Treatment of Mice with 2,3,7,8-Tetrachlorodibenzo-p-Dioxin Leads to Aryl Hydrocarbon Receptor-Dependent Nuclear Translocation of NF-{kappa}B and Expression of Fas Ligand in Thymic Stromal Cells and Consequent Apoptosis in T Cells

HOME

HELP

FEEDBACK

SUBSCRIPTIONS

Treatment of Mice with 2,3,7,8-Tetrachlorodibenzo-p-Dioxin Leads to Aryl Hydrocarbon Receptor-Dependent Nuclear Translocation of NF- ${kappa}$ B and Expression of Fas Ligand in Thymic Stromal Cells and Consequent Apoptosis in T Cells¹

Iris A. Camacho^*, Narendra Singh, Venkatesh L. Hegde^*, Mitzi Nagarkatti^* and Prakash S. Nagarkatti²^,

Departments of^* Microbiology and Immunology and Pharmacology and Toxicology, Virginia Commonwealth University Medical Center, Richmond, VA 23298

Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Disclosures
References

We investigated the role of aryl hydrocarbon receptor (AhR)in the regulation of 2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD)-inducedapoptosis in thymic T cells. AhR knockout (KO) mice were resistantto TCDD-induced thymic atrophy and apoptosis when compared withthe AhR wild-type mice. TCDD triggered the expression of severalapoptotic genes, including FasL in AhR wild-type but not AhRKOmice. TCDD-induced increase in FasL was seen only in thymicstromal but not thymic T cells. When TCDD-exposed stromal cellswere mixed with untreated thymic T cells, increased apoptosiswas detected in T cells that involved Fas-FasL interactions.Thus, apoptosis in T cells was not detected when TCDD-treatedstromal cells from FasL-defective or AhRKO mice were mixed withwild-type T cells or when TCDD-exposed wild-type stromal cellswere mixed with Fas-deficient T cells. TCDD treatment, in vivoand in vitro, led to colocalization and translocation of NF- ${kappa}$ Bsubunits (p50, p65) to the nucleus in stromal but not T cellsfrom AhR wild-type mice. NF- ${kappa}$ B activation was not observed instromal cells isolated from TCDD-treated AhRKO mice. Mutationsin NF- ${kappa}$ B-binding sites on the FasL promoter showed that TCDDregulates FasL promoter activity through NF- ${kappa}$ B. TCDD treatmentin vivo caused activation of the death receptor and mitochondrialpathways of apoptosis. Cross-talk between the two pathways wasnot necessary for apoptosis inasmuch as TCDD-treated Bid KOmice showed thymic atrophy and increased apoptosis, similarto the wild-type mice. These findings demonstrate that AhR regulatesFasL and NF- ${kappa}$ B in stromal cells, which in turn plays a criticalrole in initiating apoptosis in thymic T cells.

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Disclosures
References

Toxic manifestations of many halogenated aromatic hydrocarbons,such as 2,3,7,8-tetrachlorodibenzo-p-dioxin ((TCDD)³ or dioxin),primarily depend on the presence of the aryl hydrocarbon receptor(AhR), which is a ligand-dependent transcription factor belongingto the superfamily of basic-helix-loop-helix DNA-binding proteins(1). Unligated AhR resides in the cytosol and its inactivityis maintained by interactions with chaperone proteins and heatshock protein 90 (2). Binding of TCDD to AhR displaces chaperoneproteins and heat shock protein 90 from the complex, generatinga ligated receptor capable of translocating into the nucleusand associating with the AhR nuclear translocator (Arnt) protein.TCDD-induced modulation of gene expression is mediated throughinteractions between the Arnt/ligated AhR complex and a 5'-GCGTG-3'DNA sequence, which is the core binding motif of dioxin responsiveelements (DRE) located in the promoter regions of AhR-responsivegenes (1). DREs have been identified in several TCDD-inducedgenes and are believed to contribute to TCDD’s potentmodulation of gene expression. Furthermore, AhR knockout (KO)mice are resistant to TCDD-mediated liver toxicity, thymic atrophy,and suppression of cell-mediated and humoral immune responses,which prove that AhR is necessary for TCDD’s action (3,4).

T cells in the thymus and periphery have been shown to be highlysensitive to TCDD-induced apoptosis. Studies from our laboratoryand elsewhere, using Fas- or FasL-mutant mice, demonstratedthat TCDD induces thymic atrophy and deletion of activated Tcells by apoptosis regulated by Fas-FasL interactions (5, 6,7, 8, 9, 10). In addition, we demonstrated that Fas gene promotercontained a functional DRE inasmuch as the binding of the AhRcomplex to this DRE led to the induction of the Fas gene inthymocytes (11). Also, while TCDD has been shown to increasethe expression of the FasL gene in the thymus (5), it does nothave a DRE in its promoter. In addition to Fas and FasL, TCDDinduces the transcriptional expression of several proapoptoticgenes in the thymus and spleen (12). In vitro studies usinghuman leukemic T cell lines and EL-4 mouse thymoma cell linesdemonstrated enhanced apoptosis following TCDD treatment viaAhR-independent but caspase-dependent mechanisms (13, 14). Interestingly,TCDD-exposed leukemic T cell lines exhibited down-regulationof bcl-2 and induction of the JNK pathway (14), implicatinga possible role for the mitochondrial pathway. Despite thesestudies, the precise molecular mechanisms underlying TCDD-inducedapoptosis in vivo remain unresolved.

The aim of the present study was to elucidate the molecularpathways of TCDD-induced apoptosis in the thymus in vivo. Weinvestigated whether TCDD-induced apoptosis is an AhR-dependentprocess and involves activation of the death-receptor and/orthe mitochondrial pathway. We also studied the precise contributionsof thymic stromal cells and T cells, in the context of Fas-FasLinteractions, in the induction of apoptosis in the thymus followingexposure to TCDD.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Disclosures
References

Materials

The following reagents were obtained from Invitrogen Life Technologies:RPMI 1640, DMEM, PBS, FBS, PCR reagents, and TRIzol reagent.The following mouse mAbs were purchased from BD Pharmingen:anti-CD4-FITC (L3T4), purified anti-CD3 (145-2C11), anti-CD3-FITC( ${epsilon}$ -chain), anti-CD8-FITC (Ly-2), anti-CD44-PE (IM7), anti- ${alpha}$ ${beta}$ TCR-FITC(H57-597), anti IL-2R-FITC (7D4), anti-J11d, anti-rat IgM-FITC,anti-CD90.1 Thy 1.1-PE (OX-7), anti-FasL (Kay-10), anti-mouseIgG, FcBlock, anti-FasL-PE (Kay-10), anti-TSA-1-FITC (MTS35,clone104), anti-Fas-PE (Jo2), anti-CD69-FITC, biotinylated anti-CD45.2(clone 104), and PE-conjugated streptavidin. For Western blotting,the following primary Abs were used: caspase-9 (1:2,000; CellSignaling), Bax (1:1,000; Cell Signaling), Bcl-x_L (1:1,000;Cell Signaling), Bid (1:1,000; R& D Systems), caspase-8(3:1,000; LabVision), caspase-2 (1:2,000; Alexis Biochemicals),Smac (1:1,000; Alexis Biochemicals), ${beta}$ -actin (1:50,000; Sigma-Aldrich),and cytochrome c (2:1,000; BD Pharmingen). HRP-conjugated secondaryAbs were obtained from Jackson ImmunoResearch Laboratories.Confocal microscopy studies were performed with the followingAbs and reagents: tosyl-phe-chloromethylketone (TPCK) (Sigma-Aldrich),goat anti-NF ${kappa}$ B p65 (c-20), rabbit anti-NF ${kappa}$ B p50 (c-19) (SantaCruz Biotechnology), anti-goat Cy3 (Jackson ImmunoResearch Laboratories),anti-rabbit Cy5 (Jackson ImmunoResearch Laboratories), Hoechst33258 (Molecular Probes), and ProLong Antifade mounting medium(Molecular Probes). Transfection and luciferase assays weredone with the following reagents: pGL3-basic vector (Promega),pCMV- ${beta}$ -galactosidase (BD Clontech) vector, the QuickChange IIsite-directed mutagenesis kit (Stratagene), the Effectene transfectionkit (Qiagen), and the Dual-Light system (Applied Biosystems).The following reagents were used in RT-PCR: RNeasy Mini kit(Qiagen), RT Kit (Qiagen), Epicentre’s PCR premix F, andPlatinum Taq Polymerase (Invitrogen Life Technologies).

