Degradation of p53 by adenovirus E4orf6 and E1B55K proteins occurs via a novel mechanism involving a Cullin-containing complex

doi:10.1101/gad.926401

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Vol. 15, No. 23, pp. 3104-3117, December 1, 2001

RESEARCH PAPER
Degradation of p53 by adenovirus E4orf6 and E1B55K proteins occurs via a novel mechanism involving a Cullin-containing complex

Emmanuelle Querido,¹^,⁸ Paola Blanchette,¹ Qin Yan,³^,⁴ Takumi Kamura,⁵ Megan Morrison,¹ Dominique Boivin,¹ William G. Kaelin,⁶ Ronald C. Conaway,³^,⁷ Joan Weliky Conaway,³^,⁴^,⁷ and Philip E. Branton¹^,²^,⁹

Department of ¹ Biochemistry and the ² McGill Cancer Centre, McGill University, Montreal, Quebec H3G 1Y6, Canada; ³ Stowers Institute for Medical Research, Kansas City, Missouri 64110, USA; ⁴ Department of Biochemistry and Molecular Biology, University of Oklahoma Health Sciences Center, Oklahoma City, Oklahoma 73190, USA; ⁵ Department of Molecular and Cellular Biology, Medical Institute of Bioregulation, Kyushu University, Kawaguchi, Saitama 332-012, Japan; ⁶ Dana-Farber Cancer Institute and Harvard Medical School, Boston, Massachusetts 02115, USA; and ⁷ Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City, Kansas 66160, USA

ABSTRACT

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

Although MDM2 plays a major role in regulating the stability of the p53 tumor suppressor protein, other poorly understoodMDM2-independent pathways also exist. Human adenoviruses haveevolved strategies to regulate p53 function and stability to permitefficient viral replication. One mechanism involves adenovirusE1B55K and E4orf6 proteins, which collaborate to target p53 fordegradation. To determine the mechanism of this process, a multiproteinE4orf6-associated complex was purified and shown to contain anovel Cullin-containing E3 ubiquitin ligase that is (1) composedof Cullin family member Cul5, Elongins B and C, and the RING-H2finger protein Rbx1(ROC1); (2) remarkably similar to the von Hippel-Lindautumor suppressor and SCF (Skp1-Cul1/Cdc53-F-box) E3 ubiquitinligase complexes; and (3) capable of stimulating ubiquitinationof p53 in vitro in the presence of E1/E2 ubiquitin-activatingand -conjugating enzymes. Cullins are activated by NEDD8 modification;therefore, to determine whether Cullin complexes are requiredfor adenovirus-induced p53 degradation, studies were conductedin ts41 Chinese hamster ovary cells that are temperature sensitivefor the NEDD8 pathway. E4orf6/E1B55K failed to induce the degradationof p53 at the nonpermissive temperature. Thus, our results identifya novel role for the Cullin-based machinery in regulation ofp53.

[Key Words: p53; adenovirus; protein degradation; Cullin complexes; ubiquitination; Elongin B; Elongin C; NEDD8]

	Introduction

Top Abstract Introduction Results Discussion Materials and methods References

The p53 cellular tumor suppressor induces cell cycle arrest and apoptosis by functioning as a transcriptional regulator (forreview, see Woods and Vousden 2001). Intracellular levels of activatedp53 are known to be regulated by a variety of mechanisms, includingphosphorylation, acetylation, and targeted degradation. In mostcells p53 is degraded, at least in part, through ubiquitin-dependentproteolysis involving MDM2 (for review, see Woods and Vousden2001), which binds near the N terminus and functions as an E3ubiquitin ligase for p53 (Honda et al. 1997). Nuclear export appearsto be required for MDM2-dependent p53 degradation, which is blockedby both the drug leptomycin B (Roth et al. 1998; Lain et al. 1999)and the p53-binding protein ARF (for review, see Zhang and Xiong2001). ARF binds MDM2, thus blocking MDM2-mediated ubiquitinationand degradation. Although MDM2 is clearly a major regulator ofp53 stability, MDM2-independent cellular pathways for p53 degradationexist, including the c-Jun N-terminal kinase (JNK), which bindsto and destabilizes p53 (Fuchs et al. 1998), and calpain proteases(Gonen et al. 1997; Kubbutat and Vousden 1997; Zhang et al. 1997).

Infection of cells by many viruses induces the stabilization and activation of p53 (for review, see Roulston et al. 1999).In the case of human adenoviruses, binding of the viral earlyregion 1A (E1A) protein with either the retinoblastoma tumor suppressorfamily or p300/CBP/p400 histone acetyl transferases induces theactivation, stabilization, and accumulation of p53 (Chiou andWhite 1997; Querido et al. 1997b; Samuelson and Lowe 1997). Increasedlevels of p53 could therefore result in the induction of cellcycle arrest and early apoptotic cell death, effects that wouldseverely limit the yield of viral progeny. Adenoviruses and othersmall DNA tumor viruses have evolved various types of mechanismsto prevent the deleterious effects of p53. The large T antigenof simian virus 40 binds to the DNA-binding domain of p53 andprevents p53-mediated transcriptional effects (Sarnow et al. 1982;Bargonetti et al. 1992). This process leads to a large accumulationof p53, but it is nonfunctional. The E6 products of human papillomavirustypes 16 and 18 bind p53 (Werness et al. 1990) and target it fordegradation by the ubiquitin pathway. Targeting is mediated bya cellular E6-associated protein, E6AP-100K, that functions asa ubiquitin ligase, with E6 functioning as a bridge between theligase and the p53 substrate (Scheffner et al. 1993).

Although adenovirus E1A can induce a large accumulation of p53 when expressed alone, such increased p53 levels are not usuallyapparent in wild-type adenovirus-infected cells. Two productsof early regions 1B and 4, E1B55K and E4orf6, bind p53 near theN and C termini, respectively, and inhibit transcriptional activationby the tumor suppressor (Sarnow et al. 1982; Yew and Berk 1992;Yew et al. 1994; Dobner et al. 1996; Teodoro and Branton 1997;E. Querido, S. Gurd, and P.E. Branton, unpubl.). In addition,several studies, including our own, have shown that E4orf6 andE1B55K function together to reduce the half-life of p53 and induceefficient p53 degradation (Moore et al. 1996; Querido et al. 1997a;Steegenga et al. 1998; Cathomen and Weitzman 2000; Nevels et al.2000; Shen et al. 2001). Furthermore, the E1B55K/E4orf6 complex(Sarnow et al. 1984) can induce p53 turnover in cells lackingeither MDM2 or ARF, indicating that neither is required for thisprocess (Querido et al. 2001). E4orf6 is a nuclear protein containingboth nuclear localization and nuclear retention signals that arebelieved to be responsible for targeting E4orf6 and E4orf6/E1B55Kcomplexes to the nucleus (Goodrum et al. 1996; Orlando and Ornelles1999; Nevels et al. 2000). In addition, both E4orf6 and E1B55Khave nuclear export signals, and several groups have shown theycan shuttle between the nucleus and the cytoplasm (Dobbelsteinet al. 1997; Weigel and Dobbelstein 2000; Rabino et al. 2000;Dosch et al. 2001).

In the present studies, we have determined the mechanism of adenovirus-induced p53 degradation through the identificationof E4orf6-associated cellular proteins. Such proteins were foundto be members of a novel Cullin-containing complex that is requiredfor E4orf6-E1B55K-mediated p53 degradation and capable of inducingubiquitination of p53 in vitro. These findings suggest that similarcomplexes could also function in the regulation of p53 levelsin normalcells.

	Results

Top Abstract Introduction Results Discussion Materials and methods References

Identification of cellular E4orf6-binding proteins.

To investigate the roles of the E1B55K and E4orf6 proteins in regulating p53 destruction in adenovirus-infected cells, weaffinity purified an E4orf6-containing complex from whole cellextracts of [³⁵S]methionine/[³⁵S]cysteine-labeled p53-null human H1299 cells infected with eitheran adenovirus vector expressing Ad5 E4orf6 (AdE4orf6) or the controlvector AdLacZ. Using this procedure, we observed that approximatelystoichiometric amounts of ³⁵S-labeled cellular proteins of ~84 kD, 19 kD, and 14 kD, as wellas lower levels of a 16-kD protein, were reproducibly and specificallyimmunoprecipitated with the monoclonal antibody 1D5 raised againstE4orf6 (Fig. 1A; Boivin et al. 1999). Ion trap mass spectrometryof the E4orf6-associated proteins revealed that the ~84-kD proteinwas the Cullin family member Cul5 (Kipreos et al. 1996; Byrd etal. 1997), also known as the vasopressin-activated calcium mobilizationreceptor or VACM-1, and that the ~19-kD and 14-kD proteins wereElongins B and C, respectively.

