STAT1 Is Inactivated by a Caspase*

Peter King and Stephen GoodbournDagger

From the Division of Biochemistry, Department of Cellular and Molecular Sciences, St. George's Hospital Medical School, University of London, London SW17 0RE, United Kingdom

    ABSTRACT
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Abstract
Introduction
Procedures
Results
Discussion
References

Apoptosis involves the activation of a cascade of interleukin-1beta converting enzyme-like proteases (caspases), a group of cysteine proteases related to the prototype interleukin-1beta -converting enzyme (caspase-1). These proteases cleave specific intracellular targets such as poly(ADP-ribose) polymerase, DNA-dependent protein kinase, and nuclear lamins. We show here that apoptosis can be induced by double-stranded RNA. The induction of apoptosis by double-stranded RNA and other agents leads to the cleavage by a caspase of the signal transducer and activator of transcription factor, STAT1 which is pivotal in the signal transduction pathways of the interferons and many other cytokines and growth factors. The product of this cleavage is no longer able to mediate interferon-activated signal transduction and the cleavage event may play a role in regulating the apoptosis response itself.

    INTRODUCTION
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Abstract
Introduction
Procedures
Results
Discussion
References

Apoptosis is the process of programmed cell death, and is a common occurrence in embryogenesis and in the destruction of infected, damaged, or senescent cells (1, 2). The biochemical processes involved in apoptosis can be divided into two discrete phases. A variable period of time elapses following exposure to apoptosis-inducing signals before cells become committed to undergo apoptosis. This phase is followed by the execution phase (more correctly a suicide phase, since apoptosis is cell autonomous) which, unlike the commitment phase, is irreversible. The execution phase is the best understood, and is characterized by changes in the cytoplasmic membrane, breakdown of the nuclear envelope, condensation of chromatin structure, and eventual destruction of the chromatin (laddering). Execution is associated with the activation of a family of cysteine-proteases (caspases) which are related to the enzyme required to process interleukin-1beta (IL-1beta )1 from its precursor form (IL-1beta -converting enzyme, caspase-1). It is not clear whether any single caspase can cause cell death, since these enzymes appear to be arranged in a complex network. Furthermore, to date, although several substrates have been identified for caspases, no single substrate cleavage has been shown to be essential for apoptosis, and the consensus of opinion is that cell death occurs "by a thousand cuts" (3).

In addition to activation through occupation of surface receptors such as Fas or tumor necrosis factor, apoptosis can also be induced by intracellular signals such as DNA damage, inhibition of protein synthesis, and viral infection. We are interested in the specific means by which viral infection can cause cells to undergo apoptosis (4). Apoptosis of virally infected cells is important since it allows macrophages to destroy a cell before the completion of the viral life cycle and the release of infectious particles (5). The significance of this is reflected by the fact that many viruses encode specific inhibitors of caspases (6-11). One of the best viral inducers of apoptosis is influenza (12-14). It has been proposed that double-stranded RNA (dsRNA) is generated during influenza viral replication, and that this leads to the transcriptional activation of Fas antigen that is a key factor in inducing apoptosis (15, 16).

In this paper we show that dsRNA is capable of inducing apoptosis without the requirement for de novo protein synthesis, indicating that susceptible cells contain a pre-existing pathway for the execution of apoptosis if exposed to dsRNA. This is highly reminiscent of the transcriptional induction of beta -interferon (beta -IFN) in response to viral infection or dsRNA treatment (17). While investigating the effects of this dsRNA-induced apoptosis on the induction of beta -IFN we discovered that the signal transducer and activator of transcription molecule, STAT1, becomes cleaved after aspartic acid 694 by a caspase. STAT1 is a transcription factor that becomes phosphorylated on tyrosine 701 by members of the JAK kinase family in response to IFNs and many other cytokines and growth factors (18-20); this phosphorylation is required for dimerization and subsequent DNA binding and is thus essential for effective signal transduction. The removal of the C terminus of STAT1 by proteolysis consequently renders STAT1 unable to participate in signal transduction. This cleavage is also caused by inducers of apoptosis other than dsRNA, and may play a role in the down-regulation of cellular responses during cell death.

