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Previous Article | Next Article 
Molecular and Cellular Biology, September 2001, p. 5846-5856, Vol. 21, No. 17
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.17.5846-5856.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Role of Phosphoinositide 3-Kinase in the
Aggressive Tumor Growth of HT1080 Human Fibrosarcoma
Cells
Swati
Gupta,1
Selma
Stuffrein,1
Rina
Plattner,1,
Michael
Tencati,1
Christa
Gray,1
Young E.
Whang,2 and
Eric J.
Stanbridge1,*
Department of Microbiology and Molecular
Genetics, College of Medicine, University of California
Irvine,
Irvine, California 92697-4025,1 and
Department of Medicine, Lineberger Comprehensive Cancer Center,
School of Medicine, University of North Carolina, Chapel Hill,
North Carolina 27599-72952
Received 8 May 2001/Accepted 25 May 2001
 |
ABSTRACT |
We have developed a model system of human fibrosarcoma cell lines
that do or do not possess and express an oncogenic mutant allele of
N-ras. HT1080 cells contain an endogenous mutant allele of
N-ras, whereas the derivative MCH603 cell line contains
only wild-type N-ras. In an earlier study (S. Gupta et al.,
Mol. Cell. Biol. 20:9294-9306, 2000), we had shown that HT1080 cells
produce rapidly growing, aggressive tumors in athymic nude mice,
whereas MCH603 cells produced more slowly growing tumors and was termed weakly tumorigenic. An extensive analysis of the Ras signaling pathways
(Raf, Rac1, and RhoA) provided evidence for a potential novel pathway
that was critical for the aggressive tumorigenic phenotype and could be
activated by elevated levels of constitutively active MEK. In this
study we examined the role of phosphoinositide 3-kinase (PI 3-kinase)
in the regulation of the transformed and aggressive tumorigenic
phenotypes expressed in HT1080 cells. Both HT1080 (mutant
N-ras) and MCH603 (wild-type N-ras) have
similar levels of constitutively active Akt, a downstream target of
activated PI 3-kinase. We find that both cell lines constitutively
express platelet-derived growth factor (PDGF) and PDGF receptors.
Transfection with tumor suppressor PTEN cDNA into HT1080 and
constitutively active PI 3-kinase-CAAX cDNA into MCH603 cells,
respectively, resulted in several interesting and novel observations.
Activation of the PI 3-kinase/Akt pathway, including NF-
B, is not
required for the aggressive tumorigenic phenotype in HT1080 cells.
Activation of NF-B is complex: in MCH603 cells it is mediated by
Akt, whereas in HT1080 cells activation also involves other pathway(s)
that are activated by mutant Ras. A threshold level of activation of PI
3-kinase is required in MCH603 cells before stimulatory cross talk to
the RhoA, Rac1, and Raf pathways occurs, without a corresponding activation of Ras. The increased levels of activation seen were similar
to those observed in HT1080 cells, except for Raf and MEK, which were
more active than HT1080 levels. This cross talk results in conversion
to the aggressive tumorigenic phenotype. This latter observation is
consistent with our previous observation that overstimulation of the
activity of endogenous members of Ras signaling pathways, activated MEK
in particular, is a prerequisite for aggressive tumorigenic growth.
| |
INTRODUCTION |
Members of the Ras superfamily are
small GTP-binding proteins that function as activating transducers of
signaling pathways, whose members are commonly kinases or transcription
factors (3, 5). Three members of this family, namely,
H-ras, K-ras, and N-ras, have been
implicated in human cancers. Mutations in ras alleles have
been found in more than 30% of human cancers. The mutations invariably
result in chronic GTP binding to the Ras molecule and its consequent
chronic activation. This state results in constitutive activation of
Ras-dependent signaling pathways. Among these are the Raf, Rac1, RhoA,
and phosphoinositide (PI) 3-kinase signal transduction cascades
(29). These pathways have been shown to regulate
mitogenesis signals, motility and invasiveness, actin cytoskeletal
architecture, and cell survival, respectively (10, 21, 38,
39). Derangement of the normal regulation of these cellular
processes, as occurs when mutant Ras proteins are expressed, is
deleterious for the normal behavior of the cells in question and
contributes to the progression to a cancerous state.
A variety of experimental procedures, usually utilizing rodent cells,
have shown that downstream members of each of the signaling pathways
identified above, when mutated, function as transforming oncogenes
(23). Among these genes are PI 3-kinase and its
downstream target Akt, also known as protein kinase B
(2, 41). PI 3-kinase activates Akt, a serine threonine
kinase (25), which in turn phosphorylates a number of
substrates, including Bad, caspase 9, Forkhead transcription factors,
and IKK
(6, 9, 13, 33). Phosphorylation of Bad,
procaspase 9, and Forkhead transcription factors inactivates these
proapoptotic molecules, whereas phosphorylation of IKK activates
this kinase, leading eventually to activation of the antiapoptotic
NF-B transcription factor. Each of these substrates is implicated in
cell survival. One of the major cell survival factors is NF-B, whose
activation status is dependent upon binding to the IB protein. The
IB protein complexes with NF-B and sequesters it in the
cytoplasm, thereby preventing it from entering the nucleus. Degradation
of IB, following phosphorylation by IKK, releases NF-B, which
then enters the nucleus and activates its target genes (22, 40,
48). Activation of NF-B is associated with increased cell
survival and cell proliferation (4, 49, 50). One proposed
mechanism for the activation of IKK is phosphorylation mediated by Akt
(33, 42). However, other mechanisms also exist that do not
involve the degradation of IB (27, 44).