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Figure 1. Analysis of E4orf6 complex formation. (A) Detection of E4orf6 complexes. Extracts from H1299 cells infected with AdLacZ or AdE4orf6 and labeled with ³⁵S were immunoprecipitated with 1D5 anti-E4orf6 antibody followed by SDS-PAGE and autoradiography. Two exposures have been included: positions of migration of prestained standard size markers (left) and those of E4orf6 and coimmunoprecipitating proteins (right). Identities for these species were derived from mass spectroscopy analysis of tryptic peptides. (B) Analysis of complex formation using E4orf6 deletion mutants. H1299 cells were transfected with plasmid DNAs encoding wild-type or mutant E4orf6, and extracts were immunoprecipitated and analyzed as in A. Coimmunoprecipitation of p19 and p14 cellular proteins with E4orf6 has been summarized below as + and $-$ . Binding of p84 showed a similar pattern, as determined from other exposures of the gel (data not shown). Binding of E4orf6 to E1B55K (shown in C) and p53 turnover experiments with E4orf6 and E1B55K (D) have also been indicated as + and $-$ . (C) Complex formation between E4orf6 mutants and E1B55K. Extracts from H1299 cells transfected with plasmid DNAs expressing E1B55K (pCA14 HH55K) and wild-type or mutant E4orf6 proteins (pcDNA3E4orf6) were immunoprecipitated with anti-E1B55K antibody (2A6), and membranes were immunoblotted with anti-E4orf6 antibody (1807). (D) E4orf6/E1B55K-induced turnover of p53. H1299 cells were transfected with plasmid DNAs pcDNA3 p53wt (p53), pCA14 HH55K (E1B-55K), and pcDNA3E4orf6 (wild-type or mutant E4orf6), and extracts were analyzed by Western blotting using anti-p53 antibodies 1801 and 421.

We have previously constructed and partially characterized a series of E4orf6 in-frame deletion mutants (Querido et al. 2001).Consistent with the hypothesis that the coimmunoprecipitatingE4orf6/Cul5/ElonginBC complex is involved in the destabilizationof p53, we observed a correlation between the ability of E4orf6mutants to promote p53 degradation and to bind not only E1B55Kbut also Elongin B and Elongin C (Fig. 1B-D). To determine theability of E4orf6 mutants to participate in p53 degradation, p53-nullH1299 cells were cotransfected with cDNAs expressing human p53,histidine-tagged E1B55K (HH55Kwt), and wild-type or mutant E4orf6.As shown in Figure 1D, p53 levels were reduced in whole cell extractsfrom cells expressing E1B55K and wild-type E4orf6 or E4orf6 mutantsdl1-38 and dl35-43 (lanes 2,3,6), but not from cells expressingE4orf6 mutants dl1-55, dl1-108, dl49-64, dl65-83, dl83-94, ordl95-122. Similarly, endogenous Elongin BC could be immunoprecipitatedwith wild-type E4orf6 and mutants dl1-38 and dl35-43, but notwith any of the other mutants tested, suggesting that a regionrequired for the interaction may reside between residues 44 and108 of E4orf6. Interaction of E4orf6 with E1B55K is not sufficientto promote degradation of p53, as several of the E4orf6 mutantproteins that could still bind E1B55K but failed to bind ElonginBC also failed to support p53 degradation (Fig. 1C).

The mammalian Elongin BC complex was shown to function as a regulator of RNA polymerase II elongation factor Elongin A (forreview, see Reines et al. 1999). Elongin BC is also a componentof the large von Hippel-Lindau (VHL) tumor suppressor complex(Duan et al. 1995; Kibel et al. 1995). Binding of Elongin BC withboth Elongin A and VHL appears to involve the interaction of ElonginC with a short region termed the BC-box (consensus sequence [A,P,S,T]LXXXCXXX[A,I,L,V]),which is found in VHL and Elongin A (Duan et al. 1995; Kibel etal. 1995; Aso et al. 1996; Stebbins et al. 1999; Ohh et al. 2000).In addition, Elongin BC binds to many additional proteins, includingmembers of the so-called SOCS-box protein family, each of whichcontains an Elongin BC-binding site (Kamura et al. 1998; Zhanget al. 1999). The VHL complex was shown to function as an E3 ubiquitinligase (Iwai et al. 1999; Lisztwan et al. 1999) that targets the $alpha$ -subunits of the hypoxia-inducible transcription factors HIF1and HIF2 for ubiquitination (Maxwell et al. 1999; Cockman et al.2000; Kamura et al. 2000; Ohh et al. 2000). VHL functions as asubstrate recognition subunit (Cockman et al. 2000; Kamura etal. 2000; Ohh et al. 2000), whereas Elongins B and C serve tolink these proteins to a module containing Cul2 and Rbx1. TheCul2/Rbx1 module activates an E2 ubiquitin-conjugating enzymeto ubiquitinate HIF- $alpha$ (Kamura et al. 2000). The VHL complex isremarkably similar to the yeast and mammalian SCF ubiquitin ligasecomplexes (for review, see Patton et al. 1998), each of whichcontain an F-box protein substrate recognition subunit linkedto a Cul1(Cdc53)/Rbx1 module by the Skp1 protein (Kamura et al.1999; Ohta et al. 1999; Seol et al. 1999; Skowyra et al. 1999;Tan et al. 1999). Thus, the association of a Cullin family memberand Elongin BC with E4orf6 could suggest that the adenovirus E4orf6and E1B55K proteins target p53 for degradation by forming a CullinE3 ligase and recruiting it top53.

To confirm the interaction of Elongin BC with E4orf6, H1299 cells were infected with either the control adenovirus vectorAdLacZ (Fig. 2A, lane 1) or with vectors encoding E4orf6 (lane2) or a combination of vectors expressing E4orf6, His-tagged E1B55K,and p53 (lane 3). Western blotting with the anti-E4orf6 antibody1807, with anti-Elongin B antiserum, or with an anti-Elongin Cantibody was then performed on whole cell extracts (left) or onproteins immunoprecipitated with anti-E4orf6 1D5 monoclonal antibody(right). As expected, E4orf6 was detected only in whole cell extractsfrom E4orf6-expressing cells (top panel). Elongin B (middle panel)and Elongin C (bottom panel) were specifically precipitated withE4orf6 whether or not E1B55K and p53 were present. Figure 2B showsthat neither VHL nor Elongin A coimmunoprecipitated with E4orf6.Confirming that VHL is not required for E4orf6/E1B55K-mediatedp53 degradation, both human VHL-positive and VHL-null tumor celllines supported p53 turnover by these viral proteins at similarlevels (data not shown).

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Figure 2. Identification of E4orf6 binding proteins. (A) H1299 cells were infected with AdLacZ (lane 1), AdE4orf6 (lane 2), or AdE4orf6 plus AdHH55K plus Adp53wt (lane 3). Whole cell extracts (left three lanes) and 1D5 immunoprecipitates (right three lanes) were analyzed by Western blotting using anti-E4orf6 antibody 1807 (top), anti-Elongin B antibody (middle), and anti-Elongin C antibody (bottom). (B) Same as Figure 1A except that immunoblotting was performed with anti-VHL Ig32 antibody (top) or anti-Elongin A antibody (bottom). At the right (lane 1) is shown an immunoprecipitate prepared with anti-Elongin A and blotted with the same antibody. (C) H1299 cells were infected with AdLacZ (lane 1) or AdE4orf6 (lane 2), and cytoplasmic and nuclear extracts as well as whole cell extracts were prepared. Whole cell extracts immunoprecipitated with 1D5 anti-E4orf6 antibody were analyzed by Western blotting using either a polyclonal antibody to rabbit VACM-1 (left six lanes) or a polyclonal antibody against human Cul5 (right two lanes). E4orf6 (bottom) was detected using 1807 antibody. (D) Human Cul1, Cul2, Cul3, and Cul5 and mouse Cul4A were synthesized (top) by in vitro transcription/translation, and aliquots of these ³⁵S-labeled proteins were combined with 1D5 immunoprecipitates from AdLacZ-infected (middle) or AdE4orf6-infected (bottom) H1299 cells. (E) H1299 cells were transfected with plasmid DNAs expressing Myc-Rbx1 (lane 1), E4orf6 (lane 2), and Myc-Rbx1 plus E4orf6 (lane 3). Whole cell extracts (left lanes) or 1D5 immunoprecipitates (right lanes) were analyzed by Western blotting with anti-Myc 9E10 antibody. (F) Human 293 cells were infected with wild-type Ad5 at a MOI of 40, and at 15 h postinfection, cell extracts were prepared and immunoprecipitated with either anti-E4orf6 (1809) or anti-E1A (M73) antibodies. The pattern of associated proteins determined by Western blotting as above.

