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Department of Anatomy and Cell Biology and The Cardiovascular Center, The University of Iowa College of Medicine, Iowa City, Iowa 52242
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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The mechanisms of nitric oxide (NO)-mediated
inhibition of vascular smooth muscle (VSM) cell proliferation are still
obscure. Cyclins A and E in association with cyclin-dependent kinase 2 (cdk2) serve as positive regulators for mammalian cell cycle
progression through the G1/S
checkpoint of the cell cycle and subsequent cell proliferation.
Therefore, we have tested the effect of adenovirus-mediated transfection of the endothelial nitric oxide synthase (eNOS) gene into
guinea pig coronary VSM cells on platelet-derived growth factor (BB
homodimer) (PDGF-BB)-stimulated cell proliferation and the expression
of cell cycle regulatory molecules. Transfection of the eNOS gene
(eNOS) into VSM cells significantly
inhibited (P < 0.05)
[3H]thymidine
incorporation into the DNA in response to PDGF-BB stimulation compared
with lacZ-transfected control cells.
The eNOS transfer significantly
inhibited (P < 0.05) PDGF-BB-induced proliferating cell nuclear antigen (PCNA) and cyclin A expression in
VSM cells compared with cells transfected with the control vector. The
time course of cyclin E expression in response to PDGF-BB stimulation
was delayed in eNOS-transfected cells.
Levels of cyclin-dependent kinase inhibitors p21 and p27 were not
significantly affected by eNOS
transfer. eNOS transfer did not
decrease PDGF-
receptor number, affinity, and autophosphorylation
measured by radioreceptor assay and Western analysis. These results
suggest that inhibition of PDGF-stimulated expression of cyclin A,
cyclin E, and PCNA is the target of NO action. These findings could
explain, at least in part, NO-mediated inhibition of VSM cell proliferation.
adenovirus-mediated gene transfer; endothelial nitric oxide synthase; proliferating cell nuclear antigen; cyclins; [3H]thymidine incorporation; coronary arteries
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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THE HALLMARKS of coronary artery restenosis after angioplasty are migration and proliferation of vascular smooth muscle (VSM) cells from the media to form a neointima (24, 27). This neointima formation is also a fundamental step in aggravation of atherosclerosis (24, 27). Under physiological conditions, endothelial cells produce nitric oxide (NO) that regulates smooth muscle cell activities, such as migration, proliferation, and vascular tone (reviewed in Refs. 24 and 27). These regulatory effects are lost in vascular diseases due to damage of the endothelial cells (24, 25, 27). Experimental evidence supports the concept that NO maintains normal vascular architecture and hemodynamics and inhibits VSM cell proliferation and migration to retard vascular wall thickening (10, 24-27). NO donors and high concentrations of L-arginine have been shown to retard neointima formation in response to injury in rat carotid arteries (14, 17). Similarly, our laboratory (11) and von der Leyen and colleagues (34) have shown that endothelial NO synthase (eNOS) gene transfection to medial VSM cells at the time of balloon catheter injury to rat carotid artery decreases intimal VSM cell hyperplasia and neointima size. In cultured VSM cells, NO donors inhibit VSM cell proliferation and migration (10, 18, 26). All these reports support the concept that NO released from the endothelial cell plays an important role in maintaining VSM cells in a nonproliferating state. However, the underlying molecular mechanisms of NO-mediated inhibition of VSM cell proliferation are not fully understood.
Progression through the mammalian mitotic cycle is controlled by multiple holoenzymes composed of a catalytic subunit named cyclin-dependent kinase (cdk) and a regulatory subunit called cyclin (reviewed in Ref. 12). Functional cdk/cyclin holoenzymes are formed and activated at specific stages in the cell cycle. Mitogenic factors bind to receptors and initiate a series of events that result in the expression of cyclins and/or suppression of cyclin-dependent kinase inhibitors (CKI). This leads to the activation of cdks that in turn regulate cell cycle progression and mitosis (9, 12, 19). Recently, Wei et al. (35) demonstrated that VSM cell proliferation after arterial injury is associated with a temporally and spatially coordinated activation of cdk2 and expression of cyclins E and A and proliferating cell nuclear antigen (PCNA) in the rat carotid artery. In addition, a number of investigators have demonstrated that transfection of VSM cells with antisense oligonucleotides to cell cycle control genes (1, 20, 21) or adenovirus-mediated overexpression of negative cell cycle progression molecules, i.e., the constitutively active form of retinoblastoma gene product (pRB) (6), or the cyclin-dependent kinase inhibitor p21 (5) inhibits VSM cell proliferation and neointima formation. Although these results demonstrate the importance of cyclins and PCNA in VSM cell proliferation, the regulation of these molecular events in response to eNOS transfection in VSM cells remains unknown.
