Head Involution Defective (Hid)-triggered Apoptosis Requires Caspase-8 but Not FADD (Fas-associated Death Domain) and Is Regulated by Erk in Mammalian Cells

doi:10.1074/jbc.M206445200

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Head Involution Defective (Hid)-triggered Apoptosis Requires Caspase-8 but Not FADD (Fas-associated Death Domain) and Is Regulated by Erk in Mammalian Cells^*

Jishy Varghese, Hadassah Sade, Peter Vandenabeele^§, and Apurva Sarin^¶

From the National Centre for Biological Sciences, UAS-GKVK Campus, Bangalore 560065, Karnataka, India and ^§ Molecular Signalling and Cell Death Unit, Department of Molecular Biology, Ledeganckstraat 35, B-9000 Gent, Belgium

Received for publication, June 28, 2002, and in revised form, July 15, 2002

ABSTRACT

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The molecular machinery of apoptosis is evolutionarily conserved with some exceptions. One such example is the Drosophilaproapoptotic gene Head involution defective (Hid), whose mammalianhomologue is not known. Hid is apoptotic to mammalian cells, andwe have examined the mechanism by which Hid induces death. Wedemonstrate for the first time a role for the extracellular signal-relatedkinase-1/2 (Erk-1/2) in the regulation of Hid function in mammaliancells. Bcl-2 and an inhibitor of caspase-9 blocked apoptosis,indicative of a role for the mitochondrion in this pathway, andwe provide evidence for a role for caspase-8 in Hid-induced apoptosis.Thus, apoptosis was blocked by an inhibitor of caspase-8, deletionof caspase-8 rendered cells resistant to Hid-induced apoptosis,and Hid associated with caspase-8 in cell lysates. The Fas-associateddeath domain (FADD) was dispensable for the apoptotic functionof Hid, indicating that Hid does not require extracellular deathreceptor signaling for the activation of caspase-8. In activatedT cells, the cytokine interleukin-2 blocked caspase-8 processingand apoptosis, suggesting that survival cues from trophic factorsmay target a Hid-like intermediate present in mammalian cells.Thus, this study shows that Hid engages with conserved componentsof cellular death machinery and suggests that apoptotic paradigmscharacterized by FADD-independent activation of caspase-8 mayinvolve a Hid-like molecule in mammaliancells.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

In metazoans, apoptosis, together with cell proliferation and differentiation, regulates the balance between cell loss andcell gain required for tissue homeostasis and embryonic development(1). Basic mechanisms of apoptosis have been conserved throughoutevolution from nematodes to humans (2, 3), and key intermediatesbelonging to the caspase family of cysteine proteases, proapoptoticmembers of the Bcl-2 family, and endogenous inhibitors of apoptosishave been identified in worms (4), flies (5), and mammals(6).

There are two major death pathways that are relatively well characterized in mammalian systems. These include extracellularreceptor-mediated apoptotic signaling (7, 8) or death pathwaysprincipally integrated via the mitochondrion (9-11). These pathwaysusually culminate in the activation of the initiator caspase-8and -9, respectively. Ligand-dependent death receptor oligomerizationrecruits cytoplasmic adapter proteins such as FADD,¹ which in turn binds the pro-form of caspase-8 and triggers itsactivation. Caspase-9 is usually activated via the release ofcytochrome c into the cytosol, an event regulated by members ofthe Bcl-2 family (12). Although death receptor-FADD interactionsare the best understood mechanism of caspase-8 activation, recentstudies have described alternative pathways that lead to the activationof caspase-8. Thus, apoptotic signaling via the B-cell receptor(13), anticancer drugs (14), and cytokines such as TGF- $beta$ (15)reportedly activate FADD-independent activation of caspase-8.The death domain in many members of the tumor necrosis factorreceptor (TNFR) superfamily in mammals is present as the genereaper in Drosophila, although a receptor-mediated death pathwayis not known in flies. Caspase activity is inhibited by the inhibitorof apoptosis protein (IAP) class of proteins, which function bybinding and inactivating processed effector and initiator caspasesincluding caspase-3, -7, and -9. The IAP proteins have characteristicbaculoviral IAP repeats that are required for their antiapoptoticfunction (16).

