Previous Article | Next Article 
Molecular and Cellular Biology, August 1999, p. 5601-5607, Vol. 19, No. 8
Joslin Diabetes Center, Research Division,
Department of Cell Biology, Harvard Medical School, Boston,
Massachusetts 021381; Department of
Molecular Biology, The Skaggs Institute for Chemical Biology, The
Scripps Research Institute, La Jolla, California
920373; and Department of
Biochemistry2 and Department of
Experimental Oncology,4 St. Jude Children's
Research Hospital, Memphis, Tennessee 38105
Received 11 March 1999/Returned for modification 28 April
1999/Accepted 24 May 1999
We have examined structural differences between the proto-oncogene
c-Myb and the cyclic AMP-responsive factor CREB that underlie their
constitutive or signal-dependent activation properties. Both proteins
stimulate gene expression via activating regions that articulate with a
shallow hydrophobic groove in the KIX domain of the coactivator
CREB-binding protein (CBP). Three hydrophobic residues in c-Myb that
are conserved in CREB function importantly in cellular gene activation
and in complex formation with KIX. These hydrophobic residues are
assembled on one face of an amphipathic helix in both proteins, and
mutations that disrupt c-Myb or CREB helicity in this region block
interaction of either factor with KIX. Binding of the helical c-Myb
domain to KIX is accompanied by a substantial increase in entropy
that compensates for the comparatively low enthalpy of complex
formation. By contrast, binding of CREB to KIX entails a large entropy
cost due to a random coil-to-helix transition in CREB that accompanies
complex formation. These results indicate that the constitutive and
inducible activation properties of c-Myb and CREB reflect secondary
structural characteristics of their corresponding activating regions
that influence the thermodynamics of formation of a complex with CBP.
Gene-specific factors regulate
transcription via activating regions that interact with specific
targets in the RNA polymerase II (Pol II) machinery. Indeed, the
strength of an activating region appears to reflect its intrinsic
affinity for one or more such target proteins (20). But,
apart from a general abundance of certain amino acids such as proline,
glutamine, or acidic residues, no consensus motif for interaction with
any individual target has emerged.
Ideally, the identification of a motif that is conserved between
activating regions might best be approached with transcription factors
that associate with a common target in the Pol II apparatus. The Pol
II-associated coactivator CREB-binding protein (CBP) and its paralog
P300 (hereafter referred to as CBP/P300), for example, associate with a
number of activators via several interaction domains. One of these,
referred to as the KIX domain, has been shown to interact functionally
with the cyclic AMP-responsive factor CREB (12) as well as
with certain constitutive activators such as c-Myb (4),
SREBP (11), Stat-1 (22), Tax (9), and
cubitus interruptus (1). A three-helix structure that
contains a shallow hydrophobic groove, the KIX domain is highly
conserved in all species that express CBP/P300 homologues
(16). The functional importance of this domain for cellular
gene expression has been most extensively evaluated in the context of
cyclic AMP and CREB signaling.
CREB triggers target gene expression, following its protein kinase A
(PKA)-mediated phosphorylation at Ser133, via a kinase-inducible activation domain (KID) that binds to KIX (2, 12). Direct interactions between the Ser133 phosphate moiety and KIX account for
about half of the free energy of formation of a complex between KID and
KIX (13, 16). The Ser133 phosphate in KID forms a hydrogen
bond with Tyr658 and a salt bridge with Lys662 in KIX, and mutagenesis
of both Tyr658 and Lys662 reduces the affinity of
phospho(Ser133)KID for KIX about 1,000-fold.
Allosteric contributions from the Ser133 phosphate group also figure
prominently in this interaction. The phosphate moiety promotes
formation of an amphipathic helix in KID, termed The importance of KIX for target gene induction via numerous activators
suggests a common mode of binding, perhaps via a conserved motif, but
casual inspection of these activating regions does not reveal any
extensive sequence similarity to support that notion. The ability of
one domain in CBP to accommodate both constitutive and signal-dependent
factors has prompted us to compare the mechanisms underlying both types
of interactions, using c-Myb and CREB. Our results suggest that c-Myb-
and CREB-activating regions actually have limited sequence similarities
that reflect comparable surface interactions with the KIX domain;
however, they have remarkable differences in secondary structure that
potently affect the thermodynamics of complex formation. We propose
that these structural differences in c-Myb and CREB form the basis for
their constitutive and inducible activation properties.
Plasmids.
Wild-type and mutant KIX cDNAs were constructed by
PCR amplification and were cloned into a pGEX-LT vector. All KIX
proteins contained amino acids (aa) 586 through 672 of the murine CBP. Rous sarcoma virus (RSV)-CREB M1 (S133A) and RSV-CREB Mutagenesis.
Murine c-Myb point mutants were generated by
using Stratagene's Quickchange protocol, and mutations were confirmed
by DNA sequencing. Myb truncation mutants were made by PCR
amplification by using internal primers to c-Myb.
GST pulldown and fluorescence polarization assays.
GST-KIX
S/B fusion proteins were purified from Escherichia coli, and
glutathione S-transferase (GST) pulldown assays with 35S-labeled methionine-labeled in vitro-transcribed and
-translated c-Myb were performed as previously described
(21). About 20 µg of GST-KIX S/B was used per reaction.
