Analyses of Single-Amino-Acid Substitution Mutants of Adenovirus Type 5 E1B-55K Protein

doi:10.1128/JVI.75.9.4297-4307.2001

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Journal of Virology, May 2001, p. 4297-4307, Vol. 75, No. 9
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.9.4297-4307.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Analyses of Single-Amino-Acid Substitution Mutants of Adenovirus Type 5 E1B-55K Protein

Yuqiao Shen,^* Galila Kitzes, Julie A. Nye, Ali Fattaey, and Terry Hermiston

ONYX Pharmaceuticals, Inc., Richmond, California 94806

Received 1 September 2000/Accepted 6 February 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The E1B-55K protein plays an important role during human adenovirus type 5 productive infection. In the early phase of theviral infection, E1B-55K binds to and inactivates the tumor suppressorprotein p53, allowing efficient replication of the virus. Duringthe late phase of infection, E1B-55K is required for efficientnucleocytoplasmic transport and translation of late viral mRNAs,as well as for host cell shutoff. In an effort to separate thep53 binding and inactivation function and the late functions ofthe E1B-55K protein, we have generated 26 single-amino-acid mutationsin the E1B-55K protein. These mutants were characterized for theirability to modulate the p53 level, interact with the E4orf6 protein,mediate viral late-gene expression, and support virus replicationin human cancer cells. Of the 26 mutants, 24 can mediate p53 degradationas efficiently as the wild-type protein. Two mutants, R240A (ONYX-051)and H260A (ONYX-053), failed to degrade p53 in the infected cells.In vitro binding assays indicated that R240A and H260A bound p53poorly compared to the wild-type protein. When interaction withanother viral protein, E4orf6, was examined, H260A significantlylost its ability to bind E4orf6, while R240A was fully functionalin this interaction. Another mutant, T255A, lost the ability tobind E4orf6, but unexpectedly, viral late-gene expression wasnot affected. This raised the possibility that the interactionbetween E1B-55K and E4orf6 was not required for efficient viralmRNA transport. Both R240A and H260A have retained, at least partially,the late functions of wild-type E1B-55K, as determined by theexpression of viral late proteins, host cell shutoff, and lackof a cold-sensitive phenotype. Virus expressing R240A (ONYX-051)replicated very efficiently in human cancer cells, while virusexpressing H260A (ONYX-053) was attenuated compared to wild-typevirus dl309 but was more active than ONYX-015. The ability toseparate the p53-inactivation activity and the late functionsof E1B-55K raises the possibility of generating adenovirus variantsthat retain the tumor selectivity of ONYX-015 but can replicatemore efficiently than ONYX-015 in a broad spectrum of celltypes.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The E1B-55K protein plays an important role during the productive infection of human adenovirus type 5 (Ad5). In the earlyphase of infection, E1B-55K forms a stable complex with p53 (32)and inhibits p53-mediated transcriptional activation (38, 40).Furthermore, E1B-55K and another adenoviral protein, E4orf6, cooperateto relocate p53 to the cytoplasm for active degradation (25,28, 35). This inactivation of p53 is critical for the productivereplication of adenovirus, which requires cells to enter the Sphase. During the late phase of infection with Ad5, viral mRNAsare selectively exported to the cytoplasm and are efficientlytranslated, while the nucleocytoplasmic transport of most hostcell mRNAs is inhibited (2, 4, 24). This selective accumulationof viral mRNAs during the late phase of infection is mediatedby a protein complex that includes E1B-55K and E4orf6 (6, 12,21, 31). This complex actively shuttles between the nucleusand the cytoplasm, serving as a nucleocytoplasmic transporterfor viral mRNAs (7). The E1B-55K protein has also been demonstratedto directly inhibit host cell protein synthesis (host cell shutoff),which ensures that the cellular resources are used for viral replication(1).

ONYX-015, originally named dl1520, is a mutant adenovirus that does not express the E1B-55K protein (3). This virus containsa stop codon immediately following the translation initiationcodon ATG, plus a large deletion of the E1B-55K coding sequence.These mutations result in the complete abrogation of E1B-55K expressionbut do not alter the expression of the E1B-19K protein encodedby an overlapping open reading frame. Consequently, this viruslacks the ability to bind and inactivate p53, allowing it to replicateefficiently only in tumor cells that are defective in p53 functionbut not in normal cells where p53 function is normal (5, 15,26). This forms the foundation of utilizing ONYX-015 as an anti-tumoragent. Phase III clinical trials with ONYX-015 in the treatmentof human head-and-neck carcinomas in combination with chemotherapyareongoing.

Lack of E1B-55K function in ONYX-015 results in defective cytoplasmic accumulation and translation of the viral late mRNAs,as well as diminished host cell shutoff, compromising the abilityof the mutant virus to reproduce itself (13). Thus, it wouldbe highly desirable to create an E1B-55K mutant that fails tobind and inactivate p53 yet retains the late functions. Such mutationswould allow the virus to replicate selectively in cells that aredeficient in p53 function without compromising the ability ofthe virus to replicate in tumor cells. Creation of such mutationswill also allow us to further elucidate the mechanism of ONYX-015'stumor cell selectivity, as several groups have described in vitrostudies showing that the host range specificity of ONYX-015 isindependent of p53 gene status (9, 13, 14, 29). It hasbeen argued that the loss of E1B-55K's RNA transport activity,rather than its p53 binding and inactivation function, may accountfor the tumor cell specificity of ONYX-015. Separating these twofunctions of E1B-55K would allow us to begin to distinguish thesepossibilities.

