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1 Department of Physiology and Biophysics, University of Nebraska Medical Center, Omaha, Nebraska 68198-4575; and 2 Department of Cardiovascular Medicine, University of Oxford, Oxford, United Kingdom OX3 9DU
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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The paraventricular
nucleus (PVN) of the hypothalamus is known to be involved in the
control of sympathetic outflow. Nitric oxide (NO) has been shown to
have a sympathoinhibitory effect in the PVN. The goal of the present
study was to examine the influence of overexpression of neuronal NO
synthase (nNOS) within the PVN on renal sympathetic nerve discharge
(RSND). Adenovirus vectors encoding either nNOS (Ad.nNOS) or
-galactosidase (Ad.-Gal) were transfected into the PVN in vivo.
Initially, the dose of adenovirus needed for infection was determined
from in vitro infection of cultured fibroblasts. In Ad.nNOS-treated
rats, the local expression of nNOS within the PVN was confirmed by
histochemistry for NADPH-diaphorase-positive neurons. There was a
robust increase in staining of NADPH-diaphorase-positive cells in the
PVN on the side injected with Ad.nNOS. The staining peaked at 3 days
after injection of the virus. In 
-chloralose- and
urethane-anesthetized rats, microinjection of
NG-monomethyl-L-arginine
(L-NMMA), a NO antagonist, into the PVN produced a
dose-dependent increase in RSND, blood pressure, and heart rate. There
was a potentiation of the increase in RSND, blood pressure, and heart
rate due to L-NMMA in Ad.nNOS-injected rats compared with
Ad.-Gal-injected rats. These results suggest that the endogenous
NO-mediated effect in the PVN of Ad.nNOS-treated rats is more effective
in suppressing RSND compared with Ad.-Gal-treated rats. These
observations support the contention that an overexpression of nNOS
within the PVN may be responsible for increased suppression of
sympathetic outflow. This technique may be useful in pathological conditions know to have increased sympathetic outflow, such as hypertension or heart failure.
paraventricular nucleus; renal sympathetic nerve activity; neuronal nitric oxide synthase gene transfer
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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THE GASEOUS MOLECULE NITRIC OXIDE (NO) plays an important role in cardiovascular homeostasis. It plays this role by its action on both the central and peripheral autonomic nervous systems as well as by having direct effects on vascular smooth muscle. NO synthase (NOS) activity has been demonstrated in central and peripheral sites throughout the autonomic nervous system, including the receptors and effectors of the baroreflex pathway. Localization of neuronal populations that possess neuronal NOS (nNOS) has been achieved by histochemical staining using NADPH-diaphorase and immunohistochemistry (1, 5). This close proximity of the production of NO within central sites that are involved in cardiovascular regulation have led to the belief that NO may be involved in the regulation of autonomic outflow.
There have been relatively few studies (8, 19, 20) that have examined specific sites within the forebrain involved in mediating the effect of NO on sympathetic nervous outflow. NOS is densely localized in the paraventricular nucleus (PVN) of the hypothalamus (1, 9, 14, 17). The PVN is also known to be a site of integration for autonomic and endocrine-mediated cardiovascular responses (15, 16). PVN neurons project to several areas within the central nervous system that are known to be important in regulating cardiovascular function. These regions include the nucleus tractus solitarius (NTS) and the vagal complex present in the dorsomedial medulla, the rostral ventral medulla, and the intermediolateral cell column of the thoracolumbar spinal cord, the site of sympathetic preganglionic motor neurons. The discrete presence of NOS-positive neurons in the PVN of the hypothalamus suggests that NO may serve as a physiological regulator of the sympathetic nervous system. Perfusion of the PVN with NO-containing cerebrospinal fluid or microinjection of sodium nitroprusside (SNP) into the PVN has been shown to elicit a significant reduction in arterial blood pressure (8). Taken together, these studies led us to speculate that endogenous NO mechanisms in the PVN may be responsible for regulating renal sympathetic nerve discharge (RSND) and thus arterial blood pressure.