    EXPERIMENTAL PROCEDURES
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Abstract
Introduction
Procedures
Results
Discussion
References

Cell Culture-- HeLa (subclone E (21)) and U3A (22) cells were grown in Dulbecco's modification of Eagle's medium supplemented with Glutamax (Life Technologies) + 10% fetal bovine serum (Life Technologies). For dsRNA treatments, HeLa cells were grown until they were 80-90% confluent, primed by treatment with 500 units/ml human alpha -IFN (Wellferon, a mixture of naturally produced alpha -IFN subtypes; Glaxo-Wellcome) for 18 h, and then induced using 100 µg/ml dsRNA (poly(I)-poly(C); Pharmacia) for the lengths of times shown in the figures. Where indicated, cycloheximide was added to the medium at 50 µg/ml, at this concentration, protein synthesis is inhibited to >99.9% as determined by incorporation of labeled amino acids into total protein (23). The caspase inhibitor ZVAD (benzyloxycarbonyl-Val-Ala-Asp-fluoromethylketone; Enzyme System Products) was dissolved in Me2SO and added to cells at 100 µM at the same time as dsRNA. TPCK (Sigma) was dissolved in methanol and added to cells at 100 µM at the same time as dsRNA. Etoposide was dissolved in Me2SO and added to cells for 18 h at 50 µM. IFN treatment of U3A cells used 500 units of human alpha -IFN/ml or 500 units of human gamma -IFN/ml for 3 h where indicated.

Western Blotting Analysis-- Cells were lysed in sample buffer (24) (500 µl/9 cm plate) and extracts (15 µl) were fractionated on 7.5% polyacrylamide/SDS gels. Gels were transferred to 0.45-µm polyvinylidene difluoride membranes (Pierce), blocked, incubated with specific antisera, and washed as recommended by the manufacturers. Experiments shown in this work used a polyclonal STAT1 antibody raised against the N-terminal 194 amino acids (Transduction Laboratories catalogue number G16930); we have also used monoclonal antibodies raised against the C terminus (Santa Cruz catalogue number sc-417) and an internal fragment (Transduction Laboratories catalogue number S21120) to characterize the STAT1* product (data not shown). STAT2, STAT3, and STAT6 antibodies were all monoclonal products raised against the respective N-terminal regions (Transduction Laboratories; catalogue numbers STAT2 = S21220; STAT3 = S21320; STAT6 = S25420) while the human PARP antibody was a rabbit polyclonal raised against a synthetic internal peptide (GVDEVAKKK; Upstate Biotechnology; catalogue number 06-557). The monoclonal antibody (MAbSV5-P-k) (25) recognizing amino acids 95-108 of the P and V proteins of simian virus 5 was obtained from Dr. R. Randall (University of St. Andrews). All protein-antibody interactions were detected with enhanced chemiluminescence (Amersham) using horseradish peroxidase-conjugated sheep anti-mouse (Amersham) and donkey anti-rabbit (Amersham) IgG as secondary antibodies for monoclonal and polyclonals, respectively. For re-probing, filters were stripped as described by the manufacturers.

