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Query: UNIPROT:P04637 (
p53
)
77,613
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
p300 and the closely related
CREB binding protein
(
CBP
) are transcriptional adaptors that are present in intracellular complexes with TATA binding protein (TBP) and bind to upstream activators including
p53
and nuclear hormone receptors. They have intrinsic and associated histone acetyltransferase activity, suggesting that chromatin modification is an essential part of their role in regulating transcription. Detailed characterization of a panel of antibodies raised against p300/
CBP
has revealed the existence of a 270-kDa cellular protein, p270, distinct from p300 and
CBP
but sharing at least two independent epitopes with p300. The subset of p300/
CBP
-derived antibodies that cross-reacts with p270 consistently coprecipitates a series a cellular proteins with relative molecular masses ranging from 44 to 190 kDa. Purification and analysis of various proteins in this group reveals that they are components of the human SWI/SNF complex and that p270 is an integral member of this complex.
...
PMID:p300/CREB binding protein-related protein p270 is a component of mammalian SWI/SNF complexes. 958
Human T-cell lymphotropic/leukemia virus type 1 (HTLV-1) transforms human T cells in vitro, and Tax, a potent transactivator of viral and cellular genes, plays a key role in cell immortalization. Tax activity is mediated by interaction with cellular transcription factors including members of the CREB/ATF family, the NF-kappaB/c-Rel family, serum response factor, and the coactivators
CREB binding protein
-p300. Although
p53
is usually not mutated in HTLV-1-infected T cells, its half-life is increased and its function is impaired. Here we report that transient coexpression of
p53
and Tax results in the suppression of
p53
transcriptional activity. Expression of Tax abrogates
p53
-induced G1 arrest in the Calu-6 cell line and prevents the apoptosis induced by overexpressing
p53
in the HeLa/Tat cell line. The Tax mutants M22 and G148V, which selectively activate the CREB/ATF pathway, exert these same biological effects on
p53
function. In contrast, the NF-kappaB-active Tax mutant M47 has no effect on
p53
activity in any of these systems. Consistent with the negative effect of Tax on
p53
, no activity on a
p53
-responsive promoter was observed upon transfection of HTLV-1-infected T-cell lines. The
p53 protein
is expressed at high levels in the nucleus, and nuclear extracts of HTLV-1-infected T cells bind constitutively to a DNA oligonucleotide containing the
p53
response element, indicating that Tax does not interfere with
p53
binding to DNA. Tax is able to suppress the transactivation function of
p53
in three different cell lines, and this suppression required Tax-mediated activation of the CREB/ATF, but not the NF-kappaB/c-Rel, pathway. Tax and the active Tax mutants were able to abrogate the G1 arrest and apoptosis induced by
p53
, and this effect does not correlate with an altered localization of nuclear
p53
or with the disruption of
p53
-DNA complexes. The suppression of
p53
activity by Tax could be important in T-cell immortalization induced by HTLV-1.
...
PMID:Human T-cell lymphotropic/leukemia virus type 1 Tax abrogates p53-induced cell cycle arrest and apoptosis through its CREB/ATF functional domain. 976 30
The proliferating cell nuclear antigen (PCNA) is a highly conserved cellular protein that functions both in DNA replication and in DNA repair. Exposure of a rat embryo fibroblast cell line (CREF cells) to gamma radiation induced simultaneous expression of PCNA with the
p53 tumor suppressor protein
and the cyclin-dependent kinase inhibitor p21(WAF1/Cip1). PCNA mRNA levels transiently increased in serum-starved cells exposed to ionizing radiation, an observation suggesting that the radiation-associated increase in PCNA expression could be dissociated from cell cycle progression. Irradiation of CREF cells activated a transiently expressed PCNA promoter chloramphenicol acetyltransferase construct through
p53
binding sequences via a mechanism blocked by a dominant negative mutant p53. Electrophoretic mobility shift assays with nuclear extracts prepared from irradiated CREF cells produced four
p53
-specific DNA-protein complexes with the PCNA
p53
binding site. Addition of monoclonal antibody PAb421 (p53-specific) or AC238 (specific to the transcriptional coactivator p300/
CREB binding protein
) to the mobility shift assay distinguished different forms of
p53
that changed in relative abundance with time after irradiation. These findings suggest a complex cellular response to DNA damage in which
p53
transiently activates expression of PCNA for the purpose of limited DNA repair. In a population of nongrowing cells with diminished PCNA levels, this pathway may be crucial to survival following DNA damage.
...
