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Query: UNIPROT:P04637 (
p53
)
77,613
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
The activity of the
tumor suppressor protein p53
is controlled by a balance between E3-ligase mediated
p53 protein
degradation and protein kinase-mediated assembly of
p53
:p300 transcription machinery. Genetic studies in mice have shown that mutation of the
CK2
phospho-acceptor site in
p53
increases UV-induced skin cancer formation,(11) highlighting an unexpected role for
p53
phosphorylation in mediating
p53
-dependent tumor suppression. However, it is not known in which cell types
CK2
-mediated phosphorylation of
p53
occurs. Using human skin as a model to determine whether there is cell-selectivity in modulating
p53
phosphorylation, we have found a selective induction of
p53
phosphorylation at the
CK2
-site in the basal cells of UV irradiated human skin. Dual-immunofluorescence also revealed that Ser392 and Ser15 phosphorylation of
p53
also occur in the same basal cells, although often within distinct regions of the nucleus. Given that p63alphaDeltaN is required for
p53
activation after DNA damage, we examined and found a high proportion of cells co-express p63alphaDeltaN and
CK2
-phosphorylated
p53
after UV-irradiation. As controls, the proliferation marker Ki67 and p63alphaDeltaN generally exhibit mutually exclusive expression. These data identify a physiological model with which to identify signaling pathways that mediate cross-talk between p63alphaDeltaN and activating
p53
kinase pathways after DNA damage in basal cell populations.
...
PMID:CK2-site phosphorylation of p53 is induced in DeltaNp63 expressing basal stem cells in UVB irradiated human skin. 1710 55
The La protein interacts with a variety of small RNAs as well as certain growth-associated mRNAs such as Mdm2 mRNA. Human La (hLa) phosphoprotein is so highly conserved that it can replace the tRNA processing function of the fission yeast La protein in vivo. We used this system, which is based on tRNA-mediated suppression (TMS) of ade6-704 in S. pombe, to compare the activities of mouse and human La proteins. Prior studies indicate that hLa is activated by phosphorylation of serine-366 by
protein kinase CK2
, neutralizing a negative effect of a short basic motif (SBM). First, we report the sequence mapping of the UGA stop codon that requires suppressor tRNA for TMS, to an unexpected site in S. pombe ade6-704. Next, we show that, unlike hLa, native mLa is unexpectedly inactive for TMS, although its intrinsic activity is revealed by deletion of its SBM. We then show that mLa is not phosphorylated by
CK2
, accounting for the mechanistic difference between mLa and hLa. We found a PKA/PKG target sequence in mLa (S199) that is not present in hLa, and show that PKA/PKG efficiently phosphorylates mLa S199 in vitro. A noteworthy conclusion that comes from this work is that this fission yeast system can be used to gain insight into differences in control mechanisms used by La proteins of different mammalian species. Finally, RNA binding assays indicate that while mutation of mLa S199 has little effect on pre-tRNA binding, it substantially decreases binding to a probe derived from Mdm2 mRNA. In closing, we note that species-specific signaling through La may be relevant to the La-dependent Mdm2 pathways of
p53
metabolism and cancer progression in mice and humans.
...
PMID:Mouse and human La proteins differ in kinase substrate activity and activation mechanism for tRNA processing. 1825 91
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
Cellular senescence is a potent anti-cancer mechanism controlled by tumor suppressor genes, particularly
p53
and pRb, which is characterized by the irreversible loss of proliferation. Senescence induced by DNA damage, oncogenic stimulation, or excessive mitogenic input, serves as a barrier that counteracts cancer progression. Emerging evidence in cellular and in in vivo models revealed the involvement of additional signaling players in senescence, including PML,
CK2
, Bcl-2, PI3K effectors such as Rheb, Rho small GTPases, and cytokines. Recent studies have also implicated protein kinase C (PKC) isozymes as modulators of senescence phenotypes and showed that phorbol esters, widely used PKC activators, can induce senescence in a number of cancer cells. These novel findings suggest a complex array of cross-talks between senescence pathways and may have significant implications in cancer therapy.
...
