![[Feedback]](/icons/banner/feedbackACT.gif){kind=icon}
![[For Subscribers]](/icons/banner/subscriberACT.gif){kind=icon}
![[Archive]](/icons/banner/archiveACT.gif){kind=icon}
![[Search]](/icons/banner/searchACT.gif){kind=icon}
![[Contents]](/icons/banner/tocACT.gif){kind=icon}
|
|
|
|
|
||
Vol. 14, Issue 6, 2583-2591, June 2003
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
Dipartimento di Biologia, Università Roma Tre, V. le G. Marconi, 446, I-00146 Roma
Submitted September 30, 2002;
Revised December 16, 2002;
Accepted January 30, 2003
Monitoring Editor: Keith R. Yamamoto
 |
ABSTRACT |
|---|
 TOP ABSTRACT INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
|---|
and ERK signaling molecules. The analysis of
the cyclin D1 gene expression showed that only the MAP kinase
pathway was involved. Here, the presence of rapid/nongenomic,
estradiol-regulated, PI3K/AKT signal transduction pathway, its modulation by
the levels of the tumor suppressor PTEN, its cross-talk with the ERK pathway,
and its involvement in DNA synthesis and cyclin D1 gene promoter
activity have all been studied in HepG2 cells. 17
-Estradiol induced the
rapid and biphasic phosphorylation of AKT. These phosphorylations were
independent of each other, being the first wave of activation independent of
the estrogen receptor (ER), whereas the second was dependent on ER. Both
activations were dependent on PI3K activity; furthermore, the ERK pathway
modulated AKT phosphorylation by acting on the PTEN levels. The results showed
that the PI3K pathway, as well as ER, were strongly involved in both
G1–S progression and cyclin D1 promoter activity
by acting on its proximal region (-254 base pairs). These data indicate that
in HepG2 cells, different rapid/nongenomic estradiol-induced signal
transduction pathways modulate the multiple steps of G1–S
phase transition. |
INTRODUCTION |
|---|
|
TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
|---|
-Estradiol (E2) can trigger DNA synthesis and cell cycle
progression in different cell types
(Sutherland et al.,
1983
; Castoria et al.,
1999; Marino et al.,
2001a) by regulating the expression of the genes involved in the
cell cycle machinery (Altucci et
al., 1996; Foster et
al., 2001). In particular, E2 can induce cyclin D1
gene transcription, even though its gene promoter region does not contain any
estrogen-responsive element (ERE) or ERE-like sequence
(Herbert et al.,
1994; Sabbah et al.,
1999), recruiting different transcription factors depending on the
cell context. Moreover, the rapid (1–6 h) E2-induced cyclin
D1 gene expression reported in several cell lines, even in the
presence of an estrogen receptor lacking the DNA binding domain, suggests that
E2-induced rapid/nongenomic mechanisms are sufficient to induce cyclin
D1 overexpression (Marino
et al., 2002). Several cyclin D1 activation
mechanisms have been reported. In particular, we identified the E2-induced
rapid extranuclear molecular events in HepG2 cells (e.g., mitogen-activated
protein kinase/extracellular regulated kinase [MAPK/ERK] and phospholipase
C/protein kinase C [PLC/PKC] activation), showing also that only the
E2-induced rapid/nongenomic phosphorylation of ERK was necessary for the
E2-induced cyclin D1 transcription. Furthermore, the destruction of
the TRE motif present in the cyclin D1 promoter, -848 base pairs
(bp), caused the complete loss of estrogen responsiveness. In mammary
carcinoma cells, it has been reported
(Sabbah et al., 1999;
Castro-Rivera et al.,
2001; Nagata et al.,
2001) that the three GC-rich SP1 sites at -143 to -110 bp and the
CRE motif at -96 bp regions of the promoter are the major mediators for the
induction of the cyclin D1 promoter by E2 via protein kinase A. In
addition, recent data in MCF7 cells indicate a role for the
phosphatidylinositol 3-kinase (PI3K) but not for ERK in E2-induced cyclin
D1 -1800 bp promoter activity
(Castoria et al.,
2001).
The PI3Ks compose a family of lipid kinases that phosphorylate the 3'
position of the inositol ring of the phosphatidyl inositol(4)phosphate
(PI-4-P), the phosphatidyl inositol(4, 5)bisphosphate (PI-4,5-P2)
to generate PI-3,4-P2 and PI-3,4,5-P3, respectively
(Scheid et al.,
2002), which shows an affinity for certain protein modules, such
as pleckstrin homology domain, implicated in several cellular processes,
including cell survival, DNA synthesis, protein trafficking, and metabolism
(for review, see Scheid and Woodgett,
2001). The role of PI3K in growth involves the serine/threonine
kinase, AKT/PKB, translocation in proximity to phosphoinositide-dependent
kinase 1, PDK1, resulting in AKT/PKB phosphorylation
(Scheid and Woodgett, 2001).
The PKB/AKT activation drives cells through many biological functions,
including gene expression, cell cycle, survival, glucidic metabolism,
endocytosis and vesicular trafficking, cell transformation, and oncogenesis
(Coffer et al., 1998;
Stein and Waterfield, 2000).
AKT/PKB phosphorylation is negatively regulated by the PTEN/MMAC1/TEP1 tumor
suppressor gene protein product, which is a phosphatase that dephosphorylates
the 3' position to reverse the reactions catalyzed by PI3K
(Maehama and Dixon, 1998;
Cantley and Neel, 1999). The
overexpression of PTEN blocks cell cycle progression and induces apoptosis in
cells (Furnari et al.,
1998; Ramaswamy et
al., 1999). Although the importance of the PI3K/PTEN pathway
in cell growth is well established, its cross-talk with ERK pathway and its
role in E2-regulated cyclin D1 promoter activity are not
understood.