Plasmid Construction-- A cDNA sequence for human STAT1alpha was obtained by polymerase chain reaction and verified by partial sequencing and functional complementation in U3A cells (see Fig. 4). This cDNA was inserted between the NcoI and XbaI sites of the EF1alpha promoter vector pEFplink2 (a kind gift of Dr. R. H. Treisman, Imperial Cancer Research Fund) to generate pEFSTAT1alpha . The STAT1alpha cDNA was then epitope-tagged at the N terminus using oligonucleotides encoding the amino acids 95-108 (GKPIPNPLLGLDST) of the P and V proteins of simian virus 5 to generate pEFSTAT1alpha SV5. Single amino acid changes to alanine or glutamic acid at aspartic acid 694 or to a stop codon at glycine 695 were introduced into pEFSTAT1alpha SV5 using recombinant polymerase chain reaction to generate pEFSTAT1alpha SV5(D694A), pEFSTAT1alpha SV5(D694E), and pEFSTAT1alpha SV5(G695/STOP), respectively. The amino acid changes were confirmed by sequencing. The wild type STAT1alpha sequence and STAT1alpha genes containing the D694A and G695/STOP changes were transferred from these plasmids into the vector pT7beta plink (26) as NcoI to XbaI fragments to generate pT7beta STAT1alpha , pT7beta STAT1alpha (D694A), and pT7beta STAT1alpha (G695/STOP), respectively. The reporter plasmid for alpha -IFN contained 4 copies of the 9-27 ISRE core (27) (AGGAAATAGAAACTG) arranged in tandem upstream of the BamHI site of ptkDelta (-39)lucter (21), while the reporter plasmid for gamma -IFN contained 2 copies of the IRF-1 GAS site (28) (TTTCCCCGAAA) arranged in tandem upstream of the BamHI site of ptkDelta (-39)lucter.

Transfections-- HeLa cells were transfected with 2 µg of DNA and 8 µl of LipofectAMINE (Life Technologies Inc.) according to the manufacturers instructions. U3A cells were transfected using calcium phosphate precipitation with 10 µg of effector, 10 µg of reporter, and 2 µg of transfection control plasmid (pSV2CAT (29)). For reporter gene assays, lysates were prepared and assayed for luciferase and chloramphenicol acetyltransferase activity as described previously (21). Luciferase activity was corrected to the chloramphenicol acetyltransferase activity to normalize for variations in the transfection efficiency. Transfection experiments were repeated at least three times.

Apoptosis Assay-- Laddered cytoplasmic DNA was prepared from Triton X-100 lysates and labeled with [alpha -32P]dATP using the terminal transferase activity of Taq DNA polymerase (30). Reaction products were fractionated by electrophoresis on 1.8% agarose gels in 0.089 M Trisborate, 0.002 M EDTA, and after drying the gel, visualized by autoradiography.

In Vitro Cleavage Assay-- Bacterial lysates were prepared from Escherichia coli BL21.DE3pLysS carrying a pET plasmid encoding recombinant caspase-3 (kindly provided by Dr. N. McCarthy, ICRF) or the control plasmid pET15b, as described previously (31). One microgram of lysate was incubated with 1 µl of [35S]methionine-labeled STAT1alpha or mutant forms of STAT1alpha (prepared by in vitro translation of linearized pT7beta STAT1alpha , pT7beta STAT1alpha (D694A), or pT7beta STAT1alpha (G695/STOP) in a standard TnT T7 quick coupled transcription/translation kit reaction; Promega Corp.), in a 10-µl reaction containing 25 mM Hepes, pH 7.5, 5 mM dithiothreitol, 5 mM EDTA, 0.1% CHAPS at 37 °C for 1 h. The reactions were stopped by the addition of sample buffer (24) then analyzed by fractionation on a 7.5% polyacrylamide/SDS gel followed by autoradiography.

    RESULTS
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Abstract
Introduction
Procedures
Results
Discussion
References

We have previously shown that beta -IFN expression can be induced in HeLa cells in response to treatment with dsRNA (21, 23). Induction occurs at the level of transcriptional initiation and does not require new protein synthesis, although the extent of induction can be much enhanced by a pretreatment with type I IFN (priming). We noted that during the induction process, cells exhibited an altered morphology consistent with the activation of apoptosis. To determine whether apoptosis could be induced by dsRNA, we treated HeLa cells with poly(I)-poly(C), which was added directly to the growth medium, and prepared DNA from induced cells. Fig. 1 shows that a nucleosomal ladder characteristic of cells undergoing apoptosis is produced in response to dsRNA. When cycloheximide was included in the induction medium the degree of laddering was significantly enhanced, although consistent with results in other systems cycloheximide alone could cause some laddering (32-36). Although it is not possible to determine from these results whether dsRNA and cycloheximide induce apoptosis through a common mechanism, the fact that the extent of apoptosis seen with the combination of dsRNA and cycloheximide is greater than that seen with either inducer alone demonstrates that cycloheximide cannot be blocking the dsRNA effect. Thus de novo protein synthesis cannot be required for the induction of apoptosis by dsRNA, a result that is consistent with the recent observations of others (37). Inclusion of the caspase inhibitor ZVAD (38) in the induction mixture prevented DNA laddering (Fig. 1) and completely blocked the observed cell death (data not shown).