Animals

AhR-deficient (AhR KO) mice created by deletion of exon 2 ofthe AhR gene (15) were generously provided as breeders by Dr.C. A. Bradfield (McArdle Laboratory for Cancer Research, Universityof Wisconsin Medical School, Madison, WI). These mice have beenbackcrossed >10 generations onto the C57BL/6 background andwere generated by breeding heterozygous (AhR^+/–) femaleswith homozygous (AhR^–/–) males. For genotyping ofAHR KO mice, the QIAamp DNA mini kit (Qiagen) was used to preparegenomic tail DNA. PCR genotypic analysis of AHR KO mice wasperformed as previously described (3). Bid-deficient (Bid KO)mice were obtained as breeders from the laboratory of Dr. S.J. Korsmeyer (Dana-Farber Cancer Institute, Harvard MedicalSchool, Boston, MA) (16). These mice were backcrossed >9generations onto the C57BL/6 background and bred as homozygotesin our animal facility. C57BL/6 mice, referred as C57BL/6 wild-type,were purchased from the National Institutes of Health (Bethesda,MD) and used as control mice. B6.PL-Thy1^a/Cy (Thy 1.1⁺) femalemice were obtained from The Jackson Laboratory and used as asource of thymocytes expressing the Thy 1.1 allele. Female C57BL/6lpr/lpr (lpr) and C57BL/6 gld/gld (gld) mice were purchasedfrom The Jackson Laboratory and bred in our animal facilities.All strains of mice were used at $~$ 6 wk of age. At this age, thelpr and gld mice on the C57BL/6 background do not develop lymphoproliferativedisease and have normal thymus (5). All animals were housedin polyethylene cages equipped with filter tops and wood shavings.Each animal cage had rodent chow and tap water ad libitum. Micewere housed in an environment of constant temperature (23 ±2°C) and on a 12 h-light:12 h-dark lighting schedule.

TCDD exposure

TCDD was generously donated by Dr. K. Chae (National Instituteon Environmental Health Sciences, Research Triangle Park, NC).TCDD was dissolved in acetone and diluted in corn oil. The solutionwas gently heated to evaporate the acetone. Animals were injectedi.p. with either a single dose of TCDD (1–50 µg/kg)or the vehicle control (corn oil).

Determination of cell viability and thymic relative weights

TCDD- or vehicle-exposed animals were euthanized, weighed, anddissected to remove the thymi. The relative thymic weights werecalculated as follows: (organ weight, mg)/(body weight, g).Single cell suspensions were prepared as previously described(5). Cell viability was determined on a hemacytometer by usingtrypan blue dye and observing the cells in an inverted phasecontrast microscope. Cell viability data from four to six experimentswere pooled and depicted as mean cellularity or mean relativeorgan weights ± SEM.

Detection of phenotypic markers on thymocytes

Thymocytes (1 x 10⁶) were washed with PBS and incubated for30 min on ice with 0.5 µg of the following primary mAbs:FITC-anti CD4 (L3T4), FITC-anti CD3 ( ${epsilon}$ -chain), FITC-anti CD8(Ly-2), PE-anti CD44 (IM7), FITC-anti ${alpha}$ ${beta}$ TCR (H57-597), FITC-antiIL-2R (7D4), anti-Fas-PE (Jo2), or anti-CD69-FITC. Detectionof J11d marker was done by staining cells with J11d mAb followedby FITC- anti-rat IgM mAbs. After incubation with the mAbs,cells were then washed once with PBS. Negative controls consistedof cells that were stained with appropriate isotype-specificAbs. Stained cells were analyzed by a BD Biosciences FACScanflow cytometer. Ten thousand cells were analyzed per sample.Dead cells, clumps, and debris were excluded electronicallyby gating on forward vs side scatter. Data were depicted aspercentage positive cells expressing the surface marker, oras mean intensity of fluorescence (MIF), which represents thedensity of expression of the surface marker. The data from fourto six independent experiments were pooled and depicted as meanMIF ± SEM.

cDNA arrays

Thymi from TCDD- or vehicle-treated mice were dissected andimmediately placed in liquid nitrogen. Total RNA was isolatedfrom thymi using the TRIzol Reagent according to the manufacturer’sinstructions (Invitrogen Life Technologies). To assess RNA integrity,RNA (1–2 µg) was mixed with an equal volume of denaturingloading buffer (2x Tris-borate-EDTA buffer, pH 8.3, 13% Ficoll,0.01% bromphenol blue, and 7 M urea), incubated at 70°Cfor 10 min followed by visualization of the 28 S and 18 S ribosomalbands on a 1% agarose gel (1x Tris-borate-EDTA buffer) at 80V for 1 h. The concentration of RNA was determined spectrophotometrically.The AmpoLabeling-LPR kit (SuperArray) was used to convert RNA(1.5 µg) to biotinylated-cDNA probe. Labeled probes werehybridized to the GEArray Q Series Mouse Apoptosis Gene arrays(SuperArray) according to the manufacturer’s instructions.

After washing, the arrays were visualized by chemiluminescenceand gene expression was quantified by scanning densitometry.A complete list of the 96 apoptosis-related genes containedin each array can be found in a recent publication from ourlaboratory (11) or at $<$ www.superarray.com $>$ . Data analysis wasdone using the GEAarray Analyzer software developed by SuperArray.All raw signal intensities were corrected for background bysubtracting the signal intensity of the negative control (pUC18DNA). Loading was also normalized based on intensity of hybridizationsignals to the housekeeping gene ${beta}$ -actin. The relative levelsof cDNA expression were assessed by comparing the signals fromTCDD-treated wild-type or AHR KO thymocytes to those obtainedby the respective control sample. Microarray data were expressedas fold increase of the signal intensity of the TCDD samplerelative to the control sample.

Studies with thymic stromal cells

The thymic stromal cells, which constitute $~$ 1–2% of thecells found in the thymus, were isolated from AhR^+/+ or AhRKO mice as described by Gray et al. (17). In some experiments,nonlymphoid stromal cells were identified by the deficiencyof CD45 using flow cytometry, which enabled us to distinguishthese cells from the T cells which express CD45, and constitute> 98% of thymocytes. Also, the CD45-deficient stromal cellsexpressed the thymic shared Ag (TSA) marker. As a source ofT cells, we used whole thymocytes by isolating the thymi frommice and subjecting them to gentle homogenization in 10% FBS/RPMI1640 medium with subsequent determination of cell viability.For coculture studies, 4 x 10⁶/ml stromal cells were culturedovernight with 2 x 10⁶ thymic T cells/ml obtained from Thy 1.1or lpr mice in 24-well plates. For blocking studies, 5 µg/mlof either anti-mouse FasL mAb (Kay-10) or a control anti-mouseIgG mAb was added to the stroma/T cell cultures. In some experiments,stromal cells from untreated wild-type mice were cultured for24 h with various concentrations of TCDD (0.1, 1, or 10 nM)or the vehicle (0.01% DMSO). To stain stromal cells (1–2x 10⁶), they were preincubated with FcBlock for 20 min to blocknonspecific binding to FcRs. Subsequently, cells were incubatedfor 30 min on ice with either PE-conjugated anti-mouse FasL(Kay-10) or FITC-conjugated anti-mouse TSA-1 (MTS35) (clone104).For CD45 staining, stromal cells were first incubated with biotinylatedanti-mouse CD45.2 mAb (clone 104) followed by PE-conjugatedstreptavidin. After final incubation, cells were washed andresuspended in 200 µl of EDTA/FACS buffer for flow cytometricanalysis. Fifty thousand cells were analyzed per sample. Immunofluorescensestainings for FasL, TSA-1, and CD45 were replicated at leastthree times and representative data were depicted as the percentageof cells expressing the marker.

RT-PCR

Total RNA was isolated from thymocytes using the TRIzol reagentaccording to the manufacturer’s instructions (InvitrogenLife Technologies). Five hundred nanograms of RNA were subjectedto cDNA synthesis using the Omniscript RT kit (Qiagen). Thereverse transcriptase reaction was run at 37°C for 1 h.First-strand cDNA was amplified in 50-µl final volumecontaining 5 µl of each primer (final concentration 0.2µM), 0.5 µl of TaqDNA polymerase, 2 µl of50 mM MgCl₂, 4 µl of 2.5 mM dNTP, 5 µl of 10x PCRbuffer, 1 µl of cDNA, and water. The amplification conditionswere 2 min at 94°C, 29 cycles at 94°C for 30 s, annealingtemperature at 40 s, 72°C for 1 min, and one final cycleat 72°C for 2 min. The following primer sequences were used:Cyp1a1 U (5'-CCC ACA GCA CCA CAA GAG ATA-3'); Cyp1a1 L (5'-AAGTAG GAG GCA GGC ACA ATG TC-3'); ${beta}$ -actin U (5'-AAG GCC AAC CGTGAA AAG ATG ACC-3'); and ${beta}$ -actin L (5'-ACC GCT CGT TGC CAA TAGTGA TGA-3'). The annealing temperatures and product sizes forthese primers are as follows: Cyp1a1 (62°C, 499 bp); and ${beta}$ -actin (55 or 62°C, 427 bp). Ten microliters of ${beta}$ -actin productand 20 µl of the other mouse gene products were resolvedon a 1.5% agarose gel. The density of the bands for vehiclevs TCDD treatment was calculated using Scion Image softwareavailable at $<$ http://rsb.info.nih.gov/nih-image $>$ . To normalizeRNA loading and PCR variations, the signals of target geneswere corrected with the signals of ${beta}$ -actin mRNA. Differencesbetween vehicle and TCDD treatments were expressed as a ratioand percent change caused by TCDD treatment. Gene expressionwas checked at least in three independent experiments and tworepresentative data were depicted.