In Drosophila, head involution defective (Hid), a developmentally regulated gene (17), induces apoptosis by antagonizingDrosophila IAP (DIAP) (16, 18). Hid is apoptotic to mammaliancells, and apoptosis is inhibited by various antiapoptotic moleculesthat include baculoviral p35 (bvp35), Bcl-x_L, and Human X-linkedIAP (XIAP) (19). The 43-KDa Hid protein has, in addition tothe IAP-binding N terminus, five consensus p44/42 mitogen-activatedprotein kinase (MAPK) (Erk-1/2) phosphorylation domains (PX(S/T)P)(20) located between residues 121 and 257. Unlike other deathgenes identified in flies, expression of Hid mRNA is seen widelyin various stages of development, regardless of cell death fate(20, 21). Smac/DIABLO (second mitochondrial activator of caspases/directIAP-binding protein with low pI), believed to be the human equivalentof Hid in mammalian cells, has been recently identified (22,23). However, unlike Hid, overexpression of Smac/DIABLO doesnot induce apoptosis in cells (23).

In this study, we have analyzed the mechanism of Hid-induced apoptosis by utilizing mammalian cell lines of lymphoid originthat differ in their sensitivity to Hid-induced apoptosis. Wedemonstrate Erk-mediated negative regulation of Hid function inmammalian cells and demonstrate that Erk did not regulate Smac/DIABLO-mediatedpotentiation of apoptosis in the same cells. Hid activates anapoptotic pathway dependent on caspase-8. We show that Hid associateswith caspase-8, that the deletion of caspase-8 renders cells resistantto Hid, and that caspase-8 activation is independent of FADD-mediatedsignaling events. Caspase-8 processing in mitogen-stimulated Tcells is inhibited by the trophic factor interleukin-2 (IL-2)via an Erk-dependent event, suggesting that a Hid-like moleculemay be present in mammaliancells.

EXPERIMENTAL PROCEDURES

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Cells and Reagents-- Jurkat, a T lymphoblastoid line of human origin, and d11S, a murine T cell hybridoma, were used in all experiments. ActivatedT cells were generated as described before (24). The peptideinhibitors z-Val-Ala-Asp (O-methyl)-fluoromethyl ketone (zVAD-FMK),Ile-Glu-Thr-Asp-FMK (IETD-FMK), and Leu-Glu-His-Asp-FMK (LEHD-FMK)were obtained from Enzyme Systems Products (Dublin, CA). Hoechst33342 and PMA were obtained from Sigma. Antibodies to green fluorescentprotein (GFP), caspase-8, Erk-1, and p38MAPK were from Santa CruzBiotechnology (Santa Cruz, CA). Antibodies to phosphorylated Erkand U0126 were from Cell Signaling Technology, Inc. (Beverly,MA), and antibodies to full-length Bid (BH3-interacting domaindeath agonist) and TNFR-1 and TNFR-2 were from R&D Systems (Minneapolis,MN). PD98059 and LY294002 were obtained from Calbiochem.

Plasmids-- Hid cDNA was obtained from Kristin White (Harvard Medical School, Boston, MA) (21). The Hid construct was made by PCR amplificationof the open reading frame, which was cloned into the Bgl-11 andKpn-1 sites of the pEGFP-N3 vector (CLONTECH, Palo Alto, CA) withGFP in-frame in the C terminus. The bvp35 plasmid was a kind giftof Charlie Zacharchuk (NCI, National Institutes of Health). Constitutivelyactive or dominant negative MEK-1 plasmids were originally fromthe laboratories of M. J. Weber (University of Virginia HealthSciences Center, Charlottesville, Virginia) and C. J. Marshall(Institute of Cancer Research, London, UK) and were obtained fromShahid Jameel (International Center for Genetic Engineering andBiotechnology, New Delhi, India). The Smac plasmid was from X.Wang (University of Texas, Southwestern Medical Center at Dallas,Dallas TX and obtained from Dr. Santhosh (Rajiv Gandhi Centerfor Biotechnology, Thiruvananthapuram,India).

Transient Transfection of Cells-- A total of 3-5 × 10⁶ cells were transfected by electroporation at 250 mV and 960 microfarad as described previously (25).Cells were routinely transfected with 5 µg of relevant DNA unlessspecified otherwise. The total amount of DNA across all transfectiongroups in an experiment was kept constant and adjusted when requiredby additional amounts of the pEGFP-N3plasmid.

Treatment with Modulators-- In all experiments with peptide inhibitors of caspases or kinase inhibitors, agents were added to cells soon after transfection.In the experiments with PMA and UO126, UO126 was added to thecells immediately after transfection followed by the additionof PMA after 45 min. This protocol was followed to allow UO126to enter cells prior to the relatively rapid activation of Erktriggered by PMA.

Assays for Apoptotic Nuclear Damage-- Apoptotic damage was assessed using Hoechst 33342 by fluorescence microscopy as described (26). GFP-positive cells wereviewed under a blue filter, and nuclear morphology of GFP-positivecells was scored using the UVfilter.

