A Novel Form of DAP5 Protein Accumulates in Apoptotic Cells as a Result of Caspase Cleavage and Internal Ribosome Entry Site-Mediated Translation

doi:10.1128/MCB.20.2.496-506.2000

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Molecular and Cellular Biology, January 2000, p. 496-506, Vol. 20, No. 2
0270-7306/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

A Novel Form of DAP5 Protein Accumulates in Apoptotic Cells as a Result of Caspase Cleavage and Internal Ribosome Entry Site-Mediated Translation

Sivan Henis-Korenblit, Naomi Levy Strumpf, Dan Goldstaub, and Adi Kimchi^*

Department of Molecular Genetics, Weizmann Institute of Science, Rehovot 76100, Israel

Received 1 June 1999/Returned for modification 27 July 1999/Accepted 19 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Death-associated protein 5 (DAP5) (also named p97 and NAT1) is a member of the translation initiation factor 4G (eIF4G) familythat lacks the eIF4E binding site. It was previously implicatedin apoptosis, based on the finding that a dominant negative fragmentof the protein protected against cell death. Here we address itsfunction and two distinct levels of regulation during apoptosisthat affect the protein both at translational and posttranslationallevels. DAP5 protein was found to be cleaved at a single caspasecleavage site at position 790, in response to activated Fas orp53, yielding a C-terminal truncated protein of 86 kDa that iscapable of generating complexes with eIF4A and eIF3. Interestingly,while the overall translation rate in apoptotic cells was reducedby 60 to 70%, in accordance with the simultaneous degradationof the two major mediators of cap-dependent translation, eIF4GIand eIF4GII, the translation rate of DAP5 protein was selectivelymaintained. An internal ribosome entry site (IRES) element capableof directing the translation of a reporter gene when subclonedinto a bicistronic vector was identified in the 5' untranslatedregion of DAP5 mRNA. While cap-dependent translation from thistransfected vector was reduced during Fas-induced apoptosis, thetranslation via the DAP5 IRES was selectively maintained. Additionof recombinant DAP5/p97 or DAP5/p86 to cell-free systems enhancedpreferentially the translation through the DAP5 IRES, whereasneutralization of the endogenous DAP5 in reticulocyte lysatesby adding a dominant negative DAP5 fragment interfered with thistranslation. The DAP5/p86 apoptotic form was more potent thanDAP5/p97 in these functional assays. Altogether, the data suggestthat DAP5 is a caspase-activated translation factor which mediatescap-independent translation at least from its own IRES, thus generatinga positive feedback loop responsible for the continuous translationof DAP5 duringapoptosis.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Programmed cell death (PCD) is a fundamental cellular process that provides an intrinsic self-elimination mechanism for theremoval of unwanted cells in a wide variety of biological systems.PCD is critical for organ development, tissue remodeling, cellularhomeostasis, and elimination of abnormal and damaged cells. However,improper execution of PCD can be quite hazardous and is associatedwith pathologies including AIDS, neurodegenerative disorders,autoimmune diseases, and others. Altogether, the execution ofapoptosis must be tightly regulated. This is achieved by a stringentrequirement for an apoptotic trigger on the one hand and protectionfrom inappropriate activation of the cell death program in cellsintended to survive on the other hand. The latter mechanism isespecially important given that ample proapoptotic proteins arepresent in normally growing cells, regardless of the presenceof an apoptotictrigger.

Death-associated protein 5 (DAP5) (also named p97 and NAT1), a 97-kDa protein homologous to eukaryotic translation initiationfactor 4GI (eIF4GI), was isolated independently by several groups(15, 21, 33, 40). In our laboratory, it was rescued asa positive mediator of PCD through a functional approach to genecloning, which is based on transfections of expression cDNA librariesand selection of cells resistant to apoptosis (10, 21). Adeath-protective DAP5 cDNA fragment coding for a dominant negativeminiprotein was rescued by this method, providing the basis forthe isolation of the full-length cDNA. In parallel, Imataka etal. cloned DAP5/p97 in an effort to identify novel genes belongingto the eIF4G family (15). Shaughnessy et al. cloned the mouseDAP5 gene based on its physical linkage to a common retroviralintegration site found in myeloid leukemia of BXH2 mice (33).They mapped human DAP5 within a cluster of genes on human chromosome11p15, which harbors several unidentified tumor suppressor genes.Finally, Yamanaka et al. identified DAP5/NAT1 as a novel targetfor RNA editing in transgenic mice overexpressing Apobec-1, thecatalytic subunit of the editosome complex. In these mice DAP5/NAT1mRNA was extensively edited, creating multiple stop codons (40).Interestingly, transgenic mice and rabbits overexpressing Apobec-1developed liver dysplasia and hepatocellular carcinoma, linkingoncogenesis with the aberrant hyperediting of target mRNAs. Theidentification of DAP5 mRNA as a principal editing target in thesemice further suggests that DAP5 may be coupled to cell growthcontrol.

Two eIF4G family members, eIF4GI and eIF4GII, serve as a scaffold for the coordinated assembly of the translation initiationcomplex, leading to the attachment of the template mRNA to thetranslation machinery at the ribosome, usually through the 5'cap structure (12, 26). Interestingly, the homology betweenDAP5 and eIF4GI/GII spans over the central part of the latterproteins, which is responsible for eIF3 and eIF4A binding. Incontrast, the N-terminal part of eIF4GI/GII, which binds to thecap binding protein eIF4E, is completely missing from DAP5 protein.Consistent with these structural predictions, it was shown bya few strategies that DAP5/p97/NAT1 binds eIF3 and eIF4A and failsto bind eIF4E, which is essential for mediating cap-dependenttranslation (15, 16, 40). In this respect, DAP5 resemblesthe cleaved version of eIF4GI/GII, devoid of its N terminus, whichresults from infections by several members of the picornavirusfamily. These cleaved C-terminal fragments of eIF4GI/GII failto mediate cap-dependent translation (5, 13, 20, 35)but promote cap-independent translation via internal ribosomeentry sites (IRES) (5, 20, 29, 30). Despite this structuralresemblance, it has been reported that high levels of ectopicallyexpressed DAP5/p97/NAT1 inhibited both cap-dependent and cap-independenttranslation (from viral IRESes), suggesting that it may functionas a general negative regulator of translation (15, 16, 40).The identification of DAP5 as a translation regulator on the onehand and the rescue of the gene as a mediator of apoptosis onthe other hand suggest that further studies of this gene shouldhighlight novel mechanisms linking translational control to restrictionof cellular outgrowth by PCD (21).

While DAP5 was reported to be ubiquitously and abundantly expressed in normal tissues and growing cell lines (15, 21,33, 40), the question of its possible regulation during apoptosishas not been investigated yet. In this work, we found that inresponse to different apoptotic triggers such as activation ofFas receptors or p53 induction, DAP5 was cleaved at a conservedcaspase cleavage site to generate a novel p86 form devoid of itsC terminus. The cleavage of DAP5 did not interfere with its abilityto interact with the translation factors eIF3 and eIF4A. Interestingly,this novel DAP5 form persisted in cells during the apoptotic processat levels comparable to those of the intact p97 form in growingcells. This stood in contrast to the eIF4GI cap-dependent translationfactor, the cleavage of which yielded low steady-state levelsof products compared to the intact protein in growing cells, thuschanging the internal balance within this family of translationfactors. Under these apoptotic conditions, total translationalactivity in the cells was reduced by 60 to 70% and the rate of $beta$ -tubulin synthesis was reduced by more than 85%, whereas DAP5protein itself continued to be selectively translated. We identifiedin the 5' untranslated region (5'UTR) of DAP5 mRNA an IRES elementwhich directed cap-independent translation when placed in a bicistronicvector and continued to function during Fas-induced apoptosis,suggesting that it may contribute to the maintained translationof the endogenous DAP5 protein during apoptosis. Finally we showhere for the first time that DAP5 IRES-directed translation inrabbit reticulocyte lysate (RRL) is DAP5 dependent and that thecleaved DAP5/p86 form is more potent than the full-length DAP5in its ability to enhance DAP5 IRES-mediated translation. Altogether,our results suggest that DAP5 is a caspase-activated translationfactor responsible at least for the mediation of its own translationduringapoptosis.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell cultures and induction of apoptosis. Human SKW B-lymphoma cells and the murine myeloid leukemic cell line LTR6/M1, carrying a temperature-sensitive p53 mutant,were grown in RPMI 1640 medium supplemented with 10% heat-inactivatedfetal calf serum, L-glutamine, penicillin (100 U/ml), and streptomycin(100 µg/ml). The 293 cells were grown as previously described(18). Apoptosis in SKW B-lymphoma cells was induced by additionof soluble protein A (5 µg/ml; Sigma) and anti-Fas agonistic antibodies(100 ng/ml). For the in vivo protease inhibition experiment, SKWB cells were preincubated with the cell-permeable inhibitors BD-Fmk(BD), Z-DEVD-CH₂F (DEVD), and Z-YVAD-Fmk (YVAD) (100 µM each;Enzyme Systems Products), GM132 (100 µM), and calpain inhibitorI/ALLN (150 µM; Boehringer) 1 h prior to the addition of anti-Fasantibodies to the cells. p53-induced apoptosis in LTR6/M1 cellswas achieved by a temperature shift to 32°C (41). The HeLa-Fas-Bujard(HFB) cells were generated by transfecting a HeLa cell clone (HtTA-1)that expresses a tetracycline-controlled transactivator with atetracycline-controlled expression vector carrying the Fas receptors(4). The HFB cell line was cultured in Dulbecco modified Eaglemedium supplemented with 10% fetal calf serum, L-glutamine, penicillin(100 U/ml), streptomycin (100 µg/ml), and hygromycin B (100 µg/ml;Calbiochem). Apoptosis was induced by addition of soluble proteinA (5 µg/ml; Sigma) and anti-Fas agonistic antibodies (100 ng/ml).