The major goal of the present study was to test the hypothesis that eNOS transfer into VSM cells inhibits platelet-derived growth factor (BB homodimer) (PDGF-BB)-stimulated cell proliferation by inhibiting growth factor-induced expression of cell cycle progression molecules. The data presented in this report show that infection of VSM cells with replication-deficient adenovirus vector containing bovine eNOS (Ad5/RSVeNOS) produces a dose [1-200 plaque-forming units (PFU) per cell]- and time of incubation (10-120 min)-dependent increase in eNOS mRNA levels, NOS enzyme activity, and the robust expression of eNOS protein. Immunocytochemical visualization of eNOS protein demonstrated expression in 70-90% of cells, indicating that adenoviral vectors are highly efficient in transducing the eNOS into cultured coronary artery VSM cells. We have shown that eNOS expression in VSM cells inhibited the PDGF-BB-stimulated DNA synthesis that is associated with the inhibition of cyclin A and PCNA expression. A preliminary report of these findings has been published (31).
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MATERIALS AND METHODS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Materials. Chemicals and materials
were obtained from the following sources: TRIzol (total RNA isolation
reagent), and fibronectin (human plasma) from GIBCO BRL;
L-[2,3,4,5,-3H]-arginine
(63 Ci/mmol),
[3H]thymidine (2 Ci/mmol), [32P]dCTP
(3,000 Ci/mmol), and 125I-labeled
PDGF-BB (813 Ci/mmol) from Amersham; PDGF-BB from R&D Systems
(Minneapolis, MN); bradykinin from Bachem (Torrance, CA); Dowex
AG50W-X8 (200-mesh) from Bio-Rad; random primed DNA labeling kit from
Boehringer Mannheim; NOC-18
[1-hydroxy-2-oxo-3,3-bis(3-aminoethyl)-1-triazene, DETA
Nonoate] from Alexis (San Diego, CA). Thapsigargin,
-nicotinamide adenine dinucleotide phosphate in reduced form
(NADPH), flavin mononucleotide (FMN), flavin adenine dinucleotide
(FAD), goat anti-rabbit IgG-horseradish peroxidase (HRP), goat
anti-mouse IgG-HRP, smooth muscle-specific 
-actin monoclonal
antibody, tetrahydrobiopterin, calmodulin, and
NG-nitro-L-arginine
(L-NNA) as well as other
chemicals and cell culture additives not listed were the highest grade
available from Sigma. All other antibodies used in this study were
purchased from Santa Cruz Biotechnology. ECL Western blotting detection kits were purchased from Amersham Pharmacia Biotechnology.
Adenoviral vector (Ad5/RSVeNOS). We
have used the replication-deficient recombinant adenoviral vector
Ad5/RSVeNOS containing the bovine aortic
eNOS (22) to transfer the
eNOS into coronary artery VSM cells.
Adenoviral vectors containing transgene were prepared by the University
of Iowa Vector Core as described elsewhere (23, 30) and obtained from
Dr. Donald Heistad, Department of Internal Medicine, University of
Iowa. The DNA constructs of replication-deficient adenovirus comprise
almost a full-length copy of the adenovirus genome in which the
eNOS,
lacZ, or green fluorescent protein
(gfp) expression cassette is incorporated at the site of E1
region deletions. In this cassette, a Rous sarcoma virus (RSV) promoter
to drive transcription of eNOS
precedes eNOS. A polyadenylation sequence of SV40 is cloned downstream
of eNOS. For each vector, high titer
adenoviral stocks were prepared by double cesium gradient purification,
and virus titer (PFU) was determined by standard methods. Virus
preparations were suspended in phosphate-buffered saline containing 3%
sucrose and stored at 
70°C until used.
Cell culture. Coronary artery VSM
cells were cultured from guinea pigs (4-6 mo old, 600-800 g
body wt) obtained from a local supplier. Hearts were removed from
guinea pigs anesthetized with xylazine (1 mg/kg im) and ketamine (80 mg/kg ip) and kept in Ham's F-12 culture medium. VSM cells were
cultured according to procedures established in our laboratory (2) and
were used up to the 8th passage from two batches in this study. The
purity of VSM cells was confirmed by immunocytochemical localization of
smooth muscle-specific -actin using monoclonal antibodies against
the NH2-terminal decapeptide of a
smooth muscle -actin (2).
