Growth Suppression by an E2F-Binding-Defective Retinoblastoma Protein (RB): Contribution from the RB C Pocket

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Mol Cell Biol, July 1998, p. 4032-4042, Vol. 18, No. 7
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Growth Suppression by an E2F-Binding-Defective Retinoblastoma Protein (RB): Contribution from the RB C Pocket

Laura L. Whitaker, Heyun Su, Rajasekaran Baskaran, Erik S. Knudsen, and Jean Y. J. Wang^*

Department of Biology, Center for Molecular Genetics, and Cancer Center, University of California, San Diego, La Jolla, California 92093-0322

Received 14 January 1998/Returned for modification 24 March 1998/Accepted 22 April 1998

SUMMARY
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

SUMMARY
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Growth suppression by the retinoblastoma protein (RB) is dependent on its ability to form complexes with transcription regulators.At least three distinct protein-binding activities have been identifiedin RB: the large A/B pocket binds E2F, the A/B pocket binds theLXCXE peptide motif, and the C pocket binds the nuclear c-Abltyrosine kinase. Substitution of Trp for Arg 661 in the B regionof RB (mutant 661) inactivates both E2F and LXCXE binding. Thetumor suppression function of mutant 661 is not abolished, becausethis allele predisposes its carriers to retinoblastoma developmentwith a low penetrance. In cell-based assays, 661 is shown to inhibitG₁/S progression. This low-penetrance mutant also induces terminalgrowth arrest with reduced but detectable activity. We have constructedmutations that disrupt C pocket activity. When overproduced, theRB C-terminal fragment did not induce terminal growth arrest butcould inhibit G₁/S progression, and this activity was abolishedby the C-pocket mutations. In full-length RB, the C-pocket mutationsreduced but did not abolish RB function. Interestingly, combinationof the C-pocket and 661 mutations completely abolished RB's abilityto cause an increase in the percentage of cells in G₁ and to induceterminal growth arrest. These results suggest that the A/B orC region can induce a prolongation of G₁ through mechanisms thatare independent of each other. In contrast, long-term growth arrestrequires combined activities from both regions of RB. In addition,E2F and LXCXE binding are not the only mechanisms through whichRB inhibits cell growth. The C pocket also contributes to RB-mediatedgrowth suppression.

INTRODUCTION
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The retinoblastoma susceptibility gene, Rb1, encodes a ubiquitously expressed nuclear retinoblastoma protein (RB) which isa negative regulator of cell proliferation (28). The growth-inhibitoryactivity of RB is neutralized by phosphorylation at G₁/S transitionin a cell division cycle (27, 28). In addition to inhibitingcell proliferation, RB has also been implicated in the regulationof terminal differentiation and apoptosis (24, 26, 34).The inactivation of RB, either through mutations of the Rb1 geneitself or through mutations that enhance RB phosphorylation, hasbeen widely observed in tumor cells (22).

A major mechanism by which RB inhibits G₁/S progression is repression of E2F-regulated genes (20, 28). This transcriptionrepression mechanism is dependent on two distinct protein-bindingsites in RB: the large A/B pocket, which binds E2F, and the A/Bpocket, which binds the LXCXE peptide motif in proteins. Threerecent reports have demonstrated that RB can interact with a histonedeacetylase through the LXCXE-binding site (3, 14, 15).The simultaneous binding of E2F and histone deacetylase by RBcan therefore lead to the assembly of a transcription repressioncomplex at promoters containing E2F-binding sequences (3, 14,15). The three-dimensional structure of the A/B domain has beensolved (11). The LXCXE-binding site (i.e., the A/B pocket) isentirely within the B region, although its formation is dependenton multiple interactions between the A and B regions (11). Withinthe A/B domain crystal (which lacks the RB insert and the C-terminalregion), the binding site for an E2F peptide and the binding sitefor the LXCXE peptide are shown to be distinct from each otherby the concurrent binding of both peptides to the A/B domain (11).Thus, the three-dimensional structure of the A/B domain is consistentwith the model that RB can simultaneously bind to more than onetarget.

Germ line mutations in Rb1 result in the development of bilateral retinoblastoma in 90% of human carriers. These high-penetrancemutant alleles produce either no RB protein or an unstable product.The importance of the E2F- and LXCXE-binding sites to the tumorsuppression function of RB is underscored by the occurrence ofat least four germ line point mutations in the A/B domain (11).One of these, the C706F mutation, which produces a highly unstablemutant protein, occurs in the hydrophobic core of the B region.While a majority of the germ line mutations result in 90% predispositionto bilateral retinoblastoma, a few mutant alleles have been foundto cause retinoblastoma with a lower penetrance (13). Theselow-penetrance alleles are likely to encode RB proteins with decreasedactivities but activities that are sufficient to maintain thresholdlevels of tumor suppression. One of the low-penetrance RB mutantscontains a substitution of Trp for Arg 661 in the B region ofRB (R661W) (10, 13). The crystal structure shows that theside chain of Arg 661 (which is in the B region) participatesin the formation a hydrogen bond network between helices of theA and B regions (11). Mutation of Arg 661 is therefore likelyto disrupt the packing of these alpha helices. The R661W mutationhas been shown to disrupt both the LXCXE- and E2F-binding activitiesof RB (10, 19). However, R661W can suppress the growth ofRB-negative tumor cells (10, 19). This suppression is consistentwith the ability of R661W to confer partial protection from retinoblastomadevelopment. The partial function of R661W suggests that RB canexert some growth suppression through mechanisms that are independentof binding to E2F and LXCXE proteins (10, 19).

While the presence of the A/B domain is sufficient for RB to bind E2F subunits such as E2F-1, additional interactions providedby the C-terminal region of RB are required for binding to thefunctional E2F heterodimer (E2F-DP) (5, 17). The C-terminalregion of RB is also required for growth suppression, as the A/Bdomain alone is not functional in cell-based growth suppressionassays (17, 21, 32). The minimal functional domain, calledthe large A/B pocket, which contains RB amino acids 395 to 876,has been shown to correspond to the binding site for E2F heterodimers(5, 17). Welch and Wang have previously shown that RB canbind to the nuclear c-Abl tyrosine kinase and found that the c-Ablbinding site is outside of the A/B domain and entirely withinthe C-terminal region of RB (31). The c-Abl binding site ofRB is referred to as the C pocket. Because RB can simultaneouslybind E2F and c-Abl (32), the C-terminal E2F-binding site andthe C pocket are distinct from each other. Two lines of evidencehave indicated that C pocket activity contributes to the growthsuppression function of RB (30, 32). First, coexpression ofRB with its C-terminal fragment disrupts the ability of RB tosuppress growth, as was determined by the inhibition of colonyformation in RB-negative Saos-2 cells (32). Second, overproductionof a c-Abl mutant (c-Abl-AS2), which does not bind RB and whosekinase activity is therefore not inhibited by RB, can overridethe growth suppression function of RB (30).

To directly assess the role of the C pocket in the growth suppression function of RB, we sought to isolate RB C-terminal mutationsthat specifically disrupt RB-c-Abl interaction without affectingRB-E2F interaction. In this report, we describe the constructionand characterization of such mutations. Although the C-terminalfragment by itself cannot induce terminal growth arrest in Saos-2cells (32), we found that the overproduction of the C-terminalfragment alone can delay G₁/S transition. This G₁/S-transition-inhibitoryactivity was disrupted by the C-pocket mutations. In the contextof full-length RB, mutations of the C pocket did not affect theability of RB to inhibit G₁/S transition but reduced the growthsuppression function of RB by half. In the Saos-2 cell-based assays,the low-penetrance A/B domain mutation R661W also inhibited G₁/Stransition but produced about one-third the level of wild-typeactivity in inducing terminal growth arrest. Interestingly, however,combination of C-pocket mutations with R661W led to the completeabrogation of both the G₁/S-inhibitory and the growth suppressionfunctions of RB. Taken together, these results suggest that activitiesfrom either the A/B domain or the C region can inhibit G₁/S progression.However, the induction of terminal growth arrest appears to requirecontributions from both the A/B domain and the C region. Terminalgrowth arrest induced by the RB A/B/C region can occur withoutRB binding to the E2F and LXCXE proteins. This E2F-independentgrowth suppression requires the activity of the RB C pocket.

MATERIALS AND METHODS
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Cell culture and transfections. The human cervical carcinoma cells C33A and the osteosarcoma cells Saos-2 were obtained from the American Type Culture Collection.These cells were cultured in Dulbecco modified Eagle medium-highglucose supplemented with 15% heat-inactivated fetal bovine serumat 37°C in 5% CO₂.

Transfections were performed by the calcium phosphate method, and flat-cell assays and neomycin-resistant colony formationassays were performed with Saos-2 cells as previously described(32). To achieve the same level of protein expression, the amountof plasmid DNA used was titrated for each construct. For the competitionexperiment described in Table 2, we used a 3:1 ratio of plasmidDNA expressing the C-terminal SE fragment (see Fig. 1A) to plasmidDNA expressing the wild-type RB C-terminal SE fragment.

The repression of a Gal4-E2F1 fusion transcription factor was measured as described previously, using a reporter containingfive tandem repeats of Gal4-DNA binding sequences linked to chloramphenicolacetyltransferase (5×Gal4-CAT) (29). In general, 0.8 µg of 5×Gal4-CAT,0.8 µg of Gal4-E2F, and between 8 and 16 µg of RB constructs weretransfected into Saos-2 cells. The dehydrofolate reductase (DHFR)-Lucreporter constructs contained the wild-type DHFR promoter region( $-$ 270 to +20) or the same region with the E2F-binding site mutated(mutDHFR). One microgram of DHFR-Luc reporter or mutDHFR-Luc reporterand 5 to 10 µg of RB constructs were used. In all transfections,0.5 µg of a $beta$ -galactosidase-expressing construct was includedto correct for the transfection efficiencies. The total amountof transfected DNA was made up to 18 µg by adding the pCMV-neo-Bamvector.