Input levels of c-Myb (about 10,000 cpm) were checked by sodium dodecyl
sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) or by
trichloroacetic acid precipitation and scintillation counting and were
within ±15% of the level of wild-type c-Myb. Quantitation of
c-Myb following SDS-PAGE was performed with a Molecular Dynamics Storm
phosphorimager. For fluorescence anisotropy experiments, c-Myb (aa
276 through 315) and KID (aa 88 through 160) peptides were N-terminally
treated with fluorescein, and fluorescence polarization values were
obtained with wild-type and mutant KIX polypeptides by using a Pan Vera Beacon 2000 Variable-Temperature Fluorescence Polarization system (13). KIX proteins were added to samples containing
fluorescein-treated (fl) Myb or KID peptides (final concentration for
each, 5 to 16 nM), and binding assays were performed in a total volume
of 150 µl at 22°C after a 90-s delay with 16-s integration.
Transient-transfection assays.
For the mammalian two-hybrid
assays, COS-7 cells in 3.5-cm-diameter dishes were transfected with 0.5 µg of 5×Gal-Luc reporter plasmid, 0.5 µg of Gal-KIX S/B expression
plasmid, and 1.5 µg of RSV2×VP16-Myb, RSV-Myb, or pGR (RSV)
expression plasmid and 0.01 µg of pRL-SV40 (SV40, simian virus 40)
(Promega) by the calcium phosphate method. Cells were harvested after
approximately 23 h and assayed for luciferase derived from the
reporter. For c-Myb activity assays, 293 embryonal kidney cells in
3.5-cm-diameter dishes were transfected with 0.5 µg of reporter
plasmid, 0.5 µg of either pCMX-c-Myb, Gal-Myb 186-325, or Gal-Myb
290-315 expression vector, and 0.5 µg of RSV- ITC.
Isothermal titration of c-Myb (aa 291 to 315) (2.0 mM)
or pKID (aa 100 to 160) (0.3 mM) into KIX polypeptide (aa 586 to 672) (0.225 and 0.022 mM, respectively) was performed at 27°C in 50 mM
Tris (pH 7.0)-50 mM NaCl. The experiments were carried out by using an
MCS titration calorimeter from MicroCal, Inc. (Northampton, Mass.),
with a 250-µl injection syringe during stirring at 4,000 rpm. An
initial 1-µl injection was followed by 29 7-µl injections of pKID
or 28 10-µl injections of Myb. Integration of the thermogram and
subtraction of the blanks gave a binding isotherm that fitted best to a
model of one-site interaction. The data were fitted by using the
variables K (association constant), To determine whether CREB and c-Myb have a common KIX interaction
motif, we performed mammalian two-hybrid studies using a series of
nested fragments within the c-Myb activation domain. A c-Myb-VP16
fusion polypeptide containing residues in c-Myb that were previously
shown to associate with CBP (aa 211 to 360) (4) potently
stimulated Gal4 KIX activity on a cotransfected 5×Gal4 luciferase
reporter plasmid in COS-7 cells (Fig.
1A). Shorter polypeptides containing
residues 270 through 315 or 290 through 315 in c-Myb were also capable
of associating with KIX in two-hybrid assays, but c-Myb constructs
lacking those sequences were not (Fig. 1A). These experiments indicate
that residues 290 through 315 in c-Myb encode a minimal KIX binding
domain.
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Role of Secondary Structure in Discrimination
between Constitutive and Inducible Activators
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
B, in part by
stabilizing the helix macrodipole and also by hydrogen bonding with the
backbone Ser133 amide (16). Ser133 phosphorylation per se is
not sufficient to induce the helical transition in B, however;
complex formation with KIX is also required. Residues on the
hydrophobic face of helix B stabilize the helical transition via
contacts with a shallow hydrophobic groove in KIX.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
136-160 were
previously described (6, 7). 
411 CD13/APN Luc was previously described (18). 5×Gal-Luc (pGL-2/G5B) is
described elsewhere (8). Gal-KIX was constructed by
inserting a KIX cDNA fragment encoding CBP aa 553 through 679 into pM3
(17). Gal-Myb 186-325 was constructed by inserting a c-Myb
cDNA fragment into pM2 (17). pCMX c-Myb was constructed by
subcloning the full-length murine c-Myb cDNA from pRmb3Svneo into pCMX.
RSV2×VP16 Myb vectors were developed by ligating two repeats of VP16
in tandem into the RSV expression vector pGR. A c-Myb PCR fragment
(described below) was then inserted downstream of the VP16 sequences.
Other plasmids were constructed by using standard cloning techniques.
-Gal. After about
17 h cells were harvested and assayed for reporter plasmid-derived
luciferase activity. 411 CD13/APN Luc reporter was used to test pCMX
c-Myb activity, and 5×Gal-Luc reporter was used to test Gal-Myb
activity. F9 cell transfection assays to test CREB activity were
performed as previously described (3). Reporter gene-derived
luciferase or chloramphenicol acetyltransferase (CAT) activity was
normalized to an internal -galactosidase (RSV--Gal), luciferase
(RSV-Luc), or Renilla luciferase (pRL-SV40) control.