The regions of the E1B-55K protein responsible for p53 binding, viral mRNA transport, and host cell shutoff appear to overlap(Fig. 1). The region of E1B-55K that mediates its interactionwith p53 has been mapped to amino acids 224 to 354 (19, 39).The same region appears to be critical for E1B-55K's ability tomediate mRNA transport. The regions required for E4orf6 binding(30), the regions required to bind E1B-AP5, a cellular proteinimplicated in nucleocytoplasmic transport (8), and the regionsof E1B-55K that have putative RNA binding capability (17) allpartially overlap with the region required for p53 binding. Thusfar, all efforts to separate the p53 binding and inactivationand the late functions of the protein have been unsuccessful.

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FIG. 1. Amino acid sequence of the E1B-55K protein of Ad5. The region for p53 binding (19) is underlined, the putative RNA-binding domains (K. Leppard, personal communication) are indicated by the solid boxes, and the region required for transcription repression (P. E. Branton, personal communication) is defined by a broken box. Asterisks indicate amino acids that are mutated.

In this study, we have constructed a series of single-amino-acid substitution mutations in the p53-binding domain and thetranscriptional repression domain of the E1B-55K protein. Thesemutations were recombined into an infectious virus (dl309) background,and the resulting mutant adenoviruses were characterized for theirabilities to modulate the p53 level, interact with the E4orf6protein, mediate viral late functions, and support virus replicationin human cancer cells. Two E1B-55K mutants, R240A and H260A, appearedto lose the ability to inactivate p53 but retained, at least partially,the late functions of the wild-type protein. R240A fully restoredthe wild-type replication capacity of ONYX-015 in human cancercells, while H260A did so only partially. The ability to separatethe p53-inactivation activity and the late functions of E1B-55Kraises the possibility of creating adenovirus variants that replicatemore efficiently than ONYX-015 but retain the tumor selectivityof ONYX-015.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Tumor cell lines and culturing conditions. A549, 293, U2OS, DU145, and H1299 cells were obtained from the American Type Culture Collection. HCT116^/, a derivative of HCT116 with p53 gene knock-out, is a generousgift from F. McCormick, University of California $---$ San Francisco.All cells were grown as monolayer cultures in Dulbecco's modifiedEagle's medium (DMEM) supplemented with 10% fetal bovine serum(FBS), 100 µg of nonessential amino acids per ml, 10 U of penicillinper ml, and 10 µg of streptomycin per ml. All adenovirus infectionswere performed in DMEM-high glucose supplemented with 2% FBS,2 mM L-glutamine, 100 µg of nonessential amino acids per ml, 10U of penicillin per ml, and 10 µg of streptomycin perml.

Construction of E1B-55K alanine mutation viruses. All E1B-55K mutants were generated using Stratagene's QuikChange Site-Directed Mutagenesis kit following the manufacturer'srecommended protocol. For each mutation, a forward primer anda reverse primer were used. The mutations and their respectiveprimers are summarized in Table 1. Briefly, 20 ng of pXC-1 wasused as the template, and the cycling parameters were as follows:1 cycle of 95°C for 30 s, and 16 cycles of 95°C for 30 s, 55°Cfor 1 min, and 68°C for 20 min. The parental DNA was digestedby adding 10 U of DpnI to each sample and incubating it for 1h at 37°C. Final products were transformed into XL-1 cells andconfirmed by DNA sequencing. Viruses were constructed by cotransfectingpJM17 with plasmids containing the mutations (22) into 293 cells.Two rounds of plaque purification were done to rule out wild-typecontamination. Mutations were confirmed by PCR followed by sequencingof the E1B-55K region. All viruses, including WtD, dl309, ONYX-015,and the mutant viruses created in this study, were propagatedin 293 cells, purified on CsCl gradients (as described in reference36), and quantified by plaque assays on 293 cells.

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TABLE 1. Primer sequences of the mutations^a

Western blot analysis. A549 cells were infected with various viruses at a multiplicity of infection (MOI) of 10. At 24 h postinfection, the cellswere lysed in sodium dodecyl sulfate (SDS) gel loading buffer(100 mM Tris-Cl [pH 6.8], 5 mM EDTA, 1% SDS, 5% $beta$ -mercaptoethanol).Proteins were fractionated by electrophoresis on Bio-Rad precastprotein gels. After electrophoresis, the proteins were electrophoreticallytransferred to nylon membranes. Blots were then incubated withantibodies diluted in phosphate-buffered saline (PBS) containing1% dry milk and 0.1% Tween-20 and were visualized by ECL (Amersham).Anti-p53 antibody DO-1 (Calbiochem) was diluted 1:1,000; anti-E1B-55Kantibody 2A6 (33) and anti-E2A antibody B6-6 (generous giftfrom A. J. Levine, Rockefeller University) tissue culture supernatantswere diluted 1:10; rabbit anti-fiber antibody (American Qualex)was used at 1:1,000.