In addition to being activated by Ras-GTP, PI 3-kinase may also be
activated directly by contact with activated growth factor receptors,
including platelet-derived growth factor (PDGF) (20, 46).
Dysregulated PI 3-kinase activity is likely to play an important role
in cancer progression. One indication of this has been the
identification of the PTEN tumor suppressor gene (26, 45).
PTEN is a common target of inactivating mutations in a variety of
sporadic human cancers. In addition, germ line mutations in the PTEN
gene are associated with Cowden's disease, an inherited hamartoma
syndrome that includes an elevated risk of breast and thyroid cancers
(31). The PTEN protein functions as both a protein and a
lipid phosphatase. It is the lipid phosphatase activity that is
critical for its tumor-suppressing function (30). PTEN lipid phosphatase catalyzes the dephosphorylation of the 3 position of
PI 3,4,5-triphosphate (PIP3) and PI 3,4,-biphosphate (PIP2), both of
which are the lipid byproducts of the lipid kinase activity of PI
3-kinase. The Akt molecule binds to PIP3 via its pleckstrin homology
(PH) domain. In this complex with PIP3, Akt is then phosphorylated and
activated by the PI-dependent kinase, PDK-1 (1, 8). Thus,
normal cells integrate the activities of PI 3-kinase and PTEN to
facilitate homeostasis with respect to PI 3-kinase-mediated signal
transduction and cell cycle control. Overactivation of PI 3-kinase or
loss of PTEN function is likely to cause dysregulation of this finely
balanced control. An illustration of this is that expression of
wild-type PTEN transfected into PTEN-null cancer cells results in
induction of G1 arrest and/or apoptosis (12, 16).
Conversely, this arrest can be overridden by a constitutively active
form of Akt (52, 55).
We have developed an experimental model system comprising the human
fibrosarcoma cell line HT1080, which possesses one mutant N-ras allele, and its derivative, MCH603, which has deleted
the mutant allele and possesses only wild-type N-ras
(35). Examination of these cells has shown that HT1080 has
a typical transformed phenotype in culture, including disorganized
actin stress fibers and the ability to grow in soft agar, plus an
aggressive tumorigenic phenotype in vivo in immunodeficient mice. By
contrast, MCH603 cells have "reversed" their transformed phenotype;
they have restored a well-organized actin stress fiber distribution in
the cytoplasm and are no longer able to grow in soft agar. When
implanted into immunodeficient mice they continue to form tumors but
with much slower kinetics. We have described these cells as having a
weak tumorigenic phenotype (35).
When we examined the activation of a number of Ras signaling pathways,
namely, the Raf, Rac1, and RhoA pathways, we found that all members
were constitutively active in HT1080 but had basal activity in MCH603
cells (36). However, we noted that Akt was constitutively
active in both cell lines. Since this was not due to oncogenic Ras
expression in MCH603 cells, we looked for another explanation. In this
study we found that both cell lines constitutively synthesize and
secrete PDGF and contain cell surface PDGF receptor (PDGFR). Thus, this
provides a mechanism for constitutive activation of PI 3-kinase,
resulting in the activation of Akt.
Although HT1080 and MCH603 cells have different transformed and
tumorigenic phenotypes and yet both have constitutively active Akt, it
is formally possible that there may be quantitative and qualitative
differences in the activation of PI 3-kinase and/or Akt and their
downstream substrates in the two cell lines that play a role in the
expression of these phenotypes. In order to determine this, we have
modulated the activation of PI 3-kinase and Akt by stable transfection
of HT1080 and MCH603 cells with PTEN and an activated mutant of PI
3-kinase (hereafter termed PI3Kact), respectively.
Examination of the biochemical and biological properties of the
parental and transfectant cells has revealed several unexpected and
novel findings with respect to both signal transduction pathways and
biological behavior.
| |
MATERIALS AND METHODS |
Molecular constructs.
The expression plasmids used in
this study were as follows:
PI3Kact-pCMV(hyg)P110CAAX5'myc is derived from
pSG5P110CAAX5'myc (51) and encodes the catalytic
domain of PI 3-kinase. The constitutively active protein product,
PI3Kact, is permanently plasma membrane associated. The
construct pCDNA3PTEN(wt) (Neo) encodes a full-length wild-type PTEN
cDNA (52), whose expression is driven from a heterologous
cytomegalovirus promoter.
Cell culture and stable transfection.
The HT1080 cell line
has one mutant and one wild-type N-ras allele (28,
35). MCH603 is a variant of HT1080 and contains only wild-type
N-ras (35). The cell lines were maintained in Dulbecco minimal essential medium (DMEM) supplemented with 10% fetal calf serum (FCS; Life Technologies). The HT1080 and MCH603 cell
lines were transfected with the PTEN(wt) and PI3Kact
plasmids, respectively. Clones from each transfection were selected and
maintained in medium containing the relevant selective antibiotic (either 800 µg of Geneticin [Gibco-BRL] or 36 U of hygromycin B
[Calbiochem] per ml for the HT1080 and MCH603 transfectants, respectively). Subconfluent (70%) 100-mm dishes of MCH603 cells or
HT1080 cells were transfected with 5 µg of linearized DNA or vector
control DNA, using 30 µl of Lipofectin (Gibco-BRL) in Optimem medium
(Gibco-BRL).
Growth in soft agar.