Adenovirus-mediated eNOS transfer into coronary artery VSM cells. Cultured coronary artery VSM cells were transfected with eNOS, gfp, or lacZ as described earlier (30). Briefly, VSM cells in passages 3-8 were plated in cell culture dishes. Three to six days after plating was completed, VSM cells were transfected by incubation with Ad5/RSVeNOS [from 1 to 200 multiplicity of infection (MOI)] in DMEM supplemented with 0.1% BSA, 100 U/ml penicillin, 100 µg/ml streptomycin, and 2.5 µg/ml fungizone (serum-free defined medium). After the appropriate incubation time (30 min-2 h), the virus-containing culture medium was removed and replaced with fresh virus-free and serum-free culture medium supplemented with 0.1% BSA for 48 h. The extent of eNOS expression was quantitated after 48 h of gene transfer by Northern blotting, Western blotting, citrulline assay, and immunocytochemical localization.
Northern blotting. Total RNA was
extracted from control (gfp transfected) and
eNOS-transfected VSM cells as
described previously using a commercial guanidinium isothiocyanate
reagent (TRIzol, GIBCO BRL) (2, 29). RNA was quantified
spectrophotometrically, and equal amounts of denatured RNA samples were
separated by electrophoresis on 1.0% agarose-formaldehyde gels and
transferred by capillary action to a Nitran membrane (Schleicher and
Schuell). Ethidium bromide staining of 18 S band was used
to confirm that equal amounts of RNA were applied to each lane. The
eNOS cDNA probe was radiolabeled by the random priming technique, and
blots were prehybridized and hybridized with radiolabeled probes as
described previously. Blots were exposed to Kodak XAR-5 film with an
intensifying screen for 24-48 h at 70°C, developed, and photographed.
Measurement of eNOS activity. eNOS activity was measured in control and eNOS-transfected VSM cell homogenates by the conversion of L-[3H]arginine to L-[3H]citrulline (4, 11). Cells were homogenized on ice, using a glass homogenizer fitted with a ground glass pestle, in 50 mM Tris · HCl, pH 7.4, containing 0.1 mM EDTA, 0.1 mM EGTA, 12 mM 2-mercaptoethanol, 1 mM phenylmethylsulfonyl fluoride, 3 µM leupeptin, 1 µM aprotinin, 1 µM pepstatin, and 1 µM soybean trypsin inhibitor. The assay mixture contained 50 mM Tris · HCl, pH 7.4, 5 µM L-arginine, 0.25 µCi L-[3H]arginine, 0.5 mM NADPH, 10 µM tetrahydrobiopterin, 4 µM FMN, 4 µM FAD, 1 µg calmodulin, 1 mM calcium, and 40-80 µg cell homogenate protein in a 200-µl volume. For calcium-independent activity, calcium in the assay was replaced by 1 mM EGTA. Enzyme assays were carried out at 37°C for 15 min and terminated by adding 5.5 ml of Dowex slurry (Dowex AG50W-X8, 100-200 mesh Na+ form, prepared from the H+ form and preequilibrated in 20 mM sodium acetate, pH 5.5, containing 1 mM L-citrulline, 2 mM EDTA, and 0.2 mM EGTA) to remove unreacted L-[3H]arginine. L-[3H]citrulline production was measured using a liquid scintillation spectrometer. Specific calcium-dependent NOS activity was determined by estimating the difference between L-[3H] citrulline produced in tubes containing calcium-calmodulin and those containing calcium-calmodulin and 200 µM L-NNA.
Western blot analysis. The
gfp- and eNOS-transfected VSM
cells were serum starved for 48 h and then stimulated with 10 ng/ml PDGF-BB for the indicated times. After PDGF stimulation, cells were
washed with ice-cold phosphate-buffered saline and then lysed in 1 ml
of lysis buffer containing 10 mM Tris · HCl, pH 7.4, 150 mM NaCl, 1 mM EDTA, 1 mM EGTA, 1.5 mM
MgCl2, 50 mM sodium fluoride, 5 mM
pyrophosphate, 0.2 mM sodium vanadate, 1 mM phenylmethylsulfonyl fluoride, 2 µg/ml leupeptin, 2 µg/ml aprotinin, 10% glycerol, 1%
Triton X-100, and 0.5% NP-40 as described earlier (10, 11). The cell
lysate was centrifuged at maximum speed for 10 min at 4°C using a
microcentrifuge. The supernatant was collected, and the protein
concentration was measured using Bio-Rad reagent. Equal volumes of
2× sample buffer were added to the supernatant and boiled for 5 min. Equal amounts of proteins (10-20 µg/lane for all
measurements except for p21 60-80 µg/lane) from cells at
different time points were resolved in 10% SDS-polyacrylamide gel and
blotted onto polyvinylidene difluoride membranes. To
detect specific protein expression, the membranes were blocked in 5% nonfat milk, incubated with antibody against NOS-3 (1:500), PDGF- receptor (1:500), PY20 (1:3,000), cdk2 (1:1,000), cyclin A (1:200), cyclin E (1:500), p27 (1:500), p21 (1:200), or PCNA (1:200) for 1-1.5 h, and then incubated with goat anti-rabbit IgG-HRP
(1:10,000) or goat anti-mouse IgG-HRP (1:10,000) for 1 h. Labeled peroxidase activity was detected using ECL
Western blotting detection kit. For multiple blotting for different
proteins on the same membrane, the membrane was stripped with the
following stripping buffer containing 62.5 mM
Tris · HCl, pH 6.8, 2% SDS, and 10 mM
-mercaptoethanol for 30 min at 65°C with occasional agitation.