Assays for protein interactions. A549 cells were infected at an MOI of 10. At 24 h postinfection, cells were radiolabeled for 3 h at 37°C with methionine-and cysteine-free DMEM supplemented with 2% dialyzed FBS and 100µCi of [³⁵S]-express labeling mix (DuPont) per ml. Labeled cells were washedwith cold saline, harvested, and solubilized in a solution containing50 mM Tris-Cl (pH 8.0), 5 mM EDTA, 150 mM NaCl, 0.5% NP-40, 3mM 2-mercaptoethanol, and 1× EDTA-free protease inhibitor mix(Boehringer Mannheim). Cell lysates were cleared by microcentrifugationfor 10 min. Immunoprecipitations were carried out as describedpreviously (34). Antibodies against p53 (mAb421) or E1B-55K(2A6) were used to bring down the protein complex. Proteins wereseparated by SDS-4 to 20% polyacrylamide gel electrophoresis (PAGE)(Bio-Rad) and visualized byautoradiography.

Binding of E4orf6 by various E1B-55K mutants was examined by immunoprecipitation followed by Western blotting. A549 cellswere infected and lysed as described above, except that cellswere not labeled with radioisotope. Cleared cell extracts wereimmunoprecipitated with the anti-E1B-55K antibody 2A6. The precipitatedmaterials were separated by SDS-PAGE (a 4 to 20% gradient gel)and analyzed by Western blotting either with (i) a polyclonalantibody against E4orf6, 1807-3 (a generous gift from P. E. Branton,McGill University), or with (ii) rat anti-E1B-55K antibody (agenerous gift from C. O'Shea, University of California $---$ SanFrancisco).

In vitro binding experiments were performed essentially as described earlier (37). A549 cells were infected and lysed asdescribed above, except that cells were not labeled with radioisotope.Cleared cell extracts were mixed with in vitro-labeled p53 (generatedand labeled with [³⁵S]methionine by transcription and translation in vitro [TNT T3-system;Promega]). The mixtures were incubated at 30°C for 30 min, followedby immunoprecipitation with the monoclonal anti-E1B-55K antibody2A6 and four washing steps with the lysis buffer. p53 coprecipitatedalong with E1B-55K protein was resolved on a 10% precast proteingel (Bio-Rad) and was detected byfluorography.

Indirect immunofluorescent staining. A549 and U2OS cells were seeded on Lab-Tek II chamber slides the day before infection to roughly 60% confluency. Cells werethen infected at an MOI of 10 with the following viruses: dl309,ONYX-015, ONYX-051 (R240A), ONYX-052 (T255A), and ONYX-053 (H260A).Twenty-four hours postinfection cells were washed with PBS andfixed for 30 min at room temperature using 4% formaldehyde inPBS. Cells were permeabilized and blocked with PBS supplementedwith 0.1% Triton X-100, 0.05% Tween-20, and 10% goat serum for30 min at room temperature and then incubated for 1 h at roomtemperature with properly diluted primary antibodies. All antibodieswere diluted in the permeabilization and blocking solution. p53antibody DO-1 (Calbiochem) was diluted 1:100, anti-E1B-55K antibody9C10 (Calbiochem) was diluted 1:100, and the rabbit anti-E4orf6antibody 1807-3 was diluted 1:500. Antigens were visualized withAlexa Fluor 594 (red)- or Alexa Fluor 488 (green)-coupled secondaryantibody (MolecularProbes).

Cold-sensitivity assay. Infections of H1299 cells were performed at two temperatures, 32 and 39°C. Infections at 32°C were performed 1 h after thetemperature shift from 39°C. All infections were at an MOI of5, and infected cells were incubated at 32 and 39°C. Four daysafter infection, cells and culture media were harvested, pooled,and freeze-thawed three times to release virus particles. Viralyields were determined by enzyme-linked immunosorbent assay (L.Hawkins, Y. Wang, and T. Hermiston, unpublished data) on 293 cellmonolayers.

Assay for protein synthesis during the late phase of virus infection. A549 cells were either mock infected or infected with various adenovirus mutants at an MOI of 10. At 24 h postinfection cellswere labeled with [³⁵S]methionine-cysteine for a 3-h period. Labeled cells were washedwith cold saline, harvested, and solubilized in a solution containing50 mM Tris-Cl (pH 8.0), 5 mM EDTA, 150 mM NaCl, 0.5% NP-40, 3mM $beta$ -mercaptoethanol, and 1× EDTA-free protease inhibitor mix(Boehringer Mannheim). Cleared cell extracts were resolved bySDS-PAGE (4 to 20% gradient gel) and visualized by autoradiography.The same amount of radioactivity was loaded in eachlane.

MTT assay. DU145 and U2OS cells were seeded into 96-well plates at a density of 2.5 × 10³ cells/well using DMEM-high glucose supplemented with 2% FBS,2 mM L-glutamine, 100 µg of nonessential amino acids per ml, 10U of penicillin per ml, and 10 µg of streptomycin per ml. Thecells were infected 24 h after being seeded with the E1B-55K mutantviruses (dl309 and ONYX-015 were included as controls). All infectionswere carried out in quadruplet with serial threefold dilutionsof the viruses. A total of 10 dilutions were used for each virus,starting at an MOI of 30 and ending at an MOI of 1.5 × 10³. Cells that were mock infected were used as negative controls.Infected cells were incubated at 37°C and monitored daily. Colorimetricreactions were performed when significant cytopathic effect wasobserved in the cells infected with the wild-type virus, dl309,at the median MOI of 0.1. For most cell lines we have tested,this occurred at 4 to 7 days postinfection, allowing the virusesto go through multiple rounds of infection and spread. In theexperiments reported here, MTT reactions were carried out at 6days postinfection using Promega's CellTiter 96 Non-RadioactiveCell Proliferation assay according to the manufacturer's instructions.Cell killing curves from such MTT assays demonstrated a Poissondistribution.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