Logarithmically growing cells
(104 or 106) were plated in single-cell
suspension in a 0.3% top agar overlay in DMEM supplemented with 10%
FCS, above a 0.5% bottom agar layer (in DMEM-10% FCS) in 60-mm
dishes as previously described (35). Plates were fed periodically with 1 ml of DMEM-10% FCS. Colonies (>0.1 mm) were inspected under the microscope and counted after 3 weeks.
Actin cytoskeleton staining and morphology.
Cells grown on
glass slides (Nunc) were washed with phosphate-buffered saline (PBS)
and fixed with 3.7% paraformaldehyde in PBS for 10 min. After a wash
with PBS, cells were permeabilized with PBS containing 0.1% Triton
X-100 for 5 min. The slides were then washed, and the actin stress
fibers were visualized by staining the cells with
fluorescein-conjugated phalloidin (0.005 U/µl; Molecular Probes) for
20 min at room temperature and mounted in ProLong Fade antifade
(Molecular Probes).
Immunoblot analyses.
Subconfluent cells were serum starved
for 18 h, and the cells were then lysed in lysis buffer comprised
of 1% sodium dodecyl sulfate (SDS) in 20 mM Tris (pH 7.4), 1 mM
CaCl2, 1 mM phenylmethylsulfonyl fluoride, and 0.2 mM
sodium orthovanadate. Total cell lysates, each containing 60 µg of
protein, were electrophoresed by SDS-7.5% polyacrylamide gel
electrophoresis (PAGE) and transferred to Immobilon-P membranes
(Millipore). The membranes were then probed with the relevant
antibodies. These included PDGFR- and PDGFR-
(Santa Cruz
Biotechnology), Akt/PKB, Phospho-Akt/PKB (Ser473), total Bad,
Phospho-Bad, total IB, and Phospho-IB (New England
Biolabs). Following incubation with horseradish peroxidase-conjugated
secondary antibody, bound proteins were detected by incubation with a
chemiluminescent detection system (Pierce) as previously described
(7). In order to test for secreted PDGF in the conditioned
medium, subconfluent HT1080 and MCH603 cells were exposed to serum-free
medium for 18 h. The conditioned medium was then concentrated in
the Centricon (Millipore) apparatus, followed by PAGE under reducing or
nonreducing conditions and immunoblotting, using PDGF-A (E-10) and
PDGF-B (P-20) antibodies (Santa Cruz Biotechnology).
Activated Ras, Rac1, and RhoA assays.
Subconfluent cells
were serum starved for 18 h and then lysed with 1 × Mg2+ lysis buffer (Ras and Rac Activation Assay Kits;
Upstate Biotechnology). Each cell lysate (500 µg) was affinity
precipitated with 10 µl of Raf-1 RBD, PAK-1 PBD agarose, or
glutathione S-transferase (GST)-C21-Sepharose conjugate
(43) at 4°C overnight for the Ras, Rac-Cdc42, or RhoA
activation assays, respectively. The beads were collected, washed, and
resuspended in 6× Laemmli sample buffer. Western blot analysis was
performed as described elsewhere (7), using 1 µg of
mouse monoclonal anti-Ras, anti-Rac1 (Upstate Biotechnology), and
anti-RhoA (Santa Cruz Biotechnology) antibodies per ml. Horseradish peroxidase-conjugated anti-mouse immunoglobulin G (Santa Cruz Biotechnology) was used as the secondary antibody. A chemiluminescence detection system (Pierce) was used for detection of the relevant proteins. To determine the total Ras, Rac1, or RhoA levels, immunoblots were performed using N-Ras(F155), Rac1(C-14), or RhoA(26C4) antibodies (Santa Cruz Biotechnology) that recognize total protein.
Kinase assays.
MEK, ERK, JNK, and Akt kinase assays were
performed according to the manufacturer's protocols (New England
Biolabs), using subconfluent cultures that had been serum starved
(0.25% FCS) for 18 h, and have been described elsewhere
(18). Briefly, cells were washed twice with PBS, scraped
into 500 µl of lysis buffer, and incubated on ice for 20 min. After
centrifugation at 14,000 × g for 20 min, the
supernatants were incubated with the relevant antibodies. The resulting
immunoprecipitates were employed in kinase assays. The activated MEK
assay was carried out by incubating immunoprecipitated phospho-MEK with
ERK protein and cold ATP (New England Biolabs MEK1/2Kinase Assay Kit).
The activated ERK assay was carried out by incubating
immunoprecipitated phospho-ERK with Elk-1 fusion protein and cold ATP
(New England Biolabs p44/p42 ERK Assay Kit). The JNK assays were
carried out by incubating the JNK-c-Jun fusion protein complex with
cold ATP (New England Biolabs JNK/SAPK Assay Kit). The Akt-P assay was
carried out by incubating the immunoprecipitated total Akt with GSK3
protein and cold ATP (New England Biolabs Akt Assay Kit). For MEK, ERK, and JNK assays, the relevant gel was transferred onto an Immobilon membrane, and Western blot analysis was performed. The blots were performed using phospho-ERK (Thr202/Tyr204) monoclonal antibody for the
MEK assay, phospho-Elk-1 (Ser383) polyclonal antibody for the ERK
assay, phospho-c-Jun (Ser63) polyclonal antibody for the JNK assay,
and phospho-GSK3 / (Ser219) rabbit polyclonal antibody for the
Akt assay. The Raf-1 assay was performed as described by Graham et al.
(17). For the Raf-1 assay, the
-32P-labeled mitogen-activated protein (MAP)
Kinase (ERK) proteins in the gel were visualized by autoradiography. To
determine the total Raf, MEK, ERK, JNK, and Akt levels, immunoblots
were performed using the respective antibodies that recognize total protein.