PMID:p53-mediated regulation of proliferating cell nuclear antigen expression in cells exposed to ionizing radiation. 985 27
The
p53 tumor suppressor protein
is a sequence-specific transcription factor that modulates the response of cells to DNA damage. Recent studies suggest that full transcriptional activity of
p53
requires the coactivators
CREB binding protein
(
CBP
)/p300 and PCAF. These coactivators interact with each other, and both possess intrinsic histone acetyltransferase activity. Furthermore, p300 acetylates
p53
to activate its sequence-specific DNA binding activity in vitro. In this study, we demonstrate that PCAF also acetylates
p53
in vitro at a lysine residue distinct from that acetylated by p300 and thereby increases
p53
's ability to bind to its cognate DNA site. We have generated antibodies to acetylated
p53
peptides at either of the two lysine residues that are targeted by PCAF or p300 and have demonstrated that these antibodies are highly specific for both acetylation and the particular site. Using these antibodies, we detect acetylation of these sites in vivo, and interestingly, acetylation at both sites increases in response to DNA-damaging agents. These data indicate that site-specific acetylation of
p53
increases under physiological conditions that activate
p53
and identify
CBP
/p300 and PCAF as the probable enzymes that modify
p53
in vivo.
...
PMID:p53 sites acetylated in vitro by PCAF and p300 are acetylated in vivo in response to DNA damage. 989 Oct 54
The pleiotropic cellular coactivator
CREB binding protein
(
CBP
) plays a critical role in supporting
p53
-dependent tumor suppressor functions.
p53
has been shown to directly interact with a carboxyl-terminal region of
CBP
for recruitment of the coactivator to
p53
-responsive genes. In this report, we identify the KIX domain as a new
p53
contact point on
CBP
. We show that both recombinant and endogenous forms of
p53
specifically interact with KIX. We demonstrate that the activation domain of
p53
participates in KIX binding and provide evidence showing that this interaction is critical for
p53
transactivation function. The human T-cell leukemia virus, type-I-encoded oncoprotein Tax is a well established repressor of
p53
transcription function. Like
p53
, Tax also binds to KIX. The finding that both transcription factors bind to a common region of
CBP
suggests that coactivator competition may account for the observed repression. We demonstrate reciprocal repression between Tax and
p53
in transient transfection assays, supporting the idea of intracellular coactivator competition. We biochemically confirm coactivator competition by directly showing that both transcription factors bind to KIX in a mutually exclusive fashion. These data provide molecular evidence for the observed intracellular competition and suggest that Tax inhibits
p53
function by abrogating a novel
p53
-KIX interaction. Thus, Tax competition for the
p53
-KIX complex may be a pivotal event in the human T-cell leukemia virus, type I transformation pathway.
...
PMID:Binding of p53 to the KIX domain of CREB binding protein. A potential link to human T-cell leukemia virus, type I-associated leukemogenesis. 1047 88
Recent studies have implicated acetylation of several nuclear proteins such as histones and
p53
on their epsilon-portion of lysine residues in eukaryotic transcription. Here we raised a specific polyclonal antibody against epsilon-acetylated lysine. Using the antibody, we detected hypernuclear acetylation (HNA) in atherosclerotic vascular smooth muscle cells (VSMCs). Thrombin, a humoral factor known to cause activation and proliferation of VSMCs, strongly potentiated HNA in cultured VSMCs. MAP kinase pathway and a signal coactivator
CREB binding protein
(
CBP
) were involved in thrombin-induced HNA of VSMCs. Our results suggest that coactivators cooperating with signal-dependent transcription activators play an important role in atherosclerogenesis via HNA in VSMCs.
...
PMID:Hypernuclear acetylation in atherosclerotic lesions and activated vascular smooth muscle cells. 1060 May 18
The newly identified p53 homolog p73 mimics the transcriptional function of
p53
. We have investigated the regulation of p73's transcriptional activity by p300/
CREB binding protein
(
CBP
). p73-p300 complexes were identified in HeLa cell extracts by cofractionation and coimmunoprecipitation assays. The p73-p300 interaction was confirmed in vitro by glutathione S-transferase-protein association assays and in vivo by coimmunoprecipitating the overexpressed p300 and p73 in human
p53
-free small-cell lung carcinoma H1299 or osteosarcoma Saos-2 cells. The N terminus but not the N-terminal truncation of p73 bound to the CH1 domain (amino acids [aa] 350 to 450) of p300/
CBP
. Accordingly, this p73 N-terminal deletion was unable to activate transcription or to induce apoptosis. Overexpression of either p300 or
CBP
stimulated transcription mediated by p73 but not its N-terminally deleted mutant in vivo. The N-terminal fragment from aa 19 to 597, but not the truncated fragment from aa 242 to 1700 of p300, reduced p73-mediated transcription markedly. p73-dependent transcription or apoptosis was partially impaired in either p300- or
CBP
-deficient human breast carcinoma MCF-7 or H1299 cells, suggesting that both coactivators mediate transcription by p73 in cells. These results demonstrate that the N terminus of p73 directly interacts with the N-terminal CH1 domain of p300/
CBP
to activate transcription.