We observed that microinjection of an inhibitor of NOS, NG-monomethyl-L-arginine (L-NMMA), increased RSND, arterial blood pressure, and heart rate (19). These data indicate that the endogenous NO system within the PVN is involved in mediating sympathetic outflow. We considered that the increase of blood pressure was, at least partially, mediated by an increase of sympathetic outflow because microinjection of L-NMMA also led to a concurrent increase in efferent renal sympathetic outflow (19). Specificity of NOS inhibitors is further substantiated with the observation that administration of L-arginine reversed the increases in RSND, blood pressure, and heart rate produced by NOS inhibition. In addition, subsequent administration of NOS inhibition failed to produce the increase in RSND, blood pressure, and heart rate observed before administration of L-arginine. These results indicate that endogenous NO mechanisms within the PVN contribute to regulation of changes in RSND. In further support of this hypothesis, we observed that the microinjection of SNP, a NO donor, elicited a reduction of RSND, arterial blood pressure, and heart rate. The reduction of blood pressure was, at least partially, mediated by a reduction of sympathetic outflow because microinjection of SNP also led to a concurrent reduction in efferent renal sympathetic outflow (19). These effects of SNP on arterial blood pressure and sympathetic nerve discharge were most likely mediated by NO released by SNP (8, 19).
Adenoviral vectors provide a tool for localized overexpression of a transferred gene in a target tissue. Gene transfer of nNOS using an adenoviral vector (Ad.nNOS) generates high levels of recombinant nNOS protein and augments agonist-stimulated NO production in cultured vascular smooth muscle and endothelial cells and in vascular tissues in vivo (2, 3). In the present study, we use Ad.nNOS for gene transfer within the PVN to test if the endogenous NO production can be altered within the PVN and if this change in expression of nNOS contributes to the regulation of sympathetic outflow in a functional manner in rats.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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All procedures utilized in this study were approved by the University of Nebraska Medical Center Institutional Animal Care and Use Committee, and the experiments were conducted according to the APS "Guiding Principles for Research Involving Animals and Human Beings." Male Sprague-Dawley rats weighing 210-280 g were obtained from Sasco Breeding Laboratories (Omaha, NE). Each rat was caged individually in an environment with ambient temperature maintained at 22°C and humidity at 30-40%. Laboratory chow (Purina) and tap water were available ad libitum.
Expression of nNOS in fibroblast cells in culture and measurement
of NO production.
Ad.nNOS and adenoviral vectors encoding -galactosidase (Ad.-Gal)
were constructed, isolated, and purified by double cesium chloride
density centrifugation as previously described (2, 3).
Ad.nNOS contains a rat nNOS cDNA under the control of the cytomegalovirus immediate/early promoter and expresses functional nNOS
protein in human vascular smooth muscle cells and human umbilical vein
endothelial cells (2). The construct also expresses
functional nNOS protein when infused in carotid arteries of rabbits
(3). To determine the optimal dosage of virus that would
not cause cytotoxicity but would cause increased nNOS protein
expression in cells or neurons, 5 × 105 cells/well of
293P3 fibroblast cells were cultured in 1 ml of Dulbecco's modified
Eagle's medium containing 10% fetal calf serum in rat tail
collagen-coated chamber slides (Lab-Tek, Fisher Scientific) under 5%
CO2 in air. After 24 h of seeding, cells were infected with increasing plaque-forming units (pfu) per cell of either Ad.nNOS
or Ad.-gal for 1 h at 37°C in serum-free medium. Fresh medium
was replaced after the specified period, and cultures were continued
for an additional 72 h. Medium from Ad.nNOS-infected cultures was
saved for NO analysis using the chemiluminescence technique (NO
analyzer, model 280 NOA, Sievers Instruments). Cells were fixed with
4% freshly prepared paraformaldehyde in PBS (pH 7.4) for
NADPH-diaphorase staining. Cells infected with Ad.-Gal were fixed in
2% formaldehyde-2% glutaraldehyde and incubated at room temperature
for 15 min with a X-Gal reaction solution [final concentration: 50 mM
Tris · HCl (pH 8.0) containing 15 mM NaCl, 1 mM
MgCl2, 2.5 mM potassium ferrous cyanide, 2.5 mM potassium
ferric cyanide, and 0.5 mg/ml X-Gal]. Stained cells were dehydrated
and mounted permanently for light microscopy. NADPH-diaphorase
histochemistry was done essentially as described for the PVN (see
NADPH-diaphorase histochemistry).
Adenovirus injections in the PVN.