Cell death was assessed in SKW B cells and LTR6/M1 cells by using an ApoAlert annexin V-fluorescein isothiocyanate apoptosiskit (Clontech) according to the manufacturer's instructions. Detectionof the resulting signal was carried out by flow cytometry accordingto the manufacturer'sinstructions.

DNA constructs. Wild-type and mutant versions of DAP5 were expressed from pECE-Flag vector. pECE-DAP5/p97 was generated by subcloning DAP5SspI cDNA fragment in frame to the Flag tag in the SmaI site ofplasmid pECE-FLAG. pECE-DAP5/p86, pECE-DAP5/DETA, and pECE-DAP5/DHVAwere generated by creating point mutations in the pECE-DAP5/p97plasmid by using a QuikChange site-directed mutagenesis kit (Stratagene),using a set of primers encompassing the inserted pointmutations.

The basic luciferase (LUC)-secreted alkaline phosphatase (SeAP) bicistronic (LS) vector, used in this study for insertionof DAP5's 5'UTR element, was provided by QBI Enterprises (Nes-Ziona,Israel) (34). DAP5's 5'UTR (306 nucleotides) was obtained byPCR utilizing DAP5's EcoRI insert as the template with primersencompassing an XhoI restriction site at the 5' end (5' GGC GGGCTC GAG CAG CAG TGA GTC GGA GCT CTA TGG AGG TGG CAG CGG GTA) andan NcoI restriction site at the 3' end (5' GGA CTC CCA TGG TTGGCG CTT GAC AAC GAA GAA TCT TC). The 5'UTR was inserted betweenthe XhoI (5') and BsmBI (3') sites of the intercistronic regionof the bicistronic vector, allowing the hybrid NcoI-BsmBI siteto recreate the initiator ATG codon of SeAP, giving rise to theLS-DAP5 vector. LS-immunoglobulin heavy chain binding protein,based on the same basic LS bicistronic vector (34), was providedby Eli Keshet. LS-EMCV (encephalomyocarditis virus) was providedby QBI Enterprises (Nes-Ziona,Israel).

pcDNA3-CAT and pcDNA3-hpCAT (provided by Y. Groner, Weizmann Institute) contain CAT (chloramphenicol acetyl transferase)-ORF(open reading frame) and CAT-ORF preceded by a 30-nucleotide hairpin( $Delta$ G = $-$ 40 kcal/mol), respectively (1, 3, 37). The bicistronicvectors CAT-LUC-DAP5 and hp-CAT-LUC-DAP5 (CL-DAP5 and hpCL-DAP5,respectively) were generated by placing the DAP5 5'UTR conjugatedto LUC (originating from promoter plasmid PGL2 [Promega]) withinthe polylinker sequence, downstream of the CAT gene, at the BstXIrestrictionsites.

Cell lysates and immunoprecipitations. Cells were washed with phosphate-buffered saline and lysed in cold buffer B (100 mM KCl, 0.5 mM EDTA, 20 mM HEPES-KOH [pH7.6], 0.4% NP-40, 20% glycerol, aprotinin [4 µg/ml], pepstatin[5 µg/ml], leupeptin [5 µg/ml], and 1 mM phenylmethylsulfonylfluoride) unless indicated otherwise. For immunoprecipitationexperiments, 1 mg of protein extract was precleared by proteinA-Sepharose CL-4B beads (Pharmacia Biotech) or by protein G-PLUS-agarosebeads (Santa Cruz Biotechnology) for 30 min at room temperature.The precleared extracts were incubated with the beads and therelevant antibodies for 6 to 12 h at 4°C. Immunoprecipitates werewashed repeatedly with buffer B, eluted with Laemmli buffer, andresolved by polyacrylamide gel electrophoresis (PAGE) on a sodiumdodecyl sulfate (SDS)-7.5% polyacrylamide gel unless indicatedotherwise.

Antibodies. Anti-DAP5 rabbit polyclonal antibodies, generated against a fragment of DAP5 corresponding to amino acids 488 to 742 (21),were used at dilutions of 1:350 dilution for Western blottingand 1:50 for immunoprecipitations. Anti-DAP5 monoclonal antibodiesgenerated against a fragment of DAP5 corresponding to amino acids672 to 830 (Transduction Laboratories) were used for Western blottingat 1:500 dilution. The anti-eIF4A, anti-eIF3/p116, and anti-eIF4GIIantibodies (12, 15, 25) were kindly provided by N. Sonenberg.Polyclonal antibodies against bacterially produced N- and C-terminalfragments of eIF4GI expressed from pRSET (Invitrogen) (amino acids173 to 457 and 934 to 1390, respectively) were prepared in NewZealand White rabbits. Anti-poly (ADP-ribose) polymerase (PARP)polyclonal antibodies (BIOMOL) were used for immunoblotting at1:5,000 dilution. Anti- $beta$ -tubulin antibodies used for immunoprecipitationwere purchased from Sigma. Anti-Flag monoclonal antibodies coupledto agarose beads (M2 affinity gel; IBI/Kodak) were used for immunoprecipitationof Flag-taggedproteins.

Metabolic labeling of proteins. Exponentially growing SKW cells were incubated with methionine-depleted medium for 1 h and then labeled with 80 µCi of [³⁵S]Met per ml for an additional 1.5 h. For assessing total proteintranslation rate, SKW cells, either nontreated or pretreated for2 h with cycloheximide (CHX; 10 µg/ml; Sigma) or with anti-Fasagonistic antibodies, were starved and labeled as described aboveand harvested thereafter (treatment with CHX or with anti-Fascontinued during the methionine starvation and the radioactivepulse). Cytoplasmic extracts were prepared, applied to filterpaper (Whatman), and boiled in 10% trichloroacetic acid. The levelof acid-insoluble radioactivity per microgram of protein extractwas calculated. For comparison of DAP5 and $beta$ -tubulin translationrates, control and anti-Fas-treated extracts (1.5 × 10⁶ cpm of each) were subjected to immunoprecipitation by the correspondingantibodies. The intensity of the bands was determined with a BAS-2000phosphorimager (Fuji) or bydensitometry.

Enzymatic assays of reporter proteins. HFB or 293 cells were transiently transfected with bicistronic vectors by the standard calcium phosphate technique. LUC enzymeactivity in cell extracts was determined by using a commercialLUC assay system (Promega) as recommended by the supplier. Lightemission was quantified with a Lumac/3M BIOCOUNTER M2010 luminometer.The activity of excreted SeAP released into the growth mediumwas determined following inactivation of the endogenous SeAP byheating the medium to 65°C and clarifying it by centrifugation.Aliquots were diluted in SeAP buffer (1 M diethanolamine [pH 9.8;Sigma], 0.5 mM MgCl₂, 10 mM L-homoarginine [Sigma]) and 12 mMp-nitrophenyl phosphate substrate (Sigma). Following incubationat 37°C, the product concentration was determined by measuringabsorbency at 405 nm, within the linear range of theassay.

RNA analysis. Total cellular RNA was isolated by using Tri-Reagent (Molecular Center, Inc.) according to the manufacturer's instructions.Thirty-microgram samples of total cellular RNA were electrophoreticallyseparated on a 1% gel. The RNA was transferred onto a nylon membrane(Amersham) and covalently linked to the membrane by a UV cross-linker(Spectronics Corporation). Prehybridization was performed at 42°Cfor 4 h in hybridization solution (50% formamide, 5× SSC [1× SSCis 0.15 M NaCl plus 0.015 M sodium citrate], 4× Denhardt solution,0.1% sodium pyrophosphate, 100 µg of heat-denatured salmon spermDNA per ml). Hybridization was carried out overnight under thesame conditions and in the presence of 10⁶ cpm of [³²P]dCTP-labeled DNA probe. Washes were performed at 50°C in a 0.1%SDS-0.1% SSC-0.1% sodium pyrophosphate washing solution. The intensityof the bands was determined with a BAS-2000 phosphorimager(Fuji).

Translation in cell-free system. The pcDNA3-based CAT-LUC-DAP5 (CL-DAP5) and hp-CAT-LUC-DAP5 (hpCL-DAP5) vectors were linearized with NotI and used as templatesfor in vitro transcription from the T7 promoter with T7 RNA polymerase(Promega) for 2 h at 37°C. These RNA transcripts were then translatedin RRL (Promega) by conventional procedures, and the productswere resolved on a 10% polyacrylamide gel followed by salicylicacidamplification.

For studying the effects of DAP5 forms on translation in vitro, LS-DAP5 and LS-EMCV vectors were linearized with HpaI andserved as templates for synthesis of capped transcripts as describedabove, in the presence of m⁷GpppG (Biolabs) at a 10-fold molar excess over GTP. The recombinantproteins added to the translation reaction were prepared by thefollowing procedures: glutathione S-transferase (GST) and GST-260(see Results) were produced in bacteria and affinity purifiedon GST columns as described previously (21). DAP5/p97 and DAP5/p86recombinant proteins were immunoprecipitated via a Flag tag fromtransfected cells. To this end, 293 cells transfected with pECE,pECE-DAP5/p97, or pECE-DAP5/p86 were lysed in buffer B (withoutEDTA), immunoprecipitated with beads conjugated to anti-Flag antibodies(M2 affinity gel; IBI/Kodak) for 12 h, and then washed twice inlysis buffer and twice in Tris (pH 8) buffer. Each translationreaction mixture consisted of 17.5 µl of RRL (Promega), 0.5 µlof amino acid mixture minus Met (1 mM; Promega), 2.5 µl of [³⁵S]Met (10 µCi/µl), and 2 µl of RNA transcript. When indicated,4 µl GST or GST-260 protein (~0.3 µg) was added. Alternatively,the entire reaction mixture was added to the immunoprecipitatesand incubated at 30°C for 90 min with continuous stirring. Thereaction was terminated by boiling in Laemmli buffer. Half ofthe reaction mixture was resolved by SDS-PAGE (10%) gel, dried,and analyzed for band intensities with a BAS-2000 phosphorimager(Fuji). The other half was subjected to Western analysis anddensitometry.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Induction of a novel form of DAP5 protein during PCD. In a search for possible posttranslational regulatory events which may modify the DAP5 protein, several cell lines were inducedto undergo apoptosis by different types of stimuli. The fate ofDAP5, a 97-kDa protein, was monitored by Western blotting withpolyclonal antibodies raised against a fragment of the proteinthat shows low homology to eIF4G (amino acids 488 to 742; seeFig. 8). The choice of this specific fragment indeed yielded antibodieswhich did not cross-react with eIF4G proteins (notshown).