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Fig. 1.   Double-stranded RNA can induce apoptosis in HeLa cells. Cytoplasmic extracts were prepared from HeLa cells treated as indicated and were assayed for DNA laddering. The migration of molecular weight markers are indicated to the left of the panel and are given in base pairs. CHX, cycloheximide.

HeLa cells contain two splice variant forms of STAT1, referred to as STAT1alpha (91 kDa) and STAT1beta (84 kDa), respectively (Fig. 2A). While investigating the role of STAT1 in the induction of beta -IFN expression we discovered that exposure of HeLa cells to dsRNA for 2 h generated a novel form of STAT1 (STAT1*), migrating with slightly faster mobility than the 84-kDa form (STAT1beta ; Fig. 2A). Since the production of STAT1* occurs with similar kinetics to the activation of apoptosis, we investigated whether STAT1* generation was associated with the activation of caspases. To determine whether the production of STAT1* required de novo protein synthesis, we repeated the induction of HeLa cells with dsRNA in the presence of cycloheximide. Although cycloheximide alone could also generate STAT1* to some degree, the combined treatment of HeLa cells with dsRNA and cycloheximide led to enhanced production of STAT1* (Fig. 2B) and was accompanied by the loss of both STAT1alpha and -beta . These results suggested that STAT1* is derived from STAT1alpha and -beta by post-translational modification. To determine whether other members of the STAT family are similarly affected we examined the state of STAT2 and STAT3 (Fig. 2C) and STAT6 (data not shown) in extracts from dsRNA- and cycloheximide-treated HeLa cells without seeing equivalent changes in mobility. By contrast, the well defined caspase substrate, PARP, is cleaved under the same conditions (Fig. 2C).


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Fig. 2.   A post-translationally modified form of STAT1 (STAT1*) is generated in response to apoptosis. A, HeLa cells were treated with dsRNA for the times indicated and cell extracts analyzed for STAT1 using Western blotting. In addition to STAT1alpha and STAT1beta , a novel form of STAT1 (STAT1*) is detected in dsRNA-treated cells. By probing similar blots with additional STAT1-specific antisera, STAT1* can be shown to lack the C terminus of STAT1alpha and STAT1beta (data not shown). B, HeLa cells were treated with dsRNA or cycloheximide (CHX) alone or in combination for 3 h and cell extracts analyzed for STAT1 using Western blotting. C, HeLa cells were treated with dsRNA and cycloheximide in combination for the indicated times and cell extracts analyzed for STAT1, STAT2, STAT3, or PARP using Western blotting. D, HeLa cells were treated with dsRNA and cycloheximide in combination for 3 h in the presence of ZVAD or TPCK (left panel), or were treated with etoposide (right panel) and cell extracts analyzed for STAT1 using Western blotting.

Fig. 2D shows that STAT1* generation in cells treated with dsRNA and cycloheximide could be completely blocked by treating cells with the caspase inhibitor ZVAD, whereas the serine protease inhibitor, TPCK, was unable to affect cleavage. By contrast, TPCK completely inhibited dsRNA-dependent activation of NF-kappa B under the same conditions (39), while ZVAD had no effect (data not shown). The cleavage of PARP was similarly blocked by ZVAD but not by TPCK (data not shown). To test whether STAT1* could be generated by other inducers of apoptosis, we treated HeLa cells with the DNA topoisomerase II inhibitor etoposide (40). This treatment also resulted in the production of STAT1*, although we note that this treatment reproducibly leads to preferential cleavage of STAT1beta over STAT1alpha (Fig. 2D). Taken together, these results indicate that the dsRNA/cycloheximide induction mixture triggers apoptosis in HeLa cells and that during this process STAT1alpha and -beta are converted to a shorter form, presumably by proteolytic cleavage.