Assessment of apoptosis

FITC-dUTP nick-end labeling or TUNEL assay (Roche Applied Science)was used to detect apoptosis in thymic T cells as previouslydescribed (5, 7). In addition, double-staining studies wereconducted to determine the amount of apoptosis in Thy 1.1⁺ thymicT cells cultured with TCDD- or vehicle-exposed stromal cells.After overnight incubation of stromal cells with Thy 1.1⁺ thymicT cells, cells were harvested and washed with PBS. Cells wereincubated with 0.5 µg of PE-conjugated anti-mouse CD90.1Thy 1.1 (OX-7) mAb for 30 min on ice followed by one wash withPBS. Similarly, stromal cultures cultured with lpr thymocyteswere harvested, washed with PBS, and stained with PE-conjugatedanti-mouse Fas mAb (0.5 µg; BD Pharmingen) for 30 minon ice followed by one wash with PBS. Next, cells were subjectedto the TUNEL protocol as described above. Fluorescence of 10,000cells was collected by flow cytometry. Electronic compensationfor fluorochrome spectral overlap was performed during flowcytometric analysis of double-stained cells. Gated Thy 1.1⁺thymocytes were analyzed for TUNEL positivity. When stromalcells were cultured with lpr thymocytes, gated Fas^– cellswere analyzed for TUNEL positivity. Data from four independentexperiments were pooled and depicted as mean percentage of apoptosis± SEM.

Analysis of mitochondrial membrane potential ( ${Delta}$ ${psi}$ _m)

Freshly isolated thymic T cells (1 x 10⁶) from TCDD- or vehicle-treatedmice were resuspended in PBS and incubated with 40 nM of 3,3'-dihexyloxacarbocynine(DIOC₆; Sigma-Aldrich) and 50 µg/ml propidium iodide (finalconcentrations) for 15 min at 37°C. Ten thousand cells wereanalyzed by flow cytometry. ${Delta}$ ${psi}$ _m was evaluated in propidium iodide-negative(live) cells and at least three independent experiments weredone.

Western blots

For preparation of tissue lysates, thymi were excised and homogenizedin cold PBS. Thymocytes (50–100 x 10⁶ cells) were lysedwith 100–200 µl of CHAPS cell extract buffer (CellSignaling). Lysates were clarified by centrifugation at 14,000rpm for 5 min, and their protein content was determined by theBradford protein assay (Bio-Rad). Ten or 50 µg of totalprotein was fractionated in a SDS-acrylamide gel, transferredto nitrocellulose, and blocked for 1 h with 5% nonfat dry milkin 1x TBS/0.1% Tween 20. Membranes were exposed to the primaryAbs overnight at 4°C on a shaker, then incubated with HRP-conjugatedsecondary Abs and processed with the ECL system according tothe manufacturer’s protocol (Amersham Biosciences). Proteinvisualization of ${beta}$ -actin expression was used as a loading control.The density of the bands was quantified by densitometry. ${beta}$ -actinwas used to normalize the samples. Western data were expressedas percentage change of the band density of the TCDD samplerelative to the vehicle control sample.

Analysis of caspase-3/7 activity

Caspase-3/7 activity was measured in thymocytes from TCDD- orvehicle-exposed mice using the Apo-ONE Homogeneous Caspase-3/7Assay according to the manufacturer’s instructions (Promega).A Wallac 1420 multilabel counter (PerkinElmer) was used to measurethe relative fluorescence units of each sample at an excitationwavelength of 485 nm and at an emission wavelength of 535 nm.Data from four to six mice were pooled and depicted as meanfluorescence units ± SEM.

Immunofluorescence staining and confocal microscopy

Stromal cells were prepared from AhR^+/+ or AhR KO mice treatedwith TCDD or the vehicle for 6 h. In some experiments, stromalcells were isolated from untreated AhR^+/+ mice and then culturedovernight with the following treatments: DMSO, 1 nM TCDD, 20µM TPCK (NF- ${kappa}$ B inhibitor; Sigma-Aldrich) or 1 nM TCDD +20 µM TPCK. The cells were treated with TPCK 1 h beforeaddition of TCDD. After treatment, stromal cells were resuspendedat 5 x 10⁶ cells/ml and 100 µl of this cell suspensionwas layered onto polylysine slides. Cells were allowed to adherefor 30 min at 37°C. Next, cells were fixed in 3.7%-bufferedparaformaldehyde at room temperature for 15 min and permeabilizedin 0.2% Triton X-100 in PBS at room temperature for 5 min. Confocalmicroscopy studies were performed with the following Abs: goatanti-NF ${kappa}$ B p65 (c-20; Santa Cruz Biotechnology), rabbit anti-NF ${kappa}$ Bp50 (c-19; Santa Cruz Biotechnology), or purified hamster anti-mouseCD3 (145-2C11; BD Pharmingen). After blocking the FcRs withrat anti-mouse CD16/CD32 (Fc Block; BD Pharmingen), Abs wereadded at appropriate concentrations for 1 h at room temperature.Subsequently, cells were washed twice in PBS and stained withanti-goat Cy3, anti-rabbit Cy5, or anti-hamster Cy2 for 1 hat room temperature. Cells were washed twice with PBS and nucleiwere stained with Hoechst 33258 for 1 min before slides weremounted in ProLong Antifade mounting medium and examined usinga Zeiss LSM 510 Meta laser scanning confocal microscope. Imageswere acquired using thin optical sections ( $~$ 0.3 µm) throughthe x-y axis. Images were collected both simultaneously andsequentially to rule out bleed through from one fluorescencechannel to another. Three independent samples were evaluatedand representative data were depicted. In NF- ${kappa}$ B nuclear translocationstudies, 50 or more cells exposed to TCDD or the vehicle wereindividually analyzed and the percentage of thymocytes showingactivation of NF- ${kappa}$ B was calculated. Also, a representative pictureof the stromal cells was depicted.

Plasmid construction and mutagenesis

The FasL promoter-reporter construct (pGL-3-FasL720) made inpGL3-basic vector, a luciferase reporter plasmid (Promega),was kindly provided by Dr. T. Ratliff (University of Iowa, IowaCity, Iowa). In this construct, FasL promoter region (720 bp)spans –689 to +65 (in reference to the translational startsite) and was generated using the upstream primer 5'-GTACCTCAGTTTTCATCTGGTGACCAGAAG-3'and the downstream primer 5'-GCACCCAGCCCCAGGAAAGG-3' (18). Site-directedmutations to NF- ${kappa}$ B sites (NF- ${kappa}$ B1 and NF- ${kappa}$ B2) present in FasL promoterwere generated using the QuickChange II Site-Directed Mutagenesiskit and according to manufacturer’s instructions (Stratagene).pGL-3-FasL720 was used as the template to generate mutations.The primers used to generate mutations as indicated by underliningthe nucleotides in NF- ${kappa}$ B1 were 5'-GAGAAAGGTGTTTAAATTGACTGC-3'and its antiparallel sequence and for NF- ${kappa}$ B2 were 5'-CCTTGGTCTTTTAAACATGCCTCAGC-3'and its antiparallel sequence. Positive clones were sequencedto confirm mutations in NF- ${kappa}$ B1 and NF- ${kappa}$ B2. In this study, we usedpGL-3 basic, pGL-3 control (Promega) vectors as controls, andpcDNA3.1 with pCMV- ${beta}$ -galactosidase (BD Clontech) vector to normalizethe transfection efficiency.

Cell culture, transfection, and luciferase assays

EL-4 cells were cultured in complete medium (complete mediumcontains DMEM supplemented with 10% FBS, 10 mM HEPES, 10 mML-glutamine, and 10 µg/ml gentamicin) at 37°C, 5%CO₂. A series of FasL promoter-luciferase constructs (pGL-3-FasL270),pGL-3 basic, pGL-3 control, and pcDNA3.1 with pCMV- ${beta}$ -galactosidasewere used in transient transfection assays. Transfections intoEL-4 cells were performed using the Effectene Transfection kitand according to the manufacturer’s instructions (Qiagen).Briefly, EL-4 cells were collected, washed twice with sterilizedPBS, and cultured in six-well plates 24 h before transfection.The following day, EL-4 cells at 50–70% confluence weretransfected with 5–10 µg/well pGL-3-FasL270, pGL-3basic, and pGL-3 control plasmid vectors and 1 µg/wellpCMV ${beta}$ -galactosidase control vector. Two days after transfection,the cells were split in 24-well plates and were exposed to 100nM/ml TCDD (dissolved in DMSO) for 18 h. The cells without treatmentor those treated with DMSO were used as controls. Luciferaseand ${beta}$ -galactosidase assays were performed using Dual-Light Systemand according to manufacturer’s instructions (AppliedBiosystems). In other sets of experiments, we used 100 ng/ml ${alpha}$ -naphthoflavone (an antagonist for TCDD) with or without TCDDin culture and Luciferase and ${beta}$ -galactosidase assays were performed.The light units were assayed by luminometry (Monolight 2010;Analytical Luminescence Laboratory). Luciferase activity wasnormalized by dividing the mean control luciferase relativelight unit (RLU) by the mean ${beta}$ -galactosidase RLU. The normalizedluciferase RLU from the samples were divided by the normalizedRLU of the untreated sample and values were expressed as "normalizedfold increase." Data obtained represent the average of threetransfection experiments, each conducted in triplicate and depictedas mean ± SD.

