlyhigher Fas (p < 0.0036) and FasL (p < 0.0001) in activatedwild-type T cells compared with activated AhR KO T cells (Fig. 5D).The data clearly demonstrated that TCDD recruits AhR to up-regulatethe expression of both Fas and FasL in T cells.

TCDD Recruited AhR to Kill Activated T Cells. We tested therole of AhR in TCDD-mediated apoptosis in activated T cells.To this end, we performed a series of in vitro assays usingprimary T cells from wild-type (C57BL/6) or AhR KO mice. Weobserved significantly less TCDD-mediated apoptosis in ConA-activatedAhR KO T cells (Fig. 5E) compared with ConA-activated T cellsfrom AhR wild-type mice at all TCDD doses tested (Fig. 5E).Likewise, we observed significant reduction in TCDD-mediatedapoptosis in ConA-activated T cells in the presence of ANF,an antagonist for AhR, compared with activated T cells thatwere cultured in the absence of ANF (Fig. 5, F and G). Thesedata together demonstrated that AhR plays a critical role inTCDD-mediated signaling and T-cell apoptosis. It should be notedthat T cells from AhR KO mice did exhibit low levels of apoptosis,particularly at higher doses of TCDD (Fig. 5E), although thiswas significantly less than that seen in AhR wild-type T cells.These data suggested that higher doses of TCDD may induce apoptosisat least in part through an AhR-independent pathway.

Both Death-Receptor (Extrinsic) and Mitochondrial (Intrinsic)Pathways Were Involved in TCDD-Mediated T-Cell Apoptosis. Toinvestigate whether TCDD-mediated apoptosis in activated T cellswas caspase-dependent, we performed enzymatic assays for variouscaspases (caspase-3/7, caspase-8, and caspase-9). We observedsignificant increase in caspase enzymatic activities for allthree caspases examined in ConA-activated and TCDD-treated Tcells compared with vehicle-treated activated T cells (Fig. 6A).This activity was dose-dependent, and it was seen at TCDD concentrationsof 10 nM and higher. The role of various caspases was furtherconfirmed by blocking caspase activity using various caspasesinhibitors (caspase-3, Z-DEVD; caspase-8, Z-IETD-FMK; and caspase-9,Z-LEHD-FMK). TUNEL assays performed on ConA-activated T cellsthat were cultured in the presence of various caspase inhibitorsand treated with 100 nM TCDD demonstrated almost complete blocking( ${approx}$ 90%) of TCDD-mediated apoptosis in the presence of caspase-3inhibitor (Fig. 6, B and C), significant blocking (>65%)in the presence of caspase-8 inhibitor (Fig. 6, B and C), andpartial blocking (<50%) in the presence of caspase-9 inhibitor(Fig. 6, B and C). Furthermore, we observed similar results(Fig. 6, D and E) when we used inhibitors against caspase-8in the culture of activated T cells, treated with various doses(100-1000 nM) of TCDD. Overall, these data demonstrated thatTCDD-mediated apoptosis in activated T cells was caspase-dependent.To further corroborate the role of mitochondrial pathway, westudied ${Delta}$ ${Psi}$ _m loss using DIOC₆ dye after TCDD or vehicle treatment.We observed significant reduction (>36%) in ${Delta}$ ${Psi}$ _m in activatedand TCDD-treated T cells (Fig. 7, A and B) compared with minimalreduction in nonactivated T cells treated with TCDD (Fig. 7, A and B).

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Fig. 6. Role of caspases in TCDD-induced apoptosis in primary T cells. Enzymatic activities of caspase-3/7, -8, and -9 were determined in ConA-activated T cells 24 h after TCDD treatment. A, shows caspase-3/7, -8, and -9 activities, and the data represent mean ± S.E.M. of three independent experiments. Asterisks (^*) represent statistically significant (p < 0.0002) increase in enzymatic activities of caspase-3, -8, and -9 in TCDD-treated T cells compared with vehicle-treated T cells. B and C, inhibitors against caspases block TCDD-mediated apoptosis in T cells. The data presented are representative of three independent experiments (B) summarized in C. There was statistically significant blocking of TCDD-induced apoptosis by various caspase inhibitors as determined by Student's t test (caspase-3: p < 0.0001, e versus f, caspase-8: p < 0.0003, e versus g, and caspase-9: p < 0.0017, e versus h). In D and E, inhibitor against caspase-8 was used in the culture together with various concentrations of TCDD (100-1000 nM). Data presented represent one of the three independent experiments performed (D), and they are summarized in E. There was statistically significant (p < 0.0003) blocking of TCDD-induced apoptosis as determined by Student's t test (c versus d, e versus f, and g versus h) when caspase-8 inhibitor was used in the culture.