H
(enthalpy), and N (stoichiometric ratio), using the
isothermal titration calorimetry (ITC) data analysis software in ORIGIN
version 2.3 (MicroCal Software, Northampton, Mass.). G
and S were then obtained by the following basic
thermodynamic equations: G° = RTlnK = H° TS°. The minor
deviations of the stoichiometric ratio N from the
theoretical value of 1.0 (2% for pKID and 14% for Myb) were used to
correct H and K for concentration
determination errors. The C values (C = K × [KIX] × N) indicated that binding-constant
determination by ITC was very accurate for pKID (C = 60) and reasonably accurate for Myb (C = 10). Even
an unreasonably large error in the determination of K would
not change the sign of the calculated S.
RESULTS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
View larger version (15K):
[in a new window]
FIG. 1.
Characterization of a minimal transactivation domain in
c-Myb that binds to the KIX domain of CBP. (A) Mammalian two-hybrid
assays performed by using Gal4-KIX and c-Myb/VP16 expression vectors to
examine interactions of c-Myb with CBP. COS-7 cells were transfected
with 5×Gal4-Luc and pRL-SV40 Renilla luciferase reporters and with
expression vectors for Gal-KIX and 2×VP16-Myb fragments. The hatched
box represents the minimal KIX interaction domain of c-Myb encompassing
aa 290 to 315. Inclusive amino acid endpoints of c-Myb fragments fused
to tandem VP16 activation domains are indicated. Results are shown as
fold activation (mean ± standard deviation, n = 2) over that by empty RSV expression vector (without VP16-Myb).
c-Myb/VP16 polypeptides were expressed at comparable levels in
transfected cells (data not shown). Inclusive endpoints of c-Myb are
shown. (B) c-Myb (aa 290 to 315) stimulates target gene expression when
fused to the Gal4 DNA binding domain (DBD). 293 cells were transfected
with 5×Gal Luc and RSV- -Gal reporter plasmids as well as vectors
expressing Gal4 DBD or Gal-Myb (aa 290 to 315). Activity is reported as
fold activation over that by Gal DBD (mean ± standard deviation,
n = 3).
To evaluate the transcriptional activity of this region, we prepared a Gal4-cMyb construct containing c-Myb residues (aa 290 through 315) fused to the Gal4 DNA binding domain (aa 1 through 147). Following cotransfection with a 5×Gal4 luciferase reporter, the Gal-Myb (aa 290 through 315) polypeptide stimulated target gene activity in 293 cells sevenfold compared to the Gal4 DNA binding domain alone (Fig. 1B).
The ability of c-Myb (aa 290 through 315) to stimulate target gene activity and to bind to KIX prompted us to evaluate the functional importance of this region in the context of the full-length c-Myb protein by site-directed mutagenesis. Using a c-Myb-responsive reporter construct (CD13/APN), we identified three hydrophobic residues (Ile295, Leu298, and Leu302) that blocked target gene activation 70 to 90% when mutated individually to alanine (Fig. 2A). Alanine substitutions at basic or acidic residues within the same region (aa 290 to 315) had only minimal effects on c-Myb activity, however, suggesting that hydrophobic contacts with CBP are selectively required for target gene activation. The same three hydrophobic residues (Ile295, Leu298, and Leu302) also appear to function importantly in the context of a GAL4:c-Myb (186-325) polypeptide, arguing against nonspecific effects of these mutations on nuclear targeting or DNA binding activities of the full-length c-Myb protein (Fig. 2A). Indeed, mutant c-Myb polypeptides containing alanine substitutions at any of the three hydrophobic residues (Ile295, Leu298, and Leu302) were unable to interact efficiently with GST-KIX polypeptides in pulldown assays, indicating that target gene activation via these amino acids is CBP/P300 dependent (Fig. 2A and B).
|
2). The GST-KIX
pulldown data are presented as means ± standard deviations
(n = 3). Comparable expression of mutant c-Myb
polypeptides, either in the context of the full-length protein or as
GAL4-Myb chimeras, was verified by Western blot assay of transfected
cells (data not shown). (B) Top, representative autoradiogram obtained
following SDS-PAGE of 35S-labeled c-Myb proteins bound to
GST-KIX resin. Bottom, average input (40% of total, expressed as
counts per minute) for each c-Myb polypeptide. Data are expressed as
means ± standard deviations (n = 2). Bands of 84 and 85 kDa represent full-length c-Myb polypeptides. Although the
precise amino acid endpoints were not determined, the 65-kDa band
represents a C-terminally truncated c-Myb polypeptide extending through
the first 600 amino acids of c-Myb and containing the KIX binding
domain (aa 295 to 315). (C) Leu302 in c-Myb forms specialized contacts
with the KIX domain of CBP. The effects of conservative substitutions
at Leu298 and Leu302 in c-Myb on target gene activation and complex
formation with KIX are shown. Activities are shown as percentages of
that for WT c-Myb (hatched bars) or Gal4 Myb 186-325 (black bars)
polypeptides. Results from pulldown assays (see Fig. To evaluate the specificity with which hydrophobic residues in c-Myb
bind to KIX, we prepared mutant c-Myb polypeptides containing conservative substitutions at either Leu298 or Leu302. Mutagenesis of
Leu298 to isoleucine had a minimal impact on target gene activation or
formation of a complex with KIX in vitro, but a valine substitution at
the same position inhibited binding of mutant c-Myb to KIX 40% and
blocked reporter induction two- to fivefold (Fig. 2C). By contrast,
mutation of Leu302 to either isoleucine or valine compromised both
transactivation and KIX binding activities of c-Myb, suggesting that
Leu302 forms specialized contacts with KIX (Fig. 2C). In this regard,
the KIX binding domain of c-Myb has modest sequence similarity with the
B region of KID, particularly in the spacing of hydrophobic residues
that are critical for association with KIX (Fig.