Interactors of Hid-- Hid protein tagged with maltose-binding protein (MBP) was added to lysates made from 3 × 10⁶ Jurkat cells. MBP-tagged Hid and associated proteins were pulleddown using amylose beads, and after thorough washing, they wereanalyzed by Western blot analysis. Total cell lysates were preparedin SDS sample buffer (62.5 mM Tris-HCl, 2% w/v SDS, 10% glycerol,50 mM dithiothreitol, and 0.1% bromphenol blue), vortexed to reducesample viscosity, denatured by boiling, and then cooled on ice.Samples were resolved on 10 or 12% SDS-PAGE gels, transferredonto Hybond-ECL nitrocellulose membrane (Amersham Biosciences).Proteins were detected by chemiluminescence according to the manufacturer'sinstructions(Pierce).

T Cell Apoptosis Assays-- Freshly activated T cells were washed and cultured as such to induce spontaneous death, which could be blocked if the growthfactor interleukin-2 was added at the initiation of culture. Whenused, the blocking antibodies to TNFR-1 or TNFR-2 were also addedat the initiation of culture. For activation-induced cell death,freshly activated cells were cultured overnight in the presenceof IL-2 before being used for the assay. 0.4 × 10⁶ cells/ml were cultured for 18-20 h on dishes that had been precoatedwith 10 µg/ml anti-CD3 (clone 2C11). In all experiments with Tcell blasts, apoptotic nuclear damage was assessed using Hoechst33342.

RESULTS

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

T Cell Lines Demonstrate a Differential Susceptibility to Hid-induced Apoptosis-- In a screen of mammalian cell lines, we observed that transient overexpression of full-length Hid (Fig. 1A, Hid-FL) induceddose-dependent apoptotic nuclear damage in Jurkat T cells butnot in the d11S T cell line (Fig. 1B, solid bars). Although concentrationsas low as 1 µg of Hid-FL triggered death in Jurkat cells, d11Scells were resistant to the apoptotic effects of Hid at concentrationsas high as 20 µg (Fig. 1C, squares). Since Hid was tagged to GFP,the detection of GFP at the appropriate molecular weight by Westernblot analysis, 8-10 h after transfection (Fig. 1C, inset), confirmedexpression of the Hid protein in these cells. This time pointwas determined based on experiments that indicated near maximallevels of GFP expression by flow cytometry (data not shown). Sinceboth d11S and Jurkat cells expressed comparable levels of thetransfected gene (indicated by GFP), it appeared that resistanceto apoptosis could not be attributed to the instability of theHid protein in d11S cells. The differential effect of Hid on thesetwo cell lines was sustained if a non-tagged construct of Hidwas co-transfected with GFP (data not shown). Fig. 1D shows theinduction of apoptotic nuclear morphology (Fig. 1D, iv) in cellsexpressing Hid (Fig. 1D, iii and iv) as opposed to the normalnuclei (Fig. 1D, ii) seen in the cells expressing GFP alone (Fig.1D, i and ii). Both cell lines were equally susceptible to theproapoptotic molecule Bax, suggesting that d11S cells were specificallyresistant to Hid-induced apoptosis (Fig. 1E).

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Fig. 1. Induction of apoptosis by transient overexpression of Hid in T cell lines. Full-length Hid (Hid) includes the N terminus IAP-binding domain, Erk phosphorylation domain, and C terminus hydrophobic region tagged to GFP (A). Jurkat or d11S cells were transiently transfected with 5 µg of pEGFP-N3 plasmid (open bars) or Hid (black bars) as described under "Experimental Procedures" (B). At 18 h post-transfection, cells were harvested, and apoptotic nuclear morphology in GFP-positive cells was assessed as described in under "Experimental Procedures." Various indicated concentrations of Hid were transfected into Jurkat (circles) or d11S cells (squares) (C). The total amount of plasmid was kept constant (20 µg) by addition of appropriate concentrations of pEGFP. GFP-positive cells were assessed for apoptotic nuclei at 18 h. Inset, Western blot analysis of Hid-GFP expression probed with an antibody to GFP in Jurkat (lane 1) and d11S (lane 2) cells. Nuclear morphology (ii and iv) in cells expressing Hid (iii and iv) or GFP (i and ii) (D). Jurkat or d11S cells transfected with 5 µg of Bax (black bars) or pEGFP (open bars) were harvested at 12 h post-transfection and analyzed for apoptotic nuclear morphology (E). Results of experiments performed a minimum of three times have been shown.