Because STAT1alpha and -beta differ at their C termini, but are converted to a single product, it seemed likely that STAT1* is generated by a single cleavage event occurring near the C terminus of the protein. By using a panel of antibodies we were able to show that STAT1* lacks the C-terminal end of STAT1alpha and -beta (data not shown). Since a caspase-mediated cleavage was strongly implicated by the above data, we inspected the C-terminal end of the human STAT1 protein sequence for an appropriate motif. We noticed a potential cleavage site for caspases at the aspartic acid residue at position 694 (Fig. 3A). Cleavage at this site in STAT1 would produce a species with a predicted molecular mass of 81 kDa, in line with the observed size of STAT1*. To verify that this sequence was indeed a target for cleavage, we created an epitope-tagged wild type STAT1alpha expression vector, and ones in which the aspartic acid residue at position 694 was changed to alanine (D694A) or glutamic acid (D694E). When the epitope-tagged wild type form of STAT1alpha was expressed in HeLa cells, a protein with mobility similar to that of the endogenous form of STAT1alpha (91 kDa) could be observed (Fig. 3B). A small amount of a protein with similar mobility to STAT1* (81 kDa, Fig. 3B) could also be observed in untreated cells; this product is generated as a result of a low level of apoptosis induced by the transfection conditions, and can be blocked with ZVAD (data not shown). When cells were treated with dsRNA and cycloheximide the conversion of the 91- to the 81-kDa truncation form was much enhanced (Fig. 3B). The 81-kDa form migrated with the same mobility as a protein produced by expression of a form of STAT1alpha truncated after amino acid 694 (G695/STOP) (Fig. 3B), as expected if STAT1* is generated by cleavage at this site. In contrast to the wild type form, the D694A and D694E mutant forms of STAT1alpha were not cleaved upon induction (Fig. 3B). Reprobing the Western blot with the STAT1 antibody showed that the endogenous STAT1alpha and -beta were cleaved in each case (Fig. 3B). These results confirmed the presence of a cleavage site at aspartic acid 694 in STAT1, and demonstrated that this site is cleaved in both STAT1alpha and -beta during apoptosis. To confirm that STAT1 can be cleaved by a caspase, we tested whether recombinant STAT1 can be cleaved by recombinant caspase-3 since the cleavage site in STAT1 is similar to that seen in several caspase-3 substrates (Fig. 3A). Fig. 4 demonstrates that the 91-kDa STAT1 protein is cleaved by caspase-3 to give an 81-kDa product that has the same mobility as STAT1alpha truncated after amino acid 694 (G695/STOP). This cleavage is not seen with control extracts, nor if the aspartic acid residue in the caspase cleavage consensus site was changed to alanine (D694A).


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Fig. 3.   STAT1* is generated by cleaving STAT1 at a consensus site for a caspase. A, amino acid sequences of the C-terminal regions of STAT proteins. Proteins are aligned with respect to the signal-activated tyrosine residue (asterisk). Sequences for human STAT1, STAT2, STAT3, mouse (m)STAT4, and human STAT6 have been previously aligned (41); human STAT5B is from Ref. 42. Amino acid residues in shaded boxes indicate identity with human STAT1. The aspartic acid at amino acid 694 in STAT1 (arrow) resides within a consensus motif for caspases as indicated in the lower alignment with known substrates: PARP (43); DNA-PK, DNA-dependent protein kinase (44); DSEB/RF-C140, DNA replication complex C, large subunit (45); SREBP1a and SREBP2, sterol regulatory element-binding proteins (46); PITSLREalpha 2-1 Cdc2-like kinase (47); Rb, human retinoblastoma protein (48); Pro-IL-1beta , pro-interleukin-1beta (49, 50); Pro-IGIF, pro-gamma -IFN-inducing factor (51, 52). B, N terminally-tagged STAT1alpha , and amino acid substitution derivatives, were expressed in HeLa cells. Extracts from cells treated as indicated were analyzed using a tag-specific antibody (top panel). The blot was reprobed with a STAT1-specific antibody (middle panel). The lower panel shows the sequence of STAT1 and the substituted forms (aspartic acid at amino acid 694 is indicated by an arrow).