Detection of AhR on EL-4 cells

To detect the expression of AhR in EL4 cells, total RNA wasisolated using the RNeasy Mini kit according to the company’sprotocol (Qiagen). cDNA was synthesized using the SensiscriptRT kit (Qiagen). RT-PCR were prepared using Epicentre’sPCR premix F, Platinum Taq Polymerase (Invitrogen Life Technologies),and mouse AhR primers (mAhR forward primer: 5'-GCGGCCGCAGGAAGTGAGG-3'and mAhR reverse primer: 5'-GTGCCGTTGATT TGCGTGTGCT-3'). PCRwas performed for 30 cycles using the following parameters;30 s at 95°C, 40 s at the 60°C annealing temperature,and 60 s at 72°C, with a final incubation at 72°C for10 min. PCR product was resolved using 1.5% agarose gel. Theexpected size of the AhR PCR product was 482 bp.

Cell proliferation using [³H]thymidine assay

Lymphoid cells (5 x 10⁵ cells/well) were cultured in 96-wellplates containing 0.2 ml of medium alone or with anti-CD3 (5µg/ml; BD Pharmingen). Cells were incubated for 48 h at37°C in 5% CO₂ and pulsed with 2 µCi [³H]thymidineduring the last 8 h of incubation. Cells were harvested usingan automated cell harvester (Skatron). The amount of radioactivitywas determined using a scintillation counter (TM Analytic 6895)and the mean cpm ± SEM of triplicate cultures was calculated.Data obtained represent the average of four independent experiments,each conducted in triplicate and depicted as mean ± SD.

Statistical analysis

Results are presented as the mean ± SEM of four to sixindependent experiments per treatment group. Statistical analyseswere performed using JMP IN statistical software (SAS Institute).ANOVA was performed with a significance level of ${alpha}$ = 0.05. Comparisonamong means were made using the Tukey-Kramer honestly significantdifference test, with values of p < 0.05 considered to bestatistically significant.

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Disclosures
References

Role of AhR in regulating the effect of TCDD on thymic weight, cellularity, and apoptosis

To investigate whether TCDD-induced apoptosis in thymocytesis an AhR-dependent process, we used AhR KO mice. All mice weregenotyped as well as examined for Cyp1a1 mRNA expression inthe thymus, to confirm the genotype. Data from a representativeexperiment shown in Fig. 1A demonstrated that TCDD treatmentinduced the expression of Cyp1a1 in AhR^+/+ (wild-type) but notAhR KO mice. Next, AhR^+/+ and AhR KO mice were injected withTCDD (50 µg/kg) or the vehicle and 5 days later, thymuswas analyzed for weight, cellularity, and apoptosis. Significantreductions in relative thymic weights (Fig. 1B) and thymic cellularity(Fig. 1C) were observed in TCDD-treated AhR^+/+ but not TCDD-treatedAhR KO mice, when compared with the vehicle-treated controlgroups. We also observed that vehicle-treated AhR KO mice expressedsignificantly lower cell numbers in the thymus when comparedwith vehicle-treated AhR^+/+ mice. This resulted from the factthat AhR KO mice had smaller size thymi when compared with theAhR^+/+ mice.

View larger version (31K):
[in this window]
[in a new window]

FIGURE 1. AhR is required for TCDD-induced apoptosis in the thymus. AhR^+/+ and AhR KO mice were injected with 50 µg/kg TCDD (T) or the vehicle (V). Five days posttreatment, thymocytes were collected and used to determine Cyp1a1 mRNA expression (A), relative thymic weights (B), thymic cellularity (C), apoptosis (D), and caspase-3/7 enzymatic activity (E). D, The upper panel shows a representative histogram, and data from five to six individual experiments were pooled and summarized in the lower panel. A, Cyp1a1 expression was checked at least in three independent experiments and representative data were depicted. B, C, and E, Asterisks (_*) indicate statistically significant differences in the mean of TCDD-exposed thymocytes when compared with the vehicle controls within each group (p < 0.05).

We next examined whether the resistance to TCDD-induced thymicatrophy exhibited by AhR KO mice correlated with inability ofthymocytes to undergo apoptosis. To this end, freshly isolatedthymocytes from TCDD- or vehicle-treated AhR^+/+ and AhR KO werecultured for an additional 24 h to evaluate apoptosis usingthe TUNEL assay. This strategy offers the advantage of studyingapoptotic cells in the absence of being rapidly cleared by phagocyticcells, as known to occur in vivo (7). As seen from a representativeexperiment shown in Fig. 1D (upper panel) and pooled data fromfour to six experiments in Fig. 1D (lower panel), TCDD-treatedAhR^+/+ but not AhR KO mice showed a significant increase inpercentage of apoptotic thymocytes when compared with the vehicle-treatedmice. These data were corroborated by the observation that caspase-3/7enzymatic activity was significantly increased in thymocytesfrom AhR^+/+ but not AhR KO mice treated with TCDD (Fig. 1E).

Phenotypic and functional characterization of AhR KO mice

Because the AhR KO mice had smaller sized thymi, we performedadditional studies to test whether they had normal phenotypicand functional distribution of T cells. Double staining forCD4 and CD8 markers revealed that thymocytes from AhR KO hadnormal proportions of double-positive, double-negative, andsingle-positive T cells when compared with the AhR^+/+ mice (Fig.2A). Moreover, the thymocytes from AhR KO mice showed similarlevels and percentages of Fas⁺ and CD69⁺ T cells when comparedwith the AhR^+/+ mice (Fig. 2B). Lastly, when thymocytes wereactivated through the TCR, the proliferative response seen usingthymocytes from AhR KO mice was comparable to that seen usingAhR^+/+ mice (Fig. 2C). Together, these data suggested that thethymocytes from AhR KO mice are phenotypically and functionallysimilar to the wild-type mice.

View larger version (27K):
[in this window]
[in a new window]

FIGURE 2. Absence of AhR does not alter the phenotype and function of thymocytes. Thymocytes from untreated AhR^+/+ and AhR KO mice were double-stained with FITC-anti-CD4 and PE-anti-CD8 mAbs (A), or single-stained with PE-conjugated anti-Fas or FITC-conjugated anti-CD69 mAbs (B). Cells were then analyzed by flow cytometry. Representative dot plots or histograms are shown on the left side of A and B, respectively. The empty histograms in B represent cells stained with control Abs, and the filled histograms represent thymocytes stained for Fas or CD69. B, Also depicts the percentage of positive cells and MIF for stained cells in each histogram. On the right side of A and B, data from four to six individual experiments were collected and expressed as mean ± SEM. In C, thymocytes from untreated AhR^+/+ and AhR KO mice were cultured for 48 h with either medium alone or in the presence of anti-CD3 mAbs (5 µg/ml). Cellular proliferation was measured with a [³H]thymidine incorporation assay in four independent experiments. Data were represented as the mean cpm ± SEM of triplicate cultures of the combined experiments.

TCDD-induced phenotypic alterations in thymocytes from AhR^+/+ and AhR KO mice

Apoptotic thymocytes including those exposed to TCDD are knownto up-regulate the expression of CD3, ${alpha}$ ${beta}$ TCR, IL-2R, and CD44 markerswhile down-regulating the expression of CD4, CD8, and J11d markers(6, 19). It was possible that the thymocytes from the AhR KOmice had altered distribution of such apoptotic markers leadingto differential susceptibility to TCDD-induced apoptosis. Toaddress this, AhR^+/+ and AhR KO mice were injected with TCDDor the vehicle and analyzed for the above markers. As seen fromFig. 3, vehicle-treated AhR^+/+ and AhR KO mice exhibited similarpercentages and MIF of various T cell markers. Furthermore,TCDD-treated AhR^+/+ mice showed phenotypic alterations characteristicof apoptotic cells such as up-regulation of CD3, ${alpha}$ ${beta}$ TCR, IL-2R,and CD44 markers and down-regulation of CD4, CD8, and J11d asindicated by alterations in MIF values. Interestingly, thymocytesfrom TCDD-treated AhR KO mice failed to exhibit phenotypic changeswhen compared with their respective vehicle controls. Together,these data suggested that deficiency of AhR does not alter theexpression of several of the surface markers that we studiedin the thymus and, furthermore, it confers resistance to thephenotypic changes in the thymus induced by TCDD.