On the day of the PVN injections, each rat was anesthetized with
pentobarbital sodium (40 mg/kg). The rat was then placed in a
stereotaxic apparatus (Davis Kopf Instruments; Tujanga, CA), and a
small burr hole was placed on the skull. The coordinates for the right
PVN were determined from the Paxinos and Watson Rat Atlas
(11), which were 1.8 mm posterior, 0.4 mm lateral to the
bregma, and 7.8 mm ventral to the dura. A cannula (outer diameter, 0.5 mm; inner diameter, 0.1 mm) connected to a microsyringe (0.5 µl,
model 7000.5, Hamilton microsyringe) was advanced into the right PVN
with a manipulator (Narishige Z-1). A 200-nl solution (final
concentration, 1 × 108 pfu/ml) of Ad.nNOS or
Ad..gal was injected into the PVN. Initial experiments with Ad.nNOS
concentrations of 1 × 1010-1 × 1012 pfu/ml demonstrated destruction of neurons at the site
of injection (neurons appeared fragmented upon light microscopic
evaluation after diaphorase staining). With a concentration of 1 × 108 pfu/ml, no damage to the neurons within the PVN was
observed from light microscopic evaluation. After the injection, the
wound was sutured, and analgesics (1 ml/kg sc Nubain-Stadol) were
administered on each of the next 2 days.
NADPH-diaphorase histochemistry.
One, three, and six days after Ad.nNOS infection, the brains were
stained for NADPH-diaphorase activity (21). This stain demonstrates the presence of functional NOS protein (5).
Briefly, the rats were deeply anesthetized with pentobarbital sodium
(70 mg/kg ip) and perfused transcardially with 150 ml of heparinized saline as a vascular rinse, followed by 300 ml of freshly prepared 4%
paraformaldehyde in 0.1 M sodium phosphate buffer (pH 7.4). The brain
was removed from each rat, postfixed at 4°C for 4 h in 4%
paraformaldehyde solution, and then placed in 20% sucrose for 24 h. The brain was blocked in the coronal plane and sectioned at 30 µm
thickness in a cryostat. The sections were collected in 0.1 M phosphate
(pH 7.4) containing 0.3% Triton X-100, 0.1 mg/ml nitroblue
tetrazolium, and 1.0 mg/ml -NADPH. The sections in nitroblue
tetrazolium solution were then placed in an oven at 37°C for 60 min.
After the reaction, the sections were rinsed in phosphate buffer (pH
7.4) and mounted onto chrome-alum-coated slides. The slides were air
dried overnight, rinsed in distilled water, and then dried again.
Coverslips were then mounted directly with Permount. The intensity of
staining was assessed using Kodak 1D Image Analysis software. Our
initial studies demonstrated that there was no obvious increase in
NADPH staining after 1 or 6 days of virus injection. Thus we focused
our attention to data obtained from rats 3 days after infection.
Western blot analysis of nNOS in the PVN.
Three days after Ad.nNOS infection, the brains were sectioned, and the
PVN was punched and analyzed for nNOS protein by immunobloting (12). Briefly, the rats were deeply anesthetized with
pentobarbital sodium (70 mg/kg ip), and the brains were removed and
immediately frozen on dry ice. The brains were blocked in the coronal
plane and sectioned at 300 µm thickness in a cryostat. The PVN was
punched according to the method of Palkovits and Brownstein
(10) from the virus-injected side and the contralateral
control side. The punches were homogenized in ice-cold TRI reagent
(MRC) using a sonicator (GraLab 545) to extract RNA. The protein left
in the organic phase was extracted according to the MRC published
protocol. Protein content in the SDS-supernatant was determined using a bicinchoninic acid protein assay kit (Pierce; Rockford, IL). Because of
the higher sensitivity of the antibodies, 5 µg total protein is
sufficient to generate a clear signal. Therefore, 6 µg protein was
mixed with SDS-PAGE buffer containing -mercaptoethanol and heated at
100°C for 5 min. Protein was fractionated in a 7.5% polyacrylamide
gel along with molecular weight standards, transferred to a Immobilon
membrane, and subjected to a Western immunoblotting protocol
(12). The membrane was probed with monoclonal anti-nNOS antibody (Transduction Labs; Lexington, KY) and peroxidase-conjugated goat anti-mouse IgG, and the signal was detected using enhanced chemiluminescence substrate (Pierce) and Renaissance X-ray film (NEN-DuPont). The film was digitized using a Kodak digital camera, and
the net intensity was determined using Kodak 1D Image Analysis software.
