Down-Regulation of {beta}-Catenin by Activated p53

doi:10.1128/MCB.21.20.6768-6781.2001

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Sadot, E.
	Articles by Ben-Ze'ev, A.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Sadot, E.
	Articles by Ben-Ze'ev, A.

Previous Article | Next Article

Molecular and Cellular Biology, October 2001, p. 6768-6781, Vol. 21, No. 20
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.20.6768-6781.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Down-Regulation of $beta$ -Catenin by Activated p53

Einat Sadot, Benjamin Geiger, Moshe Oren, and Avri Ben-Ze'ev^*

Department of Molecular Cell Biology, The Weizmann Institute of Science, Rehovot 76100, Israel

Received 6 February 2001/Returned for modification 5 April 2001/Accepted 9 July 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

$beta$ -Catenin is a cytoplasmic protein that participates in the assembly of cell-cell adherens junctions by binding cadherinsto the actin cytoskeleton. In addition, it is a key componentof the Wnt signaling pathway. Activation of this pathway triggersthe accumulation of $beta$ -catenin in the nucleus, where it activatesthe transcription of target genes. Abnormal accumulation of $beta$ -cateninis characteristic of various types of cancer and is caused bymutations either in the adenomatous polyposis coli protein, whichregulates $beta$ -catenin degradation, or in the $beta$ -catenin moleculeitself. Aberrant accumulation of $beta$ -catenin in tumors is oftenassociated with mutational inactivation of the p53 tumor suppressor.Here we show that overexpression of wild-type p53, by either transfectionor DNA damage, down-regulates $beta$ -catenin in human and mouse cells.This effect was not obtained with transcriptionally inactive p53,including a common tumor-associated p53 mutant. The reductionin $beta$ -catenin level was accompanied by inhibition of its transactivationpotential. The inhibitory effect of p53 on $beta$ -catenin is apparentlymediated by the ubiquitin-proteasome system and requires an activeglycogen synthase kinase 3 $beta$ (GSK3 $beta$ ). Mutations in the N terminusof $beta$ -catenin which compromise its degradation by the proteasomes,overexpression of dominant-negative $Delta$ F- $beta$ -TrCP, or inhibition ofGSK $beta$ activity all rendered $beta$ -catenin resistant to down-regulationby p53. These findings support the notion that there will be aselective pressure for the loss of wild-type p53 expression incancers that are driven by excessive accumulation of $beta$ -catenin.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

$beta$ -Catenin plays a dual role in cells as a major structural component of cell-cell adherens junctions and as a pivotal signalingmolecule in the Wnt pathway, transmitting transcriptional cuesinto the nucleus. In adherens junctions, $beta$ -catenin bridges betweencadherin and the actin cytoskeleton through an interaction with $alpha$ -catenin (2, 10). Either the nonjunctional pool of $beta$ -cateninis degraded by the ubiquitin-proteasome system or, under certainconditions, $beta$ -catenin enters the nucleus and, together with lymphoidenhancer factor/T-cell factor transcription factors (9, 34,56), activates transcription by providing the transactivationdomain to this heterodimeric complex (82). The targeting of $beta$ -catenin to the proteasome is achieved primarily through itsphosphorylation by a multimolecular complex consisting of glycogensynthase kinase 3 $beta$ (GSK3 $beta$ ), the adenomatous polyposis coli (APC)tumor suppressor protein, and axin (38). The phosphoserine motifin the N terminus of $beta$ -catenin (91) is recognized by $beta$ -TrCP,an F-box component of the E3 ubiquitin ligase complex SCF^TrCP (29, 41, 46, 71, 88). Activation of the Wnt/wg signalingpathway leads to inhibition of $beta$ -catenin degradation by decreasingthe ability of GSK3 $beta$ to phosphorylate $beta$ -catenin. This reducesits susceptibility to degradation by the ubiquitin-proteasomesystem, leading to its accumulation (93).

Studies in recent years have suggested that $beta$ -catenin is a potent oncogene product (64), and its accumulation has been implicatedin tumorigenesis in a wide variety of human cancers (65, 66,94). In colorectal cancer (CRC) the increase in $beta$ -catenin levelis attributed to mutations in APC, which occur in about 80% ofsuch tumors (55, 65). Accumulation of $beta$ -catenin can also betriggered by mutations in the $beta$ -catenin gene itself, affectingthe amino-terminal region of the protein that contains the GSK3 $beta$ phosphorylation sites (57, 70). Such mutations are frequentin colon cancers retaining a wild-type (wt) APC gene (66) andare also prevalent in melanoma, hepatocellular carcinoma (HCC),and a variety of other tumors (13, 16, 22-24, 36, 42, 43,54, 70, 83, 87, 89, 95).

The mechanism responsible for $beta$ -catenin-associated tumorigenesis is suggested to involve $beta$ -catenin- and LEF-1/TCF-activatedgenes, including genes that control the cell cycle (such as thosefor cyclin D1 [73, 80] and c-myc [32]), genes that are involvedin cell-extracellular matrix interactions (such as those for matrilysin[14], fibronectin [26], and WISP-1 [90]), and genes forvarious transcription factors, including Tcf-1 (68), c-jun andfra-1 (48), and PPAR $delta$ (31). The oncogenic role of $beta$ -cateninis also supported by studies showing that introduction of mutantAPC, or $beta$ -catenin, into transgenic mice results in enhanced tumorformation (25, 27, 63).

Another protein which is implicated in many types of cancer is p53. Mutations in the p53 gene are found in about 50% of humancancers (reviewed in references 45 and 61). Under normal conditions,p53 is most probably latent, owing to its rapid ubiquitinationand proteolytic degradation. Mdm2, an oncoprotein possessing E3ubiquitin ligase activity, plays a major role in this process(5, 61). A variety of conditions can lead to the rapid stabilizationand activation of p53. These include damage to DNA or to the mitoticspindle, ribonucleotide depletion, hypoxia, heat shock, and exposureto nitric oxide (4, 35, 45, 61). In addition, p53 isinduced by several oncogenic proteins, such as myc, ras, and adenovirusE1A, providing a direct link between oncogenic processes and thetumor suppressor action of p53 (reviewed in references 3, 35,45, and 61). The activation of p53 by these proteins reliesmainly on ARF, a tumor suppressor protein that binds to Mdm2 andsuppresses its p53 ubiquitination activity, thereby inhibitingp53 degradation (72). Activated p53 can affect the cell cycle,apoptosis, senescence, DNA repair, cell differentiation, and angiogenesis(35, 76), mostly via its function as a transcription factorthat activates a number of target genes and by its interactionwith a variety of proteins. Some of the better-studied p53 targetgenes are those for p21 (WAF1), which is mainly involved in G₁arrest; GADD45 and 14-3-3 $sigma$ , which contribute to G₂ arrest; andBAX, Fas (APO1), PIG3, and KILLER (DR5), which lead to caspaseactivation and apoptosis (12, 18).

A possible cross talk between p53 and $beta$ -catenin is suggested by the observation that cancers accumulating $beta$ -catenin (as aresult of APC mutations) also exhibit a high frequency of p53mutations, which was first illustrated by the analysis of humanCRC (40). Direct evidence for a cross talk between $beta$ -cateninand p53 was recently provided by studies demonstrating that excess $beta$ -catenin can induce an accumulation of active p53 (15). Thismay explain, at least in part, the selective pressure for lossof p53 activity in tumors harboring deregulated $beta$ -catenin, suchas CRC andHCC.