To separate the p53 binding and inactivation function from the other activities of E1B-55K, a series of single-amino-acidmutations in the p53-binding region (19) and the region requiredfor transcriptional repression (P. E. Branton, personal communication)were generated (Fig. 1 and Table 1). In each case, one nativeamino acid was changed to Ala (Table 1). In addition, four mutations(Ala 284 to Ser, Phe 285 to Leu, Cys 288 to Ala, Trp 289 to Phe)were generated in the putative RNA-binding region of the protein.It was shown previously that some of these mutations can modulatethe RNA-binding activity of the E1B-55K protein (K. Leppard, personalcommunications). In one case (ONYX-070), two amino acid changeswere introduced inadvertently (Gly 318 to Ala and Asn 319 to Thr).All mutations were recombined into infectious virus (dl309 background),and the resulting recombinant viruses were characterized for theirability to produce stable 55K protein, modulate p53 degradation,mediate viral late-gene expression, and support virus replication.All the E1B-55K mutations and the resulting viruses are summarizedin Table 1.

Steady-state level of p53. E1B-55K cooperates with E4orf6 to target p53 for active degradation. In order to identify E1B-55K mutants that were incapableof this activity, we examined the steady-state level of p53 ininfected A549 cells by Western blot analysis (Fig. 2). In cellsinfected with dl309 or WtD, the p53 level was significantly reduceddue to the targeted degradation mediated by E1B-55K and E4orf6.In contrast, cells infected with ONYX-015 exhibited an increasein the p53 level. Most viral mutants caused a decrease in thelevel of p53. However, cells infected with ONYX-051 and -053 (expressingE1B-55K mutants R240A and H260A, respectively) displayed a significantincrease in p53 levels compared to mock-infected A549 cells. Allof the point-mutant adenoviruses accumulated E1B-55K protein tolevels comparable to WtD or dl309 upon infection (Fig. 2). Theseobservations raised the possibility that E1B-55K mutants R240Aand H260A may fail to bind p53 and/or E4orf6.

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FIG. 2. Effects of E1B-55K mutations on p53 accumulation and viral gene expression. A549 cells were either mock infected (mock) or infected with dl309, WtD, ONYX-015, or viruses harboring various E1B-55K mutants. All infections were performed at an MOI of 10. Cell extracts were prepared at 24 h postinfection and were separated by SDS-PAGE. Steady-state levels of E1B-55K mutants, p53, E2A, and fiber were determined by Western blotting with monoclonal antibodies 2A6, DO-1, B6-6, and a rabbit polyclonal anti-fiber antibody, respectively. Blots were visualized with ECL, as described in Materials and Methods.

Binding of selected E1B-55K mutants with p53 and E4orf6. To directly examine the ability of E1B-55K mutants R240A and H260A to interact with p53, we performed an immunoprecipitationexperiment using ³⁵S-labeled cell extracts from infected A549 cells (Fig. 3). Anti-p53antibody mAb421 coprecipitated small amounts of wild-type E1B-55Kprotein from dl309- and WtD-infected cells as expected (Fig. 3A).E1B-55K mutant R240A was also coprecipitated, indicating thatit is capable of binding p53. Coprecipitation of H260A E1B-55Kcould be detected only after prolonged exposure, suggesting thatthis mutant interacts with p53 rather poorly. Incubation withthe anti-E1B-55K antibody 2A6 immunoprecipitated E1B-55K proteins(Fig. 3B); however, it is difficult to determine whether p53 wascoprecipitated, as the proteins share similar molecular weightsand the E1B-55K protein was much more abundant. It is interestingto note that the amounts of p53 in ONYX-051 (R240A)- and -053(H260A)-infected cells as detected by immunoprecipitation werelower than those in mock-infected cells, whereas by Western analysis,the p53 levels were higher in ONYX-051- and -053-infected cells.This is likely due to the fact that Western blot analysis detectsthe steady-state level of p53, whereas immunoprecipitation onlydetects newly synthesized p53. We hypothesize that R240A and H260Awere able to mediate host cell shutoff (see below), causing p53to be synthesized at a reduced rate compared to that of mock-infectedcells. The slow rate of synthesis for p53 and its higher steady-statelevel in cells that are infected with ONYX-051 and -053 againsuggest that these viruses have lost their ability to target p53for degradation.

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FIG. 3. Coimmunoprecipitation of p53 by E1B-55K mutants. (A and B) Coimmunoprecipitation experiment. A549 cells were either mock infected (mock) or infected with various virus mutants at an MOI of 10. At 24 h postinfection, cells were metabolically labeled with [³⁵S]methionine-cysteine for a 3-h period. Cell extracts were immunoprecipitated with anti-p53 antibody Ab421 (A) or anti-E1B-55K antibody 2A6 (B) and analyzed by SDS-PAGE as described in Materials and Methods. E1B-55K mutant R240A was expressed from ONYX-051, and H260A was expressed from ONYX-053. (C and D) In vitro-translated (and ³⁵S-labeled) p53 was mixed with lysates prepared from infected A549 cells at 24 h post infection and immunoprecipitated with 2A6 anti-E1B-55K antibody. Immune complexes were separated by SDS-PAGE and visualized either directly by autoradiography (C) or by Western blotting with 2A6 antibody (D).