The RB mutant constructs were made by PCR-based mutagenesis and subcloned into pCMV-neo-Bam for expression. Glutathione S-transferase(GST)-SE and GST-ME (see Fig. 1A) have been previously described(31). The additional GST-RB C-terminal mutants were subclonedin frame into pGEX-KG (Pharmacia).

Binding of RB to GST-E2F-1 and GST-E7. GST-E2F-1 or GST-E7 was expressed in bacteria and adsorbed onto glutathione-agarose. Each was then incubated at 4°C for 2h with lysates from C33A cells transfected with pCMV-RB expressionplasmids. Preparation of lysates with NETN lysis buffer (0.5%Nonidet P-40, 1 mM EDTA, 50 mM Tris [pH 8.0], 120 mM NaCl) waspreviously described (9, 31). The agarose beads were washedfour times with NETN, and the bound proteins were eluted withsodium dodecyl sulfate (SDS), resolved by SDS-7.5% polyacrylamidegel electrophoresis, and then transferred to Immobilon membranes.Immunoblotting was performed with monoclonal anti-RB 245 antibody(Pharmingen, San Diego, Calif.).

Abl binding and kinase inhibition. ³⁵S-labeled in vitro-translated c-Abl was incubated for 2 h at 4°C with GST-immobilized RB C-terminal fragments expressed asGST fusion proteins (31). The agarose beads were washed fourtimes with NETN, the bound proteins were eluted with SDS and resolvedon an SDS-7% polyacrylamide gel, and the amount of GST-RB in eachsample was determined by staining with Coomassie blue. The amountof Abl was determined by autoradiography after fluoro-enhancement.

For the c-Abl kinase inhibition assay, in vitro-translated hemagglutinin (HA)-tagged c-Abl was immunoprecipitated with anti-HAantibody (Babco, Berkeley, Calif.) and then incubated with occasionalagitation for 30 min at 4°C with an ~50-fold molar excess of RBC-terminal fragments. The wild-type and mutant RB C-terminal fragmentswere expressed and purified from bacteria as GST fusion proteins.The anti-HA immunoprecipitates were then washed four times withNETN and twice with 1× kinase buffer (20 mM Tris [pH 7.4], 10mM MgCl₂, 1 mM dithiothreitol). Kinase reactions were initiatedby the addition of 100 ng of GST-C-terminal repeated domain (CTD)of RNA polymerase II (2), 5 µM cold ATP, and 20 µCi of [ $gamma$ -³²P]ATP (7,000 Ci/mmol; ICN Pharmaceuticals) in a final volume of50 µl of 1× kinase buffer. Reaction was carried out at room temperaturefor 30 min and terminated by adding an equal volume of 3× SDSsample buffer. The products were separated by SDS-7% polyacrylamidegel electrophoresis and transferred onto Immobilon-P, and theamount of ³²P incorporated into GST-CTD was determined by autoradiography.The upper portion of the Immobilon membrane corresponding to Abl'smolecular-weight region was probed with anti-Abl (8E9) antibodyto determine the amount of Abl in each of the reaction mixtures.The lower portion of the Immobilon membrane corresponding to theGST-RB molecular-weight region was stained with amido black todetermine the amount of purified GST-RB added to each reactionmixture.

Immunoprecipitation and immunoblotting of RB. Immunoprecipitation and immunoblotting of RB were performed as previously described (31). Anti-RB C36 (Pharmingen) was usedto immunoprecipitate RB complexes for the deoxycholate (DOC) release-gelshift assay; anti-RB 245 (Pharmingen) was used for immunoblottingRB proteins.

E2F electrophoretic mobility shift assay. DOC release-gel shift assays were performed as previously described, with transfected C33A cell lysate as the source of RBproteins and endogenous E2F proteins (32).

Luciferase assays. Luciferase assays were performed with the Promega Luciferase Assay System according to the manufacturer's protocol. Luciferaseactivity was corrected for $beta$ -galactosidase activity to normalizethe transfection efficiency.

Flow cytometry. RB constructs (5 µg of RB, 7S, and 13S; 10.0 µg of 661, 7S-661, and 13S-661; or 15 µg of SE, SE with amino acids 785 to 806deleted [SE $Delta$ ], and SE-13S) along with CD20 plasmid (0.5 µg) andan amount of the backbone vector sufficient to bring the amountof total DNA to 20 µg were transfected into Saos-2 or C33A cellsby the calcium phosphate method. Where indicated in Table 1,cells were treated with 0.1 µg of nocadozole per ml. Cells wereharvested and stained with anti-CD20 antibodies and propidiumiodide according to published protocols (35). The cell cycleprofile of CD20-positive cells was determined by fluorescence-activatedcell sorter (FACS) analysis with either Cell Fit or ModFit software(Becton Dickinson).

RESULTS
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Construction of RB C-pocket mutants defective in c-Abl binding. The C pocket has been defined as the binding site for the c-Abl tyrosine kinase (31). The C pocket was previously shownto be within the C-terminal region of RB, from amino acids 768to 928 (Fig. 1) (31). The E2F binding site, i.e., the largeA/B pocket, resides within amino acids 379 to 876 of RB (5,17). The C pocket and the large A/B pocket are functionallydistinct, as it is possible for RB to simultaneously bind bothE2F and c-Abl (32). An internal deletion of RB amino acids 785to 806 was previously shown to disrupt E2F binding (5) butnot c-Abl binding (32). These observations indicated that itmight be possible to isolate RB mutants which have lost C pocketfunction but that have retained E2F binding activity.

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FIG. 1. Summary of RB C-terminal mutant constructs. (A) c-Abl binding activity of C-terminal mutants of RB. The SE fragment is the wild-type RB C terminus from the SspI site to the end and contains amino acids 768 to 928. This fragment contains the C pocket, as was determined by the presence of c-Abl binding (31). $Delta$ signifies a deletion of the indicated amino acids. The ST mutant is the result of two amino acid substitutions: R828 to S and R830 to T. The Nco mutant contains an insertion at the MunI site (amino acid 834 in exon 24) of a 4-amino-acid sequence, EPWE, and the corresponding base pair sequence introducing an NcoI restriction enzyme site. SN is a combination of the ST and Nco mutations. Mutant 13 was constructed by swapping the sequence of RB which encodes amino acids 775 to 778 (RPPT) with the corresponding p130 sequence (NMDAPP), based on amino acid alignment (see panel B). Mutant 7S is a combination of the deletion of amino acids 775 to 778 and the SN mutation. Mutant 13S is a combination of the mutant 13 and SN mutations. GST-RB mutant binding to in vitro-transcribed and -translated c-Abl is measured relative to GST-SE binding. The wild-type level of activity is indicated with +++. Mutants with 50 to 60% of the wild-type level of activity are indicated with ++. Mutants with 20 to 30% of the wild-type level of activity are indicated with +. Mutants with undetectable activity are indicated with $-$ . (B) Partial amino acid sequence alignment of pRB, p107, and p130 C termini. pRB amino acids 775 to 778 and corresponding nonhomologous p107 and p130 sequence are indicated in boldface print.

Binding to c-Abl was determined by the ability of GST fusion proteins containing the C-terminal region of RB to interact within vitro-translated [³⁵S]Met-labeled c-Abl (Materials and Methods). The binding of eachRB mutant was compared to that of GST-RB-SE (from the SspI siteto the end) which contains wild-type RB amino acids 768 to 928(Fig. 1A). The GST-ME fusion, containing RB amino acids 834 to928, served as a negative control, as it has previously been shownto be defective in binding c-Abl (31, 32). As summarized inFig. 1A, deletion of amino acids 870 to 928 does not affect eitherc-Abl binding or E2F binding. Internal deletions of amino acids785 to 806 (SE $Delta$ ), 803 to 825, 841 to 850, and 850 to 870 havepreviously been shown to disrupt E2F binding (5), but thesedeletions did not have any detectable effect on c-Abl binding(Fig. 1A). Thus, RB amino acids 785 to 825 and 841 to 870 aredispensable for the formation of the C pocket.

An internal deletion of amino acids 825 to 840 decreased c-Abl binding by 60 to 70%, as did a smaller deletion eliminatingthe 10 amino acids encoded by RB exon 24 (amino acids 831 to 840)(Fig. 1A). Alternative manipulations of this region, such as substitutionsof Arg 828 and Arg 830 for Ser and Thr, respectively (mutant ST),or an insertion of 4 amino acids at position 834 (mutant Nco),also reduced c-Abl-binding activity (Fig. 1A). Further reductionof c-Abl binding was achieved when the ST and Nco mutations werecombined to create the mutant designated SN (Fig. 1A). ThoughRB-SN had reduced c-Abl-binding activity, this combination ofmutations did not completely abolish c-Abl binding (Fig. 1A).Internal deletions of a noncontiguous region, between amino acids768 and 805 or 768 and 796, were found to also reduce c-Abl-bindingactivity by 60 to 70% (Fig. 1A). Taken together, the results ofthe deletion analysis indicate that two separate regions, fromamino acids 768 to 785 and amino acids 825 to 840, are necessaryfor c-Abl binding.