[3H]thymidine incorporation. [3H]Thymidine incorporation was carried out using semiconfluent VSM cells essentially as described earlier (2, 29). Cells were cultured in 24-multiwell dishes, and 2-3 days after subculture the cells were transfected with Ad5/RSVeNOS (as described in Adenovirus-mediated eNOS transfer into coronary artery VSM cells) in serum-free medium and maintained in these serum-free conditions for 48 h in DMEM containing 0.1% BSA. Control or lacZ-transfected cells were also kept in DMEM-BSA for 48 h. Quiescent cells were stimulated with PDGF-BB for 20 h to initiate DNA synthesis. After the growth factor-containing medium was removed, cells were incubated in DMEM-BSA for 4 h with 1 µCi/ml [3H]thymidine to quantitate DNA synthesis. TCA-insoluble cellular material was solubilized in 1 N NaOH at 37°C for 60 min, and an equal volume of 1 N acetic acid was added. [3H]thymidine incorporation was determined by liquid scintillation spectrometry.
125I-labeled PDGF binding.
PDGF- receptor number and affinity was measured using semiconfluent
quiescent VSM cells by radioreceptor assay using
125I-labeled PDGF-BB essentially
as described by Bowen-Pope and Ross (3). Cells were cultured in
24-multiwell dishes, and 2-3 days after subculture the cells were
transfected with eNOS or control vector carrying reporter gene gfp (as
described in Adenovirus-mediated eNOS transfer into coronary artery
VSM cells) in serum-free medium and maintained in serum-free
conditions for 48 h in DMEM containing 0.1%
BSA. Serum-starved cells were washed once
with ice-cold binding medium (DMEM containing 0.2% BSA) and incubated
with increasing concentration of
125I-labeled PDGF-BB (0.1-6
ng/ml) in 1 ml of ice-cold binding medium. Binding assays were carried
out in triplicate by incubating the trays on ice with gentle shaking
for 5 h. Binding assays were terminated by four washes (2 ml each well)
with ice-cold binding medium and cell-associated
125I-labeled PDGF-BB extracted
with 1 ml of solubilization buffer (1% Triton X-100 containing 0.1%
BSA). Nonspecific binding was determined in the presence of 20 ng/ml
unlabeled human recombinant PDGF-BB and was subtracted to calculate
specific binding. Scatchard analysis was carried out to calculate
binding constants.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Efficiency of adenovirus-mediated eNOS transfer into
VSM cells. Incubation of cultured guinea pig coronary
artery VSM cells with Ad5/RSVeNOS viral construct for 60 min at
37°C produced a dose (MOI or PFU per cell)-dependent increase in
both mRNA levels (Fig.
1A)
and eNOS enzyme activity (Fig. 1B).
A significant increase in NOS enzyme activity was observed at as low as
1 PFU/cell of virus construct, and enzyme activity increased with
increasing virus concentration up to the maximum 200 PFU/cell tested in
this study (Fig. 1). eNOS mRNA levels remained elevated for up to 2 wk
after transfection of VSM cells with eNOS viral construct (data not
shown). Calcium-dependent NOS activity in VSM cells infected with 20 PFU/cell of Ad5/RSVeNOS for 30 min was significantly greater (P < 0.05) than the
calcium-dependent NOS activity observed in bovine aortic endothelial
cells (48 ± 8 pmol · mg
1 · min1
in bovine aortic endothelial cells vs. 147 ± 13 pmol · mg1 · min1
in eNOS-transfected VSM cells;
n = 3). We could not detect
calcium-dependent NOS enzyme activity or eNOS mRNA in nontransfected or
control vector (carrying lacZ or
gfp)-transfected cells.
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NOS enzyme activity in
eNOS-transfected VSM cells was
completely dependent on the presence of calcium in the assay medium, and no activity was observed in the presence of EGTA (Fig.
2A). In
nontransfected or lacZ-transfected
coronary artery VSM cells, we could not detect measurable
calcium-dependent or calcium-independent NOS activity (Fig.
2A).