In this study, we show that PI3K is required for E2-stimulated HepG2 cell growth. We provide evidence that the ERK pathway rapidly reduces the levels of PTEN, allowing E2-induced phosphorylation of AKT. Our data indicate that both the PI3K and the ERK pathways coordinately regulate cyclin D1 promoter activity, allowing HepG2 cell cycle progression.
|
MATERIALS AND METHODS |
|---|
|
TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
|---|
-Estradiol, 17-estradiol, gentamicin, penicillin, RPMI-1640
(with or without phenol red), fetal calf serum, and charcoal-stripped fetal
calf serum were purchased from Sigma Chemical (St. Louis, MO). The MAP kinase
cascade inhibitors PD 98059 and U 0126 and the PI3 kinase inhibitors
wortmannin and Ly 294002 were obtained from Calbiochem (San Diego, CA). The
estrogen receptor inhibitor ICI 182,780 was obtained from Tocris (Ballwin,
MO). Methyl-1-[3H]thymidine (specific activity, 81 Ci/mmol) was
purchased from Amersham-Pharmacia (Little Chalfont, UK). Lipofectamine reagent
was obtained from Gibco-BRL Life Technology (Gaithersburg, MD). The luciferase
kit was obtained from Promega (Madison, WI). The GenElute Plasmid Maxiprep Kit
was obtained from Sigma. The Bradford protein assay was obtained from Bio-Rad
Laboratories (Hercules, CA). The monoclonal anti–phospho-AKT antibody
was obtained from New England Biolabs (Beverly, MA); the monoclonal and
polyclonal anti-AKT, anti-PTEN, and anti–-actin antibodies were
obtained from Santa Cruz Biotechnology (Santa Cruz, CA). CDP-Star
chemiluminescence reagent for Western blot was obtained from NEN (Boston,
MA). All the other products were from Sigma. Analytical or reagent grade products, without further purification, were used.
Cell Culture
HepG2 cells were grown routinely in 5% CO2 in air in modified,
phenol red–free, RPMI-1640 medium containing 10% (vol/vol)
charcoal-stripped fetal calf serum, L-glutamine (2 mM), gentamicin
(10 µg/ml), and penicillin (100 U/ml). Cells were passaged every 4 d, and
media were changed every 2 d.
DNA Synthesis
DNA synthesis was assayed by incubating subconfluent cells (70–80%)
with methyl-1-[3H]thymidine (final concentration, 1 µCi/ml).
Cells were treated simultaneously with E2 (final concentration, 10 nM) or
vehicle (ethanol/PBS 1:10 vol/vol). Ly 294002 (final concentration, 10 µM)
or ICI 182,780 (final concentration, 1 µM) was added 15 min before E2 and
methyl-1-[3H]thymidine. Wortmannin (final concentration, 10 µM)
was added simultaneously to E2 and labeled thymidine. Thymidine incorporation
was assayed 1 h after E2 administration as previously reported
(Marino et al.,
2001a).
Plasmids
The gene reporter plasmids pXP2-D1-2966-luciferase,
pXP2-D1
-254-luciferase (-254), and
pXP2-D1-20-luciferase (-20) and the plasmids containing the
vector expression for pCR3.1--galactosidase have been described
previously (Herbert et al.,
1994; Marino et al.,
2002). Plasmids were purified for transfection with a plasmid
preparation kit according to the manufacturer's instructions. A luciferase
dose–response curve showed that the maximum effect was present when 1
µg of DNA was transfected with 1 µg of pCR3.1--galactosidase to
normalize transfection efficiency (
55–65%).
Transfection and Luciferase Assay
Cells were grown to 70% confluence, then transfected using
Lipofectamine reagent according to the manufacturer's instructions. Six hours
after transfection, the medium was changed, and 24 h thereafter, cells were
stimulated with 10 nM E2 for 6 h. In some experiments, the HepG2 cells were
treated with E2–BSA conjugate (-estradiol
6-(0-carboxy-methyl)oxime:BSA, 32 mol E2/mol BSA). This form of macromolecular
bound estrogen does not pass through the plasma membrane and is much more
water soluble than free E2 (Zheng et
al., 1996). Before each experiment, E2–BSA was
dissolved in phenol-free growth medium (0.2 mg/ml), mixed with dextran and
charcoal, centrifuged, and passed through a 0.22-mm filter
(Russell et al.,
2000; Marino et al.,
2002; Seo and Leclercq,
2002). In these conditions, free E2 was retained in the resin
(>3
) (Stevis et al.,
1999), and the filtrate contained E2–BSA. When indicated, Ly
294002 or wortmannin (PI3K inhibitors) was added 15 min before E2, and
reporter plasmid expression was evaluated 6 h thereafter. The cell lysis
procedure and the subsequent measurement of luciferase gene expression were
performed by use of the luciferase kit according to the manufacturer's
instructions with a EC & G Berthold luminometer.