The RB-related p107 protein does not bind c-Abl (32a). Thus, nonhomologous amino acids between RB and p107 may be requiredfor c-Abl binding by RB. RB and p107 have extensive homology inthe A and B domains. However, the RB sequence from amino acids775 to 778, immediately C terminal to the B domain, is not conservedin the corresponding p107 or p130 sequence (Fig. 1B). Deletionof these 4 amino acids (775 to 778; mutant 7) decreased c-Ablbinding to the same level as the deletion of amino acids 768 to796 (Fig. 1A). We also constructed a substitution mutation inwhich the RB sequence from amino acids 775 to 778 (RPPT) was replacedwith p130 sequence (NMDAPP), which is homologous to the p107 sequence.The p130 sequence was used instead of the p107 sequence becausethe p130 sequence introduced fewer amino acids (Fig. 1B). Thesubstitution mutant (designated mutant 13) had the same impacton c-Abl binding as the mutant in which amino acids 775 to 778were deleted (Fig. 1A).

Each of the individual mutations in either the region from amino acids 775 to 778 or the region from amino acids 825 to 840compromised but did not eliminate c-Abl binding. However, combiningtwo of the most disruptive mutations into a single mutant $---$ either7S (combining mutant 7 with SN) or 13S (combining mutant 13 withSN) $---$ was sufficient to abrogate c-Abl binding (Fig. 1A). Takentogether, these data indicate that the C pocket is composed oftwo noncontiguous regions within RB amino acids 768 to 870. Whiledisruption of either of these regions decreases c-Abl binding,disruption of both regions is required to completely eliminatec-Abl binding.

The consequence of RB binding to c-Abl is the inhibition of c-Abl tyrosine kinase activity (30, 31). This kinase inhibitioncan be recapitulated in vitro with purified GST-RB-C-terminusfusion proteins. GST-SE, which contains a functional C pocket,efficiently inhibits c-Abl kinase activity (Fig. 2, lane 2). Atruncated RB C-terminal fragment, GST-ME, which does not bindc-Abl, does not inhibit c-Abl kinase activity (lane 3). Neithermutant 13S nor mutant 7S could inhibit c-Abl tyrosine kinase (lanes4 and 6, respectively), providing a functional confirmation forthe C-pocket binding defect in mutants 7S and 13S.

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FIG. 2. RB C-pocket mutants do not inhibit c-Abl kinase activity. The indicated GST-RB C-terminal proteins purified from bacteria were incubated with in vitro-translated c-Abl. The c-Abl proteins from these incubations were then subjected to an immune-complex kinase assay, with a GST-CTD fusion protein as the substrate. Phosphorylated CTD was detected by autoradiography (A). The immune complex was also subjected to anti-Abl immunoblot analysis (B) to measure the relative amount of in vitro-translated c-Abl in each reaction. The amount of GST-RB protein present in each reaction mixture was visualized by amido black staining of the nitrocellulose membrane after transfer (C). See Fig. 1 for explanations of the RB fragments.

E2F binding and other activities of the C-pocket mutants. The C-terminal region of RB is required for RB's binding to E2F (5); we therefore examined whether the 7S and 13S mutationsaffected E2F binding activity. First, we assayed for binding ofRB proteins, transiently produced in C33A cells, to GST-E2F-1immobilized on glutathione agarose. Total cell lysates were addedto immobilized GST-E2F-1, and the input and the bound RB proteinswere then detected by anti-RB immunoblotting (Fig. 3A). The bindingof RB to E2F-1 is mediated by the A/B domain interaction witha C-terminal 18-amino-acid peptide in E2F-1 (11). Therefore,mutations in the C-terminal regions were not expected to interferewith the RB-E2F-1 interaction. The wild-type RB did not bind nonspecificallyto GST alone (Fig. 3A, lane 1). C33A cells express a mutant RBwhich is unstable and does not bind to E2F-1 (lane 2) (18).The R661W mutation, which has been shown to disrupt RB-E2F interaction(19), served as an additional control (lane 5). The C-pocketmutants, 7S (lane 4) and 13S (lane 7), were able to bind GST-E2F-1with efficiencies comparable to that of RB (lane 3). Thus, themutations in 7S and 13S did not affect A/B domain-mediated bindingto E2F-1.

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FIG. 3. Interactions of RB mutants with E2F. (A) In vitro binding of RB to GST-E2F-1. Lysates from C33A cells transfected with the indicated construct were collected 48 h posttransfection. These lysates were incubated with GST (lane 1) or GST-E2F-1 (lanes 2 to 8) immobilized on glutathione agarose beads. Relative amounts of the indicated RB proteins in each reaction mixture (input) were determined by anti-RB immunoblot analysis (upper blot). RB proteins bound to the glutathione beads are visualized in the lower blot. The RB band in lane 2 of the input blot is the endogenous mutant RB of C33A cells. wtRB, wild-type RB; ø, vector-transfected cells. (B) Binding of full-length RB mutants to E2F in vivo. Extracts were prepared from C33A cells transfected with the vector (lane 1) or the indicated RB expression constructs (lanes 2 to 7). Immunoprecipitation of E2F DNA-binding activity with anti-RB antibodies has been previously described (32). The immunoprecipitate was treated with DOC, and the released material was assayed for binding to a radiolabeled E2F oligonucleotide. Relative amounts of RB-bound E2F are indicated (upper gel). Relative amounts of the indicated RB proteins in each reaction mixture are determined by anti-RB immunoblot analysis (lower blot). (C) Inhibition of Gal4-E2F-1 activity by RB. Saos-2 cells were cotransfected with $beta$ -galactosidase, the 5×Gal4-CAT reporter, the Gal4-E2F-1 effector, and either the RB, 7S, 13S, 661, 7S-661, or 13S-661 CMV construct as described in Materials and Methods. CAT activity was normalized to $beta$ -galactosidase activity. The CAT activity of Gal4-E2F-1 alone without RB was considered 100%. Results shown are the means and standard deviations of results of three independent experiments.

The association of RB with the functional E2F was then examined by a coimmunoprecipitation-release assay. Mudryj et al. haveshown that E2F DNA-binding activity (which is mediated by theE2F-DP heterodimers) can be immunoprecipitated with anti-RB antibodyand then dissociated from RB by treatment with DOC (16). Bythis assay, E2F DNA-binding activity was found to coimmunoprecipitatewith the wild-type RB (Fig. 3B, lane 2). The mutated RB of C33Acells did not coimmunoprecipitate with E2F (lane 1), nor did mutant661 (lane 4). The 7S mutant, though expressed at the same levelas RB (Fig. 3B [Western blot]), was compromised in its abilityto coimmunoprecipitate functional E2F (lane 3). Mutant 13 coimmunoprecipitatedE2F activity as efficiently as RB (lane 6). Mutant 13S also boundfunctional E2F (lane 7). This result suggested that deletion ofamino acids 775 to 778 in 7S did affect the association of RBwith functional E2F. However, a substitution of p130 sequencefor RB amino acids 775 to 778 in 13S was less disruptive of RB-E2Finteraction.

We next examined the C-pocket mutants for their ability to inhibit the transactivating function of a Gal4-E2F-1 fusion proteinthat contains the transactivating (and RB-binding) domain of E2F-1(Fig. 3C). The 7S and the 13S mutants inhibited Gal4-E2F-1 withefficiencies similar to that of wild-type RB (Fig. 3C). The 661mutant, unable to bind E2F, did not inhibit Gal4-E2F-1 activity(Fig. 3C). These observations are in keeping with the E2F-1-bindingresults (Fig. 3A) and further confirmed that the C-pocket mutationsin 13S and 7S do not disrupt the ability of RB to inhibit thetransactivating function of E2F-1. We have tested the 7S and 13Smutants with four other promoter constructs: an artificial luciferasereporter with three tandem E2F-binding sites (33), the adenovirusE2 promoter, the human cyclin A promoter, and the human cdc2 promoter.We found that 7S and 13S inhibited all four promoters to levelscomparable to that of wild-type RB in transient-cotransfectionassays conducted with either Saos-2 cells or C33A cells (not shown).These results suggested that the two C-pocket mutants, 7S and13S, could interact with E2F at levels sufficient to block itstransactivating function.

In other functional tests, we examined the LXCXE-binding activities of the 7S and 13S mutants, using a GST-E7 fusion proteinas the ligand (9). Consistent with the crystal structure showingthat the LXCXE-binding site resides in the B region only (11),we found that the 7S and 13S mutants bound the human papillomavirustype 16 E7 protein as well as wild-type RB did (not shown). The7S and 13S mutations did not affect RB phosphorylation (see theanti-RB blot in Fig. 3B). The R661W mutation did interfere withRB phosphorylation in C33A cells, possibly because the LXCXE-bindingsite is required to recruit cyclin D, which is responsible forRB phosphorylation (22). The 7S and 13S mutants localized tothe nuclei of Saos-2 and C33A cells (not shown). In addition,the 7S and 13S mutations did not affect the binding of RB to Mdm2(33) (not shown). Taken together, the results of these analysessuggested that the 13S mutation affected only c-Abl binding butthat the 7S mutations affected both biding to c-Abl and bindingto E2F. We could not rule out the possibility that the 13S mutationalso affected other unidentified functions of RB.