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Fig. 4.   STAT1alpha can be cleaved by recombinant caspase-3. [35S]Methionine-labeled STAT1alpha , STAT1alpha with an aspartic acid to alanine change in the caspase cleavage consensus at amino acid 694 (D694A), or STAT1alpha truncated after amino acid 695 (G695/STOP) were incubated with a control extract or recombinant caspase-3 as indicated. The positions of intact STAT1alpha (91 kDa) and the 81-kDa cleavage product are indicated to the left of the panel.

Activation of STAT1 by alpha - and gamma -IFN, by cytokines such as IL-6 and growth factors such as platelet-derived growth factor, involves a single phosphorylation on tyrosine 701 (19), and for maximal activity, serine 727 (53). Once phosphorylated, STAT1 can homo- or heterodimerize to produce complexes capable of binding to DNA and activating transcription (19). Clearly, cleavage of STAT1 after amino acid 694 would produce a truncated form of the protein that cannot be phosphorylated on tyrosine 701, and thus should not be activated by alpha - or gamma -IFN. To test this, we examined the ability of STAT1* to rescue responses to alpha - and gamma -IFN in U3A cells which lack functional STAT1 (54). Responses to alpha -IFN were assessed using a reporter promoter containing a 15-mer "core" sequence that is a strong binding site for the type I-IFN-activated transcription factor ISGF3 (IFN stimulatable response element (55, 56)), while responses to gamma -IFN were assessed using a reporter promoter containing a GAS site from the IRF-1 promoter that is a strong binding site for the gamma -IFN-activated factor (GAF). In contrast to wild-type STAT1, the truncated form (G695/STOP) was completely unable to rescue either alpha -IFN (Fig. 5A) or gamma -IFN (Fig. 5B) responses. Altering amino acid 694 from an aspartic acid to an alanine (D694A) did not interfere with either signal transduction pathway (Fig. 5, A and B). These results demonstrate that the effect of the proteolytic cleavage of STAT1 during apoptosis would be to impair the ability of cells undergoing apoptosis to respond to a variety of cytokine- and growth factor-mediated signals.


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Fig. 5.   STAT1* is unable to sustain signal transduction responses to type I or type II IFN. U3A cells were transiently transfected with expressing plasmids for STAT1alpha or amino acid substitution derivatives and reporter constructs for either an alpha -IFN response (A) or a gamma -IFN response (B). Extracts were made after IFN treatment and gene expression was determined by reporter enzyme assays.

    DISCUSSION
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Abstract
Introduction
Procedures
Results
Discussion
References

The data we have presented indicate that cells contain a dsRNA-sensitive switch which triggers a pre-established program of both apoptosis and beta -IFN production. In neither case is concurrent protein synthesis required, and as a result there must be a means by which dsRNA can activate the caspases. Studies on the Fas and tumor necrosis factor receptors indicate that upon activation the receptors recruit adaptor molecules through cytoplasmic "death domains" (57-60); these adaptors in turn recruit additional molecules which contain caspase motifs (61-63). Once recruited these molecules activate the downstream caspase cascade. One possible candidate for the mediation of the dsRNA signal is the cellular enzyme protein kinase R (PKR). This kinase is known to function to down-regulate protein synthesis in virally infected cells by phosphorylating the translational initiation factor eukaryotic initiation factor-2alpha (64), but has also been shown to play a role in the activation of NF-kappa B by dsRNA (65-68). It is tempting to speculate that PKR may also signal to the apoptotic execution machinery. Consistent with this it has been shown that overexpression of PKR can cause apoptosis in cell culture (69), while mouse embryonic fibroblasts lacking PKR are unable to undergo apoptosis in response to dsRNA (37). Interestingly, PKR deficiency also impairs responses to other inducers of apoptosis (37, 70). The identification of a link between PKR and the caspases represents a significant future goal.