Electrophoresis and Immunoblotting
After treatment with inhibitors (10 µM PD 98059 or 10 µM U 0126 [MAP
kinase cascade inhibitors] or 10 µM Ly 294002 or 10 µM wortmannin [PI3K
inhibitors] or 1 µM ICI 182,780) or hormone, cells were lysed as described
previously (Marino et al.,
2001b) and solubilized in 0.125 M Tris HCl (pH 6.8) containing 10%
SDS (wt/vol), 1 mM phenylmethylsulfonyl fluoride, and 5 µg/ml leupeptin and
boiled for 2 min. Proteins were quantified using the Bradford protein assay
(Bradford, 1976). Solubilized
proteins (20 µg) were resolved using 7.5% SDS-PAGE at 100 V for 1 h. The
proteins were then electrophoretically transferred to nitrocellulose for 45
min at 150 V at 4°C. The nitrocellulose was treated with 3% bovine serum
albumin in 138 mM NaCl, 26.8 mM KCl, 25 mM Tris HCl (pH 8.0), 0.05% Tween-20,
and 0.1% BSA and then probed at room temperature for 1 h with
anti–phospho-AKT, anti–phospho-ERK, or anti-PTEN antibodies. The
nitrocellulose was stripped with Restore Western blot stripping buffer (Pierce
Chemical, Rockford, IL) for 10 min at room temperature and then probed with
anti-AKT (1 µg/ml). Anti–-actin antibody (1 µg/ml) was used
to normalize the sample loading. Antibody reaction was visualized with
chemiluminescence reagent for Western blot.
|
RESULTS |
|---|
|
TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
|---|
|
E2 Rapidly Activates PI3K-dependent AKT Phosphorylation
The serine/threonine kinase AKT/PKB is a major PI3K target, and its
activation through the phosphorylation of Thr308/Ser473 mediates many of the
downstream cellular effects of PI3K. To investigate the role of the PI3K/AKT
pathway in the E2-induced HepG2 cell cycle progression, we analyzed the
hormone's effects on AKT activity. Figure
2a shows that E2 stimulated the biphasic phosphorylation of AKT. A
transient stimulation was initially detectable after 3 min of hormonal
treatment and decreased toward basal levels after 5 min. A second wave of AKT
phosphorylation started 10 min after hormone administration, with a peak 30
min later. The total amount of AKT protein did not change, as detected when
the same filter was reprobed with anti-AKT antibody.
|
The specificity of the biphasic E2-induced AKT phosphorylation was
confirmed by the powerlessness of the stereoisomer 17--estradiol to
induce a similar activation (Figure
2b).
The role of ER was assessed by using the pure antiestrogen ICI
(Figure 3a). Surprisingly, the
ER inhibitor prevented only 30 min E2-induced AKT phosphorylation. To test
whether the E2-induced AKT phosphorylation could be mediated by the binding of
E2 to the cell surface receptors, HepG2 cells were treated with the
E2–BSA conjugate, which does not pass through the plasma membrane
(Zheng et al.,1996).
As shown in Figure 3b, after
E2–BSA stimulation, the increase in the AKT phosphorylation was similar
to that induced by the free E2, thus suggesting the probable involvement of a
membrane ER in the E2 effects.
|
Consistent with the view that AKT is a target for PI3K, the Ly 294002 and wortmannin pretreatments of HepG2 cells blocked the E2-induced AKT phosphorylation both after 3 min and after 30 min of hormone stimulation (Figure 4, a and b). The levels of PTEN were analyzed to assess a role for the tumor suppressor PTEN, which recognizes PI-3,4,5-P3 as the principal substrate in the E2-induced AKT phosphorylation. E2 decreased the PTEN levels at 15 and 30 min after the stimulation, as shown by the time course in Figure 4c.
|
Cross-Talk Between PI3K and ERK Signal Transduction Pathways and the
Effect on the Cyclin D1 Promoter Activity
The accumulation of cyclin D1 protein after E2 stimulation is a
critical event in G1 progression. We previously reported the
accumulation of E2-induced cyclin D1 mRNA and protein 1–6 h
after hormone stimulation. Furthermore, our data indicated that E2-induced DNA
synthesis and cyclin D1 transcription were strictly dependent on
rapid (10 min) and ER-dependent ERK phosphorylation; moreover, we demonstrated
that the TRE motif located at -848 bp of cyclin D1 promoter was the
target for E2-induced ERK activation
(Marino et al.,
2002). To assess whether this E2-induced pathway is synergic or
parallel to the PI3K pathway in modulating cyclin D1 transcription,
we first examined the effect of the MAP kinase pathway inhibitors on the
ER-dependent AKT phosphorylation and PTEN levels 30 min after E2 stimulation.
The MAP kinase cascade inhibitor (PD 98059 or U 0126) pretreatment completely
blocked the E2-induced AKT phosphorylation
(Figure 5a) and caused the
parallel increase of PTEN levels (Figure
5b). The cell pretreatment with the inhibitors alone did not
change AKT phosphorylation or PTEN levels.
|
The pretreatment of HepG2 cells with the PI3K inhibitors Ly 294002 or wortmannin did not affect the E2-induced ERK phosphorylation after 10 min of hormone treatment (Figure 5c), even though these concentrations completely blocked AKT phosphorylation.
To verify whether the PI3K signal transduction pathway had a role in regulating cyclin D1 promoter activity and whether this signaling pathway worked on a different regulatory element(s) present in the cyclin D1 promoter, we transiently transfected HepG2 cells with either the complete cyclin D1 promoter construct (-2966 bp) or the deletion mutants of cyclin D1 promoter construct (-254 bp and -20 bp) linked to luciferase gene. E2 induced the transcription of -2966 and -254 cyclin D1 constructs (Figure 6, a and b). PI3K inhibitor pretreatment completely prevented E2 effects on both constructs. Conversely, E2 was ineffective in stimulating the activity of the minimal cyclin D1 promoter construct (-20, Figure 6c).
|
|
DISCUSSION |
|---|
|
TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
|---|
;
Lupu et al., 1996;
Castoria et al., 1999;
Marino et al., 2001b;
Nadal et al., 2001).