To verify the interaction of E4orf6 and Cul5, nuclear and cytoplasmic extracts were prepared from cells infected with AdLacZor AdE4orf6 and immunoprecipitated with anti-E4orf6 antibody 1D5.Following Western blot analysis, an antibody raised against rabbitCul5 (VACM-1; Burnatowska-Hledin et al. 1995) detected two closelymigrating Cul5 species in cytoplasmic fractions from AdLacZ-infected(Fig. 2C, lane 1) and AdE4orf6-infected cells (Fig. 2C, lane 2);however, in 1D5 immunoprecipitates and in nuclear fractions, Cul5was only detected when E4orf6 was present (Fig. 2C, cf. lanes1 and 2). To confirm that this species represented Cul5, an antipeptidepolyclonal antiserum was raised against a synthetic peptide correspondingto the C terminus of human Cul5. Figure 2C shows that similarresults were obtained with this antiserum (see lanes 1 and 2 atright). When this work commenced, Cul5 had not been shown to playa role in ubiquitination; however, in parallel studies we havefound that it appears to be a component of a larger family ofElongin BC-based E3 ubiquitin ligases (Kamura et al. 2001). Itwas also suggested recently that Cul5 is able to form a complexthat ubiquitinates E2F1 in vitro (Ohta and Xiong 2001). To determinewhether E4orf6 can associate with other members of the Cullinfamily, in vitro translated human Cul1, Cul2, Cul3, and Cul5 ormouse Cul4a were tested for the ability to bind 1D5 immunoprecipitatesfrom AdLacZ- or AdE4orf6-infected H1299 cells. As shown in Figure2D, all Cullins were synthesized at similar levels (top); however,only Cul5 was specifically precipitated with E4orf6 (bottompanels).

The 16-kD Rbx1 (ROC1) protein is a component of both the SCF and VHL tumor suppressor complexes (Kamura et al. 1999; Ohtaet al. 1999; Seol et al. 1999; Skowyra et al. 1999; Tan et al.1999). As shown in Figure 2E, myc-tagged Rbx1 specifically co-immunoprecipitatedwith E4orf6 from cells transfected with cDNAs expressing thesetwo proteins. Thus, Rbx1 associates with E4orf6 and probably representsthe 16-kD species detected at low levels in Figure 1A.

To determine if the Cul5/ElonginB/C complex also associates with E4orf6/E1B55K during productive infection, human 293 cellswere infected with wild-type Ad5 and cell extracts prepared at15 h post-infection were immunoprecipitated using either anti-E4orf6antibodies (1807) or, as a control, anti-E1A M73 mouse monoclonalantibodies (Harlow et al. 1985). Analysis by Western blottingusing appropriate antibodies indicated that Cul 5 (appearing againas a doublet), Elongin B, and Elongin C were detected in associationwith E4orf6 but not with E1A products (Fig. 2F). E1B55K also associatedwith E4orf6, as shown many times previously (Querido et al. 2001).The material present in the position of migration of E1B55K inthe M73 immunoprecipitate was undoubtedly antibody heavy chain,as this protein has not been found previously to associate withE1Aproducts.

As a final verification of the interaction of E4orf6 and E1B55K with Cul5, Elongin BC, and Rbx1, Sf21 insect cells were infectedwith various combinations of baculoviruses encoding E4orf6, E1B55K,Elongin BC, HA-tagged Cul5 (HA-Cul5), and c-myc-tagged Rbx1 (cmyc-Rbx1),and complexes were immunoprecipitated from cell lysates with either1D5 antibodies against E4orf6 or antibodies against the HA-epitopeand subjected to immunoblotting. As shown in Figure 3, complexescontaining E4orf6, E1B55K, Cul5, Elongin BC, and Rbx1 could beisolated from insect cells. Consistent with the results obtainedin mammalian cells, the interaction of E4orf6 with Cul5, ElonginBC, and Rbx1 did not require E1B55K. In addition, Elongin BC andCul5 were able to interact with E4orf6 in lysates from cells notoverexpressing other complex components. This observation doesnot, however, necessarily imply that Cul5/Rbx1 binds directlyto E4orf6, as previous results indicate that insect Elongins Band C can assemble into functional complexes with mammalian ElonginBC-binding proteins and Cullins (Brower et al. 1999; Kamura etal. 2000). Taken together, the findings presented thus far indicatethat E4orf6 can assemble with Elongin BC, Cul5, and Rbx1 in acomplex that is distinct from the Elongin BC-containing complexesformed with VHL and Elongin A.

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Figure 3. Reconstitution of E4orf6/E1B55K/Cul5/Rbx1/Elongin B and C complexes in Sf21 cells. Sf21 cells were infected with baculoviruses encoding the proteins indicated. The lysates were immunoprecipitated using either anti-HA (12CA5) or anti-E4orf6 (1D5) antibody. Crude lysates (top) and washed immune complexes (middle, bottom) were separated by SDS-PAGE and immunoblotted with the indicated antibodies.

E4orf6 relocates Cul5 but not Cul2 to the nucleus

Given the remarkable architectural similarity between Cul1/Cdc53-containing SCF and Cul2-containing VHL ubiquitin ligasesand the E4orf6 complex, these results raise the possibility thatthe complex of E4orf6, Cul5, Elongin BC, and Rbx1 may also functionas a ubiquitin ligase. Because E4orf6 is found largely in thenucleus (Goodrum et al. 1996; Dobbelstein et al. 1997) and Cul5had been reported previously as largely cytoplasmic (Burnatowska-Hledinet al. 1999), it was important to determine whether Cul5 and E4orf6colocalize in cells. H1299 cells were transfected with cDNAs expressinghuman HA-Cul5 or HA-Cul2 and/or E4orf6, and cells were examinedby laser confocal microscopy. E4orf6 was detected using a rabbitpolyclonal antibody (1807) directed toward the E4orf6 C terminus(Boivin et al. 1999) and visualized using Alexa 594 anti-rabbitantibody (red color). The Cullins were detected using mouse monoclonalanti-HA antibodies and visualized using Alexa 488 anti-mouse antibody(green color). Figure 4 shows examples of the staining patternsobtained and are representative of the majority of cells in thepreparations. Figure 4, G and H, shows that when expressed independently,Cul2 (Fig. 4G) and Cul5 (Fig. 4H) were localized primarily tothe cytoplasm, whereas E4orf6 (Fig. 4I) was largely nuclear. Figure4, A-C and D-E, shows cells that coexpressed E4orf6 and eitherCul5 or Cul2, respectively. In the presence of E4orf6, Cul5 (Fig.4A), but not Cul2 (Fig. 4D), was present at high levels in thenucleus. The appearance of yellow nuclear fluorescence followingsuperimposition of Figure 4, panels A and B (Fig. 4C), indicatedthat Cul5 co-localized in the nucleus with E4orf6. This was notthe case with Cul2, as the nuclear fluorescence remained largelyunchanged following superimposition of Figure 4, D and E (Fig.4F). These data are consistent with our observation that E4orf6binds preferentially to Cul5, and they suggest that E4orf6 maytransport Cul5 to the nucleus, as it does E1B55K (Goodrum et al.1996). We also tested the ability of E4orf6 mutants dl1-38, dl1-55,and R240E/R241E to direct nuclear localization of Cul5. The E4orf6mutant dl1-38 was wild-type in its ability to direct Cul5 to thenucleus, whereas the other two mutants were deficient (data notshown). These observations correlate with the ability of thesemutants to cooperate with E1B55K in p53 turnover (Fig. 1; Queridoet al. 2001).