The 13S mutations abolished the G₁/S-inhibitory activity associated with the RB C-terminal fragment. Welch and Wang have previously shown that the C-terminal fragment of RB, when expressed alone, cannot suppress the growthof Saos-2 cells as determined by the induction of growth-arrestedflat cells and the inhibition of colony formation (32). Expressionof RB in Saos-2 cells also induces an increase in the G₁ population,which can be detected within 48 h of transfection (6). To assayfor an increase in the G₁ population, Saos-2 cells were cotransfectedwith plasmids expressing the RB mutants of interest and the cellsurface marker CD20. Forty-eight hours posttransfection, the DNAcontent of CD20-positive cells was determined by FACS analysis.When cotransfected with RB, ~70% of the CD20-positive cells werein G₁ whereas only ~40% of the vector-cotransfected CD20-positivecells had G₁ DNA content (Table 1). Expressing the C-terminalSE fragment (containing RB amino acids 768 to 928) (Fig. 1) ata level similar to that of RB did not induce an increase in theG₁ population (not shown). However, when SE was overproduced toa level that was threefold higher, it caused an increase in thepercentage of G₁ cells (Table 1). A C-terminal fragment (SE $Delta$ )which lacks a region required for E2F binding (5, 32) (Fig.1) also caused an increase in the G₁ population (Table 1), suggestingthat E2F binding is not essential to the G₁-inhibitory activityof SE. An SE fragment with the C-pocket mutation 13S (SE-13S),when expressed at levels equivalent to that of SE, was unableto cause an increase in the G₁ population of Saos-2 cells (Table1).

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TABLE 1. Effect of RB C-terminal fragments on cell cycle progression

To test if the increase in G₁ cells caused by SE and SE $Delta$ was the result of a G₁ arrest or a lengthening of the G₁ phase, transfectedSaos-2 cells were treated with nocadozole, which blocks cellsat G₂/M (Table 1). If cells are arrested in G₁, nocadozole willnot cause an increase in G₂/M. However, if cells are slowly progressingthrough G₁, nocadozole treatment will lead to an increase in G₂/M(12). Nocadozole treatment did not affect the percentage ofG₁, S, or G₂ cells in the RB-transfected population (Table 1),consistent with previous results demonstrating G₁ arrest (12).While nocadozole treatment did not alter the percentage of G₁cells in the SE- or SE $Delta$ -transfected population, the percentageof cells in S phase was decreased and the percentage of cellsin G₂/M phase was increased (Table 1), indicating a prolongedG₁ phase but a slow progression through the cell cycle. The cellstransfected with the SE-13S mutant showed a reduction in G₁ populationand a concomitant increase in G₂/M population after nocadozoletreatment, consistent with the inability of SE-13S to slow cellsin G₁ (Table 1).

Welch and Wang have previously constructed a c-Abl mutant (AS2) which does not bind RB and is therefore resistant to the inhibitoryeffect of RB. When overproduced, AS2 can antagonize RB in flat-cellformation and colony inhibition assays (30). Because SE, butnot SE-13S, can induce an increase in the G₁ population, we testedwhether the binding and/or the inhibition of c-Abl tyrosine kinasewas required for this activity. Towards this end, we coexpressedSE and c-Abl-AS2 in Saos-2 cells. If the G₁-inhibitory activityof SE were due to the inhibition of c-Abl tyrosine kinase, thenc-Abl-AS2 would be expected to override that activity. However,this was not the case. The expression of c-Abl-AS2 did not alterthe cell cycle distribution of transfected, CD20-positive Saos-2cells (not shown). Moreover, coexpression of c-Abl-AS2 did nothave any detectable effect on an SE-induced increase in the percentageof cells in G₁ (not shown). Taken together, these results showthat the SE-mediated increase in the G₁ population is disruptedby the 13S mutation; however, this effect cannot be reversed bya constitutive Abl-AS2 kinase that does not interact with RB.

The 7S, 13S, or 661 mutations do not affect the G₁/S-inhibitory function of full-length RB. The 13S mutation had no effect on the G₁/S-inhibitory activity of the full-length RB. The percentages of G₁ cells of one representativeexperiment are shown in Fig. 4A. Overall, CD20-positive cellscotransfected with RB were between 70 and 85% G₁ whereas vector-cotransfectedcells were between 40 and 55% G₁. Both the 7S and 13S mutantscaused consistent increases in percentages of G₁ cells to levelscomparable to that of wild-type RB (Fig. 4A). The 661 mutant alsoinduced an increase in G₁ cells comparable to that of RB in Saos-2cells (Fig. 4A). In these experiments, different amounts of expressionplasmids were used to achieve the same levels of RB accumulationat 48 h posttransfection (for example, see Fig. 5C). Thus, neitherthe A/B domain mutation nor the C-region mutations affected theability of full-length RB to induce an increase in the percentageof cells in G₁.

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FIG. 4. Abilities of RB mutants to induce G₁ arrest. (A) Induction of an increase in the G₁ population of Saos-2 cells. Saos-2 cells were cotransfected with CMV- $beta$ -galactosidase, CD20, the DHFR-Luc reporter, or the mutDHFR-Luc reporter and either the vector, wild-type RB (wtRB), 7S, 13S, 661, 7S-661, or 13S-661 (as described in Materials and Methods). One-half of each transfection mixture was used for cell cycle analysis, and the other half was used for a luciferase assay (B). Transfected cells were stained for CD20 and DNA (see Materials and Methods). The gated CD20-positive cells were analyzed by FACS analysis for DNA content. Results of a representative experiment are shown. Similar results were obtained from three additional independent experiments. %G₁, percent increase in number of cells in G₁. (B) Repression of the DHFR promoter in Saos-2 cells. One-half of the transfected Saos-2 cells in panel A were analyzed for luciferase activity, which was normalized to cotransfected $beta$ -galactosidase activity to correct for transfection efficiency. The normalized luciferase activities are represented as percentages of the luciferase activity of vector-cotransfected cells (ø), which is considered 100%. Results shown are the means and standard deviations of results from four independent experiments. (C) Inability of RB to induce an increase in the G₁ population of C33A cells. C33A cells were cotransfected with CMV- $beta$ -galactosidase, CD20, the DHFR-Luc reporter, or the mutDHFR-Luc reporter and either the vector, RB, 7S, 13S, 661, 7S-661, or 13S-661 as described for panel A. Transfected cells were stained for CD20 and DNA, and the percentages of cells in G₁ were determined as described in Materials and Methods. (D) Repression of the DHFR promoter in C33A cells. C33A cells were analyzed as described for panel B. Normalized luciferase activities are represented as percentages of the luciferase activity of vector-cotransfected cells (ø), which is considered 100%. Results shown are the means and standard deviations of results from four independent experiments.

The ability to cause an increase in the G₁ population correlated with the repression of the DHFR promoter by the RB mutants.The DHFR promoter contains an E2F-binding sequence which is responsiblefor the repression of this promoter in G₀/G₁ cells (7, 20,23). The effect of RB mutants on DHFR promoter activity wasexamined with a reporter that contains the region from $-$ 270 to+20 of the DHFR gene. A mutant promoter lacking the E2F-bindingsite was also examined for comparison (Fig. 4B). Mutation of theE2F-binding site did not abolish promoter activities in Saos-2cells or C33A cells (Fig. 4B and D, compare the ø samples of DHFR-Lucand mutDHFR-Luc). These results showed that transcription fromthis promoter fragment in Saos-2 and C33A cells is stimulatedby factors other than E2F (20, 23). Cotransfection with RBrepressed DHFR promoter activity in Saos-2 cells (Fig. 4B, lanewith wild-type RB and DHFR-Luc), and this repression was abolishedby the mutation of the E2F site (Fig. 4B, lane with wild-typeRB and mutDHFR-Luc). In Saos-2 cells, 7S and 13S also repressedthe DHFR promoter and this was again dependent on the E2F site(Fig. 4B). The 661 mutant, although unable to bind E2F (19),also repressed the DHFR promoter in Saos-2 cells (Fig. 4B). Mutationof the E2F site reduced but did not abolish the repressive activityof 661 on the DHFR promoter (Fig. 4B, compare lanes with 661 tolanes with wild-type RB), suggesting that 661 might repress theDHFR promoter through a mechanism that does not require a stableRB-E2F interaction.

The repression of the DHFR promoter may be mediated by one of two mechanisms: (i) a direct RB-E2F interaction at the promoterand (ii) an increase in the G₁ population that leads to repression,possibly through endogenous p130-p107-E2F complexes (7, 23).To distinguish between these two possibilities, we repeated theDHFR promoter assays with the RB-negative C33A cells, which donot become arrested in G₁ with the introduction of exogenous RB(35). As shown in Fig. 4C, expression of RB or the various mutantsdid not increase the G₁ population. In C33A cells, RB was ableto repress the DHFR promoter, albeit at only a twofold reduction,compared to the eightfold reduction observed with Saos-2 cells(compare lanes with wild-type RB and DHFR-Luc in Fig. 4B and D).Interestingly, 7S, 13S, and 661 were unable to repress the DHFRpromoter in these C33A cells (Fig. 4D). These results suggestthat the repression of the DHFR promoter by the RB mutants isthe result of an increase in the G₁ population in Saos-2 cells.Since the E2F-binding sites are involved, it is possible thatthis repression is mediated by endogenous p107-p130. Because the7S, 13S, and 661 mutants did not repress the DHFR promoter inC33A cells, these results also suggest that both the A/B domainand the C pocket are required to achieve the twofold repressionof the DHFR promoter by wild-type RB in C33A cells.