To elucidate why retention of functional p53 is disadvantageous to such tumors, we studied the effect of p53 on the leveland transcriptional activity of $beta$ -catenin. We report here thatelevated levels of wt p53 down-regulate $beta$ -catenin in a varietyof cell types. This down-regulation depends on the integrity andfunctionality of p53 and is not observed with a common tumor-associatedp53 mutant. Moreover, this effect of p53 is exerted on wt $beta$ -cateninbut not on the stable S33Y $beta$ -catenin mutant, and it is blockedby the proteasome inhibitor MG132, a dominant-negative componentof the E3 ubiquitin ligase complex $Delta$ F- $beta$ -TrCP, and by LiCl, whichinhibits GSK3 $beta$ activity. Furthermore, p53 can lead to a decreasein the level of the endogenous wt $beta$ -catenin in SW480 cells butnot in that of the $Delta$ S45 $beta$ -catenin mutant of HCT116 cells. Togetherwith the observations of Damalas et al. (15), our findings outlinea negative feedback control involving $beta$ -catenin and p53, whereexcess $beta$ -catenin induces the accumulation of p53, while high p53levels down-regulate $beta$ -catenin. Disruption of this feedback looplikely affects tumorigenesis driven by deregulated $beta$ -catenin activityand may therefore underlie the high frequency of p53 inactivationobserved in CRC, HCC, and probably other types ofcancer.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells and transfections. The HCT116 and SW480 human colon carcinoma cell lines, the human H1299 lung adenocarcinoma cell line, and the 293 adenovirus-transformedhuman embryo kidney cell line were cultured in Dulbecco's modifiedEagle's medium supplemented with 10% bovine calf serum (BCS).wt mouse embryonal fibroblasts (MEF), p53^/ MEF, and double-mutant p53^/ Mdm2^/ MEF (15) were cultured in Dulbecco's modified Eagle's mediumplus 10% BCS, 100 µM nonessential amino acid mixture (BiologicalIndustries Israel), and 50 µM $beta$ -mercaptoethanol. WI38 normal humanembryonic lung fibroblasts were cultured in minimum essentialmedium with 20% BCS. For transfections, cells were plated to forma 50 to 70% confluent culture in a 30-mm-diameter dish. The SW480and HCT116 cell lines were transfected using Lipofectamine (GIBCOBRL), while the 293 cells were transfected by the calcium phosphatemethod. The treatment with 30 mM LiCl in some experiments wasovernight, the treatment with 10 µM MG132 was for 4 h, and thetreatment with 5 µg of doxorubicin (DOX) per ml or 5 µg of cisplatinper ml was for periods ranging from 2 to 48h.

Plasmids. The following expression plasmids encoding various p53 constructs were employed: mouse wt p53 (20), mouse mutant p53 $Delta$ 13-52(30), hemagglutinin (HA)-tagged human p53 (HA-p53) (50), humanwt p53 (7), and the human R175H mutant p53 (7, 60). Thereporter plasmid containing the cyclin G promoter-luciferase (30),the LEF/TCF reporter plasmids TOPFLASH and FOPFLASH (82), the $Delta$ F- $beta$ -TrCP-expressing plasmid (71), and the vectors expressingvarious $beta$ -catenin forms (HA- $beta$ -catenin, HA-S33Y $beta$ -catenin, andvesicular stomatitis virus [VSV]- $beta$ -catenin) (73, 74, 93)were as describedpreviously.

Protein analysis. Protein levels were monitored by Western blotting. The following antibodies were used. Polyclonal anti- $beta$ -catenin and monoclonalantivinculin were from Sigma; monoclonal anti- $beta$ -catenin (clone14c19220) was from Transduction Laboratories. The 14c19220 antibodywas generated against amino acids 571 to 781 and recognizes thecaspase-cleaved 65-kDa product of $beta$ -catenin (11, 81). Monoclonalantibodies against p53 included anti-human p53 DO1 (84), PAb1801(8), anti-mouse p53 (which cross-reacts with human p53), andPAb421 (28). A polyclonal anti-p53 was kindly provided by VardaRotter, Weizmann Institute of Science). Monoclonal anti-HA clone12CA5 way from Boehringer Mannheim), and polyclonal anti-HA Y11sc-805 was from Santa Cruz Biotechnology. Fractionation of proteinsinto Triton X-100-soluble and -insoluble fractions was performedas previously described (71), and equal volumes of lysates fromthe two fractions were analyzed by Western blotting. Western blotswere developed using the ECL method (Amersham). Autoradiogramswere scanned with a GS-700 imaging densitometer (Bio-Rad Laboratories)using the FotoLook PS 2.07.2 software. The intensity of the bandswas quantitated using the NIH image 1.61software.

Luciferase assay For transactivation assays, 1 µg of luciferase reporter plasmid was cotransfected with 2 µg of the $beta$ -catenin construct and2 µg of the various p53 constructs, as indicated. A $beta$ -galactosidase-expressingvector was included as an internal control for transfection efficiency.After 24 h, the cells were lysed and both luciferase and $beta$ -galactosidaseactivities were determined with enzyme assay kits (Promega). Luminescencewas quantitated using a TD-20e luminometer (Turner Design) fromduplicate plates. The results represent data from at least fiveindependentexperiments.

Immunofluorescence microscopy Cells were cultured on glass coverslips, fixed with 3% paraformaldehyde in phosphate-buffered saline, and permeabilized with0.5% Triton X-100. The coverslips were incubated with the primaryantibodies as described above. The secondary antibodies were Alexa488-conjugated goat anti-mouse or anti-rabbit immunoglobulin G(Molecular Probes) and Cy3-conjugated goat anti-mouse or anti-rabbitimmunoglobulin G (Jackson ImmunoResearch Laboratories). Imageswere acquired using the DeltaVision system (Applied Precision)equipped with a Zeiss (Oberkochen, Germany) Axiovert 100 microscopeand a Photometrics (Tucson, Ariz.) 300 series scientific-gradecooled charge-coupled device camera (reading 12-bit images), usinga 100×, 1.3 numerical-aperture plan-Neofluar objective (Zeiss).For quantitative image processing, the Priism software was employed(37). At least 50 transfected and 50 nontransfected cells wereexamined in eachexperiment.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Excess p53 reduces $beta$ -catenin protein levels Since recent studies have shown that excess $beta$ -catenin can promote the accumulation of p53 (15), we examined the possibilitythat there is a reciprocal relationship between p53 and $beta$ -catenin.We have addressed this question by monitoring the level of endogenous $beta$ -catenin in cells in which p53 was induced by DNA damage. MEFfrom wt mice (p53^+/+) and from p53 knockout mice (p53^/) were treated for 24 h with 5 µg of DOX per ml, which effectivelyinduces p53 stabilization and accumulation (4). DOX treatmentelicited a strong nuclear p53 accumulation in the p53^+/+ MEF (Fig. 1C; compare to Fig. 1A). $beta$ -Catenin was present in thecytoplasm and adherens junctions in both p53^+/+ and p53^/ cells before DOX treatment (Fig. 1B and F), but following DOXtreatment, adherens junctions were disrupted in both cell types(Fig. 1D and H). However, while in p53^/ MEF the intensity of $beta$ -catenin staining remained unchanged andthe protein was strongly visible in the cytoplasm and at the edgesof the disrupted junctions (Fig. 1H), in p53^+/+ MEF $beta$ -catenin staining was significantly reduced in the majorityof cells (Fig. 1D). During the 24 h of DOX treatment, no morphologicalsigns of apoptosis were observed in these cells (Fig. 1C, D, G,and H and data not shown).To quantify the effect of p53 on $beta$ -cateninlevels, cell lysates isolated after 0, 2, 8, 16, and 24 h of DOXtreatment were immunoblotted with anti- $beta$ -catenin antibody. Todistinguish between free cytosolic and cytoskeletal or nuclear $beta$ -catenin, cells were fractionated into Triton X-100-soluble andTriton X-insoluble pools (Fig. 2A). In p53^+/+ MEF, p53 levels peaked at 16 h after DOX treatment and declinedat later times (Fig. 2A). This p53 was largely Triton insoluble,reflecting its nuclear accumulation. $beta$ -Catenin, in both the TritonX-100-soluble and -insoluble fractions, decreased considerablyafter 24 h of DOX treatment (Fig. 2A and A'), while no significantdecrease in the vinculin level was observed under these conditions(Fig. 2A and A'). In contrast, in p53^/ MEF neither $beta$ -catenin nor vinculin levels decreased followingDOX treatment (Fig. 2B and B'). When p53 expression was inducedby cisplatin treatment of p53^+/+ MEF (Fig. 2C), a comparable decrease in $beta$ -catenin was observed(Fig. 2C'). Cisplatin did not induce a detectable change in $beta$ -cateninlevels of p53^/ MEF (Fig. 2D and D'). The effect of p53 on $beta$ -catenin was alsoobserved in normal WI38 human embryonic lung fibroblasts (Fig.2E). p53 was strongly induced in these cells after DOX treatment,and its localization shifted from the Triton X-100-soluble tothe Triton-insoluble fraction, probably reflecting its translocationfrom the cytoplasm to the nucleus. In these cells, treatment withDOX for 48 h induced a fivefold reduction in the Triton X-100-soluble $beta$ -catenin (Fig. 2E'), while the Triton X-100-insoluble fractionwas only moderately affected (Fig. 2E and E'). In contrast, thelevels of vinculin in the Triton X-100-soluble fraction of thesecells did not change significantly (Fig. 2E and E'). Immunofluorescenceanalysis of WI38 cells treated with DOX for 24 or 48 h revealedintact nuclei and well-spread cells (data not shown), implyingthat the DOX treatment did not induce apoptosis in these cells.

