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From the
Received for publication, July 27, 2001, and in revised form, November 15, 2001
Genetic alteration of the p53 tumor suppressor
gene, which monitors DNA damage and operates cell cycle checkpoints, is
a major factor in the development of human malignancies. The p53
protein belongs to a family that also includes two structurally related proteins, p63 and p73. Although all three proteins share similar transcriptional functions and antiproliferative effects, each of them
appears to play a distinct role in development and tumor suppression.
One of the principal regulators of p53 activity is the MDM2 protein.
The interaction of MDM2 with p53 inhibits p53 transcriptional activity
and targets p53 for ubiquitin-dependent degradation. The
ability of MDM2 to inhibit p53 functions is antagonized by the ARF
oncosuppressor protein. We show here that like p53, the p63 The p63 gene, which maps on the 3q27-28 region, is one of the
members of the p53 gene family. Unlike p53, it shows a complex pattern
of expression due to alternative splicing and promoter usage that
results in multiple isoforms with different biological activities (1,
2). Initiation of transcription in exon 1 produces the TA isotypes,
containing the evolutionarily conserved transactivation, DNA-binding,
and oligomerization domains, whereas initiation in exon 3' gives rise
to the In contrast with the ubiquitous expression of p53, p63 exhibits a
rather tissue-specific distribution in that it is most detectable in
the basal layer of stratified epithelia, including the epidermis, where
the All three members of the p53 family share similar transcriptional
functions, as p63 and p73 can also activate many of the p53 target
genes, although with varying efficiency (5). Moreover, like p73, p63 is
able to induce apoptosis and growth suppression in a manner similar to
p53 (4).
Molecular alterations of p63 or p73 in human cancers appear to be rare;
unlike p53-deficient mice, those lacking p73 or p63 show no increased
susceptibility to spontaneous tumorigenesis (6, 7). Viral oncoproteins
such as SV40 large T antigen, adenovirus E1B, and human
papilloma virus E6, which bind and inactivate p53, do not target p73
and p63 (2, 8). Thus, it seems likely that p63 and p73 are not potent
suppressors of abnormal proliferation.
Unlike p53, both p73 (6) and p63 appear to contribute to normal
development. This is most dramatically illustrated by reports showing
that p63-deficient mice have severe defects in limb and skin
development (9). Moreover, heterozygous germ-line mutations in the p63
gene are the cause of ectrodactyly-ectodermal dysplasia-clefting (10) and ankyloblepharon-ectodermal dysplasia-clefting (11) syndromes in humans.
p53 is normally a short-lived protein. Regulation of the p53 protein
occurs to a large extent through control of protein stability, and the
MDM2 (murine double minute
2) protein has been shown to play a key role in targeting
p53 for degradation (2). The ARF (alternative
reading frame) protein, one of the alternative
products of the INK4a locus, binds to the MDM2
protein, preventing MDM2-dependent p53 degradation and
transcriptional silencing (12). Concerning the other members of the p53
family, it has recently been demonstrated that p73 also binds MDM2.
MDM2 inhibits p73-dependent transcription by masking the
p73 transactivation domain and/or disrupting the interaction of p73
with p300/CBP (cAMP-responsive element-binding protein-binding protein), but it is clearly not
involved in the degradation of p73 (13). Here, we have investigated
whether HDM2 (human homolog of murine double
minute 2) and ARF are involved in the control
of p63 functions. We have found that p63 is able to physically interact
with HDM2. Overexpression of HDM2 increased the steady-state level of
intracellular p63 and enhanced its transcriptional activity. Both
effects were counteracted by ARF coexpression. Because of its opposite
effects on p53 and p63 protein stability and transcriptional activity,
MDM2 expression could support p63-specific transcriptional functions on
a common set of genes, at the same time reducing interference by p53.
Plasmids--
The p63 Cell Culture and Transfection--
Saos2, C33A, and COS-7 cell
lines were maintained in Dulbecco's modified Eagle's medium
supplemented with 10% fetal calf serum. For CAT assays, C33A cells
(1 × 105) were seeded in 100-mm diameter dishes and
transiently transfected (16 h later) using the calcium phosphate
precipitation method. Equal amounts of expression plasmids for p53,
p63
Saos2 cells (2.5 × 105) were seeded into six-well
multiplates and transfected using LipofectAMINE 2000 (Invitrogen) under the conditions suggested by the manufacturer.
At 48 h after transfection, equal quantities of proteins
(determined by the Bradford method) were assayed for CAT activity. The
amounts of MDM2 and ARF expression plasmids used in the transactivation
experiments are indicated in the legends.