The 7S, 13S, and 661 mutations affect the growth suppression function to various degrees. Because the increase in the G₁ population at 48 h posttransfection may have been the result of a lengthening of the G₁ phasebut not a permanent G₁ arrest, we tested the mutants by two otherassays: a flat cell induction assay and a colony formation inhibitionassay (Fig. 5). When transfected into Saos-2 cells, RB can inhibitthe formation of drug-resistant colonies, measured at 14 daysposttransfection (17, 32) (Fig. 5A). In our assay, cotransfectionwith RB led to a fivefold reduction in colony numbers relativeto the number for the vector control (Fig. 5A, bar wtRB). The13S mutant was compromised in its ability to suppress G418-resistantcolonies, producing ~50% of the level of activity produced bythe wild type in repeated experiments (Fig. 5A, bar 13S). The7S mutant, though capable of inducing an increase in the G₁ population(Fig. 4A), was unable to suppress colony formation (Fig. 5A, bar7S) at an expression level equivalent to that of RB (Fig. 5C,lane 7S). The 661 mutant exhibited consistent but weak activityin colony suppression, producing only 25 to 30% of the level ofactivity produced by the wild type (Fig. 5A).

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FIG. 5. Effects of C-pocket mutations on terminal growth arrest. (A) Inhibition of neomycin-resistant colony formation. The vector used to express RB and the various mutants contained a neomycin resistance gene. The expression plasmid DNA was transfected into Saos-2 cells. Transfectants were subjected to G418 selection for 2 to 3 weeks. The number of neomycin-resistant colonies arising from each transfectant was counted and expressed as a percentage relative to the number of such colonies in the vector-alone transfectant, which was considered 100%. Results shown are the means and standard deviations of results of four independent experiments. wtRB, wild-type RB; ø, vector-cotransfected cells. (B) Induction of flat-cell formation. Saos-2 cells were cotransfected with pCMVneo-RB, -7S, -13S, -661, -7S-661, -13S-661, or -vector and a puromycin resistance plasmid. Transfected cells were selected with puromycin for 7 days. Resulting flat cells were counted in each dish, and the number of flat cells formed for each transfectant was expressed a percentage of the number of flat cells formed by RB, which was considered 100%. Results shown are the means and standard deviations of results from four independent experiments. (C) Protein expression levels. The amount of plasmid transfected was titrated to yield equal levels of RB protein expression. Saos-2 cells transfected with RB, 7S, 661, 7S-661, 13S, or 13S-661 were divided into three equal parts: one-third of the cells was used for the colony formation assay (A), one-third was used for the flat-cell assay (B), and one-third was collected at 48 h posttransfection for protein analysis (C). Equal amounts of total protein from lysates collected from the transfected cells were separated on an SDS-7.5% polyacrylamide gel. RB proteins were detected with anti-RB 245 antibody (Pharmingen). The transfected pCMV-RB expression construct for each lysate is indicated.

Expression of RB in Saos-2 cells also induced the formation of large flat cells whose state appeared to be senescent and/ordifferentiated (19, 25). Previous work showed that both theA/B and C regions of RB are required for flat-cell formation (5,17, 30). In our flat-cell assay, 13S exhibited 60% of thelevel of activity exhibited by the wild type whereas 7S was completelydefective (Fig. 5B). The 661 mutant was capable of inducing flatcells with approximately 30% efficiency relative to that of RB(Fig. 5B). Taken together, these results showed that the inductionof flat cells and the inhibition of colony formation by RB aredifferentially affected by the 7S, 13S, and 661 mutations (Fig.5). This finding is in direct contrast to results from inductionof an increase in the G₁ population, which is not affected byany of the three mutations alone (Fig. 4).

Combining the 7S or 13S mutations with R661W abrogates the G₁/S and the growth suppression activities of RB. The tumor suppression function of 661 is compromised; however, this mutant retains sufficient activity to protect againstretinoblastoma in some carriers. As the C-terminal region of 661is intact, the residual biological function of 661 may dependon the function of the C pocket. To test this idea, we inactivatedthe C pocket of 661 through the construction of 7S-661 and 13S-661.

The 7S-661 and 13S-661 mutants could be stably expressed in Saos-2 cells (Fig. 5C) and C33A cells (Fig. 3B). At expressionlevels comparable to that of RB, 7S-661 and 13S-661 did not increasethe G₁ population at 48 h after transfection (Fig. 4A) or represstranscription from the DHFR promoter (Fig. 4B). These mutantsdid not suppress colony formation (Fig. 5A), and they did notinduce flat-cell formation (Fig. 5B). Abrogation of the G₁/S-inhibitoryactivity of 661 by 7S or 13S suggests that an intact C-terminalregion is required for this activity. This suggestion is consistentwith the observations that SE alone can cause an increase in theG₁ population and that this increase is inactivated by the 13Smutations. Conversely, the G₁/S-inhibitory activity of 13S mustrequire an intact A/B domain, which is disrupted by 661. Regardingthe growth suppression functions as measured by flat-cell formationor colony inhibition, the 7S-661 mutant was uninformative because7S itself has no detectable growth suppression function. Becausethe C-terminal fragment alone did not have any growth suppressionfunction, the partial activity of 661 could not be attributedto the C region alone. However, an intact C region is requiredfor the biological activity of this low-penetrance retinoblastomamutation because 661-13S is defective in growth suppression assays.

Fusion with the E2F-1 DNA-binding domain does not rescue the 13S-661 mutant. Although 661 did not detectably bind to E2F (Fig. 3), the residual activity of 661 in the growth suppression assays may havebeen due to weak binding to E2F mediated by the mutant's C-terminalregion. It might be argued that the defect of 13S-661 was dueto the disruption of this weak E2F interaction by the 13S mutation.If this were the case, then the fusion of the E2F-1 DNA-bindingdomain with 13S-661 would be expected to rescue the 13S-661 mutant.Sellers et al. previously demonstrated that fusion of the A/Bdomain of RB with the DNA-binding and dimerization domain of E2F-1generates a transcription repressor that can induce an increasein the G₁ population of Saos-2 cells (21). Following their strategy,we constructed two fusion proteins in which the E2F-1 DNA-bindingand dimerization domain (E2F-1 amino acids 1 to 368 [DBD]) waslinked in frame with the A/B/C region (amino acids 379 to 928)of either 661 or 13S-661 (DBD-661 and DBD-13S-661, respectively)(Fig. 6A). As a control, we used the fusion construct previouslydescribed by Sellers et al. DBD-A/B (21), in which the DNA-bindingdomain of E2F-1 is linked in frame with RB amino acids 379 to793 (Fig. 6A). The DBD-A/B fusion, therefore, lacks a functionalC pocket.

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FIG. 6. Loss of function of the RB 13S-661 mutant cannot be rescued by fusion with the E2F DNA-binding domain. (A) E2F-RB mutant fusion constructs. An E2F-1 fragment from amino acids (aa) 1 to 368 containing the E2F DNA binding domain was fused in frame to RB amino acids 379 to 928 containing either the 661 mutation (DBD-661) or the 661 mutation plus the 13S C-pocket mutation (DBD-13S-661). The E2F-1 DBD and DBD-A/B have been previously described (21). (B) Fusion of an E2F DNA binding domain does not enhance the formation of flat cells. DBD, RB, DBD-A/B, DBD-661, 661, DBD-13S-661, 13S-661, or pCMVneo was cotransfected with a puromycin resistance plasmid into Saos-2 cells. Cells were selected for 7 days in medium containing puromycin, and flat cells were counted. The number of flat cells formed for each transfectant was expressed as a percentage of the number of flat cells formed by RB, which was considered 100%. Results shown are the means and standard deviations of results from three independent experiments. ø, vector-transfected cells.

These fusion constructs were tested for their ability to induce flat Saos-2 cells (Fig. 6B). Both DBD-661 and 661 inducedflat-cell formation at ~30% of the wild-type level of efficiency(Fig. 6B). Thus, the addition of the E2F DNA-binding domain didnot increase the growth suppression function of 661. The E2F DBD-13S-661fusion protein, like 13S-661, did not induce flat-cell formation(Fig. 6B). Thus, the addition of the E2F-1 DNA-binding domaindid not rescue the defect of 13S-661. Sellers et al. have previouslyreported that the A/B fragment alone (amino acids 379 to 792)does not have any biological activities but that the fusion proteinDBD-A/B can inhibit E2F-dependent transcription and induce anincrease in the G₁ population (21). In our hands, DBD-A/B alsocaused an increase in the G₁ population (not shown). However,this DBD-A/B fusion did not induce flat-cell formation (Fig. 6B).Taken together, these results showed that the tethering of 13S-661to E2F sites did not restore the growth suppression function.In addition, the lack of C-pocket activity was correlated withthe inability of DBD-A/B and 13S-661 to induce flat Saos-2 cells.

Coexpression of SE, but not SE-13S, disrupts the growth suppression activity of wild-type RB. The partial growth suppression activity of 661 could not be attributed entirely to its intact C region. This is because theC-terminal region alone cannot induce flat cells and it cannotinhibit colony formation (32). Consistently with previous results(32), expression of the SE, SE $Delta$ , and SE-13S C-terminal fragmentsdid not induce flat cells or inhibit neomycin-resistant-colonyformation (Table 2). Welch and Wang have reported that coexpressionwith SE or SE $Delta$ can abrogate the growth suppression activity offull-length RB and showed that SE and SE $Delta$ could compete with RBfor binding to c-Abl (32). If binding to c-Abl is required forSE and SE $Delta$ to disrupt the function of RB, then SE-13S should notinterfere with RB. This was indeed the case (Table 2). Usingthe flat-cell formation assay, we found that the coexpressionof SE or SE $Delta$ with RB caused a 10- to 20-fold reduction in thenumber of flat cells. However, coexpression with SE-13S did notreduce the number of flat cells induced by RB (Table 2). Theseobservations show that the ability to bind c-Abl is necessaryfor the C-terminal RB fragment to exert a dominant negative effecton the growth suppression function of wild-type RB.