3). In this alignment, Leu302 of c-Myb
should correspond to Leu141 in CREB, a critical residue that anchors
the KID domain by projecting into a deep hydrophobic pocket in KIX
(16).
|
The importance of a random coil-to-helix transition in the B region
of phospho(Ser133)KID for high-affinity interaction with KIX
(13) prompted us to examine whether the KIX binding domain in c-Myb also folds into a helical structure. Circular dichroism spectroscopy revealed that the helical content of this domain (aa 290 to 315), estimated by its 
222-nm/203-nm ratio, was about 30%
(Fig. 3). By contrast, the B region in KID (aa 128 to 147) was only
1% helical, reflecting the random coil structure of this peptide in
the unbound state (12) (Fig. 3). Helical wheel analysis of
the c-Myb (aa 290 to 315)-activating region indicates that this peptide
may form an amphipathic helix, with the three functionally important
hydrophobic residues (Ile295, Leu298, and Leu302) clustering on one
face and, like Tyr134, Ile137, and Leu141 in CREB, interacting with the
hydrophobic groove in KIX (Fig. 3).
The ability of c-Myb to form an amphipathic helix led us to examine the importance of helical structure for complex formation and for target gene activation. We selected residues in c-Myb (Leu301 and Glu299) that do not appear to form surface contacts with KIX, because alanine substitutions at these positions have little effect on complex formation or target gene activation (Fig. 4). Consistent with the notion that the secondary structure of c-Myb is essential for its activation properties, mutagenesis of either Leu301 or Glu299 to proline, however, severely compromised target gene activation and disrupted KIX binding in vitro (Fig. 4).
|
The presence of comparably positioned hydrophobic residues in both
c-Myb (aa 290 to 315) and KID (B) helices prompted us to evaluate
whether these domains could functionally substitute for one another. In
transient assays of F9 cells, wild-type CREB stimulated a CRE-CAT
reporter plasmid 12-fold in response to PKA (7), and
deletion of B sequences in KID (aa 136 to 160) blocked reporter
induction, demonstrating the importance of this region for CBP/P300
recruitment (Fig. 5A).
|
Inserting c-Myb (295-315) in place of B partially restored PKA
inducibility in the context of full-length CREB protein (Fig. 5A).
Reflecting the constitutive helical structure of Myb (aa 295 to 315),
the basal activity of the CREB::Myb295-315 chimera was also
two- to threefold higher than that of wild-type CREB (Fig. 5A). By
contrast, substitution of a KIX interaction-defective c-Myb L302A
mutant fragment for B had no such effect, indicating that both
constitutive and PKA-inducible activities of the CREB::Myb295-315 chimera are dependent on recruitment of CBP (Fig. 5A). In reciprocal exchange experiments, residues 137 to 141 in the B region of CREB
(ILNDL) were found to substitute for c-Myb residues 298 to 302 (LELLL)
in the context of the full-length c-Myb protein (Fig. 5B). However,
B residues 134 to 138 (YRKIL) did not support c-Myb activity when
inserted in place of aa 295 to 299 (IKELE) in c-Myb, potentially
reflecting a negative determinant of helicity in this region of CREB
(Fig. 5B).
Structure-function studies showing that an amphipathic B helix in
KID articulates with a shallow hydrophobic groove in KIX (13,
16) led us to examine whether c-Myb binds to KIX by forming similar contacts. To evaluate the relative importance of surface residues in KIX for formation of a complex with c-Myb and CREB, we
performed fluorescence anisotropy experiments. In equilibrium binding
assays, an fl-Myb (aa 276 to 315) peptide associated with KIX with a
predicted Kd of 2 ± 0.3 µM, whereas a
mutant L302A fl-Myb did not bind detectably (Kd > 50 µM; data not shown) to KIX under the same conditions (Fig.
6). By contrast, the
Kd for complex formation between
fl-phospho(Ser133)KID (aa 88 to 160) and KIX was 75 ± 30 nM,
suggesting that KID forms surface contacts with KIX additional to those
formed by c-Myb.
|
On average, alanine substitution at hydrophobic residues (Leu652, Leu653, Lys606, and Tyr650) within the shallow groove of KIX lowered the Kd values for both CREB and c-Myb binding, although these effects were more drastic in the case of c-Myb (Fig. 6B). Tyr650 appeared to be the most important of the shallow groove residues for complex formation, reflecting its combined contribution to both shallow groove structures and deep pocket structures in KIX. Correspondingly, mutagenesis of Tyr650 in KIX to alanine reduced the apparent affinity about 10-fold for KID (Kd = 803 ± 57 nM) and about 25-fold for c-Myb (Kd = 51 ± 3.9 µM) (Fig. 6).
By contrast with these shallow groove contacts, residues in KIX that coordinate with the phosphate moiety in CREB did not appear to be essential for c-Myb binding. Notably, Tyr658 forms a hydrogen bond with the Ser133 phosphate group in CREB, and mutagenesis of this residue to phenylalanine lowered the apparent Kd for phospho(Ser133)KID 60-fold, from 75 nM to 4.6 µM (13) (Fig. 6). Mutagenesis of Tyr658 to Phe in KIX reduced c-Myb binding only 4.5-fold, however, indicating that hydrogen bond contributions from the Tyr658 hydroxyl group are unlikely to stabilize complex formation with c-Myb significantly.