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Fig. 7. Effect of TCDD on ${Delta}$ ${Psi}$ _m in ConA-activated T cells. A, ConA-activated or nonactivated T cells were treated with vehicle (DMSO) or 100 to 1000 nM TCDD as described in Fig. 1, and then they were stained with DIOC₆ to evaluate ${Delta}$ ${Psi}$ _m. Results are representative of three independent experiments, and they are summarized in B. There was a statistically significant (p < 0.0038) increase in ${Delta}$ ${Psi}$ _m in TCDD-treated activated T cells compared with vehicle-treated activated T cells (f versus g, h, i, and j) as determined by ANOVA and Tukey-Kramer multiple comparisons test. In nonactivated T cells, TCDD failed to increase the percentage of cells with loss of ${Delta}$ ${Psi}$ _m (p > 0.05; a versus b, c, d, and e).

TCDD Down-Regulated c-FLIP to Allow Apoptosis in T Cells. Presenceof c-FLIP has been shown to block Fas/FasL-mediated death-receptorpathway (Golks et al., 2005; Lavrik et al., 2005a,b). In thiscontext, expression of c-FLIP in TCDD-treated activated T cellswas evaluated by performing RT-PCR and Western blot analysis.Nonactivated T cells showed high levels of c-FLIP; furthermore,TCDD treatment did not alter the expression of cFLIP (Fig. 8, A and B).Activated T cells also showed c-FLIP expression, but interestingly,TCDD treatment caused a significant decrease in c-FLIP in activatedT cells (Fig. 8, A and B). Upon Western blot analysis, we alsoobserved significant reduction in c-FLIP expression in TCDD-treatedactivated T cells compared with vehicle-treated T cells (Fig. 8, C and D).These data suggested that c-FLIP may play a crucial role indictating the susceptibility of T cells to TCDD-induced apoptosis.

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Fig. 8. Expression of c-FLIP in primary T cells. A, nonactivated or ConA-activated T cells were treated with vehicle or 100 to 1000 nM TCDD for 24 h as described in Fig. 1 legend, and then they were evaluated for c-FLIP expression by RT-PCR. β-Actin was used as an internal control for normalization of c-FLIP expression. In B, results represent mean ± S.E.M. of three independent experiments. Expression of c-FLIP is presented as percentage of β-actin expression in the y-axis, and expression of β-actin was considered to be 100% for each experiment. There was significant (p < 0.0001) reduction in expression of c-FLIP in TCDD-treated activated T cells compared with nonactivated T cells as determined by Student's t test (d versus e, f versus g, h versus i, and j versus k). There was no significant change in c-FLIP levels in nonactivated T cells incubated with vehicle or TCDD (p > 0.05; b versus d, f, h, and j) as well as between nonactivated versus activated T cells exposed to vehicle (p > 0.05; b versus c). C, immunoprecipitation of c-FLIP using primary antibody against anti-mouse c-FLIP in ConA-activated T cells. D, results represent mean ± S.E.M. of three independent experiments. Expression of c-FLIP is presented as percentage of β-actin expression on the y-axis, and expression of β-actin was considered to be 100% for each experiment. There was statistically significant (p < 0.0003) reduction in expression of c-FLIP in TCDD-treated T cells compared with vehicle-treated T cells, as determined by ANOVA and Tukey-Kramer multiple comparisons test (c-FLIP_L: a versus c, e, and g, and i and c-FLIPs: b versus d, f, h, and j).

To further confirm the role of c-FLIP in TCDD-induced apoptosisof primary T cells in vitro, we used a RNA interference approach.siRNA consisting of 21-bp double-stranded RNA has been shownto mediate RNA interference effect in mammalian cells. We usedmouse-specific c-FLIP siRNA (Dharmacon RNA Technologies) targetingfour different sites of c-FLIP as described under Materialsand Methods. As shown in Fig. 9A, we observed more than 59%of naive T cells were siRNA-transfected. Upon Western blot analysis,we observed that c-FLIP siRNAs were able to significantly reducec-FLIP expression, whereas control siRNA had no significanteffect (Fig. 9, B and C). We also observed that blocking ofc-FLIP expression using c-FLIP siRNA in primary T cells allowedsignificant TCDD-induced apoptosis in primary T cells comparedwith T cells that were not transfected (Fig. 9D) or transfectedwith control siRNA (Fig. 9E). These data further corroboratedour earlier results showing the crucial role of c-FLIP in TCDD-inducedapoptosis in T cells in vitro.

