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Query: UNIPROT:P04637 (
p53
)
77,613
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
p19
(ARF) is a potent tumor suppressor. By inactivating Mdm2,
p19
(ARF) upregulates
p53
activities to induce cell cycle arrest and sensitize cells to apoptosis in the presence of collateral signals. It has also been demonstrated that cell cycle arrest is induced by overexpressed
p19
(ARF) in
p53
-deficient mouse embryonic fibroblasts, only in the absence of the Mdm2 gene. Here, we show that apoptosis can be induced without additional apoptosis signals by expression of
p19
(ARF) using an adenovirus-mediated expression system in
p53
-intact cell lines as well as
p53
-deficient cell lines. Also, in primary mouse embryonic fibroblasts (MEFs) lacking
p53
/ARF,
p53
-independent apoptosis is induced irrespective of Mdm2 status by expression of
p19
(ARF). In agreement,
p19
(ARF)-mediated apoptosis in U2OS cells, but not in Saos2 cells, was attenuated by coexpression of Mdm2. We thus conclude that there is a
p53
-independent pathway for
p19
(ARF)-induced apoptosis that is insensitive to inhibition by Mdm2.
...
PMID:p53-independent apoptosis is induced by the p19ARF tumor suppressor. 1209 84
Parathyroid adenomas (PTAs) are the main cause of primary hyperparathyroidism. Cell cycle regulation in normal parathyroid tissue (NPT) and PTA remains largely unknown. We have systematically explored several components involved in the
p53
/MDM2/
p19
(ARF) pathway in PTA and compared the results were with NPT. Forty-six PTA and 12 NPT were immunostained with anti-p21(WAF-1), MDM2,
p53
, and p27(KP1) antibodies. The slides were processed by cytometry and the results were statistically analyzed using nonparametric methods (Mann-Whitney test). p2l(WAF-1) and MDM2 expression were significantly higher in PTA compared with NPT (p < 0.05). The opposite results were found for p27(KIP1) (p< 0.05). Occasional
p53
staining was found in some PTA, albeit no significant difference was found in comparison with NPT. In conclusion, MDM2 and p2l(WAF-1) are the proteins more overexpressed in PTA. These findings are surprising taking into account the benign nature of PTA, making them suitable candidates for further molecular analysis.
...
PMID:p53/MDM2 Pathway Aberrations in Parathyroid Tumors: p21(WAF-1) and MDM2 Are Frequently Overexpressed in Parathyroid Adenomas. 1211 97
Inactivation of the neurofibromatosis-1 (NF1) gene de-regulates RAS and cooperates with mutation or loss of the
p53 tumor suppressor
to induce tumorigenesis.
p19
(ARF) acts upstream of
p53
in an oncogene checkpoint to induce apoptosis in response to activated RAS and other factors that stimulate proliferation. Therefore, we bred
p19
(ARF-/-) to NF1(+/-) mice to determine if loss of these genes collaborates in tumorigenesis. As expected from the embryonic lethality of NF1 null mice, no mice lacking both
p19
(ARF) and NF1 were born. Unexpectedly, the loss of one allele of NF1 did not greatly shorten the time to tumor formation in a
p19
(ARF) null background. The tumor types observed were characteristic of
p19
(ARF) null animals, not those associated with neurofibromatosis or those observed with NF1(+/-)/
p53
(+/-) mice. However, seven out of 12 animals developed multiple tumors, some with metastases. This multiple tumor phenotype was not previously observed with
p19
(ARF)-null mice and suggests a distinct form of cooperation between the loss of these tumor suppressors.
...
