Viral Oncoproteins Discriminate between p53 and the p53 Homolog p73

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Molecular and Cellular Biology, November 1998, p. 6316-6324, Vol. 18, No. 11
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Viral Oncoproteins Discriminate between p53 and the p53 Homolog p73

Maria Carmen Marin,¹ Christine A. Jost,¹ Meredith S. Irwin,¹ James A. DeCaprio,¹ Daniel Caput,² and William G. Kaelin Jr.¹^,³^,^*

Dana-Farber Cancer Institute and Harvard Medical School¹ and Howard Hughes Medical Institute,³ Boston, Massachusetts 02115, and Sanofi Recherche, Labege, France²

Received 30 April 1998/Returned for modification 11 June 1998/Accepted 27 July 1998

	ABSTRACT

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p73 is a recently identified member of the p53 family. Previously it was shown that p73 can, when overproduced in p53-defectivetumor cells, activate p53-responsive promoters and induce apoptosis.In this report we describe the generation of anti-p73 monoclonalantibodies and confirm that two previously described p73 isoformsare produced in mammalian cells. Furthermore, we show that thesetwo isoforms can bind to canonical p53 DNA-binding sites in electrophoreticmobility shift assays. Despite the high degree of similarity betweenp53 and p73, we found that adenovirus E1B 55K, simian virus 40T, and human papillomavirus E6 do not physically interact withp73. The observation that viral oncoproteins discriminate betweenp53 and p73 suggests that the functions of these two proteinsmay differ under physiological conditions. Furthermore, they suggestthat inactivation of p73 may not be required for transformation.

	INTRODUCTION

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p53 is the most frequently mutated human tumor suppressor gene identified to date. In model systems, restoration of p53 functionin tumor cells leads either to a cell cycle block or to apoptosis.These activities have been linked to the ability of p53 to bindto specific DNA sequences and activate transcription. Among thegenes that are activated by p53 are the cyclin-dependent kinaseinhibitor p21 and a family of genes involved in oxidative stress(10, 36).

Recently, Kaghad et al. serendipitously identified a cDNA encoding a novel p53-like protein (22). The protein, called p73,is approximately 60% identical to p53 in the region correspondingto the p53 DNA-binding domain. Furthermore, all of the residuesthat contact DNA in the p53-DNA crystal structure are conservedin p73 (7). In addition, the N terminus of p73 is similar (~25%identity) to the N-terminal transactivation domain of p53, andthe C terminus of p73 contains a region which is comparably similarto a C-terminal oligomerization domain within p53 (34, 44,48). Finally, the genomic organizations of p53 and p73 are highlysimilar, suggesting that they have a common ancestry (22). Inkeeping with this high degree of similarity, p73 can, at leastwhen overproduced, activate transcription from p53-responsivepromoters and induce tumor cell apoptosis (20, 22).

The p73 gene maps to chromosome 1p36, a region that is frequently deleted in a variety of human cancers (22). Nonetheless,to date no mutations have been identified in the remaining p73allele in such tumors. Thus, p73, unlike many tumor suppressorgene products such as the retinoblastoma protein (pRB) and p53,does not appear to conform to a two-hit model of tumorigenesis.It has been suggested that this may be due to epigenetic silencingof the p73 allele retained in tumors (22). Alternatively, itis possible that p73 is not a tumor suppressor gene product andis not the relevant target of 1p36 deletions.

A number of unrelated DNA tumor viruses can inactivate pRB. Inactivation of pRB leads to derepression of E2F-responsive promoters,which, in turn, allows quiescent cells to enter S phase. In modelsystems, untimely derepression of E2F-responsive promoters canalso lead to both p53-dependent and p53-independent apoptosis(17, 25, 35, 37, 43, 50). These viruses, however,encode a variety of antiapoptotic proteins. For example, polyomaviruses,papillomaviruses, and adenoviruses encode T, E6, and E1B 55K proteins,respectively, which bind to and inactivate p53 (1, 3, 8,11, 16, 19, 26, 30, 32, 40, 42, 49, 51). Indeed,p53 was first identified as a cellular T-binding protein (26,30). In this manner, the host DNA replication machinery is usurpedfor viral replication.

T, E6, and E1B each target different regions of p53. T binds to p53's core DNA-binding domain (27, 38), whereas E1B 55Kbinds to, and silences, p53's N-terminal transactivation domain(4, 23, 29, 51). E6 interacts with p53's core DNA-bindingdomain and C terminus and targets p53 for ubiquitin-dependentproteolysis (28, 31, 32, 39, 40). In short, viral oncoproteinshave been valuable reagents for studying the structure and functionsof p53. Given the apparent similarity of p53 and p73, we askedwhether viral oncoproteins that inactivate p53 were likewise capableof inactivating p73. Surprisingly, none of these viral oncoproteinsinteract with p73. Thus, small DNA tumor viruses can discriminatebetween p53 and p73.