Lys662 in KIX forms a salt bridge with the Ser133 phosphate, and substitution of Lys662 with alanine disrupted binding to phospho(Ser133)KID 12-fold (Kd = 0.9 µM) (13) (Fig. 6), but complex formation between fl-Myb and Lys662Ala KIX was reduced only 2.6-fold. Taken together, these results indicate that, whereas binding of KIX to KID requires both phosphate group interactions and shallow groove interactions, binding to c-Myb may depend primarily on hydrophobic contacts via the shallow groove in KIX (Fig. 6).
Differences in secondary structure between the unbound c-Myb and KID
domains prompted us to compare the relative thermodynamics of formation
of complexes with KIX. In agreement with Kd
measurements obtained by fluorescence anisotropy, the G
for the KID/KIX complex evaluated by ITC was 8.8 kcal/mol, whereas it
was 6.0 kcal/mol for the c-Myb/KIX complex (Fig.
7). Reflecting in part the random coil-to-helix transition in KID, binding of phospho(Ser133)KID to KIX
entailed a substantial entropy penalty of 6 cal/mol/°K that offset
the high enthalpy of complex formation (H = 10.6 kcal/mol ± 0.5%).
|
By contrast, binding of c-Myb (aa 291 to 315) to KIX was accompanied by
a large positive change in entropy (S = +7.5
cal/mol/°K) that compensated for the relatively low enthalpy of
complex formation (H = 4.1 kcal/mol ± 1%)
(Fig. 7). Preliminary nuclear magnetic resonance (NMR) analysis
indicates that the secondary structure of KIX remains unchanged in the
free and bound states for both KID:KIX and c-Myb:KIX complexes
(23). Thus, the entropy of complex formation, in both cases,
reflects the positive contribution of removal of ordered water
molecules from the hydrophobic surfaces offset by the negative
contribution of conformational changes in the activation domains. The
dramatic rearrangement of pKID was observed directly by NMR
(16) and by circular dichroism (Fig. 3) as well as
indirectly by ITC (Fig. 7). Taken together, these results indicate that
formation of a complex between KID and KIX is enthalpy driven, whereas
the c-Myb:KIX complex is dependent on both enthalpy and entropy components.
| |
DISCUSSION |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Activating regions have been proposed to interact with the transcriptional apparatus via simple interactions that do not require elements of secondary structure (15). Our results indicate, on the contrary, that the constitutive and inducible properties of certain activators in part reflect their intrinsic helical propensity.
Both CREB and c-Myb appear to stimulate transcription via surface contacts with hydrophobic residues lining the shallow groove in KIX. Fluorescence anisotropy and ITC experiments reveal that c-Myb binds to KIX with affinity nearly 50-fold lower than that of CREB, due in large part to the absence of hydrogen bond and salt bridge contributions from Tyr658 and Lys662 in KIX with the phosphate moiety. Indeed, binding of phospho(Ser133)CREB to mutant Y658F KIX is comparable to that of c-Myb, suggesting that the Ser133 phosphate interactions account, in large part, for affinity differences between c-Myb and CREB.
Why then is CREB unable to bind KIX in the unphosphorylated state?
Circular dichroism and NMR studies reveal that KID assumes a random
coil structure in the unbound state, and ITC experiments indicate that
the helical transition in KID entails a substantial entropy cost that
is not compensated by hydrophobic contacts with the shallow groove
sufficiently to permit KIX binding. The S for formation
of a complex between KID and KIX thus effectively precludes recruitment
of CBP to the promoter in unstimulated cells and ensures low levels of
target gene expression in the basal state. Indeed, replacement of the
B region in KID with the helical c-Myb (aa 290 to 315) region
stimulated basal reporter expression, demonstrating the importance of
the structural transition in CREB for optimal transcriptional control.
The difference between KID and c-Myb in affinity for KIX (50-fold) is difficult to reconcile with their comparable activities in transient-transfection assays. However, this discrepancy may be explained, at least in part, by differing kinetic profiles for transcriptional activation via the two factors. Cyclic AMP stimulates CREB phosphorylation and target gene expression with burst-attenuation kinetics: CREB activity is maximal within 15 to 30 min of induction, but declines to baseline levels after 2 to 4 h, due to Ser133 dephosphorylation by the Ser/Thr phosphatase PP-1 (7a). By contrast, c-Myb stimulates target gene expression constitutively, and the cumulative effect of Myb activity may therefore be comparable to that of CREB.