Elk-1 and NF-B luciferase reporter assays.
To measure
Elk-1 activation, a dual luciferase reporter assay kit (Promega) was
used as previously described (18). For NF-B assays,
approximately 2 × 105 parental HT1080 and MCH603
cells and the MCH603/PI3Kact or HT1080/PTEN stable
transfectant cells were cotransfected in six-well plates with the
pUC13-based 
56FosdE-luc plasmid (measures basal expression but is
not Ras responsive) and the NF-B reporter, (HIV-kB)3-luc
(54). The latter plasmid has three tandem copies of the
two adjacent NF-B sites from the human immunodeficiency virus
enhancer (six total tandem NF-B sites) inserted just upstream of the
minimal Fos promoter present in 56FosdE-luc. The
Effectene kit (Qiagen) was used for these transient transfections.
Following transfection, the cells were kept in serum-starved medium for 24 h. Tumor necrosis factor alpha (TNF-; 10 ng/ml) was then added to
the culture medium, and both treated and untreated control cultures
were incubated for a further 4-h period. The luciferase activity of
each sample was measured with the dual luciferase assay kit (Promega)
and normalized with an internal control Renilla luciferase.
Tumorigenicity assays.
Cells were trypsinized and
resuspended in 0.2 ml of DMEM, and then 107 cells were
injected subcutaneously into the flanks of 4- to 6-week-old nude
athymic mice. Tumors were measured in three dimensions with linear
calipers at weekly intervals.
| |
RESULTS |
We have shown previously that HT1080 (mutant N-ras)
cells have constitutively active Raf-dependent (Raf/MEK/ERK/Elk-1),
Rac1 (Rac1/Cdc42/JNK), and RhoA signaling pathways (18).
Conversely, MCH603 (wild-type N-ras) cells have basal levels
of activity of these signal transduction proteins (18).
Interestingly, both HT1080 and MCH603 cells have significant levels of
constitutively active Akt. The fact that MCH603 does not possess a
mutant ras allele and yet has constitutively active levels
of Akt, approximating those found in HT1080 cells, infers an
alternative mechanism of chronic activation.
HT1080 and MCH603 constitutively secrete PDGF.
Concentrated
conditioned media and cell lysates from both HT1080 and MCH603
serum-starved cell cultures were electrophoresed and immunoblotted with
antibodies to PDGF-A and PDGF-B. Both forms of PDGF were expressed at
similar levels by both cell types. However, whereas PDGF-A is secreted
into the medium, PDGF-B remains associated with the cells (Fig.
1A). Analyses of PDGF dimers under
nonreducing conditions indicated that the predominant secreted form is
PDGF-AA (data not shown). Immunoblotting of cell lysates showed
that both the and forms of the PDGFR are expressed (Fig. 1B).
Constitutive secretion of PDGF-A and subsequent binding to and
activation of its cognate receptor is, therefore, the
probable mechanism for downstream activation of PI 3-kinase and
Akt. It is known that the catalytic subunit of PI 3-kinase associates
with, and is activated by, the autophosphorylated PDGFR (20, 34,
46).
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FIG. 1.
Western blot analysis performed on HT1080 and MCH603
cell lysates or their respective conditioned media to determine the
levels of secreted PDGF-A and PDGF-B (A) or surface membrane-bound
PDGFR- and PDGFR- (B). HT, HT1080; 603, MCH603; CM, conditioned
medium.
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Modulation of PI 3-kinase and Akt/PKB activity. (i) HT1080
cells.
We wished to downregulate constitutive activity of PI
3-kinase and/or Akt in HT1080 cells. Initially, we attempted
downregulation of PI 3-kinase activity via stable transfection with PI
3-kinase dominant-negative cDNAs. Unfortunately, none of the constructs tested (24) had the desired effect (data not shown). Thus,
we resorted to expressing the tumor suppressor protein PTEN in these cells. PTEN is a dual-specificity phosphatase that catalyzes the dephosphorylation of PIP3, thereby inhibiting the activation of Akt
(30). As shown in Fig. 2A,
severalfold-higher levels of expression of PTEN were observed in the
HT1080/PTEN stable transfectants, compared to parental HT1080 cells.
Correspondingly, there was a decline in the level of expression of
activated phospho-Akt. This decline in activity was confirmed in Akt
assays (Fig. 3A).
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FIG. 2.
Western blot analysis of the cell lysates from
HT1080/PTEN transfectants (A) and MCH603/PI3Kact
transfectants (B) to determine the levels of PTEN (A), myc-tagged PI
3-kinase (B), phospho-Akt, and total Akt. Three independent HT1080/PTEN
and MCH603/PI3Kact clones were analyzed. The fold level of
the individual proteins (PTEN and phospho-Akt) is relative to 1.0 for
HT1080 control cells. HT, HT1080; 603, MCH603.
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FIG. 3.
In vitro Raf, MEK, ERK, and JNK kinase assays and Elk-1
activation assays performed on HT1080/PTEN (A) and
MCH603/PI3Kact (B) transfectants. For the kinase assays the
fold level is relative to 1.0 for HT1080 control cells, and for the
Elk-1 luciferase reporter the activities are expressed as the percent
relative to 100% for HT1080. Three independent HT1080/PTEN clones and
MCH603/PI3Kact clones were analyzed. HT, HT1080; 603, MCH603; V, vector only (control). The error bars indicate the standard
deviations.
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(ii) MCH603 cells.