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TABLE 2. Effects of RB C-terminal fragments on terminal growth arrest

While SE and SE $Delta$ can interfere with RB in flat-cell and colony formation assays, they did not interfere with the inductionof an increase in the G₁ population by RB (not shown). This resultis consistent with the observations that SE and SE $Delta$ alone caninduce an increase in the number of cells in G₁ and that the DBD-A/Bfusion of Sellers et al. can also induce such an increase (21).Thus, the A/B and C regions of RB appear to be able to cause anincrease in the G₁ population independently of each other.

DISCUSSION
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Definition of the RB C pocket. The mutational analysis described here has further characterized the RB C pocket, defined as the c-Abl binding site. First,the C pocket is within the minimal functional domain of RB (RBamino acids 395 to 876). Second, two nonconsecutive amino acidsequences in the C-terminal region, from 768 to 785 and from 825to 840, are important for the c-Abl-binding function (Fig. 1).Third, the c-Abl-binding function requires RB amino acids thatare not conserved in p107-p130. The mutational analysis supportsthe previous conclusion that c-Abl and E2F can simultaneouslybind to RB (32), as mutations that disrupt E2F binding do notaffect c-Abl binding; conversely, mutations that disrupt c-Ablbinding do not disrupt E2F binding.

The C-terminal region of RB also binds to Mdm2 (33). Janicke et al. have recently shown that Mdm2 binding requires the extremeC-terminal sequences of RB (8). RB is cleaved at a caspaseconsensus site at amino acid 884 during apoptosis (reviewed inreference 24). Caspase-cleaved RB, which is shortened by only44 amino acids, does not bind Mdm2 (8, 24). Cleavage by caspaseat amino acid 884 does not affect c-Abl binding (23a), consistentwith the mapping results shown in Fig. 1. Because Mdm2 bindingrequires amino acids C terminal to the minimal functional domainof RB (amino acids 395 to 876), the RB-Mdm2 interaction may notcontribute to growth suppression but may be important in the regulationof apoptosis (reviewed in references 24 and 26).

Induction of an increase in the percentage of cells in G₁ can be distinguished from the growth suppression function of RB. Previous studies of RB mutations have generated a simple picture in which the loss of E2F binding is correlated with the completeinactivation of RB (28). Results obtained from the analysesof the 7S, 13S, and 661 mutations (see Table 3 for a summary),however, have allowed the separation of two distinct functionsof RB in Saos-2 cell-based assays: (i) inhibition of G₁/S progression,as measured by an increase in the percentage of cells in G₁, and(ii) long-term growth arrest, as measured by the inhibition ofcolony formation and the induction of flat cells.

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TABLE 3. Summary of growth-inhibitory activities of RB mutants

(i) The A/B and C regions of RB can each induce an increase in the percentage of cells in G₁. Three different types of RB mutants $---$ 7S, the DBD-A/B fusion (21), and a C-terminal fragment (SE or SE $Delta$ ) $---$ can cause an increasein the G₁ population but are unable to induce terminal growtharrest (Table 3). The 7S mutant does not bind c-Abl and is compromisedfor binding to E2F (Fig. 2 and 3). The DBD-A/B fusion does notbind to c-Abl or E2F; however, it can be tethered to E2F sitesthrough fusion with E2F-1 DBD (21). The SE and SE $Delta$ fragmentsdo not contain the A/B domain. The fact that all three types ofmutants can cause an increase in the percentage of cells in G₁suggests (i) that the A/B domain can increase the G₁ populationwhen it is tethered to E2F sites without the C-terminal regionand (ii) that the C-terminal region can increase the G₁ populationwithout the A/B domain. The conclusion that the A/B and C regionscan each inhibit G₁/S progression is further supported by thefollowing observations. Disruption of the A/B domain by 661 didnot affect G₁/S-inhibitory activity. Disruption of the C pocketby 13S also had no detectable effect on this activity of RB. However,combination of these two mutations completely abolished G₁/S-inhibitoryactivity (Table 3).

The negative effect of RB on G₁/S progression has been attributed to the repression of E2F-regulated genes (28). A recentstudy conducted with Rb-deficient mouse embryo fibroblasts demonstratedthat the expression of many E2F-regulated genes was not significantlyaltered; however, the G₁ phase was shortened in the absence ofRB function (7). It thus appears that critical genes involvedin G₁/S progression and controlled by RB are yet to be identified.The recent demonstration of RB binding to a histone deacetylasecan account for the RB-mediated repression of promoters containingE2F sites (3, 14, 15). The 7S and the DBD-A/B mutants containa functional LXCXE-binding site, and they may inhibit G₁/S progressionby recruiting histone deacetylase to E2F-regulated promoters.Sellers et al. have shown that introduction of either the C706For the R661W mutation into the DBD-A/B fusion can inactivate itsfunction (21). Thus, an intact LXCXE-binding site is importantfor the A/B domain to cause an increase in the percentage of cellsin G₁ when the domain is tethered to E2F sites.

The observation that 661 and SE, both of which do not bind E2F or LXCXE proteins, can also cause an increase the G₁ populationsuggests that RB may do so through mechanisms other than the bindingto E2F and histone deacetylase. Introduction of the 13S mutationcan eliminate the G₁/S-inhibitory functions of both 661 and SE(Table 3). Introduction of the mutation deleting amino acids785 to 806, which disrupts E2F binding but not c-Abl binding,does not affect this activity of SE (Table 3). Thus, the G₁/S-inhibitoryactivity associated with the C-terminal region of RB can be correlatedwith binding to c-Abl. Since constitutively active c-Abl-AS2 (30)cannot overcome SE, the inhibition of c-Abl kinase activity isnot important for the lengthening of G₁ phase. This, however,does not rule out the possibility that binding to c-Abl is requiredfor SE to induce an increase in the G₁ population. In additionto binding RB, the c-Abl protein contains two distinct bindingsites for CTD of RNA polymerase II and has been shown to associatewith RNA polymerase II in vivo (1, 2, 4). Binding toc-Abl may be required to bring the SE fragment to the transcriptionmachinery. At present, we cannot rule out that the 13S mutationsmay have also inactivated other functions of RB. Welch and Wanghave previously argued that c-Abl binding is not the only biologicallyimportant function of the C region of RB (30, 32). The G₁-inhibitoryactivity of the RB SE fragment may well be mediated through asyet unidentified mechanisms unrelated to RB-c-Abl interaction.

(ii) The A/B and C regions cooperate to induce growth arrest. The minimal functional domain of RB includes the A/B and C regions of RB, between amino acids 395 and 876 (5, 17). Thisfunctional domain can bind to E2F, histone deacetylase, c-Abl,and other targets (reviewed in references 20, 26, and 27).Because the tethering of a functional A/B domain to E2F sites(achieved with the DBD-A/B fusion) cannot induce flat-cell formation,the C region is required for growth suppression (Table 3). Becausethe C-terminal fragment of RB is also unable to induce flat cells,the A/B domain is required as well (Table 3). Moreover, coexpressionof the SE fragment with RB disrupts its growth suppression function(32). These results suggest that activities associated withthe A/B and C regions may have to cooperate to induce growth arrest.The A/B and C regions clearly cooperate to bind E2F (5, 17),and E2F binding has been proposed to be the only reason why theC region is required for growth suppression. This model cannotexplain how 661, which does not bind to E2F, can induce growtharrest (see also the report of Sellers et al. [19]). Sellerset al. have proposed that 661 suppresses Saos-2 growth by inducinga terminal differentiation program (19). We show here that the661 function can be inactivated by the 13S mutations (Table 3).The precise mechanism by which 661 suppresses growth is presentlyunknown. Analyses performed in this study suggest that the A/Band C regions of 661 also cooperate to provide the reduced butsignificant growth suppression function.

The role of C pocket in growth suppression. Three lines of evidence have argued for the importance of an RB-c-Abl interaction in the induction of growth arrest. First,overproduction of c-Abl-AS2 can override the growth suppressionfunction of RB (30). Second, coexpression with SE, but not SE-13S,can disrupt the growth suppression function of RB. Third, thetethering of the A/B domain to E2F sites (DBD-A/B) can inducean increase in the G₁ population but not increase the number offlat cells. However, those results did not prove the C pocketto be essential. The contribution of C-pocket activity can beassessed only through analyses of the C-pocket mutations.

Effects of the C-pocket mutations on the biological activities of RB are complex. In the context of the C region alone, whichby itself can delay G₁/S progression, disruption of the C pocketinactivated this biological function. In the context of the full-lengthRB, however, the disruption of RB-c-Abl interaction did not havea significant effect on growth suppression. The 7S mutations abolishedgrowth suppression (Table 3), but the severity of the 7S mutationsmay be due to a combined defect in c-Abl and E2F binding (Fig.2 and 3). It should be noted that 7S binds E2F better than 661(Fig. 3), yet 7S is defective and 661 has partial function. Thecombined mutations of 13S and 661 also completely abolished biologicalactivities. Taken together, these results show that C-pocket activitybecomes essential to growth suppression in the context of otherRB mutations that weaken the RB-E2F interaction.