Remarkably, the KIX interaction domain of c-Myb contains an LXXLL motif
(aa 298 to 302) that has been shown to mediate binding of members of
the SRC family of coactivators to the nuclear hormone receptors
(5, 10, 19). Crystal structures of liganded SRC-1:PPAR
and GRIP-1:TR complexes reveal that the LXXLL motif folds into a
helical structure that articulates with a shallow groove in the ligand
binding domain of each type of receptor (5, 10). Although it
is unclear whether c-Myb interacts functionally with certain nuclear
receptors, the importance of this motif for KIX binding illustrates a
potentially conserved mechanism by which unrelated activators recruit
the transcriptional apparatus. In this regard, it should be of
considerable interest to evaluate whether the presence of an LXXLL
motif in c-Myb contributes to cross-coupling with nuclear receptor
pathways (14), whereby certain nuclear receptors compete
with CBP for binding to the activation domain of c-Myb.
| |
ACKNOWLEDGMENTS |
|---|
We thank Meghan Mitchell, Stephen Kelly, Xiaoying Wang, Mike Long, and Geli Gao for technical assistance. We also thank Steve Harrison and Chris Walsh for helpful suggestions and Gerry Zambetti and Jan van Deursen for comments on the manuscript.
This work was supported by NIH grants CA70909 (L.H.S.), RO1 CA76385 (P.K.B.), and R01GM37828 (M.M.), by National Cancer Institute Cancer Center Support (CORE) grant P30 CA21765, and by the American Lebanese Syrian Associated Charities (ALSAC) of St. Jude Children's Research Hospital.
D.P. and M.R. contributed equally to this work.
| |
FOOTNOTES |
|---|
* Corresponding author. Present address: Salk Institute, 10010 N. Torrey Pines Rd., La Jolla, CA 92037. Phone: (619) 453-4100. Fax: (619) 552-1546.
| |
REFERENCES |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
| 1. | Akimaru, H., Y. Chen, P. Dai, D. Hou, M. Nonaka, S. Smolik, S. Armstrong, R. Goodman, and S. Ishii. 1997. Drosophila CBP is a co-activator of cubitus interruptus in hedgehog signalling. Nature 386:735-738[Medline]. |
| 2. | Arias, J., A. Alberts, P. Brindle, F. Claret, T. Smeal, M. Karin, J. Feramisco, and M. Montminy. 1994. Activation of cAMP and mitogen responsive genes relies on a common nuclear factor. Nature 370:226-228[Medline]. |
| 3. | Brindle, P., S. Linke, and M. Montminy. 1993. Analysis of a PK-A dependent activator in CREB reveals a new role for the CREM family of repressors. Nature 364:821-824[Medline]. |
| 4. |
Dai, P.,
H. Akimaru,
Y. Tanaka,
D. Hou,
T. Yasukawa,
C. Kanei-Ishii,
T. Takahashi, and S. Ishii.
1996.
CBP as a transcriptional coactivator.
Genes Dev.
10:528-540 |
| 5. |
Darimont, B.,
R. Wagner,
J. Apriletti,
M. Stallcup,
P. Kushner,
J. Baxter,
R. Fletterick, and K. Yamamoto.
1998.
Structure and specificity of nuclear receptor-coactivator interactions.
Genes Dev.
12:3343-3356 |
| 6. |
Gonzalez, G. A.,
P. Menzel,
J. Leonard,
W. H. Fischer, and M. R. Montminy.
1991.
Characterization of motifs which are critical for activity of the cyclic AMP-responsive transcription factor CREB.
Mol. Cell. Biol.
11:1306-1312 |
| 7. | Gonzalez, G. A., and M. R. Montminy. 1989. Cyclic AMP stimulates somatostatin gene transcription by phosphorylation of CREB at serine 133. Cell 59:675-680[Medline]. |
| 7a. | Hagiwara, M., A. Alberts, P. Brindle, J. Meinkoth, J. Feramisco, T. Deng, M. Karin, S. Shenolikar, and M. Montminy. 1992. Transcriptional attenuation following cAMP induction requires PP-1-mediated dephosphorylation of CREB. Cell 70:105-113[Medline]. |
| 8. |
Kasper, L. H.,
P. K. Brindle,
C. A. Schnabel,
C. E. J. Pritchard,
M. L. Cleary, and J. M. A. van Deursen.
1999.
CREB binding protein interacts with nucleoporin-specific FG repeats that activate transcription and mediate NUP98-HOXA9 oncogenicity.
Mol. Cell. Biol.
19:764-776 |
| 9. | Kwok, R., M. Laurance, J. Lundblad, P. Goldman, H. Shih, L. Connor, S. Marriott, and R. Goodman. 1996. Control of cAMP-regulated enhancers by the viral transactivator Tax through CREB and the co-activator CBP. Nature 380:642-646[Medline]. |
| 10. |
McInerney, E.,
D. Rose,
S. Flynn,
S. Westin,
T. Mullen,
A. Krones,
J. Inostroza,
J. Torchia,
R. Nolte,
N. Assa-Munt,
M. Milburn,
C. Glass, and M. Rosenfeld.
1998.
Determinants of coactivator LXLL motif specificity in nuclear receptor transcriptional activation.
Genes Dev.
12:3357-3368 |
| 11. |
Oliner, J.,
J. Andresen,
S. Hansen,
S. Zhou, and R. Tjian.
1996.
SREBP transcriptional activity is mediated through an interaction with the CREB-binding protein.
Genes Dev.
10:2903-2911 |
| 12. |
Parker, D.,
K. Ferreri,
T. Nakajima,
V. J. LaMorte,
R. Evans,
S. C. Koerber,
C. Hoeger, and M. Montminy.
1996.
Phosphorylation of CREB at Ser-133 induces complex formation with CREB-binding protein via a direct mechanism.
Mol. Cell. Biol.