L-NNA, a specific inhibitor of
NOS, completely inhibited NOS activity in
eNOS-transfected VSM cells (data
not shown) and was used as a control in all assays for eNOS activity measurements. Expression of eNOS enzyme activity increased with increasing time of incubation of VSM cells with the Ad5/RSVeNOS viral
construct (100 PFU/cell) and reached near maximum in 60-120 min
(Fig. 2B). A brief 10-min incubation
period of VSM cells with 100 PFU/cell of eNOS viral construct resulted
in expression of significant enzyme activity measured 48 h after the
infection of cells with eNOS viral construct (Fig.
2B).
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Immunocytochemical localization of eNOS protein in transfected cells
revealed robust eNOS protein expression in 70-90% of VSM cells
after a 30-min incubation period with 100 PFU/cell of Ad5/RSVeNOS viral
construct (data not shown). In
eNOS-transfected VSM cells there was
robust expression of eNOS protein that was completely absent in control
vector carrying gfp-transfected cells (Fig. 3). These results demonstrate that
the Ad5/RSVeNOS viral construct rapidly and efficiently transferred a
functional eNOS into cultured coronary
artery smooth muscle cells.
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eNOS transfer inhibits PDGF-BB-stimulated VSM cell
proliferation. PDGF released from platelet aggregation
at restenotic or atherosclerotic lesions is an important
chemoattractant and a proliferative agent for VSM cells (2, 29). We
have shown earlier that cultured VSM cells express predominantly
PDGF- receptors (8). To test the effect of
eNOS transfer on VSM cell
proliferation, we measured
[3H]thymidine
incorporation as an index of DNA synthesis and cell proliferation.
[3H]thymidine
incorporation in VSM cells was measured 3 days after the infection with
the viral constructs. PDGF-BB stimulation of both Ad5/RSVlacZ- and
Ad5/RSVeNOS-infected cells was associated with dose-dependent increase
in [3H]thymidine
incorporation during the 20 h of stimulation (Fig. 4). This time point was chosen because the
doubling time for guinea pig coronary artery smooth muscle cells is
16-20 h in the presence of 10% fetal bovine serum (2).
eNOS transfer significantly (P < 0.5) inhibited PDGF-stimulated
[3H]thymidine
incorporation compared with lacZ
control vector-transfected cells (Fig. 4). Removal of
L-arginine 24 h before PDGF
stimulation reversed eNOS
transfer-mediated inhibition of thymidine incorporation (data not
shown). The extent of inhibition was 40-50% at both concentrations of PDGF-BB.
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Effect of eNOS transfer on PDGF- receptor number
and autophosphorylation. To understand the molecular
mechanisms of NO-mediated inhibition of VSM cell proliferation, we have
investigated the effects of eNOS
transfer into VSM cells on PDGF receptor number and activation. We have
previously shown that cultured VSM cells express predominantly PDGF-
receptors (8). Therefore, we first checked the effect of
eNOS transfer on PDGF--receptor
levels. eNOS transfer did not
significantly alter PDGF- receptor number or affinity compared with
gfp-transfected cells [maximal
binding (in fmol/106 cells) = 120 ± 23 gfp vs. 134 ± 15 eNOS; dissociation constant (in pM) = 77 ± 6 gfp vs. 84 ± 4 eNOS; means ± SE,
n = 4]. Similarly, Western
analysis demonstrated that PDGF--receptor density was slightly
increased in eNOS-transfected VSM
cells compared with gfp-transfected
cells, but the differences did not reach statistical significance (Fig.
3). The amount of PDGF- receptor rapidly decreased on PDGF-BB
stimulation (>70% decrease in 2 h), implying rapid internalization
and degradation of the ligand-receptor complex (Fig. 3); however, no
significant differences were observed between eNOS- and
gfp-transfected VSM cells in the time
course of receptor internalization and degradation. Activation of
PDGF- receptors was estimated by quantifying receptor
autophosphorylation after PDGF-BB stimulation (Fig. 3). PDGF-BB
stimulation of VSM cells rapidly increased PDGF- receptor tyrosine
phosphorylation that reached a maximum in 5 min (first time point
analyzed) and then decreased rapidly. No significant differences were
observed in the receptor autophosphorylation in
eNOS- and
gfp-transfected VSM cells (Fig. 3).
These results suggest that eNOS
transfer does not alter PDGF--receptor activation in VSM cells and
that signaling events responsible for NO-mediated inhibition of VSM
cell proliferation are downstream of receptor activation.
eNOS transfer into VSM cells inhibits cyclin A and
cyclin E expression. Mammalian cell cycle progression
is regulated by sequential expression of cyclins and subsequent
activation and inactivation of cyclin-dependent kinases (9, 12, 19).