	MATERIALS AND METHODS

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Cell lines and transfections. SK-N-SH, SK-N-AS, SK-N-DZ, and IMR-32 neuroblastoma cells, SK-N-MC neuroepithelioma cells, and IM-9 myeloma cells were obtainedfrom the American Type Culture Collection (Rockville, Md.) andwere grown in RPMI 1640 supplemented with 10% heat-inactivatedfetal bovine serum at 37°C in the presence of 10% CO₂. COS monkeykidney cells, 293 human embryonic kidney cells, and SAOS2 osteosarcomacells were from the laboratory stocks of David Livingston andwere maintained in Dulbecco's modified Eagle medium supplementedwith 10% fetal bovine serum at 37°C in the presence of 10% CO₂.Transfections were performed by the N,N-bis(2-hydroxyethyl)-2-aminoethanesulfonicacid (BES)-buffered saline (BBS) method as described earlier (21).Briefly, cells growing in monolayers were transfected when approximately70 to 80% confluent with 20 to 30 µg of plasmid DNA. The DNA precipitateswere removed 18 h later and the cells were fed fresh medium. Proteinand reporter assays were performed 24 h later.

Plasmids. The mammalian expression plasmids encoding hemagglutinin (HA)-tagged versions of simian p73 $alpha$ and p73 $beta$ were described earlier(20). The human p53 cDNAs in pGEX2T-p53 (wild type) and pGEX2T-p53(135Tyr) (18) (gifts of John Huibregtse and Peter Howley) wereexcised by digestion with BamHI and EcoRI and ligated into pcDNA3-HAthat had been cut with these two enzymes to make pcDNA3-HAp53and pcDNA3-HAp53(135Tyr), respectively.

The mammalian expression plasmid pSG5-T was described previously (52). pSG5-T(dl357-370), a gift of Herta Chao, was madeby replacing the PflMI-PstI cDNA fragment in pSG5-T, containingthe wild-type p53-binding site, with the corresponding fragmentfrom a cDNA encoding T dl357-370 (24), which contains a mutantp53-binding site. pGEX2T-E6 was a gift of Peter Howley. pGEX2T-E4(ORF 6/7) was a gift of Joseph Nevins. 2XRGC-CAT was a gift ofErik Flemington and was described previously (20). pRcCMV-HAp51Awas a gift of Shuntaro Ikawa (33). The corresponding p51 isoformresembles p73 $beta$ .

Antibodies. Monoclonal antibodies were generated by standard techniques (14). RBF/DNJ (BnR) mice were immunized with either glutathioneS-transferase (GST)-p73 $alpha$ (amino acids [aa] 380 to 637) for theER antibodies or GST-p73 $beta$ (aa 380 to 499) for the GC antibodies.The antibodies were screened based on their ability to immunoprecipitate³⁵S-radiolabelled p73 ( $alpha$ and $beta$ ) translation products and their abilityto detect the original GST immunogens by Western blot analysis.ER13, ER15, and GC15 were selected for further characterizationas described in Results.

Murine monoclonal anti-HA (12CA5) was obtained from Boehringer Mannheim. Murine monoclonal anti-T (PAb419) (13) and monoclonalanti-p53 (PAb421) hybridoma cells were a gift from Ed Harlow.Hybridoma supernatants were prepared by standard techniques (14).

Purified anti-p53 PAb1801 (Ab-2) murine monoclonal antibody was obtained from Oncogene Science. Purified anti-adenovirus type5 E1B 55K (Ab-1) rat monoclonal antibody was obtained from Calbiotech.Purified rabbit anti-HA (Y11) antiserum was obtained from SantaCruz.

Immunoprecipitation and immunoblot analysis. To detect endogenous p73, cells growing in monolayers were removed from plastic dishes by scraping and collected, along withfloating cells, by centrifugation. The cells were then washedonce with ice-cold phosphate-buffered saline and lysed, exceptwhere indicated, in EBC buffer (50 mM Tris [pH 8.0], 120 mM NaCl,0.5% Nonidet P-40) supplemented with aprotonin (11.5 µg/ml), phenylmethylsulfonylfluoride (50 µg/ml), NaF (100 mM), and Na orthovanadate (0.2 mM).In some experiments the cells were lysed in Triton 1% buffer (25mM Tris [pH 7.4], 25 mM NaCl, 1% Triton X-100) or radioimmunoprecipitationassay buffer (50 mM Tris [pH 8.0], 150 mM NaCl, 1.0% Nonidet P-40,0.5% deoxycholate, 0.1% sodium dodecyl sulfate [SDS]) supplementedwith the same inhibitors. For some transfection experiments, cellswere lysed directly in EBC buffer without scraping. Lysates wereclarified by centrifugation at 14,000 × g for 15 min at 4°C. Proteinconcentrations were determined by the Bradford method.

For immunoblot analysis, proteins were resolved by SDS-polyacrylamide gel electrophoresis and transferred to nitrocellulose(Bio-Rad). The filters were blocked in TBST (10 mM Tris [pH 8.0],150 mM NaCl, 0.05% Tween 20 [Sigma]) supplemented with 5% (wt/vol)powdered milk for 1 h at room temperature and then incubated withprimary antibody. Anti-p73 hybridoma supernatants were used ata dilutions of 1:50 to 1:100 (vol/vol) overnight at 4°C. Anti-HA(12CA5) hybridoma supernatant was used at a dilution of 1:50 (vol/vol)for 1 h at room temperature. Anti-p53 (PAb421) hybridoma supernatantwas used at a dilution of 1:100 (vol/vol) overnight at 4°C. Purifiedanti-p53 (Ab-2) was used at a dilution of 1:1,000 (vol/vol) for1 h at room temperature. The filters were then washed three timeswith TBST at room temperature and incubated with a horseradishperoxidase-conjugated goat antimouse antibody (Pierce) diluted1:5,000 (vol/vol) in TBST supplemented with 2% (wt/vol) powderedmilk and 1% goat serum for 1 h at room temperature. The filterswere then washed three times with TBST, and bound secondary antibodywas detected by enhanced chemiluminescence with Supersignal (Pierce)according to the manufacturer's protocol.