SKW B-lymphoma cells respond to anti-Fas agonistic antibodies in a well-synchronized execution of the cell death program.As early as 5 h after treatment with the anti-Fas antibodies,approximately 70% of the SKW cells exhibit an altered plasma membranecomposition, as assessed by flow cytometry analysis with annexinV conjugated to fluorescein isothiocyanate (Fig. 1A). The kineticsof cell death was followed at the level of caspase activationas well. Detection of the caspase cleavage product of PARP wasused as a marker for caspase activity. As early as 2 h after activationof the Fas receptors, no intact 112-kDa PARP could be detected,as it was all converted into its cleaved product. This demonstratesboth the rapid kinetics of the execution of apoptosis and thesynchronized response of SKW cells to Fas activation, making itan ideal system for studying different cell death-associated events.In growing cells, DAP5 appeared as a 97-kDa protein which couldbe resolved into two bands, depending on the gel fractionationand resolution: a major DAP5 band and a rapidly migrating minorband just beneath, as reported earlier (15). These bands probablyreflect some posttranslational modifications of DAP5 protein (Fig.1A). After Fas stimulation, DAP5 protein displayed a typical patternof alterations. The level of DAP5/p97 decreased considerably asthe apoptotic program progressed, and an 86-kDa protein, recognizedby the same anti DAP5 polyclonal antibodies, appeared instead(Fig. 1A). These DAP5 protein alterations could be detected asearly as 2 h after activation of the Fas receptors. Again, a minorrapidly migrating band was detected below the major 86-kDa proteinas well (Fig. 1A).

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FIG. 1. A novel DAP5/p86 form appears in Fas- and p53-induced apoptosis. (A) Exponentially growing SKW B-lymphoma cells (3 × 10⁶, total cell number) were treated with agonistic anti-Fas antibodies for 0, 2, 5, and 8 h. Treatment was terminated by harvesting all cells and immediately boiling the pellets in Laemmli sample buffer. Immunoblots were reacted with anti-DAP5 polyclonal antibodies (top) and anti-PARP antibodies (bottom). Apoptotic cell death was assessed by detection of changes in the membrane composition by the annexin V fluorescence-activated cell sorting analysis. (B) HFB cells were exposed to anti-Fas agonistic antibodies, for the indicated time periods, in the presence or absence of CHX. The fate of DAP5 was followed by reacting the immunoblots with anti-DAP5 polyclonal antibodies. (C) LTR6/M1 cells, expressing a temperature-sensitive p53 mutant, were induced to undergo apoptosis by a temperature shift to 32°C. Apoptotic cell death was assessed by detection of changes in the membrane composition by annexin V fluorescence-activated cell sorting analysis. The fate of DAP5 was assessed by Western blotting. The sizes of protein markers (in kilodaltons) are shown on the right. The positions of DAP5/p97 and DAP5/p86 are marked by arrows (dashed arrows point to the minor rapidly migrating p97 and p86 bands). The asterisk marks a nonspecific band lightened by the anti-DAP5 antibodies.

The reduction in the level of DAP5/p97 and the concomitant appearance of an 86-kDa protein as apoptosis execution progressedwere not confined to a certain cell line or apoptotic trigger.Treatment of HFB cells with anti-Fas agonistic antibodies (Fig.1B) and activation by temperature shift of a temperature-sensitivep53 mutant expressed in LTR6/M1 cell line (Fig. 1C) resulted inthe same alterations of DAP5 protein. However, the extent andtime kinetics of these alterations differed from those for theFas-activated SKW cells, in accordance with the slower kineticsand decreased synchrony of these systems (Fig. 1C).

To confirm that the novel 86-kDa protein appearing during apoptosis is a derivative of DAP5, we attempted to detect it viaalternative, nonoverlapping antibodies. Recombinant N-terminallyFlag-tagged DAP5 was transfected into HFB cells, and its fateupon death induction was assessed by immunoprecipitation withanti-Flag antibodies. In the normally growing transfectants, onlya single tagged protein, approximately 97 kDa in size, was detected,whereas two Flag-tagged proteins of 97 and 86 kDa were recoveredupon Fas treatment (Fig. 2C, lanes 3 and 4). The ability of twodifferent epitopes to detect the same novel protein strongly suggeststhat the 86-kDa protein that appears during cell death is a novelDAP5 form which we have accordingly named DAP5/p86.

DAP5/p97 is converted to DAP5/p86 by proteolytic cleavage at the C terminus. Next, we set out to understand the mechanism underlying the induction of DAP5/p86. Its induction even in the presence of theprotein synthesis inhibitor CHX proved that the appearance ofDAP5/p86 did not depend on de novo protein synthesis. As shownin Fig. 1B, the DAP5/p86 form was readily detected in HeLa cellsstimulated by agonistic anti-Fas antibodies in the presence ofCHX. Pulse-chase experiments performed with nontreated and Fas-stimulatedSKW cells determined that the half-life of DAP5 protein in growingcells is longer than 5 h and further demonstrated that DAP5/p86was derived from preexisting labeled DAP5/p97 (notshown).

Wide varieties of posttranslational modifications may affect the migration pattern of a protein on polyacrylamide gels; suchmodifications include phosphorylation, acetylation, glycosylation,and proteolysis. Since the observed decrease in DAP5's molecularweight was of a relatively great magnitude, and since proteasesare well-established regulators and executioners of PCD, we furtherexplored the issue of proteolysis. Because the N-terminal Flagwas readily detected by the anti-Flag antibodies in the DAP5/p86form (Fig. 2C, lanes 4 and 8), the possibility of N-terminal truncationswas excluded. To test the possibility that DAP5/p97 is convertedto DAP5/p86 by cleavage at its C terminus, monoclonal antibodiesdirected against DAP5's C-terminal portion (amino acids 672 to830; see Fig. 8) were used to monitor DAP5 in control and Fas-stimulatedSKW cell lysates. The monoclonal antibodies failed to recognizeDAP5/p86 in the treated cultures and instead reacted mainly witha protein fragment of approximately 10 kDa (Fig. 2A). These resultsare consistent with the possibility of a proteolytic cleavageoccurring during cell death at the C terminus of DAP5.

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FIG. 2. DAP5/p97 is converted to DAP5/p86 by caspase cleavage. (A) SKW B-lymphoma cells were treated with anti-Fas agonistic antibodies for 5 h. Samples were fractionated on a 10% or 15% polyacrylamide gel, and DAP5 was assessed by reacting the Western blot (WB) with anti-DAP5 polyclonal or monoclonal antibodies ( $alpha$ DAP5 Abs), as indicated (see Fig. 8 for antibody epitopes). A nonspecific band is marked by an asterisk. (B) SKW B-lymphoma cells were treated with agonistic anti-Fas antibodies for 5 h after a 1-h preincubation period with caspase inhibitors (BD, DEVD, and YVAD), proteosome inhibitor (MG132), and calpain I inhibitor (ALLN). As a control, cells were preincubated with dimethyl sulfate solvent alone. Immunoblots were reacted with anti-DAP5 polyclonal antibodies (top) and anti-PARP antibodies (bottom). (C) HFB cells were transiently transfected with the following N-terminal Flag-tagged DAP5 constructs: wild-type DAP5 (DAP5/p97 [lanes 3 and 4]) and two constructs each carrying a potential disrupted caspase cleavage site (DAP5/p97 DETA⁷⁹⁰ [lanes 5 and 6]; DAP5/p97 DHVA⁸²⁴ [lanes 7 and 8]). An empty pECE vector served as a control (lanes 1 and 2); 24 h posttransfection the cells were exposed to anti-Fas agonistic antibodies for 12 h or to fresh medium alone. The exogenic DAP5 forms were pulled down by immunoprecipitation with anti-Flag antibodies followed by Western blotting with anti-DAP5 polyclonal antibodies.

DAP5/p97 is cleaved at a conserved caspase cleavage site at position 790. To assess the contribution of different cellular proteases to the cleavage of DAP5/p97, SKW cells were stimulated with agonisticanti-Fas antibodies in the presence or absence of a panel of proteaseinhibitors: a proteosome inhibitor (MG132), a calpain I inhibitor(ALLN), and caspase inhibitors (BD, YVAD, and DEVD) (Fig. 2B).Proteosome and calpain I inhibitors did not abrogate the appearanceof DAP5/p86 at the expense of DAP5/p97. In contrast, caspase inhibitorsprevented the cleavage of DAP5. The ability of the various proteaseinhibitors to prevent DAP5's cleavage correlated with their abilityto abrogate PARPcleavage.

