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Query: UNIPROT:P43146 (
tumour suppressor
)
5,935
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
The ARF
tumour suppressor
protein plays a critical role in the activation of p53 in response to oncogenic stress. ARF can activate p53 through nucleolar sequestration of
Mdm2
. However, several lines of evidence indicate that this is not the only way of action of ARF, and alternative mechanisms must exist. p33ING1 is a putative tumour suppresor, which induces cell-cycle arrest and apoptosis in a p53-dependent manner. Here, we describe that ARF and p33ING1 can interact in vivo. We also show that the subcellular localization of ING1 can be modulated by ARF protein levels, causing a displacement from nuclear to nucleolar localization. Finally, the ability of p33ING1 to cause cell-cycle arrest and induction of p21CIP1, or
Mdm2
, is impaired in ARF-deficient primary mouse fibroblasts. Based on these observations, we propose that the interaction with p33ING1 represents a novel mechanism for the tumour suppression function of ARF.
...
PMID:A functional link between the tumour suppressors ARF and p33ING1. 1660 80
When the genomic integrity of a cell is challenged, its fate is determined in part by signals conveyed by the p53
tumour suppressor
protein. It was observed recently that such signals are not simple gradations of p53 concentration, but rather a counter-intuitive limit-cycle behaviour. Based on a careful mathematical interpretation of the experimental body of knowledge, we propose a model for the p53 signalling network and characterise the p53 stability and oscillatory dynamics. In our model, ATM, a protein that senses DNA damage, activates p53 by phosphorylation. In its active state, p53 has a decreased degradation rate and an enhanced transactivation of
Mdm2
, a gene whose protein product
Mdm2
tags p53 for degradation. Thus the p53-
Mdm2
system forms a negative feedback loop. However, the feedback in this loop is delayed, as the pool of
Mdm2
molecules being induced by p53 at a given time will mark for degradation the pool of p53 molecules at some later time, after the
Mdm2
molecules have been transcribed, exported out of the nucleus, translated and transported back into the nucleus. The analysis of our model demonstrates how this time lag combines with the ATM-controlled feedback strength and effective dampening of the negative feedback loop to produce limit-cycle oscillations. The picture that emerges is that ATM, once activated by DNA damage, makes the p53-
Mdm2
oscillator undergo a supercritical Hopf bifurcation. This approach yields an improved understanding of the global dynamics and bifurcation structure of our time-delayed, negative feedback model and allows for predictions of the behaviour of the p53 system under different perturbations.
...
PMID:p53-Mdm2 loop controlled by a balance of its feedback strength and effective dampening using ATM and delayed feedback. 1698 75
The p53
tumour suppressor
has a key role in the control of cell growth and differentiation, and in the maintenance of genome integrity. p53 is kept labile under normal conditions, but in response to stresses, such as DNA damage, it accumulates in the nucleus for induction of cell-cycle arrest, DNA repair or apoptosis.
Mdm2
is an ubiquitin ligase that promotes p53 ubiquitination and degradation.
Mdm2
is also self-ubiquitinated and degraded. Here, we identified a novel cascade for the increase in p53 level in response to DNA damage. A new SUMO-specific protease, SUSP4, removed SUMO-1 from
Mdm2
and this desumoylation led to promotion of
Mdm2
self-ubiquitination, resulting in p53 stabilization. Moreover, SUSP4 competed with p53 for binding to
Mdm2
, also resulting in p53 stabilization. Overexpression of SUSP4 inhibited cell growth, whereas knockdown of susp4 by RNA interference (RNAi) promoted of cell growth. UV damage induced SUSP4 expression, leading to an increase in p53 levels in parallel with a decrease in
Mdm2
levels. These findings establish a new mechanism for the elevation of cellular p53 levels in response to UV damage.
...