For the experiments depicted in Fig. 3A and 6A, monoclonal antibodies were directly coupled to protein A-Sepharose prior toimmunoprecipitation as described elsewhere (14). Briefly, hybridomasupernatants were incubated overnight at 4°C with protein A-Sepharosethat had been preequilibrated in 50 mM Tris (pH 8.0)-150 mM NaCl-5mM EDTA, 0.1% Nonidet P-40. The Sepharose was then resuspendedin 0.1 M sodium borate (pH 9.0) containing 40 mM dimethylpimelimidate.Following a 1-h incubation at room temperature, the reaction wasstopped by resuspending the Sepharose in 40 mM ethanolamine in0.1 M sodium borate (pH 8.0). One hour later, the Sepharose waswashed with NETN (20 mM Tris [pH 8.0], 100 mM NaCl, 1 mM EDTA,0.5% Nonidet P-40) and stored in NETN with 0.01% merthiolate.Aliquots of Sepharose containing approximately 1 µg of coupledantibody were used per immunoprecipitation reaction.

To immunoprecipitate endogenous p73, approximately 1 mg of EBC cell extract was incubated with 50 µl of anti-p73 or anti-Thybridoma supernatant, 1 µg of rat monoclonal anti-E1B, or 1 µgof anti-p53 (Ab-2). To immunoprecipitate ectopically producedproteins, 250 µl of EBC extract, corresponding to approximatelyone-half of the cells grown in a nearly confluent 100-mm-diameterdish, was incubated with 50 µl of anti-HA or anti-T hybridomasupernatant, 1 µg of anti-HA rabbit polyclonal antibody (SantaCruz), or 1 µg of anti-E1B monoclonal antibody. Immunoprecipitationof in vitro translation products was performed with 5 µl of invitro translation product and 50 µl of hybridoma supernatant in500 µl of NETN. In some experiments the in vitro translation productswere first denatured by boiling in 50 µl of 2% SDS-50 mM Tris(pH 8.0). Immunoprecipitates were collected on protein A-Sepharose,washed five times with NETN, and eluted by boiling in SDS-containingsample buffer.

In vitro translation. In vitro translation was performed with the TNT translation system (Promega) according to the manufacturer's protocol.

Electrophoretic mobility shift assay. A 23-mer oligonucleotide corresponding to a wild-type (5'-AGCTTAGGCATGTCTAGGCATGTCTA-3') p53 DNA-binding site (10) was synthesized,annealed to a complementary synthetic oligonucleotide in vitro,and radiolabelled with [ $gamma$ -³²P]ATP by using polynucleotide kinase (New England Biolabs). DNAbinding reactions were performed in 20 µl containing 2 µl of theindicated protein in vitro translation product (or unprogrammedreticulocyte lysate), 10 µl of 2× DNA binding buffer (50 mM Tris[pH 7.5], 40% glycerol, 100 mM KCl, 100 mM dithiothreitol, 2 mgof bovine serum albumin per ml, and 0.2% [vol/vol] Triton X-100),1 ng of radiolabelled p53 DNA-binding site, and 300 ng of salmonsperm DNA. Where indicated, 40 ng of nonlabelled wild-type orsequence-scrambled (sense strand, 5'-CCAGCTAGCAGGCAGCATCAGTACTT)duplex oligonucleotides was added as specific and nonspecificcompetitors, respectively. Antibody supershift experiments wereperformed by adding 2 µl of a 1:10 (vol/vol) dilution of the indicatedhybridoma supernatant. Binding reaction mixtures were incubatedfor 15 min at room temperature and then resolved by electrophoresisat 4°C in a 4% nondenaturing polyacrylamide gel containing 0.5×Tris-borate-EDTA buffer. Electrophoresis was conducted for 2 to3 h at 200 V. The gels were then dried and exposed to film at $-$ 70°C with an intensifying screen.

p53 degradation assay. The E6 destruction and GST-E6 binding assays were performed as described elsewhere (1, 31, 40).

CAT assay. SAOS2 cells were transiently transfected with 5 µg of reporter plasmid, 2 µg of pCMV- $beta$ gal, 0.5 µg of p73 or p53 expressionplasmid, and 10 µg of wild-type or mutant large-T-antigen plasmid.The total amount of DNA was brought up to 24 µg with pRcCMV carrierplasmid (Invitrogen). At 48 h after transfection, chloramphenicolacetyltransferase (CAT) assays were performed as described previously(21).

