CASH, a Novel Caspase Homologue with Death Effector Domains
1997; Elsevier BV; Volume: 272; Issue: 32 Linguagem: Inglês
10.1074/jbc.272.32.19641
ISSN1083-351X
AutoresYury V. Goltsev, Andrew Kovalenko, Ekaterina Arnold, Eugene Varfolomeev, Vadim M. Brodianskii, David Wallach,
Tópico(s)Trace Elements in Health
ResumoCASP-8 and CASP-10, members of a cysteine protease family that participates in apoptosis, interact with MORT1/FADD, an adapter protein in the CD120a (p55 tumor necrosis factor receptor), and CD95 (Fas/Apo-1) death-inducing signaling pathways, through a shared N-terminal sequence motif, the death effector domain. We report cloning of two splice variants of a novel protein, CASH, that contain two N-terminal death effector domains and can bind through them to each other, to MORT1/FADD, to CASP-8, and to CASP-10. The unique C-terminal part of the longer variant shows marked sequence homology to the caspase protease region yet lacks several of the conserved caspase active site residues, suggesting that it is devoid of cysteine protease activity. Overexpression of the short CASH splice variant strongly inhibited cytotoxicity induction by CD120a and CD95. Expression of the longer variant, while inhibiting cytotoxicity in HeLa cells, had a marked cytocidal effect in 293 cells that could be shown to involve its protease homology region. The findings suggest that CASH acts as an attenuator and/or initiator in CD95 and CD120a signaling for cell death. CASP-8 and CASP-10, members of a cysteine protease family that participates in apoptosis, interact with MORT1/FADD, an adapter protein in the CD120a (p55 tumor necrosis factor receptor), and CD95 (Fas/Apo-1) death-inducing signaling pathways, through a shared N-terminal sequence motif, the death effector domain. We report cloning of two splice variants of a novel protein, CASH, that contain two N-terminal death effector domains and can bind through them to each other, to MORT1/FADD, to CASP-8, and to CASP-10. The unique C-terminal part of the longer variant shows marked sequence homology to the caspase protease region yet lacks several of the conserved caspase active site residues, suggesting that it is devoid of cysteine protease activity. Overexpression of the short CASH splice variant strongly inhibited cytotoxicity induction by CD120a and CD95. Expression of the longer variant, while inhibiting cytotoxicity in HeLa cells, had a marked cytocidal effect in 293 cells that could be shown to involve its protease homology region. The findings suggest that CASH acts as an attenuator and/or initiator in CD95 and CD120a signaling for cell death. The caspases, conserved cysteine proteases that cleave specific cellular proteins downstream of aspartate residues, play a critical role in all known programmed cell death processes (reviewed in Refs. 1Kumar S. Trends Biochem. Sci. 1995; 20: 198-202Abstract Full Text PDF PubMed Scopus (366) Google Scholarand 2Henkart P.A. Immunity. 1996; 4: 195-201Abstract Full Text Full Text PDF PubMed Scopus (416) Google Scholar). These proteases (also called the CED3/ICE proteases, after the first described members of the family) (3Ellis H.M. Horvitz H.R. Cell. 1986; 44: 817-829Abstract Full Text PDF PubMed Scopus (1362) Google Scholar, 4Cerretti D.P. Kozlosky C.J. Mosley B. Nelson N. Van Ness K. Greenstreet T.A. March C.J. Kronheim S.R. Druck T. Cannizzaro L.A. Huebner K. Black R.A. Science. 1992; 256: 97-100Crossref PubMed Scopus (1005) Google Scholar, 5Thornberry N.A. Bull H.G. Calaycay J.R. Chapman K.T. Howard A.D. Kostura M.J. Miller D.K. Molineaux S.M. Weidner J.R. Aunins J. et al.Nature. 