Recording of efferent RSND.
On the day of the experiment, the rat was anesthetized with urethane
(0.75 g/kg ip) and -chloralose (70 mg/kg ip). The left femoral vein
was cannulated with polyethylene (PE) tubing (PE-50 filled with saline)
for drug administration if necessary, and the left femoral artery was
cannulated and connected to a computer-based data acquisition system
(MacLab) via a pressure transducer (Gould P231D) for recording of
arterial blood pressure and heart rate.
Microinjections.
Experiments were performed to examine if the endogenous NO-mediated
inhibitory effects in the PVN on renal sympathetic outflow are enhanced
in rats with gene transfer of nNOS in the PVN. In five
Ad.-Gal-injected control rats and five Ad.nNOS-injected experimental
rats, an inhibitor of NOS, L-NMMA, was consecutively injected (50, 100, and 200 pmol in 50, 100 and 200 nl, respectively, using 1 mM solution of L-NMMA over 2 min) into the PVN in
intervals of 20-30 min. The vehicle solution was artificial
cerebrospinal fluid (pH 7.4) for all compounds. The responses in mean
arterial blood pressure, heart rate, and RSND over the 20-30 min
were recorded after each dose of L-NMMA.
Brain histology for identification of site of injection.
At the end of the experiments, monastral blue dye was injected into the
brain for histological verification of injection. After the rat was
euthanized, the brain was removed and fixed in 4% formaldehyde for at
least 24 h. The brain was then frozen, and serial transverse
sections (30 µm) were cut using a cryostat (IEC, model CT,
International-Harris Cryostat) at 
20°C. The sections were thaw
mounted on microscope slides and stained with 1% aqueous neutral red
staining procedures. Presence of the blue dye within the PVN was
verified microscopically.
Data analysis. Responses of RSND to the various doses of drugs were expressed as the percent change over the basal value. Responses of arterial blood pressure and heart rate to drugs were expressed as the difference between the basal value and the value after each dose of drug. The data were subjected to one-way repeated-measures ANOVA, followed by comparison for individual differences using the Newman-Keuls test (18). Blood pressure, heart rate, and NADPH-diaphorase staining intensities were compared between groups using the unpaired t-test. P < 0.05 was considered to indicate statistical significance. All data are presented as means ± SE.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Adenovirus-mediated gene transfer of nNOS to cultured fibroblasts.
No staining was observed for cells cultured without any viral
particles, suggesting that 293P3 fibroblast cells do not express either
nNOS or -galactosidase (Fig. 1).
However, distinct -galactosidase or diaphorase staining was visible
for cells infected with the either viral construct. That the
nNOS-infected cells expressed functional nNOS was evident from the
linear increase in NO accumulation in the medium after an increasing
concentration of virus exposure (Fig. 1). However, viral concentration
over 50 pfu/cell appeared to affect cell morphology and their ability
to stay attached on the culture surface (data not shown). Therefore, 50 pfu/cell were found to be the optimum concentration for fibroblast
cells, and the dosage was used to estimate the optimum dosage for in
vivo injection.
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Adenovirus-mediated gene transfer of nNOS within the PVN:
NADPH-diaphorase histochemistry.
We evaluated the efficacy of Ad.nNOS gene transfer in the PVN by
comparing the NADPH-diaphorase staining of the PVN infected with
Ad.nNOS with the contralateral PVN in the same rat. An example of the
differences in staining of the infected versus uninfected PVN is shown
in Fig. 2, A-C. There was
a significant increase in the number of diaphorase-positive cells as
well as the intensity of NADPH-diaphorase staining in the
Ad.nNOS-infected PVN compared with the contralateral uninfected PVN
(Fig. 2D). Similarly, Ad.-Gal demonstrated infection of
cells in the ipsilateral injected PVN and no labeled cells in the
contralateral PVN (Fig. 2E).
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Western blot analysis of nNOS in the PVN.