16:694-703 |
| 13. | Parker, D., U. Jhala, I. Radhakrishnan, M. Yaffe, C. Reyes, A. Shulman, L. Cantley, P. Wright, and M. Montminy. 1998. Analysis of an activator: coactivator complex reveals an essential role for secondary structure in transcriptional activation. Mol. Cell 2:353-359[Medline]. |
| 14. |
Pfitzner, E.,
J. Kirfel,
P. Becker,
A. Rolke, and R. Schule.
1998.
Physical interaction between retinoic acid receptor and the oncoprotein Myb inhibits retinoic acid-dependent trans-activation.
Proc. Natl. Acad. Sci. USA
95:5539-5544 |
| 15. | Ptashne, M., and A. Gann. 1997. Transcriptional activation by recruitment. Nature 386:569-577[Medline]. |
| 16. | Radhakrishnan, I., G. Perez-Alvarado, D. Parker, H. J. Dyson, M. Montminy, and P. E. Wright. 1997. Solution structure of the KIX domain of CBP bound to the transactivation domain of CREB: a model for activator-coactivator interactions. Cell 91:741-752[Medline]. |
| 17. | Sadowski, I., B. Bell, P. Broad, and M. Hollis. 1992. Gal4 fusion vectors for expression in yeast or mammalian cells. Gene 118:137-141[Medline]. |
| 18. |
Shapiro, L.
1995.
Myb and Ets proteins cooperate to transactivate an early myeloid gene.
J. Biol. Chem.
270:8763-8767 |
| 19. | Torchia, J., D. Rose, J. Inostroza, Y. Kannei, S. Westin, C. K. Glass, and M. G. Rosenfield. 1997. The transcriptional co-activator p/CIP binds CBP and mediates nuclear-receptor function. Nature 387:677-684[Medline]. |
| 20. | Wu, Y., R. Reece, and M. Ptashne. 1996. Quantitation of putative activator-target affinities predicts transcriptional activating potentials. EMBO J. 15:3951-3963[Medline]. |
| 21. |
Yang, C.,
L. Shapiro,
M. Rivera,
A. Kumar, and P. K. Brindle.
1998.
A role for CREB binding protein and P300 transcriptional coactivators in Ets-1 transactivation functions.
Mol. Cell. Biol.
18:2218-2229 |
| 22. |
Zhang, J.,
U. Vinkemeier,
W. Gu,
D. Chakravarti,
C. Horvath, and J. Darnell.
1996.
Two contact regions between Stat1 and CBP/P300 in interferon signaling.
Proc. Natl. Acad. Sci. USA
93:15092-15096 |
| 23. | Zor, T., and P. E. Wright. Unpublished observations. |
Molecular and Cellular Biology, August 1999, p. 5601-5607, Vol. 19, No. 8
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
This article has been cited by other articles:
-
Pattabiraman, D. R., Sun, J., Dowhan, D. H., Ishii, S., Gonda, T. J.
(2009). Mutations in Multiple Domains of c-Myb Disrupt Interaction with CBP/p300 and Abrogate Myeloid Transforming Ability. Mol Cancer Res
7: 1477-1486
[Abstract] [Full Text] -
Kauppi, M., Murphy, J. M., de Graaf, C. A., Hyland, C. D., Greig, K. T., Metcalf, D., Hilton, A. A., Nicola, N. A., Kile, B. T., Hilton, D. J., Alexander, W. S.
(2008). Point mutation in the gene encoding p300 suppresses thrombocytopenia in Mpl-/- mice. Blood
112: 3148-3153
[Abstract] [Full Text] -
Wood, M. A., Attner, M. A., Oliveira, A. M.M., Brindle, P. K., Abel, T.
(2006). A transcription factor-binding domain of the coactivator CBP is essential for long-term memory and the expression of specific target genes. Learn. Mem.
13: 609-617
[Abstract] [Full Text] -
Chi, S.-W., Lee, S.-H., Kim, D.-H., Ahn, M.-J., Kim, J.-S., Woo, J.-Y., Torizawa, T., Kainosho, M., Han, K.-H.
(2005). Structural Details on mdm2-p53 Interaction. J. Biol. Chem.
280: 38795-38802
[Abstract] [Full Text] -
Bayly, R., Chuen, L., Currie, R. A., Hyndman, B. D., Casselman, R., Blobel, G. A., LeBrun, D. P.
(2004). E2A-PBX1 Interacts Directly with the KIX Domain of CBP/p300 in the Induction of Proliferation in Primary Hematopoietic Cells. J. Biol. Chem.
279: 55362-55371
[Abstract] [Full Text] -
Best, J. L., Amezcua, C. A., Mayr, B., Flechner, L., Murawsky, C. M., Emerson, B., Zor, T., Gardner, K. H., Montminy, M.
(2004). Identification of small-molecule antagonists that inhibit an activator:coactivator interaction. Proc. Natl. Acad. Sci. USA
101: 17622-17627
[Abstract] [Full Text] -
Chen, W. G., West, A. E., Tao, X., Corfas, G., Szentirmay, M. N., Sawadogo, M., Vinson, C., Greenberg, M. E.
(2003). Upstream Stimulatory Factors Are Mediators of Ca2+-Responsive Transcription in Neurons. J. Neurosci.
23: 2572-2581
[Abstract] [Full Text] -
Goto, N. K., Zor, T., Martinez-Yamout, M., Dyson, H. J., Wright, P. E.