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Figure 4. Intracellular colocalization of E4orf6 and Cul5. H1299 cells were transfected with plasmid DNAs expressing HA-Cul2, HA-Cul5, or E4orf6, and cells were fixed and examined by laser confocal microscopy. E4orf6 was detected using rabbit polyclonal antibody (1807) and Alexa 594 (red) anti-rabbit IgG antibody. HA-tagged human Cul2 and Cul5 were detected using mouse monoclonal anti-HA antibody (HA.11) and Alexa 488 (green) anti-mouse IgG antibody. (A-C) HA-Cul5 and E4orf6. (D-F) HA-Cul2 and E4orf6. C and F were generated by scanning for both the red and the green signal to detect any colocalization as bright yellow. (G) HA-Cul2 alone. Bar, 20 µm; cells shown are representative. (H) HA-Cul5 alone. (I) E4orf6 alone.

E4orf6 complex ubiquitinates p53 in vitro

To test directly the possibility that the E4orf6 complex can function as an E3 ubiquitin ligase that targets p53, we examinedthe ability of immunopurified E4orf6 complexes to support theubiquitination of recombinant p53 in vitro. Conjugation of ubiquitinto target proteins requires, in addition to an E3 ubiquitin ligase,an E1 ubiquitin-activating enzyme that transfers ubiquitin tothe active site cysteine of an E2 ubiquitin-conjugating enzyme.E2 and E3 then act together to catalyze the formation of an isopeptidebond between lysine residue(s) on the target protein and the Cterminus of ubiquitin. The E3 binds both the target protein andE2 and accordingly plays a central role in determining the substratespecificity of the reaction. Cul5, E1B55K, Rbx1, and ElonginsB and C were expressed in insect cells, with or without E4orf6,and insect cell lysates were immunoprecipitated with anti-E4orf61D5 antibodies. Immunoprecipitated complexes were supplementedwith various concentrations of recombinant p53 and with recombinantyeast ubiquitin-activating enzyme (yUba1), the E2 ubiquitin-conjugatingenzyme hUbc5A, ATP, and GST-ubiquitin^K48R. Ubiquitination of p53 was assessed by the appearance of slower-migratingforms of p53, as detected by Western blotting using an anti-p53monoclonal antibody. The ~35-kD GST-ubiquitin fusion protein GST-ubiquitin^K48R was used in these reactions because it causes a larger and moreeasily visualized shift in the migration of p53 than does the~7-kD ubiquitin molecule. In addition, GST-ubiquitin^K48R does not efficiently form polyubiquitinated products, resultingin a simpler pattern of GST-ubiquitin-p53 conjugates. Figure 5A(left three lanes) shows that in the absence of 1D5 immunoprecipitate,low levels of ubiquitinated p53 could be detected in the presenceof 65 ng of recombinant p53, but not in the absence of p53 orwith 20 ng of p53. Identical background levels of p53 ubiquitinationwere observed in reactions containing no immunoprecipitates (leftthree lanes) or 1D5 immunoprecipitates from cells not expressingE4orf6 (middle three lanes). In the presence of immunoprecipitatesfrom cells expressing E4orf6 (right three lanes), significantlyhigher levels of ubiquitinated p53 were formed in reactions containingeither 20 or 65 ng of p53. As expected, formation of p53-ubiquitinconjugates depends on the presence of E1 ubiquitin-activatingenzyme, E2 ubiquitin-conjugating enzyme, and GST-ubiquitin (Fig.5B). Only background levels of ubiquitinated p53 were formed inreactions performed with immunoprecipitates from cells expressingE4orf6 alone, in the absence of other proteins of the E4orf6 complex(data not shown). Taken together, these results argue that theE4orf6 complex can function with a ubiquitin-activating enzymeand a ubiquitin-conjugating enzyme to facilitate p53 ubiquitinationin vitro, and they are consistent with the idea the E4orf6/E1B55Kcomplex targets p53 for ubiquitination and subsequent degradationvia this Cul5/Elongin BC/Rbx1 complex in cells.

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Figure 5. In vitro ubiquitination of p53 by E4orf6 complexes. (A) Lysates from Sf21 cells infected with baculoviruses encoding E1B55K, Elongin B, Elongin C, HA-Cul5, and Myc-Rbx1, with or without baculovirus encoding E4orf6, were immunoprecipitated with anti-E4orf6 antibody (1D5). Increasing amounts of purified p53 protein were incubated with the immunoprecipitates and with yUba1, hUbc5a, and GST-UbK48R in ubiquitination reaction buffer. Reaction mixtures were incubated for 30 min at 25°C and analyzed by Western blotting using anti-p53 antibody (421). (B) p53 was incubated with immunoprecipitates and with various combinations of yUba1, hUbc5a, and GST-UbK48R. The indicated components were omitted from reactions: E1, yUba1; E2, hUBC5a; GST-Ub, GST-UbK48R. HC indicates heavy chain.

Degradation of p53 by E4orf6-E1B55K requires functional Cullins

Although we have shown that E4orf6 binds to a Cul5/Elongin BC/Rbx1 complex that is capable of the in vitro ubiquitinationof p53 and that this interaction correlates with the ability ofE4orf6/E1B55K to degrade p53, we wished to show that Cullins arerequired for adenovirus-mediated p53 degradation. Some time ago,a Chinese hamster ovary (CHO) cell line, ts41, was isolated (Hirschbergand Marcus 1982). ts41 cells are temperature sensitive for progressioninto G₂/M and thus undergo multiple rounds of DNA synthesis withoutcell division (Handeli and Weintraub 1992). Recently, ts41 cellshave been shown to be defective in the NEDD8 activation pathway.The ts41 mutation can be complemented by overexpression of amyloidprecursor protein-binding protein 1 (APP-BP1), which togetherwith hUba3 forms the NEDD8-specific E1-activating enzyme (Gongand Yeh 1999; Chen et al. 2000). NEDD8, and its yeast counterpartRub1, are highly conserved ubiquitin-like proteins that, followingcleavage, are conjugated with a number of proteins (Kamitani etal. 1997). Like ubiquitination, conjugation of NEDD8 to targetproteins requires E1-3 activating, conjugating, and ligating enzymes,which are distinct from enzymes of the ubiquitin conjugation pathway(Osaka et al. 1998; Gong and Yeh 1999; for review, see Yeh etal. 2000). A number of reports now indicate that Cullins requiremodification by NEDD8 to participate in the degradation of targetproteins (Freed et al. 1999; Hori et al. 1999; Liakopoulos etal. 1999; Wada et al. 1999). Recently, it has been shown usingts41 cells that ongoing neddylation is required by the SCF andVHL-Elongin C-Cullin 2 complexes for the degradation of targetsin mammalian cells, including HIF1 $alpha$ , p27, and I $kappa$ B $alpha$ (M. Ohh, J.J.Moslehi, Y. Chen, V. Chau, M.A. Read, and W.G. Kaelin, in prep.).Thus, it appeared possible to use ts41 cells to confirm that aCullin-mediated pathway is involved in the degradation of p53by the adenovirus E4orf6/E1B55K complex. Wild-type CHO and ts41cells were incubated at 33°C, and following infection with adenovirusvectors expressing human p53 and E1B55K or E4orf6, either singlyor in combination, some cultures were shifted to the nonpermissivetemperature of 39°C. Cell extracts were prepared and analyzedby Western blotting using antibodies against p53, E4orf6, or E1B55K.Figure 6A (right panel) shows that in wild-type CHO cells, expressionof both E4orf6 and E1B55K resulted in the degradation of p53 atboth temperatures. Little degradation was apparent with E4orf6alone; however, as observed previously (Querido et al. 2001),some degradation was seen in both cell types using the E1B55Kvector alone, as low levels of E4orf6 are produced from the vectorbackbone, which contains the E4 region. In the case of ts41 cells(Fig. 6A, left panel), p53 degradation by E4orf6/E1B55K was alsoapparent at 33°C, but little degradation occurred at the nonpermissivetemperature of 39°C. Although these results leave open the possibilitythat the defect in ts41 cells also affects other targets thatare indirectly involved, they do suggest that the mechanism ofdegradation of p53 by E4orf6-E1B55 is dependent on neddylationand is likely to require functional Cullins, which are the bestknown targets of this form of modification. As we found in Figure2 that Cul5 was the only Cullin to associate with E4orf6, it islikely that Cul5 is the Cullin responsible for this process.