GST Fusion Protein Association Assay--
The GST-HDM2 fusion
protein cloned into bacterial pGEX4T3 was expressed in
Escherichia coli under the inducible lac promoter and purified on a glutathione-Sepharose 12B column. Protein-protein association assay was conducted as follows. 20 µl of in
vitro translated, 35S-labeled p63 Co-immunoprecipitation--
Saos2 cells (three 60-mm dishes)
were transfected with 2 µg of parental pcDNA3-His, p63 Analysis of Protein Levels and Half-life
Determination--
Saos2 and COS-7 cells (2.5 × 105
in six-well plates) were transfected using the LipofectAMINE 2000 reagent. The pEGFP-C1 expression vector was included in these
experiments as a control of transfection efficiency. At 48 h
post-transfection, the cells were harvested by scraping in 100 µl of
immunoprecipitation buffer containing 0.5% deoxycholate and lysed by
sonication. Expression levels of both the transfected p63 and ARF
proteins were determined by Western blotting using the anti-Xpress
antibodies. The identity of the p63 bands was confirmed using anti-p63
antibodies (N-18, Santa Cruz Biotechnology). The p21WAF protein
was revealed using mouse anti-human p21 antibody 6B6 (Pierce). Human
MDM2 (HDM2) was detected with antibody smp14. The p53 protein was
detected with the anti-Xpress antibodies or monoclonal mouse anti-human
p53 antibody Pab240 (Pierce) as indicated. Bands were visualized with
an enhanced chemiluminescence system (Pierce). To compare the stability
of p63 Comparison of Transcriptional Properties of p63
C33A (p53
Although the ARF promoter does not contain p53-binding
elements, it is trans-repressed by p53 (18),2
suggesting the existence of an autoregulatory feedback loop limiting the effect of ARF on p53 stabilization. Based on the functional similarity between p53 and p63, we tested whether or not p63 was also
able to inhibit transcription driven by the human ARF
promoter. C33A cells were cotransfected with the ARF-CAT
reporter plasmid and the p53, p63
To investigate whether the differences observed in the transcriptional
properties of p63 HDM2 Enhances the Transcriptional Activity of p63--
Because
MDM2 inhibited both p53 and p73 transcriptional activity, we wanted to
determine whether it also affected p63-driven transcription. To
investigate this point, we cotransfected Saos2 cells with the BP100-CAT
reporter plasmid, p63 In Vitro and in Vivo Association of p63 with HDM2--
The
interaction between MDM2 and p53 inhibits the p53 transactivation
ability and targets p53 for ubiquitin-dependent
degradation. Taking into account the effect of HDM2 on p63
transactivation ability, we decided to assess the effect of HDM2
expression on the level of the p63 protein. First, we wanted to test
whether p63 may physically interact with HDM2. Extensive mutational
analyses of the HDM2-binding domain of p53 (FSDLW) have identified
Phe19, Leu22, and Trp23 as the
critical residues for transcriptional activation and p53 binding by
MDM2. We observed that these amino acid residues, except for a
conservative Leu22-to-Ile substitution, are present in the
p63 MDM2-binding domain (FQHIW). The p63
To confirm the interaction between p63 and HDM2 in intact cells, we
cotransfected Saos2 cells with p63 HDM2 Increases p63 Protein Levels--
Binding of MDM2 to p53 is
required for targeting p53 for degradation (21); p73, however, binds to
MDM2, but is refractory to MDM2-mediated degradation (13), indicating
that binding to MDM2 is necessary but not sufficient for degradation.
Recent findings indicate that a proline-rich sequence (from amino acid
92 to 112) of p53 is a degradation signal (19). This degradation signal is not present in the p73 and p63 proteins. To elucidate the effect of
HDM2 on p63 protein levels, we transiently transfected COS-7 cells with
equal amounts of p53 (Fig. 5A)
and p63
To determine whether the elevation in the p63 ARF Abolishes p63 Stabilization and Transcriptional Activation
Induced by HDM2--
Among the growing number of proteins that
interact with MDM2, particular interest has recently been focused on
ARF, which is encoded by the INK4a locus. Because ARF binds
to the MDM2 protein, preventing MDM2-dependent p53
degradation and transcriptional silencing (12, 22), we predicted that
ARF could counteract the effect of MDM2 on p63. To test this
hypothesis, we cotransfected, in Saos2 cells, the BP100-CAT
(Fig. 7A) or
WAF-CAT (data not shown) reporter with a fixed amount of
HDM2 and increasing amounts of ARF. We used a molar ratio (4:1) of HDM2
to p63 Although there exists extensive information on the relationship
between MDM2 and p53, far less is known about a possible functional interaction of MDM2 with p63. In this study, we report that MDM2 overexpression causes an increase in overall p63 protein levels due, at
least in part, to a reduced rate of p63 protein degradation. Moreover,
although MDM2 represses p53 transcriptional activity, enforced MDM2
expression causes instead a considerable enhancement of p63-mediated
transcription, which can be ascribed to the increase in
transcriptionally active p63 protein.
While this paper was in preparation, several studies were published
reporting conflicting results on the functional relationship between
p63 and the MDM2 protein. For instance, it was reported that
exogenously expressed MDM2 represses p63-mediated transcription (23).