(2002). Cooperativity in Transcription Factor Binding to the Coactivator CREB-binding Protein (CBP). THE MIXED LINEAGE LEUKEMIA PROTEIN (MLL) ACTIVATION DOMAIN BINDS TO AN ALLOSTERIC SITE ON THE KIX DOMAIN. J. Biol. Chem.
277: 43168-43174
[Abstract] [Full Text] -
Zor, T., Mayr, B. M., Dyson, H. J., Montminy, M. R., Wright, P. E.
(2002). Roles of Phosphorylation and Helix Propensity in the Binding of the KIX Domain of CREB-binding Protein by Constitutive (c-Myb) and Inducible (CREB) Activators. J. Biol. Chem.
277: 42241-42248
[Abstract] [Full Text] -
Suzuki, T., Yamakuni, T., Hagiwara, M., Ichinose, H.
(2002). Identification of ATF-2 as a Transcriptional Regulator for the Tyrosine Hydroxylase Gene. J. Biol. Chem.
277: 40768-40774
[Abstract] [Full Text] -
Reid, J., Kelly, S. M., Watt, K., Price, N. C., McEwan, I. J.
(2002). Conformational Analysis of the Androgen Receptor Amino-terminal Domain Involved in Transactivation. INFLUENCE OF STRUCTURE-STABILIZING SOLUTES AND PROTEIN-PROTEIN INTERACTIONS. J. Biol. Chem.
277: 20079-20086
[Abstract] [Full Text] -
Asahara, H., Tartare-Deckert, S., Nakagawa, T., Ikehara, T., Hirose, F., Hunter, T., Ito, T., Montminy, M.
(2002). Dual Roles of p300 in Chromatin Assembly and Transcriptional Activation in Cooperation with Nucleosome Assembly Protein 1 In Vitro. Mol. Cell. Biol.
22: 2974-2983
[Abstract] [Full Text] -
Simon, A. L., Stone, E. A., Sidow, A.
(2002). Inference of functional regions in proteins by quantification of evolutionary constraints. Proc. Natl. Acad. Sci. USA
99: 2912-2917
[Abstract] [Full Text] -
Twigg, P. D., Parthasarathy, G., Guerrero, L., Logan, T. M., Caspar, D. L. D.
(2001). Disordered to ordered folding in the regulation of diphtheria toxin repressor activity. Proc. Natl. Acad. Sci. USA
98: 11259-11264
[Abstract] [Full Text] -
Ernst, P., Wang, J., Huang, M., Goodman, R. H., Korsmeyer, S. J.
(2001). MLL and CREB Bind Cooperatively to the Nuclear Coactivator CREB-Binding Protein. Mol. Cell. Biol.
21: 2249-2258
[Abstract] [Full Text] -
Shaywitz, A. J., Dove, S. L., Kornhauser, J. M., Hochschild, A., Greenberg, M. E.
(2000). Magnitude of the CREB-Dependent Transcriptional Response Is Determined by the Strength of the Interaction between the Kinase-Inducible Domain of CREB and the KIX Domain of CREB-Binding Protein. Mol. Cell. Biol.
20: 9409-9422
[Abstract] [Full Text] -
Zhang, Q., Vo, N., Goodman, R. H.
(2000). Histone Binding Protein RbAp48 Interacts with a Complex of CREB Binding Protein and Phosphorylated CREB. Mol. Cell. Biol.
20: 4970-4978
[Abstract] [Full Text] -
Goodman, R. H., Smolik, S.
(2000). CBP/p300 in cell growth, transformation, and development. Genes Dev.
14: 1553-1577
[Full Text] -
Du, K., Asahara, H., Jhala, U. S., Wagner, B. L., Montminy, M.
(2000). Characterization of a CREB Gain-of-Function Mutant with Constitutive Transcriptional Activity In Vivo. Mol. Cell. Biol.
20: 4320-4327
[Abstract] [Full Text] -
Cardinaux, J.-R., Notis, J. C., Zhang, Q., Vo, N., Craig, J. C., Fass, D. M., Brennan, R. G., Goodman, R. H.
(2000). Recruitment of CREB Binding Protein Is Sufficient for CREB-Mediated Gene Activation. Mol. Cell. Biol.
20: 1546-1552
[Abstract] [Full Text] -
Xu, W., Chen, H., Du, K., Asahara, H., Tini, M., Emerson, B. M., Montminy, M., Evans, R. M.
(2001). A Transcriptional Switch Mediated by Cofactor Methylation. Science
294: 2507-2511
[Abstract] [Full Text] -
Ostedgaard, L. S., Baldursson, O., Welsh, M. J.
(2001). Regulation of the Cystic Fibrosis Transmembrane Conductance Regulator Cl- Channel by Its R Domain. J. Biol. Chem.
276: 7689-7692
[Full Text] -
Ostedgaard, L. S., Baldursson, O., Vermeer, D. W., Welsh, M. J., Robertson, A. D.
(2000). A functional R domain from cystic fibrosis transmembrane conductance regulator is predominantly unstructured in solution. Proc. Natl. Acad. Sci. USA
97: 5657-5662
[Abstract] [Full Text]
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
Copyright © 2010 by the American Society for Microbiology. For an alternate route to Journals.ASM.org, visit: http://intl-journals.asm.org | More Info»