Because of the variability in the level of p53 in infected cell extracts (see Fig. 2), it is impossible to determine the relativebinding efficiency of various E1B-55K mutant proteins to p53 fromthe coimmunoprecipitation experiment described above. In orderto more accurately compare the efficiencies of binding of differentE1B-55K mutant proteins to p53, we used an in vitro binding assay(37). Lysates of A549 cells infected with various adenoviruseswere incubated with in vitro-translated ³⁵S-labeled p53, and the anti-E1B-55K antibody 2A6 was used forimmunoprecipitation. It was apparent from this experiment (Fig.3C) that R240A (ONYX-051) and H260A (ONYX-053) bound p53 withsignificantly lower affinity than the wild-type E1B-55K protein.This inefficient precipitation of p53 was not due to lower levelsof mutant E1B-55K protein in cells infected with ONYX-051 or -053;Western analysis confirmed that a similar or slightly higher levelof E1B-55K protein was present in cell extracts derived from ONYX-051-and -053-infected cells (Fig. 3D). The inefficient binding ofR240A and H260A to p53 may explain, at least in part, why p53was not efficiently targeted for degradation in cells infectedwith ONYX-051 and -053.

Wild-type E1B-55K protein forms a complex with E4orf6 protein during adenovirus infection (6, 23). It has been suggestedthat this complex plays an important role in targeting p53 foractive degradation (25, 28, 35) and in the regulation ofthe nuclear export of late viral mRNAs and cellular mRNAs (7,12). Thus, it is important to determine if the mutations weintroduced into E1B-55K changed the ability of this protein tocomplex with E4orf6. We examined this interaction by coimmunoprecipitationwith an antibody against E1B-55K followed by Western analysisfor E4orf6 (Fig. 4). The E1B-55K mutant R240A binds E4orf6 aswell as the wild-type protein. However, the H260A mutant bindsE4orf6 only very weakly. It is possible that the reduced bindingto E4orf6 by H260A may also contribute to the lack of p53 degradationin ONYX-053 infection. T255A (ONYX-052) was included as a control,mainly because this mutation lies between the two mutations thatdisrupt binding to p53. Interestingly, T255A completely lost itsability to bind E4orf6 yet is still capable of degrading p53,as shown in Fig. 2. These results suggest that E1B-55K and E4orf6may not need to form a stable complex to target p53 for activedegradation.

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FIG. 4. Binding of E4orf6 by the E1B-55K mutants. A549 cells were either mock infected (mock) or infected with indicated virus mutants at an MOI of 10. At 24 h postinfection cells were lysed; cleared cell extracts were immunoprecipitated with anti-E1B-55K antibody 2A6. The precipitated materials were separated by SDS-PAGE and analyzed by Western blotting with a rat polyclonal antibody against E4orf6 (A) or with a rat anti-E1B-55K polyclonal antibody (B). (C) The level of E4orf6 expression in the infected cells by straight Western analysis using a polyclonal anti-E4orf6 antibody. dl355* is a dl309 derivative lacking the E4orf6 gene.

Immunofluorescent staining of p53 and E1B-55K. Next, we examined whether E1B-55K mutants R240A, T255A, and H260A are able to relocate p53 to the cytoplasm (Fig. 5). In mock-infectedA549 cells, p53 was detected exclusively in nuclei. In cells infectedwith the wild-type virus dl309, p53 was present at a very lowlevel, exclusively in the cytoplasm, and colocalized with theE1B-55K protein. Infection with ONYX-015 resulted in an elevatedlevel of p53 localized in cell nuclei, as expected. In A549 cellsinfected with the R240A mutant virus (ONYX-051), the p53 levelwas elevated (compare ONYX-051 and mock-infected cells) in nuclei,as in the case of ONYX-015 infection. This is consistent withthe fact that R240A binds p53 very weakly. Infection with theT255A mutant virus (ONYX-052) showed results similar to thosefor dl309, indicating that T255A can relocate p53 to the cytoplasmfor degradation. Unexpectedly, cells that were infected with H260Avirus (ONYX-053) showed variable p53 levels. Approximately two-thirdsof the infected cells had undetectable levels of p53, whereasthe rest showed high levels of p53 in nuclei. While the reasonfor this inconsistency is unclear, it is possible that this mayreflect the cell cycle status of the cells when they were infected.Interestingly, this phenomenon was observed only in A549 cells.In U2OS cells (which harbor wild-type p53), p53 was present athigh levels in nuclei when infected with ONYX-015, -051, and -053but at low levels when infected with dl309 and ONYX-052 (datanot shown).

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FIG. 5. Indirect immunofluorescent staining of adenovirus- and mock-infected (mock) cells. A549 cells grown on chamber slides were infected with dl309 or ONYX-015, -051, -052, or -053 at an MOI of 10 or were mock infected. At 24 h postinfection the cells were fixed, permeabilized, and analyzed by indirect immunofluorescent staining using the E1B-55K-specific monoclonal antibody 9C10 ( $alpha$ E1B), p53-specific monoclonal antibody DO-1 ( $alpha$ p53), and E4orf6-specific polyclonal antibody 1807-3 ( $alpha$ E4). Representative fields are shown for all cases.