PMID:Hallmarks for senescence in carcinogenesis: novel signaling players. 1916 23
SIRT1, an NAD(+) (nicotinamide adenine dinucleotide)-dependent deacetylase, protects cells from stress-induced apoptosis, and its orthologues delay aging in lower eukaryotes. SIRT1 increases survival in response to stress such as DNA damage by deacetylating a number of substrates including pro-apoptotic protein
p53
. The molecular mechanism by which DNA-damage activates SIRT1 is not known. By screening a kinase inhibitor library, we identified
CK2
as a SIRT1 kinase.
CK2
is a pleiotropic kinase with more than 300 substrates and well-known anti-apoptotic and pro-growth activities. We find that
CK2
is recruited to SIRT1 after ionizing radiation (IR) and phosphorylates conserved residues Ser 154, 649, 651 and 683 in the N- and C-terminal domains of mouse SIRT1. Phosphorylation of SIRT1 increases its deacetylation rate but not if the four Ser residues are mutated. In addition, phosphorylation of SIRT1 increases its substrate-binding affinity.
CK2
-mediated phosphorylation increases the ability of SIRT1 to deacetylate
p53
and protect cells from apoptosis after DNA damage. Based on these findings, we propose that
CK2
protects against IR-induced apoptosis partly by phosphorylating and activating SIRT1. Thus, this work suggests that SIRT1 is a component of the expansive anti-apoptotic network controlled by
CK2
. Since expression of both
CK2
and SIRT1 is upregulated with tumorigenesis and downregulated with senescence, the
CK2
-SIRT1 link sheds new light on how
CK2
may regulate cancer development and aging.
...
PMID:CK2 is the regulator of SIRT1 substrate-binding affinity, deacetylase activity and cellular response to DNA-damage. 1968 May 52
Human mesenchymal stem cells (hMSC) are critical for tissue regeneration. How hMSC respond to genotoxic stresses and potentially contribute to aging and cancer remain underexplored. We showed that ionizing radiation induced cellular senescence of hMSC over a period of 10 days, showing a critical transition between days 3 and 6. This was confirmed by senescence-associated beta-galactosidase staining, protein expression profiles of key cell cycle regulators (retinoblastoma protein,
p53
, p21(waf1/Cip1), and p16(INK4A)), and senescence-associated secretory phenotypes (interleukin-8, interleukin-12, GRO, and MDC). We observed dramatic cytoskeletal reorganization of hMSC through reduction of myosin-10, redistribution of myosin-9, and secretion of profilin-1. Using a SILAC-based phosphoproteomics method, we detected significant reduction of myosin-9 phosphorylation at Ser(1943), coinciding with its redistribution. Importantly, through treatment with cell-permeable inhibitors (4,5,6,7-tetrabromo-1H-benzotriazole and 2-dimethylamino-4,5,6,7-tetrabromo-1H-benzimidazole) and gene knockdown using RNA interference, we identified
CK2
, a kinase responsible for myosin-9 phosphorylation at Ser(1943), as a key factor contributing to the radiation-induced senescence of hMSC. We showed that individual knockdown of
CK2
catalytic subunits CK2alpha and CK2alpha' induced hMSC senescence. However, only knockdown of CK2alpha resulted in morphologic phenotypes resembling those of radiation-induced senescence. These results suggest that CK2alpha and CK2alpha' play differential roles in hMSC senescence progression, and their relative expression might represent a novel regulatory mechanism for
CK2
activity.
...
PMID:Protein kinase CK2 regulates cytoskeletal reorganization during ionizing radiation-induced senescence of human mesenchymal stem cells. 1982 41
We have previously shown that the down-regulation of protein kinase
CKII
activity is tightly associated with cellular senescence of human fibroblast IMR-90 cells. Here, we examined the roles of
p53
and p21(Cip1/WAF1) in senescence development induced by
CKII
inhibition using wild-type, isogenic
p53
-/- and isogenic p21-/- HCT116 human colon cancer cell lines. A senescent marker appeared after staining for senescence-associated beta-galactosidase activity in wild-type HCT116 cells treated with
CKII
inhibitor or CKIIalpha siRNA, but this response was almost abolished in
p53
- or p21(Cip1/WAF1)-null cells. Increased cellular levels of
p53
and p21(Cip1/WAF1) protein occurred with the inhibition of
CKII
.