On the other hand, it was proposed that MDM2 is unable to affect its
half-life or its transcriptional function (24), in conflict with the
present and above-mentioned papers. It is well documented that
transiently transfected p63 is able to strongly induce the endogenous
MDM2 protein (25), and we repeatedly observed that only at a low level
of p63 exogenous expression is the induction of endogenous MDM2
negligible, so that the stabilization effect by transfected MDM2
becomes apparent. However, compared with our results, both Kadakia
et al. (23) and Little and Jochemsen (24) obtained remarkably higher levels of p63 Moreover, we also demonstrate that p63 proteins are able to form a
complex with HDM2 both in vitro and in mammalian cells, suggesting that the mechanism through which HDM2 regulates p63 expression requires a physical interaction between these proteins. Because it is well established that ARF stabilizes p53 by binding and
sequestering MDM2, we expected ARF to exert an inhibitory effect on p63
protein stabilization. In fact, ARF coexpression abolishes both
MDM2-induced p63 protein stabilization and transcriptional activation,
giving further evidence that p63-MDM2 interaction has a functional role.
A recent analysis of the molecular interactions of p63 in a yeast
two-hybrid system (26) suggested that p63 does not associate with MDM2
family proteins. However, this analysis was performed using only the
N-terminal portion of the p63 protein (amino acids 1-111), so it
cannot be excluded that other regions of the protein are essential for
the p63-MDM2 interaction or that some tertiary structure formed by a
more extended region may also be required for the binding. On the other
hand, Little and Jochemsen (24) detected a weak interaction by
an in vitro assay, but this could not be confirmed by
co-immunoprecipitation in mammalian cells. Because we observed that
MDM2 displays a lower affinity for p63 than it does for p53, it is
possible that the use of less efficient antibodies or more stringent
washing conditions could have hampered the analysis of the
protein-protein interaction by immunoprecipitation. Remarkably, MDM2
has been reported to facilitate p63 export from the nucleus (23), but
whether a direct MDM2 association with p63 is required for this
activity remains to be elucidated.
Until recently, a similarly controversial question has been how MDM2
regulates the stability and transcriptional activity of the third
member of the p53 family, the p73 protein (27, 28). Now a clear picture
is emerging: MDM2 interacts with p73, stabilizing and enhancing its
growth-suppressive function (29). Moreover, in sharp contrast to p53,
MDM2 induces p73 to form nuclear aggregates that colocalize with MDM2
(30). Furthermore, p73 levels are increased in MDM2-expressing cells
(30). Both p63 and p73 therefore bind to MDM2, but are refractory to
MDM2-mediated degradation, indicating that binding is necessary but not
sufficient for degradation. These results are not surprising given
that, although the N-terminal MDM2-binding motif of p53 is conserved in
both p63 and p73 (31), p53 has a unique sequence element (amino acids
92-112) that functions as a signal for MDM2-mediated degradation
(19). How this sequence of p53 functions as a degradation signal
remains to be defined.
Although we have not determined the precise mechanism by which MDM2
increases p63 protein levels, our data argue that, like the proteasome
inhibitor ALLN, MDM2 may act by preventing p63 proteasome-dependent degradation. In addition to MDM2, the
p300/CBP protein has also been shown to play a role in allowing
efficient p53 degradation. Surprisingly, loss of p300 activity results
in an inability to stabilize p53 in response to DNA damage, indicating that there is a complex relationship between p300 and p53 stability (32). It has been proposed that the reason why p73 is refractory to
MDM2 degradation might be related to the observation that, unlike p53,
p73 is unable to bind both MDM2 and p300 simultaneously (13). A similar
mechanism could also explain the p63 resistance to MDM2 degradation. We
are currently investigating the relationship between p63 and the
p300/CBP coactivator as well as the exact pathway through which MDM2
induces an increase in p63 intracellular levels.
In conclusion, MDM2 seems to regulate p53 and its homologs through
completely opposite mechanisms, suggesting that both p73 and p63 could
be involved in specific cellular defense mechanisms against the
deregulated expression of MDM2. We can also speculate that, in cells
expressing both p63 and p53 proteins, certain stimuli that up-regulate
MDM2 can, at the same time, activate p63 functions by keeping p53
activity at a minimum, whereas oncogenic stimuli that induce the ARF
protein can cause the opposite. Moreover, once activated, p63 might
contribute to its activation by keeping the level of ARF transcription
low. These considerations suggest that the role of p63 may not be as
central as that of p53 in tumor suppression, although it cannot be
excluded that p63 could provide a protection from cancer development in
tissues expressing both p53 and p63 proteins.
The role of p73 and p63 during normal development, the identification
of differentiation genes specifically activated by p63 and p73 but not
by p53 (33), and the difference in the ability to transactivate p53
target genes all strongly support the notion that these proteins,
although closely related, have differentiated distinct physiological
functions. The difference observed in the mechanisms adopted by MDM2 to
control their functions further supports this emerging view.