Analysis of late functions of the E1B-55K mutants. Forming a complex with E4orf6, E1B-55K actively facilitates nuclear export of the late viral mRNAs while concomitantly inhibitingthe nuclear export of the cellular mRNAs. E1B-55K may also beinvolved in the active translation of late viral mRNAs (13).In the absence of E1B-55K, nuclear export and translation of lateviral mRNAs do not occur efficiently, resulting in lower expressionof the late viral proteins than of the wild-type virus (2,6, 12, 20). To examine whether our E1B-55K mutant virusesexpressed late proteins efficiently, we examined the synthesisof the adenovirus fiber protein. Previous work indicated thatthe mRNA for fiber protein depends on the E1B-55K/E4orf6 complexfor efficient nuclear export and expression (24). Whereas theability of ONYX-015 to express fiber protein was severely compromisedcompared to that of wild-type virus, all other mutant adenovirusesexpressed fiber protein at a level similar to that of the wild-typevirus (Fig. 2). As a control, we examined the expression of E2A,an early protein involved in viral DNA replication. The E2A proteinlevel was uniform among all samples, suggesting that the differencein fiber expression was not due to variance in viral DNA replication.Thus, the E1B-55K protein of ONYX-051 and -053 was unable to inactivatep53 yet retained the ability to promote high levels of structuralproteinsynthesis.

Several groups have reported that the replication of E1B-55K mutant adenoviruses is temperature dependent (9, 13, 16,21). Whereas replication of E1B-55K mutant adenoviruses is equivalentto that of wild-type virus at 39°C, at 32°C replication of E1B-55Kmutant viruses is significantly reduced compared to that of wild-typevirus. This cold-sensitive phenotype of the E1B-55K-defectiveviruses presumably reflects the more severe defects in mRNA transportor late-gene expression at the colder temperature (9, 13).To determine whether ONYX-051 (R240A) and -053 (H260A) have acold-sensitive phenotype, we performed the cold-sensitivity assay,using dl309 and ONYX-015 as controls (Fig. 6). As expected, allviruses replicated similarly at 39°C. The yield of dl309 was approximatelyfourfold higher than that of ONYX-015, and the yields of ONYX-051and -053 fell between. However, at 32°C the ONYX-015 yield wasreduced nearly 35-fold compared to that of dl309, consistent withprevious reports. Replication of ONYX-051 was essentially identicalto that of dl309, while replication of ONYX-053 was only slightlyreduced (fourfold). These results indicated that mutant R240Acan completely rescue the cold-sensitive phenotype of the E1B-55K-defectiveadenovirus, whereas H260A is partially functional.

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FIG. 6. Replication of dl309, ONYX-015, ONYX-051, and ONYX-053 as a function of time postinfection in p53-null H1299 cells at 32 and 39°C. H1299 cells were infected and maintained at two temperatures, 32 and 39°C. Infections at 32°C were performed 1 h after the temperature shift from 39°C. All infections were performed at an MOI of 5. Infected cells were incubated at 32 and 39°C, respectively. Ninety-six hours postinfection cells and culture media were harvested, pooled, and freeze-thawed three times to release virus particles. Viral yields were determined by enzyme-linked immunosorbent assay on a 293 cell monolayer. Total viral yields were divided by the number of cells at the time of infection to determine viral production per cell. Results are the average from two independent experiments that are highly consistent with each other.

When total protein expression from infected cells was compared (Fig. 7), it was clear that expression of late viral proteinswas lower in ONYX-015-infected cells than in dl309- and WtD-infectedcells. At the same time, de novo synthesis of the cellular proteinswas substantially reduced in cells infected with dl309 and WtD(compared to mock infection), presumably due to host cell shutoff.In ONYX-015-infected cells, however, shutoff of host protein synthesiswas deficient, as evidenced by the smeared background in the lanelabeled ONYX-015. The protein synthesis profile in cells infectedwith ONYX-051 and -053 was similar to that in cells infected withwild-type viruses dl309 and WtD. This observation suggested thatmutants R240A and H260A are capable of modulating mRNA traffickingin favor of late viral mRNA nuclear export and promoting hostcell shutoff.

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FIG. 7. Protein expression during the late phase of adenovirus infection. A549 cells were either mock infected (mock) or infected with various adenovirus mutants at an MOI of 10. At 24 h postinfection, cells were metabolically labeled with [³⁵S]methionine-cysteine for a 3-h period. Cell extracts were resolved by SDS-PAGE (4 to 20% gradient gel). The positions of the molecular mass markers are indicated at the right.

Taken together, these results suggest that the E1B-55K mutant R240A may entirely maintain the normal late functions of thewild-type protein, whereas mutant H260A appeared to be at leastpartially active in the latefunctions.