View larger version (40K):
[in this window]
[in a new window]

FIGURE 3. Effect of TCDD on phenotypic markers in the thymus of AhR^+/+ and AhR KO mice. AhR^+/+ and AhR KO mice were injected with 50 µg/kg TCDD or the vehicle. Five days posttreatment, thymocytes were stained with FITC- or PE-conjugated mAbs against CD3, ${alpha}$ ${beta}$ TCR, IL-2R, CD44, CD4, CD8, or J11d. Cells were then analyzed by flow cytometry. Representative histograms are shown for each experimental group on the left side of the figure. The empty histograms represent cells stained with control Abs, and the filled histograms represent thymocytes stained for Abs against various surface markers. The percentage of positive cells and MIF for stained cells have been depicted for each histogram. On the right side of the figure, data from four to six individual experiments were collected and expressed as mean MIF ± SEM. Asterisks (_*) indicate statistically significant differences in TCDD-exposed thymocytes when compared with the vehicle controls within each group (p < 0.05).

Identification of AhR-regulated apoptotic genes using cDNA microarray analysis

cDNA microarray analysis was used to profile apoptotic genesregulated through the AhR-signaling pathway. To this end, thymiwere collected from AhR^+/+ and AhR KO mice, 24 h after treatmentwith 50 µg/kg TCDD, and analyzed for 96 genes regulatingapoptosis. A list of the genes is available at the manufacturer’swebsite ( $<$ www.superarray.com $>$ ). Of these genes, the expressionof 14 genes appeared to be dependent on AhR expression as theywere increased >2-fold in TCDD-treated AhR^+/+ but not AhRKO mice when compared with the respective vehicle controls.Significant decrease in gene expression (>2-fold) was notdetected after TCDD treatment in either AhR^+/+ or AhR KO mice.We categorized the AhR-regulated genes into five groups as shownin Table I: 1) Bcl-2 family (Bad, Bcl-w, bid, and bok/mtd);2) TNF superfamily (FasL, OX40L, OPG, and TNFSF11); 3) apoptosis-relatedenzymes (caspase-1 and DAP kinase); 4) inhibitors of apoptosis(NAIP1 and IAP2); and 5) adaptor molecules (CRADD and TRAF5).In addition, we used MatInspector software (20) to analyze forthe presence of potential DREs in those genes that were up-regulatedby TCDD and had published promoter sequences. At least one potentialDRE sequence was found in the following genes: Bad, Bid, andOPG (data not shown). No DREs were predicted in the promoterregions of FasL. The rest of the genes in Table I were not analyzedas promoter sequences are not currently available.

View this table:
[in this window]
[in a new window]

Table I. Identification of AhR-responsive apoptotic genes by cDNA microarray^a

TCDD up-regulates FasL expression in thymic stromal cells

Interactions between thymic stromal cells and immature T cellsare known to play a critical role during T cell development.FasL, one of the triggers of the death receptor pathway, isexpressed on stromal cells but not T cells from the thymus (21).In the current study, we therefore tested whether TCDD treatmentwould up-regulate the expression of FasL on thymic stromal cellsand, if so, whether this would induce increased apoptosis inthymic T cells. To this end, we examined CD45 expression oncells isolated from the thymus, which enabled us to discriminatebetween lymphoid CD45⁺ (thymocytes) and nonlymphoid CD45^–cells (stromal cells). To further confirm that the CD45^–cells were stromal cells, we determined the expression of TSA,which is a specific marker for thymic stromal cells. Thus, whenthe CD45^– cells were gated and analyzed for TSA, over90% of the cells were TSA⁺ (Fig. 4A). Next, we enriched thethymocytes for stromal cells 24 h after injecting wild-typemice with vehicle or TCDD and examined the levels of FasL byflow cytometry. When the CD45^– cells were gated and analyzedfor FasL by flow cytometry, we noted a significant increasein the percentage of FasL⁺ cells following exposure to TCDDalong with an increase in the levels of FasL, when comparedwith vehicle-treated controls (Fig. 4B). When CD45⁺ cells fromthe thymus were similarly analyzed, the cells from vehicle-treatedmice failed to express FasL (Fig. 4C), consistent with the observationthat FasL is expressed on thymic stromal but not T cells (21).Moreover, TCDD treatment failed to induce FasL in these cells(Fig. 4C). Together, these data suggested that TCDD up-regulatesthe expression of FasL on thymic stromal cells but not on Tcells.

View larger version (23K):
[in this window]
[in a new window]

FIGURE 4. TCDD increases the expression of FasL on thymic stromal cells. A, Stromal cells from the thymi were stained with anti-CD45 mAbs and anti-TSA Abs. The CD45^– cells were gated and analyzed for TSA expression. The empty histogram represents cells stained with control Abs, and the filled histogram represents cells stained with anti-TSA Abs. B, The stromal cells exposed to TCDD or vehicle as described above were stained with anti-CD45 Abs and anti-FasL Abs. Then, the CD45^– cells were gated and analyzed for FasL. The percent FasL⁺ cells has been depicted. The histogram in red shows cells stained with Abs against FasL and the dark histogram represents cells stained with isotype control Abs. C, Thymocytes were stained with anti-CD45 mAbs and anti-FasL Abs. The CD45⁺ cells were gated and analyzed for FasL expression. The empty histogram represents cells stained with control Abs, and the filled histogram represent cells stained with anti-FasL Abs. Results are representative of at least three separate experiments.

Cell-mixing experiments to study the mechanism of TCDD-induced apoptosis in T cells

Thymic T cells express high levels of Fas. Thus, we wanted todetermine whether the TCDD-induced increase in expression ofFasL on stromal cells was sufficient to mediate higher levelsof apoptosis in T cells that come in contact with stromal cells.To this end, we tested whether coculture of FasL⁺ stromal cellsfrom TCDD-treated wild-type mice with normal untreated Fas⁺thymic T cells would lead to increased apoptosis in the latterpopulation. To ensure that we were not analyzing any T cellsfound in the stromal cell preparations from TCDD-treated mice,which could influence the results on apoptosis, we conductedmixing experiments in which Thy 1.2⁺ stromal cells isolatedfrom TCDD- or vehicle-treated mice exposed for 24 h were mixedwith freshly isolated Thy 1.1⁺ thymic T cells from untreatedThy 1.1 mice. Next, we analyzed the Thy 1.1⁺ T cells for apoptosisas described below. To confirm that the interactions betweenstromal cells and T cells involved FasL, the cultures were alsoincubated with isotype control Abs or anti-FasL mAbs. Afterovernight coculture, the cells were double-stained with PE-anti-Thy1.1 mAb and FITC-dUTP (TUNEL) to selectively detect apoptosisin Thy 1.1⁺ thymic T cells. Analysis of gated Thy 1.1⁺ cellsshowed that overnight culture of untreated Thy 1.1⁺ thymic Tcells with vehicle-exposed Thy 1.2⁺ stromal cells along withcontrol Abs resulted in significant apoptosis in Thy 1.1⁺ cells(64.3%) (Fig. 5A). This can be attributed to spontaneous apoptosisand/or FasL-induced apoptosis because normal stromal cells expressFasL as shown earlier (Fig. 4) (21). Interestingly, cultureof untreated Thy 1.1⁺ thymic T cells with TCDD-exposed Thy 1.2⁺stromal cells along with control Abs resulted in higher levelsof apoptosis in Thy 1.1⁺ cells (83.2%) (Fig. 5A). When similarmixing experiments were performed in the presence of anti-FasL(Kay-10) Abs, there was $~$ 30% decrease in Thy 1.1⁺ apoptotic cellscultured with vehicle-treated stromal cells, whereas, $~$ 50% blockingwas displayed in apoptotic Thy 1.1⁺ cells cultured with TCDD-treatedstromal cells. These data suggested that the apoptosis inducedin Thy 1.1⁺ thymic T cells following culture with TCDD-exposedstromal cells resulted at least in part from Fas-FasL interactions.Furthermore, when untreated Thy 1.1⁺ thymic T cells were mixedwith TCDD-treated stromal cells from FasL-defective (gld/gld)mice, no significant increase in apoptosis was detected in Thy1.1⁺ thymic T cells when compared with the controls (Fig. 5B).Similarly, when TCDD-exposed wild-type stromal cells were mixedwith Fas-deficient thymic T cells, there was no significantincrease in apoptosis in the latter cells when compared withthe controls (Fig. 5B). Moreover, when untreated Thy 1.1⁺ thymicT cells from wild-type mice were mixed with TCDD-treated stromalcells from AHR KO mice, no significant apoptosis was detectedin Thy 1.1⁺ thymocytes when compared with the controls (Fig.5B). These studies conclusively demonstrated that interactionsbetween TCDD-treated FasL⁺ stromal cells and untreated Fas⁺T cells can trigger increased levels of apoptosis in the lattercells. Also, AhR expression in stromal cells played a criticalrole in the apoptosis of thymocytes following TCDD treatment.