These experiments showed that Hid was not generally cytotoxic and that its activity was regulated in mammalian cells. We thentested whether molecules that regulate Hid function in flies werealso conserved in mammalian cells. Members of the Ras family ofprotein kinases are key manipulators of many apoptotic pathways(27), and the Erk pathway regulates Hid-induced apoptosis inflies either via transcriptional mechanisms or via modificationof the Hid protein (20, 21). Hid has five consensus p44/42MAPK (Erk-1/2) phosphorylation domains (PX(S/T)P) (20) locatedbetween residues 121 and 257. In subsequent experiments, we testedwhether negative regulation of Hid function by Erk signaling wasalso seen in mammaliancells.

Erk Blocks Hid-induced Apoptosis in Mammalian Cells-- We compared levels of endogenous, phosphorylated Erk (pErk) in both Hid-resistant (d11S) and Hid-sensitive (Jurkat) cells.As shown in Fig. 2A, d11S cells (lanes 1 and 3) expressed higherlevels of endogenous pErk as compared with Jurkat cells (upperpanel, lanes 2 and 4), although total Erk protein was detectedin both cell lines (Fig. 2A, lower panel). The antiapoptotic roleof Erk was examined by utilizing two reagents that can inhibitMEK1/2, the kinase that phosphorylates Erk (28). Both UO126(Fig. 2B, lane 2) (29) and PD98059 (Fig. 2B, lane 3) (30)reduced levels of pErk (Fig. 2B, lane 1) following a 2-h treatmentin d11S cells. An inhibitor of phosphatidylinositol 3-kinase,LY294002 (Fig. 2B, lane 4), was without effect on pErk in thesame experiment and served as a specificity control. The inhibitorswere used to probe the functional role of the kinase in Hid-inducedapoptosis. At concentrations that reduced phosphorylation of Erk,both inhibitors revealed a sensitivity to Hid-induced apoptosisin d11S cells (Fig. 2C). These inhibitors were without effecton Hid-induced killing in Jurkat cells (data not shown). To ruleout the possibility that the protective effect of Erk was an artifactof the d11S cell line, we tested the effect of activating Erkon Hid-induced apoptosis in Jurkat cells.

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Fig. 2. Erk regulation of Hid-induced apoptosis in d11S cells. A, 10⁶ or 5 × 10⁵ d11S (lanes 1 and 3) or Jurkat cells (lanes 2 and 4) were lysed and immunoblotted with an antibody to phospho-Erk (panel 1). The same blot was stripped and reprobed for total Erk (panel 2). B, Western blot analysis of endogenous pErk in d11S cells left untreated (lane 1) or treated with 20 µM U0126 (lane 2) or 25 µM PD98059 (lane 3) or 10 µM LY294002 (lane 4) for 2 h. C, percent apoptotic damage after 18 h in d11S cells transfected with pEGFP-N3 (open bars) or Hid (black bars) and left untreated (medium) or cultured in the presence of either of the two inhibitors shown in the panel. Results derived from three to five separate analysis have been shown.

Effect of Modulating Erk on Hid-induced Death in Jurkat Cells-- Phorbol esters such as PMA activate Erk (31), and in Jurkat cells, 10 ng/ml PMA increased pErk (Fig. 3A, i and iv), whichwas blocked by UO126 (Fig. 3A, iv, lane 3). In functional assays,the same concentration of PMA reduced Hid-induced death closeto background levels (Fig. 3B), and pretreatment with UO126 priorto addition of PMA reversed the protective effect of this agenton Hid-induced apoptosis (Fig. 3B) in Jurkat cells. These experimentssuggest that PMA could act at the level of MEK1/2 since its effectwas blocked by UO126 in cells. PMA has pleiotropic effects oncells, and in subsequent experiments, we used other approachesto confirm the antiapoptotic role of Erk in this system.

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Fig. 3. Effect of modulating Erk on Hid-induced apoptosis. A, i-iii, Western blot analysis of PMA-treated Jurkat cells. Total lysates of Jurkat cells cultured in medium (lane 1) or with 10 ng/ml (lane 2) or 100 ng/ml (lane 3) PMA for 2 h have been probed for pErk (i), total Erk (ii), and total p38 MAPK (iii). Total lysates of Jurkat cells treated with PMA and U0126 were probed with antibodies to pErk (iv) and total Erk (v): lane 1, medium; lane 2, 10 ng/ml PMA; lane 3, 10 ng/ml PMA + 20 µM U0126 for 2 h. B, apoptotic damage in Jurkat cells transfected with 5 µg of Hid cultured as such, with PMA or PMA + UO126. C, apoptotic damage in Jurkat cells transfected with pEGPF-N3, Hid, Hid + CA-MEK-1, or Hid + DN-MEK-1 in the presence or absence of PMA. All experiments were performed three-five times.