Recently, it has been shown that differentiation and proliferation of
postmitotic VSM cells in response to injury in rat carotid arteries is
accompanied by temporally and spatially coordinated expression of
cyclins A and E, cdk2, and PCNA (35). Therefore, we used Western blot analysis to determine the effects of
eNOS transfer on PDGF-BB-stimulated expression of cyclins A and E and cdk2. In the initial set of experiments, we tested the effect of PDGF-BB stimulation on the expression of these molecules at 0, 2, 4, 6, 12, 16, and 24 h after
addition of 10 ng/ml PDGF to the 72-h serum-deprived cells. In this set
of experiments, we observed that cyclin E and A were maximally
stimulated in 4-8 h and then remained elevated above basal levels.
Therefore, subsequent experiments were undertaken at shorter time
intervals. Levels of cdk2 were high in quiescent VSM cells and did not
increase significantly on PDGF-BB stimulation (Fig.
5). eNOS
transfer did not alter cdk2 levels compared with gfp-transfected cells. Cyclin A
was expressed at low levels in nonstimulated cells, and its
expression increased rapidly on PDGF-BB stimulation. Increase in
cyclin A expression in response to PDGF-BB was biphasic: it first
peaked at 30 min and then slightly declined and was followed by a
second peak starting at 6-8 h (Fig. 5). eNOS transfer
significantly decreased (P < 0.05)
PDGF-BB-stimulated expression of cyclin A at 30 min, 2 h, 4 h,
and 8 h after stimulation. Cyclin E was also expressed in quiescent VSM
cells at low levels and it rapidly increased on PDGF-BB stimulation,
reaching a maximum in gfp-transfected
cells at 30 min and then remained elevated above basal levels up to 8 h
(Fig. 5). PDGF-BB-stimulated expression of cyclin E was markedly
delayed in eNOS-transfected VSM cells compared with
gfp-transfected cells (Fig. 5). However, maximum expression was comparable between both eNOS- and
gfp-transfected cells at 2, 4, and 8 h after PDGF-BB
stimulation.
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Effect of eNOS transfer on p27, p21, and PCNA
expression in VSM cells. In addition to the positive
regulation of cdks by specific cyclins, cdk activities are also
negatively regulated by CKI proteins (5, 12, 33). These inhibitory
proteins bind to and inactivate the cyclin-cdk complexes. p21 (also
known as CIP1/WAF1/CAP20/and SD11) and p27 (also known as KIP1) are
related proteins that preferentially bind to and inhibit cdk2-cyclin E,
cdk2-cyclin A, and cdk4-cyclin D activities (12, 19). Overexpression of
p27 (12, 19, 33) and p21 (5, 12) blocks entry of various cell types into the S phase in response to growth factors and oncogenic
transformation, suggesting that CKI-dependent regulation of cdks plays
a crucial role in cell cycle progression from
G1 to S phase. Because CKIs are
regulated positively and negatively at the transcription level by
positive and negative stimuli of cell proliferation (12, 19), we tested
whether NO may increase the expression of p27 or p21 in VSM cells to
produce cell cycle arrest of VSM cells. Initially, we observed that p27
expression was high in the
G0/G1 phase cell cycle-arrested cells, and levels started to decrease 2 h
after PDGF-BB stimulation. p27 expression reached steady-state levels
(50% decrease) in 6-12 h and then remained low up to 24 h (data
not shown). Therefore, subsequent experiments were planned at shorter
time intervals to determine the real time course of decrease in p27
expression after PDGF-BB stimulation (Fig.
6). Levels of p27 were lower in
eNOS-transfected cells compared with gfp-transfected cells; however,
differences between the two groups were not statistically significant
except at the 10-min interval after PDGF-BB stimulation (Fig. 6). In
both treatment groups, p27 levels decreased by 50% 8 h after PDGF-BB
stimulation. These data would suggest that altered expression of p27 in
eNOS-transfected cells is not involved
in NO-mediated inhibition of VSM cell proliferation.
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In contrast to p27, levels of p21 are very low in quiescent VSM cells. In these experiments, 60-80 µg protein/lane were resolved to test the effect of eNOS transfer on p21 expression. p21 levels slightly increased initially after the addition of PDGF-BB and then declined gradually to undetectable levels after 24 h of stimulation. p21 levels were slightly higher in eNOS-transfected VSM cells, and the PDGF-BB-stimulated decrease in p21 levels was delayed compared with gfp-transfected cells; however, these differences were not statistically different in three separate experiments (Fig. 6).