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Fig. 9. c-FLIP plays a critical role in TCDD-induced apoptosis in primary T cells in vitro. A, primary T cells were transfected with SiGLO RISK-free control siRNA. Efficiency of transfection was determined by performing flow cytometry (Cytomics FC 500; Beckman Coulter) analysis. B, primary T cells were transfected with mouse-specific c-FLIP siRNAs. c-FLIP expression level was analyzed by Western blotting using antibody against c-FLIP. C, signal intensity of c-FLIP expression compared with β-actin. Expressions of c-FLIP is presented as percentage of β-actin expression on the y-axis, and expression of β-actin was considered to be 100% for each experiment. Vertical bars represent mean ± S.E.M. of three independent experiments, and asterisks (^*) represent statistically significant (p < 0.0002) reduction in expression of c-FLIP in T cells (b versus d) transfected with c-FLIP siRNA as determined by Student's t test. D, primary T cells untransfected (nonactivated or ConA-activated) were treated with vehicle or 10 nM TCDD for 24 h, and then they were analyzed for apoptosis using TUNEL assay. Vertical bars on the right represent mean ± S.E.M. of three independent experiments, and asterisks (^*) represent statistically significant (p < 0.0001) TCDD-induced apoptosis in activated T cells compared with vehicle-treated activated T cells as determined by Student's t test. E, primary T cells transfected with control siRNA (top) or c-FLIP siRNAs (bottom) were cultured in the presence of vehicle or 100 nM TCDD for 24 h, and then apoptosis was determined using TUNEL assay. Vertical bars (right) represent mean ± S.E.M. of three independent experiments, and asterisks (^*) represent statistically significant (p < 0.0001) TCDD-induced apoptosis in c-FLIP siRNA-transfected primary T cells compared with control siRNA-transfected primary T cells as determined by Student's t test.

Discussion

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Abstract
Materials and Methods
Results
Discussion
References

TCDD-mediated immunotoxicity has been well characterized invarious animal models (Faith and Luster, 1979; Nagarkatti etal., 1984; Greenlee et al., 1985; Fine et al., 1990; Lundberget al., 1990a,b; Holladay et al., 1991; Esser, 1994; Kerkvlietet al., 2002). Currently, the consensus is that TCDD-mediatedtoxicity is initiated by TCDD-AhR interaction, AhR-ARNT interactionwith DRE present in regulatory regions of TCDD-sensitive genes,their induction, and resultant immunotoxicity. However, theprecise molecular mechanisms underlying the immunotoxicity areyet to be fully characterized, mainly due to lack of an appropriatein vitro model. Although thymocytes and antigen-activated Tcells are highly sensitive to TCDD-mediated toxicity in vivo,it has been difficult to reproduce such findings in vitro. Tothis end, the present study demonstrates for the first timethat activated but not naive T cells are more susceptible toTCDD-mediated apoptosis in vitro.

The data obtained from our present in vitro studies demonstratethat TCDD causes apoptosis in primary T cells in vitro primarilyupon activation and triggers both death-receptor and mitochondrialpathways. These observations are based on the following findings:1) TCDD triggered apoptosis to a greater extent in activatedT cells compared with nonactivated cells; 2) TCDD induced apoptosisin antigen-specific activated T cells; 3) TCDD-mediated earlyevents/signals were initiated primarily through activation ofAhR, leading to up-regulated expression of Fas and FasL; 4)interaction of FasL with Fas triggered death-receptor pathwayby activating caspase-8 and caspase-3, culminating in apoptosis;and 5) loss of ${Delta}$ ${Psi}$ _m in activated and TCDD-treated T cells. It shouldbe noted that the nonactivated T cells showed low levels ofapoptosis. This can be explained because we had used T cellsthat were $~$ 90% enriched. Thus, the 10% cells consisting of APCsmay facilitate TCDD-induced apoptosis as evidenced by the additionof purified DCs to T-cell cultures further enhancing TCDD-inducedapoptosis. In our studies, we did not use more enriched T cellsbecause a small proportion of APCs are necessary to activateT cells using ConA (Fikri et al., 2002). We noted that if weuse highly enriched primary nonactivated T cells (>95% purity),they are completely resistant to TCDD-induced apoptosis (datanot shown).