View larger version (33K):
[in this window]
[in a new window]

FIGURE 5. TCDD-induced FasL on stromal cells causes enhanced apoptosis in Fas⁺ target cells. A, Thymic stromal cells (Thy1.2⁺) were isolated 24 h posttreatment of wild-type mice with 50 µg/kg TCDD or the vehicle and cocultured overnight with Thy 1.1⁺ thymocytes, either in the presence of control Abs or anti-FasL Abs (Kay-10). Cells were then double-stained with PE-conjugated anti-Thy1.1 mAb and FITC-dUTP for TUNEL. The Thy1.1⁺ cells were gated and analyzed for apoptosis. B, Thy 1.2⁺ thymic stromal cells from (a) gld/gld, (b) wild-type, or (c) AhR KO mice exposed to 50 µg/kg TCDD or the vehicle, were cultured for 24 h with thymocytes from untreated wild-type (Thy1.1⁺) mice (a and c) or from lpr/lpr (Thy1.2⁺) mice (b). Cells were then double-stained with PE-conjugated anti-Thy1.1 (a and c) or PE-conjugated anti-Fas mAbs (b), and FITC-dUTP for TUNEL. Next, the Thy1.1⁺ (a and b) or Fas^– cells (b) were gated and analyzed for apoptosis. The right panels in A and B show pooled data from four to six experiments. Data were expressed as mean percent apoptosis ± SEM. Asterisks (_*) indicate statistically significant differences in the mean of TCDD-exposed thymocytes when compared with the vehicle controls within each group (p < 0.05).

TCDD induces activation of NF- ${kappa}$ B in thymic stromal cells

Previous studies have demonstrated that NF- ${kappa}$ B transcription factorsare involved in the expression of FasL, consequently increasingapoptosis (22, 23). Thus, we next investigated whether TCDDinduces NF- ${kappa}$ B activation in stromal cells. To this end, we usedconfocal microscopy to study nuclear translocation of NF- ${kappa}$ B inindividual stromal cells. As seen from Fig. 6A, morphologically,the stromal cells were easily distinguishable from T cells inasmuchas stromal cells were CD3 negative, larger in size and weremore granular with abundant cytoplasm, while T cells were CD3⁺,smaller in size with large nucleus. Analysis of NF- ${kappa}$ B subunits,p50 and p65, showed that they were expressed in the cytoplasmof stromal cells and T cells of vehicle-treated mice as previouslydescribed (24, 25). Interestingly, following in vivo TCDD treatment,both p50 and p65 subunits translocated to and colocalized inthe nucleus of stromal cells but not thymic T cells from AhR^+/+and AhR KO mice (Fig. 6B). Upon enumeration, 38% of the stromalcells from vehicle-treated AhR^+/+ mice were found to exhibitnuclear translocation of NF- ${kappa}$ B as against 78% in TCDD-treatedAhR^+/+ mice (data not depicted). It should be noted that unlikethe stromal cells, only 9% of T cells from vehicle-treated and11% from TCDD-treated AhR^+/+ mice showed nuclear translocationof NF- ${kappa}$ B. In vitro treatment of stromal cells with TCDD alsoshowed strong nuclear translocation and colocalization of NF- ${kappa}$ Bsubunits (p50 and p65), which was blocked by the known NF- ${kappa}$ Binhibitor TPCK (Fig. 7). Together, the confocal studies suggestedthat TCDD activates NF- ${kappa}$ B in thymic stromal cells through anAhR-dependent pathway.

View larger version (57K):
[in this window]
[in a new window]

FIGURE 6. TCDD induces activation of NF- ${kappa}$ B in thymic stromal cells. AhR^+/+ and AHR KO mice were injected with 50 µg/kg TCDD or the vehicle. Stromal cells were isolated 6 h posttreatment and used for the analysis of CD3 (A) expression and intracellular localization of NF- ${kappa}$ B p65 (green) and p50 (red) (B) in stromal cells (_*) and T cells by confocal microscopy. Cell morphology (Nomarski), colocalization of p50/p65 (yellow), and Hoechst-33258 nuclear staining (blue) are also shown. Three independent samples were evaluated and representative data were depicted.

View larger version (51K):
[in this window]
[in a new window]

FIGURE 7. Effect of NF- ${kappa}$ B inhibitor on the nuclear translocation of NF- ${kappa}$ B subunits after TCDD treatment of stromal cells in vitro. Stromal cells from untreated AhR^+/+ mice were cultured overnight with the following treatments: vehicle (DMSO), 1 nM TCDD, 1 nM TCDD + 20 µM TPCK, or 20 µM TPCK as described in Materials and Methods. Intracellular localization of NF- ${kappa}$ B p65 (green) and p50 (red) in stromal cells (_*) and T cells was visualized by confocal microscopy. Cell morphology (Nomarski), colocalization of p50/p65 (yellow), and Hoechst-33258 nuclear staining (blue) are also shown. Three independent samples were evaluated and representative data were depicted.

Role of NF- ${kappa}$ B in the activation of FasL by TCDD

As mentioned earlier, we were unable to detect DREs in the promotersequence of the mouse FasL gene as analyzed using MatInspectorsoftware (20). However, we were able to identify two NF- ${kappa}$ B siteson the promoter designated NF- ${kappa}$ B1 and NF- ${kappa}$ B2 (Fig. 8A). Therefore,we conducted a series of experiments to determine the role ofNF- ${kappa}$ B, activated by TCDD, on FasL induction using the luciferasereporter system. First, to further corroborate the ability ofTCDD to induce FasL, we used a mouse FasL promoter reporterconstruct (pGL-3-FasL720) to transfect EL-4 cells. This transformedT cell line expresses FasL and has previously been used in studyingthe regulation of gene expression (26, 27, 28). Moreover, EL-4cells also expressed the AhR as detected by RT-PCR analysis(Fig. 8B). We observed a >15-fold increase in luciferaseexpression when EL-4 cells transfected with FasL promoter weresubjected to TCDD treatment (Fig. 8C). In the same experimentalsettings, we observed very minimal (1- to 2-fold) expressionof luciferase when the cells were not treated or treated withDMSO (Fig. 8C). When ${alpha}$ -naphthoflavone, an antagonist for TCDDthat interacts with AhR, was used in combination with TCDD,luciferase induction was significantly inhibited. Furthermore,we observed no or minimal effects on luciferase induction (1-to 2-fold) when ${alpha}$ -naphthoflavone was used alone in the culture(Fig. 8C).

View larger version (37K):
[in this window]
[in a new window]

FIGURE 8. TCDD regulates FasL promoter activity through NF- ${kappa}$ B. A, Sequence of a 689-bp mouse FasL promoter upstream of the FasL translational start site has been depicted. NF- ${kappa}$ B-binding sites in the FasL promoter are underlined. B, EL-4 cells were analyzed for AhR expression using RT-PCR. C, EL-4 cells were transiently transfected with various luciferase constructs (pGL-3-FasL720, pGL-3 control) and pcDNA3.1 with pCMV- ${beta}$ -galactosidase. Two days posttransfection, the transfected cells were left untreated or treated with DMSO, 100 nM/ml TCDD, 100 nM/ml TCDD + 100 ng/ml ${alpha}$ -naphthoflavone (TCDD + AN), or 100 ng/ml ${alpha}$ -naphthoflavone alone (AN). The luciferase activity was normalized to ${beta}$ -galactosidase activity and expressed as normalized fold induction. The vertical bars represent mean ± SEM from three independent experiments. D, EL-4 cells were transiently transfected with normal NF- ${kappa}$ B luciferase construct (pGL-3-FasL720) or with various NF- ${kappa}$ B mutant luciferase constructs of FasL promoter (pGL-3-FasL720-NF- ${kappa}$ B1 mutant, pGL-3-FasL720-NF- ${kappa}$ B2 mutant, pGL-3-FasL720-NF- ${kappa}$ B1 and B2 mutants). Two days posttransfection, the transfected cells were left untreated or treated with DMSO or 100 nM/ml TCDD. Vertical bars represent mean ± SEM from three independent experiments.

Mouse FasL promoter contains at least two NF- ${kappa}$ B sites (Fig. 8A)which we designated as NF- ${kappa}$ B1 (GGTGTTTCCC) and NF- ${kappa}$ B2 (GGTCTTTTCCC).To determine the role of NF- ${kappa}$ B in up-regulation of the FasL promoter,we generated pGL-3-FasL720 constructs that carried mutationsas indicated by underlining the nucleotides in NF- ${kappa}$ B1 (GGTGTTTAAATT),NF- ${kappa}$ B2 (GGTCTTTTAAACAT), and in both NF- ${kappa}$ B1 and NF- ${kappa}$ B2. These mutantconstructs were then used in transfection of EL-4 cells. Thedata shown in Fig. 8D indicated that mutations in either NF- ${kappa}$ B1or NF- ${kappa}$ B2 caused a significant decrease in TCDD-induced luciferaseexpression (from $~$ 15- to $~$ 1–2-fold). Furthermore, mutationsin both NF- ${kappa}$ B1 and NF- ${kappa}$ B2 almost completely blocked TCDD-inducedluciferase activity. These data showed that TCDD may inducethe expression of FasL by directly regulating FasL promoteractivity through NF- ${kappa}$ B.