In addition to cyclins and cdks, growth factor-stimulated expression of
PCNA, a cofactor for DNA polymerase-
, plays an important role in DNA
synthesis during the S phase and cell proliferation (21). Moreover, it
has been suggested that cdk-mediated phosphorylation of retinoblastoma
gene product (pRB) plays an
important role in PCNA expression during the
G1/S phase of the cell cycle after growth factor stimulation (6, 12, 21). PCNA was expressed at low levels
in quiescent VSM cells and increased gradually, reaching maximum levels
at 4-8 h after PDGF-BB stimulation, and remained elevated above
the levels observed in nonstimulated cells for up to 24 h (data not
shown). PDGF-BB-stimulated PCNA expression was significantly inhibited
(P < 0.05) in
eNOS-transfected cells compared with
gfp-transfected cells at 10 min, 30 min, 2 h, 4 h, and 8 h (Fig. 6). PCNA expression in
eNOS-transfected VSM cells was at least 50% lower compared with that in
gfp-transfected control cells. These
results would suggest that decreased expression of PCNA in
response to PDGF-BB stimulation in
eNOS-transfected cells may, in
part, explain the inhibitory effects of
eNOS expression on VSM cell DNA
synthesis and proliferation.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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The major findings of the present study are
1)
eNOS transfer into VSM cells inhibits
PDGF-stimulated DNA synthesis; and
2) eNOS transfection into VSM cells
inhibits PDGF-stimulated expression of cell cycle progression molecules
like cyclin A and PCNA and delays the expression of cyclin E. These
changes in PDGF-BB-mediated signaling events in
eNOS-transfected VSM cells appear to
be downstream of PDGF--receptor activation because neither the
PDGF- receptor number and affinity (measured by radioreceptor assay)
nor the receptor density and autophoshorylation (measured by Western
blotting) are altered in VSM cells expressing the
eNOS compared with cells expressing
the gfp reporter gene. These results
demonstrate that cell cycle regulatory molecules are targets of the NO
action in VSM cells and may explain, at least in part, the molecular
mechanism of NO-mediated inhibition of VSM cell proliferation in
response to PDGF.
Several studies have demonstrated that pharmacological intervention with NO donors and high concentrations of L-arginine inhibit neointima formation in injured arteries (14, 17). In cultured VSM cells, NO donors inhibit VSM cell proliferation (18, 28). Von der Leyen et al. (34) demonstrated that in vivo eNOS transfer into balloon-injured rat carotid arteries using Sendai virus/liposomes system can restore normal NO production and inhibit neointima formation by 70%. Similarly, we have recently demonstrated that adenovirus-mediated eNOS transfer into medial VSM cells of balloon-injured rat common carotid artery significantly inhibits intima hyperplasia up to 4 wk after injury by augmenting the recovery of injury-induced downregulation of paxillin in VSM cells (11). Results presented here confirm and extend these observations in an in vitro system using VSM cells cultured from the coronary artery. eNOS transfer into coronary artery VSM cells significantly inhibited PDGF-stimulated DNA synthesis, an indicator of VSM cell proliferation (Fig. 4).
The effects of eNOS transfer on VSM cell proliferation are due to NO-mediated inhibition of cell cycle regulatory molecules expression rather than selection of cells expressing specific differential phenotypes after infection with adenovirus containing eNOS or reporter genes for the following reasons. First, cells are infected with viral vectors for a short time, and the experiments are completed in <48-72 h after gene transfer in the absence of serum, conditions, and time not sufficient for clonal expansion of differentiated VSM cell phenotype. Second, we (30) have shown earlier that transfection of VSM cells with adenovirus vector containing lacZ reporter gene has no effect on VSM cells survival or morphology up to 3 wk after gene transfer. Third, similarly we have demonstrated that eNOS transfection-mediated inhibition of VSM cell migration and paxillin tyrosine phosphorylation in response to PDGF are reversed by L-NNA, a specific inhibitor of NOS (10). Finally, we (11) have also demonstrated that eNOS transfer at the time of vascular injury significantly (P < 0.05) inhibited neointima formation at 2 and 4 wk after vascular injury. All this information taken together would indicate that eNOS transfer-mediated inhibition of VSM cell proliferation and migration is due to NO-mediated inhibition of specific signaling events.
As discussed above, it is well documented that NO inhibits VSM cell proliferation; however, the molecular mechanisms of NO-mediated inhibition of PDGF-stimulated VSM cell proliferation are not well understood. Treatment of VSM cells with antisense oligonucleotides to protooncogenes (13) and positive cell cycle control genes (1, 20, 21) (in vitro as well as in vivo) inhibit growth factor-stimulated as well as injury-induced VSM cell proliferation and neointima formation. Similarly, gene transfer of negative cell cycle control molecules has been shown to inhibit VSM cell proliferation and neointima formation (5, 6). Moreover, many agents that inhibit mammalian cell proliferation have been shown to inhibit G1/S transition by inhibiting cyclin-dependent kinase activity (9, 12, 19, 33). A recent study has demonstrated that vascular injury leads to time-dependent expression of cyclin A, cyclin E, and PCNA, suggesting an important role for these molecules in injury-induced VSM cell proliferation (35). Thus regulation of cell cycle regulatory molecules expression by NO may explain eNOS transfer-mediated inhibition of VSM cell proliferation.