Since both PD98059 and UO126 can inhibit kinases other than MEK1/2, a constitutively active form of MEK1 (S218/222D, CA-MEK)(32) was tested for its effect on Hid-triggered apoptosis. Asshown in Fig. 3C, overexpression of this construct blocked Hid-induceddeath to the same levels as those achieved by PMA. In addition,overexpression of a dominant negative form (S217/A, DN-MEK) ofthis kinase (33) reversed the protective effect of PMA on Hid-induceddeath (Fig. 3C), an observation consistent with the data usingUO126 (Fig. 3B). Thus, Hid-induced apoptosis was suppressed bythe hyperactivation of Erk as the protective effect of PMA wasreversed by the genetic approaches and pharmacological reagentsthat block phosphorylation of Erk in oursystem.

Potentiation of UV-induced Apoptosis by Smac/DIABLO Is Not Regulated by Erk Signaling-- Smac/DIABLO (a mammalian protein with some similarity to Hid) is a mitochondrial localized protein that can bind IAP and potentiateapoptosis induced by diverse stimuli (22, 23). Both Smac/DIABLOand Hid function by relieving the inhibitory effect of IAP oncaspases. Therefore we tested whether Erk signaling similarlyinhibited Smac/DIABLO potentiation of UV-induced apoptosis inJurkat cells. As shown in Fig. 4, overexpression of Smac/DIABLOincreased apoptosis triggered by UV irradiation in these cells.Overexpression of CA-MEK (Fig. 4A) or PMA (Fig. 4B) at concentrationsthat blocked the apoptotic function of Hid did not block the proapoptoticeffect of Smac/DIABLO. Since serum can protect cells during theprocess of irradiation, we show data using protocols in whichcells are irradiated in the absence (experiment 1) or presence(experiment 2) of serum containing medium for the duration ofUV exposure. Following the exposure, cells are washed and continuedin culture in complete medium.

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Fig. 4. Effect of Erk signaling on potentiation of UV-induced apoptosis by Smac/DIABLO. A, Jurkat cells transfected with control vector pEGFP-N3 or Smac/DIABLO (10 µg of each) co-transfected with or without CA-MEK. Cells were cultured overnight to allow for expression of transfected genes. Transfected groups were untreated or exposed to UV light for 6 s in the absence (experiment 1, Exp1) or presence (experiment 2, Exp2) of serum and apoptotic nuclear morphology assessed after 4 h. The graph shows results of two representative experiments. In B, Jurkat cells were transfected with 10 µg of pEGFP-N3 or Smac/DIABLO and cultured overnight. Transfected groups were exposed to UV and then cultured in the presence or absence of PMA (10 ng/ml). Apoptotic nuclear damage in all experimental groups was assessed 4 h after UV irradiation.

Hid Activates a Caspase-dependent Pathway of Apoptosis in Mammalian Cells-- In subsequent experiments, we investigated the involvement of caspases in Hid-induced apoptosis. In accordance with the literature,Hid-induced apoptosis in Jurkat cells was blocked by the antiapoptoticprotein Bcl-2 and the baculoviral pan-caspase inhibitor bvp35(Fig. 5A) (19). Death was blocked by the broad spectrum caspaseinhibitory peptide ZVAD-FMK (34, 35), the caspase-9 inhibitorypeptide LEHD-FMK, and somewhat unexpectedly by the peptide IETD-FMK,a more specific inhibitor of caspase-8 (Fig. 5B). Previous studieshave shown that Hid activates a caspase-9-dependent apoptoticdeath pathway (19), and our data with LEHD-FMK and inhibitionby Bcl-2 are consistent with this observation. However, the indicationof caspase-8 functioning as a rate-limiting step in this pathwaywas unexpected, and we used additional approaches to confirm thisobservation.

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Fig. 5. Effect of caspase inhibitors on Hid-induced apoptosis and interaction of Hid with caspase-8. Apoptotic damage after 15 h in the following conditions. A, Jurkat cells transfected with control vector or Bcl-2 or bvp35 (open bars), or Hid, Hid + Bcl-2, or Hid + bvp35 (black bars). In B, Jurkat cells transfected with 5 µg of pEGFP-N3 (open bars) or Hid (black bars) were left untreated (control) or treated with 10 µM IETD-FMK or LEHD-FMK or zVAD-FMK. C, wild type Jurkat cells, Jurkat cells deficient in caspase-8 (Caspase 8 $-$ ), or FADD (FADD $-$ ) were transfected with 5 µg of pEGFP-N3 or 5 µg of Hid. In D, total lysates of Jurkat cells transfected with 5 µg of pEGFP-N3 (lane 1) or Hid (lane 2) and cultured for 10 h were probed for Bid (panel 1) or total p38 MAPK (panel 2) by Western blot analysis. In E, MBP-tagged Hid protein or MBP alone were incubated with amylose beads for 1 h, and the Hid-MBP or MBP bound to amylose beads was incubated in Jurkat cell lysate. The amylose bead-Hid-MBP/MBP complex and associated proteins were analyzed using Western blot. The figure shows an interaction of Hid-MBP with caspase-8, cIAP-1, and cIAP-2 (lane 2), and MBP alone (lane 1) shows no association with these proteins. Expression of antiapoptotic proteins in Jurkat whole cell lysates (WCL) is also shown. Experiments were performed a minimum of three times.

