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Department of Physiology, West Virginia University School of Medicine, Morgantown, West Virginia 26506-9229
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Increased salt intake attenuates the endothelium-dependent dilation of skeletal muscle arterioles by abolishing local nitric oxide (NO) activity. There is evidence of oxidative stress in arteriolar and venular walls of rats fed a high-salt diet, and depressed arteriolar responses to acetylcholine (ACh) in these rats are reversed by scavengers of reactive oxygen species (ROS). In this study, we tested the hypothesis that this salt-dependent increase in microvascular ROS and the resulting attenuation of endothelium-dependent dilation are due to increased expression and/or activity of oxidant enzymes in the microvascular wall. Resting arteriolar and venular wall oxidant activity, as assessed by tetranitroblue tetrazolium reduction, was consistently higher in the spinotrapezius muscle of rats fed a high-salt diet (7% NaCl, HS) for 4-5 wk than in those fed a normal diet (0.45% NaCl, NS) for the same duration. Western analysis of protein from isolated microvessels showed no difference between HS and NS rats in the expression of NAD(P)H oxidase or xanthine oxidase. Inhibition of NAD(P)H oxidase and/or xanthine oxidase with diphenyleneiodonium chloride and oxypurinol, respectively, reduced resting arteriolar wall oxidant activity to normal levels in HS rats but had no effect in NS rats, suggesting that the basal activities of NAD(P)H oxidase and xanthine oxidase are increased in HS microvessels. However, inhibition of these enzymes in HS rats did not restore normal arteriolar responses to ACh, suggesting that this stimulus activates an alternate source of ROS that eliminates the role of NO in the subsequent dilation.
dietary salt; reactive oxygen species; nitric oxide; endothelium-dependent dilation
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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CONSUMPTION OF A HIGH-SALT DIET can lead to structural and functional changes in the microcirculation that are independent of any change in arterial pressure (4, 5, 17, 18, 24, 30-32). For example, this laboratory has previously reported that in normotensive rats fed a high-salt diet for 2-5 wk, the endothelium-dependent dilation of spinotrapezius muscle arterioles in response to acetylcholine (ACh) or increased shear stress is impaired due a selective loss of nitric oxide (NO) activity (4, 5). Chronic or acute ingestion of high dietary salt also leads to attenuated endothelium-dependent responses in arterioles of the rat cremaster muscle (17, 18) and cerebral cortex (32) and small feed arteries of the rat gracilis muscle (31).
Recently, we have found evidence of oxidative stress in spinotrapezius
muscle arterioles and venules of normotensive rats fed a high-salt
diet (30). Exposure of the muscle to different scavengers of reactive oxygen species (ROS) for as little as 30 min
reduces this oxidative stress and restores normal arteriolar responsiveness to ACh, suggesting that the increased oxidant activity in these salt-fed animals is decreasing the bioavailability of arteriolar NO. Superoxide anion (O
Under normal conditions, NAD(P)H oxidase and xanthine oxidase are considered to be the major enzymatic sources of ROS in the peripheral vasculature (20, 38, 44). An increase in the expression and/or activity of these enzymes has been reported in various conditions that also exhibit increased ROS levels and vascular dysfunction, such as hypertension (10, 49, 51, 56,), atherosclerosis (33), diabetes (10), and aging (23). In this study, we tested the hypothesis that increases in the expression or activity of vascular NAD(P)H oxidase and/or xanthine oxidase contribute to the increased levels of ROS and reduced endothelium-dependent dilation in the microcirculation of rats fed a high-salt diet.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Surgical Preparation and Intravital Microscopy
All surgical and experimental procedures for this study were approved by the West Virginia University Animal Care and Use Committee. Weanling male Sprague-Dawley rats (Harlan Sprague Dawley; Indianapolis, IN) were placed on a whole grain diet containing either 0.45% NaCl (normal salt, NS) or 7% NaCl (high salt, HS) by weight (NS, TD88311; HS, TD92100; Teklad; Madison, WI). All rats were studied 4-5 wk after being placed on their respective diets.Protocols 2 and 3 (see Experimental Protocols) involved the evaluation of microvascular characteristics in the exteriorized spinotrapezius muscle. For those experiments, each rat was anesthetized with thiopental sodium (100 mg/kg ip) and placed on a heating mat to maintain a 37°C rectal temperature. The trachea was intubated to ensure a patent airway, and the right carotid artery was cannulated to measure arterial blood pressure. The spinotrapezius muscle was surgically exteriorized as previously described (5). With this approach, the muscle is gently drawn away from the body wall without disturbing any feed vessels or surface fascia and secured at its in situ length over a transparent observation pedestal. Throughout the surgical preparation and subsequent experimental period, the exteriorized muscle was continuously superfused with an electrolyte solution (in mM: 119 NaCl, 25 NaHCO3, 6 KCl, and 3.6 CaCl2) warmed to 35°C and equilibrated with 95% N2-5% CO2. Superfusate flow rate was set at 4-6 ml/min to minimize equilibration with atmospheric oxygen (7).