Although these cells already express
significant levels of constitutively active Akt, and presumably PI
3-kinase, we wanted to elevate the activity levels even further in
order to determine if this may have an effect on in vitro transformed
phenotypic traits and in vivo tumorigenicity. To accomplish this,
MCH603 cells were stably transfected with a constitutively activated PI
3-kinase-CAAX expression vector (PI3Kact) that contains a
myc epitope tag. As shown in Fig. 2B, the transfectants express high levels of the myc epitope tag and,
correspondingly, higher levels of activated Akt.
Effects on other Ras-dependent signaling pathways. (i)
HT1080/PTEN cells.
The lipid phosphatase activity of
PTEN dephosphorylates phosphoinositides and would be expected to have
inhibitory effects on PI 3-kinase-mediated activation of RhoA-, Rac1-,
and Raf-dependent signaling pathways. The protein phosphatase acivity
of this dual-specificity phosphatase may also have PIP3-independent
effects on signal transduction. In the case of the HT1080/PTEN
transfectants, however, levels of constitutively active RhoA, Rac1, and
JNK and members of the Raf-dependent pathway (Raf/MEK/ERK/Elk-1)
remained high, approximating the levels found in parental HT1080 cells
(Fig. 3A and 4). These levels of
constitutive activity are presumably mediated by the mutant N-Ras
protein (see Fig. 3A) in a PI 3-kinase-independent manner.
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FIG. 4.
Pull-down assays of activated Ras, Rac, and Rho. The
GTP-bound forms of Ras, Rac, and Rho were pulled down with GST fusion
proteins, corresponding to the Ras-binding domain of Raf-1 (Raf-1 RBD),
the p21-binding domain (PBD) of human PAK-1, and the C21 binding
domain of Rho, respectively, conjugated to agarose beads. The
Ras-GTP, Rac-GTP, and Rho-GTP proteins bound to the beads were
identified using anti-Ras (A), anti-Rac (B), and anti-Rho (C)
antibodies, respectively, in a Western immunoblot. Immunoblot analysis
of total cell lysates identified the levels of total protein.
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(ii) MCH603/PI3Kact cells.
Clear evidence of
activation of multiple signaling pathways was found in these cells
(Fig. 3B and 4). Persistent activation of RhoA, Rac1, and JNK and
members of the Raf-dependent pathway (Raf/MEK/ERK/Elk-1) were observed.
However, no activation of Ras was seen (Fig. 4A). Thus, the activation
of these pathways was independent of Ras activation and was due either
to direct signaling from activated PI 3-kinase or via cross talk
between members of the distinct pathways. Quantitation of the levels of
activity of the various members of the signaling pathways examined
revealed approximately twofold-higher levels of Akt activity in the
transfectants, as expected. Levels of activated RhoA and Rac1
approximated that seen in HT1080 cells. A modest but reproducible
increase in levels of activated Raf-1 (approximately 1.5-fold) and MEK
(1.5- to 1.8-fold) over that seen in HT1080 was observed. The levels of
activated ERK and Elk-1 were approximately the same as seen in the
HT1080 cells. All levels of constitutive activity were markedly higher than those found in the parental MCH603 cells.
Effects on NF-B activation.
Akt activation, either mediated
by PI 3-kinase or other signal transduction pathways, has been shown to
be an antiapoptotic survival factor via activation of NF-B and/or
Bad (2, 27, 42). This property may well contribute to the
tumor-forming properties of cancer cells. Thus, we wished to determine
if activation or downregulation of the activities of these factors
affected the tumorigenic phenotypes of HT1080 and MCH603 cells. Akt
activation has been reported to activate NF-B via IB degradation
(33, 42), although other mechanisms of activation have
been reported (27, 44). In our studies we examined the
status of IB- and NF-B in the parental and transfectant cells.
(i) IB- phosphorylation.
Degradation of IB subunits
is facilitated by their phosphorylation by IKK (22, 40,
48). Thus, the level of phosphorylated IB-, relative to
the levels of total IB- protein, is indicative of the degradative
process. In Fig. 5A we see that HT1080
and MCH603 have comparable levels of phospho-IB- relative to the total IB protein levels. In contrast, the HT1080/PTEN transfectants clones have reduced levels of phospho-IB-. Interestingly, the levels of total IB- protein increased in these transfectants. Presumably, this is due to the increased stability of the
unphosphorylated IB-. Thus, lowered Akt activity, mediated by the
PTEN lipid phosphatase, results in decreased degradation of IB-.
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FIG. 5.
Western blot analysis performed on HT1080/PTEN
transfectants (A) and MCH603/PI3Kact (B) transfectants to
determine the levels of phospho-IkB and total IkB in these cells.
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The MCH603/PI3Kact transfectants exhibit the opposite
characteristics. Increased levels of phospho-IB- were seen (Fig.
5B) with correspondingly greatly reduced levels of total IB-
protein. This is consistent with the increased levels of constitutive
Akt activity in these transfectants (Fig. 1B) and is indicative of an
increased rate of degradation of IB- protein, presumably resulting in a release of IB-bound NF-B.
(ii) NF-B activation. The levels of NF-B activity in
the parental and transfectant cells were assayed, using an NF-B reporter assay (54). The relative fold activity was
determined using an internal control, the 56FosdE-luc expression vector.