View larger version (102K):
[in this window]
[in a new window]

FIG. 1. Effect of DOX-induced p53 expression on $beta$ -catenin organization and level. MEF cells were plated on coverslips, treated with 5 µg of DOX per ml for 24 h, fixed, and double stained for p53 using an anti-mouse p53 polyclonal antibody (A, C, E, and G) and for $beta$ -catenin ( $beta$ -cat) using a monoclonal anti- $beta$ -catenin antibody (B, D, F, and H). Bar, 10 µm.

View larger version (24K):
[in this window]
[in a new window]

FIG. 2. Effect of p53 elevation on $beta$ -catenin levels in the Triton X-100-soluble and -insoluble fractions of different cell types. Cells were treated with 5 µg of DOX per ml (A and B) or 5 µg of cisplatin per ml (C and D) for the indicated time periods. Proteins were fractionated into Triton X-100-soluble (lanes s) and -insoluble (lanes i) fractions, resolved by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, and subjected to Western blot analysis using the antibodies indicated in the legend to Fig. 1 and with an antivinculin (vin) antibody. The intensities of the bands from representative gels of MEF p53^+/+ (A and C) and MEF p53^/ (B and D) cells were quantified and plotted (A', C', B', and D', respectively). Extracts from WI38 cells (E and E') were blotted with the monoclonal anti- $beta$ -catenin antibody ( $beta$ -cat), vinculin (vin), and a mixture of the anti-human p53 antibodies DO1 and 1801 and analyzed as described for MEF cells. a.u., arbitrary units.

The ability of excess p53 to reduce $beta$ -catenin levels was also observed in 293 cells transfected with a p53 expression plasmid(Fig. 3). Transfection of p53 into these cells resulted in a majordecrease in the level of endogenous Triton X-100-soluble $beta$ -catenin(which is believed to represent the signaling pool of $beta$ -catenin)but not in that of vinculin (Fig. 3A). To determine whether p53can also affect the signaling activity of $beta$ -catenin, p53 and $beta$ -cateninwere cotransfected into 293 cells together with the LEF-1 reporterplasmid TOPFLASH (82) or with a variety of control plasmids.The transfected p53 was transcriptionally active as seen fromits ability to strongly activate the p53-responsive cyclin G promoter(Fig. 3B, bars 1 and 2). The cytomegalovirus promoter, a targetfor nonspecific repression by high levels of p53 (78), was repressedonly slightly under these conditions (Fig. 3B, bars 3 and 4),while p53 had no effect on the control FOPFLASH reporter plasmid(Fig. 3B, bars 6 and 8). In contrast, p53 very strongly suppressedthe $beta$ -catenin-mediated luciferase activity driven from the TOPFLASHreporter (Fig. 3B, bars 11 and 12). Analysis of protein levelsrevealed that in these cotransfected 293 cells, p53 caused a dramaticreduction in the steady-state $beta$ -catenin levels (Fig. 3C). In contrast,the levels of the closely related HA-plakoglobin protein (94),transduced with the same expression vector, were not affectedby p53 (Fig. 3C). This specific down-regulation of $beta$ -catenin islikely responsible for the inhibitory effect of p53 on $beta$ -catenin-dependenttranscriptional activity.

View larger version (31K):
[in this window]
[in a new window]

FIG. 3. Reciprocal effects of p53 and $beta$ -catenin overexpression on the levels of these proteins and the transcriptional activity of $beta$ -catenin. (A) p53 or a control empty vector was transfected into 293 cells. After 20 h, cells were fractionated into Triton X-100-soluble (lanes s) and -insoluble (lanes i) fractions and subjected to Western blot analysis. The positions of $beta$ -catenin ( $beta$ -cat), p53, and vinculin (vin) are marked. (B) Transactivation assays with reporter plasmids expressing luciferase under the transcriptional control of different promoters in the presence of p53 and $beta$ -catenin. Bars 1 and 2, cyclin G (CycG) promoter; bars 3 and 4, cytomegalovirus promoter; bars 5 to 8, FOPFLASH; bars 9 to 12, TOPFLASH. Cells were collected 20 h after transfection and subjected to luciferase and $beta$ -galactosidase assays. The standard error is indicated. (C) Effect of transfected p53 on the levels of cotransfected HA- $beta$ -catenin or HA-plakoglobin (PG) blotted with anti-HA antibody. The positions of $beta$ -catenin, plakoglobin, and p53 are indicated. (D) H1299 cells (which are p53 deficient) were transfected with increasing amounts of HA- $beta$ -catenin (0 to 4 µg) and a constant amount of p53 (100 ng) (lanes 1 to 3) or with a constant amount of HA- $beta$ -catenin (4 µg) and increasing amounts of p53 (0 to 600 ng) (lanes 4 to 7). The levels of HA- $beta$ -catenin ( $beta$ -cat) and p53 were determined by Western blot analysis. The endogenous vinculin served as loading control.

Reciprocal relationship between $beta$ -catenin and p53 expression. Since in a recent study we have shown that excess $beta$ -catenin can promote the accumulation of exogenously introduced p53 inH1299 cells (which lack p53) (15), we wished to examine, inthe same cellular system, the predicted reciprocal relationshipbetween $beta$ -catenin and p53 expression. The results shown in Fig.3D clearly demonstrate that when a constant level of p53 was cotransfectedinto H1299 cells with increasing levels of $beta$ -catenin, the increasein the expression of p53 was highest when high levels of $beta$ -cateninwere transfected (Fig. 3D, compare lanes 2 and 3). In contrast,when a constant high level of $beta$ -catenin was cotransfected withincreasing amounts of p53, a decrease in the level of $beta$ -cateninwas already apparent with the initial low level of p53 (Fig. 3D,lanes 4 and 5), and a dramatic reduction in $beta$ -catenin was seenwith the higher concentrations of p53 (Fig. 3D, lanes 4 to 7).Taken together, these results demonstrate the dose-dependent reciprocalrelationship between $beta$ -catenin and p53 expression in the samecells and that p53 can reduce the levels and transcriptional activityof $beta$ -catenin, irrespective of whether $beta$ -catenin is expressed fromthe endogenous gene or from an expressionplasmid.

p53 mutants fail to reduce $beta$ -catenin levels Next, we examined the ability of mutant forms of p53 to down-regulate $beta$ -catenin. Unlike wt p53, which strongly reduced thelevels and transcriptional activity of $beta$ -catenin in 293 cells,the mouse p53 deletion mutant p53 $Delta$ 13-52, which lacks transactivationand Mdm2 binding activities (the transactivation domain is onlypartially deleted but is apparently nonfunctional) (Fig. 4A),had no detectable effect on $beta$ -catenin level and transcriptionalactivity (Fig. 4B and C). Importantly, the cancer-associated hotspot human p53 mutant (p53R175H) (7, 60) was also unableto down-regulate $beta$ -catenin (Fig 4D). The presence of Mdm2 wasapparently not required for the p53-mediated reduction in $beta$ -cateninlevel, since in double-mutant MEF (deficient in both p53 and Mdm2),transfection of p53 was still capable of efficiently decreasing $beta$ -catenin expression (Fig. 4E). Hence, the integrity and functionalityof p53 are required for its ability to down-regulate $beta$ -cateninand are apparently independent of Mdm2.