The caspase inhibitors could exert their effects on DAP5 either directly, by blocking a specific caspase responsible for DAP5/p97cleavage, or indirectly, by interfering with early caspase-dependentevents operating upstream to DAP5's conversion. Examination ofthe amino acid sequence of DAP5 protein revealed the existenceof four potential caspase cleavage sites of the motif DXXD (aminoacid 185, 592, 790, 824), yet only two of these sites (DETD⁷⁹⁰ and DHVD⁸²⁴) seemed capable of yielding a cleavage product of the expectedmolecular weight. To examine directly whether these sites arerequired for the cleavage of DAP5, we constructed two Flag-taggedDAP5/p97 mutants carrying individual Asp-to-Ala mutations in thesepotential sites (DXXD $right-arrow$ DXXA). We followed the ability of each mutationto abolish the appearance of exogenous DAP5/p86 in Fas-stimulatedHFB cells (Fig. 2C). While the p86 form was detected upon transfectionwith wild-type Flag-DAP5/p97 (lanes 3 and 4) and Flag-DAP5/DHVA⁸²⁴ (lanes 7 and 8), transfection with the DAP5/DETA⁷⁹⁰ construct failed completely to yield the DAP5/p86 form (lanes5 and 6). This indicates that DAP5/p97 is converted to DAP5/p86directly by caspase cleavage and maps the exact cleavage to theDETD⁷⁹⁰site.

Caspases are known to alter the function of their protein substrates by causing their activation or inactivation or othertypes of functional modulations (28, 31). We first testedwhether the cleavage of DAP5 influenced the binding to translationinitiation factors eIF3 and eIF4A. In one line of experiments,endogenous DAP5 was immunoprecipitated with anti-DAP5 polyclonalantibodies from growing or Fas-stimulated SKW cells, and the levelsof coimmunoprecipitated eIF4A were subsequently monitored (Fig.3A). We found that both DAP5/p97 (exclusively appearing in nontreatedgrowing cells) and DAP5/p86 (exclusively appearing in treatedcultures at the 5-h point) pulled down very efficiently the endogenouseIF4A. This line of experiments indicated that DAP5/p86 retainedits binding capacity to eIF4A and that these complexes exist incells during apoptosis. In a second line of experiments, we comparedeIF3 binding to ectopically expressed p97 and p86 DAP5 forms.The recombinant DAP5/p97 or DAP5/p86 proteins were transientlyexpressed in 293 cells and immunoprecipitated with anti-Flag antibodies;the levels of the eIF3/p116 subunit in the complex were assessed.Similar to the full-length protein, the truncated p86 form alsopulled down the eIF3 protein (Fig. 3B). Hence, the cleavage ofDAP5 does not seem to affect its overall ability to bind thesecritical translation initiation factors.

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FIG. 3. Coimmunoprecipitation of eIF4A and eIF3 with the two DAP5 forms. (A) Growing SKW cells or SKW cells exposed for 2 or 5 h to anti-Fas agonistic antibodies were gently extracted in B buffer. Protein extract (1 mg) was subjected to immunoprecipitation with anti-DAP5 polyclonal antibodies. Coimmunoprecipitation of endogenous eIF4A was assessed by Western blotting the immunoprecipitates with anti-eIF4A antibodies (middle panel). Samples of 100 µg of total cell extracts were assessed for DAP5 and eIF4A levels by direct Western blotting (top and bottom panels, respectively). (B) 293 cells were transiently transfected with Flag-tagged DAP5 constructs in a pECE vector. The constructs included wild-type DAP5 (DAP5/p97), a mutant of DAP5 carrying a stop codon at position 790 (DAP5/p86), and an empty vector (pECE). At 48 h posttransfection the cells were extracted gently in B buffer. The ectopically expressed DAP5 was immunoprecipitated with anti-Flag antibodies and assessed with anti-DAP5 antibodies after resolution of the immunoprecipitates on gels (top); coimmunoprecipitation of endogenous eIF3 was assessed by Western blotting the immunoprecipitates with antibodies against the eIF3/p116 subunit (middle); total endogenous eIF3/p116 was measured by direct Western blotting (bottom).

DAP5 is preferentially translated in apoptotic cells, in the absence of intact eIF4G proteins. The finding that DAP5 is cleaved during cell death into a novel protein form prompted us to study the fate of the other eIF4Gfamily members during apoptosis. The fate of eIF4GI and eIF4GII,the two main mediators of cap-dependent translation, was assessedin both HFB and SKW cells stimulated by Fas agonistic antibodies.Intact eIF4GI could not be detected at all by polyclonal antibodiesraised against its C or N terminus as early as 2 h following treatment(Fig. 4A shows data for SKW cells; similar results were obtainedin HFB cells). A more detailed analysis revealed that eIF4GI hadalready disappeared at 1 h after treatment of SKW cells with anti-Fasagonistic antibodies (not shown). Low levels of truncated eIF4GIforms, about 110-kDa in size (Fig. 4A, left panel) were detectedin apoptotic cells with the N-terminal antibodies (an averagedrop of at least 80% compared to the levels of the intact proteinin growing cells, as assessed by densitometry). The C-terminalantibodies could also detect very small amounts of proteins of40, 50, and 76 kDa in treated cells (Fig. 4A, two right panels).Again, the amounts of the cleaved proteins detected by the anti-eIF4GIantibodies in the treated cells were in the range of 5 to 20%of intact protein levels in control cells. The disappearance ofintact eIF4G and the detection of cleaved products is consistentwith previous work which showed caspase-mediated cleavage of eIF4GIin different cell systems and in response to various apoptotictriggers (6, 7, 22, 27). Similarly, the eIF4GII proteindid not remain in its intact form as well, as assessed by immunoblotanalysis of extracts from Fas-induced SKW cells with polyclonalantibodies raised against the N-terminus fragment of the protein(not shown). Thus, the steady-state levels of these two importantfamily members, which are critical for cap-dependent translation,were markedly reduced in the apoptotic cells.

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FIG. 4. Disappearance of intact eIF4GI during cell death. (A) SKW B-lymphoma cells were treated with anti-Fas agonistic antibodies for 0, 2, and 5 h. The fate of eIF4GI was assessed by Western blotting (WB) with polyclonal antibodies generated against eIF4GI N terminus (left panel) or C terminus (two right panels). The position of full-length eIF4GI is indicated by an arrow. Bands exclusively recognized by either anti-eIF4G antibody in the Fas-treated cells are marked by their approximated molecular sizes (in kilodaltons) (p110, p76, p50, and p40). The asterisks mark nonspecific bands lightened by the anti-eIF4GI antibodies. (B) SKW B-lymphoma cells, either nontreated or pretreated for 2 h with CHX or with anti-Fas agonistic antibodies, were incubated in methionine-free medium for 1 h, labeled with [³⁵S]Met for 1.5 h, and harvested thereafter (the treatment with CHX or with anti-Fas continued during the methionine starvation and the radioactive pulse). The level of insoluble radioactivity incorporated per microgram of protein extract was set as 100% in control cells. The results represent the average of four independent experiments.

The well-established fact that cleavage of eIF4GI and eIF4GII during some viral infections leads to a shutdown in cap-dependentcellular translation (13, 20, 35), together with the observationthat the apoptotic cells undergo depletion of these key proteins,prompted us to study whether the degradation of these proteinsduring apoptosis is also correlated with translation shutdown.The overall rate of protein synthesis in SKW cells was measuredby incorporation of [³⁵S]methionine into acid-insoluble material. Both control and Fas-pretreatedcells were labeled. Fas-treated cells showed a reduced translationrate in the range of 30 to 40% of the control rate (Fig. 4B).Pretreatment with the translation elongation inhibitor CHX, whichserved as a reference for complete translational shutdown, resultedin a 1 to 10% translation rate compared to control cells. Thisfinding implies that during apoptosis, some translational eventsstilloccur.

Since overall translation did not cease completely, it was interesting to explore whether the translation of some specificproteins could preferentially continue under these conditions.Being a positive mediator of cell death, DAP5 by itself couldbelong to this putative group of proteins that continue to besynthesized under this kind of apoptotic stress on translation.Therefore, we compared changes in the translation rate of DAP5between control and FAS-stimulated SKW cells versus the changein the translation rate of another arbitrarily chosen protein, $beta$ -tubulin. Translation rate was determined by metabolically labelingnaive or 3-h-Fas-treated cells with [³⁵S]Met for a 1.5-h pulse (a point where intact eIF4GI and eIF4GIIwere already below detection levels). The labeled cells were lysed,and equal amounts (counts per minute) were immunoprecipitatedby the corresponding antibodies. Interestingly, DAP5's synthesisrate was only marginally affected in the apoptotic cells (7% reduction),whereas $beta$ -tubulin was reduced by 88% (Fig. 5). Northern blot analysisof DAP5 and $beta$ -tubulin RNAs was performed to normalize the translationvalues. The results clearly showed that the differences in theprotein's synthesis rate took place at the translation level,as the levels of both RNA species dropped to the same extent uponFas activation (not shown).

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FIG. 5. Preferential translation of DAP5 during cell death. SKW cells were treated for 3 h with anti-Fas agonistic antibodies (Abs) or were left untreated. During the last hour, cells were transferred to methionine-depleted medium supplemented with their corresponding treatments; they were then pulse-labeled with 80 µCi [³⁵S]Met per ml for 1.5 h and harvested. Samples of cytoplasmic extracts containing 1.5 × 10⁶ cpm were subjected to immunoprecipitation with anti-DAP5 polyclonal antibodies (top) and with anti- $beta$ -tubulin antibodies (bottom). The first lane in each panel represents nonspecific background bound to the Sepharose beads. The asterisks mark protein bands that reacted with the beads or the antibodies nonspecifically. Values from the densitometric analysis of the DAP5 and $beta$ -tubulin bands are shown at the right. The translation rate of each protein in the growing cells was set as 100%, and the translation rate of each protein following Fas treatment was calculated accordingly. Similar results were obtained in three additional independent experiments.