We and others have previously shown that TCDD is not toxic tonaive T cells, but it can suppress the immune response of Tcells that are activated by an antigen in vivo (Camacho et al.,2001, 2002). This raises an important question as to why TCDDcan suppress T-cell response to an antigen in vivo, whereasit is not directly toxic to T cells in vitro. Recent studiesfrom our laboratory shed some light in this regard by demonstratingthat TCDD-induced apoptosis in thymic T cells is dependent ontheir interactions with thymus stromal cells (Camacho et al.,2004a,b, 2005). We have demonstrated previously that in vivoadministration of TCDD leads to up-regulation of Fas on T cellsand FasL on thymic stromal cells and that interaction betweenthese cells is critical for T cells to undergo apoptosis (Camachoet al., 2005). With respect to peripheral T cells, the currentstudy demonstrates that T-cell activation or interaction betweenT cells and APCs such as DCs is critical for induction of TCDD-mediatedapoptosis. The present study also demonstrates that activatedT cells become more susceptible to TCDD-mediated apoptosis becausethey express higher levels of AhR, Fas, and FasL compared withnonactivated T cells. These molecules have been shown to playa critical role in TCDD-mediated apoptosis (Fernandez-Salgueroet al., 1996; Hossain et al., 1998; Kamath et al., 1999; Camachoet al., 2001, 2002, 2004b, 2005). In addition to T-cell activation,we also noted that the presence of DCs in the culture increasedthe levels of apoptosis in T cells caused by TCDD. This observationon the role of DCs in inducing apoptosis in T cells by TCDDis somewhat similar to thymic stromal cells triggering apoptosisin thymic T cells, as described by us (Camacho et al., 2005).TCDD-mediated up-regulation of FasL in mature and Ova peptide-pulsedmature DCs explains the mechanism through which DCs may facilitateTCDD-mediated T-cell apoptosis. Our findings are consistentwith previous reports demonstrating that specific sets of DCsexpress FasL (O'Connell et al., 2000). Based on these findings,we suggest that during T-cell-DC interactions, increased levelsof FasL on DCs induced by TCDD may facilitate enhanced apoptosisin T cells.

We have also recently shown that TCDD regulates Fas and FasLpromoters through DRE and/or nuclear factor- ${kappa}$ B motifs via AhR(Camacho et al., 2005). The data obtained from the present studycorroborates the critical role played by AhR in peripheral activatedT-cell apoptosis by demonstrating 1) up-regulated expressionof AhR, Fas, and FasL upon T-cell activation; 2) minimal apoptosisin activated T cells from AhR KO mice; and 3) complete blockof TCDD-mediated apoptosis of T cells in the presence of ANF,an AhR antagonist. It should be noted that Park et al. (2003)have shown that TCDD triggered apoptosis in AhR-deficient EL4cells through insulin-like growth-binding protein-6. In primaryactivated T cells from AhR KO mice, we also noticed that athigher concentrations of TCDD (1000 nM), there was a low levelof apoptosis, thereby suggesting that TCDD at very high concentrationsmay mediate apoptosis through AhR-independent mechanisms.

Yet another reason as to why naive T cells are resistant toTCDD-mediated apoptosis could be the inability of TCDD to inhibitc-FLIP as shown in the current study. c-FLIP plays a criticalrole in the regulation of death receptor-induced apoptosis (Golkset al., 2005; Lavrik et al., 2005a,b). It is known that c-FLIPcan prevent apoptosis triggered by death-inducing ligands bybinding to the FAS-associated death domain protein and/or caspase-8and -10 at the level of the death-inducing signaling complex.It has also been shown that down-regulation of c-FLIP leadsto caspase-8 activation at the death-inducing signaling complex,and it allows death receptor-mediated pathway to proceed leadingto apoptosis (Palao et al., 2004; Golks et al., 2005; Lavriket al., 2005a,b; Salon et al., 2006). There are also reportsdemonstrating constitutive expression of c-FLIP in primary Tcells (Strauss et al., 2003; Golks et al., 2005; Lavrik et al.,2005a,b; Salon et al., 2006) and its down-regulation in T cellsallowed death receptor-mediated T-cell apoptosis (Suhara etal., 2001; Strauss et al., 2003; Tran et al., 2003; Uriarteet al., 2005). In the current study, we noted that nonactivatedT cells expressed high levels of c-FLIP. In addition, the levelsof c-FLIP expression remained unchanged in ConA-activated butvehicle-treated cells. It is noteworthy that TCDD treatmentof activated but not naive T cells caused a dramatic decreasein c-FLIP. Based on previous reports and our findings, the presenceof c-FLIP in primary T cells may be one of the important factorsprohibiting TCDD-mediated apoptosis in naive T cells in vitro.Down-regulation of c-FLIP in activated T cells induced by TCDDas seen in the current study may play a critical role in inductionof apoptosis. Moreover, down-regulation of c-FLIP expressionby siRNA led to marked susceptibility of primary T cells toTCDD-induced apoptosis in vitro.