In addition to the accepted model for the E2 action mechanism, there is
emerging evidence that E2-regulated mitogenesis starts with the activation of
rapid/nongenomic signaling molecules often originating from the cell membrane
(Castoria et al.,
1999; Marino et al.,
2001a,
2001b,
2002). This activation has
been investigated with the primary focus on the MAP kinase pathway in mammary
gland cells, MCF7, but with contradictory results
(Migliaccio et al.,
1996; Improta-Brears et
al., 1999; Lobenhofer
et al., 2000; Caristi
et al., 2001; Castoria
et al., 2001). Similar contradictions, although less well
documented, are reported on E2-induced PI3K/AKT activation and on its role in
regulating DNA synthesis and the cyclin D1 promoter activity
(Lobenhofer et al.,
2000; Castoria et al.,
2001; Sun et al.,
2001); furthermore, an acceptable definition of the cross-talk
with other signaling pathways (i.e., MAP kinase) is lacking. The failure in
summarizing a general model of E2 action working in MCF7 cells is probably
attributable to the changes in the cell context occurring in these cells.
Either synchronization procedures or the different ER-to-ER ratio
present in MCF7 cells, depending on their malignancy
(Roger et al., 2001;
Liu et al., 2002),
could turn signal transduction pathways on or off differently.
Conversely, the HepG2 cell line represents a valuable experimental model
for studying the role played by E2-induced nongenomic actions on hepatic cell
proliferation. In fact, these cells retain many of the differentiated
characteristics of quiescent hepatocytes, including E2 responsiveness (Archer
et al., 1985,
1986;
Chen et al., 1999;
Graf et al., 2001).
Like other liver-derived cells, HepG2 cells cultured in a medium not
supplemented with estrogen maintain only the ER expression
(Tam et al., 1986;
Couse et al., 1997;
Farsetti et al.,
1998; Taylor and Al-Azzawi,
2000), although at levels insufficient to induce a
ligand-dependent trans-activation of synthetic ERE-containing target genes
(Marino et al.,
2001b). In this experimental model, we have recently identified
two nongenomic actions of E2 (PKC- and ERK-2 activation) that work in
parallel to modulate distinct steps of E2-induced cell cycle progression
(Marino et al.,
2002).
Here, using a pharmacological approach, we found that the disruption of the PI3K cascade by specific inhibitors prevented the ability of HepG2 cells to enter the S phase in response to E2. We also demonstrated that E2 activates the AKT phosphorylation via PI3K and ERK. In fact, only after ERK activation (15 min after E2 administration) was a sustained, ER-dependent AKT phosphorylation detected (15–30 min). The ERK modulation of AKT phosphorylation is connected to the tumor suppressor PTEN levels, as demonstrated by the ability of MAP kinase cascade inhibitors to prevent E2-induced reduction of the PTEN levels. Both the PI3K inhibitors used prevented the cyclin D1 promoter activity. Noteworthy was the effect also present in the deletion mutant of cyclin D1 promoter construct (i.e., -254 bp), which contains the GC-rich region of SP1 and CRE motif.
These results showed a peculiar biphasic PI3K/AKT activation, partially
related to PTEN levels, and identified the region of cyclin D1
promoter affected by this activation cascade. The timing of E2-induced AKT
phosphorylation agrees with those reported in MCF7 (i.e., 2–10 min)
(Improta-Brears et al.,
1999; Castoria et al.,
2001), neuronal, and astroglial cells (from 15 min with the
highest level at 30 min) (Ivanova et
al., 2002). Furthermore, we have shown the biphasic AKT
phosphorylation with the earliest activation (3 min) to be unresponsive to the
pure anti-ER, ICI, and the second (30 min) to be prevented by ICI. No
activation was induced after the administration of the stereoisomer
17-E2, indicating the specificity of E2-induced AKT phosphorylation.
Moreover, both waves of AKT activation were mimicked by the plasma
membrane–nonpermeating E2–BSA and were strictly linked to PI3K.
These data, together with the rapidity of AKT phosphorylation (3 and 30 min),
imply that the activation of PI3K starts from the plasma membrane. It has been
proposed that a putative plasma membrane ER might be involved in
rapid/nongenomic effects of E2 in several cell types
(Levin, 2002), although its
characterization remains unsolved. Recently, a 
-adrenergic membrane ER,
which could be responsible for E2 initiating rapid signal in pancreatic
cells (i.e., increase of Ca2+ entry), has been described
(Ropero et al.,
2002). This receptor seems to be structurally unrelated to
ER, being activated even in the presence of ICI. It is possible that
the first activation of AKT, unresponsive to ICI, is dependent on this kind of
receptor. By contrast, a fraction of ER appears to be able to
translocate from the nucleus (Song et
al., 2002) and localize close to the plasma membrane
(Norfleet et al.,
1999; Marino et al.,
2002; Razandi et al.,
2002). This kind of ER could be accounted for in the second wave
of AKT phosphorylation.
Conversely, it is known that PI3K catalyzes the phosphorylation in the
3' position of the inositol ring of phosphoinositides (mainly PI-4-P and
PI-4,5-P2), producing an accumulation of second messengers (i.e.,
PI-3,4-P2, PI-3,4,5-P3) that are poor substrates for PLC
but can recruit a variety of cytosolic signaling proteins on plasma membrane.