An IRES element in DAP5's 5'UTR is activated in apoptotic cells. One possible explanation for the continuous residual translation during cell death, in the absence of detectable intact eIF4GI/GII,is that mechanisms of cap-independent translation may be preferentiallyutilized. Along this line, we wondered whether DAP5's preferredtranslation rate during apoptosis could be mediated by an IRESelement in its 5'UTR. The 5'UTR of DAP5 mRNA possesses some characteristicsof IRES elements, as it is relatively long (about 300 bp) andencompasses two polypyrimidine-rich tracts (21). The abilityof this element to function as an IRES, which directs internaltranslation initiation, was examined. A stretch of 306 bp fromthe 5'UTR of DAP5 was inserted between the two cistrons of a bicistronicvector in which the first cistron encodes LUC and the second cistronencodes SeAP. The first cistron is proximal to the mRNA's capstructure and therefore is expected to be translated by the conventionalcap-dependent translation mode. The second cistron is distal fromthe cap site and is separated from the first cistron by multiplestop codons to decrease leaky translation; therefore it is expectedto undergo translation only upon insertion of an IRES elementbetween the twocistrons.

The bicistronic vectors were transiently expressed in 293 or HFB cells, and the resulting SeAP/LUC ratio was determined. Avector lacking an IRES insertion (termed an LS vector) was usedas well to estimate the background levels of SeAP. Insertion ofDAP5's 5'UTR between the two cistrons (LS-DAP5 vector) enhancedthe SeAP/LUC ratio approximately 11-fold both in 293 and HFB cellsrelative to the LS vector (Fig. 6A; see figure legends for rawdata). This value was two- to threefold higher than that for anotherwell-established cellular IRES, BiP, which was examined in parallel.We excluded the presence of a cryptic promoter within the DAP55'UTR insert by confirming the existence of a single bicistronicRNA message by Northern blotting (Fig. 6A, inset). To verify thatthe translation of the second cistron does not result from leakytranslation continuing from the first cistron, we switched toa CAT-LUC bicistronic system and interfered with the translationof the first cistron (CAT) by insertion of a stable hairpin atits 5' end. The effect of the hairpin insertion on the translationof both cistrons was examined by in vitro translation in an RRL.We found that the hairpin insertion led to a strong reductionin the translation of the first cistron (CAT), while the translationfrom the second cistron (LUC) was significantly less affected(Fig. 6C; eight independent translation experiments yielded averagereductions in translation of 70 and 16% from the first and secondcistrons, respectively, indicating that the major portion of thetranslation events from the second cistron were not a consequenceof translation initiated at the first cistron).

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FIG. 6. DAP5's 5'UTR possesses an IRES which directs cap-independent translation and is selectively sustained during cell death. (A) 5'UTRs of DAP5 and of BiP were inserted between the two cistrons of a basic bicistronic LS vector, in which the LUC reporter gene is translated in a cap-dependent manner from the first cistron and SeAP is translated in a cap-independent manner from the second cistron, to generate LS-DAP5 and LS-BiP respectively. 293 or HFB cells were transfected with a vector lacking an insert in the intercistronic region (LS), LS-DAP5, or LS-BiP and further assessed 48 h posttransfection. For each experiment, the SeAP/LUC ratio obtained by the LS vector was designated 1, and the relative fold increase in SeAP/LUC ratio in the other vectors was calculated. The results represent the average of three independent experiments. In 293 cells, the average values (in arbitrary units) of the reporter activities for LS, LS-BiP, and LS-DAP5 vectors, respectively, were 995, 784, and 1,167 for LUC and 14, 56, and 189 for SeAP. In HFB cells, the average values (in arbitrary units) of the reporter activities for LS and LS-DAP5 vectors, respectively, were (98 and 85) for LUC and (27 and 286) for SeAP. The inserts correspond to Northern blots of nontransfected (left lane of each) and LS-DAP5 transfected (right lane of each) 293 or HFB cells, respectively, probed by the SeAP cDNA. (B) HFB cells were transfected with LS-DAP5 vector. After 36 h, the medium was replaced by medium containing or lacking anti-Fas agonistic antibodies; 12 h later, the enzymatic activity of each reporter enzyme was determined. For each experiment, the SeAP or LUC value obtained for the control cells was designated 1 and served for normalization of the corresponding reporter activity under Fas-stimulated conditions. These results represent the average of seven independent experiments. The raw data from control and Fas-treated cells, respectively, were 197 and 63, 124 and 24, 767 and 246, 192 and 70, 133 and 35, 606 and 253, and 1290 and 229 for LUC and 138 and 135, 111 and 85, 178 and 148, 147 and 119, 296 and 227, 112 and 105, and 383 and 281 for SeAP. (C) DAP5's 5'UTR was inserted into a bicistronic vector in which CAT is translated from the first cistron and LUC is translated from the second cistron, generating CL-DAP5. Insertion of DAP5's 5'UTR into a bicistronic vector in which CAT, the first cistron, is preceded by a stable hairpin generated hpCL-DAP5. These constructs were transcribed and translated in vitro in the presence of [³⁵S]methionine. The intensity of each band was determined by phosphorimager analysis.

Next, the function of the DAP5 IRES under apoptotic conditions was examined. To this end, the LS and LS-DAP5 bicistronic vectorswere transiently expressed in HFB cells, and the effects of anti-Fasagonistic antibodies on SeAP and LUC expression levels were examinedby comparing their values to that for control, nontreated cells(Fig. 6B; see the legend for raw data). It was found that as aresult of Fas treatment, the extent of DAP5 IRES-mediated translationwas not significantly changed and was maintained at approximately90% of the control rate (n = 14) whereas that of cap-dependenttranslation was severely impaired, as it dropped to 30% of thecontrol rate (n = 14, P < 0.05). As a consequence, the SeAP/LUCratio of the LS-DAP5 vector was enhanced almost threefold underapoptotic conditions. In transfections with the LS vector, whichlacks a functional IRES element, the SeAP/LUC ratio remained unaltered(not shown). Interestingly, these results matched the data onthe preferential in vivo labeling of the endogenous DAP5 proteinduring cell death (Fig. 5), suggesting that the maintained translationof DAP5 under apoptotic conditions is at least partially attributedto an IRES element in its 5'UTR.

DAP5 protein mediates DAP5-IRES-driven translation. Translation via the DAP5 IRES is preferentially maintained during cell death despite the absence of detectable intact eIF4GI/GII.Under these apoptotic circumstances, DAP5 protein seemed to bethe most dominant among the different members of the eIF4G family.It therefore became of interest to test whether DAP5 protein mightmediate its own translation in a cap-independent manner. We showedin Fig. 6C that insertion of the DAP5 IRES in a bicistronic vectorenables translation of the second cistron in an RRL. Is thereDAP5 in the RRL that might contribute to this process? Westernanalysis of RRL revealed that indeed DAP5 is present in the lysate(Fig. 7A, left panel). To test whether DAP5 IRES-driven translationmay be mediated by DAP5 present in the RRL, we attempted to counteractits activity by introducing into the translation reaction a dominantnegative fragment of DAP5 (named fragment 260 or DAP5 miniprotein[21]). To this end, we chose to introduce into the translationreaction a bacterially produced GST-fused DAP5 miniprotein (GST-260)purified as previously described (21). The recombinant proteinwas added to the RRL in excess as shown in Fig. 7A (left panel).Its effect on the translation of both cistrons of the LS-DAP5bicistronic transcript was measured by comparing the results tothe pattern obtained with GST alone (Fig. 7A, right panel). Wefound that addition of DAP5 miniprotein to RRL significantly interferedwith the translation of the second cistron mediated through theDAP5 IRES, causing an average drop to 32% of the translation ratesobtained with the GST control reactions (n = 5, P < 0.05). Onthe other hand, the cap-dependent translation of the first cistronwas not significantly affected by the presence of DAP5 miniprotein,as its average value was 93% of its original value (n = 5, P >0.05). The reduction in the cap-independent translation via theDAP5 IRES and the sustained level of cap-dependent translation,in the presence of the dominant negative DAP5 form, lowered significantlythe overall ratio of cap-independent versus cap-dependent translationfrom the LS-DAP5 vector. Interestingly, when the same procedurewas carried out with an LS-EMCV vector, the addition of GST-260miniprotein to the RRL did not alter the ratio between the twocistrons (not shown), suggesting that the EMCV IRES is not influencedby the miniprotein as is the DAP5 IRES.

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FIG. 7. Translation via the DAP5 IRES in vitro is mediated by DAP5 protein. Capped transcripts of the bicistronic vectors LS-DAP5 or LS-EMCV were translated in vitro in the presence of [³⁵S]methionine. The translation reactions were supplemented with bacterially produced GST-260, using GST supplement as a control (A), or with Flag-DAP5/p97 or Flag-DAP5/p86 immunoprecipitated from transiently transfected 293 cells, using immunoprecipitates from nontransfected 293 cells a control (B and C). Intensities of the LUC and SeAP bands were quantified with a phosphorimager. The SeAP/LUC ratio in the control reaction was set as 1, and that of the DAP5-supplemented reactions was calculated accordingly. (A) LS-DAP5 transcripts were translated as described above, supplemented by equivalent amounts of GST-260 or GST proteins. A typical autoradiogram of the resulting translation products is presented (right). Corresponding amounts of RRL and GST-260, as present in the translation reactions, were separated on a 12% gel and immunoblotted with anti-DAP5 polyclonal antibodies (left). (B) Capped LS-DAP5 transcripts were translated as described above, supplemented with anti-Flag immunoprecipitates from transiently transfected 293 cells overexpressing DAP5 protein forms. The resulting autoradiogram of the translation products is presented at the right. The same translation reactions were separated on 10% gel and immunoblotted with anti-DAP5 polyclonal antibodies (left). The solid and dashed arrows on the left indicate endogenous DAP5 within the RRL; the dashed arrow indicates the minor fast-migrating DAP5 form, present both in cells (Fig. 1) and in RRL. Exogenous DAP5 forms from the immunoprecipitations are marked by the arrows to the right. (C) An experiment similar to that in panel B was performed on both LS-DAP5 and LS-EMCV transcripts in parallel, supplemented by equivalent amounts of exogenous DAP5 proteins (compare within bar pairs) as follows: bar 1, control; bar 2, DAP5/p86; bars 3 to 5, increasing amounts of DAP5/p97. The quantity of supplemented exogenous DAP5 proteins was determined by densitometry of immunoblots of the translation reactions, reacted with anti-DAP5 antibodies. The level of endogenous DAP5 in the RRL was scored as 1, and the calculated relative levels of exogenous DAP5 are presented below each bar pair. The raw band intensity data of the LS-DAP5 translation reactions presented in the graph are detailed in the form of bar no. (luciferase, SeAP, SeAP/LUC ratio): 1 (894, 417, 0.47), 2 (1207, 948, 0.79), 3 (1222, 617, 0.50), 4 (1131, 812, 0.72), and 5 (937, 661, 0.71).