Analysis of cytolytic activity in human cancer cells. Each E1B-55K mutant virus was tested for its ability to replicate in and to kill human tumor cells. Although A549 cells wereused to characterize the functional interaction between p53 andvarious 55K point mutants, this cell line has been reported tobe rather permissive for the replication of the 55K-mutant viruses(18). Therefore, we used two other human cancer cell lines,U2OS and DU145, to examine the oncolytic activity of our mutantviruses. A quantitative assay, the MTT assay, was used for thisanalysis (see Materials and Methods). The MOI at which 50% ofthe cells were killed was determined and plotted (Fig. 8). Inboth cell lines, ONYX-015 was attenuated compared to its wild-typecounterpart dl309. Among the viruses that were generated for thisstudy, most (including ONYX-051) were comparable to dl309 in theirability to infect and kill tumor cells, though some (ONYX-053,-083, and -085) were significantly less potent than the wild-typevirus but were more active than ONYX-015. In the case of ONYX-053,its tumor cytolytic activity was 35- to 100-fold lower than thatof dl309 but was more active than ONYX-015 by a factor of four-to fivefold.

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FIG. 8. Cytolytic activity in tumor cells. DU145 and U2OS cells were seeded into 96-well plates at a density of 2.5 × 10³ cells/well. Twenty-four hours after seeding, cells were infected with serial threefold dilutions of E1B-55K mutant viruses, ranging from an MOI of 30 to an MOI of 1.5 × 10³. dl309 and ONYX-015 were included as controls. MTT assays were performed 6 days after infection as described in Materials and Methods. The MOIs that resulted in 50% cell killing were defined as IC50 and were plotted for each virus. Results from one of the two independent experiments are shown here. Similar results were obtained in the other experiment.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We have constructed and analyzed a series of single-amino-acid substitution mutations of the adenovirus E1B-55K protein inan effort to separate the p53 binding and inactivation functionand late functions of this protein. Analysis of each mutant indicatedthat all of the E1B-55K proteins were expressed in infected cells.Of the 26 mutants, 24 mediated p53 degradation as efficientlyas the wild-type protein. Two mutants, R240A (ONYX-051) and H260A(ONYX-053), failed to degrade p53 (Fig. 2). In fact, p53 levelsin A549 cells infected with ONYX-051 and ONYX-053 were noticeablyhigher than that in the mock-infected A549 cells, although theywere slightly lower than that in cells infected with ONYX-015.In in vitro assays, R240A and H260A mutant E1B-55K proteins associatedwith p53 with a greatly reduced affinity compared to the wild-typeprotein (Fig. 3). H260A also lost the ability to bind the E4orf6protein, while R240A was fully functional in this interaction(Fig. 4). Immunofluorescent staining experiments confirmed thatp53 was present at high levels in the nuclei of cells that wereinfected with ONYX-051 (Fig. 5). In cells that were infected withONYX-053, p53 levels varied (Fig. 5), a phenomenon that deservesfurther detailed analysis. Both ONYX-051 (R240A) and ONYX-053(H260A) expressed adenoviral fiber protein efficiently (Fig. 2),mediated shutoff of host cell protein synthesis (Fig. 7), anddid not display the cold-sensitive growth phenotype (Fig. 6).Finally, ONYX-051 (R240A) replicated efficiently in human cancercells, while ONYX-053 (H260A) did so only partially (Fig. 8).

Taken together, these data suggest that we have successfully isolated two E1B-55K mutants that are defective in p53 bindingand inactivation yet retain many of the late functions of thewild-type protein which are essential for efficient replicationof adenovirus. These results suggest that these distinct E1B-55Kfunctions are separable. The implication of the functional separationis twofold. First, these E1B-55K mutants will allow us to betterinvestigate the molecular mechanisms of the tumor-selective adenovirusONYX-015. Second, by incorporating these mutations, we can createadenoviruses that maintain the tumor selectivity of ONYX-015 butreplicate more efficiently in tumor cells than ONYX-015. It isgratifying that both ONYX-051 and -053 showed higher cytolyticactivity in tumor cells than ONYX-015 (Fig. 8). We are currentlytesting whether these mutant viruses retained the tumor cell selectivityof ONYX-015.

It was hypothesized that deletion of the E1B-55K gene in ONYX-015 allows this virus to replicate efficiently only in tumorcells that are defective in p53 function but not in normal cellswhere p53 function is normal (5). This hypothesis has gainedsupport from a number of in vitro and in vivo studies (15, 27).Recently, it was reported (26) that the loss of p14ARF functionfacilitates ONYX-015 replication. This finding demonstrated forthe first time that the integrity of the p53 functional pathwayrather than the p53 gene itself may determine the outcome of ONYX-015infection. Nonetheless, several groups have described in vitrostudies showing that the host range specificity of ONYX-015 isindependent of p53 gene status (9, 13, 14, 29). It hasbeen suggested that the loss of E1B-55K's RNA transport activityrather than its p53 binding and inactivation function may accountfor the tumor cell specificity of ONYX-015. The mutant viruseswe created in this study, particularly ONYX-051 and -053, canbe used to explore some of thesedifferences.

Grand et al. (11) reported that the region of E1B-55K essential for p53 interaction lies between amino acids 216 and 235.This domain only partially overlaps the p53-binding region identifiedby Kao et al. and Yew et al. (19, 39), which maps to aminoacids 224 to 354. The reason for this apparent discrepancy isnot clear. Since Grand et al. used fusion proteins between Ad2E1B-55K and Ad12 E1B-55K in their analysis, it is possible thatadditional domains in the Ad12 E1B-55K protein may be involvedin p53 binding. Our results indicate that amino acids 240 and260 are critical for p53 binding and inactivation, consistentwith the results of Kao et al. Further studies are necessary toidentify the minimal essential region of the E1B-55K protein forp53interaction.