A possible interpretation of the various phenotypes of these RB mutants is to consider that the A/B and C regions of RB canalso bind targets other than E2F, histone deacetylase, and c-Abl.Each of these multiple targets of RB may contribute to the growthsuppression activities measured in Saos-2 cell-based assays. Thecrippled A/B domain of 661 may retain some activity in bindingto proteins other than E2F and histone deacetylase. In the contextof 661, an intact C region becomes critical for either the formationor the functioning of these alternative protein complexes thatcause growth inhibition. In the context of wild-type RB, the Cpocket is less important as the assembly of E2F and LXCXE proteincomplexes may be sufficient to suppress growth. In any event,the complete loss of function associated with the 13S-661 doublemutant supports a role for the RB C pocket in the induction oflong-term growth arrest.

ACKNOWLEDGMENTS
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We thank Paolo Vigneri, Lauren Wood, and Pam Woodring for critically reading the manuscript. We also thank the following researchersfor the generous provision of reagents: B. Vogelstein (Johns HopkinsUniversity); E. Harlow (Massachusetts General and Harvard); H.Land (Imperial Cancer Research Fund, London, United Kingdom);W. Krek, D. Livingston, W. Sellers, and W. Kaelin, Jr. (Dana-FarberCancer Institute); S. Hiebert (St. Jude Children's Hospital);C. Murre (University of California, San Diego); and A. Means andP. Farnham (McArdle Laboratory for Cancer Research, Universityof Wisconsin Medical School).

H.S. was supported by National Institutes of Health grant CA66314. R.B. was supported by Council for Tobacco Research grantCTR3762. This research was supported by National Institutes ofHealth grant CA58320 to J.Y.J. Wang.

FOOTNOTES

^* Corresponding author. Mailing address: Department of Biology, Bonner Hall 3326, UCSD, 9500 Gilman Dr., La Jolla, CA 92093-0322.Phone: (619) 534-6253. Fax: (619) 534-2821. E-mail: jywang{at}ucsd.edu.

In memory of Laura L. Whitaker, 25 February 1998.

REFERENCES
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3. Brehm, A., E. Miska, D. McCane, J. Reid, A. Bannister, and T. Kouzarides. 1998. Retinoblastoma protein recruits histone deacetylase to repress transcription. Nature 391:597-601[Medline].

4. Duyster, J., R. Baskaran, and J. Y. J. Wang. 1995. Src homology 2 domain as a specificity determinant in the c-Abl mediated tyrosine phosphorylation of the RNA polymerase II carboxyl-terminal repeated domain. Proc. Natl. Acad. Sci. USA 92:1555-1559[Abstract/Free Full Text].

5. Hiebert, S. W. 1993. Regions of the retinoblastoma gene product required for its interaction with the E2F transcription factor are necessary for E2 promoter repression and pRb-mediated growth suppression. Mol. Cell. Biol. 13:3384-3391[Abstract/Free Full Text].

6. Hinds, P. W., S. Mittnacht, V. Dulic, A. Arnold, S. I. Reed, and R. A. Weinberg. 1992. Regulation of retinoblastoma protein functions by ectopic expression of human cyclins. Cell 70:993-1006[Medline].

7. Hurford, R. K., D. Cobrinik, M.-H. Lee, and N. Dyson. 1997. pRB and p107/p130 are required for the regulated expression of different sets of E2F responsive genes. Genes Dev. 11:1447-1463[Abstract/Free Full Text].

8. Janicke, R. U., P. A. Walker, X. Y. Lin, and A. G. Porter. 1996. Specific cleavage of the retinoblastoma protein by an ICE-like protease in apoptosis. EMBO J. 15:6969-6978[Medline].

9. Knudsen, E. S., and J. Y. J. Wang. 1996. Differential regulation of retinoblastoma protein function by specific cdk phosphorylation sites. J. Biol. Chem. 271:8313-8320[Abstract/Free Full Text].

10. Kratzke, R. A., G. A. Otterson, A. Hogg, A. B. Coxon, J. Geradts, J. K. Cowell, and F. J. Kaye. 1994. Partial inactivation of the RB product in a family with incomplete penetrance of familial retinoblastoma and benign retinal tumors. Oncogene 9:1321-1326[Medline].

11. Lee, J.-O., A. Russo, and N. Pavletich. 1998. Structure of the retinoblastoma tumor suppressor pocket domain bound to a peptide from HPV E7. Nature 391:859-865[Medline].

12. Lees, E., B. Faha, V. Dulic, S. I. Reed, and E. Harlow. 1992. Cyclin E/cdk2 and cyclin A/cdk2 kinases associate with p107 and E2F in a temporally distinct manner. Genes Dev. 6:1874-1885[Abstract/Free Full Text].

13. Lohmann, D., B. Brandt, W. Hooping, E. Passarge, and B. Horsthemke. 1994. Distinct Rb1 gene mutations with low penetrance in hereditary retinoblastoma. Hum. Genet. 94:349-354[Medline].

14. Luo, R., A. Postigo, and D. Dean. 1998. RB interacts with histone deacetylase to repress transcription. Cell 92:463-473[Medline].

15. Magnaghi-Jaulin, L., R. Groisman, I. Naguibneva, P. Robin, S. Lorain, J. L. Villain, F. Troalen, D. Trouche, and A. Harel-Bellan. 1998. Retinoblastoma protein represses transcription by recruiting a histone deacetylase. Nature 391:601-605[Medline].

16. Mudryj, M., S. H. Devoto, S. W. Hiebert, T. Hunter, J. Pines, and J. R. Nevins. 1991. Cell cycle regulation of the E2F transcription factor involves an interaction with cyclin A. Cell 65:1243-1253[Medline].

17. Qin, X.-Q., T. Chittenden, D. M. Livingston, and W. G. Kaelin, Jr. 1992. Identification of a growth suppression domain within the retinoblastoma gene product. Genes Dev. 6:953-964[Abstract/Free Full Text].

18. Scheffner, M., K. Munger, J. Byrne, and P. Howley. 1991. The state of the p53 and retinoblastoma genes in human cervical carcinoma cell lines. Proc. Natl. Acad. Sci. USA 88:5523-5527[Abstract/Free Full Text].

19. Sellers, W., B. Novitch, S. Miyake, A. Heith, G. Otterson, F. Kaye, A. Lassar, and W. G. Kaelin, Jr. 1998. Stable binding to E2F is not required for the retinoblastoma protein to activate transcription, promote differentiation and suppress tumor cell growth. Genes Dev. 12:95-106[Abstract/Free Full Text].

20. Sellers, W. R., and W. G. Kaelin, Jr. 1996. RB as a modulator of transcription. Biochim. Biophys. Acta 1288:1-5.

21. Sellers, W. R., J. W. Rodgers, and W. G. Kaelin, Jr. 1995. A potent transrepression domain in the retinoblastoma protein induces a cell cycle arrest when bound to E2F sites. Proc. Natl. Acad. Sci. USA 92:11544-11548[Abstract/Free Full Text].

22. Sherr, C. 1996. Cancer cell cycles. Science 274:1672-1677[Abstract/Free Full Text].

23. Slanksy, J. E., and P. J. Farnham. 1996. Introduction to the E2F family: protein structure and gene regulation. Curr. Top. Microbiol. Immunol. 208:1-30[Medline].

23a. Tan, X.-Q., H. Su, and J. Y. J. Wang. Unpublished data.

24. Tan, X.-Q., and J. Y. J. Wang. 1998. The caspase-RB connection in cell death. Trends Cell Biol. 8:116-120. [Medline]

25. Templeton, D. J., S. H. Park, L. Lanier, and R. A. Weinberg. 1991. Nonfunctional mutants of the retinoblastoma protein are characterized by defects in phosphorylation, viral oncoprotein association, and nuclear tethering. Proc. Natl. Acad. Sci. USA 88:3033-3037[Abstract/Free Full Text].

26. Wang, J. Y. J. 1997. Retinoblastoma protein in growth suppression and death protection. Curr. Opin. Genet. Dev. 7:39-45[Medline].

27. Wang, J. Y. J., E. S. Knudsen, and P. J. Welch. 1994. The retinoblastoma tumor suppressor protein. Adv. Cancer Res. 64:25-85[Medline].

28. Weinberg, R. A. 1995. The retinoblastoma protein and cell cycle control. Cell 81:323-330[Medline].

29. Weintraub, S. J., K. N. B. Chow, R. X. Luo, S. H. Zhang, S. He, and D. C. Dean. 1995. Mechanism of active transcriptional repression by the retinoblastoma protein. Nature 375:812-815[Medline].

30. Welch, P. J., and J. Y. J. Wang. 1995. Abrogation of retinoblastoma protein function by c-Abl through tyrosine kinase-dependent and -independent mechanisms. Mol. Cell. Biol. 15:5542-5551[Abstract].

31. Welch, P. J., and J. Y. J. Wang. 1993. A C-terminal protein-binding domain in the retinoblastoma protein regulates nuclear c-Abl tyrosine kinase in the cell cycle. Cell 75:779-790[Medline].

32. Welch, P. J., and J. Y. J. Wang. 1995. Disruption of retinoblastoma protein function by coexpression of its C pocket fragment. Genes Dev. 9:31-46[Abstract/Free Full Text].

32a. Welch, P. J., and J. Y. J. Wang. Unpublished data.

33. Xiao, Z.-X., J. Chen, A. Levine, N. Modjtahedi, J. Xing, W. R. Sellers, and D. M. Livingston. 1995. Interaction between the retinoblastoma protein and the oncoprotein MDM2. Nature 375:694-698[Medline].