In a reciprocal approach, we tested how DAP5 IRES-mediated translation is affected by addition of recombinant DAP5/p97 orDAP5/p86 on top of the endogenous DAP5 present in the reticulocytes.Exogenous DAP5 proteins were immunoprecipitated from 293 cellsoverexpressing Flag-DAP5/p97 or Flag-DAP5/p86. Immunoprecipitatesfrom 293 cells transfected with an empty vector were used as acontrol. The effect of these recombinant proteins on in vitrotranslation of the LS DAP5 transcript was examined. It was foundthat addition of either DAP5 form to the cell-free translationsystem significantly altered the ratio between the two cistrons,resulting in more than a 1.5-fold increase in favor of cap-independenttranslation from the DAP5 IRES (Fig. 7B, right panel). Westernblot analysis of the translation reactions confirmed the presenceof each exogenous DAP5 form in the reactions and enabled comparisonof their levels to those of the endogenous DAP5 (Fig. 7B, leftpanel; note that the recombinant p97 form was in large excessover the p86 form). To make more accurate comparisons betweenDAP5/p97 and DAP5/p86 in these functional assays, we scaled downthe amount of DAP5/p97 added to the reactions. Quantitation ofexogenous DAP5/p97 and DAP5/p86 protein levels in each reactionmixture of RRL and of their effects on the resulting translationproducts from LS-DAP5 transcript revealed that DAP5/p86 was morepotent than DAP5/p97 in these assays (see the legend to Fig. 7Cfor the raw data). While low levels of DAP5/p86 (16% of endogenouslevels) sufficed to enhance the ratio of DAP5 IRES-mediated translationto cap-dependent translation 1.6-fold, much higher levels of DAP5/p97(74% of endogenous levels) were required to achieve a similareffect (compare bars 1, 2, and 4 in Fig. 7C). In addition, furtherdilution of the exogenous DAP5/p97 level to 28% of endogenouslevels (still twice the amount of recombinant protein relativeto DAP5/p86) hardly affected DAP5 IRES-mediated translation (Fig.7C, compare bars 1, 2, and 3). These results further suggest thatthe DAP5/p86 form is more potent in its ability to stimulate DAP5IRES-mediated translation than the DAP5/p97form.

Finally, when the same procedure was carried out in parallel with an LS-EMCV transcript, the ratio between cap-dependent andcap-independent translation did not change in any given concentrationof the DAP5 recombinant proteins (Fig. 7C). This finding complementsprevious results showing that EMCV IRES-mediated translation isrefractory to GST-260 inhibitory effect. Thus, we conclude thatDAP5 IRES-mediated translation, unlike EMCV IRES-mediated translation,is supported by both DAP5 proteins in thissystem.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The requirement for ongoing protein synthesis in PCD differs among various apoptotic systems. Some apoptotic processes arebased primarily on activation of preexisting death proteins suchas the caspases and do not require any de novo-synthesized proteins.Furthermore, in some instances blockage of protein synthesis perse is a critical event in guiding the cell to undergo apoptosis,as in the case of tumor necrosis factor receptor-mediated apoptosis,where a transcription-translation-dependent death-protective pathwayis activated in parallel to the death pathway (2, 38). Conversely,certain scenarios of PCD are translation dependent, as they areabrogated by translation inhibitors. These translation-dependentapoptotic scenarios employ both preexisting and de novo-synthesizeddeath proteins. Some examples are the apoptotic processes in insectand vertebrate embryonic development and the death of tropic factor-deprivedsympathetic neurons (9, 23, 24). The relationship betweenthe translation-dependent and translation-independent apoptoticpathways, how they are interconnected, when one is favored overthe other, and what determines the dominance of one pathway overthe other, are yet unresolvedissues.

The functional cloning of a novel eIF4G homolog, DAP5, as a positive mediator of apoptosis provided a molecular tool for understandingtranslation regulation during apoptosis. DAP5 is one of severalgenes which were isolated by the technical knockout strategy designedfor targeting functionally relevant, rate-limiting death genes(10, 17). The cDNA fragment that served as the basis for DAP5selection directed the synthesis of a miniprotein (amino acids488 to 742) that modulated the function of DAP5 and thus conveyedresistance to gamma interferon-induced cell death (21).

In this work we found that in response to two different apoptotic stimuli and in several cell lines, DAP5/p97 was cleavedat a single conserved caspase cleavage site, generating a novelDAP5/p86 form devoid of its C terminus. In addition, we discoveredthat while there was a general decrease in the translation rateduring Fas-induced apoptosis, in accordance with the degradationof eIF4GI and eIF4GII proteins, DAP5 protein was selectively translated.Examination of the 5'UTR sequence of DAP5 revealed the presenceof a functional IRES which was preferentially utilized over cap-dependenttranslation during Fas-induced apoptosis. Such a quality can providean advantage for a positive mediator of apoptosis under thesetranslation-limiting conditions. However, it should be stressedthat unlike the p53-induced death of LTR/M1 cells or the gammainterferon-induced apoptosis, Fas-induced cell death can proceedin the absence of new protein synthesis. Thus, some apoptoticsystems clearly utilize dominant protein synthesis-independentpathways although they still display the typical pattern of DAP5regulation and the described changes in the translation machinery.This further documents the complexity and diversity of apoptoticpathways, which may be differently utilized in various scenarios.Further evidence for this complexity stems from the finding thatectopic expression of DAP5/p86 did not culminate in cell death(not shown), suggesting that DAP5 by itself is not sufficientto induce apoptosis and that additional death signals may berequired.

An important aspect highlighted by this work refers to the alterations of the protein translation initiation machinery underapoptotic stress. Early reports noted an eventual shutdown oftranslation that occurs as apoptosis proceeds (9). Recentlythe reduction in translation rate in apoptotic cells was correlatedwith the caspase cleavage of eIF4GI in a wide range of cell typesand apoptotic triggers (6, 7, 22, 27). We also correlatedthe reduction in protein translation rate during Fas-induced apoptosiswith the rapid degradation of eIF4GI and eIF4GII. However, wenoticed that the protein translation machinery was not completelyturned off and that translation continued at one-third of itsnormal rate. This raised the possibility that the residual translationactivity resulted from an alternative translation mechanism whichis eIF4GI/GIIindependent.

Is there a subgroup of death-associated proteins translated under apoptotic stress? Although we failed to detect a uniquepattern of metabolically labeled proteins in apoptotic cells bycomparing their profile by one-dimensional gel electrophoresis(not shown), a more sensitive comparison might be required toreveal subtle changes in the synthesis of specific proteins. However,by following the translation rate of DAP5 itself, we found thisfirst candidate and further examined the possibility that itsadvantageous translation in apoptosis may occur via cap-independentmechanisms. Indeed, we found that DAP5's 5'UTR can drive cap-independenttranslation in reporter studies using bicistronic vectors. Furthermore,transfections with a bicistronic vector containing the DAP5 IRESshowed that translation via this IRES was maintained, while cap-dependenttranslation was strongly reduced, in response to an apoptotictrigger. This observation implies that the DAP5 IRES drives translationunder apoptotic stress. Recently, another cellular IRES, the X-linkedinhibitor of apoptosis (XIAP) IRES, was also shown to enable continuoustranslation during apoptosis induced by serum deprivation (14).Identification of additional IRES-containing cellular messages,preferentially translated during cell death, might open a newhorizon for identification of major apoptotic genes. It shouldbe mentioned that cap-independent translation has already beenassociated with stressful cellular situations in which overallprotein synthesis (mostly cap-dependent in nature) is significantlyinhibited. These situations include heat shock (11) and hypoxia(19, 34).

What is the biochemical activity of DAP5 (in particular DAP5/p86), and how does it contribute to cell death? DAP5 is one ofseveral novel members of the expanding eIF4G protein family whichincludes, besides eIF4GI and eIF4GII (12), the recently identifiedpoly(A) binding protein-interacting protein (PAIP) (8), allof which share homology in the middle eIF4A and eIF3 binding segment(Fig. 8). According to one working model, DAP5 might functionas a translation inhibitor, titrating out initiation factors eIF4Aand eIF3. The titrator model is based on the finding that DAP5/p97overexpression in transient transfection assays led to a twofoldreduction in both cap-dependent and cap-independent translation(15, 40). Recently it was found that DAP5, like eIF4GI, interactswith Mnk1 and thus may interfere with the phosphorylation of eIF4Eas a second possible titrating mechanism (32, 39). The death-promotingactivity of DAP5, according to the titrator model, might be todisrupt the maintenance of cap-dependent synthesis of prosurvivalproteins. It should be noted that in transfection-based functionalassays, nonphysiological effects due to large excess of the ectopicallyexpressed DAP5 protein may be observed. Moreover, the findingthat during apoptosis translation is shut down rapidly and efficientlyby cleavage of eIF4GI/GII (6, 7, 22, 27) reduces theneed for DAP5 to function as a translation titrator under thesecircumstances.