We thank Rosaria Terracciano for technical
help and Drs. G. Del Sal, S. Soddu, A. J. Levine, and B. Vogelstein for the generous gift of some of the plasmids used in this study.
*
This work was supported by grants from the Italian
Association for Cancer Research, Ministero
dell'Università e della Ricerca Scientifica, and the Consiglio
Nazionale delle Ricerche (to G. L. M.).The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
Present address: DNAX Research Inst., 901 California Ave., Palo
Alto, CA 94304.
Published, JBC Papers in Press, November 19, 2001, DOI 10.1074/jbc.M107173200
2
T. Parisi, A. Pollice, A. Di Cristofano, V. Calabrò, and G. LaMantia, submitted for publication.
The abbreviations used are:
CAT, chloramphenicol
acetyltransferase;
GST, glutathione S-transferase;
ALLN, N-acetyl-leucyl-leucyl-norleucinal-CHO;
GFP, green
fluorescent protein.
The Human MDM2 Oncoprotein Increases the Transcriptional Activity
and the Protein Level of the p53 Homolog p63*
,,§,,
Department of Genetics and General and
Molecular Biology, University of Naples "Federico II," via
Mezzocannone 8, 80134 Napoli, Italy and the ¶ Department of
Clinical and Biological Sciences, S. Luigi Hospital, Orbassano,
10043 Torino, Italy
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
and
p63
isoforms are able to associate with human MDM2 (HDM2).
Overexpression of HDM2 increased the steady-state level of
intracellular p63 and enhanced its transcriptional activity. Both
effects appeared to be counteracted by ARF coexpression. These data
indicate that p63 can be activated by HDM2 under conditions in which
p53 is inhibited. Therefore, HDM2 expression could support p63-specific
transcriptional functions on a common set of genes, keeping
interference by p53 at a minimum.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
N isotypes that lack the TA domain (3). p63 shows a
remarkable structural similarity to p53 and to the related p73 protein:
~60% of the amino acids of the human p63 and p73 proteins in the
region corresponding to the DNA-binding domain are identical to those
of p53 (4).
Np63 isotype is predominantly expressed (3). However, it is
still not known how the expression of different isoforms of p63 is
regulated in different tissues and during development.
EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
and p63 cDNAs were isolated from
a human skeletal muscle cDNA library using a PCR-based technique
and cloned into the BamHI site of the pcDNA3-His
expression vector (Invitrogen) to express them as Xpress epitope-tagged
proteins. The amplification sequence consisted of 35 cycles of 98 °C
for 1 min, 62 °C for 1 min, and 72 °C for 1 min, after starting
with a denaturation step at 95 °C and ending with an
extending step at 72 °C for 10 min. A common p63 forward primer
(5'-CGGGATCCATGTCCCAGAGCACACAGACAAATG) and a p63-specific
(5'-GCGTAGTTTCTCCTCCCCCTCACTCCTAGGCG) or a p63-specific
(5'-GGTTTGGCTAGTCACATGGTATCCCTAGGCG) reverse primer were employed
to obtain p63 and p63, respectively. Wild-type p53 in pcDNA3
and the L22Q/W23S p53 mutant in the pCMV vector were from Dr. G. Del
Sal (originally from Dr. A. J. Levine). The 1.8-kb fragment
containing the wild-type p53 cDNA was retrieved by EcoRI
digestion and ligated into the pcDNA3-His vector to express p53 as
an Xpress epitope-tagged protein. The human Mdm2
(HDM2) cDNA cloned into the bacterial pGEX4T3 expression
vector was from Dr. S. Soddu (originally from Dr. D. George). The
BP100-CAT reporter, containing two copies of the p53RE motif derived
from the HDM2 intronic promoter, was provided by Dr. G. Del
Sal (originally from Dr. B. Vogelstein, Johns Hopkins University,
Baltimore). Human Mdm2 (HDM2) was from Dr.
B. Vogelstein. The 2.4-kb fragment containing the p21WAF
promoter was retrieved from the pGL3-p21 (pWWP) plasmid (14) and
ligated into the HindIII site of the pCAT0 plasmid to obtain the WAF-CAT1 reporter
construct. The 680-bp SalI-PstI
ARF-CAT reporter from the ARF promoter will be
described elsewhere.2 The
ARF cDNA, previously described (15), was cloned into the pcDNA3.1-His mammalian expression vector (Invitrogen). The pEGFP-C1 expression vector (CLONTECH) containing DNA
sequences for the enhanced green fluorescent protein was used for
normalization of transfection efficiency.