	RESULTS

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In order to study the p73 protein, we generated monoclonal anti-p73 antibodies. Two alternatively spliced p73 mRNA isoforms,designated p73 $alpha$ and p73 $beta$ , were identified by Kaghad et al. (22).The p73 $beta$ isoform lacks exon 13. Consequently, p73 $beta$ contains aframeshift and terminates prematurely after the addition of a5-aa sequence not present in the alpha isoform. Bacterial expressionplasmids that encoded GST fused to the C terminus of either simianp73 $alpha$ or p73 $beta$ were made (Fig. 1). These fusion proteins, whichwere designed so as to minimize the likelihood of generating antibodiesthat would cross-react with p53, were then used to immunize mice.Hybridomas were generated by standard techniques, and monoclonalantibodies were screened based on their ability to immunoprecipitatep73, but not p53, in vitro translation products. At least threesuch monoclonal anti-p73 antibodies, named ER13, ER15, and GC15,were identified in this fashion.

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FIG. 1. GST-p73 fusion proteins used to generate monoclonal antibodies. Shown schematically are p53, p73 $alpha$ , and p73 $beta$ . Mice were immunized with GST fused to either the C terminus of p73 $alpha$ (ER mice) or the C terminus of p73 $beta$ (GC mice). The p73 $beta$ cDNA lacks exon 13, resulting in a frameshift at residue 495. p73 $beta$ therefore contains five residues (black box) not present in p73 $alpha$ .

ER13 bound to p73 $alpha$ , but not p73 $beta$ , in immunoprecipitation and immunoblot assays (Fig. 2A and D), suggesting that the ER13 epitopeis located within the C-terminal region that is unique to p73 $alpha$ (Fig. 1). Of note, however, ER13 did immunoprecipitate p73 $beta$ inthe presence of p73 $alpha$ under native, but not denaturing, conditions(Fig. 2B [compare lanes 3 and 7] and 3 and data not shown). Thissuggests that p73 $alpha$ and p73 $beta$ can heterodimerize in solution. ER15and GC15 bound to both p73 $alpha$ and p73 $beta$ in immunoprecipitation andimmunoblot assays (Fig. 2A and D). The ability of GC15 to immunoprecipitatep73 $alpha$ , however, was diminished under denaturing conditions (Fig.2A, compare lanes 6 and 10). This, coupled with the differentband patterns observed in the immunoblot assays shown in Fig.2D, implies that ER15 and GC15 recognize different epitopes commonto p73 $alpha$ and p73 $beta$ (note that multiple bands are seen in Fig. 2Ddue to limited proteolysis of GST fusion proteins during theirproduction and purification). None of the anti-p73 antibodiesrecognized p53 or the recently identified p53-related proteinp51/Ket (33, 41, 46) (Fig. 2C and D).

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FIG. 2. Characterization of anti-p73 antibodies. (A) p73 $alpha$ and p73 $beta$ ³⁵S-labelled in vitro translation products were immunoprecipitated with either control (anti-T; PAb419) or anti-p73 (ER13, ER15, and GC15) antibodies, as indicated, under native (lanes 3 to 6 and 11 to 14) or denaturing (lanes 7 to 10 and 15 to 18) conditions. Two microliters of the indicated in vitro translation product was loaded directly in lanes 1 and 2. (B) p73 $alpha$ and p73 $beta$ were cotranslated in vitro in the presence of [³⁵S]methionine and immunoprecipitated with either control (anti-T; PAb419) or anti-p73 (ER13, ER15, and GC15) antibodies, as indicated, under native (lanes 2 to 5) or denaturing (lanes 6 to 10) conditions. Two microliters of the indicated in vitro translation product was loaded directly in lanes 1, 11, and 12. (C) p51A, p53, and p73 $beta$ ³⁵S-labelled in vitro translation products were immunoprecipitated with either control (anti-T; PAb419) or anti-p73 (ER13, ER15, and GC15) antibodies, as indicated. Two microliters of the indicated in vitro translation product was loaded directly in lanes 1 to 3. For panels A to C, proteins were resolved by SDS-polyacrylamide gel electrophoresis and detected by fluorography. (D) GST-p53 (lanes 1 to 5), GST-p73 $beta$ (aa 380 to 499) (lanes 6 to 10), and GST-p73 $alpha$ (aa 380 to 637) (lanes 11 to 15) were produced in bacteria, purified by using glutathione-Sepharose, resolved by SDS-polyacrylamide gel electrophoresis in preparative wells, and transferred to a membrane. The membrane was cut into strips and immunoblotted with either control (anti-T; PAb419) or anti-p73 (ER13, ER15, and GC15) antibodies, as indicated. Bound antibody was detected colorimetrically with an alkaline phosphatase-conjugated antimouse antibody.

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FIG. 3. Identification of p73 $alpha$ and p73 $beta$ in cell extracts. (A) COS cells were lysed in the presence of 0.5% Nonidet P-40 (EBC buffer) (lanes 1 to 3), in radioimmunoprecipitation assay buffer (lanes 4 to 6), or in the presence of 1% Triton (lanes 7 to 9) and immunoprecipitated (IP) with a control antibody (anti-T [PAb419]), anti-p73 (ER13), or anti-p73 (GC15) as indicated. Antibodies were cross-linked to protein A-Sepharose prior to immunoprecipitation. (B) COS cells (lanes 1 to 4) and SK-N-AS cells (lanes 5 to 8) were lysed in EBC buffer and immunoprecipitated with a control antibody (anti-T [PAb419]), anti-p73 (ER13), anti-p73 (ER15), or anti-p73 (GC15) as indicated. For both panels, Bound proteins were resolved by electrophoresis in an SDS-8% polyacrylamide gel and immunoblotted with anti-p73 (ER15) by using a horseradish peroxidase-conjugated antimouse antibody and enhanced chemiluminescence.