PMID:SUMO-specific protease SUSP4 positively regulates p53 by promoting Mdm2 self-ubiquitination. 1708 74
CDKN2A locus on chromosome 9p21 encodes two
tumour suppressor
proteins pl6INK4A, which is a regulator of the retinoblastoma (RB) protein, and p14ARF, which is involved in the ARF-
Mdm2
-p53 pathway. The aim of this study was to determine if CDKN2A gene products are implicated in differentiated thyroid carcinogenesis and progression. We used real-time quantitative RT-PCR and immunohistochemistry to assess both transcripts and proteins levels in 60 tumours specimens. Overexpression of p14ARF and pl6INK4A was observed in follicular adenomas, follicular carcinomas and papillary carcinomas, while downregulation was found in oncocytic adenomas compared to nontumoral paired thyroid tissues. These deregulations were statistically significant for pl6INK4a (P=0.006) in follicular adenomas and close to statistical significance for p14ARF in follicular adenomas (P=0.06) and in papillary carcinomas (P=0.05). In all histological types, except papillary carcinomas, we observed a statistically significant relationship between p14ARF and E2F1 (r=0.64 to 1, P<0.05). Our data are consistent with involvement of CDKN2A transcript upregulation in thyroid follicular tumorigenesis as an early event. However, these deregulations do not appear to be correlated to the clinical outcome and they could not be used as potential prognostic markers.
...
PMID:The status of CDKN2A alpha (p16INK4A) and beta (p14ARF) transcripts in thyroid tumour progression. 1711 77
The p53
tumour suppressor
is regulated mainly by
Mdm2
, an E3 ubiquitin ligase that promotes the ubiquitylation and proteasome-mediated degradation of p53. Many agents that induce p53 are inhibitors of transcription, suggesting that the p53 pathway can detect a signal(s) arising from transcriptional malfunction.
Mdm2
associates with TAFII250, a component of the general transcription factor TFIID. Inactivation of TAFII250 in ts13 cells, which express a temperature-sensitive mutant of TAFII250, leads to the induction of p53 and cell cycle arrest. In the present study, we show that TAFII250 stimulates the ubiquitylation and degradation of p53 in a manner that is dependent upon
Mdm2
and requires its acidic domain. Mechanistically, TAFII250 downregulates
Mdm2
auto-ubiquitylation, leading to
Mdm2
stabilization, and promotes p53-
Mdm2
association through a recently defined second binding site in the acidic domain of
Mdm2
. These data provide a novel route through which TAFII250 can directly influence p53 levels and are consistent with the idea that the maintenance of p53 turnover is coupled to the integrity of RNA polymerase II transcription.
...
PMID:Transcription factor TAFII250 promotes Mdm2-dependent turnover of p53. 1723 21
Mdm2
is an E3 ubiquitin ligase that promotes its own ubiquitination and also ubiquitination of the p53
tumour suppressor
. In a bacterial two-hybrid screen, using
Mdm2
as bait, we identified an
Mdm2
-interacting peptide that bears sequence similarity to the deubiquitinating enzyme USP2a. We have established that full-length USP2a associates with
Mdm2
in cells where it can deubiquitinate
Mdm2
while demonstrating no deubiquitinating activity towards p53. Ectopic expression of USP2a causes accumulation of
Mdm2
in a dose-dependent manner and consequently promotes
Mdm2
-mediated p53 degradation. This differs from the behaviour of HAUSP, which deubiquitinates p53 in addition to
Mdm2
and thus protects p53 from
Mdm2
-mediated degradation. We further demonstrate that suppression of endogenous USP2a destabilises
Mdm2
and causes accumulation of p53 protein and activation of p53. Our data identify the deubiquitinating enzyme USP2a as a novel regulator of the p53 pathway that acts through its ability to selectively target
Mdm2
.
...
PMID:The deubiquitinating enzyme USP2a regulates the p53 pathway by targeting Mdm2. 1729 Feb 20
Mdm2
, an E3 ubiquitin ligase, negatively regulates the
tumour suppressor
p53. Loss of
Mdm2
in mice results in p53-dependent apoptosis and embryonic lethality. This phenotype was rescued by the p53(515C) allele, which encodes an apoptosis-deficient p53R172P protein. However, these mice died within 2 weeks of birth, due to a severe impairment of progenitor cell expansion during postnatal haematopoiesis and cerebellar development, leading to p53-dependent cell cycle arrest. Loss of
Mdm2
led to phosphorylation of the p53R172P protein, p53R172P stability and activation of the cell cycle inhibitor p21 in proliferating cells, but not in differentiated cells, in multiple tissue compartments. Proliferating cells of epithelial origin were not affected. The haematopoietic and neural defects were alleviated in mice lacking
Mdm2
and containing one p53(515C) and one p53-null allele, but spermatogenesis was arrested. These findings establish a crucial role for the p53-
Mdm2
network in regulating proliferation and progenitor expansion in many cell lineages and have important implications for the use of drugs that aim to disrupt the p53-
Mdm2
interaction.