Consistent with their essentially equal levels of constitutive Akt
activity, HT1080 and MCH603 cells had approximately the same fold
NF-B activities. In the HT1080/PTEN transfectants the level of
activated NF-B decreased but did not decline to the level seen in
normal human diploid fibroblast (HDF) cells (Fig. 6A). Since the RhoA, Rac1, and Raf
signaling pathways remain constitutively active in HT1080 cells, we
interpret this to indicate that activation of NF-B occurs via
Akt-dependent and -independent pathways in these cells. In an attempt
to clarify this further, we treated the various cell lines with
TNF-, a cytokine that stimulates NF-B activation via multiple
pathways (15, 22). Both HT1080 and HT1080/PTEN NF-B
activity levels were elevated by TNF-, whereas the level of NF-B
activity in MCH603 cells was unaffected by TNF- (Fig. 6B). However,
the level of NF-B activity in the MCH603/PI3Kact
transfectants was substantially increased in the presence of TNF-
(Fig. 6B). It should be noted here that the MCH603/PI3Kact
cells possess constitutively active RhoA, Rac1, and Raf pathways but
not constitutively active Ras (Fig. 3 and 4). Taken together, these
data suggest that NF-B activation in MCH603 cells is Akt dependent,
whereas in HT1080 and MCH603/PI3Kact cells activation is
mediated by both Akt-dependent and independent pathways.
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FIG. 6.
In vitro luciferase reporter assays were performed to
determine NF-B activities in HT1080, HT1080/PTEN, MCH603, and
MCH603/PI3Kact cells with (B) or without (A)
TNF- (TNF) treatment. Normal HDFs were used as a control
for basal level activity. The NF-B luciferase reporter activities
are presented as the average fold activation. HT, HT1080; 603, MCH603.
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Effects on Bad.
Another mechanism whereby activated Akt may
function as a survival factor is by phosphorylating the proapoptotic
protein Bad, thereby inactivating it and inhibiting the
Bad-mediated apoptotic pathway (13). This is, indeed, what
was observed: the levels of phosphorylated Bad decreased in the
HT1080/PTEN transfectants and increased in the
MCH603/PI3Kact transfectants, relative to their respective
parental cells (Fig. 7).
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FIG. 7.
Western blot analysis performed on HT1080/PTEN
transfectants (A) and 603/PI3Kact transfectants (B) to
determine the level of Phospho-Bad and total Bad in these cells
relative to the levels in the parental HT1080 and MCH603 cells.
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|
Biological effects of modulating PI 3-kinase and Akt activity.
Activation of PI 3-kinase has been shown to have dramatic effects on
the biological behavior of cells, including the transformation of
rodent cells (24). We therefore examined a number of
phenotypic traits expressed in culture that are associated with
neoplastic transformation, plus tumorigenic growth in vivo.
(i) Actin stress fibers.
We had earlier shown
(18), as is illustrated in Fig. 8A and
B, that HT1080 cells have disorganized
actin, whereas MCH603 cells have restored an extensive cytoskeleton of
actin stress fibers. There was no restoration of actin stress fibers in
the HT1080/PTEN transfectants (Fig. 8C). Thus, it appears that
phosphoinositide-mediated activation of the Akt pathway is not the
determining factor with respect to regulation of actin stress fiber
formation. However, as seen in Fig. 8D, increased activation of Akt in
the MCH603/PI3Kact transfectants is associated with a
dramatic loss of actin stress fibers. It should be noted that these
cells have also constitutively activated RhoA, Rac1, and
Raf/MEK/ERK/Elk-1 signaling pathways (Fig. 3 and 4) and, therefore,
more closely resemble HT1080 cells in this regard.
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FIG. 8.
Actin stress fiber organization in HT1080, MCH603,
HT1080/PTEN, and MCH603/PI3Kact cells. The cells
were stained with fluorescein-conjugated phalloidin. Magnification,
×160.
|
|
(ii) Anchorage-independent growth. Our earlier studies had
shown that HT1080 cells grow well in soft agar, whereas MCH603 cells
are incapable of forming colonies in this medium (18).
Downregulation of constitutive Akt activity in the HT1080/PTEN transfectants had no effect on this ability to form colonies in soft
agar (Fig. 9), whereas
MCH603/PI3Kact transfectants had a partially restored
ability to grow. Colonies were able to form when cells were plated at
high density (106 cells per dish) but not when plated at
low density (104 cells per dish). The HT1080 cells form
colonies at both plating densities. It should again be noted that the
expression of PI3Kact in the transfectants activates the
RhoA, Rac1, and Raf/MEK/ERK/Elk-1 signaling pathways (Fig. 3 and 4).
These same pathways remain constitutively active in the HT1080/PTEN
transfectants. Thus, the partial restoration of anchorage-independent
growth is not dependent on the constitutive activity of Akt per se but
is associated with activation of other Ras-associated signaling
pathways.
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FIG. 9.
Anchorage-independent assays. Totals of 104
cells (A) or 106 cells (B) were plated per 60-mm petri dish
in soft agar. Colonies (>0.1 mm) were counted after incubation for 3 weeks at 37°C, with periodic refeeding with fresh growth medium. The
error bars indicate standard deviations.
|
|
(iii) Tumor formation.
HT1080 and MCH603 cells both form
tumors in immune-deficient mice. However, the kinetics of tumor
formation differ dramatically. HT1080 cells form aggressively
growing tumors that reach a large size within 3 weeks, whereas MCH603
cells form tumors much more slowly. We have termed these phenotypes as
aggressive and weak tumorigenic phenotypes, respectively (18,
35). Stable elevated levels of expression of the tumor
suppressor protein PTEN in HT1080/PTEN transfectants had no effect on
the aggressive tumorigenic phenotype (Fig.