PMID:Loss of neurofibromatosis-1 and p19(ARF) cooperate to induce a multiple tumor phenotype. 1211 76
During adeno-associated virus (AAV) type 2 productive infections, the
p19
promoter of AAV is activated by the AAV Rep78 and Rep68 proteins. Rep-induced activation of
p19
depends on the presence of one of several redundant Rep binding elements (RBEs) within the p5 promoter or within the terminal repeats (TR). In the absence of the TR, the p5 RBE and the
p19
Sp1 site at position -50 are essential for
p19
transactivation. To determine how a Rep complex bound at p5 induces transcription at
p19
, we made a series of
p19
promoter chloramphenicol acetyltransferase constructs in which the p5 RBE was inserted at different locations upstream or downstream of the
p19
mRNA start site. The RBE acted like a repressor element at most positions in the presence of both Rep and adenovirus (Ad), and the level of repression increased dramatically as the RBE was inserted closer to the
p19
promoter. We concluded that the RBE by itself was not a conventional upstream activation signal and instead behaved like a repressor. To understand how the Rep-RBE complex within p5 activated
p19
, we considered the possibility that its role was to function as an architectural protein whose purpose was to bring other p5 transcriptional elements to the
p19
promoter. In order to address this possibility, we replaced both the p5 RBE and the
p19
Sp1 site with GAL4 binding sites. The modified GAL4-containing constructs were cotransfected with plasmids that expressed GAL4 fusion proteins capable of interacting through
p53
and T-antigen (T-ag) protein domains. In the presence of Ad and the GAL4 fusion proteins, the
p19
promoter exhibited strong transcriptional activation that was dependent on both the GAL4 fusion proteins and Ad infection. This suggested that the primary role of the p5 RBE and the
p19
Sp1 sites was to act as a scaffold for bringing transcription complexes in the p5 promoter into close proximity with the
p19
promoter. Since Rep and Sp1 themselves were not essential for transactivation, we tested mutants within the other p5 transcriptional elements in the context of GAL4-induced looping to determine which of the other p5 elements was necessary for
p19
induction. Mutation of the p5 major late-transcription factor site reduced
p19
activity but did not eliminate induction in the presence of the GAL4 fusion proteins. However, mutation of the p5 YY1 site at position -60 (YY1-60) eliminated GAL4-induced transactivation. This implicated the YY1-60 protein complexes in
p19
induction by Rep. In addition, both basal
p19
activity and activity in the presence of Ad increased when the YY1-60 site was mutated even in the absence of Rep or GAL4 fusion proteins. Therefore, there are likely to be alternative p5-
p19
interactions that are Rep independent in which the YY1-60 complex inhibits
p19
transcription. We concluded that transcriptional control of the
p19
promoter was dependent on the formation of complexes between the p5 and
p19
promoters and that activation of the
p19
promoter depends largely on the ability of Rep and Sp1 to form a scaffold that positions the p5 YY1 complex near the
p19
promoter.
...
PMID:Studies of the mechanism of transactivation of the adeno-associated virus p19 promoter by Rep protein. 1213 28
The p16(INK4a)/pRB/E2F and
p19
(ARF)/
p53 tumor suppressor
pathways are disrupted in most human cancers. Both
p19
(ARF) and
p53
are required for the induction of senescence in primary mouse embryonic fibroblasts (MEFs), but little is known about their downstream targets. Disruption of E2F-mediated transcriptional repression in MEFs caused a general increase in the expression of E2F target genes, including p19ARF. We detected no contribution of E2F-mediated transactivation in this setting, indicating that a predominant role of endogenous E2F in asynchronously growing primary MEFs is to repress its target genes. Moreover, relief of transcriptional repression by E2F rendered MEFs resistant to senescence induced by either
p19
(ARF),
p53
, or RAS(V12). Thus, E2F transcriptional repressor complexes are critical downstream targets of antiproliferative
p19
(ARF)/
p53
signaling.
...
PMID:E2F transcriptional repressor complexes are critical downstream targets of p19(ARF)/p53-induced proliferative arrest. 1215 Aug 25
The INK4a locus on chromosome 9p21 encodes two structurally distinct tumor suppressor proteins, p16(INK4a) and the alternative reading frame protein, ARF (
p19
(ARF) in mouse and p14(ARF) in human). Each of these proteins has a role in senescence of primary cells and activates pathways for cell cycle control and tumor suppression. The current prevailing model proposes that
p19
(ARF) activates
p53
function by antagonizing its degradation by MDM2. It was, however, recently shown that stabilization of
p53
by p14(ARF) occurs independent of the relocalization of MDM2 to the nucleolus. We have identified a novel collaborator of ARF, CARF. It co-localizes and interacts with ARF in the nucleolus. We demonstrate that CARF is co-regulated with ARF, cooperates with it in activating
p53
, and thus acts as a novel component of the ARF-
p53
-p21 pathway.
...
PMID:CARF is a novel protein that cooperates with mouse p19ARF (human p14ARF) in activating p53. 1215 87
Expression of the Kaposi's sarcoma-associated herpesvirus (KSHV) cyclin D homolog, K cyclin, is thought to contribute to viral oncogenesis. We show that K cyclin expression in primary cells sensitizes to apoptosis and induces growth arrest, both of which are dependent on
p53
but independent of E2F1 or
p19
(ARF). DNA synthesis, but not cytokinesis, continues in K cyclin-expressing cells, leading to multinucleation and polyploidy. Such polyploid cells exhibit pronounced centrosome amplification and consequent aneuploidy. Our data suggest that K cyclin expression leads to cytokinesis defects and polyploidy, which activates
p53
. However, in the absence of
p53
, such cells survive and expand as an aneuploid population. Corroborating these findings, in vivo Emu; K cyclin expression cooperates with
p53
loss in the induction of lymphomas.