...
PMID:The p53-Mdm2 network in progenitor cell expansion during mouse postnatal development. 1797 40
Induction and activation of the p53
tumour suppressor
protein occurs in response to a number of cellular stresses, including disruption of RNA polymerase II-mediated transcription. Both p53 itself and its principle negative regulator, the E3 ubiquitin ligase
Mdm2
, are substrates for phosphorylation by the protein kinase CK2 in vitro. CK2 phosphorylates
Mdm2
within its central acidic domain, a region that is critical for making a second point of contact with p53 and mediating p53 ubiquitylation and turnover. Additionally, there is evidence that CK2 interacts with, and regulates, both p53 and
Mdm2
within the cell but the molecular mechanisms through which CK2-mediated regulation of the p53 response can occur are only poorly understood. Previously, we showed that the basal transcription factor TAFII250, a critical component of TFIID, can interact with
Mdm2
and promote the association of the
Mdm2
acidic domain with p53. In the present study, we show that immunoprecipitates of TAFII250, either from mammalian cell extracts or from baculovirus-infected cells expressing elevated levels of HA-tagged TAFII250, can phosphorylate
Mdm2
in vitro within its acidic domain. We show that CK2 is tightly associated with TAFII250 and is the principal activity responsible for TAFII250-mediated phosphorylation of
Mdm2
. Our data fit with recent observations that phosphorylation of the acidic domain of
Mdm2
stimulates its association with p53 and are consistent with a model in which recruitment of CK2 by TAFII250 may play a contributory role in the maintenance of
Mdm2
phosphorylation and function.
...
PMID:Transcription factor TAFII250 phosphorylates the acidic domain of Mdm2 through recruitment of protein kinase CK2. 1854
Mdm2
(murine double minute 2)-mediated ubiquitination of the p53
tumour suppressor
requires interaction of the ligase at two distinct binding sites that form general multiprotein-docking sites for the p53 protein. The first
Mdm2
-binding site resides in the transactivation domain of p53 and is an allosteric effector site for
Mdm2
-mediated p53 ubiquitination; the second site requires the acid domain of
Mdm2
to recognize a 'ubiquitination signal' within p53's DNA-binding core. In order to expand on fundamental requirements for a protein to function as an
Mdm2
substrate and the role of the acid domain in recognition, we have carried out a bioinformatics search for open reading frames that have homology with the
Mdm2
-docking sites in p53. IRF-2 [IFN (interferon) regulatory factor-2], an IFN-regulated transcription factor, has been identified as an Mdm2-binding protein and substrate requiring interactions with both the hydrophobic pocket and the acid domain of
Mdm2
. Mutation of either of the two
Mdm2
-binding sites on IRF-2 can attenuate substrate ubiquitination, confirming the requirement of a dual-site substrate interaction mechanism. Ligands that bind to the hydrophobic pocket are not sufficient to inhibit
Mdm2
E3-ligase activity. Rather, acid domain-binding ligands act as E3-ligase inhibitors, lending additional support to the idea that the acid domain of
Mdm2
is key to understanding its mechanism of action. The ability of
Mdm2
and IRF-2 to form a complex in cells complements the biochemical assays and together establishes a novel substrate with which to develop insights into E3-ubiquitin ligase-substrate interactions in vitro and in cells.
...
PMID:Role of Mdm2 acid domain interactions in recognition and ubiquitination of the transcription factor IRF-2. 1903 50
The E3 ubiquitin ligase
Mdm2
is a focal regulator of p53
tumour suppressor
activity. It binds p53, promoting its polyubiquitination and degradation, and also controls p53 synthesis. However, it is not known how this dual function of
Mdm2
on p53 synthesis and degradation is achieved. Here we show that the p53 mRNA region encoding the
Mdm2
-binding site interacts directly with the RING domain of
Mdm2
. This impairs the E3 ligase activity of
Mdm2
and promotes p53 mRNA translation. We also show that introduction of cancer-derived single silent point-mutations in the p53 mRNA weakens its binding to
Mdm2
and results in reduced p53 activity. These data are consistent with a mechanism by which changes in silent nucleotides can affect the function of the encoded protein, and indicate that
Mdm2
-mediated control of p53 synthesis and degradation has evolved in the p53 mRNA sequence and its encoded amino acids.
...
PMID:P53 mRNA controls p53 activity by managing Mdm2 functions. 1916 Apr 91
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