View larger version (28K):
[in this window]
[in a new window]

FIG. 4. p53 mutants fail to reduce $beta$ -catenin ( $beta$ -cat) levels and transactivation capacity. (A) Schematic representation of the p53 $Delta$ 13-52 mutant. TAD, transactivation domain. (B) Transactivation in 293 cells, using the TOPFLASH reporter plasmid transfected either alone (bar 1) or with HA- $beta$ -catenin (bars 2 to 4) in the presence of wt mouse p53 (bar 3) or the mutant $Delta$ 13-52 mouse p53 (bar 4). Cells were harvested 20 h after transfection and subjected to luciferase activity assay. The standard error is indicated. (C) Western blot analysis for $beta$ -catenin, p53, and p53 $Delta$ 13-52 in cell lysates from the experiment in panel B. (D) Human wt p53 or a human p53R175H mutant was cotransfected with HA- $beta$ -catenin into 293 cells and subjected to Western blot analysis. (E) p53 can reduce the levels of $beta$ -catenin in Mdm2-deficient MEF. p53^/ Mdm2^/ double-mutant MEF were transfected with 5 µg of $beta$ -catenin plasmid in the presence or absence of 300 ng of p53 plasmid. The level of the transfected (HA-tagged) $beta$ -catenin was determined by Western blot analysis. The positions of $beta$ -catenin and p53 are indicated. The asterisks in panels C, D, and E represent a nonspecific band obtained with the anti-HA antibody.

Involvement of GSK3 $beta$ and the proteasome system in p53-mediated down-regulation of $beta$ -catenin. The targeting of $beta$ -catenin to the proteasome is achieved through its phosphorylation by GSK3 $beta$ in a multiprotein complex, followedby its recognition by $beta$ -TrCP, a component of the E3 ubiquitinligase system (29, 41, 46, 71, 88). To examine whetherthe reduction in $beta$ -catenin level by p53 requires the activityof GSK3 $beta$ , the effect of p53 on $beta$ -catenin in cells treated withLiCl, which inhibits the activity of GSK3 $beta$ (91), was determined.As shown in Fig. 5A, incubation with LiCl blocked the abilityof p53 to lower $beta$ -catenin levels (Fig. 5A, compare lanes 3 and4). The effect of p53 on cotransfected $beta$ -catenin was also blockedin the presence of the proteasome inhibitor MG132 (Fig. 5B, lanes3 and 4), implying that p53 promotes the degradation of $beta$ -cateninthrough the proteasome system. Furthermore, p53 did not reducethe level of the S33Y mutant $beta$ -catenin, which is relatively refractoryto phosphorylation by GSK3 $beta$ and hence to proteasomal degradation(21, 29, 46), in either the presence (Fig. 5B, lanes 7 and8) or in the absence (Fig. 5B, lanes 5 and 6) of MG132. When HA-taggedubiquitin was cotransfected with $beta$ -catenin in the presence orabsence of p53, an increase in ubiquitinated $beta$ -catenin was detectedin immunoprecipitates obtained from cells overexpressing p53 (datanot shown). Further support for the notion that p53 overexpressionstimulates $beta$ -catenin degradation via the classical Wnt pathwaywas obtained from cotransfection of 293 cells with $Delta$ F- $beta$ -TrCP,which binds to serine-phosphorylated $beta$ -catenin and blocks itsdegradation (71). As shown in Fig. 5C, expression of $Delta$ F- $beta$ -TrCPpartially blocked the p53-induced reduction in $beta$ -catenin levels.These results suggest that p53 can promote the turnover of $beta$ -cateninby augmenting its $beta$ -TrCP-mediated proteasomal degradation andthat typical oncogenic mutations of $beta$ -catenin (such as the S33Ymutation) can render it resistant to high levels of p53.

View larger version (26K):
[in this window]
[in a new window]

FIG. 5. Blocking of GSK3 $beta$ activity, polyubiquitination, and proteasomal degradation inhibit the effect of p53 on $beta$ -catenin ( $beta$ -cat). (A) wt HA- $beta$ -catenin was transfected into 293 cells with p53 (lanes 3 and 4) or without p53 (lanes 1 and 2), and half of the cultures were treated overnight with 30 mM LiCl (lanes 2 and 4) before harvesting of the cells and determination of the levels of HA- $beta$ -catenin and p53 by Western blot analysis. (B) wt $beta$ -catenin (lanes 1 to 4) or the HA-S33Y $beta$ -catenin mutant (lanes 5 to 8) was cotransfected with p53 into 293 cells. After 16 h, MG132 (25 µM) was added to the indicated samples (lanes 3, 4, 7, and 8). The cells were harvested 4 h later and subjected to Western blot analysis. The upper panel shows the levels of $beta$ -catenin (wt or S33Y mutant). The lower panel shows the transfected p53. (C) VSV-tagged $beta$ -catenin (1 µg) was transfected alone (lane 1) or cotransfected with p53 (1 µg) (lane 2) and increasing concentrations (2 µg [lane 3] and 4 µg [lane 4]) of the dominant-negative HA-tagged $Delta$ F- $beta$ -TrCP. The transfected wt $beta$ -catenin was detected by anti-VSV antibody, while $Delta$ F- $beta$ -TrCP expression was monitored with an anti-HA tag antibody. The asterisk indicates a nonspecific band obtained with the anti-HA antibody.

p53 can repress wt but not mutant $beta$ -catenin in colon cancer cell lines. The SW480 CRC cell line expresses a truncated APC that is deficient in its ability to promote $beta$ -catenin degradation (58).Nevertheless, these cells contain phosphorylated $beta$ -catenin thatcoprecipitates with the E3 ubiquitin ligase component $beta$ -TrCP (29),suggesting that the proteasomal degradation pathway responsiblefor $beta$ -catenin turnover is only partially attenuated in these cells.The endogenous p53 in SW480 cells has a mutation of Arg to Hisat position 273 and another mutation of Pro to Ser at position309 (1). Transfection of wt p53 into these cells led to a substantialdrop in nuclear $beta$ -catenin levels (Fig. 6A and B). Computerizedquantitation of the immunofluorescence images revealed about atwofold decrease in nuclear $beta$ -catenin levels (Fig. 6C) and a fourfoldreduction in $beta$ -catenin-mediated transactivation in these cells(Fig. 6D).

View larger version (46K):
[in this window]
[in a new window]

FIG. 6. wt p53 down-regulates $beta$ -catenin in SW480 CRC cells. (A and B) SW480 cells were transfected with HA-p53 (4 µg) and immunostained for HA (A) and $beta$ -catenin ( $beta$ -cat) (B) 20 h after transfection. The arrows point to the p53-transfected cells. (C) Computerized quantitation of nuclear $beta$ -catenin in control, nontransfected cells and in p53-transfected cells. (D) Transactivation in SW480 cells cotransfected with p53 and either TOPFLASH or FOPFLASH reporter plasmid. Cells were harvested 20 h after transfection and subjected to luciferase assay and Western blot analysis for the transfected HA-p53. The position of HA-p53 on the Western blot is indicated. Bar, 10 µm.

The effect of p53 on mutant $beta$ -catenin was also examined in the HCT116 CRC cell line. These cells express mutant $beta$ -cateninwith a deletion of serine 45 ( $Delta$ S45) and contain wt APC (57)and wt p53 (19). Treatment of HCT116 cells with DOX for 24 hled to the nuclear accumulation of p53 (Fig. 7A [compare to Fig.7C]), but no significant change in the $beta$ -catenin staining patternor disruption of adherens junctions was observed in these cells(Fig. 7B [compare to Fig. 7D]). The analysis of the Triton X-100-solubleand -insoluble fractions from these cells also failed to reveala significant change in $beta$ -catenin levels (Fig. 7E and F). Consistentwith these observations, transfection of p53 into HCT116 cellsalso had no effect on the levels of the endogenous mutant $beta$ -catenin(data not shown).

View larger version (84K):
[in this window]
[in a new window]

FIG. 7. p53 fails to affect the mutant $beta$ -catenin $Delta$ S45 of HCT116 CRC cells. (A to D) HCT116 cells were cultured on coverslips for 24 h in either the presence (A and B) or the absence (C and D) of 5 µg of DOX per ml. After fixation, the cells were double immunostained for p53 using a mixture of DO1 and 1801 antibodies (A and C) and for $beta$ -catenin ( $beta$ -cat) (B and D) using a polyclonal anti- $beta$ -catenin antibody. Bar, 10 µm. (E) HCT116 cells were treated with 5 µg of DOX per ml for the indicated times and fractionated into Triton X-100-soluble (lanes s) and -insoluble (lanes i) fractions. The lysates were subjected to Western blot analysis. The positions of $beta$ -catenin, p53, and vinculin (vin) (as a control) are indicated. (F) Quantitative analysis of the intensities of the bands shown in panel E. au, arbitrary units.