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Figure 6. E4orf6/E1B55K require NEDDylated Cullins to degrade p53. (A) Wild-type and ts41 Chinese hamster ovary (CHO) cells maintained at 33°C were infected with various combinations of adenovirus vectors for 48 h (see + at top). Vectors included AdrtTA (vector control), Adp53wt, AdE4orf6, and AdHH55K. Some cultures were shifted to the 39°C for the last 15 h of incubation. Whole cell extracts analyzed by Western blotting using to detect p53 (1801), E4orf6 (1807), E1B55K (2A6), and actin. (B) CHO cells infected with various combinations of adenovirus vectors (as in A). Proteasome inhibitors MG132, lactacystin, or their solvents were added for the last 6 h of infection. Cell extracts were analyzed as in A.

Treatment of CHO cells with the proteasome inhibitors lactacystin or MG132 inhibited the degradation of p53 by the E4orf6/E1B55Kcomplex (Fig. 6B), confirming that p53 turnover in these cellsrequired functionalproteasomes.

	Discussion

Top Abstract Introduction Results Discussion Materials and methods References

We and others had shown previously that the adenovirus proteins E4orf6 and E1B55K function together to promote degradationof p53; however, little was known about the mechanism of thisprocess. Our previous work using the inhibitor MG132 suggestedthat such degradation requires functional proteasomes (Queridoet al. 2001). In this report, we have presented evidence thatassembly of E4orf6 into a multiprotein complex containing E1B55K,Elongins B and C, Cul5, and Rbx1 is required for E4orf6/E1B55K-dependentp53 turnover in cells. In addition, we have shown that this E4orf6-containingcomplex functions as an E3 ubiquitin ligase that promotes ubiquitinationof p53 in vitro. As modeled in Figure 7, the E4orf6 complex isstrikingly similar to VHL and SCF E3 ubiquitin ligase complexes,in that each contains a substrate recognition module linked toa Cullin-Rbx1 subcomplex via either Elongin BC or the ElonginC-like protein Skp1. The Cks1 cyclin-dependent kinase-bindingprotein, recently shown to be required for SCF-mediated degradationof p27^Kip1 in vivo, is shown in the SCF complex (Bartek and Lukas 2001;Spruck et al. 2001). Figure 7 also shows the positions of thesubstrate (diamond), the E2-conjugating enzyme, and ubiquitinproteins based on computer modeling and the recent elucidationof the X-ray crystallographic structure of the Skp1/Skp2/Cul1/Rbx1complex (N. Zheng and N.P. Pavletich, pers. comm.). It shouldbe noted that the interaction interface between E4orf6 and theCul5/Elongin BC/Rbx1 complex has not yet been determined. E4orf6contains two putative BC-box sequences; however, the interactionbetween E4orf6 and Elongins B and C was unaffected by mutationof either BC-box sequence individually (Q. Yin, J.W. Conaway,and R.C. Conaway, unpubl.). Thus, it is possible that the interactionoccurs by a novel mechanism, and further studies will be requiredto establish the precise nature of this interaction.

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Figure 7. Parallels between the SCF, VHL, and E4orf6 ubiquitin ligase complexes. The SCF (top), VHL (middle), and E4orf6 (bottom) ubiquitin ligase complexes have been illustrated. (B) Elongin B; (C) Elongin C; (p27) p27^Kip1; (Ub) ubiquitin; (orf6) Ad5 E4orf6; (55K) Ad5 E1B55K; (Cul1) the mammalian homolog of Cdc53; and (Rbx1) Rbx1/ROC1. The architecture of the SCF complex shown is based on the X-ray structure of a Skp1/Skp2/Cul1/Rbx1 crystal determined recently (N. Zheng and N.P. Pavletich, pers. comm.). Models of the VHL and E4orf6 complexes are theoretical only, and the interaction interface between E4orf6 and the Cul5/Elongin BC/Rbx1 complex has not yet been determined.

In addition, we are still unsure of the identity of the ubiquitin-conjugating enzyme used by this complex. Our in vitro studiesused hUbc5; however, in vivo assays detected HA-E2Cdc34 in associationwith E4orf6 complexes (data not shown). Further studies will berequired to identify the conjugating enzyme(s)involved.

Several other questions also exist. Ubiquitination of p53 in vitro was observed to occur at similar levels in the presenceor absence of E1B55K (data not shown). It is possible that E4orf6present in Cul5 complexes is no longer able to bind p53 efficiently,and thus, E1B55K is required to introduce high levels of the p53substrate. Additionaly, the role of E1B55K in vivo may be to positionp53 in the complex for optimal ubiquitination. In support of thishypothesis, previous studies have shown that E1B55K and E4orf6must bind each other for p53 destabilization to occur (Cathomenand Weitzman 2000; Querido et al. 2001). Furthermore, a recentstudy of E1B55K single amino-acid substitution mutants found thatE1B55K R240A, although still able to bind E4orf6 and support virallate gene expression, was defective in binding p53 (Shen et al.2001). Significantly, an adenovirus encoding this mutant as wellas wild-type E4orf6, ONYX-051, lost the ability to target p53for degradation. It is also possible that E1B55K is required tosupply a nuclear export signal (Kratzer et al. 2000; Dosch etal. 2001). Previous studies indicated that deletion of the E4orf6NES had little effect on p53 degradation by E4orf6/E1B55K (Queridoet al. 2001); however, it is still unclear if degradation occursvia cytoplasmic proteasomes following shuttling to the cytoplasm,as is the case with MDM2-mediated p53 degradation (Lain et al.1999), or if it occurs via nuclear proteasomes. One final questionarises because of our observation that the efficiency of p53 ubiquitinationin our reconstituted system is relatively inefficient. Many SCFubiquitin ligases specifically recognize phosphorylated substrates(Patton et al. 1998). Similarly, recognition of HIF1 $alpha$ by the VHLubiquitin ligase depends on prior hydroxylation of a proline residuewithin the HIF1 $alpha$ oxygen-dependent degradation domain (Ivan etal. 2001; Jaakkola et al. 2001). By analogy, it is possible thatthe majority of the recombinant p53 used in our reactions is notappropriately modified and accordingly is not recognized by theE4orf6 complex. An interesting recent finding suggests that p53must be phosphorylated by the COP9 signalosome before being recognizedby the HPV E6/E6AP and MDM2 E3 ligases for ubiquitin-mediateddegradation to take place (Bech-Otschir et al. 2001). This ora related process may represent a general requirement for degradationof p53 by ubiquitin-dependent pathways and may explain the lowlevels of p53 ubiquitination observed in vitro. Alternatively,efficient ubiquitination of p53 may require additional activitiesnot present in our reconstitutedreactions.

Information on the mechanism of action of viral proteins has often led to insights into previously unrecognized normal cellularpathways. The present studies indicate that E4orf6 may have evolvedfunctions that parallel those of unidentified cellular regulatorsof p53 degradation. It is tempting to speculate that cells maycontain cellular E4orf6 homologs that function with Cullin-containingcomplexes to regulate the degradation ofp53.

	Materials and methods

Top Abstract Introduction Results Discussion Materials and methods References

Cells

Human small cell carcinoma H1299 cells carrying a homologous deletion of the p53 gene (Mitsudomi et al. 1992), CHO cells,and derivative ts41 cells (Hirshberg and Marcus 1982) were maintainedin Dulbecco's modified Eagle's medium (GIBCO BRL) supplementedwith 10% fetal calf serum (CanSera). Sf21 insect cells were culturedas described previously (Kamura et al. 1998).