...
PMID:The N-terminal domain of p73 interacts with the CH1 domain of p300/CREB binding protein and mediates transcriptional activation and apoptosis. 1064 16
The transcriptional coactivators p300 and
CREB binding protein
(
CBP
) are important regulators of the cell cycle, differentiation, and tumorigenesis. Both p300 and
CBP
are targeted by viral oncoproteins, are mutated in certain forms of cancer, are phosphorylated in a cell cycle-dependent manner, interact with transcription factors such as
p53
and E2F, and can be found complexed with cyclinE-Cdk2 in vivo. Moreover, p300-deficient cells show defects in proliferation. Here we demonstrate that transcriptional activation by both p300 and
CBP
is stimulated by coexpression of the cyclin-dependent kinase inhibitor p21(WAF/CIP1). Significantly this stimulation is independent of both the inherent histone acetyltransferase (HAT) activity of p300 and
CBP
and of the previously reported carboxyl-terminal binding site for cyclinE-Cdk2. Rather, we describe a previously uncharacterized transcriptional repression domain (CRD1) within p300. p300 transactivation is stimulated through derepression of CRD1 by p21. Significantly p21 regulation of CRD1 is dependent on the nature of the core promoter. We suggest that CRD1 provides a novel mechanism through which p300 and
CBP
can switch activities between the promoters of genes that stimulate growth and those that enhance cell cycle arrest.
...
PMID:A novel transcriptional repression domain mediates p21(WAF1/CIP1) induction of p300 transactivation. 1073 70
CREB binding protein
(
CBP
) is a 270-kDa nuclear protein required for activated transcription of a large number of cellular genes. Although
CBP
was originally discovered through its interaction with phosphorylated CREB (pCREB), it is utilized by a multitude of cellular transcription factors and viral oncoproteins. Both CREB and the
tumor suppressor p53
have been shown to directly interact with the KIX domain of
CBP
. Although coactivator competition is an emerging theme in transcriptional regulation, we have made the fortuitous observation that protein kinase A-phosphorylated CREB strongly enhances
p53
association with KIX. Phosphorylated CREB also facilitates interaction of a
p53
mutant, defective for KIX binding, indicating that CREB functions in a novel way to bridge
p53
and the coactivator. This is accomplished through direct interaction between the bZIP domain of CREB and the amino terminus of
p53
; a protein-protein interaction that is also detected in vivo. Consistent with our biochemical observations, we show that stimulation of the intracellular cyclic AMP (cAMP) pathway, which leads to CREB phosphorylation, strongly enhances both the transcriptional activation and apoptotic properties of
p53
. We propose that phosphorylated CREB mediates recruitment of
CBP
to
p53
-responsive promoters through direct interaction with
p53
. These observations provide evidence for a novel pathway that integrates cAMP signaling and
p53
transcriptional activity.
...
PMID:p53 recruitment of CREB binding protein mediated through phosphorylated CREB: a novel pathway of tumor suppressor regulation. 1084 10
The non-structural protein NS1, encoded by the parvovirus minute virus of mice (MVM), is a potent regulator of viral gene expression in addition to prominent roles in viral replication and cytopathic effects associated with parvoviral infection. Although NS1 involves the modulation of viral and cellular transcription, the primary activation mechanism of MVM NS1 remains unclear. In the present study, we show here that the coactivator
CREB binding protein
, CBP, could potentiate NS1-mediated transcription as measured on the P38 promoter, which drives expression of the MVM capsid genes. NS1 bound to the two related cysteine-histidine-rich regions of CBP, referred to as C/H1 and C/H3, the former of which has an antagonistic function to CBP upon the NS1-transactivation. Furthermore, NS1 inhibited the synergistic transactivation by CBP and
p53
. These findings suggested that CBP as a transcriptional coactivator is required for NS1-mediated viral and cellular transcription in parvovirus-infected cells, resulting in cell proliferation and differentiation to achieve its lytic cycle.
...
PMID:Effects of interaction between parvovirus minute virus of mice NS1 and coactivator CBP on NS1- and p53-transactivation. 1111 8
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