Role of caspases in TCDD-induced apoptosis in thymocytes

To test whether FasL-mediated apoptotic signaling in thymocytesoccurred via activation of caspase-8, Western blot analysiswas conducted with thymocytes isolated from vehicle or TCDD-treatedwild-type mice (Fig. 9A). At 18 h post-TCDD exposure, a significantincrease in cleavage of caspase-8 (47 kDa) was detected in thymocytes,when compared with levels in the vehicle controls (Fig. 9).

View larger version (29K):
[in this window]
[in a new window]

FIGURE 9. Effect of TCDD on activation of members of the death receptor and the mitochondrial pathway. Wild-type mice were injected with 50 µg/kg TCDD (T) or the vehicle (V). Cell lysates were isolated from thymocytes 12 or 18 h posttreatment. A and B, Proteins (50 µg/lane) were resolved by SDS-PAGE gel electrophoresis and probed with Abs against anti-caspase-8, caspase-9, caspase-2, bid, bax, bcl-x_L, cytochrome c (cyt C), and Smac. As a loading control, blots were stripped and reprobed with ${beta}$ -actin Abs. C, Bands were quantified, normalized to ${beta}$ -actin, and expressed as the percentage change of the band density of the TCDD sample relative to the vehicle control sample.

To address whether the mitochondrial pathway was also involved,Western blot analysis was conducted to evaluate the expressionof critical proteins involved in this pathway of apoptosis.Data shown in Fig. 9, B and C, revealed that thymocytes fromTCDD-treated wild-type mice exhibited release of cytochromec at 12 h. Moreover, TCDD treatment caused increased expressionof the Bax protein at 12 h and caspase-9 at 18 h. Cleavage ofBid, a substrate of caspase-8, was enhanced at 18 h in TCDD-exposedthymocytes, suggesting cross-talk between the two pathways ofapoptosis. No significant changes in protein expression weredetected in Smac, Bcl-x_L, and the cleaved form of caspase-2in TCDD-exposed thymocytes when compared with control groups.It should be noted that the increased levels of caspase cleavageand induction of other apoptotic molecules following TCDD treatmentwas not robust when compared with the vehicle controls. Thismay have resulted from the fact that the vehicle controls alsoshowed significant levels of caspase cleavage, which was expecteddue to spontaneous ongoing apoptosis in normal thymus. Moreover,TCDD-induced apoptotic thymocytes are rapidly cleared in vivoby phagocytic cells, thereby leaving very few apoptotic cellsto be detected upon isolation from the mice (7).

Next, we analyzed changes in the ${Delta}$ ${psi}$ _m using the DIOC₆ dye. Whenthymocytes from wild-type mice harvested 6–18 h followinginjection with 50 µg/kg TCDD were screened, a strikingreduction in ${Delta}$ ${psi}$ _m was observed at 12 h (Fig. 10A). At longer exposuretimes (>18 h), no changes in ${Delta}$ ${psi}$ _m were detected in TCDD-exposedthymocytes when compared with control cells (data not shown),possibly due to clearing of apoptotic cells in vivo. Moreover,a dose-dependent loss of ${Delta}$ ${psi}$ _m was observed in TCDD-treated thymocytesstarting at a dose of 10 µg/kg or higher (Fig. 10B).

View larger version (18K):
[in this window]
[in a new window]

FIGURE 10. Effect of TCDD on the ${Delta}$ ${psi}$ _m of thymocytes. Thymocytes were obtained from wild-type mice treated with 50 µg/kg TCDD (T) or the vehicle (V) 6, 12, or 18 h posttreatment, and then stained with DIOC₆ to evaluate ${Delta}$ ${psi}$ _m. Empty histograms represent thymocytes from vehicle-treated mice, whereas filled histograms represent thymocytes from TCDD-treated mice (A). ${Delta}$ ${psi}$ _m was also measured in thymocytes exposed in vivo for 12 h with different doses of TCDD (1, 5, 10, 25, or 50 µg/kg) (B). Results are representative of at least three separate experiments.

To further address the role of Bid in TCDD-induced apoptosis,wild-type or Bid KO mice were exposed to 50 µg/kg TCDDor the vehicle for 3 days. Both strains exhibited significantreduction in thymic cell numbers (Fig. 11A) and showed enhancedapoptosis (Fig. 11B) following TCDD treatment. It should benoted that the thymus from Bid KO mice was also sensitive toatrophy induced by TCDD when administered at 10 µg/kg(data not shown). These data suggested that Bid is dispensablefor TCDD-induced apoptosis in the thymus.

View larger version (23K):
[in this window]
[in a new window]

FIGURE 11. Role of Bid in TCDD-induced apoptosis in the thymus. Wild-type (Bid^+/+) and Bid-deficient mice were injected with 50 µg/kg TCDD or the vehicle. Three days posttreatment, thymocytes were collected and used to determine thymic cellularity (A) and apoptosis (B). The bar diagrams represent data from five to six individual mice. Asterisks (_*) indicate statistically significant between TCDD-exposed thymocytes when compared with the vehicle controls within each group (p < 0.05).

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

Previous studies from our laboratory have shown that C57BL/6mice with mutations in Fas and FasL are resistant to TCDD-inducedthymic atrophy at concentrations <50 µg/kg body weight(5, 6, 7, 8, 9, 10). However, at higher than this dose, thesemice were sensitive to thymic atrophy, thereby suggesting thatadditional alternative pathways may play a role (5). This observationwas also supported by our recent demonstration that TCDD inducesexpression of several proapoptotic genes besides Fas and FasL(11, 12). The precise mechanisms by which TCDD-induced Fas/FasLinteractions or other apoptotic genes trigger apoptosis in thymicT cells are unclear. In the current study, we conducted in-depthanalysis of the in vivo effects of TCDD on thymic apoptoticsignaling pathways. First, our results indicated that susceptibilityto TCDD-induced apoptosis in thymocytes is dependent on AhRexpression. Second, we showed that this apoptotic process mightinvolve members of the death receptor pathway and the recruitmentof caspase 8. Third, we demonstrated that TCDD treatment mightincrease FasL expression on the surface of thymic stromal cells,and that Fas⁺ T cells might undergo enhanced apoptosis wheninteracting with such stromal cells. Fourth, we found that TCDDtreatment leads to nuclear translocation of NF- ${kappa}$ B in thymic stromalcells but not T cells through an AhR-dependent process thatregulates FasL promoter activity. Last, TCDD, at higher doses,was also able to induce mitochondrial pathway of cell deathin the thymus by activating proapoptotic members of the Bcl-2family, promoting loss of ${Delta}$ ${psi}$ _m, inducing cleavage of caspase-9,and releasing cytochrome c.

Our laboratory demonstrated for the first time that thymic atrophyinduced by TCDD can be accounted for, at least in part, by inductionof apoptosis (5, 6, 7, 8). Subsequently, several studies haveextended this observation to a wide range of target tissues.TCDD is known to induce apoptosis in human T lymphoblastic andleukemic cell lines (14, 29), luteinized granulosa cells (30),central nervous tissue of zebra fish embryos (31), several tissuesof developing Fundulus heteroclitus embryos (32), vascular tissueof medaka embryos (33), and dental epithelium (34). Despitethis evidence, the mechanisms of apoptosis induced by TCDD arenot clear and may vary based on the cell type. For example,in vitro studies using T cell lines such as Jurkat, have shownthat TCDD activates MAPK-signaling pathways including JNK andERK, suggesting that MAPK pathways may be involved in TCDD-inducedcell death (35). In EL-4 T cells, it was shown that insulin-likegrowth factor-binding protein-6 was found to mediate the immunotoxiceffects of TCDD in an AhR-independent pathway (13).

The current study investigated the in vivo effects of TCDD anddemonstrated that up-regulation of FasL on thymic stromal cellsplays a crucial role in T cell apoptosis. Previous studies fromour laboratory demonstrated that FasL was up-regulated in thethymus following TCDD treatment (5). In these studies, we hadused the whole thymus and analyzed for FasL expression usingRT-PCR. In the current study, we used purified stromal cellsand T cells from the thymus and found that FasL is expressedonly in the stromal but not T cells. These data are consistentwith a recent study showing that FasL is constitutively expressedin thymic stromal cells but not in T cells. Moreover, we notedthat upon TCDD treatment, FasL was up-regulated only in thymicstromal cells but not in T cells. These data suggested thatTCDD may facilitate the expression of FasL on cells that alreadyexpress this molecule rather than induce its expression on cellsthat fail to express FasL.