Vectors

The adenovirus vectors used in this study are derivatives of vectors described by Bacchetti and Graham (1993). They are deletedin the E1 and E3B regions, and the gene of interest is insertedin the E1 region under the cytomegalovirus (CMV) promoter. Becausethe E1A coding region is absent, the resident Ad5 vector genesare expressed at almost undetectable levels. AdLacZ expressesthe Escherichia coli $beta$ -galactosidase gene, and Adp53wt expresseshuman wild-type p53 (Bacchetti and Graham 1993). The adenovirusvectors AdHH55K, expressing HMK and histidine-tagged Ad5 E1B55K,and AdE4orf6, expressing Ad5 E4orf6, were described previously(Querido et al. 1997a). AdrtTA, which was used as a control vectorin some cases, expresses reverse tetracycline transactivator protein(Gossen et al. 1995) and was produced by standard methods (Bettet al. 1994). The HPC4-Elongin B, HSV-Elongin C, and MYC-Rbx1baculovirus vectors are described in Kamura et al. (1999), andthe HA-Cul5 baculovirus vector is described in Kamura et al. (2001).E4orf6 and E1B55K were subcloned into BacPAK8, and recombinantbaculoviruses were generated with the BacPAK baculovirus expressionsystem (Clontech). HA-Cul2 and HA-Cul5 were expressed in mammaliancells using pcDNA3 and pCI-neo vectors, respectively. The followingplasmids were also used: MycRbx1 encodes myc-tagged murine Rbx1(Kamura et al. 1999), HA-E2cdc34 expresses HA-tagged human E2cdc34(Lisztwan et al. 1998), and Flag-VHL encodes human Flag-taggedVHL (Kamura et al. 1999). Plasmids encoding human Cul1, Cul2,Cul3, and Cul5 and mouse Cul4A, are described in Michel and Xiong(1998). The plasmid pcDNA3 p53 wt encodes human wild-type p53,and pCA14 HH55K encodes HMK and histidine-tagged Ad5 E1B55K. ThepcDNA3 E4orf6 wild-type plasmid, as well as all in-frame deletionmutants generated using PCR-based protocols, are described inQuerido et al. 2001.

Antisera

Anti-E4orf6 mouse monoclonal antibody 1D5 was described in Querido et al. (2001), and E4orf6-specific rabbit polyclonal antibody1807 was described in Boivin et al. (1999). Anti-p53 pAb421 andpAb1801 hybridoma supernatants were prepared as described in Queridoet al. (2001). E1B55K was detected with the 2A6 monoclonal antibody(Sarnow et al. 1982). Anti-Elongin A, anti-Elongin B, and anti-ElonginC goat polyclonal antibodies were purchased from Santa Cruz Biotechnology,and Ig32 anti-VHL mouse monoclonal antibody was from Pharmingen.The rabbit polyclonal antibody generated against the C terminusof rabbit VACM-1 was a generous gift from Maria Burnatowska-Hledin(Hope College, Holland, MI). A rabbit polyclonal antibody againsthuman Cul5 was made for us by Genemed Synthesis Inc. using a syntheticpeptide (EHKIRRDESDINTFIYMA) corresponding to the C terminus ofhuman Cul5. Anti-Myc 9E10 antibody (Santa Cruz), anti-HA mousemonoclonal HA.11 (BAbCO) and mouse monoclonal 12CA5 (Boehringer-Mannheim),and anti-Flag M2 antibody (Sigma), were used to detect the taggedepitopes. The anti- $gamma$ -actin mouse monoclonal antibody was a generousgift from Gordon Shore (McGill University, Quebec,Canada).

Identification of E4orf6-binding proteins

H1299 cells growing on 100-mm-diameter dishes (Corning Glass Works, NY) were infected at a multiplicity of infection (MOI)of 30 plaque-forming units (pfu) per cell with the indicated adenovirusvectors. Cell cultures were labeled from 18 to 22 h postinfectionwith 200 µCi per plate of [35S]methionine/[35S]cysteine EasyTagExpress protein labeling mix (>1000 Ci/mmole; DuPont NEN) in methionine/cysteine-freemedium. Whole cell extracts were then prepared in nonionic detergentlysis buffer X (50 mM Tris-HCl at pH 8.0, containing 250 mM NaCl,1% NP-40, 1 mM EDTA, 1 mM EGTA, and 2 µg/mL each of aprotinin,leupeptin, and pepstatin), immunoprecipitated using 1D5 anti-E4orf6antibody, and analyzed by SDS-PAGE and autoradiography, as describedpreviously (Boivin et al. 1999). Prestained standard size markers(Bio-Rad) were used, and their positions are indicated in Figure1A. The potential identities shown for the p84, p19, and p14 specieswere derived from mass spectroscopy analysis of tryptic peptidesderived from gel-purified material (Borealis Biosciences, Toronto,Canada). For the analysis of complex formation using E4orf6 deletionmutants, a study similar to that of Figure 1A was performed inH1299 cells, except that cells in 100-mm-diameter plates weretransfected according to the GIBCO BRL Lipofectin protocol with10 µg of pcDNA3 plasmid DNA encoding wild-type or mutantE4orf6.

E4orf6 protein-binding assays

In some cases, H1299 cells growing in 100-mm-diameter dishes were infected with adenovirus vectors, whereas in other cases,H1299 cells were seeded in 60-mm plates and lipofected accordingto the GIBCO BRL Lipofection protocol with 2 µg total of plasmidDNA. After 24 h, whole cell extracts were prepared in buffer X,immunoprecipitations were performed with the indicated antibodies,and samples were separated by SDS-PAGE. Following transfer tonitrocellulose (Schleicher & Schuell/Optitran), Western blottingwas performed, and species were visualized by enhanced chemiluminescence(NEN LifeScience). For the binding assays of E4orf6 with the variousCullins, immunoprecipitates were prepared from AdLacZ- or AdE4orf6-infectedH1299 cells using 1D5 anti-E4orf6 antibody. Following the finalwash, the precipitates were divided into five equal portions,resuspended in 100 µL of buffer X and combined with a 10 µL aliquotof samples containing various Cullins, human Cul1, Cul2, Cul3,and Cul5 and mouse Cul4A (Michel and Xiong 1998), which were synthesizedusing a standard in vitro transcription/translation kit (TnT,Promega) in the presence of 40 µCi of translation grade [35S]methionine(Dupont-NEN). The mixtures were incubated at room temperaturefor 1 h, and after five washes with buffer X, the precipitateswere separated by SDS-PAGE. The presence of labeled Cullins wasassessed byautoradiography.

In vivo p53 degradation assays

The E4orf6/E1B55K-induced p53 turnover was studied using either plasmids or adenovirus vectors to introduce the viral proteinsand p53 into cells, as described more fully in Querido et al.(2001). H1299 cells were grown on 60-mm dishes and transfectedusing 12 µL of Lipofectin reagent (GIBCO BRL) with the followingplasmid DNAs: 1 µg of pcDNA3 p53wt, 4 µg of pCA14 HH55K, and 4µg of pcDNA3 E4orf6 (expressing wild-type or mutant E4orf6 proteins).Total plasmid DNA was kept equal by adding empty pcDNA3 plasmidDNA. Expression from all plasmid DNAs was under the CMV promoter.After 24 h, cells were harvested and lysed in Western blot lysisbuffer (50 mM HEPES at pH 7.9, containing 400 mM KCl, 0.1% NP-40,4 mM NaF, 4 mM NaVO₄, 0.2 mM EDTA, 0.2 mM EGTA, 2 mg/mL aprotinin,leupeptin, and pepstatin, and 1 mM dithiothreitol). Protein concentrationswere measured by the Bradford assay (Bio-Rad), and 40 µg of eachextracts was separated by SDS-PAGE and immunoblotted with anti-p53,anti-E1B55K, or anti-E4orf6 antibody. The E4orf6 immunoblots werechecked for the equivalent expression of each E4orf6 mutant, andthe E1B55K expression, which did not vary, allowed us to verifyequal transfection efficiency. Equal sample loading was verifiedby staining the membranes with Ponceau S red (Sigma) after transfer.Wild-type CHO cells and ts41 cells (Hirschberg and Marcus 1982)were infected with various combinations of adenovirus vectorsat an MOI of 90 pfu per cell for each virus. Vectors includedAdrTTA, Adp53wt, AdE4orf6, and AdHH55K. The total amount of viruswas kept constant at 270 pfu per cell by adding AdrTTA (vectorcontrol) virus as needed. Cells were harvested 48 h after infection,and cell extracts were prepared and analysed as above. Westernblotting was performed with anti-p53, anti-E1B55K, anti-E4orf6,or anti-actin antibody. In some cases, wild-type CHO cells werealso treated with proteasome inhibitors MG132 (20 µM, Calbiochem),lactacysteine (20 µM, Calbiochem) or their solvents, ethanol (0.2%)and DMSO (0.2%) for the last 6 h ofinfection.