AKT is one of these proteins: the link with the phosphoinositides enables AKT
to localize on the plasma membrane and to open up the catalytic site. A second
serine/threonine kinase, PDK1, also binds the phosphoinositides and
colocalizes with AKT, phosphorylating the activation loop of the exposed
catalytic domain (Scheid et al.,
2002). The prevalent paradigm is that AKT phosphorylation is
regulated by PTEN levels. Characterization of the lipid phosphatase activity
of PTEN demonstrates that it shows specificity for phosphatidyl inositols
phosphorylated at the 3' position, and indeed, overexpression of PTEN in
mammalian cells disrupted the PI3K-dependent production of
PI-3,4,5-P3. Furthermore, the expression of the PTEN catalytically
inactive mutant PTEN-C124S, which may function as a substrate trap, resulted
in the accumulation of PI-3,4,5-P3, indicating that PTEN may
function in vivo to antagonize the PI3K-dependent signaling
(Furnari et al.,
1997; Weng et al.,
2001). These results could explain the presence of the growth
factor–induced PI3K/AKT activations, probably mediated by the other PI3K
product, PI-3,4-P2, which was still observed in the presence of
high levels of PTEN (Cantley and Neel,
1999). In our system, the high levels of PTEN, parallel to the
E2-induced earlier AKT phosphorylation, suggest that such activation may be
dependent on PI-3,4-P2; furthermore, it is transient and redundant
with respect to E2-induced proliferation, because no ER-independent effects on
E2-induced DNA synthesis have been detected in HepG2 cells.
The second, prolonged and ER-dependent, AKT phosphorylation may be linked
primarily to the production of PI-3,4,5-P3; in fact, it is
paralleled by the decrease of PTEN levels. Remarkably, the disruption of the
MAP kinase cascade by specific inhibitors prevented the E2-induced PTEN level
reduction, suggesting that ERK may modulate the PTEN levels. PTEN was
discovered only in 1997, and it has been the focus of particularly intense
interest because of its central role in suppressing malignancy, functioning
primarily as a PI-3,4,5-P3 phosphatase to regulate the crucial
signal transduction pathway of PI3K (Myers
et al., 1998; Yamada
and Araki, 2001). Here, for the first time, a PTEN role in
E2-induced cell proliferation has been reported.
Our results show that the disruption of the PI3K cascade by specific
inhibitors prevents the E2-induced thymidine incorporation in DNA and confirm
the role of cyclin D1 as a key intermediate in the E2-induced
progression of cells through the G1 phase of the cell cycle, even
though no ERE-like sequence in the promoter of cyclin D1 gene has
been detected (Herbert et al.,
1994). The E2 activation of cyclin D1 promoter is ER
dependent, despite the HepG2 cells' containing low levels of ER unable to
trans-activate ERE-containing reporter genes. Altogether, these data indicate
that E2-induced cyclin D1 transcription is independent of the DBD
domain of ER (Marino et al.,
2002), and we have further demonstrated here that it depends on
the rapid/nongenomic effects. The effect of E2 on cyclin D1
promoter is present with the mutant -254, which still contains the Oct/Sp1 and
the CRE motifs but lacks the TRE, the E2F, and the E-box
(Herbert et al.,
1994). All these data sustain the notion that the effect of PI3K
pathway on the cyclin D1 promoter is addressed to the regulatory
elements present in this proximal promoter region. Thus, the E2-dependent
activation of cyclin D1 must be considered a multifactorial process
involving distinct regulatory elements localized in the cyclin D1
promoter (Sabbah et al.,
1999; Castro-Rivera et
al., 2001; Liu et
al., 2002), each of which can be affected by rapid/nongenomic
mechanisms.
In conclusion, E2 induces parallel signaling pathways, which, in turn, play
different roles in modulating HepG2 cell proliferation. In particular, the
E2-induced PKC- is strongly related to DNA synthesis but is not
involved in cyclin D1 promoter activity
(Marino et al.,
2002), which suggests that its role is focused on the steps after
cyclin D1 induction. Conversely, E2-induced MAP kinase and PI3K
pathways are strongly involved in both DNA synthesis and cyclin D1
promoter activity (Marino et al.,
2002 and present results). Altogether, these findings, summarized
in Figure 7, represent a new
model of E2-induced cell proliferation.
|
|
ACKNOWLEDGMENTS |
|---|
|
TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
|---|
* Corresponding author. E-mail address: m.marino{at}uniroma3.it.
|
REFERENCES |
|---|
|
TOPABSTRACTINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONACKNOWLEDGMENTSREFERENCES |
|---|
-Estradiol induces cyclin D1 gene
transcription, p36D1-p34cdk4 complex activation and
p105Rb phosphorylation during mitogenic stimulation of
G1-arrested human breast cancer cell. Oncogene
12,
2315-2324.[Medline]
Archer, T.K., Tam, S.P., and Deeley, R.G. (1986).
Kinetics of estrogen-dependent modulation of apolipoprotein A-I synthesis in
human hepatoma cells. J. Biol. Chem.
261,
5067-5074.
Archer, T.K., Tam, S.P., Deugau, K.V., and Deeley, R.G.
(1985). Apolipoprotein C-II mRNA levels in primate liver:
induction by estrogen in the human hepatocarcinoma cell line, HepG2. J.
Biol. Chem. 260,
1676-1681.
Bradford, M.M. (1976). A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal. Biochem. 772, 248-254.[CrossRef]
Cantley, L.C., and Neel, B.G. (1999). New insights
into tumor suppression: PTEN suppresses tumor formation by restraining the
phosphoinositide 3-kinase/AKT pathway. Proc. Natl. Acad. Sci.
USA 96,
4240-4245.
Caristi, S., Galera, J.L., Matarese, F., Imai, M., Caporali, S.,
Cancemi, M., Altucci, L., Cicatiello, L., Teti, D., Bresciani, F., and Weisz,
A. (2001). Estrogens do not modify MAP kinase-dependent nuclear
signaling during stimulation of early G(1) progression in human breast cancer
cells. Cancer Res. 61,
6360-6366.