CKII
inhibition upregulated
p53
and p21(Cip1/WAF1) expression at post-transcriptional level and transcription level, respectively. RB phosphorylation significantly decreased in cells treated with
CKII
inhibitor. Taken together, this study shows that the activation of the
p53
-p21(Cip1/WAF1) pathway acts as a major mediator of cellular senescence induced by
CKII
inhibition.
...
PMID:The p53-p21(Cip1/WAF1) pathway is necessary for cellular senescence induced by the inhibition of protein kinase CKII in human colon cancer cells. 1985 35
Post-translational modifications play important roles during the stabilisation and activation of
p53
by various genotoxic and non-genotoxic stresses. Ser392 has been reported to be a major UV-stimulated phosphorylation site that is modified through the p38 MAPK pathway in a manner that may involve recruitment of
CK2
. Here we show that phosphorylation of Ser392 is an integral event that occurs not only in response to UV, but also during the induction of
p53
by a range of stimuli including treatment of cells with the MDM2 inhibitor, Nutlin 3a. Strikingly, phosphorylation of Ser392 and Ser33 was also observed following induction of the
p53
pathway by ARF which has previously been thought to induce
p53
in a phosphorylation-independent manner. The induction of Ser392 phosphorylation by diverse stimuli can be explained by a common mechanism in which its phosphorylation at a low rate, coupled with the rapid turnover of
p53
, limits the accumulation of phosphorylated molecules until a stimulus stabilises
p53
and allows the Ser392-phosphorylated
p53
to accumulate. We also provide biological evidence that Ser392 phosphorylation is not mediated by a UV-associated route involving p38 MAPK, either directly or indirectly via
CK2
. These data suggest that, physiologically, Ser392 may be phosphorylated by an, as yet, unidentified protein kinase.
...
PMID:Phosphorylation of serine 392 in p53 is a common and integral event during p53 induction by diverse stimuli. 1993 75
We have shown that protein kinase
CKII
(
CKII
) inhibition induces senescence through the
p53
-dependent pathway in HCT116 cells. Here we examined the molecular mechanism through which
CKII
inhibition activates
p53
in HCT116 cells.
CKII
inhibition by treatment with
CKII
inhibitor or CKIIalpha small-interfering RNA (siRNA) increased intracellular hydrogen peroxide and superoxide anion levels. These effects were significantly blocked by pretreatment of cells with the antioxidant N-acetylcysteine. Additionally, NADPH oxidase (NOX) inhibitor apocynin and p22(phox) siRNA significantly reduced
p53
expression and suppressed the appearance of senescence markers.
CKII
inhibition did not affect mitochondrial superoxide generation. These data demonstrate that
CKII
inhibition induces superoxide anion generation via NOX activation, and subsequent superoxide-dependent activation of
p53
acts as a mediator of senescence in HCT116 cells after down-regulation of
CKII
.
...
PMID:NADPH oxidase is involved in protein kinase CKII down-regulation-mediated senescence through elevation of the level of reactive oxygen species in human colon cancer cells. 2062 41
The von Hippel-Lindau tumour suppressor gene encodes a protein with 213 amino acids, which is known to be part of an E3-ubiquitin ligase targeting the HIF-1alpha transcription factor as well as to form a complex with
p53
. The VHL protein can be phosphorylated by
protein kinase CK2
at serines 33, 38 and 43. However, the role of VHL phosphorylation in the context of
p53
and HIF-1alpha regulation remained so far unknown. In the present study we investigated whether phosphorylation of VHL by
CK2
might affect the function of
p53
and HIF-1alpha. By using 4,5,6,7-tetrabromobenzotriazole (TBB), a
CK2
-specific inhibitor, as well as a mutant VHL where serines 33, 38 and 43 were replaced by alanines we found that
CK2
phosphorylation affected the VHL protein half-life and increased VHL protein stability. Further, we found that inhibition of VHL phosphorylation by
CK2
reduced
p53
function. In addition, the enhanced levels of VHL due to
CK2
inhibition contributed to the down-regulation of HIF-activity and degradation of HIF-1alpha. Thus, these results demonstrate that phosphorylation of VHL by
CK2
plays an important role in the regulation of VHL protein stability and may contribute to the survival of tumour cells.
...
PMID:Phosphorylation of the von Hippel-Lindau protein (VHL) by protein kinase CK2 reduces its protein stability and affects p53 and HIF-1alpha mediated transcription. 2063 92
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