Reconstitution of E4orf6 complexes in Sf21 cells

Plates containing 1 × 10⁶ Sf21 cells were infected with baculoviruses encoding various proteins. Cells were lysed in 1 mL of40 mM HEPES-NaOH (pH 7.9), containing 150 mM NaCl, 1 mM DTT, 0.5%(v/v) Triton X-100, 10% (v/v) glycerol, 5 µg/mL leupeptin, 5 µg/mLantipain, 5 µg/mL pepstatin A, and 5 µg/mL aprotinin. Approximately100 µg of Sf21 cell lysate was immunoprecipitated with either2 µg of anti-HA (12CA5) or 2 µg of anti-E4orf6 (1D5) antibodyand 10 µL of protein A Sepharose. Crude lysates and washed immunecomplexes were separated by SDS-PAGE and immunoblotted with theindicatedantibodies.

In vitro p53 ubiquitination assay

Lysates from Sf21 cells infected with baculoviruses encoding E1B55K, Elongin B, Elongin C, HA-Cul5, and Rbx1, with or withoutE4orf6 baculovirus, were immunoprecipitated with 1D5 antibody.To the precipitates was added 0, 20, or 65 ng of recombinant histidine-taggedp53 protein (Wang et al. 1993) that had been expressed in insectcells and purified by nickel chromatography, as described previously(Kamura et al. 1999) and the mixtures were incubated with 50 ngof yUba1, 100 ng of hUbc5a, or 500 ng of GST-UbK48R in 10 µL ofubiquitination reaction buffer (40 mM HEPES-NaOH at pH 7.9, containing60 mM potassium acetate, 2 mM DTT, 6 mM MgCl₂, and 0.5 mM EDTAat pH 7.9, 10% [v/v] glycerol, and 1.5 mM ATP). Reaction mixtureswere incubated for 30 min at 25°C, separated by SDS-PAGE, andanalyzed by Western blotting with anti-p53 antibody(pAB421).

Confocal microscopy

H1299 cells were seeded in four-chamber culture slides (Falcon) and transfected with 0.4 µg of plasmid DNA according to theGIBCO BRL Lipofection protocol. After 24 h, cells were fixed with4% paraformaldehyde and permeabilized with PBS 0.1% Triton X-100.A solution of PBS with 3% bovine serum albumin was used for blockingand antibody incubation. E4orf6 was detected using rabbit polyclonal1807 antibody and Alexa 594 (red) anti-rabbit IgG antibody (MolecularProbes). Recombinant Cullin proteins tagged with the HA epitopewere detected using mouse monoclonal anti-HA.11 antibody (BAbCO)and Alexa 488 (green) anti-mouse antibody (Molecular Probes).The fluorophores were visualized using a laser confocal Zeissmicroscope.

	Acknowledgments

We wish to thank Rachael Neve for ts41 cells; Maria Burnatowska-Hledin for the rabbit VACM-1 antibodies; Yue Xiong for plasmidsexpressing human Cul1, Cul2, Cul3, and Cul5 and murine Cul4A;Peter Tegtmeyer for the p53 baculovirus; Wilhelm Krek for theplasmid expressing HA-E2Cdc34; and Dennis Takayesu for technicalassistance. We also thank Ning Zheng and Nikola Pavletich forinformation about their structure of the SCF complex before publication.This work was supported by grants from the Canadian Institutesof Health Research and the National Cancer Institute of Canada(P.E.B.) and the National Institute of General Medicine (GM41628,R.C.C.). This work was performed while J.W.C. was an associateinvestigator of the Howard Hughes Medical Institute. E.Q. wassupported by a studentship from the Fonds FRSQ-FCAR-Santé du Québec;and P.B., a postdoctoral fellowship from Défi CorporatifCanderel.

The publication costs of this article were defrayed in part by payment of page charges. This article must therefore be herebymarked "advertisement" in accordance with 18 USC section 1734solely to indicate thisfact.

	Footnotes

Received July 6, 2001; revised version accepted October 10, 2001.

⁸ Present address: Cold Spring Harbor Laboratory, 1 Bungtown Road, P.O. Box 100, Cold Spring Harbor, NY 11724,USA.

⁹ Correspondingauthor.

E-MAIL branton{at}med.mcgill.ca; FAX (514) 398-8845.

Article and publication are at http://www.genesdev.org/cgi/doi/10.1101/gad.926401.

References

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Abstract
Introduction
Results
Discussion
Materials and methods
References