...
PMID:The oncogenic potential of Kaposi's sarcoma-associated herpesvirus cyclin is exposed by p53 loss in vitro and in vivo. 1224 55
The WEHI 231 B cell lymphoma is used as a model of self-tolerance by clonal deletion because B cell receptor (BCR) ligation results in apoptosis. Two critical events precede cell death: an early rise and fall in expression of MYC and cell-cycle arrest associated with enhanced expression of p21, p27, and
p53
. CTCF is a transcription factor identified as a repressor of MYC recently shown to cause cell growth inhibition. The present studies demonstrate that BCR ligation of WEHI 231 as well as of normal immature B cells greatly increased expression of CTCF in association with down-regulation of MYC followed by growth arrest and cell death. Conditional expression of CTCF in WEHI 231 mimicked BCR ligation with activated cells showing repressed expression of MYC, enhanced expression of p27, p21,
p53
, and
p19
(ARF), and inhibition of cell growth and induction of apoptosis. In keeping with a central role for CTCF in control of B cell death, conditional expression of a CTCF antisense construct in WEHI 231 resulted in inhibition of p27, p21,
p53
, and
p19
(ARF) in association with enhanced expression of MYC. Activation of the endogenous CTCF locus by BCR ligation was also mimicked by three other routes to apoptotic death in WEHI 231: inhibition of the phosphoinositide 3-kinase or mTORFRAP signaling cascades and treatment with transforming growth factor (TGF)-beta. Rapid activation of CTCF by BCR ligation or treatment with TGF-beta was suppressed by ligation of CD40. These results demonstrate that CTCF is a common determinant to different pathways of death signaling in immature B cells.
...
PMID:CTCF functions as a critical regulator of cell-cycle arrest and death after ligation of the B cell receptor on immature B cells. 1252 57
Lung tumors from AC3F1 mice treated with aflatoxin B(1) (AFB(1)), were examined for loss of alleles, point mutations and hypermethylation of CpG sites within the promoters of the two genes in the Ink4a/Arf gene locus. Loss of microsatellite alleles in the Ink4a/Arf region occurred in 22 of 74 (30%) AFB(1)-induced lung tumors. Fifty-one of 61 (83%) tumors had at least partial methylation of CpG sites within the p16Ink4a promoter-exon 1alpha region. At least partial methylation of CpG sites was observed in 43 of 49 (88%) tumors analyzed for p19Arf promoter hypermethylation, with methylation of identified transcription factor binding sites or consensus sequences occurring in 21 tumors (DMP1/Ets in two tumors, CTCF in four tumors, E2F in three tumors, Sp1 in 16 tumors). Two tumors contained point mutations in the p19Arf promoter. Nuclear staining for
p19
(Arf) was decreased by 80-100% in 41 of 71 (58%) tumors. The concordance between p19Arf molecular perturbations and altered protein expression was 63%. However, upon comparing p19Arf promoter perturbations (i.e. methylation of functional transcription factor binding sites and point mutations) and altered
p19
(Arf) expression, the concordance was 86%, suggesting a mechanism for changes in protein expression in some tumors. There was an absence of a mutually exclusive relationship between disruption of
p53
and
p19
(Arf), since the concordance was 62%. Similarly, no evidence was found of inverse relationships between perturbation of p16Ink4a and
p19
(Arf) (43% concordance) or p16Ink4(a) and
p53
(37% concordance), suggesting that inactivation of these genes occurs independently and provides evidence that, although these genes may participate in cooperative cellular pathways, they also have functions in independent pathways that are important in mouse lung tumorigenesis.
...
PMID:Perturbations of the Ink4a/Arf gene locus in aflatoxin B1-induced mouse lung tumors. 1253 57
Senescence is generally defined as an irreversible state of G(1) cell cycle arrest in which cells are refractory to growth factor stimulation. In mouse embryo fibroblasts (MEFs), induction of senescence requires the presence of
p19
(ARF) and
p53
, as genetic ablation of either of these genes allows escape from senescence and leads to immortalization. We have developed a lentiviral vector that directs the synthesis of a
p53
-specific short hairpin transcript, which mediates stable suppression of
p53
expression through RNA interference. We show that suppression of
p53
expression in senescent MEFs leads to rapid cell cycle re-entry, is associated with loss of expression of senescence-associated genes, and leads to immortalization. These data indicate that senescence in MEFs is reversible and demonstrate that both initiation and maintenance of senescence is
p53
-dependent.
...
PMID:Reversal of senescence in mouse fibroblasts through lentiviral suppression of p53. 1255 91
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