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Query: EC:2.7.11.22 (
cdc2
)
8,319
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Overexpression of wild-type p53 protein has been shown to induce arrest in the G1 stage of the cell cycle and to transactivate expression of the gene that encodes the 21-kDa Waf1/Cip1 protein, a potent inhibitor of cyclin-dependent kinase activity. p53-dependent G1 arrest is accompanied by decreased expression of the B-myb gene, a relative of the c-myb cellular oncogene. In this study we show that B-myb expression is required for cells to progress from G1 into S phase and that high levels of ectopic B-myb expression uncoupled from cell cycle regulation rescues cells from p53-induced G1 arrest even in the presence of Waf1/Cip1 transactivation and inhibition of cyclin E/
Cdk2
kinase activity. Cotransfection experiments with p53 expression plasmids and expression plasmids encoding in-frame deletion mutations in B-myb coding sequences indicate that the DNA-binding domain of the
B-Myb
protein is required for this activity. These results provide evidence of a bypass of p53-induced Waf1/Cip1-mediated cell cycle regulatory pathways by a member of the myb oncogene family.
...
PMID:Constitutive expression of B-myb can bypass p53-induced Waf1/Cip1-mediated G1 arrest. 793 41
Previous studies revealed that transcription of
B-Myb
, which encodes a transcription factor related to the c-Myb proto-oncoprotein, is cell-cycle regulated by an E2F transcription factor-mediated repression mechanism operating in G0/G1. To begin to determine the consequences of transcriptional regulation on
B-Myb
function, we report here further studies of
B-Myb
protein expression in the cell cycle. We found that G0-arrest of serum-deprived mouse fibroblasts was achieved without significant reduction in
B-Myb
levels, moreover, over-expression of
B-Myb
in stably transfected cells did not prevent their entry into G0. Following serum-induction of arrested fibroblasts,
B-Myb
abundance increased as cells entered S phase to levels significantly greater than found in cycling cells. This was accompanied by the appearance of a novel phosphorylated form of
B-Myb
(112 kDa) of distinctly lower electrophoretic mobility than
B-Myb
present in G1 (110 kDa). The 112 kDa species was S phase-specific even in transfected cells overexpressing
B-Myb
. Consistent with modification in the S phase of the cell cycle, preliminary evidence suggested that a cyclin A/
cdk2
, but not cyclin E/
cdk2
or cyclin D1/
cdk4
, complex could induce a similar electrophoretic mobility change in baculovirus-specified
B-Myb
. These findings show that
B-Myb
expression may be subject to two levels of control during the cell cycle, transcription and protein phosphorylation.
...
PMID:Cell-cycle regulation of B-Myb protein expression: specific phosphorylation during the S phase of the cell cycle. 864 45
Transcription of the
B-Myb
gene is cell cycle regulated by an E2F-dependent mechanism and its product,
B-Myb
, is itself a transcription factor required for S-phase entry. Previously, we have shown that
B-Myb
is specifically phosphorylated during S-phase and that similar modification to a less electrophoretically mobile form could be induced by baculovirus-expressed cyclin A/
Cdk2
kinase. We report here that cyclin A-mediated phosphorylation of
B-Myb
is associated with a marked increase in transactivation function in U-2 OS cells. In contrast to previous studies, transactivation of the luciferase reporter was dependent upon Myb binding sites located upstream of the promoter. Enhancement of
B-Myb
activation function was also obtained by truncation of the C-terminus just downstream of a domain conserved in evolution. Potentiation of
B-Myb
activity by phosphorylation was not simply a consequence of overcoming the negative effect of the C-terminus, however, as the truncated protein was to a lesser extent also activated by cyclin A/
Cdk2
. Whereas wild-type
B-Myb
transactivation activity could not be potentiated by cyclin A/
Cdk2
in NIH3T3 cells, the truncated protein was hyperactive. Finally, we showed that
B-Myb
synergises with cyclin A to promote U-2 OS cells into S-phase.
...
PMID:B-Myb function can be markedly enhanced by cyclin A-dependent kinase and protein truncation. 918 59
Expression of the
B-Myb
transcription factor is upregulated during late G1 phase of the cell cycle by an E2F-dependent transcriptional mechanism.