Our results show that eNOS transfection in VSM cells inhibited PDGF BB-stimulated expression of cyclin A and delayed the time course of cyclin E expression (Fig. 5); both of these cyclins are essential for the activation of cdk2 and progression of cell cycle from the G1/S phase (9, 12, 19). Recently, Ishida et al. (16) observed that while NO donors decrease the message levels for cyclin A and cyclin E, they do not affect their protein levels in response to fetal bovine serum or fibroblast growth factor stimulation of VSM cells. They have further shown that NO donors increase p21 expression that may be responsible for the decrease in cdk2 activity. It is possible that sustained increase in the high levels of NO produced by NO donors and subsequent metabolism of NO to peroxynitrite may produce p53 induction in response to DNA damage that can lead to p21 expression as demonstrated in other cell types (15). Data presented in this paper show that p21 is expressed at very low levels in cultured VSM cells, and its expression is slightly but not significantly increased by eNOS transfer. These differences in our study and that of Ishida et al. (16) could be due to differences in the time and dose of NO exposure. Alternatively, it is possible that culture conditions and growth medium may lead to differential expression of p21. Moreover, recent efforts to demonstrate p21 protein expression in quiescent cultured VSM cells or in medial smooth muscle cells in vivo have produced negative results (5, 32, 35). In addition, it has been shown that p21 levels are not altered during VSM cell proliferation in response to growth factors or vascular injury, suggesting that under normal circumstances p21 may not play an important role in regulating VSM cell cycle (5, 32, 35).
In addition to p21, another cdk inhibitor, p27, has been shown to play an important role in the restriction point control of the fibroblast cell cycle (7, 9, 12, 19, 33). p27 levels were high in G0/G1-arrested VSM cells and decreased on PDGF-BB stimulation with a 50% decrease observed after 8 h of treatment that persisted up to 24 h. These findings are consistent with those reported in nontransformed fibroblasts where growth arrest has been shown to upregulate p27 expression, whereas growth stimulation decreased p27 expression (7). However, we did not find a significant change in p27 levels in eNOS-transfected cells, except at early time points, compared with gfp vector-transfected control cells. These results suggest that although p27 may play a role in regulating VSM cell cycle progression (since its levels decrease as cells progress in the G1/S phase of the cell cycle on PDGF-BB stimulation), regulation of p27 is not a target of NO-mediated inhibition of cell cycle engine.
Data presented in this paper also show that PDGF-BB-stimulated
expression of PCNA was decreased by 50% or more in
eNOS-transfected VSM cells compared
with gfp vector-transfected control
cells (Fig. 6). Because PCNA is a cofactor for DNA polymerase-, the
eNOS transfer-mediated decrease in
PCNA may inhibit DNA replication in the S phase of the cell cycle and
thus inhibit or prolong the cell cycle (12). This decrease in PCNA
expression in eNOS-transfected VSM
cells could be, in part, responsible for the cytostatic effects of
eNOS expression in VSM cells.
In summary, we have shown that functional
eNOS transfer into VSM cells did not
alter PDGF--receptor protein levels or receptor autophosphorylation.
eNOS transfer significantly decreased
cyclin A and PCNA expression and markedly delayed cyclin E expression in response to PDGF-BB stimulation. These data suggest that signaling events affected by NO are downstream of PDGF receptor activation and
that NO-mediated delay in the expression of cyclin E along with the
inhibition of cyclins A and PCNA expression may play an important role
in the inhibition of PDGF-BB-stimulated cell cycle progression.
| |
ACKNOWLEDGEMENTS |
|---|
We are thankful to our colleague Dr. Martin Cassell for critically reading the paper. Finally, we appreciate the help of the University of Iowa Vector Core, which is supported in part by a trust from the Carver Foundation, for the preparation and supply of virus constructs used in this study.
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FOOTNOTES |
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This work was supported by National Heart, Lung, and Blood Institute Grant HL-14388 and a Grant-in-Aid from the American Heart Association (Iowa affiliate).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. §1734 solely to indicate this fact.
Address for reprint requests and additional correspondence: R. C. Bhalla, Dept. of Anatomy and Cell Biology, 1-611 Bowen Science Bldg., The Univ. of Iowa College of Medicine, Iowa City, IA 52242 (E-mail: ramesh-bhalla{at}uiowa.edu).
Received 18 February 1998; accepted in final form 29 December 1998.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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