In these studies we have also demonstrated that the transcription factor STAT1, which is required for the ability of cells to respond to a wide variety of signals, is cleaved during apoptosis by a caspase. The protease inhibitor ZVAD used in our studies is a general caspase inhibitor (38), and we have yet to identify which specific member(s) of the caspase family is involved in generating STAT1* in vivo, although we have demonstrated that caspase-3 can cleave STAT1 efficiently in vitro. Although the cleavage site in STAT1 has a number of similarities to the sites known to be substrates for caspase-3 (Fig. 3A), we note that it also has some similarity with substrates for caspase-1, especially the minor caspase-1 cleavage product of pro-IL-1beta (49, 50). While we have yet to test it directly, we speculate that STAT1 may also be a caspase-1 substrate, since caspase-1 appears to be rather promiscuous in its preferences (71-73). It is also interesting to note that STAT1 is not cleaved at amino acid 143 despite containing an ELDS motif in this region, and that STAT3 and STAT6 are also refractory to cleavage despite containing possible caspase cleavage sites (Fig. 3A). We speculate that cleavage by caspases could be prevented by the tertiary structure of some proteins.

The C-terminal cleavage product of STAT1 has lost the tyrosine residue at position 701 and thus cannot be activated by alpha - and gamma -IFN as shown here, or presumably by the other ligands that activate by promoting this phosphorylation. It is pertinent to ask what role STAT1 inactivation could play in the apoptotic response. It has previously been observed that many cell types, including fibroblast (74) and hematopoeitic cells (75) can undergo apoptosis as a result of becoming depleted of growth factors or cytokines and can be rescued by the addition of defined survival factors, which include STAT1 activators such as platelet-derived growth factor (74), colony-stimulating factor (76), and gamma -IFN (77). It is interesting to speculate that one consequence of apoptosis is to down-regulate the ability of a cell to respond to such factors. Since multiple growth factors can protect cells against apoptosis, we think it unlikely that STAT1 cleavage alone would be sufficient to render cells insensitive to protection by survival factors. Nevertheless, inactivation of STAT1 function may be an example of a class of modifications that ensures that the commitment phase of apoptosis is irreversible. An alternative role for STAT1 cleavage is suggested by the recent demonstration that STAT1 can play a role in apoptosis by up-regulating the level of caspase-1 in response to cytokines (78). Consistent with this we have determined that the degree of apoptotic death we observe in response to dsRNA and cycloheximide is much enhanced if cells are primed by a prior exposure to either type I or type II IFN (data not shown). When cells are challenged with an apoptosis-inducing signal, the inactivation of STAT1 would lower the levels of caspase, and thus might play a role in limiting the propensity of a cell to undergo apoptosis. The resolution of this issue awaits further study.

    ACKNOWLEDGEMENTS

We thank George Stark and Ian Kerr for U3A cells, Di Watling for Wellferon and gamma -IFN, Richard Treisman for the pEFplink2 plasmid, Rick Randall for MAbSV5-P-k, Victoria Heaton for etoposide, Nichola McCarthy for pETCPP32 and helpful discussions, and Mike Westby, Jo Brown, and David Slack for comments on the manuscript.

    FOOTNOTES

* This work was supported by a Wellcome Trust University Award.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Dagger To whom correspondence should be addressed: Div. of Biochemistry, Dept. of Cellular and Molecular Sciences, St. George's Hospital Medical School, University of London, London SW17 0RE, United Kingdom. Tel: 44-181-725-5942; Fax: 44-181-725-2992; E-mail: s.goodbourn{at}sghms.ac.uk.

1 The abbreviations used are: IL, interleukin; STAT, signal transducer and activator of transcription; PARP, poly(ADP-ribose) polymerase; IFN, interferon; TPCK, Nalpha -p-tosyl-L-phenylalanine chloromethyl ketone; dsRNA, double-stranded RNA; PKR, protein kinase R; ZVAD, benzyloxycarbonyl-Val-Ala-Asp-fluoromethylketone; CHAPS,3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonic acid.

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Abstract
Introduction
Procedures
Results
Discussion
References

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