Caspase-8 Is Required for Hid-induced Apoptosis-- To confirm the role of caspase-8 in this pathway, Jurkat cells that have a deletion of caspase-8 were tested for their susceptibilityto Hid. As shown in Fig. 5C (Caspase 8 $-$ ), a Jurkat line deficientfor caspase-8 (JI 9.2) was resistant to Hid, implicating caspase-8in Hid-induced apoptosis. Minimal activation of caspase-8 cleavesthe proapoptotic molecule Bid, which translocates to the mitochondrionand results in the activation of caspase-9 (36). Hid-inducedapoptotic death was accompanied by a loss of full-length Bid protein,which indicated a possible truncation of the full-length Bid protein(Fig. 5D, lane 2-Hid) in Jurkat cells. It may be noted that atthe time we detect the loss of Bid, total protein expression ofp38MAPK is unchanged in Hid-treated cells. We also tested foran interaction of Hid with caspase-8. Lysates of Jurkat cellswere incubated with purified Hid protein, and the associated complexwas isolated by immunoprecipitation of Hid. These experimentsrevealed an interaction of Hid with caspase-8, IAP-1, and IAP-2(Fig. 5E). We did not detect interactions with Bid/Bcl-2 in theseexperiments (data not shown). All these proteins are expressedin Jurkat cells (Fig. 5E, WCL).

Caspase-8 is usually activated via ligand-dependent oligomerization of cell surface receptors belonging to the superfamilyof TNFR. There are no models of death receptor-induced apoptosisin flies that have been described thus far, whereas receptor-independentactivation of caspase-8 has been described in some apoptotic paradigmsin mammalian cells (13-15). We used a Jurkat cell line with a deletionof the death adaptor protein FADD (J12.1) to test the involvementof death receptor signaling in Hid-induced apoptosis. As shownin Fig. 5C, FADD negative cells (FADD $-$ ) remained susceptible toHid-inducedapoptosis.

These experiments indicate that Hid-triggered apoptosis is dependent on caspase-8 and that apoptosis is suppressed by MEK1/2signaling in mammalian cells. In the d11S cell line, inhibitionof Erk rendered cells susceptible to Hid-induced apoptosis. Wetested whether in these experimental conditions caspases functionedas effectors of apoptosis in the d11S cell line as well. BothPD98059 (Fig. 6A) and UO126 (Fig. 6B) revealed a sensitivity toHid-induced apoptosis in the d11S cell line. Apoptosis triggeredby Hid in these conditions was blocked by the broad spectrum caspaseinhibitor bvp35 as well as the peptide inhibitors of caspase-8or -9 (Fig. 6B), thereby recreating the pathway described in Jurkatcells (Fig. 6, A and B).

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Fig. 6. Effect of caspase inhibitors on Hid-induced apoptosis in d11S cells in the presence of MEK inhibitors. A, d11S cells transfected with pEGFP-N3 or Hid or Hid+bvp35 and left untreated (control) or cultured without (open bars) or with 25 µM PD98059 (black bars). In B, d11S cells transfected with Hid were cultured as such (second bar) or in the presence of UO126 (third bar), UO126+LEHD-FMK (fourth bar), or UO126+IETD-FMK (fifth bar), and apoptotic nuclear damage was assessed for each condition after 18 h. Cells transfected with pEGFP-N3 alone were used as controls. Data plotted are means of three separate experiments.