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FIG. 8. Amino acid homology alignment of eIF4GI and DAP5. eIF4GI and DAP5 are divided into regions based on the high homology of the central region of eIF4GI with the N-terminal region of DAP5. The shaded boxes indicate binding sites of translation initiation factors: 4E, eIF4E, the cap binding protein; 4A, eIF4A, an ATP-dependent RNA helicase; and 3, eIF3, a ribosome adapter. The site of cleavage of eIF4GI by 2A protease is indicated by a dashed line at position 490. The identified caspase cleavage site of DAP5 is indicated by a dashed line at position 790. DAP5 protein fragments corresponding to amino acids 488 to 742 and 672 to 830 were used for the production of polyclonal and monoclonal antibodies, respectively, against DAP5. Regional homologies at the amino acid level of the conserved N-terminal region and of the less homologous DAP5 miniprotein region between DAP5 and eIF4GI are indicated. Alignment was performed as previously published (21), and homology was determined by using the Dayhoff PAM250 residue weight table. ID, identity; SIM, similarity.

An alternative working model proposes that DAP5 itself might be an active functional member of the eIF4G family, capable ofsupporting cap-independent translation, especially under conditionswhere cap-dependent translation is unfavorable. According to thismodel, DAP5 may drive the cell down the apoptotic pathway by selectivelytranslating death genes via "death IRESes." In this work, we providenew support for this alternative model. The finding that DAP5/p86becomes the predominant eIF4G form in the dying cells, capableof binding eIF3 and eIF4A, made it an attractive candidate forsupporting residual translation, including its own, in the dyingcells. Indeed, we found that DAP5 can function as an active translationfactor in cell-free systems. We show here that translation fromthe IRES element found in the DAP5 5'UTR was preferentially stimulatedover cap-dependent translation by adding excess of recombinantDAP5 proteins into the RRL. Conversely, it was preferentiallysuppressed by adding a dominant negative fragment of DAP5. Takingthese observations together, we suggest that DAP5 may mediateits own translation under conditions that are unfavorable forcap-dependent translation and thus be responsible for its sustainedtranslation during apoptosis. The next step will be to determinewhether it mediates the translation of other proapoptotic genesaswell.

Last, we have identified DAP5 as a caspase substrate. Despite the fact that the list of caspase cellular substrates that arecleaved during the execution of the cell death program is expandingrapidly, it is important to keep in mind that caspases are highlyselective proteases (28, 31, 36). Cell death is characterizedby highly regulated and selective cleavage of discrete, specificproteins rather than by a bulk, nonspecific proteolysis of cellularproteins. We found that the caspase cleavage of DAP5 potentiatesits ability to support DAP5 IRES translation in vitro. Furtherstudies will be required to assess more accurately the mechanismby which the C-terminal truncation changes DAP5'sproperties.

	ACKNOWLEDGMENTS

The first two authors contributed equally to thiswork.

We thank Nahum Sonenberg for kindly providing the anti-eIF4A, eIF3, and eIF4GII antibodies. We thank Eli Keshet, Yoram Groner,and Orna Stein for the different DNA constructs. We thank DavidWallach for kindly providing the HFB cellline.

This work was supported by the Israel Foundation, which is administered by the Israel Academy of Sciences and Humanities,and by QBI Enterprises. A.K. is the incumbent of Helena RubinsteinChair of CancerResearch.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Genetics, Weizmann Institute of Science, Rehovot 76100, Israel.Phone: 972-8-9342428. Fax: 972-8-9344108. E-mail: lvkimchi{at}weizmann.weizmann.ac.il.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Akiri, G., D. Nahari, Y. Finkelstein, S. Y. Le, O. Elroy-Stein, and B. Z. Levi. 1998. Regulation of vascular endothelial growth factor (VEGF) expression is mediated by internal initiation of translation and alternative initiation of transcription. Oncogene 17:227-236[CrossRef][Medline].

2. Ashkenazi, A., and V. M. Dixit. 1998. Death receptors: signaling and modulation. Science 281:1305-1308[Abstract/Free Full Text].

3. Bernstein, J., O. Sella, S. Y. Le, and O. Elroy-Stein. 1997. PDGF2/c-sis mRNA leader contains a differentiation-linked internal ribosomal entry site (D-IRES). J. Biol. Chem. 272:9356-9362[Abstract/Free Full Text].

4. Boldin, M. P., E. E. Varfolomeev, Z. Pancer, I. L. Mett, J. H. Camonis, and D. Wallach. 1995. A novel protein that interacts with the death domain of Fas/APO1 contains a sequence motif related to the death domain. J. Biol. Chem. 270:7795-7798[Abstract/Free Full Text].

5. Borman, A. M., R. Kirchweger, E. Ziegler, R. E. Rhoads, T. Skern, and K. M. Kean. 1997. eIF4G and its proteolytic cleavage products: effect on initiation of protein synthesis from capped, uncapped, and IRES-containing mRNAs. RNA 3:186-196[Abstract].

6. Bushell, M., L. McKendrick, R. U. Janicke, M. J. Clemens, and S. J. Morley. 1999. Caspase-3 is necessary and sufficient for cleavage of protein synthesis eukaryotic initiation factor 4G during apoptosis. FEBS Lett. 451:332-336[CrossRef][Medline].

7. Clemens, M. J., M. Bushell, and S. J. Morley. 1998. Degradation of eukaryotic polypeptide chain initiation factor (eIF) 4G in response to induction of apoptosis in human lymphoma cell lines. Oncogene 17:2921-2931[CrossRef][Medline].

8. Craig, A. W., A. Haghighat, A. T. Yu, and N. Sonenberg. 1998. Interaction of polyadenylate-binding protein with the eIF4G homologue PAIP enhances translation. Nature 392:520-523[CrossRef][Medline].

9. Deckwerth, T. L., and E. M. Johnson, Jr. 1993. Temporal analysis of events associated with programmed cell death (apoptosis) of sympathetic neurons deprived of nerve growth factor. J. Cell Biol. 123:1207-1222[Abstract/Free Full Text].

10. Deiss, L. P., and A. Kimchi. 1991. A genetic tool used to identify thioredoxin as a mediator of a growth inhibitory signal. Science 252:117-120[Abstract/Free Full Text].

11. Duncan, R. F. 1996. Translational control during heat shock, p. 271-293. In J. W. B. Hershey, M. B. Mathews, and N. Sonenberg (ed.), Translational control. CSHL Press, Cold Spring Harbor, N.Y.

12. Gradi, A., H. Imataka, Y. V. Svitkin, E. Rom, B. Raught, S. Morino, and N. Sonenberg. 1998. A novel functional human eukaryotic translation initiation factor 4G. Mol. Cell. Biol. 18:334-342[Abstract/Free Full Text].

13. Gradi, A., Y. V. Svitkin, H. Imataka, and N. Sonenberg. 1998. Proteolysis of human eukaryotic translation initiation factor eIF4GII, but not eIF4GI, coincides with the shutoff of host protein synthesis after poliovirus infection. Proc. Natl. Acad. Sci. USA 95:11089-11094[Abstract/Free Full Text].

14. Holcik, M., C. Lefebvre, C. Yeh, T. Chow, and R. G. Korneluk. 1999. A new internal-ribosome-entry-site motif potentiates XIAP-mediated cytoprotection. Nat. Cell Biol. 1:190-192[CrossRef][Medline].

15. Imataka, H., H. S. Olsen, and N. Sonenberg. 1997. A new translational regulator with homology to eukaryotic translation initiation factor 4G. EMBO J. 16:817-825[CrossRef][Medline].

16. Imataka, H., and N. Sonenberg. 1997. Human eukaryotic translation initiation factor 4G (eIF4G) possesses two separate and independent binding sites for eIF4A. Mol. Cell. Biol. 17:6940-6947[Abstract].

17. Kimchi, A. 1998. DAP genes: novel apoptotic genes isolated by a functional approach to gene cloning. Biochim. Biophys. Acta 1377:F13-F33[Medline].

18. Kissil, J. L., O. Cohen, T. Raveh, and A. Kimchi. 1999. Structure-function analysis of an evolutionary conserved protein, DAP3, which mediates TNF-alpha- and Fas-induced cell death. EMBO J. 18:353-362[CrossRef][Medline].

19. Kraggerud, S. M., J. A. Sandvik, and E. O. Pettersen. 1995. Regulation of protein synthesis in human cells exposed to extreme hypoxia. Anticancer Res. 15:683-686[Medline].

20. Lamphear, B. J., R. Kirchweger, T. Skern, and R. E. Rhoads. 1995. Mapping of functional domains in eukaryotic protein synthesis initiation factor 4G (eIF4G) with picornaviral proteases. Implications for cap-dependent and cap-independent translational initiation. J. Biol. Chem. 270:21975-21983[Abstract/Free Full Text].

21. Levy-Strumpf, N., L. P. Deiss, H. Berissi, and A. Kimchi. 1997. DAP-5, a novel homolog of eukaryotic translation initiation factor 4G isolated as a putative modulator of gamma interferon-induced programmed cell death. Mol. Cell. Biol. 17:1615-1625[Abstract].

22. Marissen, W. E., and R. E. Lloyd. 1998. Eukaryotic translation initiation factor 4G is targeted for proteolytic cleavage by caspase 3 during inhibition of translation in apoptotic cells. Mol. Cell. Biol. 18:7565-7574[Abstract/Free Full Text].

23. Martin, D. P., R. E. Schmidt, P. S. DiStefano, O. H. Lowry, J. G. Carter, and E. M. Johnson, Jr. 1988. Inhibitors of protein synthesis and RNA synthesis prevent neuronal death caused by nerve growth factor deprivation. J. Cell Biol. 106:829-844[Abstract/Free Full Text].

24. McCall, K., and H. Steller. 1997. Facing death in the fly: genetic analysis of apoptosis in Drosophila. Trends Genet. 13:222-226[CrossRef][Medline].