1992; 356: 768-774Crossref PubMed Scopus (2227) Google Scholar, 6Yuan J. Shaham S. Ledoux S. Ellis H.M. Horvitz H.R. Cell. 1993; 75: 641-652Abstract Full Text PDF PubMed Scopus (2255) Google Scholar) are produced as inactive precursors and become activated by proteolytic processing upon death induction. In addition to their homologous C-terminal region from which the mature proteases are derived, the precursor proteins contain unique N-terminal regions. Interactions of these "prodomains" with specific regulatory molecules allow differential activation of the various caspases by different death-inducing signals (7Boldin M.P. Goncharov T.M. Goltsev Y.V. Wallach D. Cell. 1996; 85: 803-815Abstract Full Text Full Text PDF PubMed Scopus (2113) Google Scholar, 8Muzio M. Chinnaiyan A.M. Kischkel F.C. O'Rourke K. Shevchenko A. Ni J. Scaffidi C. Bretz J.D. Zhang M. Gentz R. Mann M. Krammer P.H. Peter M.E. Dixit V.M. Cell. 1996; 85: 817-827Abstract Full Text Full Text PDF PubMed Scopus (2743) Google Scholar, 9Duan H. Dixit V.M. Nature. 1997; 385: 86-89Crossref PubMed Scopus (469) Google Scholar, 10Van Criekinge W. Beyaert R. Van de Craen M. Vandenabeele P. Schotte P. De Valck D. Fiers W. J. Biol. 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A. 1996; 93: 7646-7649Crossref Scopus (693) Google Scholar) and CASP-10 (Mch4/FLICE2) (12Fernandes-Alnemri T. Armstrong R.C. Krebs J. Srinivasula S.M. Wang L. Bullrich F. Fritz L.C. Trapani J.A. Tomaselli K.J. Litwack G. Alnemri E.S. Proc. Natl. Acad. Sci. U. S. A. 1996; 93: 7646-7649Crossref Scopus (693) Google Scholar, 13Vincent C. Dixit V.M. J. Biol. Chem. 1997; 272: 6578-6583Abstract Full Text Full Text PDF PubMed Scopus (240) Google Scholar), interact through their prodomains with MORT1/FADD (14Boldin M.P. Varfolomeev E.E. Pancer Z. Mett I.L. Camonis J.H. Wallach D. J. Biol. Chem. 1995; 270: 7795-7798Abstract Full Text Full Text PDF PubMed Scopus (941) Google Scholar, 15Chinnaiyan A.M. O'Rourke K. Tewari M. Dixit V.M. Cell. 1995; 81: 505-512Abstract Full Text PDF PubMed Scopus (2163) Google Scholar), an adapter protein in the death-signaling cascades activated by two closely related receptors of the TNF 1The abbreviations used are: TNF, tumor necrosis factor; DED, death effector domain; PCR, polymerase chain reaction. /nerve growth factor family, CD120a (the p55 TNF receptor) and CD95 (Fas/Apo-1). This interaction, which is required for the signaling to death, involves a protein-binding motif called the "death effector domain" (DED) or the "MORT" motif, found in the N-terminal part of MORT1/FADD and in duplicate in the prodomains of CASP-8 and CASP-10. Here we report cloning of a novel protein, CASH, that contains duplicated DED at its N terminus and binds through this region to MORT1/FADD. The C-terminal part of the protein shows marked sequence homology to the corresponding regions in CASP-8 and CASP-10 yet lacks several of the residues that are crucial for cysteine protease activity. Functional tests demonstrated an ability of the novel protein to trigger as well as to inhibit signaling for death. CASHβ was cloned by two-hybrid screening (16Fields S. Song O. Nature. 1989; 340: 245-246Crossref PubMed Scopus (4875) Google Scholar) of a Gal4 activation domain-tagged human Jurkat T cell library (donated by J. H. Camonis, Curie Institute) for proteins that bind to CASP-10 using the HF7c yeast reporter strain (CLONTECH, Palo Alto, CA). Screening was performed in the absence of 3-aminotriazole according to the Matchmaker Two-Hybrid System Protocol (CLONTECH). The binding properties of CASHβ, as well as CASHα were assessed in the yeast SFY526 reporter strain (CLONTECH) using the pGBT9-GAL4 DNA-binding domain and the pGAD1318 and pGADGH-GAL4 activation-domain vectors. Quantification of the binding in yeast by the β-galactosidase expression filter assay was performed as described (17Boldin M.P. Mett I.L. Varfolomeev E.E. Chumakov I. Shemer-Avni Y. Camonis J.H. Wallach D. J. Biol. Chem. 1995; 270: 387-391Abstract Full Text Full Text PDF PubMed Scopus (351) Google Scholar). An expressed sequence tag clone (GenBank accession number