34. Zacksenhaus, E., Z. Jiang, D. Chung, J. D. Marth, R. A. Phillips, and B. L. Gallie. 1996. pRb controls proliferation, differentiation, and death of skeletal muscle cells and other lineages during embryogenesis. Genes Dev. 10:3051-3064[Abstract/Free Full Text].

35. Zhu, L., S. van den Heuvel, K. Helin, A. Fattaey, M. Ewen, D. Livingston, N. Dyson, and E. Harlow. 1993. Inhibition of cell proliferation by p107, a relative of the retinoblastoma protein. Genes Dev. 7:1111-1125[Abstract/Free Full Text].

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1.	Baskaran, R., G. Chiang, T. Mysliwiec, G. Krul, and J. Y. J. Wang. 1997. Tyrosine phosphorylation of RNA polymerase II carboxyl-terminal domain by Abl-related gene (Arg) encoded tyrosine kinase. J. Biol. Chem. 272:18905-18909[Abstract/Free Full Text].
2.	Baskaran, R., G. G. Chiang, and J. Y. J. Wang. 1996. Identification of a binding site in c-Abl tyrosine kinase for the C-terminal repeated domain of RNA polymerase II. Mol. Cell. Biol. 16:3361-3369[Abstract].
3.	Brehm, A., E. Miska, D. McCane, J. Reid, A. Bannister, and T. Kouzarides. 1998. Retinoblastoma protein recruits histone deacetylase to repress transcription. Nature 391:597-601[Medline].
4.	Duyster, J., R. Baskaran, and J. Y. J. Wang. 1995. Src homology 2 domain as a specificity determinant in the c-Abl mediated tyrosine phosphorylation of the RNA polymerase II carboxyl-terminal repeated domain. Proc. Natl. Acad. Sci. USA 92:1555-1559[Abstract/Free Full Text].
5.	Hiebert, S. W. 1993. Regions of the retinoblastoma gene product required for its interaction with the E2F transcription factor are necessary for E2 promoter repression and pRb-mediated growth suppression. Mol. Cell. Biol. 13:3384-3391[Abstract/Free Full Text].
6.	Hinds, P. W., S. Mittnacht, V. Dulic, A. Arnold, S. I. Reed, and R. A. Weinberg. 1992. Regulation of retinoblastoma protein functions by ectopic expression of human cyclins. Cell 70:993-1006[Medline].
7.	Hurford, R. K., D. Cobrinik, M.-H. Lee, and N. Dyson. 1997. pRB and p107/p130 are required for the regulated expression of different sets of E2F responsive genes. Genes Dev. 11:1447-1463[Abstract/Free Full Text].
8.	Janicke, R. U., P. A. Walker, X. Y. Lin, and A. G. Porter. 1996. Specific cleavage of the retinoblastoma protein by an ICE-like protease in apoptosis. EMBO J. 15:6969-6978[Medline].
9.	Knudsen, E. S., and J. Y. J. Wang. 1996. Differential regulation of retinoblastoma protein function by specific cdk phosphorylation sites. J. Biol. Chem. 271:8313-8320[Abstract/Free Full Text].
10.	Kratzke, R. A., G. A. Otterson, A. Hogg, A. B. Coxon, J. Geradts, J. K. Cowell, and F. J. Kaye. 1994. Partial inactivation of the RB product in a family with incomplete penetrance of familial retinoblastoma and benign retinal tumors. Oncogene 9:1321-1326[Medline].
11.	Lee, J.-O., A. Russo, and N. Pavletich. 1998. Structure of the retinoblastoma tumor suppressor pocket domain bound to a peptide from HPV E7. Nature 391:859-865[Medline].
12.	Lees, E., B. Faha, V. Dulic, S. I. Reed, and E. Harlow. 1992. Cyclin E/cdk2 and cyclin A/cdk2 kinases associate with p107 and E2F in a temporally distinct manner. Genes Dev. 6:1874-1885[Abstract/Free Full Text].
13.	Lohmann, D., B. Brandt, W. Hooping, E. Passarge, and B. Horsthemke. 1994. Distinct Rb1 gene mutations with low penetrance in hereditary retinoblastoma. Hum. Genet. 94:349-354[Medline].
14.	Luo, R., A. Postigo, and D. Dean. 1998. RB interacts with histone deacetylase to repress transcription. Cell 92:463-473[Medline].
15.	Magnaghi-Jaulin, L., R. Groisman, I. Naguibneva, P. Robin, S. Lorain, J. L. Villain, F. Troalen, D. Trouche, and A. Harel-Bellan. 1998. Retinoblastoma protein represses transcription by recruiting a histone deacetylase. Nature 391:601-605[Medline].
16.	Mudryj, M., S. H. Devoto, S. W. Hiebert, T. Hunter, J. Pines, and J. R. Nevins. 1991. Cell cycle regulation of the E2F transcription factor involves an interaction with cyclin A. Cell 65:1243-1253[Medline].
17.	Qin, X.-Q., T. Chittenden, D. M. Livingston, and W. G. Kaelin, Jr. 1992. Identification of a growth suppression domain within the retinoblastoma gene product. Genes Dev. 6:953-964[Abstract/Free Full Text].
18.	Scheffner, M., K. Munger, J. Byrne, and P. Howley. 1991. The state of the p53 and retinoblastoma genes in human cervical carcinoma cell lines. Proc. Natl. Acad. Sci. USA 88:5523-5527[Abstract/Free Full Text].
19.	Sellers, W., B. Novitch, S. Miyake, A. Heith, G. Otterson, F. Kaye, A. Lassar, and W. G. Kaelin, Jr. 1998. Stable binding to E2F is not required for the retinoblastoma protein to activate transcription, promote differentiation and suppress tumor cell growth. Genes Dev. 12:95-106[Abstract/Free Full Text].
20.	Sellers, W. R., and W. G. Kaelin, Jr. 1996. RB as a modulator of transcription. Biochim. Biophys. Acta 1288:1-5.
21.	Sellers, W. R., J. W. Rodgers, and W. G. Kaelin, Jr. 1995. A potent transrepression domain in the retinoblastoma protein induces a cell cycle arrest when bound to E2F sites. Proc. Natl. Acad. Sci. USA 92:11544-11548[Abstract/Free Full Text].
22.	Sherr, C. 1996. Cancer cell cycles. Science 274:1672-1677[Abstract/Free Full Text].
23.	Slanksy, J. E., and P. J. Farnham. 1996. Introduction to the E2F family: protein structure and gene regulation. Curr. Top. Microbiol. Immunol. 208:1-30[Medline].
23a.	Tan, X.-Q., H. Su, and J. Y. J. Wang. Unpublished data.
24.	Tan, X.-Q., and J. Y. J. Wang. 1998. The caspase-RB connection in cell death. Trends Cell Biol. 8:116-120. [Medline]
25.	Templeton, D. J., S. H. Park, L. Lanier, and R. A. Weinberg. 1991. Nonfunctional mutants of the retinoblastoma protein are characterized by defects in phosphorylation, viral oncoprotein association, and nuclear tethering. Proc. Natl. Acad. Sci. USA 88:3033-3037[Abstract/Free Full Text].
26.	Wang, J. Y. J. 1997. Retinoblastoma protein in growth suppression and death protection. Curr. Opin. Genet. Dev. 7:39-45[Medline].
27.	Wang, J. Y. J., E. S. Knudsen, and P. J. Welch. 1994. The retinoblastoma tumor suppressor protein. Adv. Cancer Res. 64:25-85[Medline].
28.	Weinberg, R. A. 1995. The retinoblastoma protein and cell cycle control. Cell 81:323-330[Medline].
29.	Weintraub, S. J., K. N. B. Chow, R. X. Luo, S. H. Zhang, S. He, and D. C. Dean. 1995. Mechanism of active transcriptional repression by the retinoblastoma protein. Nature 375:812-815[Medline].
30.	Welch, P. J., and J. Y. J. Wang. 1995. Abrogation of retinoblastoma protein function by c-Abl through tyrosine kinase-dependent and -independent mechanisms. Mol. Cell. Biol. 15:5542-5551[Abstract].
31.	Welch, P. J., and J. Y. J. Wang. 1993. A C-terminal protein-binding domain in the retinoblastoma protein regulates nuclear c-Abl tyrosine kinase in the cell cycle. Cell 75:779-790[Medline].
32.	Welch, P. J., and J. Y. J. Wang. 1995. Disruption of retinoblastoma protein function by coexpression of its C pocket fragment. Genes Dev. 9:31-46[Abstract/Free Full Text].
32a.	Welch, P. J., and J. Y. J. Wang. Unpublished data.
33.	Xiao, Z.-X., J. Chen, A. Levine, N. Modjtahedi, J. Xing, W. R. Sellers, and D. M. Livingston. 1995. Interaction between the retinoblastoma protein and the oncoprotein MDM2. Nature 375:694-698[Medline].
34.	Zacksenhaus, E., Z. Jiang, D. Chung, J. D. Marth, R. A. Phillips, and B. L. Gallie. 1996. pRb controls proliferation, differentiation, and death of skeletal muscle cells and other lineages during embryogenesis. Genes Dev. 10:3051-3064[Abstract/Free Full Text].
35.	Zhu, L., S. van den Heuvel, K. Helin, A. Fattaey, M. Ewen, D. Livingston, N. Dyson, and E. Harlow. 1993. Inhibition of cell proliferation by p107, a relative of the retinoblastoma protein. Genes Dev. 7:1111-1125[Abstract/Free Full Text].