B-Myb
is specifically phosphorylated during S phase, suggesting that a cyclin-dependent kinase (Cdk) regulates its activity. Consistent with this notion, the S phase-specific cyclin A/
Cdk2
was found previously to enhance
B-Myb
transactivation activity in cotransfected cells. In this study we provide evidence that
B-Myb
is a direct physiological target for cyclin A/
Cdk2
. We demonstrate that
B-Myb
is an in vitro substrate for cyclin A/
Cdk2
, but not for cyclin D1/Cdk4 or cyclin E/
Cdk2
. By mutating candidate
Cdk2
phosphorylation sites, we show that
B-Myb
is phosphorylated at Thr447, Thr490, Thr497 and Ser581 by cyclin A/
Cdk2
in vitro and that these sites are also phosphorylated in cycling U-2 OS cells. Inhibition of endogenous
Cdk2
by dominant negative
Cdk2
attenuated phosphorylation of Thr447, Thr490 and Thr497, but had no effect upon Ser581 modification.
B-Myb
transactivation activity was significantly reduced in a mutant containing amino acid substitutions at all four identified cyclin A/
Cdk2
sites and was constitutively low in Saos-2 cells where endogenous cyclin A/
Cdk2
activity was unable to phosphorylate ectopically expressed
B-Myb
. These data indicate that phosphorylation by cyclin A/
Cdk2
is directly involved in enhancing
B-Myb
transactivation activity and that levels of endogenous cyclin A/
Cdk2
activity may contribute to cell line-specific
B-Myb
function.
...
PMID:The cell-cycle regulated transcription factor B-Myb is phosphorylated by cyclin A/Cdk2 at sites that enhance its transactivation properties. 984 Sep 32
B-myb is a highly conserved member of the myb proto-oncogene family that encodes a ubiquitously expressed 110-kDa sequence-specific DNA-binding protein. Transactivation of Myb-inducible promoters by
B-Myb
is repressed by a regulatory domain located at the C-terminus of the protein. Cyclin A/
Cdk2
-mediated phosphorylation apparently releases the negative constraint and triggers
B-Myb
transactivation potential. Two-dimensional tryptic phosphopeptide analysis indicated that the majority of the sites phosphorylated in vivo are targeted in vitro by cyclin A/
Cdk2
. Six sites in
B-Myb
fulfil the requirements for recognition by
Cdk2
. Using point mutation of the phosphorylation sites to nonphosphorylatable amino acids, we show that five of these sites are targets for
Cdk2
in vivo. Mutation of one of these residues (T524) to alanine diminished the ability of
B-Myb
to promote transcription of a reporter gene, suggesting that phosphorylation of
B-Myb
at this site is important for the regulation of its activity by cyclin A/
Cdk2
.
...
PMID:Identification of cyclin A/Cdk2 phosphorylation sites in B-Myb. 1009 72
The transcription factor B-Myb is a cell cycle-regulated phosphoprotein and a potent regulator of cell cycle progression. Previous studies demonstrated that
B-Myb
was phosphorylated at the onset of S phase, suggesting that it could be due to cyclin-dependent kinases. We identified 10
B-Myb
phosphorylation sites by automated peptide radiosequencing of tryptic phosphopeptides derived from in vivo (32)P-labeled
B-Myb
. Each
B-Myb
phosphorylation site contained a phosphoserine or phosphothreonine followed by a proline, suggesting that this phosphorylation is due to a proline-directed kinase. Cyclin A-
Cdk2
and cyclin E-
Cdk2
complexes each phosphorylated
B-Myb
in a cell-free system on the same sites as in intact cells. Furthermore, the ability of
B-Myb
to activate a reporter plasmid was enhanced by the cotransfection of cyclin A, whereas mutagenesis of the 10 identified phosphorylation sites from
B-Myb
blocked the effect of cyclin A coexpression. Additional analysis revealed that the effect of phosphorylation on
B-Myb
transactivation potential was enhanced by phosphorylation sites in its carboxyl-terminal half. One phosphorylation site (Ser(581)) appeared to negatively regulate DNA binding, as mutation of this site enhanced the ability of
B-Myb
to bind a Myb-binding sequence. These data suggest that
B-Myb
is a target for phosphorylation by cyclin-
Cdk2
and that phosphorylation of
B-Myb
regulates its transcriptional activity.
...
PMID:Phosphorylation of B-Myb regulates its transactivation potential and DNA binding. 1059 81
Evidence obtained during recent years suggests that
B-Myb
, a highly conserved member of the Myb transcription factor family, plays a key role in cell proliferation. We have shown previously that the activity of
B-Myb
is stimulated by cyclin A/
Cdk2
-dependent phosphorylation of the carboxyl-terminus of
B-Myb
. We have now investigated in more detail the effect of other cyclins on
B-Myb
. Here, we show that cyclin D1, in contrast to cyclin A, strongly inhibits the activity of
B-Myb
. This inhibitory effect does not involve increased phosphorylation of
B-Myb
but seems to rely on the formation of a specific complex of
B-Myb
and cyclin D1. Our work identifies
B-Myb
as an interacting partner for cyclin D1 and suggest that the activity of
B-Myb
during the cell cycle is controlled by the antagonistic effects of cyclin D1 and A. The results presented here suggest a more general role of cyclin D1 as regulator of transcription in addition to the known effect on RB phosphorylation.