It has not been formally proven that mammalian cells produce both p73 $alpha$ and p73 $beta$ proteins. To address this, COS monkey kidneycells were lysed with a variety of detergents and immunoprecipitatedwith anti-p73 antibodies, or a control antibody, under conditionsof antibody excess (Fig. 3A, lanes 1 to 9; Fig. 3B, lanes 1 to4). Specifically bound proteins were detected by immunoblot analysiswith an anti-p73 antibody (ER15). Two proteins, with apparentmolecular masses of ~80 and 70 kDa, were detected in the anti-p73,but not control, immunoprecipitates. These two proteins comigratedwith the in vitro translation products of simian p73 $alpha$ and p73 $beta$ cDNAs, respectively, under a variety of SDS-polyacrylamide gelelectrophoresis conditions (data not shown). As an additionalspecificity control, SK-N-AS human neuroblastoma cells, whichdo not produce detectable levels of p73 mRNA (22), were analyzedin parallel (Fig. 3B, lanes 5 to 8). As expected, these cellslacked the 80- and 70-kDa species (Fig. 3B, compare lanes 6 to8 with lanes 2 to 4). We have thus far been unable to purify enoughof the 80- and 70-kDa species to perform partial proteolytic peptidemapping or to obtain peptide sequence data. Nonetheless, the factsthat they (i) are recognized by multiple, independent, anti-p73monoclonal antibodies, (ii) comigrate with p73 $alpha$ and p73 $beta$ in vitrotranslation products, and (iii) are absent in a cell line thatlacks p73 mRNA strongly suggest that they are p73 $alpha$ and p73 $beta$ , respectively.

p73 maps to chromosome 1p36, a region that is frequently deleted in a variety of human tumors, including neuroblastomas (5,45, 47). Although no intragenic p73 mutations have been identifiedto date, it has been suggested that the p73 gene locus might besubject to epigenetic regulation. In the next set of experiments,whole-cell extracts were prepared from COS cells, IM9 human myelomacells, and a panel of neuroblastomas and neuroepitheliomas (Fig.4). These extracts were resolved by SDS-polyacrylamide gel electrophoresisand immunoblotted with an anti-p73 antibody (ER15). p73 $alpha$ and p73 $beta$ were readily detected in both COS cell extracts and IM9 cell extracts(Fig. 4, lanes 1 and 2). Thus, the failure to detect p73 $alpha$ andp73 $beta$ in SK-N-AS cells (Fig. 3B, lanes 6 to 8, and 4, lane 5) cannotbe attributed to species differences. p73 $alpha$ and p73 $beta$ were eitherabsent or barely detectable in all of the neuroblastoma and neuroepitheliomacell lines tested (Fig. 4, compare lanes 4 to 8 with lanes 1 and2). Some of these cell extracts, including those prepared fromCOS, SK-N-SH, and SK-N-DZ cells, contained faster-migrating speciesthat reacted with the ER15 antibody (data not shown). Whetherthese proteins represent additional p73 isoforms, additional p53/p73family members, or unrelated proteins that share the ER15 epitopeis currently under investigation. We find that most human tumorcell lines, like the neuroblastoma cell lines studied here, producelow or undetectable levels of p73 $alpha$ and p73 $beta$ (unpublished data).

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FIG. 4. p73 $alpha$ and p73 $beta$ protein levels in neuroblastoma cell lines. Cell extracts prepared from the indicated cell lines were resolved by electrophoresis in an SDS-8% polyacrylamide gel and immunoblotted with an anti-p73 antibody (ER15). Each lane contained ~300 µg of total cell extract. Bound antibody was detected by using a horseradish peroxidase-conjugated antimouse antibody and enhanced chemiluminescence.

The availability of anti-p73 antibodies allowed us to next test directly whether p73 could, as predicted, bind to canonicalp53 DNA-binding sites. A radiolabelled p53 DNA-binding site wasincubated with either p53 (Fig. 5A, lanes 4 to 9) or p73 $beta$ (lanes10 to 15) synthesized in vitro by using a rabbit reticulocytelysate. Unprogrammed rabbit reticulocyte lysate served as a negativecontrol (lanes 1 to 3). As expected, p53 bound to this site (Fig.5A, lane 4, arrow). This complex was specific, as it was abolishedin the presence of excess, unlabelled competitor DNA that containedp53-binding sites and was unaffected by a competitor DNA thatlacked such sites (Fig. 5A, compare lanes 6 and 5 to lane 4).In contrast, the complex indicated by the asterisk, detectableeven with unprogrammed reticulocyte lysate, was abolished by bothspecific and nonspecific competitor DNA. The complex labelledp53/DNA contained p53, as it was supershifted by an anti-p53 antibody(Fig. 5A, lane 7) but not by anti-p73 or control (anti-T) antibodies(lanes 8 and 9). Similarly, p73 $beta$ formed a specific complex withDNA that was supershifted by an anti-p73 antibody but not by theanti-p53 and anti-T antibodies (Fig. 5A, lanes 10 to 15). Comparableresults were obtained with p73 $alpha$ (Fig. 5B, compare lanes 1 to 5with lanes 6 to 10). Thus, as predicted, p73 $alpha$ and p73 $beta$ can bindto p53 DNA-binding sites in a specific manner.