Aso, T., Haque, D., Barstead, R.J., Conaway, R.C., and Conaway, J.W. 1996. The inducible elongin A elongation activation domain: Structure, function, and interaction with the elongin BC complex. EMBO J. 15: 5557-5566[Medline].
Bacchetti, S. and Graham, F.L. 1993. Inhibition of cell proliferation by an adenovirus vector expressing the human wild type p53 protein. Int. J. Oncol. 3: 781-788.
Bargonetti, J., Reynisdottir, I., Friedman, P.N., and Prives, C. 1992. Site-specific binding of wild-type p53 to cellular DNA is inhibited by SV40 T antigen and mutant p53. Genes & Dev. 6: 1886-1898[Abstract/Free Full Text].
Bartek, J. and Lukas, J. 2001. p27 destruction: Cks1 pulls the trigger. Nat. Cell Biol. 3: E95-E98[Medline].
Bech-Otschir, D., Kraft, R., Huang, X., Henklein, P., Kapelari, B., Pollmann, C., and Dubiel, W. 2001. COP9 signalosome-specific phosphorylation targets p53 to degradation by the ubiquitin system. EMBO J. 20: 1630-1639[CrossRef][Medline].
Bett, A.J., Haddara, W., Prevec, L., and Graham, F.L. 1994. An efficient and flexible system for construction of adenovirus vectors with insertions or deletions in early regions 1 and 3. Proc. Natl. Acad. Sci. 91: 8802-8806[Abstract/Free Full Text].
Boivin, D., Morrison, M.R., Marcellus, R.C., Querido, E., and Branton, P.E. 1999. Analysis of synthesis, stability, phosphorylation, and interacting polypeptides of the 34-kilodalton product of open reading frame 6 of the early region 4 protein of human adenovirus type 5. J. Virol. 73: 1245-1253[Abstract/Free Full Text].
Brower, C.S., Shilatifard, A., Mather, T., Kamura, T., Takagi, Y., Haque, D., Treharne, A., Foundling, S.I., Conaway, J.W., and Conaway, R.C. 1999. The elongin B ubiquitin homology domain: Identification of Elongin B sequences important for interaction with Elongin C. J. Biol. Chem. 274: 13629-13636[Abstract/Free Full Text].
Burnatowska-Hledin, M., Spielman, W.S., Smith, W.L., Shi, P., Meyer, J.M., and Dewitt, D.L. 1995. Expression cloning of an AVP-activated calcium-mobilizing receptor from rabbit kidney medulla. Am. J. Physiol. 268: F1198-F1210[Abstract/Free Full Text].
Burnatowska-Hledin, M., Lazdins, I.B., Listenberger, L., Zhao, P., Sharangpani, A., Folta, V., and Card, B. 1999. VACM-1 receptor is specifically expressed in rabbit vascular endothelium and renal collecting tubule. Am. J. Physiol. 276: F199-F209[Abstract/Free Full Text].
Byrd, P.J., Stankovic, T., McConville, C.M., Smith, A.D., Cooper, P.R., and Taylor, A.M. 1997. Identification and analysis of expression of human VACM-1, a cullin gene family member located on chromosome 11q22-23. Genome Res. 7: 71-75[Abstract/Free Full Text].
Cathomen, T. and Weitzman, M.D. 2000. A functional complex of adenovirus proteins E1B-55kDa and E4orf6 is necessary to modulate the expression level of p53 but not its transcriptional activity. J. Virol. 74: 11407-11412[Abstract/Free Full Text].
Chen, Y., McPhie, D.L., Hirschberg, J., and Neve, R.L. 2000. The amyloid precursor protein-binding protein APP-BP1 drives the cell cycle through the S-M checkpoint and causes apoptosis in neurons. J. Biol. Chem. 275: 8929-8935[Abstract/Free Full Text].
Chiou, S.-K. and White, E. 1997. p300 binding by E1A cosegregates with p53 induction but is dispensable for apoptosis. J. Virol. 71: 3515-3525[Abstract].
Cockman, M.E., Masson, N., Mole, D.R., Jaakkola, P., Chang, G.-W., Clifford, S.C., Maher, E.R., Pugh, C.W., Ratcliffe, P.J., and Maxwell, P.H. 2000. Hypoxia inducible factor- $alpha$ binding and ubiquitylation by the von Hippel-Lindau tumor suppressor protein J. Biol. Chem. 275: 25733-25741[Abstract/Free Full Text].
Dobbelstein, M., Roth, J., Kimberly, W.T., Levine, A.J., and Shenk, T. 1997. Nuclear export of the E1B-55-kDa and E4 34-kDa adenoviral oncoproteins mediated by a rev-like signal sequence. EMBO J. 16: 4276-4282[CrossRef][Medline].
Dobner, T., Horikoshi, N., Rubenwolf, S., and Shenk, T. 1996. Blockage by adenovirus E4orf6 of transcriptional activation by the p53 tumor suppressor. Science 272: 1470-1473[Abstract].
Dosch, T., Horn, F., Schneider, G., Kratzer, F., Dobner, T., Hauber, J., and Stauber, R.H. 2001. The adenovirus type 5 E1B-55K oncoprotein actively shuttles in virus-infected cells, whereas transport of E4orf6 is mediated by a CRM1-independent mechanism. J. Virol. 75: 5677-5683[Abstract/Free Full Text].
Duan, D.R., Pause, A., Burgess, W.H., Aso, T., Chen, D.Y., Garrett, K.P., Conaway, R.C., Conaway, J.W., Linehan, W.M., and Klausner, R.D. 1995. Inhibition of transcriptional elongation by the VHL tumor suppressor protein. Science 269: 1402-1406[Abstract/Free Full Text].
Freed, E., Lacey, K.R., Huie, P., Lyapina, S.A., Deshaies, R.J., Stearns, T., and Jackson, P.K. 1999. Components of an SCF ubiquitin ligase localize to the centrosome and regulate the centrosome duplication cycle. Genes & Dev. 13: 2242-2257[Abstract/Free Full Text].
Fuchs, S.Y., Adler, V., Buschmann, T., Yin, Z., Wu, X., Jones, S.N., and Ronai, Z. 1998. JNK targets p53 ubiquitination and degradation in nonstressed cells. Genes & Dev. 12: 2658-2663[Abstract/Free Full Text].
Gonen, H., Shkedy, D., Barnov, S., Kosower, N.S., and Ciechanover, A. 1997. On the involvement of calpains in the degradation of the tumor suppressor protein p53. FEBS Lett. 406: 17-22[CrossRef][Medline].
Gong, L. and Yeh, E.T.H. 1999. Identification of the activating and conjugating enzyme of the NEDD conjugation pathway. J. Biol. Chem. 274: 12036-12042[Abstract/Free Full Text].
Goodrum, F.D., Shenk, T., and Ornelles, D.A. 1996. Adenovirus early region 4 34-kilodalton protein directs the nuclear localization of the early region 1B 55-kilodalton protein in primate cells. J. Virol. 70: 6323-6335[Abstract].
Gossen, M., Freundlieb, S., Bender, G., Muller, G., Hillen, W., and Bujard, H. 1995. Transcriptional activation by tetracyclines in mammalian cells. Science 268: 1766-1769[Abstract/Free Full Text].
Handeli, S. and Weintraub, H. 1992. The ts41 mutation in Chinese hamster cells leads to successive phases in the absence of intervening G2, M, and G1. Cell 71: 599-611[CrossRef][Medline].
Harlow, E., Franza, B.R., Jr., and Schley, C. 1985. Monoclonal antibodies specific for adenovirus early region 1A proteins: Extensive heterogeneity in early region E1A products. J. Virol. 55: 533-546[Abstract/Free Full Text].
Hirschberg, J. and Marcus, M. 1982. Isolation by a replica-plating technique of Chinese hamster temperature-sensitive cell cycle mutants. J. Cell. Physiol. 113: 159-166[CrossRef][Medline].
Honda, R., Tanaka, H., and Yasuda, H. 1997. Oncoprotein MDM2 is a ubiquitin ligase E3 for tumor suppressor p53. FEBS Lett. 420: 25-27[CrossRef][Medline].
Hori, T., Osaka, F., Chiba, T., Miyamoto, C., Okabayashi, K., Shimbara, N., Kato, S., and Tanaka, K. 1999. Covalent modification of all members of human cullin family proteins by NEDD8. Oncogene 18: 6829-6834[CrossRef][Medline].
Ivan, M., Kondo, K, Yang, H., Kim, W., Valiando, J., Ohh, M., Salic, A., Asara, J.M., Lane, W.S., and Kaelin, W.G., Jr. 2001. HIF $alpha$ targeted for VHL-mediated destruction by proline hydroxylation: Implications for O₂ sensing. Science 292: 464-468[Abstract/Free Full Text].
Iwai, K., Yamanaka, K., Kamura, T., Minato, N., Conaway, R.C., Conaway, J.W., Klausner, R.D., and Pause, A. 1999. Identification of the von Hippel-Lindau tumor suppressor protein as the substrate recognition subunit of an E3 ubiquitin ligase complex. Proc. Natl. Acad. Sci. 96: 12436-12441[Abstract/Free Full Text].
Jaakkola, P., Mole, D.R., Tian, Y.M., Wilson, M.I., Gielbert, J., Gaskell, S.J., von Kriegsheim, A., Hebestreit, H.F., Mukherji, M., Schofield, C.J. et al. 2001. Targeting of HIF- $alpha$ to the von Hippel-Lindau ubiquitylation complex by O₂-regulated prolyl hydroxylation. Science 292: 468-472[Abstract/Free Full Text].
Kamitani, T., Kito, K., Nguyen, H.P., and Yeh, E.T. 1997. Characterization of NEDD8, a developmentally down-regulated ubiquitin-like protein. J. Biol. Chem. 272: 28557-28562[Abstract/Free Full Text].
Kamura, T., Sato, S., Haque, D., Liu, L., Kaelin, W.G., Conaway, R.C., and Conaway, J.W. 1998. The Elongin BC complex interacts with the conserved SOCS-box motif present in members of the SOCS, ras, WD-40 repeat, and ankyrin repeat families. Genes & Dev. 12: 3872-3881[Abstract/Free Full Text].
Kamura, T., Koepp, D.M., Conrad, M.N., Skowyra, D., Moreland, R.J., Iliopoulos, O., Lane, W.S., Kaelin, W.G., Elledge, S.J., Conaway, R.C. et al. 1999. Rbx1, a component of the VHL tumor suppressor complex and SCF ubiquitin ligase. Science 284: 657-661[Abstract/Free Full Text].
Kamura, T., Sato, S., Iwai, K., Czyzyk-Krzeska, M., Conaway, R.C., and Conaway, J.W. 2000. Activation of HIF1 $alpha$ ubiquitination by a reconstituted von Hippel-Lindau (VHL) tumor suppressor complex. Proc. Natl. Acad. Sci. 97: 10430-10435[Abstract/Free Full Text].
Kamura, T., Burian, D., Yan, Q., Schmidt, S.L., Lane, W.S., Querido, E., Branton, P.E., Shilatifard, A., Conaway, R.C., and Conaway, J.W. 2001. MUF1, a novel elongin BC-interacting leucine-rich repeat protein that can assemble with Cul5 and Rbx1 to reconstitute a ubiquitin ligase. J. Biol. Chem. 276: 29748-29753[Abstract/Free Full Text].
Kibel, A., Iliopoulos, O., DeCaprio, J.A., and Kaelin, W.G. 1995. Bindin

RESEARCH PAPER Degradation of p53 by adenovirus E4orf6 and E1B55K proteins occurs via a novel mechanism involving a Cullin-containing complex

RESEARCH PAPER
Degradation of p53 by adenovirus E4orf6 and E1B55K proteins occurs via a novel mechanism involving a Cullin-containing complex