, and p63 were cotransfected along with the
p21WAF-CAT, BP100-CAT, or ARF promoter reporter
construct. The total amount of transfected DNA (20 µg) was kept
constant using empty vector DNA when necessary. Cells were collected
30-48 h after transfection; equal quantities of proteins, determined
by the Bradford method (Bio-Rad, Munchen, Germany), were assayed for CAT activity using 0.1 µCi of [14C]chloramphenicol and
4 mM acetyl-CoA. Separated products were detected and
quantitated by a PhosphorImager (Molecular Dynamics, Inc.) and
ImageQuant software. The pCMV-
gal plasmid (1.5 µg) was used to
normalize CAT values for transfection efficiency.
, p63,
L22Q/W23S p53, or wild-type p53 (TNT, Promega) were incubated for
1 h at 4 °C with the GST-HDM2 fusion protein coupled to
glutathione-Sepharose beads (200-µl total reaction volume). The
mixtures were washed three times with 50 mM Tris-HCl (pH
7.4), 1 mM EDTA (pH 8.0), 100 mM NaCl, 0.1%
Nonidet P-40, 1 mM dithiothreitol, and 1 mM
phenylmethylsulfonyl fluoride. The bound proteins were analyzed on an
8% SDS-polyacrylamide gel and detected by autoradiography.
, and
p63 with or without 2 µg of HDM2 expression plasmid with
LipofectAMINE 2000. Cells were harvested 24 h after transfection
and lysed in immunoprecipitation buffer (150 mM
NaCl, 50 mM Tris-HCl, 0.5% Nonidet P-40, 1 mM
phenylmethylsulfonyl fluoride, 10 µg/ml leupeptin, 10 µg/ml
pepstatin, 10 µg/ml aprotinin, and 10 µg/ml trypsin inhibitor).
Debris was removed by centrifugation. Lysates (0.5 mg of protein) were
precleared with 30 µl of protein A-agarose (50% slurry) and then
incubated for 1 h at 4 °C with 2 µg of polyclonal anti-p63
antibody (H-137, Santa Cruz Biotechnology). Fresh protein A beads (30 µl) were added and incubated overnight at 4 °C. The beads were
loaded directly onto an SDS-polyacrylamide gel after two washes with
immunoprecipitation buffer. The co-immunoprecipitated proteins were
detected by Western blotting using anti-MDM2 (smp14, Santa Cruz
Biotechnology) and anti-Xpress (Invitrogen) antibodies.
and p63, Saos2 cells expressing the indicated cDNAs
were treated with cycloheximide (final concentration of 80 µg/ml) and
harvested at the indicated time points. Cells were processed for
Western blotting as described above. The 26 S proteasome inhibitor ALLN
(50 µM; Sigma) was used. Tubulin was detected with an
anti-tubulin antibody (C-20, Santa Cruz Biotechnology). For reverse
transcriptase-PCR, 24 h after transfection, cells were collected,
and total RNA was isolated using the Trizol LS reagent (Invitrogen)
following the manufacturer's instructions. 500 µg of total RNA were
reverse-transcribed using 200 units of Superscript II (Invitrogen) and
PCR-amplified as described above. The 600-bp fragment of the human
hypoxanthine phosphoribosyltransferase gene was amplified using
the following primers: 5'-CCTGCTGGATTACATTAAAGCACTG and
5'- CCTGAAGTACTCATTATAGTCAAGG.
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
and p63 in
Mammalian Cell Lines--
The p63 and p63 cDNAs encode
proteins of 448 and 641 amino acids, respectively (4). The longer isoform possesses an extended C-terminal region of 187 residues; but
the rest of the protein, with the exception of the last 40 residues of
the isoform, is shared by the two protein isoforms. The C-terminal
region of p63 includes a sterile -motif that has been described
as a putative protein-protein interaction domain (16). The three major
domains of p53 (NH2-terminal transactivation, DNA-binding,
and oligomerization domains) are conserved in both the and isoforms. We isolated the p63 and p63 cDNAs by reverse
transcriptase-PCR from a human skeletal muscle library and cloned them
into the pcDNA3.1-His expression vector. Before assessing the
effect of HDM2 on the transcriptional activity of both p63 isoforms, it
was of interest to compare the transcriptional properties of the two
p63 isotypes on two canonical p53-responsive promoters, p21WAF
and HDM2 (BP100-CAT).
/) and Saos2 cell lines, which not only lack
endogenous p53, but also exhibit low levels of p73 (17), were
transfected with equal amounts of p63 or p63 expression vector
together with the CAT reporter plasmids. As a positive control, we also transfected a p53 expression vector. As shown in Fig.
1 (A and B), both
p63 isoforms stimulated CAT activity, although a significant difference
in efficiency was observed: p63 enhanced CAT expression driven from
either promoter less strongly than p63 in both cell lines.
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Fig. 1.
Transcriptional activity of p63 in mammalian
cells. A, C33A cells were transfected with the
p21WAF-CAT (1 µg) or BP100-CAT (1 µg) reporter plasmid.