AA198928) was identified as the mouse homologue of part of the DED region in CASH. Based on this sequence we cloned the mouse CASHα and CASHβ splice variants from mouse liver mRNA by reverse transcription-PCR. The reverse transcriptase reaction was performed with an oligo(dT) adapter primer (5′-GACTCGAGTCTAGAGTCGAC(T)17-3′) and the avian myeloblastosis virus reverse transcriptase (Promega) used according to the manufacturer's instructions. The first round of PCR was carried out with the Expand Long Template PCR System (Boehringer Mannheim) using the following sense and antisense primers: 5′-GGCTTCTCGTGGTTCCCAGAGC-3′ and 5′-GACTCGAGTCTAGAGTCGAC-3′ (adapter) respectively. The second round was performed with Vent polymerase (NEB) using the nested sense primer 5′-TGCTCTTCCTGTGTAGAGATG-3′ and adapter. A radiolabeled mRNA probe corresponding to the DED module region of CASH was prepared using the T7 RNA polymerase (Promega) and used for analysis of human multiple tissue blots (CLONTECH) according to the manufacturer's instructions. Sequence alignment and homology evaluation were performed using the GAP and PILEUP programs of the GCG package and by the CLUSTAL 1.5 software. Sequence data base search was performed using the BLAST program. As parameter of homology significance we used "smallest sum probability" (P(N)), i.e. the probability of observing by chance a score or a group of scores as high as the observed ones when performing a search of the same size. The consensus for the DED region sequence was deduced from the alignment of the DED modules in MORT/FADD (14Boldin M.P. Varfolomeev E.E. Pancer Z. Mett I.L. Camonis J.H. Wallach D. J. Biol. Chem. 1995; 270: 7795-7798Abstract Full Text Full Text PDF PubMed Scopus (941) Google Scholar, 15Chinnaiyan A.M. O'Rourke K. Tewari M. Dixit V.M. Cell. 1995; 81: 505-512Abstract Full Text PDF PubMed Scopus (2163) Google Scholar), MACH/FLICE/Mch5 (7Boldin M.P. Goncharov T.M. Goltsev Y.V. Wallach D. Cell. 1996; 85: 803-815Abstract Full Text Full Text PDF PubMed Scopus (2113) Google Scholar, 8Muzio M. Chinnaiyan A.M. Kischkel F.C. O'Rourke K. Shevchenko A. Ni J. Scaffidi C. Bretz J.D. Zhang M. Gentz R. Mann M. Krammer P.H. Peter M.E. Dixit V.M. Cell. 1996; 85: 817-827Abstract Full Text Full Text PDF PubMed Scopus (2743) Google Scholar, 12Fernandes-Alnemri T. Armstrong R.C. Krebs J. Srinivasula S.M. Wang L. Bullrich F. Fritz L.C. Trapani J.A. Tomaselli K.J. Litwack G. Alnemri E.S. Proc. Natl. Acad. Sci. U. S. A. 1996; 93: 7646-7649Crossref Scopus (693) Google Scholar), Mch4/FLICE2 (12Fernandes-Alnemri T. Armstrong R.C. Krebs J. Srinivasula S.M. Wang L. Bullrich F. Fritz L.C. Trapani J.A. Tomaselli K.J. Litwack G. Alnemri E.S. Proc. Natl. Acad. Sci. U. S. A. 1996; 93: 7646-7649Crossref Scopus (693) Google Scholar, 13Vincent C. Dixit V.M. J. Biol. Chem. 1997; 272: 6578-6583Abstract Full Text Full Text PDF PubMed Scopus (240) Google Scholar), PEA-15 (18Araujo H. Danziger N. Cordier J. Glowinsky J. Chneiweiss H. J. Biol. Chem. 1993; 268: 5911-5920Abstract Full Text PDF PubMed Google Scholar), M159, E-8 (19Bertin J. Armstrong R.C. Ottilie S. Martin D.A. Wang Y. Banks S. Wang G.-H. Senkevich T.G. Alnemri E.S. Moss B. Lenardo M.J. Tomaselli K.J. Cohen J.I. Proc. Natl. Acad. Sci. U. S. A. 1997; 94: 1172-1176Crossref PubMed Scopus (384) Google Scholar), and K13 (20Hu S. Vincenz C. Buller M. Dixit V.M. J. Biol. Chem. 1997; 272: 9621-9624Abstract Full Text Full Text PDF PubMed Scopus (268) Google Scholar), and the consensus for the protease-homology region was deduced from the alignment of CASP-1, 2, 3, 6, 7, 8, and 10 (21Alnemri E.S. Livingston D.J. Nicholson D.W. Salveson G. Thornberry N.A. Wong W.W. Yuan J. Cell. 1996; 87: 171Abstract Full Text Full Text PDF PubMed Scopus (2146) Google Scholar) and CED3 (3Ellis H.M. Horvitz H.R. Cell. 1986; 44: 817-829Abstract Full Text PDF PubMed Scopus (1362) Google Scholar). Residues occurring in more than six of the aligned proteins were included in the consensus. The CASHα deletion mutants and the CD120a/CD95 chimera were produced by PCR and/or conventional cloning techniques. The CASH splice variants, the CD95 or CD120a signaling-cascade proteins (all of human origin), and the baculovirus p35 protein were expressed in mammalian cells using the pcDNA3 expression vector (Invitrogen). β-Galactosidase was expressed using the pCMV-β-gal vector (Promega). The human embryonic kidney 293-T, 293-EBNA, and 293 cells and human cervical carcinoma HeLa cells (HeLa-Fas; the HtTA-1 clone (obtained from Dr. H. Bujard)) stably expressing transfected human CD95 (established in our laboratory) were grown in Dulbecco's modified Eagle's minimal essential medium supplemented with 10% fetal calf serum, nonessential amino acids, 100 units/ml penicillin and 100 μg/ml streptomycin. Cells (5 × 105 293 cells or 3 × 105HeLa cells per 6-cm dishes) were transiently transfected with the cDNAs of the indicated proteins together with the pCMV-β-gal, using the calcium phosphate precipitation method. Each dish was transfected with 5 μg of the pcDNA3 construct of interest or, when transfecting two different constructs, 2.5 μg of each, and 1.5 μg of β-galactosidase expression vector. Cells were rinsed 6–10 h after transfection and then incubated for a further 14 h without additional treatment. Anti-CD95 monoclonal antibody (CH11 (Oncor, Gaithersburg, MD), 0.5 μg/ml) and human recombinant TNFα (100 ng/ml) were applied to the cells together with cycloheximide (10 μg/ml) and incubated for an additional 4 h. Cells were then stained with 5-bromo-4-chloro-3-indoxyl-β-d-galactopyranoside (22Kumar S. Kinoshita M. Noda M. Copeland N.G. Jenkins N.A. Genes & Dev. 1994; 8: 1613-1626Crossref PubMed Scopus (587) Google Scholar) and examined by phase contrast microscopy. In all experiments shown, death was assessed 24 h after transfection for HeLa-Fas cells and 20 h after transfection for 293 cells. To search for the proteins that bind to CASP-10 (Mch4/FLICE2), we performed two-hybrid screening of human Jurkat T cell cDNA library using CASP-10 as a bait. This screen yielded cDNA clones of MORT1/FADD, previously shown to bind to CASP-10 (13Vincent C. Dixit V.M. J. Biol. Chem. 1997; 272: 6578-6583Abstract Full Text Full Text PDF PubMed Scopus (240) Google Scholar). It also yielded a partial clone of a novel cDNA, which like CASP-8 and CASP-10, contained two death effector (MORT) modules (7Boldin M.P. Goncharov T.M. Goltsev Y.V. Wallach D. Cell. 1996; 85: 803-815Abstract Full Text Full Text PDF PubMed Scopus (2113) Google Scholar, 8Muzio M. Chinnaiyan A.M. Kischkel F.C. O'Rourke K. Shevchenko A. Ni J. Scaffidi C. Bretz J.D. Zhang M. Gentz R. Mann M. Krammer P.H. Peter M.E. Dixit V.M. Cell. 1996; 85: 817-827Abstract Full Text Full Text PDF PubMed Scopus (2743) Google Scholar, 12Fernandes-Alnemri T. Armstrong R.C. Krebs J. Srinivasula S.M. Wang L. Bullrich F. Fritz L.C. Trapani J.A. Tomaselli K.J. Litwack G. Alnemri E.S. Proc. Natl. Acad. Sci. U. S. A. 1996; 93: 7646-7649Crossref Scopus (693) Google Scholar) just downstream of its N terminus (Fig. 1). Because of the similarity of the protein to the caspases (see below) it was dubbed CASH, for caspase homologue. Northern blot analysis revealed that the molecule exists in at least three distinct transcript sizes, 1.5, 2.4, and 4.0 kilobase pairs (data not shown), whose proportions vary greatly among different tissues. To obtain the full-length cDNA of CASH, we screened human skin fibroblast cDNA library (CLONTECH) with a cDNA probe corresponding to the CASH sequence. We obtained two cDNA species, apparently corresponding to two splice variants of CASH. The proteins encoded by these two cDNAs shared the death effector domain-containing N-terminal region, but their C