The current study demonstrates for the first time inductionof apoptosis in T cells by TCDD in vitro. We have identifiedseveral mechanisms that explain this phenomenon. First, T-cellactivation leads to increased AhR expression, which may makethe T cells more susceptible to TCDD. Second, T-cell activationup-regulates Fas and FasL, molecules that play a critical rolein TCDD-induced apoptosis. Third, TCDD down-regulates c-FLIP,an apoptosis inhibitory molecule in activated T cells. Fourth,DCs seem to play a significant role in facilitating TCDD-mediatedapoptosis in activated T cells. The in vitro model will providethe basis for further investigating the molecular pathways throughwhich TCDD triggers apoptosis in T cells.

Acknowledgements

We thank Daniel Sisco and Shweta Hegde for technical help.

Footnotes

This work was funded in part by National Institutes of HealthGrants P01-AT03961, R01-ES09098, R01-DA016545, R01-AI058300,R01-AI053703, R01-HL058641, and R21-DA014885; A. D. WilliamsTrust Funds (to N.P.S.); and an American Cancer Society Institutionalgrant (to N.P.S.).

ABBREVIATIONS: TCDD, 2,3,7,8-tetrachlorodibenzo-p-dioxin; AhR,aryl hydrocarbon receptor; ARNT, aryl hydrocarbon receptor nucleartranslocator; DRE, dioxin responsive elements; c-FLIP, cellularFLICE inhibitory protein; DC, dendritic cell; AhR KO, aryl hydrocarbonreceptor knockout; Ova, ovalbumin; DMSO, dimethyl sulfoxide;PBS, phosphate-buffered saline; PE, phycoerythrin; FasL, Fasligand; HRP, horseradish peroxidase; Ab, antibody; PCR, polymerasechain reaction; TUNEL, terminal deoxynucleotidyl transferasedUTP nick-end labeling; ANOVA, analysis of variance; ANF, ${alpha}$ -naphthoflavone;ConA, concanavalin A; FITC, fluorescein isothiocyanate; LPS,lipopolysaccharide; RT-PCR, reverse transcriptase-polymerasechain reaction; bp, base pair(s); ${Delta}$ ${Psi}$ _m, mitochondrial membranepotential; DiOC₆,3'-dihexyloxacarboeczyme; siRNA, small interferingRNA; APC, antigen-presenting cell; mAb, monoclonal antibody;Z-, N-benzyloxycarbonyl-; FMK, fluoromethyl ketone.

Address correspondence to: Dr. Prakash S. Nagarkatti, Department of Pathology, Microbiology, and Immunology, University of South Carolina School of Medicine, Columbia, SC 29208. E-mail: pnagark{at}gw.med.sc.edu

References

Top
Abstract
Materials and Methods
Results
Discussion
References

Bock KW and Kohle C (2006) Ah receptor: dioxin-mediated toxic responses as hints to deregulated physiologic functions. Biochem Pharmacol 72: 393-404.[CrossRef][Medline]

Camacho IA, Hassuneh MR, Nagarkatti M, and Nagarkatti PS (2001) Enhanced activation-induced cell death as a mechanism of 2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD)-induced immunotoxicity in peripheral T cells. Toxicology 165: 51-63.[CrossRef][Medline]

Camacho IA, Nagarkatti M, and Nagarkatti PS (2002) 2,3,7,8-Tetrachlorodibenzo-p-dioxin (TCDD) induces Fas-dependent activation-induced cell death in superantigen-primed T cells. Arch Toxicol 76: 570-580.[CrossRef][Medline]

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