To confirm the results of histochemistry, we evaluated the efficacy of
Ad.nNOS gene transfer in the PVN by comparing the nNOS protein levels
of the PVN infected with Ad.nNOS with the contralateral PVN in the same
rat. An example of the differences in levels of nNOS protein of the
infected versus uninfected PVN is shown in Fig.
3A. There was a significant
increase in the intensity of the bands of nNOS in the Ad.nNOS-infected
PVN compared with the contralateral uninfected PVN (Fig.
3B).
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RSND responses to adenovirus-mediated gene transfer of nNOS within
the PVN.
There were no significant differences in mean arterial pressure, heart
rate, or RSND in the Ad.nNOS group compared with the Ad.-Gal
group (Table 1). Typically,
microinjection of L-NMMA produced a gradual increase in
RSND, blood pressure, and heart rate that peaked between 6-12 min
from the start of the injection, followed by a gradual decrease back to
the preinjection level (within 20-30 min). Microinjections of 50, 100, and 200 pmol L-NMMA elicited significant increases in
efferent RSND, arterial blood pressure, and heart rate, reaching
49 ± 7%, 14 ± 2 mmHg, and 22 ± 4 beats/min,
respectively, at the highest dose in Ad.-Gal-injected rats (Fig.
4). The increase in RSND, arterial blood
pressure, and heart rate to L-NMMA in rats injected with
Ad.nNOS were significantly potentiated (84 ± 13%, 21 ± 3 mmHg, and 37 ± 5 beats/min at the highest dose) compared with
Ad.-Gal-injected rats. These data indicate that blockade of
endogenous NO synthesis in rats with Ad.nNOS transfection is more
effective in raising RSND, blood pressure, and heart rate.
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-Gal.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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The results of the present study demonstrate for the first time the efficacy of adenoviral gene transfer of NOS into cells of the PVN of rats. We show that Ad.nNOS infects cells in the PVN and leads to a functional effect on renal sympathetic nerve activity mediated by the PVN. Our results provide a novel approach to restore neuronal levels of NOS, thus providing a potentially important candidate gene for cardiovascular gene therapy in diseases states, such as heart failure and hypertension lacking central nNOS (7, 21).
We used adenovirus vectors encoding the -galactosidase gene or the
nNOS gene to transfect fibroblasts to determine the dose of virus to
use in the PVN. The successful gene transfer was confirmed by several
methods. First, -galactosidase protein expression was confirmed by
histochemical staining of -galactososidase in fibroblasts. Second,
nNOS protein expression/activity was confirmed by NADPH-diaphorase
staining of fibroblasts. Third, NO production by the fibroblasts was
measured by monitoring the nitrite or nitrate (NOx) levels
in the medium from fibroblasts infected with Ad.nNOS. There was
increasing production of NOx with increasing concentration of the virus exposure. Taken together, this evidence indicates that 50 pfu/cell of Ad.nNOS is the optimal concentration for infecting fibroblasts that can be used for the optimal dose when injecting into
the PVN.
Subsequently, we injected this dose of Ad.nNOS into the PVN of rats.
Our initial results of time course (1, 3, and 6 days) demonstrated that
there was lack of dramatic changes in NADPH-diaphorase in the PVN of
rats infected for 1 day. However, there was a robust increase in
NADPH-diaphorase-positive cells, both in the number and intensity of
staining in the PVN of Ad.nNOS-infected rats compared with the
contralateral uninfected PVN in the same rat, 3 days after viral
injection. These data demonstrate a successful transfer of the nNOS
gene into cells in the PVN. Consistent with this observation, we also
observed successful gene transfer of the -galactosidase gene into
cells in the PVN when Ad.-Gal was injected. The intensity and number
of NADPH-positive cells in the PVN of Ad.nNOS-injected rats was
decreased in rats examined 6 days after the infection. Taken together,
these data indicate that Ad.nNOS at a dose of 50 pfu/cell in the PVN is
efficient in transferring the nNOS gene into the cells in the PVN 3 days after infection. However, the transient expression of nNOS protein after Ad.nNOS injection limits this mode of gene transfer to acute studies. On the contrary, adenovirus-associated viruses, such as human
parvovirus and retrovirus vectors, have been successfully used for gene
therapy (for a review, see Ref. 6) because of the weaker
immune response and long-term effects. A variety of experimental manipulations, including the use of recombinant virus particles and improvement of intracellular trafficking, have been used
to improve the efficacy of adenovirus-associated viruses in long-term
gene therapy (6). Therefore, further experiments need to
be done using improved adenovirus-associated virus-nNOS constructs for
maintaining the long-term effect of nNOS in the PVN; hence, the
beneficial effect of NO in the PVN in chronic disease conditions such
as hypertension and heart failure.