10A). Conversely, elevated levels of
activated PI 3-kinase protein in the MCH603/PI3Kact
transfectants resulted in a conversion from a weak to an aggressive tumorigenic phenotype, albeit not one as aggressive as that seen with
HT1080 and HT1080/PTEN cells (Fig. 10B). As with the other biological
phenotypes examined, the aggressive and weak tumorigenic phenotypes
cannot be a direct consequence of PI 3-kinase or Akt activity. Thus,
the antiapoptotic function of NF-B and inactivation of the
proapoptotic factor, Bad, do not seem to influence the aggressive and
weak tumorigenic phenotypes of HT1080 and MCH603, respectively. As
discussed in more detail below, the activation of MEK in the
MCH603/PI3Kact transfectants is a likely candidate for
orchestrating the conversion from weak to aggressive tumor-forming
ability.
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FIG. 10.
Tumorigenicity assays of HT1080, MCH603, HT1080/PTEN,
and 603/PI3Kact cells. Each point is the average size of
the tumor sizes of all sites inoculated (total of 6 for the parental
cells and 18 for the transfectants, combining three independent
clones).
|
|
| |
DISCUSSION |
We have developed an experimental model system that utilizes the
HT1080 human fibrosarcoma cell line, possessing a mutant N-ras allele, and its derivative, MCH603, in which the
mutant N-ras allele has been deleted (35). In
the HT1080 cells all Ras-dependent pathways examined, namely, the Raf,
Rac1, RhoA, and PI 3-kinase/Akt pathways, were constitutively active,
presumably as a consequence of the permanent activated status of the
mutant N-Ras protein (18). In contrast, the derivative
MCH603 cells exhibit only basal levels of activity of these pathways,
with the singular exception of Akt and p38 MAP kinase. We show here that this is probably due to constitutive expression of PDGF and the
activation of its cognate PDGFR.
Elevated levels of expression of the lipid phosphatase PTEN protein in
HT1080 cells resulted in a significant decrease in activity of Akt.
This indicates that the constitutive activation of Akt is mediated via
PI 3-kinase generated PIP3, rather than some other pathway, for example
Ca2+-calmodulin-dependent protein kinase II
(53). Although Akt activity was significantly decreased,
the levels of constitutive activity of the RhoA-, Rac1-, and
Raf-dependent pathways remained high. Presumably, this is due to the
continued stimulation by the endogenous mutant N-Ras protein, whose
constitutive activity was unaffected by PTEN.
It is interesting that elevated levels of expression of the PTEN
protein did not affect the proliferation of the HT1080/PTEN transfectants, since others have reported that overexpression of PTEN
induces G1 arrest and/or apoptosis (12, 16).
However, most of these studies employed transient-transfection
methodologies. Also, the cell lines examined were null for PTEN
activity (37). Stable transfections of endogenous
wild-type PTEN glioma cells with wild-type PTEN cDNA and its subsequent
overexpression did not noticeably affect the proliferation of the cells
in culture (16). We experienced a similar lack of effect
on the growth of HT1080 cells, which are PTEN wild type (data not
shown), even though the HT1080/PTEN transfectants express
severalfold-higher levels of PTEN protein than the endogenous levels of
wild-type PTEN expressed in HT1080. However, the increased levels of
PTEN protein did correspond with a decrease in Akt activity. This
suggests that the physiological level of endogenous wild-type PTEN in
both HT1080 and MCH603 cells did not influence the PIP3-mediated
constitutive activation of Akt and further suggests that a threshold
level of PTEN protein is required for its inhibitory effect.
Elevating the level of activity of PI 3-kinase in the
MCH603/PI3Kact transfectants had dramatic effects on the
constitutive activities of other putative Ras-dependent pathways
examined. The RhoA-, Rac1-, and Raf-dependent pathways were all
activated, presumably in an activated PI 3-kinase-dependent fashion
involving positive cross talk (47, 51). Interestingly,
endogenous Ras was not activated. There has been some debate as to
whether low or high levels of activated PI 3-kinase stimulate the
activation of Ras (51). In these cells there is clearly no
activation of endogenous Ras: thus, PI 3-kinase-mediated activation of
these "Ras-dependent" pathways occurs downstream of Ras. It is
noteworthy that activation of members of the Raf pathway, in particular
MEK, exceeded the levels seen in HT1080 cells even though Ras itself
was not activated.
The fact that MCH603 cells have significant levels of Akt activity,
which is PI 3-kinase mediated, and yet do not exhibit activation of the
RhoA-, Rac1-, and Raf-dependent pathways, suggests that a threshold
level of activation is required to initiate the cross talk activation
of multiple pathways. Whether this reflects an on/off switch to the
activated state, as posited by Ferrell (14), will require
further experimentation to determine.
PI 3-kinase-mediated activation of Akt and its subsequent upregulation
of the activity of the transcription factor, NF-B, have been shown
to be important modulators of antiapoptotic cell survival (33,
42). Additionally, both Akt and PI 3-kinase, in their activated
form, have been shown to have transforming activity in experimental
rodent and avian cell systems (2, 11, 24).
Examination of NF-B activity in the HT1080 and MCH603 parental and
HT1080/PTEN and MCH603/PI3Kact transfectant cells revealed
evidence of complex, multiple pathways of regulation. The complexity of
NF-B activation has been addressed by many investigators. Activation
may be effected by oncogenic Ras through Raf-dependent and
Raf-independent MAP kinase signaling pathways (15, 19,
32). The Raf-independent pathway appears to signal via Rac and
p38 or a closely related kinase. Raf-dependent activation also
converges with Raf-independent activation at the level of p38
activation. Furthermore, activation may be effected by PI 3-kinase,
either as a consequence of activation of PI 3-kinase by oncogenic Ras
or independently of Ras (27, 44).