Erk Regulation of Apoptotic Death in Activated T Cells-- Regulation by Erk and the activation of caspase-8 appear to be consistent features of the Hid-induced apoptotic pathway inlymphocytes. Trophic factors regulate survival of many cell types,and activated T cells undergo apoptosis in the absence of exogenoussurvival factors such as the cytokine IL-2 (37). As shown inFig. 7, A-C, apoptosis induced by the withdrawal of IL-2 in Tcell blasts is independent of Fas and TNFR-mediated signaling.Thus, activated T cell blasts generated from splenocytes fromnormal C57Bl/6 (triangles) or mutant Fas (C57Bl/6^lpr/lpr squares) mice undergo apoptosis in the absence of IL-2 (No IL-2,solid lines A and B), which is not blocked by soluble blockingantibodies to TNFR1 (Fig. 7A) or TNFR2 (Fig. 7B). The levels ofapoptosis were comparable in both normal and lpr/lpr mice. Theexperiment in panel C confirms that T cell blasts from lpr/lprmice are resistant to Fas ligand-Fas mediated apoptosis inducedby cross-linking the T cell receptor complex. When cultured inthe absence of IL-2 (Fig. 7D), activated T cells undergo apoptosischaracterized by the processing of caspase-8, assessed by theloss of the full-length 55-kDa pro-form over time. The progressivedisappearance of the pro-form of caspase-8 correlated with increasedlevels of apoptotic damage (Fig. 7D, values below the blot) andpreceded the loss of caspase-3 in these cells. The loss of caspase-8was blocked by IL-2 or PMA (Fig. 7E). Both reagents also inducedthe phosphorylation of Erk in these cells (Fig. 7E). Furthermore,the inhibition of caspase-8 processing and the antiapoptotic effectof IL-2 (Fig. 7, F and G) or PMA (Fig. 7G) was reversed by UO126,indicating a role for Erk in the regulation of this caspase inT cells.

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Fig. 7. Regulation of spontaneous death in T cells by Erk. In A and B, activated T cell blasts from C57Bl/6 or C57Bl/6^lpr/lpr mice were washed and cultured with or without IL-2 in the presence of various concentrations of blocking antibodies to TNFR1 or TNFR2 as shown in the figure. In C, anti-CD3 induced apoptosis in T cell blasts from C57Bl/6 or C57Bl/6^lpr/lpr mice. In D, T cell blasts were cultured in the absence of IL-2. Cells were harvested at indicated time points and assayed for expression of unprocessed caspase-8, caspase-3, and Bcl-x_L by Western blot analysis. Numbers below the blot represent apoptotic nuclei scored in a typical experiment. In E, cell lysates prepared from T cell blasts cultured overnight in the presence or absence of IL-2 or PMA were probed for caspase-8 and phosphorylation of Erk. In F, lysates from T cell blasts cultured in the presence (IL-2) and absence of IL-2 (GFW) and UO126 were assessed for expression of caspase-8. G, in an experiment similar to that described in panel F, cells were cultured overnight in various conditions described in the figure and analyzed for levels of apoptotic nuclear damage.

	DISCUSSION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

In this study, we demonstrate that Hid-induced apoptosis is dependent on both caspase-8 and -9 and, as demonstrated in flies,the apoptotic pathway is regulated by Erk in mammalian cells aswell. The antiapoptotic function of Erk in this death pathwaywas inferred from the following experiments: a cell line thatwas resistant to Hid-induced apoptosis had high constitutive expressionof pErk, and inhibition of MEK-1/2 revealed sensitivity to Hid-inducedapoptosis in these cells (Fig. 2). In the Jurkat cell line, aconstitutively active form of MEK1 blocked Hid-induced apoptosis(Fig. 3C), the phorbol ester PMA blocked Hid-induced apoptosis,and protection was reversed by UO126 (an inhibitor of MEK) ora dominant negative MEK construct, identifying MEK as a key componentof the PMA-induced antiapoptoticpathway.

Erk is a member of the family of MAPKs downstream of Ras and is recruited into multiple signaling cascades (27). Prosurvivalfunctions have been described for other members of this familyof kinases (26, 38), and their function is conserved acrossvarious species of metazoans (39). Hid function is negativelyregulated by Ras through the Drosophila Erk homologue, rolled,which down-regulates Hid expression (21) and inactivates Hidby phosphorylation (20). Our data are consistent with the latterstudy and show that despite enforced expression of Hid, apoptoticactivity was regulated by endogenous Erk in mammalian cells. Theinvolvement of this key regulatory event laid the foundation forthe analysis of the mechanism by which Hid triggered apoptosisin mammalian cells. Our experiments show that Smac/DIABLO-inducedpotentiation of death is not regulated by Erk signaling (Fig.4), consistent with the absence of conventional Erk phosphorylationsites on thismolecule.