The presence of deregulated mutant $beta$ -catenin in HCT116 cells results in constitutive $beta$ -catenin-mediated transcriptional activity(Fig. 8A, lane 7). In contrast to the case in SW480 cells, excesswt p53 failed to inhibit the transcriptional activity of the endogenousmutant ( $Delta$ S45) $beta$ -catenin in HCT116 cells (Fig. 8A, lane 8 [compareto lane 7]). However, p53 repressed transactivation driven byexcess transfected wt $beta$ -catenin (Fig. 8A, lanes 9 and 10). Thisinhibition was accompanied by a reduction in the level of thetransfected wt $beta$ -catenin (Fig. 8A, lanes 9 and 10). In contrast,transfection of the more stable tumor-associated mutant $beta$ -cateninS33Y resulted in augmented transactivation that was resistantto wt p53 coexpression (Fig. 8A, lanes 11 and 12). We also examinedthe ability of the endogenous wt p53 in HCT116 cells to affect $beta$ -catenin-mediated transactivation by inducing p53 expressionwith DOX. The results demonstrate that increasing endogenous p53levels by this approach led to the inhibition of transactivationdriven by the transfected wt $beta$ -catenin (Fig. 8B, compare bars5 and 10 to bar 4) but not by the mutant endogenous $Delta$ S45 $beta$ -cateninor the transfected mutant $beta$ -catenin S33Y, which were resistantto elevated p53 (Fig, 8B, compare bars 4 to 10 and 6 to 12). Theseresults suggest that the cellular machinery necessary for theinhibitory effect of p53 on $beta$ -catenin is intact in HCT116 cellsand that the inability of wt p53 to down-regulate the endogenous $beta$ -catenin ( $Delta$ S45) or the transfected S33Y is due to the N-terminalmutations in the serine motifs that regulate $beta$ -catenin degradation.

View larger version (25K):
[in this window]
[in a new window]

FIG. 8. p53 does not inhibit transactivation by the $Delta$ S45 $beta$ -catenin of HCT116 cells and of transfected S33Y but inhibits the activity of wt $beta$ -catenin in these cells. (A) HCT116 cells were transfected with FOPFLASH (lanes 1 to 5) or TOPFLASH (lanes 7 to 12), together with p53 (lanes 2, 4, 6, 8, 10, and 12), HA- $beta$ -catenin (lanes 3, 4, 9, and 10), or p53 and HA-S33Y $beta$ -catenin (lanes 5, 6, 11, and 12). Luciferase activity was determined 20 h after transfection, and Western blot analyses of the cell lysates for the expression of $beta$ -catenin ( $beta$ -cat) (wt) and the mutant (S33Y) and for p53 were performed. (B) HCT116 cells were transfected with wt and S33Y $beta$ -catenin and either treated with DOX (to elevate p53 levels) as described for Fig. 7 (bars 7 to 12) or left untreated (bars 1 to 6). Transactivation driven by the FOPFLASH and TOPFLASH reporter plasmids was determined. The standard error is shown.

Taken together, the results imply that mutations within the GSK3 $beta$ phosphorylation domain of $beta$ -catenin that render it moreresistant to proteasomal degradation also make $beta$ -catenin moreresistant to down-regulation by activated p53. Importantly, such $beta$ -catenin mutations are prevalent in a variety of humancancers.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

This study demonstrated that high levels of functional p53 could down-regulate the amount and transcriptional activity of $beta$ -catenin. This effect was eliminated by blocking the activitiesof components that regulate the turnover of $beta$ -catenin, such asGSK3 $beta$ , a dominant-negative form of $beta$ -TrCP, and the proteasomalsystem. p53 therefore most probably exerted its effect by acceleratingthe degradation of $beta$ -catenin by the proteasome. While p53 coulddown-regulate wt $beta$ -catenin in the presence of wt or even mutantAPC, it failed to affect mutants of $beta$ -catenin that are resistantto the APC-GSK3 $beta$ -axin-mediated degradation. It is unlikely thatthe basal low levels of p53 in nonstressed cells are sufficientto cause $beta$ -catenin down-regulation. Rather, it is conceivablethat this inhibitory effect is exerted only by high levels ofactivated p53, as seen in cells exposed to extensive genotoxicstress (Fig. 2). Constitutive activity of $beta$ -catenin can exertboth proliferative and antiapoptotic effects (62). Hence, thedown-regulation of $beta$ -catenin by activated p53 is likely to contributeto the antiproliferative effects of p53 and possibly also facilitatesp53-mediated apoptosis. While in our experiments p53 activationwas attained by treatment of cultured cells with DNA-damagingagents, it is conceivable that a similar situation may pertainalso in emerging colorectal tumors with multiple genomic aberrations,which is typical of late stages in colorectalcarcinogenesis.

The exact molecular mechanism responsible for the down-regulation of $beta$ -catenin by p53 remains to be elucidated. So far, wehave been unable to demonstrate a direct protein-protein interactionbetween p53 and $beta$ -catenin (data not shown), suggesting that additionalproteins are likely to play a role in mediating $beta$ -catenin down-regulation.p53 is a transcription factor, which is capable of direct sequence-specifictranscription activation and indirect, albeit target gene selective,transcriptional repression. We have shown that p53 mutants deficientin transcriptional activity, owing either to deletion of the transactivationdomain (p53 $Delta$ 13-52) or to a more global conformational change affectingboth the DNA binding and the transactivation domains (p53R175H),failed to reduce $beta$ -catenin levels. These findings support theview that the down-modulation of $beta$ -catenin depends on the transcriptionalactivities of p53. For example, the decrease in $beta$ -catenin mightbe mediated by the action of the products of one or several p53target genes whose expression is induced in cells exposed to highlevels of activated p53. One interesting possibility is suggestedby studies showing that APC mRNA is induced by excess p53 in severalcell types (59). Such induction of APC expression by p53 maycontribute to enhanced $beta$ -catenin degradation in cells carryinga functional APC gene and may account for part of the observedreduction in $beta$ -catenin protein following p53 elevation. This observationcannot, however, explain the ability of p53 to reduce $beta$ -cateninexpression in SW480 CRC cells, which harbor a mutant APC geneand are devoid of functional APCprotein.

Another potential contributor to the inhibitory effect of p53 on $beta$ -catenin is the Dickkopf protein, whose gene has recentlybeen reported to be subject to transcriptional activation by p53(85). Dickkopf-1 blocks low-density lipoprotein (LDL) receptor-relatedprotein 6-mediated Wnt/ $beta$ -catenin signaling by directly interactingwith LDL receptor-related protein 6 (49). In addition to transactivation,transcriptional repression by p53 may also play a role in suppressing $beta$ -catenin. One potential mediator of such an effect may be presenilin1, whose expression is repressed by p53 (69). Since presenilin1 can stabilize $beta$ -catenin (92), its down-regulation by p53 mightlead to destabilization of $beta$ -catenin. It is conceivable that additionalp53-regulated genes may also play a role in the down-regulationof $beta$ -catenin, and p53 might turn on a coordinated transcriptionalprogram designed to inhibit $beta$ -catenin-mediatedsignaling.