Expression plasmids for p53, p63 , and p63 (10 µg each) were
cotransfected. After 48 h, cells were harvested, and CAT was
activity determined as described under "Experimental Procedures."
The results of triplicate transfections are reported as the mean -fold
activation with each of the effectors (activity with effector/activity
with empty expression vector). The values presented were normalized
with an internal control as described under "Experimental
Procedures." S.D. values are shown by error bars.
B, Saos2 cells were transfected with the p21WAF-CAT
or BP100-CAT reporter plasmid (0.2 µg). The expression vectors
indicated (0.2 µg each) were cotransfected. Transfection was
performed as described under "Experimental Procedures." The results
of triplicate transfections are reported as the mean -fold activation
with each of the effectors (activity with effector/activity with empty
expression vector). The values presented were normalized with an
internal control as described under "Experimental Procedures." S.D.
values are shown by error bars. C, C33A cells
were transfected with 10 µg of ARF-CAT reporter construct
in combination with 10 µg of the indicated expression vectors. The
CAT assay was performed as described under "Experimental
Procedures." The basal activity of the ARF-CAT reporter
was set to 100%. Values represent the means ± S.D. of three
independent experiments.
, or p63 expression plasmid.
Fig. 1C shows that both p63 and p63 reduced
ARF-CAT expression, although less efficiently than
p53. These results indicate that p63 also shares the
trans-repression ability with p53. Again, p63 appears to
be more efficient than the isoform.
and p63 were due to different expression levels
of the and isoforms, we measured the protein levels of the two
isotypes 48 h after transfection in the Saos2 cell line. The
stronger transcriptional activity of p63 cannot be attributed to a
higher expression level, as Western blot analysis revealed that p63
levels exceeded those of p63 (Fig.
2A). Similar results were
obtained in COS-7 cells (data not shown). These results suggest that
the extended C-terminal region, which distinguishes p63 from p63,
could influence the level of the p63 protein, perhaps altering its
half-life. We assessed this possibility by introducing expression
vectors for p63 and p63 into Saos2 cells and following their
protein levels after treatment with cycloheximide (19). Because
cycloheximide inhibits de novo protein synthesis, the
half-life of the proteins could be determined by Western blot analysis
in cells treated with the drug. As Fig. 2B clearly shows, p63 had a markedly prolonged half-life.
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Fig. 2.
Levels of p63 isoforms. A, Saos2
cells were transiently transfected either with 2 µg of empty vector
(pcDNA) or expression plasmids (2 µg each) encoding p53, p63 ,
and p63. The pEGFP-1C vector (0.5 µg) was included as a control of
transfection efficiency. Extracts from transfected cells were
immunoblotted with anti-Xpress and anti-GFP antibodies as indicated.
B, for measuring half-lives of p63 and p63, Saos2
cells were transfected with 2 µg of the indicated vectors. The cells
were treated with cycloheximide (80 µg/ml) at 24 h
post-transfection and harvested 0, 60, 180, and 360 min later. To
obtain comparable starting levels of p63 and p63, 10 µg of
extract from p63-transfected cells and 50 µg of extract from
p63-transfected cells were analyzed by Western blotting and detected
with the anti-Xpress antibodies.
(Fig.
3A), or p63 (Fig.
3B) as transactivator and increasing amounts of HDM2. As
shown in Fig. 3 (A and B, third and
fourth bars), cotransfection of p63 or p63 and HDM2
expression plasmids in 1:2 and 1:4 molar ratios produced a remarkable
enhancement of p63 transcriptional activity. As a control, we performed
the same experiment using p53 as transactivator. As expected,
coexpression of HDM2 considerably reduced the p53 transcriptional
activity measured on the BP100-CAT reporter (Fig. 3C). A 1:1
molar ratio (second bar) of p53 to HDM2 was already
sufficient to reduce the p53 transcriptional activity to 46% with
respect to that observed without HDM2, and increasing amounts of HDM2
caused no more than an additional 10-16% reduction of p53
transcriptional activity.
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Fig. 3.
Transcriptional activity of
p63 and p63 in the
presence of HDM2. Saos2 cells were transfected with the BP100-CAT
reporter plasmid (0.2 µg/dish) and expression plasmids for p63
(0.2 µg; A), p63 (0.2 µg; B), and p53 (0.1 µg; C). Increasing amounts of HDM2 (corresponding to 1:1,
1:2, and 1:4 molar ratios of p63 (A), p63
(B), and p53 (C) to the HDM2 expression vector)
were cotransfected. The values obtained with p63, p63, or p53
alone were set to 100%. All CAT activities measured in the presence of
HDM2 are given as a percent of the values obtained with p53, p63, or
p63 alone. Values represent the means ± S.D. of four
independent experiments.
and p63 proteins were
synthesized and [35S]Met-labeled by an in
vitro transcription/translation assay. The L22Q/W23S p53 mutant
protein, which is unable to interact with MDM2 (20), and wild-type p53
were obtained in a similar way. SDS-PAGE followed by autoradiography
revealed that proteins of the expected size and in comparable amounts
were obtained in all cases (data not shown). The reticulocyte lysates
were then incubated with the GSH-agarose-immobilized GST-HDM2 fusion
protein. After appropriate washing, the bound proteins were subjected
to SDS-PAGE and detected by autoradiography. Fig.