It could be possible that inflammation and cytotoxicity caused by
adenovirus infection might have affected the present findings (4). Adenoviral infection can cause a dose-dependent acute inflammatory injury (4). To avoid this, we conducted our
studies at a relatively low infectious titer (1 × 108
pfu/ml), a dose that we have shown yields maximal transgene expression without apparent neuronal injury or vascular injury (3).
Furthermore, Ad.-Gal gene transfer did not alter basal arterial
blood pressure or heart rate, and the responses in RSND responses to
L-NMMA were not significantly different in
Ad.-Gal-treated rats compared with untreated control rats. These
results suggest that changes in these variables in the rats with nNOS
gene transfer in the PVN did not result from inflammation or
cytotoxicity but were mediated by the increase in NO production in the PVN.
The presence of NOS-positive neurons in the PVN of the hypothalamus
suggests NO may serve as a physiological regulator of the sympathetic
nervous system. Horn et al. (8) observed that both
perfusion of the PVN with NO-containing cerebrospinal fluid and
microinjection of SNP into the PVN elicited a significant reduction of
arterial blood pressure. These effects of NO within the PVN were
attributed to inhibition of neurons mediating sympathetic outflow via
the intermediolateral call column of the spinal cord (8).
This initial functional evidence is supported more recently by direct
measurement of RSND (19, 20) showing that endogenous NO
within the PVN is involved in the regulation of sympathetic outflow.
The microinjection of L-NMMA into the PVN elicited
significant increases in efferent RSND, mean arterial blood pressure,
and heart rate in rats (19). Consistent with these
observations, we saw similar responses in rats injected with Ad.-Gal
into the PVN. However, the responses to L-NMMA were larger
in rats infected with Ad.nNOS, suggesting a larger endogenous component
due to NO. These data indicate that the overexpression of the nNOS gene in the PVN resulted in an increased endogenous production of NO, which
in turn has a functional role in dictating renal sympathetic nerve
activity. These results indicate that overexpression of nNOS in the PVN
contributes to the basal level of sympathetic tone in rats.
A recent study by Sakai et al. (13) demonstrated that overexpression of endothelial NOS in the NTS of rats produces hypotension, bradycardia, and a decrease in urinary excretion of norepinephrine in conscious rats 7 days after transfection. Although we did not observe statistically significant decreases in arterial blood pressure and heart rate in this study, there was a trend toward a decrease in these parameters. Furthermore, there are a number of notable differences between the two studies: 1) Sakai et al. (13) used endothelial NOS vs. nNOS, 2) they injected the virus in the NTS versus the PVN, 3) their maximal expression was at 7 days versus our 3 days, and 4) they conducted the studies in conscious rats versus anesthetized rats. These differences in experimental design and methodologies may account for the differences in the observations in blood pressure and heart rate. However, overall, the two studies are in general agreement that overexpression of NOS within the central nervous system decreases overall sympathetic tone (13).
In summary, we demonstrated a technique of nNOS gene transfer into the PVN of rats. We demonstrated that Ad.nNOS into the PVN generates a high level of NOS in cells in the PVN and that the expressed nNOS is functional in inhibiting renal sympathetic nerve activity by the PVN. Ad.nNOS injection in the PVN provides a novel approach to replacing NOS activity in the PVN of disease conditions known to have depleted levels of NOS, such as heart failure and hypertension.
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ACKNOWLEDGEMENTS |
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This work was supported by National Heart, Lung, and Blood Institute Grant PO1-HL-62222.
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FOOTNOTES |
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Address for reprint requests and other correspondence: K. P. Patel, Dept. of Physiology and Biophysics, Univ. of Nebraska Medical Center, 984575 Nebraska Medical Center, Omaha, NE 68198-4575.
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. Section 1734 solely to indicate this fact.
10.1152/ajpheart.00503.2001
Received 8 June 2001; accepted in final form 10 October 2001.
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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