While this paper was under revision, two studies were published suggesting that Siah-1, a transcriptional target of p53, candown-regulate $beta$ -catenin. Liu et al. (47) and Matsuzawa and Reed(51) reported that a p53-inducible gene product(Siah-1) canmediate the down-regulation of $beta$ -catenin by a novel degradationpathway mediated by SIP, Ebi, and the carboxy terminus of APC.This novel pathway may provide an additional means by which p53can inhibit the accumulation of $beta$ -catenin, especially of the oncogenic $beta$ -catenin mutants with mutations in the GSK phosphorylation sites,since this pathway operates independently of GSK3 $beta$ (47). Itis of note that whereas overexpression of Siah-1 in SW480 cellswas unable to inhibit $beta$ -catenin signaling (47), transfectionof p53 into these cells did cause a marked reduction in the levelof nuclear $beta$ -catenin and LEF-dependent transcription (Fig. 6).Taken together, these observations imply that p53 can block $beta$ -cateninsignaling through multiple downstream effectors, with Siah-1 beingjust one of those. Minimally, the data argue that there are atleast two major alternative pathways for p53-induced suppressionof $beta$ -catenin: a canonical cascade involving components of theWnt pathway and a second mechanism involving Siah-1, SIP, andEbi. Both pathways are probably turned on simultaneously whenp53 levels become sufficiently elevated, and they may synergizeto achieve a more effective response. This could be particularlyimportant when the target is an abundant protein such as $beta$ -catenin.The relative contribution of each of the two pathways to the eliminationof $beta$ -catenin signaling probably varies with cell type and cellcontext and may be modulated by additional genetic alterationsthat occur in the course of tumorigenesis. Furthermore, the existenceof multiple parallel pathways for down-regulating $beta$ -catenin byactivated p53 may provide a fail-safe mechanism in case one ofthe components along either of the pathways becomesinactivated.

Alternatively, p53 and $beta$ -catenin may compete for a common interacting molecule required for $beta$ -catenin stabilization. A possiblecandidate is the p300 (also called CBP) transcriptional coactivator,since both p53 and $beta$ -catenin can bind to p300 (6, 33, 79)and a recent study has shown that p53 and $beta$ -catenin compete forp300 binding (53). A similar competition for p300 binding betweenp53 and NF- $kappa$ B, resulting in the inhibition of the transcriptionalactivity of each of these proteins by an excess of the other,has been described (86). Our preliminary results indicate thatoverexpression of p300 can protect wt $beta$ -catenin from down-regulationby p53 (data not shown). It is thus tempting to speculate thatwhen p300 is present in limited amounts, increased p53 levelscan displace the endogenous $beta$ -catenin from its complex with p300and render it more susceptible to ubiquitination anddegradation.

A simple explanation that needs to be ruled out is that the reduction in $beta$ -catenin protein is merely a consequence of p53-mediatedapoptosis. Such a possibility may rely on previous observationsthat $beta$ -catenin is subject to cleavage by caspases, mainly caspases3, 6, and 8, in cells undergoing apoptosis (11, 81). We believethat this is an unlikely explanation for the effects of p53 on $beta$ -catenin for several reasons. First, no morphological changessuggestive of apoptosis were noted in any of the cell types usedin this study when the cells were harvested for biochemical andimmunohistochemical analysis (Fig. 1, 6, and 7 and data not shown).In addition, using the same antibody which was employed to demonstratecaspase-mediated $beta$ -catenin cleavage (11, 81), we did not detectcleaved forms of $beta$ -catenin in extracts of cells exposed to highp53 activity (Fig. 1A, C, and E and 7E and data not shown). Hence,we suggest that the effect of p53 on $beta$ -catenin most probably isexerted through the pathway responsible for the normal proteasomaldegradation of $beta$ -catenin.

A previous study has shown that excess deregulated $beta$ -catenin can lead to the induction of active p53 (15) and that thisis also achieved through changes in the rate of proteasomal degradationof the affected protein (p53). In the present study, we demonstratea reciprocal relationship between p53 and $beta$ -catenin in the samecell system by comparing the levels of the two proteins underconditions in which one protein was in excess over the other (Fig.3D). It is clear from these results that increasing levels of $beta$ -catenin augment the levels of p53 when a constant amount ofp53 is cotransduced into the same cells. On the other hand, whenhigh levels of $beta$ -catenin are transfected, elevation of p53 resultsin a specific, dose-dependent down-regulation of $beta$ -catenin expression(Fig. 3D). Taken together, these studies delineate an autoregulatoryloop in which excess $beta$ -catenin induces p53 activation, which inturn leads to down-regulation of $beta$ -catenin levels and activity.This control loop might serve as an effective means for curbingthe potential oncogenic effects of deregulated $beta$ -catenin. Itsdisruption may unleash the oncogenic activity of $beta$ -catenin, therebycontributing to tumor progression. The disruption of such autoregulationmay occur through mutations in the p53 gene that will render itunable to repress $beta$ -catenin activity or by inactivation of thetumor suppressor ARF, which stabilizes p53 (72). It is noteworthythat the ability to repress $beta$ -catenin is lost in the p53R175Hmutant, which is frequently seen in human CRC where $beta$ -cateninis deregulated through the loss of functional APC (39, 60).This loop may also be disrupted by mutations in $beta$ -catenin thatrender it resistant to the inhibitory effect of p53, as is thecase with the S33Y $beta$ -catenin mutant. In this regard, it is ofinterest that while p53 mutations predominate in the major classof CRC (involving $beta$ -catenin deregulation through APC gene inactivation),they are significantly less frequent in CRC carrying direct stabilizingmutations within $beta$ -catenin itself (17, 44, 52, 75, 77).Moreover, in a recent study employing N-myc transgenic mice, themajority of liver tumors arising on a p53^+/ background displayed either a $beta$ -catenin mutation or a loss ofthe remaining p53 allele (67). This further suggests that thesetwo mutational events often tend to be mutually exclusive duringtumorigenesis. Our findings offer an appealing explanation forthese observations by predicting that early mutations in $beta$ -cateninwill render it refractory to down-regulation by p53, thereby significantlyreducing the pressure for subsequent mutational inactivation ofp53. Conversely, the predominance of p53 mutations in the majorclass of CRC, which are associated with APC inactivation, suggeststhat the ability of wt p53 to restrain the deregulated wt $beta$ -cateninis a key component of its tumor suppressor function and a majorcause for the elimination of p53 function in suchtumors.

	ACKNOWLEDGMENTS

This study was supported by grants from the German-Israeli Foundation for Scientific Research and Development, the CooperationProgram in Cancer Research between the German Cancer ResearchCenter (DKFZ) and the Israeli Ministry of Science and Arts (IMOSA),CaP CURE, The Israel Science Foundation, The Crown Endowment Fundfor Immunological Research, The M. D. Moross Institute for CancerResearch, NIH (grant RO1 CA-40099), and the German-Israel ProjectCooperation (DIP). B.G. holds the E. Neter Chair of Cell and TumorBiology, and A.B.-Z. holds the Lunenfeld-Kunin Chair in Geneticsand CellBiology.

We thank G. Del Sal and J. Zhurinsky for illuminatingdiscussions.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Cell Biology, The Weizmann Institute of Science, Rehovot 76100,Israel. Phone: (972) 8-934 2422. Fax: (972) 8-946 5261. E-mail:avri.ben-zeev{at}weizmann.ac.il.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Abarzua, P., J. E. LoSardo, M. L. Gubler, and A. Neri. 1995. Microinjection of monoclonal antibody PAb421 into human SW480 colorectal carcinoma cells restores the transcription activation function to mutant p53. Cancer Res. 55:3490-3494[Abstract/Free Full Text].

2. Adams, C., and W. Nelson. 1998. Cytomechanics of cadherin-mediated cell-cell adhesion. Curr. Opin. Cell Biol. 10:572-577[CrossRef][Medline].

3. Albrechtsen, N., I. Dornreiter, F. Grosse, E. Kim, L. Wiesmuller, and W. Deppert. 1999. Maintenance of genomic integrity by p53: complementary roles for activated and non-activated p53. Oncogene 18:7706-7717[CrossRef][Medline].

4. Ashcroft, M., Y. Taya, and K. H. Vousden. 2000. Stress signals utilize multiple pathways to stabilize p53. Mol. Cell. Biol. 20:3224-3233[Abstract/Free Full Text].

5. Ashcroft, M., and K. H. Vousden. 1999. Regulation of p53 stability. Oncogene 18:7637-7643[CrossRef][Medline].

6. Avantaggiati, M. L., V. Ogryzko, K. Gardner, A. Giordano, A. S. Levine, and K. Kelly. 1997. Recruitment of p300/CBP in p53-dependent signal pathways. Cell 89:1175-1184[CrossRef][Medline].

7. Baker, S. J., E. R. Fearon, J. M. Nigro, S. R. Hamilton, A. C. Preisinger, J. M. Jessup, P. vanTuinen, D. H. Ledbetter, D. F. Barker, Y. Nakamura, R. White, and B. Vogelstein. 1989. Chromosome 17 deletions and p53 gene mutations in colorectal carcinomas. Science 244:217-221[Abstract/Free Full Text].