4A shows that the interaction
of both p63 and p63 with the GST-HDM2 protein was comparable to
that of wild-type p53. Using the mutant p53 protein, a negligible
amount of protein was detected.
View larger version (18K):
[in a new window]
Fig. 4.
HDM2 binds to p63. A, GST-HDM2
fusion proteins immobilized on Sepharose were incubated with 20 µl of
in vitro translated, 35S-labeled p53, L22Q/W23S
p53, p63 , or p63 at 4 °C for 1 h as indicated. Bound
proteins were analyzed as described under "Experimental
Procedures." A control of binding with GST alone is also shown.
B, Saos2 cells were transfected with plasmid encoding p63
or p63 with or without HDM2 as indicated. At 24 h
post-transfection, cells were harvested for immunoprecipitation
(IP). p63-HDM2 complexes were analyzed by
immunoprecipitation using polyclonal anti-p63 antibodies. Proteins were
revealed with anti-Xpress and anti-MDM2 antibodies (as indicated). The
positions of molecular mass marker are indicated to the left.
WB, Western blot.
or p63 and the HDM2-encoding expression vector. Cellular lysates were immunoprecipitated with polyclonal anti-p63 antibody H-137 and probed with the monoclonal anti-MDM2 antibody. As shown in Fig. 4B, HDM2 was
co-immunoprecipitated with the polyclonal anti-p63 antibody when
coexpressed with p63 or p63.
(Fig. 5B) and increasing amounts of HDM2
expression vector. 0.5 µg of plasmid pEGFP-C1 were included as the
transfection control. Cellular lysates were subjected to immunoblotting
with antibodies against the Xpress epitope (Fig. 5B).
The identity of the p63 bands was then confirmed using an antibody
raised against the N terminus of the p63 protein (data not shown). The
p53 protein was revealed with an antibody raised against an epitope
corresponding to amino acids 156-214 of the human p53 protein (Fig.
5A), whereas the HDM2 protein was revealed with an antibody
raised against an epitope corresponding to amino acids 154-167 of the
human MDM2 protein (Fig. 5, A and B). Anti-GFP
immunoblotting demonstrated that, in all cases, comparable transfection
efficiency was achieved. HDM2-induced degradation of the p53 protein
was detected easily, and the effect was found to be
dose-dependent (Fig. 5A). Moreover, as the COS-7
cells expressed detectable levels of the endogenous p53 protein (Fig.
5A, lanes 1-3), a reduction of the endogenous
p53 protein level was seen when HDM2 was overexpressed. In contrast,
overexpression of HDM2 resulted in a remarkable increase in the level
of the p63 protein (Fig. 5B). Moreover, a parallel
increase in the level of endogenous p21WAF was observed (Fig.
5B). Because we observed an effect of HDM2 on the p63
transcriptional activity in Saos2 cells, we performed similar
experiments in this cell line with both p63 isoforms; and again, we
noticed a progressive rise in the level of the p63 protein when
increasing amounts of HDM2 were cotransfected (Fig. 5C).
View larger version (13K):
[in a new window]
Fig. 5.
HDM2 increases p63 intracellular levels.
A, COS-7 cells were transfected with the pcDNA3 or p53
expression vector (0.2 µg/dish) in combination with increasing
amounts of HDM2: 0.2 µg (lanes 2 and 5) and 1.6 µg (lanes 3 and 6). Extracts from COS-7 cells
were subjected to immunoblotting with antibodies against p53, MDM2, and
GFP as indicated. B, COS-7 cells were transfected with the
p63 expression plasmid (0.2 µg/dish; lanes
1-5) in combination with increasing amounts of HDM2:
0.2 µg (lane 2), 0.4 µg (lane 3), 0.8 µg
(lane 4), and 1.6 µg (lane 5). Extracts from
COS-7 cells were subjected to immunoblotting with antibodies against
the Xpress epitope, MDM2, p21WAF, and GFP as indicated.