Castoria, G., Barone, M.V., Di Domenico, M., Bilancio, A., Ametrano, D., Migliaccio, A., and Auricchio, F. (1999). Non-transcriptional action of oestradiol and progestin triggers DNA synthesis. EMBO J. 18, 2500-2510.[CrossRef][Medline]
Castoria, G., Migliaccio, A., Bilancio, A., Di Domenico, M., de Falco, A., Lombardi, M., Fiorentino, R., Varricchio, L., Barone, M.V., and Auricchio, F. (2001). PI3-kinase in concert with Src promotes the S-phase entry of oestradiol-stimulated M.C.F-7 cells. EMBO J. 20, 6050-6059.[CrossRef][Medline]
Castro-Rivera, E., Samudio, I., and Safe, S. (2001).
Estrogen regulation of cyclin D1 gene expression in Z.R-75 breast
cancer cells involves multiple enhancer elements. J. Biol.
Chem. 276,
30853-30861.
Chen, J., Lavigne, J.A., Trush, M.A., and Yager, J.D.
(1999). Increased mitochondrial superoxide production in rat
liver mitochondria, rat hepatocytes, and HepG2 cells following
ethinyl-estradiol treatment. Toxicol. Sci.
51,
224-235.
Coffer, P.J., Jin, J., and Woodgett, J.R. (1998). Protein kinase B (c-Akt): a multifunctional mediator of phosphatidylinositol 3-kinase activation. Biochem. J. 335, 1-13.
Couse, J.F., Lindzey, J., Grandien, K., Gustafsson, J.A., and
Korach, K.S. (1997). Tissue distribution and quantitative
analysis of estrogen receptor-alpha (ER) and estrogen receptor-beta
(ER) messenger ribonucleic acid in the wild-type and ER-knockout mouse.
Endocrinology 138,
4613-4621.
Farsetti, A., Moretti, F., Narducci, M., Misiti, S., Nanni, S.,
Andreoli, M., Sacchi, A., and Pontecorvi, A. (1998). Orphan
receptor hepatocyte nuclear factor-4 antagonises estrogen receptor-mediated
induction of human coagulation factor XII gene. Endocrinology
139,
4581-4589.
Foster, J.S., Henley, D.C., and Ahamed, S. (2001). Estrogens and cell-cycle regulation in breast cancer. Trends Endocrinol. Metab. 12, 320-327.[CrossRef][Medline]
Furnari, F.B., Huang, H.J., and Cavenee, W.K. (1998).
The phosphoinositol phosphatase activity of PTEN mediates a serum-sensitive G1
growth arrest in glioma cells. Cancer Res.
58,
5002-5008.
Furnari, F.B., Lin, H., Huang, H.S., and Cavenee, W.K.
(1997). Growth suppression of glioma cells by PTEN requires a
functional phosphatase catalytic domain. Proc. Natl. Acad. Sci.
USA 94,
12479-12484.
Graf, G.A., Roswell, K.L., and Smart, E.J. (2001).
17-Estradiol promotes the up-regulation of SR-BII in HepG2 cells and in
rat liver. J. Lipid Res. 42,
1444-1449.
Herbert, B., Truss, M., Beato, M., and Müller, R. (1994). Inducible regulatory elements in the human cyclin D1 promoter. Oncogene 9, 1295-1304.[Medline]
Improta-Brears, T., Whorton, A.R., Codazzi, F., York, J.D., Meyer,
T., and McDonnell, D.P. (1999). Estrogen-induced activation of
mitogen-activated protein kinase requires mobilization of intracellular
calcium. Proc. Natl. Acad. Sci. USA
96,
4686-4691.
Ivanova, T., Mendez, P., Garcia-Segura, L.M., and Beyer, C. (2002). Rapid stimulation of the PI3-kinase/Akt signalling pathway in developing midbrain neurones by oestrogen. J. Neuroendocrinol. 14, 73-79.[CrossRef][Medline]
Lee, A.V., and Yee, D. (1995). Insulin-like growth factors and breast cancer. Biomed. Pharmacother. 49, 415-421.[CrossRef][Medline]
Levin, E.R. (2002). Cellular functions of plasma membrane estrogen receptors. Steroids 67, 471-475.[CrossRef][Medline]
Liu, M.M., Albanese, C., Anderson, C.M., Hilty, K., Webb, P., Uht,
R.M., Price, R.H., Jr., Pestell, R.G., and Kushner, P.J. (2002).
Opposing action of estrogen receptors and on cyclin D1 gene
expression. J. Biol. Chem. 277,
24353-24360.
Lobenhofer, E.K., Huper, G., Iglehart, J.D., and Marks, J.R.
(2000). Inhibition of mitogen-activated protein kinase and
phosphatidylinositol 3-kinase activity in MCF-7 cells prevents
estrogen-induced mitogenesis. Cell Growth Differ.
11,
99-110.
Lupu, R., Cardillo, M., Cho, C., Harris, L., Hijazi, M., Perez, C., Rosenberg, K., Yang, D., and Tang, C. (1996). The significance of heregulin in breast cancer tumor progression and drug resistance. Breast Cancer Res. Treat. 38, 57-66.[CrossRef][Medline]
Maehama, T., and Dixon, J.E. (1998). The tumor
suppressor, PTEN/MMAC1, dephosphorylates the lipid second messenger,
phosphatidylinositol 3,4,5-trisphosphate. J. Biol. Chem.
273,
13375-13378.