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FIG. 5. p73 binds to canonical p53 DNA-binding sites. A ³²P-radiolabelled p53 DNA-binding site was incubated with p53 in vitro translation product (A, lanes 4 to 9), p73 $alpha$ in vitro translation product (A, lanes 10 to 15, and B, lanes 1 to 5), p73 $beta$ in vitro translation product (B, lanes 6 to 10), or unprogrammed reticulocyte lysate (A, lanes 1 to 3) and subjected to electrophoretic mobility shift analysis. Binding reactions were carried out in the presence of a vast molar excess of unlabelled specific or nonspecific competitor DNA where indicated. Anti-p53, anti-p73, or a control antibody (anti-T) was added prior to the electrophoretic mobility shift assay as indicated. The asterisk indicates a nonspecific complex.

These results, together with earlier reports, suggest that p73 can, at least when overproduced, mimic the ability of p53 tobind to DNA, to activate transcription, and to inhibit tumor cellgrowth. DNA tumor viral oncoproteins have been invaluable reagentsfor elucidating the normal functions of tumor suppressor proteins,such as pRB and p53. Simian virus 40 (SV40) T antigen binds tothe central region of p53 responsible for DNA binding (27, 38).The adenovirus E1B 55K protein interacts with residues withinthe N-terminal p53 transactivation domain that are highly conservedbetween p73 and p53 (4, 23, 29, 51). The human papillomavirusE6 protein interacts with the C terminus and the core structureof p53 (18, 31, 32, 39, 40). Given the high degree ofsimilarity between p53 and p73, we next asked whether these viraloncoproteins could likewise physically interact with p73.

293 human embryonic kidney cells are stably transformed with a fragment of the adenovirus genome and produce E1B 55K (12).In the first set of experiments, these cells were immunoprecipitatedwith an anti-E1B 55K or control monoclonal antibody (Fig. 6A,lanes 2 and 1, respectively). The immunoprecipitates were resolvedby SDS-polyacrylamide gel electrophoresis and immunoblotted withan anti-p73 antibody (left panel) or anti-p53 antibody (rightpanel). Anti-p73 and anti-p53 immunoprecipitates prepared in parallelserved as additional controls (lanes 4 and 3, respectively). Asexpected, p53 coimmunoprecipitated with E1B 55K (Fig. 6A, lane2, right panel). In contrast, p73 was not detectable in anti-E1B55K immunoprecipitates (Fig. 6A, lane 2, left panel) despite thepresence of p73 in these cells (Fig. 6A, lane 4, left panel).

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FIG. 6. Differential binding of p53 and p73 to E1B 55K. (A) 293 human embryonic kidney cells were lysed and immunoprecipitated (IP) with the indicated antibodies. Specifically bound proteins were resolved by electrophoresis in an SDS-10% polyacrylamide gel and detected by immunoblotting with anti-p73 antibody (left panel) or anti-p53 antibody (right panel). Bound antibodies were detected by using a horseradish peroxidase-conjugated antimouse antibody and enhanced chemiluminescence. The asterisk indicates faster-migrating species, previously noted by others, that interact with anti-p53 antibodies. (B) 293 human embryonic kidney cells were transfected with 1 or 10 µg, as indicated by the triangles, of expression plasmids encoding HA-tagged p53 (lanes 2, 7, and 8) or HA-tagged p73 $alpha$ (lanes 4, 5, 9, and 10) or with 10 µg of the backbone expression plasmid (lanes 1 and 6). Cell extracts were prepared and immunoprecipitated with anti-HA (lanes 1 to 5) or anti-E1B 55K antibodies (lanes 6 to 10). Specifically bound proteins were resolved by electrophoresis in an SDS-10% polyacrylamide gel and detected by immunoblotting with anti-HA antibody (12CA5) by using a horseradish peroxidase-conjugated antimouse antibody and enhanced chemiluminescence. The asterisks indicate nonspecific bands.

These results left open the possibility that the failure to detect an association between p73 and E1B 55K reflected differencesin the abundances of p73 and p53 in these cells. To address thisconcern, 293 cells were transiently transfected with an emptyexpression plasmid (Fig. 6B, lanes 1 and 6) or plasmids encodingHA-tagged p53 (lanes 2, 3, 7, and 8) or p73 $alpha$ (lanes 4, 5, 9, and10). Cell extracts were prepared and immunoprecipitated with anti-HAantibody (lanes 1 to 5) or anti-E1B 55K (lanes 6 to 10) underconditions of antibody excess. Bound proteins were detected byanti-HA immunoblot analysis. Both p73 $alpha$ and p53 were produced atcomparable levels (compare lanes 2 and 3 to lanes 4 and 5, respectively).Despite this, p53 was readily detected in anti-E1B 55K immunoprecipitates,whereas p73 was not (compare lane 7 to lane 9). Thus, we havebeen unable to detect stable complex formation between E1B 55Kand p73 $alpha$ . Similar results were obtained for p73 $beta$ (data not shown).