25. Methot, N., E. Rom, H. Olsen, and N. Sonenberg. 1997. The human homologue of the yeast Prt1 protein is an integral part of the eukaryotic initiation factor 3 complex and interacts with p170. J. Biol. Chem. 272:1110-1116[Abstract/Free Full Text].

26. Morley, S. J., P. S. Curtis, and V. M. Pain. 1997. eIF4G: translation's mystery factor begins to yield its secrets. RNA 3:1085-1104[Medline].

27. Morley, S. J., L. McKendrick, and M. Bushell. 1998. Cleavage of translation initiation factor 4G (eIF4G) during anti-Fas IgM-induced apoptosis does not require signalling through the p38 mitogen-activated protein (MAP) kinase. FEBS Lett. 438:41-48[CrossRef][Medline].

28. Nicholson, D. W., and N. A. Thornberry. 1997. Caspases: killer proteases. Trends Biochem. Sci. 22:299-306[CrossRef][Medline].

29. Ohlmann, T., M. Rau, V. M. Pain, and S. J. Morley. 1996. The C-terminal domain of eukaryotic protein synthesis initiation factor (eIF) 4G is sufficient to support cap-independent translation in the absence of eIF4E. EMBO J. 15:1371-1382[Medline].

30. Pestova, T. V., I. N. Shatsky, and C. U. Hellen. 1996. Functional dissection of eukaryotic initiation factor 4F: the 4A subunit and the central domain of the 4G subunit are sufficient to mediate internal entry of 43S preinitiation complexes. Mol. Cell. Biol. 16:6870-6878[Abstract].

31. Porter, A. G., P. Ng, and R. U. Janicke. 1997. Death substrates come alive. Bioessays 19:501-507

1.	Akiri, G., D. Nahari, Y. Finkelstein, S. Y. Le, O. Elroy-Stein, and B. Z. Levi. 1998. Regulation of vascular endothelial growth factor (VEGF) expression is mediated by internal initiation of translation and alternative initiation of transcription. Oncogene 17:227-236[CrossRef][Medline].
2.	Ashkenazi, A., and V. M. Dixit. 1998. Death receptors: signaling and modulation. Science 281:1305-1308[Abstract/Free Full Text].
3.	Bernstein, J., O. Sella, S. Y. Le, and O. Elroy-Stein. 1997. PDGF2/c-sis mRNA leader contains a differentiation-linked internal ribosomal entry site (D-IRES). J. Biol. Chem. 272:9356-9362[Abstract/Free Full Text].
4.	Boldin, M. P., E. E. Varfolomeev, Z. Pancer, I. L. Mett, J. H. Camonis, and D. Wallach. 1995. A novel protein that interacts with the death domain of Fas/APO1 contains a sequence motif related to the death domain. J. Biol. Chem. 270:7795-7798[Abstract/Free Full Text].
5.	Borman, A. M., R. Kirchweger, E. Ziegler, R. E. Rhoads, T. Skern, and K. M. Kean. 1997. eIF4G and its proteolytic cleavage products: effect on initiation of protein synthesis from capped, uncapped, and IRES-containing mRNAs. RNA 3:186-196[Abstract].
6.	Bushell, M., L. McKendrick, R. U. Janicke, M. J. Clemens, and S. J. Morley. 1999. Caspase-3 is necessary and sufficient for cleavage of protein synthesis eukaryotic initiation factor 4G during apoptosis. FEBS Lett. 451:332-336[CrossRef][Medline].
7.	Clemens, M. J., M. Bushell, and S. J. Morley. 1998. Degradation of eukaryotic polypeptide chain initiation factor (eIF) 4G in response to induction of apoptosis in human lymphoma cell lines. Oncogene 17:2921-2931[CrossRef][Medline].
8.	Craig, A. W., A. Haghighat, A. T. Yu, and N. Sonenberg. 1998. Interaction of polyadenylate-binding protein with the eIF4G homologue PAIP enhances translation. Nature 392:520-523[CrossRef][Medline].
9.	Deckwerth, T. L., and E. M. Johnson, Jr. 1993. Temporal analysis of events associated with programmed cell death (apoptosis) of sympathetic neurons deprived of nerve growth factor. J. Cell Biol. 123:1207-1222[Abstract/Free Full Text].
10.	Deiss, L. P., and A. Kimchi. 1991. A genetic tool used to identify thioredoxin as a mediator of a growth inhibitory signal. Science 252:117-120[Abstract/Free Full Text].
11.	Duncan, R. F. 1996. Translational control during heat shock, p. 271-293. In J. W. B. Hershey, M. B. Mathews, and N. Sonenberg (ed.), Translational control. CSHL Press, Cold Spring Harbor, N.Y.
12.	Gradi, A., H. Imataka, Y. V. Svitkin, E. Rom, B. Raught, S. Morino, and N. Sonenberg. 1998. A novel functional human eukaryotic translation initiation factor 4G. Mol. Cell. Biol. 18:334-342[Abstract/Free Full Text].
13.	Gradi, A., Y. V. Svitkin, H. Imataka, and N. Sonenberg. 1998. Proteolysis of human eukaryotic translation initiation factor eIF4GII, but not eIF4GI, coincides with the shutoff of host protein synthesis after poliovirus infection. Proc. Natl. Acad. Sci. USA 95:11089-11094[Abstract/Free Full Text].
14.	Holcik, M., C. Lefebvre, C. Yeh, T. Chow, and R. G. Korneluk. 1999. A new internal-ribosome-entry-site motif potentiates XIAP-mediated cytoprotection. Nat. Cell Biol. 1:190-192[CrossRef][Medline].
15.	Imataka, H., H. S. Olsen, and N. Sonenberg. 1997. A new translational regulator with homology to eukaryotic translation initiation factor 4G. EMBO J. 16:817-825[CrossRef][Medline].
16.	Imataka, H., and N. Sonenberg. 1997. Human eukaryotic translation initiation factor 4G (eIF4G) possesses two separate and independent binding sites for eIF4A. Mol. Cell. Biol. 17:6940-6947[Abstract].
17.	Kimchi, A. 1998. DAP genes: novel apoptotic genes isolated by a functional approach to gene cloning. Biochim. Biophys. Acta 1377:F13-F33[Medline].
18.	Kissil, J. L., O. Cohen, T. Raveh, and A. Kimchi. 1999. Structure-function analysis of an evolutionary conserved protein, DAP3, which mediates TNF-alpha- and Fas-induced cell death. EMBO J. 18:353-362[CrossRef][Medline].
19.	Kraggerud, S. M., J. A. Sandvik, and E. O. Pettersen. 1995. Regulation of protein synthesis in human cells exposed to extreme hypoxia. Anticancer Res. 15:683-686[Medline].
20.	Lamphear, B. J., R. Kirchweger, T. Skern, and R. E. Rhoads. 1995. Mapping of functional domains in eukaryotic protein synthesis initiation factor 4G (eIF4G) with picornaviral proteases. Implications for cap-dependent and cap-independent translational initiation. J. Biol. Chem. 270:21975-21983[Abstract/Free Full Text].
21.	Levy-Strumpf, N., L. P. Deiss, H. Berissi, and A. Kimchi. 1997. DAP-5, a novel homolog of eukaryotic translation initiation factor 4G isolated as a putative modulator of gamma interferon-induced programmed cell death. Mol. Cell. Biol. 17:1615-1625[Abstract].
22.	Marissen, W. E., and R. E. Lloyd. 1998. Eukaryotic translation initiation factor 4G is targeted for proteolytic cleavage by caspase 3 during inhibition of translation in apoptotic cells. Mol. Cell. Biol. 18:7565-7574[Abstract/Free Full Text].
23.	Martin, D. P., R. E. Schmidt, P. S. DiStefano, O. H. Lowry, J. G. Carter, and E. M. Johnson, Jr. 1988. Inhibitors of protein synthesis and RNA synthesis prevent neuronal death caused by nerve growth factor deprivation. J. Cell Biol. 106:829-844[Abstract/Free Full Text].
24.	McCall, K., and H. Steller. 1997. Facing death in the fly: genetic analysis of apoptosis in Drosophila. Trends Genet. 13:222-226[CrossRef][Medline].
25.	Methot, N., E. Rom, H. Olsen, and N. Sonenberg. 1997. The human homologue of the yeast Prt1 protein is an integral part of the eukaryotic initiation factor 3 complex and interacts with p170. J. Biol. Chem. 272:1110-1116[Abstract/Free Full Text].
26.	Morley, S. J., P. S. Curtis, and V. M. Pain. 1997. eIF4G: translation's mystery factor begins to yield its secrets. RNA 3:1085-1104[Medline].
27.	Morley, S. J., L. McKendrick, and M. Bushell. 1998. Cleavage of translation initiation factor 4G (eIF4G) during anti-Fas IgM-induced apoptosis does not require signalling through the p38 mitogen-activated protein (MAP) kinase. FEBS Lett. 438:41-48[CrossRef][Medline].
28.	Nicholson, D. W., and N. A. Thornberry. 1997. Caspases: killer proteases. Trends Biochem. Sci. 22:299-306[CrossRef][Medline].
29.	Ohlmann, T., M. Rau, V. M. Pain, and S. J. Morley. 1996. The C-terminal domain of eukaryotic protein synthesis initiation factor (eIF) 4G is sufficient to support cap-independent translation in the absence of eIF4E. EMBO J. 15:1371-1382[Medline].
30.	Pestova, T. V., I. N. Shatsky, and C. U. Hellen. 1996. Functional dissection of eukaryotic initiation factor 4F: the 4A subunit and the central domain of the 4G subunit are sufficient to mediate internal entry of 43S preinitiation complexes. Mol. Cell. Biol. 16:6870-6878[Abstract].
31.	Porter, A. G., P. Ng, and R. U. Janicke. 1997. Death substrates come alive. Bioessays 19:501-507