8. Banks, L., G. Matlashewski, and L. Crawford. 1986. Isolation of human-p53-specific monoclonal antibodies and their use in the studies of human p53 expression. Eur. J. Biochem. 159:529-534[Medline].

9. Behrens, J., J. von Kries, M. Kuhl, L. Bruhn, D. Wedlich, R. Grosschedl, and W. Birchmeier. 1996. Functional interaction of beta-catenin with the transcription factor LEF-1. Nature 382:638-642[CrossRef][Medline].

10. Ben-Ze'ev, A., and B. Geiger. 1998. Differential molecular interactions of beta-catenin and plakoglobin in adhesion, signaling and cancer. Curr. Opin. Cell Biol. 10:629-639[CrossRef][Medline].

11. Brancolini, C., D. Lazarevic, J. Rodriguez, and C. Schneider. 1997. Dismantling cell-cell contacts during apoptosis is coupled to a caspase-dependent proteolytic cleavage of beta-catenin. J. Cell. Biol. 139:759-771[Abstract/Free Full Text].

12. Burns, T. F., and W. S. El-Deiry. 1999. The p53 pathway and apoptosis. J. Cell. Physiol. 181:231-239[CrossRef][Medline].

13. Chan, E., U. Gat, J. McNiff, and E. Fuchs. 1999. A common human skin tumour is caused by activating mutations in beta-catenin. Nat. Genet. 21:410-413[CrossRef][Medline].

14. Crawford, H., B. Fingleton, L. Rudolph-Owen, K. Goss, B. Rubinfeld, P. Polakis, and L. Matrisian. 1999. The metalloproteinase matrilysin is a target of beta-catenin transactivation in intestinal tumors. Oncogene 18:2883-2891[CrossRef][Medline].

15. Damalas, A., A. Ben-Ze'ev, I. Simcha, M. Shtutman, J. Leal, J. Zhurinsky, B. Geiger, and M. Oren. 1999. Excess $beta$ -catenin promotes accumulation of transcriptionally active p53. EMBO J. 18:3054-3063[CrossRef][Medline].

16. de La Coste, A., B. Romagnolo, P. Billuart, C. A. Renard, M. A. Buendia, O. Soubrane, M. Fabre, J. Chelly, C. Beldjord, A. Kahn, and C. Perret. 1998. Somatic mutations of the beta-catenin gene are frequent in mouse and human hepatocellular carcinomas. Proc. Natl. Acad. Sci. USA 95:8847-8851[Abstract/Free Full Text].

17. Delattre, O., S. Olschwang, D. J. Law, T. Melot, Y. Remvikos, R. J. Salmon, X. Sastre, P. Validire, A. P. Feinberg, and G. Thomas. 1989. Multiple genetic alterations in distal and proximal colorectal cancer. Lancet 2:353-356[CrossRef][Medline].

18. el-Deiry, W. S. 1998. Regulation of p53 downstream genes. Semin. Cancer Biol. 8:345-357[CrossRef][Medline].

19. el-Deiry, W. S., J. W. Harper, P. M. O'Connor, V. E. Velculescu, C. E. Canman, J. Jackman, J. A. Pietenpol, M. Burrell, D. E. Hill, Y. Wang, et al. 1994. WAF1/CIP1 is induced in p53-mediated G1 arrest and apoptosis. Cancer Res. 54:1169-1174[Abstract/Free Full Text].

20. Eliyahu, D., D. Michalovitz, S. Eliyahu, O. Pinhasi-Kimhi, and M. Oren. 1989. Wild-type p53 can inhibit oncogene-mediated focus formation. Proc. Natl. Acad. Sci. USA 86:8763-8767[Abstract/Free Full Text].

21. Fuchs, S. Y., A. Chen, Y. Xiong, Z. Q. Pan, and Z. Ronai. 1999. HOS, a human homolog of Slimb, forms an SCF complex with Skp1 and Cullin1 and targets the phosphorylation-dependent degradation of IkappaB and beta-catenin. Oncogene 18:2039-2046[CrossRef][Medline].

22. Fukuchi, T., M. Sakamoto, H. Tsuda, K. Maruyama, S. Nozawa, and S. Hirohashi. 1998. Beta-catenin mutation in carcinoma of the uterine endometrium. Cancer Res. 58:3526-3528[Abstract/Free Full Text].

23. Gamallo, C., J. Palacios, G. Moreno, J. Calvo de Mora, A. Suarez, and A. Armas. 1999. Beta-catenin expression pattern in stage I and II ovarian carcinomas: relationship with beta-catenin gene mutations, clinicopathological features, and clinical outcome. Am. J. Pathol. 155:527-536[Abstract/Free Full Text].

24. Garcia-Rostan, G., G. Tallini, A. Herrero, T. G. D'Aquila, M. L. Carcangiu, and D. L. Rimm. 1999. Frequent mutation and nuclear localization of beta-catenin in anaplastic thyroid carcinoma. Cancer Res. 59:1811-1815[Abstract/Free Full Text].

25. Gat, U., R. DasGupta, L. Degenstein, and E. Fuchs. 1998. De novo hair follicle morphogenesis and hair tumors in mice expressing a truncated beta-catenin in skin. Cell 95:605-614[CrossRef][Medline].

26. Gradl, D., M. Kuhl, and D. Wedlich. 1999. The Wnt/Wg signal transducer beta-catenin controls fibronectin expression. Mol. Cell. Biol. 19:5576-5587[Abstract/Free Full Text].

27. Harada, N., Y. Tamai, T. Ishikawa, B. Sauer, K. Takaku, M. Oshima, and M. M. Taketo. 1999. Intestinal polyposis in mice with a dominant stable mutation of the beta-catenin gene. EMBO J. 18:5931-5942[CrossRef][Medline].

28. Harlow, E. D., L. V. Crawford, D. C. Pim, and N. M. Williamson. 1981. Monoclonal antibodies specific for simian virus 40 tumor antigens. J. Virol. 39:861-869[Abstract/Free Full Text].

29. Hart, M., J. Concordet, I. Lassot, I. Albert, R. del los Santos, H. Durand, C. Perret, B. Rubinfeld, F. Margottin, R. Benarous, and P. Polakis. 1999. The F-box protein beta-TrCP associates with phosphorylated beta-catenin and regulates its activity in the cell. Curr. Biol. 9:207-210[CrossRef][Medline].

30. Haupt, Y., Y. Barak, and M. Oren. 1996. Cell type-specific inhibition of p53-mediated apoptosis by mdm2. EMBO J. 15:1596-1606[Medline].

31. He, T., T. Chan, B. Vogelstein, and K. Kinzler. 1999. PPARdelta is an APC-regulated target of nonsteroidal anti-inflammatory drugs. Cell 99:335-345[CrossRef][Medline].

32. He, T., A. Sparks, C. Rago, H. Hermeking, L. Zawel, L. da Costa, P. Morin, B. Vogelstein, and K. Kinzler. 1998. Identification of c-MYC as a target of the APC pathway. Science 281:1509-1512[Abstract/Free Full Text].