Signaling through AhR may be necessary to induce the expressionof FasL inasmuch as FasL was not up-regulated in TCDD-treatedAhR-deficient mice. We confirmed these data using the luciferasereporter assay. It is interesting to note that the FasL promoterdoes not have a DRE site as analyzed by MatInspector software,thereby suggesting that its activation may be mediated throughother transcription factors. The FasL promoter contained twoNF- ${kappa}$ B sites and mutations in either or both of these sites ledto virtual abrogation of FasL promoter activity. These datasuggested that TCDD-induced activation of NF- ${kappa}$ B plays a crucialrole in the up-regulation of FasL on thymic stromal cells. NF- ${kappa}$ Btranscription factors have been previously reported to mediateFasL up-regulation and induction of apoptosis in T cells (22,23). Exposure of hepatoma cells to TCDD activates NF- ${kappa}$ B and AP-1in an AhR-dependent manner (36), consistent with the currentobservation. Induction of NF- ${kappa}$ B activity has also been shownin the immature rat thymus following TCDD treatment (37). Itshould be noted that TCDD has also been shown to inhibit theactivation of NF- ${kappa}$ B in hepatoma cells, thereby suggesting thatTCDD may exert differential effects in different cell types(38). NF- ${kappa}$ B is constitutively expressed in some subsets of immatureT cells in the thymus but not in majority of the mature T cells(25). This is consistent with our results that NF- ${kappa}$ B was notexpressed at significant levels in thymic T cells, whereas instromal cells, increased levels of NF- ${kappa}$ B were detected. Furthermore,TCDD treatment led to nuclear translocation of NF- ${kappa}$ B in the stromalcells but not T cells by an AhR-dependent manner. NF- ${kappa}$ B has beenprimarily known to function as an antiapoptotic transcriptionfactor, although some studies have suggested that it can alsoact as a proapoptotic protein depending on cell type and thenature of apoptotic inducers (39, 40). The current study isnovel inasmuch as it demonstrates that activation of NF- ${kappa}$ B byTCDD in thymic stromal cells may regulate apoptosis inductionin the thymus.

In the current study, we noted that the thymi from AhR KO micewere smaller in size and cellularity. However, comprehensiveanalysis revealed that AhR deficiency did not alter the proportionsof various T cell subsets and the expression of Fas and othermolecules were normal. Also, the T cells from the thymus respondednormally to activation through the TCR. These data suggestedthat AhR deficiency might not affect the T cell maturation orfunctions in the thymus. Thus, it is possible that the decreasedsize of the thymus in AhR KO mice may result from decreasedhoming of bone marrow stem cell precursors to the thymus, anaspect that needs further investigation. Our studies are alsoconsistent with the previous findings that peripheral immunefunctions in AhR KO mice are normal (3). It should be notedthat in an earlier study, we reported that TCDD increased theexpression of Fas in the thymus in an AhR-dependent fashion(11). The Fas gene expressed DRE in its promoter and chromatinimmunoprecipitation studies showed that the AhR complex bindsto potential DREs in the Fas gene promoter (11). Thus, whileup-regulation of Fas on T cells may further facilitate inductionof apoptosis, our studies suggest that increased expressionof FasL on thymic stromal cells is sufficient to induce enhancedapoptosis inasmuch as when Fas⁺ untreated thymic T cells wereadded to TCDD-treated stromal cells, the T cells underwent increasedapoptosis. Fig. 12 shows a schematic representation of the mechanismsof up-regulation of Fas and FasL on thymic T cells and stromalcells leading to induction of apoptosis.

View larger version (19K):
[in this window]
[in a new window]

FIGURE 12. Schematic diagram showing the mechanism by which TCDD may mediate apoptosis in thymic T cells. Ligation of AhR on thymic stromal cells leads to activation and nuclear translocation of NF- ${kappa}$ B. The FasL gene promoter has at least two NF- ${kappa}$ B-binding sites and TCDD regulates FasL promoter activity through NF- ${kappa}$ B. Such a pathway may lead to up-regulation of FasL on thymic stromal cells. In contrast, binding of TCDD to AhR on T cells leads to DRE-dependent up-regulation of Fas because the Fas gene promoter has a functional DRE as shown previously (11 ). The interactions between thymic stromal cells expressing high levels of FasL induced by TCDD and T cells expressing Fas is responsible for inducing apoptosis in the latter cells.

The current study made the novel observation that TCDD activatesboth the death receptor and mitochondrial pathways of apoptosisin thymocytes. Hepatocytes have been shown to resemble typeII cell lines in which Fas-induced death is dependent on mitochondriathrough cross-talk (16). Thus, while wild-type mice injectedwith anti-Fas Abs die from hepatocellular apoptosis, Bid-deficientmice survive from such a challenge (16). In contrast, thymocytesmay resemble type I cells inasmuch as they do not absolutelyrequire Bid for Fas-induced death, although Bid deficiency delaysapoptosis (16). Thus, in the current study, we investigatedwhether TCDD-induced apoptosis was Bid dependent. Although wenoted that Bid was cleaved in TCDD-exposed thymocytes, it wasdispensable inasmuch as Bid KO mice were as sensitive to TCDD-inducedthymic atrophy and apoptosis as the wild-type mice. Thus, inTCDD-induced apoptosis of thymocytes, the death receptor andthe mitochondrial pathways may be triggered independently. Thecoactivation of these two pathways offers an explanation asto why earlier studies found that Bcl-2 transgenic mice weresensitive to TCDD-induced thymic atrophy (41, 42).

Previous studies from a laboratory failed to detect apoptosisin thymocytes in vivo when tested for apoptosis immediatelyfollowing their isolation (41, 42, 43). These studies are similarto our previous studies that freshly isolated thymocytes fromTCDD-treated mice do not exhibit apoptosis due to rapid clearanceof apoptotic cells in the thymus by phagocytic cells, in vivo(7). Detecting apoptosis can be improved by incubating freshlyisolated thymocytes for 24 h in vitro because committed apoptoticcells can die without being removed by phagocytic cells (5,7, 9, 10, 44). Also, it is necessary to use multiple approaches(5, 6, 7, 8, 11, 12, 44) and not just a single assay to detectapoptosis (41, 42, 43).

A recent study also demonstrated that TCDD treatment led toan increase in the percentage of thymocytes in the G₁ phaseof the cell cycle and a significant decrease in the percentageof S + G₂/M thymocytes, especially in the CD4^–CD8^–CD3^–triple-negative intrathymic progenitor cell population (43).Although, clearly, multiple mechanisms of thymic atrophy inducedby TCDD could be operating in vivo, it is also likely that theTCDD-induced cell cycle arrest can subsequently trigger activationof death pathways.

As seen from the current study, in addition to Fas and FasL,we believe that DRE-linked transcriptional targets of AhR mayalso include other molecules that regulate apoptosis in thymocytesthrough death receptors and/or the mitochondria. For instance,two potential DRE sequences were reported in the Bax promoter(45), although we discovered a third DRE site using MatInspectorsoftware (20). Our analysis also revealed that promoter sequencesof Bad, Bid, and OPG genes contained potential DNA binding sequencesfor the Arnt/AhR heterodimeric complex (data not shown). Furthermore,our studies raised the possibility that Bax and Bid genes aredirectly regulated by TCDD-activated AhR as supported by increasedlevels of Bax and Bid proteins in TCDD-exposed thymocytes.

In the current study, we also noted using cDNA microarray analysisthat several genes regulating apoptosis were induced in AhR^+/+but not AhR KO mice, thereby suggesting that the induction ofthese genes may be regulated by activation through the AhR.However, it should be noted that the microarray analysis wasperformed at 24 h post-TCDD treatment and may have missed additionalgenes activated in the early or intermediate hours. In an earlierstudy, we found that, in the thymus, 23 of 37 apoptotic genesscreened were up-regulated by TCDD by a factor of two or morewhen compared with the vehicle-treated controls (12). In thecurrent study, although we used a different array for analysisconsisting of 96 apoptotic genes, it was worth noting that severalof the genes that were previously shown to be induced (12) werealso found to be regulated by the AhR. Some of these moleculesincluded Bad, Bcl-w, FasL, Caspase-1, and caspase and RIP adaptorwith death domain.

The nature of cells

Treatment of Mice with 2,3,7,8-Tetrachlorodibenzo-p-Dioxin Leads to Aryl Hydrocarbon Receptor-Dependent Nuclear Translocation of NF-B and Expression of Fas Ligand in Thymic Stromal Cells and Consequent Apoptosis in T Cells1

Treatment of Mice with 2,3,7,8-Tetrachlorodibenzo-p-Dioxin Leads to Aryl Hydrocarbon Receptor-Dependent Nuclear Translocation of NF- ${kappa}$ B and Expression of Fas Ligand in Thymic Stromal Cells and Consequent Apoptosis in T Cells¹