termini differed. One (CASHβ) had a short C terminus, corresponding to that of the originally cloned cDNA. The other (CASHα) had a long C terminus. The amino acid sequence in this longer C-terminal region showed rather high homology to those of the protease-precursor regions in CASP-8 and CASP-10 (Fig. 1). However, it lacked several of the residues believed to be crucial for protease activity, suggesting that the protein is devoid of cysteine protease activity. Interestingly, CASHα contains a caspase-substrate sequence at the site corresponding to the proteolytic-processing site within the protease regions in CASP-8 and CASP-10 (shaded in Fig. 1). Preliminary data suggest that CASHα can indeed be cleaved at this site by CASP-8. Based on the nucleotide sequence of an expressed sequence tag clone found to correspond to the mouse homologue of part of the DED region in CASH, we cloned the cDNAs of both the mouse CASHα and CASHβ splice variants from mouse liver mRNA by reverse transcriptase-PCR. Sequence comparison revealed high conservation throughout the CASHα molecule (71% identity in DED region and 59% in protease homology region), suggesting that both the DED and protease homology regions in the protein contribute to its function (Fig. 1). Two-hybrid testing of the interactive properties of CASHα and CASHβ (Fig. 2) revealed that both variants interact with MORT1/FADD and CASP-8, most probably through their shared DED regions. Notably, although initially cloned by two-hybrid screening for proteins that bind to CASP-10, CASHβ was found in this test to bind rather weakly to CASP-10, and CASHα did not bind to it at all. The two CASH variants also self-associated and bound to each other, but did not bind RIP or TRADD (adapter proteins that, like MORT1/FADD, contain death domains but lack DEDs), nor did they bind to a number of irrelevant proteins used as specificity controls. To examine the function of CASH, we expressed its two variants transiently in HeLa and 293-T cells and assessed the effects of the transfected proteins on the CD120a-induced signaling for cytotoxicity triggered by TNF or by overexpression of the receptor, as well as on the CD95-induced signaling for cytotoxicity triggered by antibody cross-linking of CD95 or by overexpression of a chimeric receptor comprised of the extracellular domain of CD120a and the intracellular domain of CD95 (Fig. 3). In both cell lines, expression of CASHβ by itself had no effect on cell viability, but it strongly inhibited the induction of cell death by CD120a as well as by CD95. Expression of the CASHα variant affected the two cell lines very differently. In HeLa cells it inhibited the cytotoxicity of CD120a and CD95, similarly to CASHβ. In the 293-T cells, however, it resulted in marked cytotoxicity. Similar cytotoxicity was observed when the protein was expressed in 293-EBNA cells or 293 cells (not shown). This cytotoxic effect could be completely blocked by coexpression of p35, a baculovirus-derived caspase inhibitor (23Clem R.J. Fechheimer M. Miller L.K. Science. 1991; 254: 1388-1390Crossref PubMed Scopus (708) Google Scholar, 24Xue D. Horvitz H.R. Nature. 1995; 377: 248-251Crossref PubMed Scopus (439) Google Scholar). To assess the contribution of the region of protease homology in CASHα to its cytocidal effect, we examined the functions of two mutants of the protein, CASHα(1–385) and CASHα(1–408), with C-terminal deletions at the region corresponding to that part of the protease domain from which the small subunit of the mature protease is derived. Both mutants were devoid of any cytotoxic effect. Moreover, like CASHβ they protected the 293 cells from death induction by CD120a and CD95 (Fig. 3 C). The above findings indicate that CASH can interact with components of the signaling complexes of CD120a and CD95 and that it affects death induction in a way that may differ depending on the identity of the splice variant of CASH and on the cell type in which it is expressed. The inhibition of cytotoxicity induction by CASHβ, and in the case of the HeLa cells also by CASHα, is apparently mediated by the DED region in this protein. It probably reflects competition of the DED of CASH with the corresponding regions in CASP-8 and CASP-10 for binding to MORT1/FADD. Less easy to explain is the way in which CASHα causes death of the 293 cells. The ability of the p35 protein to block this cytotoxic effect indicates that the cytotoxicity is mediated by the activity of caspases. Yet CASHα, even though displaying marked sequence homology to the caspases is unlikely to have cysteine-protease activity because it lacks several of the conserved caspase active site residues. A more likely explanation is that it acts by activating other molecules that do have caspase activity. An intriguing possibility is that CASHα, though unable to act alone as a protease, can still constitute part of an active protease molecule. Crystallographic studies of CASP-1 and CASP-3 structure indicate that the small and large protease subunits in each processed enzyme are derived from distinct proenzyme molecules (25Walker N.P. Talanian R.V. 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In view of the observed dependence of the CASHα cytotoxic activity on intactness of the region corresponding to the small protease subunit (Fig. 3 C), it is tempting to speculate that this region in CASHα can associate with the large subunit region of certain caspase(s) in a way that results in reconstitution of an enzymatically active molecule. The resulting active heterotetramer should then be capable of activating other caspases, thus triggering cell death. The discovery of CASP-8 and CASP-10 and of their association through MORT1/FADD with CD120a and CD95 (7Boldin M.P. Goncharov T.M. Goltsev Y.V. Wallach D. Cell. 1996; 85: 803-815Abstract Full Text Full Text PDF PubMed Scopus (2113) Google Scholar, 8Muzio M. Chinnaiyan A.M. Kischkel F.C. O'Rourke K. Shevchenko A. Ni J. Scaffidi C. Bretz J.D. Zhang M. Gentz R. Mann M. Krammer P.H. Peter M.E. Dixit V.M. Cell. 1996; 85: 817-827Abstract Full Text Full Text PDF PubMed Scopus (2743) Google Scholar, 13Vincent C. Dixit V.M. J. Biol. Chem. 1997; 272: 6578-6583Abstract Full Text Full Text PDF PubMed Scopus (240) Google Scholar) indicates a plausible mechanism for initiation of the death-inducing cascades by the two receptors. It does not, however, provide any clue to the cause of the marked variation in effectivity of death induction by these receptors, even among cells that express the receptors, their adapter proteins, and the caspases at similar levels. Nor does it explain the frequently observed differences in effectivity of death induction by the two receptors. CASH, through its effects on the signaling for death by CD120a and CD95, which vary depending on the identity of the CASH splice variant expressed and perhaps also on the identity of the specific caspases expressed in the cell, may well contribute to these variations in cytotoxicity induction. It should be stressed, however, that transfection studies such as those described here can provide only a partial view of the function of a protein. It is conceivable that at least part of the effects observed when expressing a protein in amounts far higher than its normal levels will turn out to be unrelated to its real function. Complementing these overexpression tests by assessing the effect of decreased expression of CASH, e.g. by deleting the CASH gene, should provide a more reliable notion of the physiological role of this protein. We thank Jacques Camonis for the Jurkat T cell two-hybrid library, Mark Boldin for advice, and Sveta Boldin and Giuseppina Cantarella for assistance.
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