...
PMID:Regulation of B-Myb activity by cyclin D1. 1064 9
Expression of the
B-Myb
transcription factor is directed by an E2F-dependent transcriptional mechanism to late G1 and S phases of the cell cycle, where its transactivation properties are enhanced post-translationally by cyclin A/
Cdk2
-mediated phosphorylation. Other experiments have shown that removal of the
B-Myb
C-terminus constitutively activates both transactivation and DNA-binding activities, suggesting that autoregulation by this inhibitory domain is counteracted by phosphorylation. We report here on further experiments to examine this hypothesis. The importance of this modification was first emphasized by showing that co-transfected dominant-negative
Cdk2
(Cdk2DN) substantially reduced
B-Myb
transactivation activity. We then attempted to map the autoregulatory domain by analysing a series of progressively deleted C-terminal
B-Myb
mutants. Removal of just 29 C-terminal aa increased transactivation appreciably, however, maximal activity required removal of 143 amino acids (as in
B-Myb
+ 561). Enhanced
B-Myb
+ 561 function correlated with the acquisition of DNA binding activity to a single Myb binding site (MBS) oligonucleotide as determined by bandshift assays, however, further assays showed that even wt
B-Myb
could bind a DNA fragment containing three MBS. Although transactivation by
B-Myb
was severely dependent on hyperphosphorylation, neither inhibiting this activity by co-transfecting Cdk2DN nor augmenting it with cyclin A resulted in significant effects on DNA-binding. We also found that
B-Myb
could synergize with the CBP coactivator and that this cooperativity was cyclin A/
Cdk2
-dependent. Despite this, the physical association between these proteins was not influenced by the
B-Myb
phosphorylation status. We discuss these findings in relation to the autoregulation of
B-Myb
by the C-terminal domain.
...
PMID:Inhibition of cyclin A/Cdk2 phosphorylation impairs B-Myb transactivation function without affecting interactions with DNA or the CBP coactivator. 1142 88
The
B-Myb
transcription factor has been implicated in coordinating the expression of genes involved in cell cycle regulation. Although it is expressed in a ubiquitous manner, its transcriptional activity is repressed until the G(1)-S phase of the cell cycle by an unknown mechanism. In this study we used biochemical and cell-based assays to demonstrate that the nuclear receptor corepressors N-CoR and SMRT interact with
B-Myb
. The significance of these
B-Myb
-corepressor interactions was confirmed by the finding that
B-Myb
mutants, which were unable to bind N-CoR, exhibited constitutive transcriptional activity. It has been shown previously that phosphorylation of
B-Myb
by
cdk2
/cyclin A enhances its transcriptional activity. We have now determined that phosphorylation by
cdk2
/cyclin A blocks the interaction between
B-Myb
and N-CoR and that mutation of the corepressor binding site within
B-Myb
bypasses the requirement for this phosphorylation event. Cumulatively, these findings suggest that the nuclear corepressors N-CoR and SMRT serve a previously unappreciated role as regulators of
B-Myb
transcriptional activity.
...
PMID:The transcription factor B-Myb is maintained in an inhibited state in target cells through its interaction with the nuclear corepressors N-CoR and SMRT. 1199 3
B-Myb
is a cell-cycle regulated transcription factor which is implicated in cell proliferation and has an essential role in early embryonic development. In this study we examined the functions of
B-Myb
required to overcome G1 arrest in Saos-2 cells induced by the retinoblastoma-related p107 protein. Our results demonstrated that this activity was independent of
B-Myb
transactivation function, but correlated with its capacity to form an in vivo complex with p107. A large proportion of
B-Myb
formed complexes with p107 in cotransfected cells, however,
B-Myb
bound weakly to the related p130 protein and not at all to pRb. In contrast to the E2F transcription factors, which bind the p107 C-terminal pocket domain,
B-Myb
recognizes an N-terminal p107 region which overlaps the larger cyclin-binding domain.
B-Myb
and cyclin A2 formed mutually exclusive complexes with p107, and
B-Myb
enhanced the activity of co-transfected
cyclin E kinase
activity, implying that
B-Myb
affects the cell cycle by preventing sequestration of active cyclin/
cdk2
complexes. This study defines a novel function of
B-Myb
and further suggests that the p107 N-terminus provides an interaction domain for transcription factors involved in cell cycle control.
...
PMID:B-Myb overcomes a p107-mediated cell proliferation block by interacting with an N-terminal domain of p107. 1243 43
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