33. Hecht, A., K. Vleminckx, M. Stemmler, F. van Roy, and R. Kemler. 2000. The p300/CBP acetyltransferases function as transcriptional coactivators of beta-catenin in vertebrate

1.	Abarzua, P., J. E. LoSardo, M. L. Gubler, and A. Neri. 1995. Microinjection of monoclonal antibody PAb421 into human SW480 colorectal carcinoma cells restores the transcription activation function to mutant p53. Cancer Res. 55:3490-3494[Abstract/Free Full Text].
2.	Adams, C., and W. Nelson. 1998. Cytomechanics of cadherin-mediated cell-cell adhesion. Curr. Opin. Cell Biol. 10:572-577[CrossRef][Medline].
3.	Albrechtsen, N., I. Dornreiter, F. Grosse, E. Kim, L. Wiesmuller, and W. Deppert. 1999. Maintenance of genomic integrity by p53: complementary roles for activated and non-activated p53. Oncogene 18:7706-7717[CrossRef][Medline].
4.	Ashcroft, M., Y. Taya, and K. H. Vousden. 2000. Stress signals utilize multiple pathways to stabilize p53. Mol. Cell. Biol. 20:3224-3233[Abstract/Free Full Text].
5.	Ashcroft, M., and K. H. Vousden. 1999. Regulation of p53 stability. Oncogene 18:7637-7643[CrossRef][Medline].
6.	Avantaggiati, M. L., V. Ogryzko, K. Gardner, A. Giordano, A. S. Levine, and K. Kelly. 1997. Recruitment of p300/CBP in p53-dependent signal pathways. Cell 89:1175-1184[CrossRef][Medline].
7.	Baker, S. J., E. R. Fearon, J. M. Nigro, S. R. Hamilton, A. C. Preisinger, J. M. Jessup, P. vanTuinen, D. H. Ledbetter, D. F. Barker, Y. Nakamura, R. White, and B. Vogelstein. 1989. Chromosome 17 deletions and p53 gene mutations in colorectal carcinomas. Science 244:217-221[Abstract/Free Full Text].
8.	Banks, L., G. Matlashewski, and L. Crawford. 1986. Isolation of human-p53-specific monoclonal antibodies and their use in the studies of human p53 expression. Eur. J. Biochem. 159:529-534[Medline].
9.	Behrens, J., J. von Kries, M. Kuhl, L. Bruhn, D. Wedlich, R. Grosschedl, and W. Birchmeier. 1996. Functional interaction of beta-catenin with the transcription factor LEF-1. Nature 382:638-642[CrossRef][Medline].
10.	Ben-Ze'ev, A., and B. Geiger. 1998. Differential molecular interactions of beta-catenin and plakoglobin in adhesion, signaling and cancer. Curr. Opin. Cell Biol. 10:629-639[CrossRef][Medline].
11.	Brancolini, C., D. Lazarevic, J. Rodriguez, and C. Schneider. 1997. Dismantling cell-cell contacts during apoptosis is coupled to a caspase-dependent proteolytic cleavage of beta-catenin. J. Cell. Biol. 139:759-771[Abstract/Free Full Text].
12.	Burns, T. F., and W. S. El-Deiry. 1999. The p53 pathway and apoptosis. J. Cell. Physiol. 181:231-239[CrossRef][Medline].
13.	Chan, E., U. Gat, J. McNiff, and E. Fuchs. 1999. A common human skin tumour is caused by activating mutations in beta-catenin. Nat. Genet. 21:410-413[CrossRef][Medline].
14.	Crawford, H., B. Fingleton, L. Rudolph-Owen, K. Goss, B. Rubinfeld, P. Polakis, and L. Matrisian. 1999. The metalloproteinase matrilysin is a target of beta-catenin transactivation in intestinal tumors. Oncogene 18:2883-2891[CrossRef][Medline].
15.	Damalas, A., A. Ben-Ze'ev, I. Simcha, M. Shtutman, J. Leal, J. Zhurinsky, B. Geiger, and M. Oren. 1999. Excess $beta$ -catenin promotes accumulation of transcriptionally active p53. EMBO J. 18:3054-3063[CrossRef][Medline].
16.	de La Coste, A., B. Romagnolo, P. Billuart, C. A. Renard, M. A. Buendia, O. Soubrane, M. Fabre, J. Chelly, C. Beldjord, A. Kahn, and C. Perret. 1998. Somatic mutations of the beta-catenin gene are frequent in mouse and human hepatocellular carcinomas. Proc. Natl. Acad. Sci. USA 95:8847-8851[Abstract/Free Full Text].
17.	Delattre, O., S. Olschwang, D. J. Law, T. Melot, Y. Remvikos, R. J. Salmon, X. Sastre, P. Validire, A. P. Feinberg, and G. Thomas. 1989. Multiple genetic alterations in distal and proximal colorectal cancer. Lancet 2:353-356[CrossRef][Medline].
18.	el-Deiry, W. S. 1998. Regulation of p53 downstream genes. Semin. Cancer Biol. 8:345-357[CrossRef][Medline].
19.	el-Deiry, W. S., J. W. Harper, P. M. O'Connor, V. E. Velculescu, C. E. Canman, J. Jackman, J. A. Pietenpol, M. Burrell, D. E. Hill, Y. Wang, et al. 1994. WAF1/CIP1 is induced in p53-mediated G1 arrest and apoptosis. Cancer Res. 54:1169-1174[Abstract/Free Full Text].
20.	Eliyahu, D., D. Michalovitz, S. Eliyahu, O. Pinhasi-Kimhi, and M. Oren. 1989. Wild-type p53 can inhibit oncogene-mediated focus formation. Proc. Natl. Acad. Sci. USA 86:8763-8767[Abstract/Free Full Text].
21.	Fuchs, S. Y., A. Chen, Y. Xiong, Z. Q. Pan, and Z. Ronai. 1999. HOS, a human homolog of Slimb, forms an SCF complex with Skp1 and Cullin1 and targets the phosphorylation-dependent degradation of IkappaB and beta-catenin. Oncogene 18:2039-2046[CrossRef][Medline].
22.	Fukuchi, T., M. Sakamoto, H. Tsuda, K. Maruyama, S. Nozawa, and S. Hirohashi. 1998. Beta-catenin mutation in carcinoma of the uterine endometrium. Cancer Res. 58:3526-3528[Abstract/Free Full Text].
23.	Gamallo, C., J. Palacios, G. Moreno, J. Calvo de Mora, A. Suarez, and A. Armas. 1999. Beta-catenin expression pattern in stage I and II ovarian carcinomas: relationship with beta-catenin gene mutations, clinicopathological features, and clinical outcome. Am. J. Pathol. 155:527-536[Abstract/Free Full Text].
24.	Garcia-Rostan, G., G. Tallini, A. Herrero, T. G. D'Aquila, M. L. Carcangiu, and D. L. Rimm. 1999. Frequent mutation and nuclear localization of beta-catenin in anaplastic thyroid carcinoma. Cancer Res. 59:1811-1815[Abstract/Free Full Text].
25.	Gat, U., R. DasGupta, L. Degenstein, and E. Fuchs. 1998. De novo hair follicle morphogenesis and hair tumors in mice expressing a truncated beta-catenin in skin. Cell 95:605-614[CrossRef][Medline].
26.	Gradl, D., M. Kuhl, and D. Wedlich. 1999. The Wnt/Wg signal transducer beta-catenin controls fibronectin expression. Mol. Cell. Biol. 19:5576-5587[Abstract/Free Full Text].
27.	Harada, N., Y. Tamai, T. Ishikawa, B. Sauer, K. Takaku, M. Oshima, and M. M. Taketo. 1999. Intestinal polyposis in mice with a dominant stable mutation of the beta-catenin gene. EMBO J. 18:5931-5942[CrossRef][Medline].
28.	Harlow, E. D., L. V. Crawford, D. C. Pim, and N. M. Williamson. 1981. Monoclonal antibodies specific for simian virus 40 tumor antigens. J. Virol. 39:861-869[Abstract/Free Full Text].
29.	Hart, M., J. Concordet, I. Lassot, I. Albert, R. del los Santos, H. Durand, C. Perret, B. Rubinfeld, F. Margottin, R. Benarous, and P. Polakis. 1999. The F-box protein beta-TrCP associates with phosphorylated beta-catenin and regulates its activity in the cell. Curr. Biol. 9:207-210[CrossRef][Medline].
30.	Haupt, Y., Y. Barak, and M. Oren. 1996. Cell type-specific inhibition of p53-mediated apoptosis by mdm2. EMBO J. 15:1596-1606[Medline].
31.	He, T., T. Chan, B. Vogelstein, and K. Kinzler. 1999. PPARdelta is an APC-regulated target of nonsteroidal anti-inflammatory drugs. Cell 99:335-345[CrossRef][Medline].
32.	He, T., A. Sparks, C. Rago, H. Hermeking, L. Zawel, L. da Costa, P. Morin, B. Vogelstein, and K. Kinzler. 1998. Identification of c-MYC as a target of the APC pathway. Science 281:1509-1512[Abstract/Free Full Text].
33.	Hecht, A., K. Vleminckx, M. Stemmler, F. van Roy, and R. Kemler. 2000. The p300/CBP acetyltransferases function as transcriptional coactivators of beta-catenin in vertebrate

Down-Regulation of -Catenin by Activated p53

Down-Regulation of $beta$ -Catenin by Activated p53