To determine whether E6 could interact with p73, we first performed GST pull-down assays with GST-E6 (Fig. 7A). As expected,radiolabelled p53 bound to GST-E6, whereas p73 $alpha$ and p73 $beta$ did not(compare lanes 4 to 6 with lanes 7 to 12). None of these proteinsbound to GST alone (lanes 13 to 15). Next we used an in vitrodegradation assay developed by Scheffner et al. (40). This assayexploits the fact that rabbit reticulocyte lysate contains allof the proteins required for ubiquitin-dependent proteolysis ofp53. Coincubation of bacterially produced E6 with radiolabelledp53 in vitro translation product led to virtual disappearanceof the latter within 30 min (Fig. 7B, compare right and left panels).In contrast, under identical assay conditions, recombinant E6had no discernible effect on the stability of p73 $alpha$ or p73 $beta$ (Fig.7B, compare right and left panels). Thus, E6 can not physicallyinteract with p73 and is unable to target it for ubiquitin-dependentproteolysis.

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FIG. 7. E6 targets p53, but not p73, for degradation in vitro. (A) p53, p73 $alpha$ , and p73 $beta$ ³⁵S-labelled in vitro translation products were incubated with immobilized GST-E6 (lanes 4 to 12) or GST (lanes 13 to 15) as indicated. Each binding reaction mixture contained 40 µl (lanes 4, 7, 10, and 13 to 15), 20 µl (lanes 5, 8, and 11), or 10 µl (lanes 6, 9, and 12) of in vitro translation product. Specifically bound proteins were resolved by SDS-polyacrylamide gel electrophoresis and detected by fluorography. Five microliters of the indicated in vitro translation product was loaded directly in lanes 1 to 3. (B) p53, p73 $alpha$ , and p73 $beta$ ³⁵S-labelled in vitro translation products were incubated at 30°C with a lysate prepared from bacteria producing GST-E6 (right panel) or GST-E4 (left panel). The proteins were then resolved by electrophoresis in an SDS-10% polyacrylamide gel and detected by fluorography.

T antigen binds to the region that is most highly conserved between p53 and p73 (27, 38). This region has been implicatedin p53's ability to bind to specific DNA sequences and is alsofrequently altered in human tumors (2, 15, 34, 48). p73was first identified in COS cells, a cell line that stably producesT antigen. We noted, however, that p73 was not present in anti-Timmunoprecipitates prepared from these cells (Fig. 3A, lanes 1,4, and 7, and Fig. 3B, lane 1), raising the possibility that Tantigen does not bind to p73. To address this further, COS cellswere transiently transfected with plasmids encoding HA-taggedversions of wild-type p53, a tumor-derived p53 mutant (p53 135Tyr)(6), p73 $alpha$ , and p73 $beta$ or with the empty vector (Fig. 8A). Cellextracts were prepared and immunoprecipitated with anti-HA antibody(lanes 1 to 5) or anti-T antibody (lanes 6 to 10). Bound proteinswere resolved by SDS-polyacrylamide gel electrophoresis and immunoblottedwith an anti-HA antibody. All of the ectopically expressed proteinswere produced at comparable levels (compare lanes 2 through 5).As expected, T antigen bound to wild-type p53 and, to a lesserextent, to the tumor-derived p53 mutant (lanes 7 and 8). In contrast,p73 was not detectable in the anti-T immunoprecipitates (lanes9 and 10).

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FIG. 8. Differential binding of p53 and p73 to SV40 T. (A) COS cells, which stably produce SV40 T, were transfected with expression plasmids encoding the indicated HA-tagged proteins or with the backbone expression plasmid (Mock). Cell extracts were prepared and immunoprecipitated (IP) with anti-HA (lanes 1 to 5) or anti-T (lanes 6 to 10) antibodies. Specifically bound proteins were resolved by electrophoresis in an SDS-10% polyacrylamide gel and detected by immunoblotting with anti-HA antibody (12CA5) by using a horseradish peroxidase-conjugated antimouse antibody and enhanced chemiluminescence. (B) SAOS2 cells were transfected a CAT reporter plasmid containing a minimal promoter consisting of two p53-binding sites upstream of a TATA box together with expression plasmids for wild-type p53 or p73 $alpha$ . In each case, the amount of CAT activity, in the absence of T antigen, was set to 100%. Where indicated, the cells were also transfected with a plasmid encoding wild-type (wt) or mutant (mut) T antigen. Error bars represent one standard deviation.

In the final set of experiments, SAOS2 cells were transfected with a reporter plasmid in which the CAT gene was placed underthe control of a p53-responsive promoter (2XRGC-CAT) along withexpression plasmids encoding either p53 or p73 $alpha$ (Fig. 8B). Thesecells have both copies of the p53 gene deleted and consequentlydo not contain p53 protein (9). In addition, they contain eitherno or barely detectable levels of p73 (reference 22 and datanot shown). In keeping with earlier studies, both p53 and p73 $alpha$ activated this reporter (20). Coexpression of wild-type T, butnot a T-antigen mutant (dl357-370) that is incapable of bindingto p53 (24), reproducibly inhibited the ability of p53 to activatethis reporter. In contrast, neither wild-type T nor the T mutantsignificantly inhibited p73 function in these assays. Note thatthese experiments were performed with a 20-fold excess of T-antigenexpression plasmid relative to the p53 or p73 expression plasmid.Similar results were obtained when a reporter containing the p53-responsivep21 promoter was used instead of 2XRGC-CAT (data not shown). Insummary, both the biochemical data and transcriptional activationdata suggest that T antigen, like E1B and E6, discriminates betweenp53 and p73.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Viral oncoproteins, as well as high-affinity monoclonal antibodies, have proven to be invaluble reagents for studying thefunctions of tumor suppressor proteins. In this report, we havedescribed the generation and validation of multiple anti-p73 monoclonalantibodies. Using these reagents, we have confirmed that the twopreviously recognized p73 isoforms are produced in mammalian cellsand can, as predicted, bind to canonical p53 DNA-binding sites.

To date no intragenic p73 mutations have been identified in human cancer cells. It has been suggested, however, that p73 ismonoallelically expressed (22). If this was true, then lossof the transcriptionally active allele, as a result of a chromosomaldeletion, might contribute to human carcinogenesis. On the otherhand, others have found evidence of biallelic p73 expression inhuman T cells. It remains to be determined whether monoallelicexpression of p73 might be restricted to certain tissues or whetherthe ability to imprint the p73 locus might itself be a polymorphictrait. p73 transcript analysis is further complicated by the existenceof alternative promoters as well as of alternatively spliced mRNAs(4a). In summary, while a role for epigenetic control of p73expression cannot be excluded, there are currently no geneticdata that firmly establish that p73 is a tumor suppressor geneproduct.

At the protein level, we found that many tumor cell lines, including neuroblastoma cell lines, produce low levels of p73 $alpha$ and p73 $beta$ . In the absence of p73 gene mutations, however, it isimpossible to know whether this reflects pathology or physiology.Thus, one possibility is that p73 $alpha$ and p73 $beta$ are, indeed, suppressedepigenetically. Alternatively, it is possible that the precursorcells that give rise to these tumors normally produce low levelsof p73 $alpha$ and p73 $beta$ . In addition, it is possible that p73 levelsfall as a result of, rather than as a cause of, the malignanttransformation of these cells.

One would have predicted that viral oncoproteins that inactivate p53 would also inactivate p73 if p53 and p73 played similarroles in cells. A potential precedent would be the inactivationof multiple retinoblastoma protein family members by adenovirusE1A, SV40 T, and human papillomavirus E7. Instead, we were unableto detect stable complexes between these proteins and p73 by usingboth biochemical and functional assays. One possible explanationis that p73 is not produced in those cells that are susceptibleto transformation by these viruses. We found, however, that p73is produced in COS cells and 293 cells. These cell lines are transformedby T and the left half of the adenovirus genome, respectively.Thus, stable binding of T or E1B 55K to p73 is apparently notnecessary for transformation.

The high degree of similarity to p53 might have led to viral oncoprotein binding even if, as suggested above, inactivationof p73 is not required for transformation. In other words, ifnot by natural selection, then p73 might have bound to adenovirusE1B 55K, SV40 T, or human papillomavirus E6 by chance. The observationthat viral oncoproteins discriminate between p53 and p73 raisesthe possibility that preservation of one or more p73 functionsfacilitates viral replication. In this light, the high levelsof p73 seen in COS cells and 293 cells raise two interesting possibilities.The first is that high levels of p73 render a cell permissivefor viral replication or transformation. The second is that p73is induced following transformation with these agents.

In summary, despite the similarity between p53 and p73, only the former is a recurrent target of mutations in human cancerand a direct target of viral oncoproteins. This suggests thatp53 and p73 are not functionally equivalent. In this regard, experimentsperformed to date suggest that p73, unlike p53, is not inducedby DNA damage. Thus, p53 may have uniquely evolved to respondto genotoxic stress. Clearly, additional experiments are neededto decipher the normal functions of p73 and to determine whetherit plays a role in human carcinogenesis.

	ACKNOWLEDGMENTS

M.C.M. and C.A.J. contributed equally to this work.

We thank Arnold Berk, Herta Chao, Erik Flemington, Ed Harlow, Peter Howley, John Huibregste, Shuntaro Ikawa, and Joseph Nevinsfor reagents, Sorab Dalal for help with the GST-E6 binding assays,Ratna K. Vadlamudi for help with the p53 degradation assays, andmembers of the Kaelin laboratory for useful discussions.

M.C.M. was supported by an NIH training grant to the Cancer Biology Program at the Dana-Farber Cancer Institute. W.G.K. receivedsupport from the NIH and Novartis Pharmaceuticals and is a HowardHughes Medical Institute assistant investigator.

	FOOTNOTES

^* Corresponding author. Mailing address: Dana-Farber Cancer Institute, 44 Binney St., Boston, MA 02115. Phone: (617) 632-3975.Fax: (617) 632-4760. E-mail: william_kaelin{at}dfci.harvard.edu.

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Top
Abstract
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Materials & Methods
Results
Discussion
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