Marino, M., Acconcia, F., Bresciani, F., Weisz, A., and
Trentalance, A. (2002). Distinct nongenomic signal transduction
pathways controlled by 17-estradiol regulate DNA synthesis and cyclin
D1 gene transcription in HepG2 cells. Mol. Biol.
Cell 13,
3720-3729.
Marino, M., Distefano, E., Pallottini, V., Caporali, S., Ceracchi,
G., and Trentalance, A. (2001a). -Estradiol stimulation of
DNA synthesis requires different PKC isoforms in HepG2 and MCF7 cells.
J. Cell. Physiol. 188,
170-177.[CrossRef][Medline]
Marino, M., Distefano, E., Trentalance, A., and Smith, C.L. (2001b). Estradiol-induced IP3 mediate the estrogen receptor activity expressed in human cells. Mol. Cell. Endocrinol. 182, 19-26.[CrossRef][Medline]
Migliaccio, A., Di Domenico, M., Castoria, G., de Falco, A., Contempo, P., Nola, E., and Auricchio, F. (1996). Tyrosine kinase/p21ras/MAP-kinase pathway activation by estradiol-receptor complex in MCF-7 cells. EMBO J. 15, 1292-1300.[Medline]
Myers, M.P., Pass, I., Batty, I.H., Van der Kaay, J., Stolarov,
J.P., Hemmings, B.A., Wigler, M.H., Downes, C.P., and Tonks, N.K.
(1998). The lipid phosphatase activity of PTEN is critical for
its tumor suppressor function. Proc. Natl. Acad. Sci. USA
95,
13513-13518.
Nadal, A., Ropero, A.B., Fuentes, E., and Soria, B. (2001). The plasma membrane estrogen receptor: nuclear or unclear? Trends Pharmacol. Sci. 22, 597-599.[CrossRef][Medline]
Nagata, D., Suzuki, E., Nishimatsu, H., Satonaka, H., Goto, A.,
Omata, M., and Hirata, Y. (2001). Transcriptional activation of
the cyclin D1 gene is mediated by multiple cis-elements, including
SP1 sites and a cAMP-responsive element in vascular endothelial cells.
J. Biol. Chem. 276,
662-669.
Norfleet, A.M., Thomas, M.L., Gametchu, B., and Watson, C.S.
(1999). Estrogen receptor- detected on the plasma membrane
of aldehyde-fixed GH3/B6/F10 rat pituitary tumor cells by enzyme-linked
immunocytochemistry. Endocrinology
140,
3805-3814.
Ramaswamy, S., Nakamura, N., Vazquez, F., Batt, D.B., Perera, S.,
Roberts, T.M., and Sellers, W.R. (1999). Regulation of G1
progression by the PTEN tumor suppressor protein is linked to inhibition of
the phosphatidylinositol 3-kinase/Akt pathway. Proc. Natl. Acad. Sci.
USA 96,
2110-2115.
Razandi, M., Oh, P., Pedram, A., Schnitzer, J., and Levin, E.R.
(2002). ERs associate with and regulate the production of
caveolin: implications for signaling and cellular actions. Mol.
Endocrinol. 16,
100-115.
Roger, P., Sahla, M.E., Makela, S., Gustafsson, J.A., Baldet, P.,
and Rochefort, H. (2001). Decreased expression of estrogen
receptor beta protein in proliferative preinvasive mammary tumors.
Cancer Res. 61,
2537-2541.
Ropero, A.B., Soria, B., and Nadal, A. (2002). A
nonclassical estrogen membrane receptor triggers rapid differential actions in
the endocrine pancreas. Mol. Endocrinol.
16,
497-505.
Russell, K.S., Haynes, M.P., Sinha, D., Clerisme, E., and Bender,
J.R. (2000). Human vascular endothelial cells contain membrane
binding sites for estradiol, which mediate rapid intracellular signaling.
Proc. Natl. Acad. Sci. USA 97,
5930-5935.
Sabbah, M., Courilleau, D., Mester, J., and Redeuilh, G.
(1999). Estrogen induction of the cyclin D1 promoter: involvement
of a camp response-like element. Proc. Natl. Acad. Sci. USA
96,
11217-11222.
Scheid, M.P., Marignani, P.A., and Woodgett, J.R.
(2002) Multiple phosphoinositide 3-kinase-dependent steps in
activation of protein kinase B. Mol. Cell. Biol.
22,
6247-6260.
Scheid, M.P., and Woodgett, J.R. (2001). PKB/AKT: functional insights from genetic models. Nat. Rev. Mol. Cell. Biol. 2: 760-768.[CrossRef][Medline]
Seo, H.S., and Leclercq, G. (2002). Evaluation of
potential implication of membrane estrogen binding sites on ERE-dependent
transcriptional activity and intracellular estrogen receptor-
regulation in MCF-7 breast cancer cells. J. Steroid Biochem. Mol.
Biol. 80,
109-123.[CrossRef][Medline]
Song, R.X.-D., McPherson, R.A., Adam, L., Bao, Y., Shupnik, M.,
Kumar, R., and Santen, R.J. (2002). Linkage of rapid estrogen
action to MAPK activation by ER-Shc association and Shc pathway
activation. Mol. Endocrinol.
16,
116-127.
Stein, R.C., and Waterfield, M.D. (2000). PI3-kinase inhibition: a target for drug development? Mol. Med. Today 6, 347-357.[CrossRef][Medline]
Stevis, P.E., Deecher, D.C., Suhadolnik, L., Mallis, L.M., and
Frail, D.E. (1999). Differential effects of estradiol and
estradiol-BSA conjugates. Endocrinology
140,
5455-5458.