That Hid-induced death may be integrated by the mitochondrion, culminating in the activation of caspase-9, has been reportedearlier (19). Activation or recruitment of caspase-9 requiresthe formation of an apoptogenic complex that includes co-factorsdATP, Apaf-1, and cytochrome c (40). Apoptogenic complex formationis regulated by antiapoptotic members of the Bcl-2 family, whichregulate the release of cytochrome c. Inhibition of Hid-inducedapoptosis by Bcl-2, bvp35, and LEHD-FMK is consistent with a rolefor the mitochondrion in this pathway. However, the followingexperiments, unexpectedly, also indicated a role for caspase-8in this pathway: Hid-induced apoptosis was blocked by a peptideinhibitor specific for this caspase; enforced expression of Hidtriggered the truncation of Bid, a preferred substrate for caspase-8,and more conclusively, a Jurkat mutant with a deletion for caspase-8was resistant to Hid-induced apoptosis. Furthermore, purifiedHid protein, when used as a probe, immunoprecipitated caspase-8,cIAP-1, and cIAP-2 from Jurkat cell lysates. We did not detectan interaction between Bid/Bcl-xL although these proteins areexpressed in Jurkat cells. The latter experiments are consistentwith the model that Hid promotes caspase activity by binding andantagonizing IAP function. Thus, we propose that Hid activatescaspase-8, thereby triggering a cascade that involves the mitochondrion,culminating in the activation of caspase-9 and the death ofcells.

Caspase-8 activation is linked to the oligomerization of death receptors and recruitment of adaptors containing death domains.However, no death domain has thus far been identified in Hid,prompting us to determine whether caspase-8 was activated by recruitmentof the adaptor protein FADD. Since Jurkat cells with a deletionin the FADD gene were susceptible to Hid-induced apoptosis, ourdata suggest a FADD-independent mechanism of caspase-8 activationdescribed in other systems (13-15).

Caspases similar to caspase-8 (DREDD, Ref. 41) and caspase-9 (DRONC, Ref. 42) have been described in the apoptotic machineryin Drosophila. However, death receptor signaling has not so farbeen demonstrated in flies. It should be noted that a deficiencythat removed the DREDD gene suppressed Hid-induced apoptosis inthe fly eye (43). The mechanism of Hid-induced apoptosis andits regulation appears to be highly conserved in mammalian cells(19). Our analysis in mammalian cells proposes a model of Hidinteraction with the caspase-network and members of the Bcl-2family that may likely be conserved in flies aswell.

Cell survival in most tissues is dependent on survival cues from neighboring cells or the extracellular matrix. Thus, it isof interest to understand the mechanisms by which molecules suchas trophic factors block intrinsic death programs. EGF signalingvia Erk has been reported to block Hid-induced apoptosis in Drosophila(44). Our experiments show that caspase-8 is an intermediatein a death pathway in T cells where both caspase processing andapoptosis are blocked by MEK1/2. Thus, inhibition of a Hid-likemolecule may be a conserved component of trophic factor-mediatedsurvival in Drosophila and mammaliancells.

ACKNOWLEDGEMENTS

We thank Gaiti Hasan, M. K. Mathew, and K. VijayRaghavan for comments on the manuscript. We are grateful to Xavier Saelens,Wilma Burm, and Ann Meeus at DMB, RUG. We acknowledge travel assistancefrom the Sarojini Damodaran International Fellowship, TIFR, India;Wood Whelan IUBMB; and Company of Biologists UK and BoehringerIngelheim, Germany (to J. V.).

	FOOTNOTES

^* This study was funded by a core grant from NCBS, TIFR (to A. S.).The costs of publication of this article were defrayed inpart by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

^¶ To whom correspondence should be addressed. Tel.: 91-80-3636420; Fax: 91-80-3636662; E-mail: sarina@ncbs.res.in.

Published, JBC Papers in Press, July 16, 2002, DOI 10.1074/jbc.M206445200

ABBREVIATIONS

The abbreviations used are: FADD, Fas-associated death domain; Hid, Head involution defective; Erk, extracellular signal-regulated kinase; pErk, phosphorylated Erk; MAPK, mitogen-activated protein kinase; MEK, MAPK/Erk kinase; CA-MEK, constitutively active MEK; DN-MEK, dominant negative MEK; TNFR, tumor necrosis factor receptor; IAP, inhibitor of apoptosis protein; IL, interleukin; FMK, fluoromethyl ketone; zVAD-FMK, z-Val-Ala-Asp (O-methyl)-fluoromethyl ketone; IETD-FMK, Ile-Glu-Thr-Asp-FMK; LEHD-FMK, Leu-Glu-His-Asp-FMK; PMA, phorbol 12-myristate 13-acetate; GFP, green fluorescent protein; EGFP, enhanced GFP; MBP, maltose-binding protein; FL, full length; Smac, second mitochondrial activator of caspases; DIABLO, direct IAP-binding protein with low pI; c, cytoplasmic.

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