It was reported (19, 39) that a four-amino-acid insertional mutation at amino acid 380 of the E1B-55K protein (S380) reducedits interaction with p53, while the ability of the virus to replicatewas not compromised. Furthermore, this mutant virus (S380) resemblesthe wild-type virus with respect to late viral protein synthesisand host cell shutoff. Thus, S380 appears to be very similar toONYX-051 and -053. It should be noted that the characterizationof this mutant, S380, was performed in HeLa cells, where humanpapillomavirus oncoproteins exist and may complicate the analysisdue to interactions between human papillomavirus 18 E6 proteinand p53. Recently, Gabler et al. reported that S380 failed tobind E1B-AP5, suggesting that this mutant may be defective inmediating late viral mRNA transport (8). Further characterizationof this mutant with respect to its interaction with E4orf6, itssubcellular localization, its activity in mRNA transport, andits ability to rescue the cold-sensitive phenotype would allowONYX-051 and -053 and S380 to be directlycompared.

Two of the E1B-55K mutant proteins we have tested, T255A (ONYX-052) and H260A (ONYX-053), are defective in binding the E4orf6protein, as determined by the coimmunoprecipitation experiment(Fig. 4). No interaction between the E1B-55K T255A mutant andE4orf6 could be detected. However, in cells that were infectedwith ONYX-052, p53 was clearly exported to the cytoplasm (Fig.5) and degraded (Fig. 2 and 5). These results suggest that E1B-55Kand E4orf6, both shown to be necessary for p53 degradation (25,28, 35), may not need to be in a stable complex to targetp53 for degradation. Moreover, T255A appeared to be active inmediating fiber expression (Fig. 2) and did not display the cold-sensitivephenotype (Fig. 6), suggesting that its function in mRNA traffickingduring the late phase of adenovirus infection was intact. Similarly,H260A bound E4orf6 poorly yet was still capable of mediating efficientfiber expression and other late functions. These observationsare in contrast to previous literature, which suggests that E1B-55Kand E4orf6 need to interact to modulate mRNA transport. It ispossible that other cellular or viral proteins may interact withthese adenoviral proteins and keep them in the same complex (10,23). It was reported recently (19a) that the E1B-55K proteinitself is a highly active shuttle protein capable of shuttlingindependent of E4orf6. Whether this finding supports our observationsremains to betested.

Phase I and II clinical trials with the head-and-neck cancer patients have indicated that ONYX-015 replicates in and destroystumor cells at the exclusion of surrounding normal tissue. Incombination with standard chemotherapy, intratumoral injectionof ONYX-015 resulted in tumor regression in more than two-thirdsof the patients treated. However, the deletion of E1B-55K in ONYX-015has compromised the replication capability of this virus. Comparedto wild-type virus, ONYX-015 is attenuated in a number of tumorcell lines (9, 13), possibly limiting its potential as ananticancer drug. One can imagine that virus mutants that haveimproved replication capacity yet retain the tumor selectivityof ONYX-015 would provide more efficient treatment for cancerpatients. In this regard, ONYX-051 and -053 and viruses like themmay serve as candidates for clinical development. Additional studiesare underway in our laboratory to determine the replication capacityof these viruses in the presence and absence of normal p53 activityand to compare their replication efficiency in normal primarycells and tumorcells.

	ACKNOWLEDGMENTS

We thank Adam Sampson-Johannes, Sandy McCoy, and Wen Yan for excellent technical support, Josh Watanabe for virus production,and Jaina Sumortin for DNA sequencing. We also thank Tom Alber,Matthias Dobbelstein, Leisa Johnson, and Keith N. Leppard forhelpful discussions, Philip E. Branton for the E4orf6 antibodies,Clodaugh O'Shea for the rat anti-E1B-55K antibodies, and AllanBalmain and Tom Dubensky for critical reading of themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: ONYX Pharmaceuticals, Inc., 3031 Research Dr., Richmond, CA 94806. Phone: (510) 243-3679.Fax: (510) 222-9758. E-mail: jshen{at}onyx-pharm.com.

Present address: Berlex Laboratories, Inc., Richmond, CA 94804-0099.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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	Articles by Shen, Y.
	Articles by Hermiston, T.

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34.	Shen, Y., and T. Shenk. 1994. Relief of p53-mediated transcriptional repression by the adenovirus E1B 19-kDa protein or the cellular Bcl-2 protein. Proc. Natl. Acad. Sci. USA 91:8940-8944[Abstract/Free Full Text].
35.	Steegenga, W. T., N. Riteco, A. G. Jochemsen, F. J. Fallaux, and J. L. Bos. 1998. The large E1B protein together with the E4orf6 protein target p53 for active degradation in adenovirus infected cells. Oncogene 16:349-357[CrossRef][Medline].
36.	Tollefson, A. E., T. W. Hermiston, and W. S. M. Wold. 1998. Preparation and titration of CsCl-banded adenovirus stock. Methods Mol. Med. 20:1-9.
37.	Wienzek, S., J. Roth, and M. Dobbelstein. 2000. E1B 55-kilodalton oncoproteins of adenovirus type 5 and 12 inactivate and relocalize p53, but not p51 or p73, and cooperate with E4orf6 proteins to destabilize p53. J. Virol. 74:193-202[Abstract/Free Full Text].
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