C, Saos2 cells were transfected with expression plasmids
(total of 2 µg of DNA) for p63 (0.2 µg/dish; lanes
1-4) and p63 (0.2 µg/dish; lanes 5-8) in
combination with increasing amounts of HDM2: 0.2 µg (lane
2 and 6), 0.4 µg (lanes 3 and
7), and 0.8 µg (lanes 4 and 8). At
48 h post-transfection, the cells were harvested and extracted as
described under "Experimental Procedures." Western blotting was
performed with anti-Xpress, anti-MDM2, and anti-GFP antibodies as
indicated. The pEGFP-1C vector was included as a control of
transfection efficiency.
protein level was due
to an increase in transcription or stability of p63 mRNA, we
performed reverse transcriptase-PCR experiments. Fig. 6A shows that the relative
level of p63 mRNA was similar in the presence and absence of
HDM2, suggesting that the effect of MDM2 on p63 may be
post-translational. Fig. 6B shows that, after treatment with
ALLN, a proteasome inhibitor, more p63 protein was detected, suggesting that the p63 protein may be degraded by a
proteasome-dependent pathway. Significantly, ALLN did not
further increase the level of p63 in the presence of HDM2,
suggesting that HDM2 and ALLN may both act to prevent
proteasome-dependent degradation. Similar results were
obtained with the p63 isotype (data not shown). Hence, HDM2
increases p63 protein levels under conditions in which p53 is
degraded.
View larger version (8K):
[in a new window]
Fig. 6.
Regulation of p63 expression by HDM2.
A, COS-7 cells were transfected with p63 (0.5 µg) and
empty vector or HDM2 (2 µg). The relative amount of p63 mRNA
was analyzed by reverse transcriptase (RT)-PCR using p63
forward and reverse primers. HPTR, reverse transcriptase-PCR
products obtained using oligonucleotides of the hypoxanthine
phosphoribosyltransferase (HPTR) gene. B, COS-7
cells were transfected with p63 (0.5 µg) and empty vector or HDM2
(2 µg). After transfection, the cells were divided into two identical
plates (vector (lanes 1 and 2) and HDM2
(lanes 3 and 4)) and allowed to grow for 24 h. Buffer (lanes 1 and 3) or ALLN
(ALLnL; 50 µM; lanes 2 and
4) was added to the medium, and the cells were incubated for
another 12 h. Cell extracts were subjected to immunoblotting for
Xpress or tubulin.
that we know results in a strong enhancement of p63
transcriptional activation and protein stabilization (Figs.
3B, fourth bar; and 5C, lane 4). As shown in Fig. 7A, when increasing amounts of ARF
were added, the increase in p63 transcriptional activity induced by
HDM2 was progressively abolished. No effect was observed on the
p63-driven transcription of the reporter plasmids when only ARF was
expressed (Fig. 7A, sixth bar). We then tested
whether or not ARF was also able to reduce the HDM2-induced enhancement
of the p63 protein level. The p63 expression plasmid was transfected
in the Saos2 cell line with or without a fixed amount of HDM2
expression vector and increasing amounts of ARF vector (Fig.
7B). Exogenous expression of HDM2 produced an increase in
the p63 level (Fig. 7B, lane 5) that was
progressively abolished by the addition of increasing amounts of ARF
expression vector (lanes 6-8). Moreover, as the Saos2 cells
expressed detectable levels of endogenous HDM2 proteins (Fig.
7B, lane 1), a slight reduction of the p63
protein level was also seen when ARF alone was overexpressed
(lanes 2-4). Similar results were obtained using the p63
expression vector (data not shown).
View larger version (14K):
[in a new window]
Fig. 7.
ARF counteracts HDM2-mediated p63 protein
stabilization and transcriptional activation. A, Saos2
cells were transfected with the indicated combinations of the following
expression plasmids (total of 2 µg of DNA): BP100-CAT (0.2 µg/dish;
first through sixth bars), p63 (0.2 µg/dish;
first through sixth bars), HDM2 (0.8 µg/dish;
second through fifth bars), and/or ARF (0.2 µg/dish (third bar), 0.4 µg/dish (fourth
bar), and 0.8 µg/dish (fifth and sixth
bars). CAT activities measured with p63 and HDM2; p63 and
ARF; and p63, HDM2, and ARF are given as a percent of the values
obtained with p63 alone. Values represent the means ± S.D. of
three independent experiments. B, Saos2 cells were
transfected with expression plasmids (total of 2 µg of DNA/dish) for
p63 (0.2 µg/dish; lanes 1-8) and HDM2 (0.8 µg/dish;
lanes 5-8) and with increasing amounts of ARF expression
plasmid: 0.2 µg (lanes 2 and 6), 0.4 µg
(lanes 3 and 7), and 0.8 µg (lanes 4 and 8). Western blot analysis of cellular lysates were
carried out with the indicated antibodies. The pEGFP-1C vector was
included as a control of transfection efficiency.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
and p63 exogenous
expression, already sufficient to induce expression of endogenous MDM2.
A possible explanation of the apparent discrepancy with our results is
that, under their experimental conditions, p63 exogenous protein had
already undergone stabilization, so that addition of exogenous MDM2
caused no further effect.
ACKNOWLEDGEMENTS
FOOTNOTES
To whom correspondence should be addressed. Tel.:
39-81-2535189; Fax: 39-81-2535000; E-mail: lamantia@unina.it.
ABBREVIATIONS
REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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