In the case of the parental HT1080 and MCH603 cells, the basal levels
of NF-B activity were similar and significantly higher than those of
normal HDFs. The fact that HT1080 and MCH603 cells have similar levels
of constitutive activity of NF-B under conditions of serum
starvation is interesting, given that HT1080 has the capacity to
stimulate activity via oncogenic Ras-dependent signaling, as well as
PDGF-mediated PI 3-kinase and Akt signaling, whereas MCH603 cells
possess only the latter mechanism. This presumably reflects an upper
threshold level of activity under this physiological condition. In both
HT1080 and MCH603 cells, activation of NF-B appears to be associated
with, and presumably dependent upon, IB degradation and the release
of NF-B sequestered in the cytosol. The parental HT1080 and MCH603
cells, however, differ dramatically in their responsiveness to TNF-
stimulation of NF-B activity. Whereas the activity in HT1080 cells
is amplified manyfold, the activity in MCH603 cells is unaltered, as is
the case with HDF cells. Thus, it would seem that TNF- stimulatory
effects are mediated only through oncogenic Ras or one or more
downstream signaling partners, independently of PI 3-kinase-mediated
Akt activation.
Support for this notion is given by the fact that elevated PTEN
expression in HT1080/PTEN transfectants reduces the level of
constitutive NF-B activity below that seen in MCH603 cells but not
to the level seen in HDFs. This indicates that the constitutive activation of NF-B in HT1080 is dependent on both PI 3-kinase/Akt and oncogenic Ras signaling. Also, overexpression of activated PI
3-kinase in MCH603/PI3Kact transfectants results in levels
of constitutive NF-B activity that are somewhat higher than those
seen in MCH603 or HT1080 cells. In these cells exposure to TNF- does
result in an amplification of NF-B activity to levels approximating
those seen in TNF--stimulated HT1080 cells. This result is
consistent with the observation that the RhoA, Rac1 and Raf signaling
pathways all become constitutively activated in these transfectants. It
also indicates that Ras-GTP per se is not directly required for
TNF--mediated stimulation.
A major goal of this study was to determine whether constitutive
activation of PI 3-kinase and Akt contributed to the aggressive tumorigenic phenotype of HT1080 fibrosarcoma cells. Our data, which are
summarized in Fig. 11, clearly
demonstrate that downregulation of this antiapoptotic survival pathway
does not demonstrably affect the aggressive tumorigenic phenotype in
HT1080/PTEN transfectants. The fact that the HT1080/PTEN transfectants
retain the oncogenic Ras-dependent constitutive activation of the RhoA,
Rac1, and Raf signaling pathways seems the most likely mechanism for
retaining the aggressive tumorigenic phenotype. Consistent with this
notion is the observation that overexpression of activated PI 3-kinase in the MCH603/PI3Kact transfectants results in constitutive
activation of the RhoA-, Rac1-, and Raf-dependent signaling pathways,
accompanied by a conversion from the weak to the aggressive tumorigenic
phenotype (Fig. 11).
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FIG. 11.
Summary of levels of constitutive activity of members
of the PI 3-kinase, RhoA, Rac1, and Raf signaling pathways and of the
tumorigenic phenotypes in parental HT1080 and MCH603 cells and their
respective transfectants, HT1080/PTEN and MCH603/PI3Kact.
*, Proteins constitutively active in HT1080 or MCH603;  or  , decrease or increase, respectively, in the constitutive
activity of individual factors tested in HT1080/PTEN and
MCH603/PI3Kact relative to their respective parental cells;
, activity higher than that seen in HT1080 cells;  , not
tested.
|
|
In earlier studies we have shown that, in the absence of mutant N-Ras
in the MCH603 cells, overexpression of activated MEK results in the
conversion to an aggressive tumorigenic phenotype (18).
This overexpression, coupled with a lack of effect when activated Raf
or Rac1 were expressed, led us to speculate that the overexpression of
activated MEK in these cells stimulated the activation of a possibly
novel pathway that is critical for the conversion to an
aggressive tumorigenic phenotype. Consistent with this notion is the
observation in this study that the levels of endogenous activated MEK
in MCH603/PI3Kact transfectants are higher than that seen
in HT1080 cells. Thus, the same putative novel pathway may be
activated in these cells. Further experimentation is required to test
this hypothesis.
The generality of the phenomena described here with respect to other
human cancers and cell lines must await further examination. If a novel
pathway is confirmed and found to be general for human cancers that
express mutant Ras proteins, this may provide an important target for
cancer therapy.
| |
ACKNOWLEDGMENTS |
We thank Julian Downward and Craig Hauser for the gifts of
plasmids and Albert Baldwin, Jr., for critical reading of the manuscript.
These studies were supported by NCI grants CA69515 (E.J.S.) and CA85772
(Y.E.W.) and DOD grant DAMD17-00-1-0037.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Microbiology and Molecular Genetics, University of California, Irvine, College of Medicine, 240 Med. Sci. Bldg. I, Bldg. B, Irvine, CA 92697-4025. Phone: (949) 824-7042. Fax: (949) 824-8598. E-mail: ejstanbr{at}uci.edu.
Present address: Department of Pharmacology and Cancer Biology Duke
University Medical Center, Durham, NC 27710.
| |
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Molecular and Cellular Biology, Septembe
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Abstract
Introduction