Sun, M., Paciga, J.E., Feldman, R.I., Yuan, Z., Coppola, D., Lu,
Y.Y., Shelley, S.A., Nicosia, S.V., and Cheng, J.O. (2001).
Phosphatidylinositol-3-OH kinase (PI3K)/AKT2, activated in breast cancer,
regulates and is induced by estrogen receptor alpha (ER) via interaction
between ER and PI3K. Cancer Res.
61,
5985-5991.
Sutherland, R.L., Reddel, R.R., and Green, M.D. (1983). Effects of estrogens on cell proliferation and cell cycle kinetics: a hypothesis on the cell cycle effects of antiestrogens. Eur. J. Cancer Clin. Oncol. 19, 307-318.[CrossRef][Medline]
Tam, S.P., Hachè, R.J.G., and Deeley, R.G.
(1986). Estrogen memory effect in human hepatocytes during
repeated cell division without hormone. Science
234,
1234-1237.
Taylor, A.H., and Al-Azzawi, F. (2000). Immunolocalisation of oestrogen receptor beta in human tissues. J. Mol. Endocrinol. 24, 145-155.[Abstract]
Weng, L.P., Brown, J.L., and Eng, C. (2001). PTEN
coordinates G(1) arrest by down-regulating cyclin D1 via its
protein phosphatase activity and up-regulating p27 via its lipid phosphatase
activity in a breast cancer model. Hum. Mol. Genet.
10,
599-604.
Yamada, K.M., and Araki, M. (2001). Tumor suppressor
PTEN: modulator of cell signalling, growth, migration and apoptosis. J.
Cell Sci. 114,
2375-2382.
Zheng, J., Ali, A., and Ramirez, V.D. (1996). Steroids conjugated to bovine serum albumin as tools to demonstrate specific steroid neuronal membrane binding sites. J. Psychiatry Neurosci. 21, 187-197.[Medline]
This article has been cited by other articles:
|
|
 |
|
  I. Plo, C. Laulier, L. Gauthier, F. Lebrun, F. Calvo, and B. S. Lopez AKT1 Inhibits Homologous Recombination by Inducing Cytoplasmic Retention of BRCA1 and RAD51 Cancer Res., November 15, 2008; 68(22): 9404 - 9412. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 H. Roca, Z. Varsos, and K. J. Pienta CCL2 Protects Prostate Cancer PC3 Cells from Autophagic Death via Phosphatidylinositol 3-Kinase/AKT-dependent Survivin Up-regulation J. Biol. Chem., September 5, 2008; 283(36): 25057 - 25073. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 P. Galluzzo, P. Ascenzi, P. Bulzomi, and M. Marino The Nutritional Flavanone Naringenin Triggers Antiestrogenic Effects by Regulating Estrogen Receptor {alpha}-Palmitoylation Endocrinology, May 1, 2008; 149(5): 2567 - 2575. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
T. Wang, Y. Wang, Y. Kontani, Y. Kobayashi, Y. Sato, N. Mori, and H. Yamashita Evodiamine Improves Diet-Induced Obesity in a Uncoupling Protein-1-Independent Manner: Involvement of Antiadipogenic Mechanism and Extracellularly Regulated Kinase/Mitogen-Activated Protein Kinase Signaling Endocrinology, January 1, 2008; 149(1): 358 - 366. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 D. Gentilini, M. Busacca, S. Di Francesco, M. Vignali, P. Vigano, and A.M. Di Blasio PI3K/Akt And ERK1/2 signalling pathways are involved in endometrial cell migration induced by 17{beta}-estradiol and growth factors Mol. Hum. Reprod., May 1, 2007; 13(5): 317 - 322. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 P. Galluzzo, F. Caiazza, S. Moreno, and M. Marino Role of ER{beta} palmitoylation in the inhibition of human colon cancer cell proliferation Endocr. Relat. Cancer, March 1, 2007; 14(1): 153 - 167. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 D. M. McKay, J. L. Watson, A. Wang, J. Caldwell, D. Prescott, P. M. J. Ceponis, V. Di Leo, and J. Lu Phosphatidylinositol 3'-Kinase Is a Critical Mediator of Interferon-{gamma}-Induced Increases in Enteric Epithelial Permeability J. Pharmacol. Exp. Ther., March 1, 2007; 320(3): 1013 - 1022. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
M Marino, P Galluzzo, S Leone, F Acconcia, and P Ascenzi Nitric oxide impairs the 17{beta}-estradiol-induced apoptosis in human colon adenocarcinoma cells. Endocr. Relat. Cancer, June 1, 2006; 13(2): 559 - 569. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
F. Acconcia, C. J. Barnes, and R. Kumar Estrogen and Tamoxifen Induce Cytoskeletal Remodeling and Migration in Endometrial Cancer Cells Endocrinology, March 1, 2006; 147(3): 1203 - 1212. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 Z. T. Ruiz-Cortes, S. Kimmins, L. Monaco, K. H. Burns, P. Sassone-Corsi, and B. D. Murphy Estrogen Mediates Phosphorylation of Histone H3 in Ovarian Follicle and Mammary Epithelial Tumor Cells via the Mitotic Kinase, Aurora B Mol. Endocrinol., December 1, 2005; 19(12): 2991 - 3000. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 P. Totta, F. Acconcia, F. Virgili, A. Cassidy, P. D. Weinberg, G. Rimbach, and M. Marino Daidzein-Sulfate Metabolites Affect Transcriptional and Antiproliferative Activities of Estrogen Receptor-{beta} in Cultured Human Cancer Cells J. Nutr., November 1, 2005; 135(11): 2687 - 2693. [Abstract] [Full Text] [PDF] |