The rat was then transferred to the stage of an Olympus BX50WI intravital microscope fitted with a CCD video camera (Dage-MTI; Michigan City, IN). Video images were displayed on a Panasonic high-resolution video monitor and stored on videotape for offline analysis. Arteriolar inner diameters were measured during videotape replay with a video caliper (Microcirculation Research Institute, Texas A&M University).
The blood supply to the spinotrapezius muscle is carried by arteriolar branches of three small feed arteries that interconnect within the muscle to form a structure known as the "arcade bridge" (43). In protocols 2 and 3, we studied the arcade arterioles that branch directly from the arcade bridge to form an extensive anastomosing network.
Experimental Protocols
Protocol 1: Expression of oxidant enzymes.
Western blot analysis was used to assess the expression of NAD(P)H
oxidase (by determining levels of p67phox, one of the
enzyme's cytosolic subunits) and xanthine oxidase in isolated
arterioles and venules from each dietary group. After induction of
thiopental sodium anesthesia, the right and left spinotrapezius muscles
were removed, rinsed in 4°C electrolyte solution, and pinned out in a
Silastic-coated petri dish filled with 100% methanol at 4°C. With
the use of a dissecting microscope, arcade arterioles and their paired
venules were identified and excised from both muscles. To obtain enough
protein for reliable Western blot analysis, the microvessels from three
rats (i.e., from 6 spinotrapezius muscles) were pooled for each sample.
The amount of protein needed for reliable analysis was found to be 3 µg, as determined in an initial series of trials to find the amount
that would consistently give bands that were sufficiently well defined
for densitometry. The isolated vessels were placed in 4°C storage
buffer (pH 7.25, 30% glycerol, containing 100 mM KPO4, 1 mM dithiothreitol, and 0.1 mM phenylmethylsulfonyl fluoride) and
centrifuged at 1,370 g for 5 min. Microvessels were then
homogenized and centrifuged at 3,100 g for 15 min at 4°C,
and the supernatant was stored at 
70°C until use. Three micrograms
of vessel protein (measured with a Bio-Rad protein assay kit) from each
dietary group were separated on a NuPage 4-12% Bis-Tris
polyacrylamide gel (Novex; San Diego, CA) and transferred onto a
nitrocellulose membrane. The membrane was probed with either goat
anti-p67phox (1:100; Santa Cruz Biotechnology; Santa Cruz,
CA) or rabbit anti-xanthine oxidase (1:1000; Biodesign; Saco, ME) and
then incubated with horseradish peroxidase-conjugated anti-goat IgG
antibody fragment [F(ab')2] (1:12,000; Santa Cruz Biotechnology) or
goat anti-rabbit F(ab')2 (1:15,000 Biodesign) for 1 h. After
treatment with SuperSignal (Pierce; Rockford, IL), membranes were
exposed to autoradiography film. X-ray images were digitally captured,
and optical density measurements were made from the images using
MetaMorph 3.5 image analysis software.
Protocol 2: Effect of enzyme inhibition on microvascular oxidant
activity.
To assess the effect of a high-salt diet on the in vivo activities of
NAD(P)H oxidase and xanthine oxidase, we investigated the degree to
which microvascular wall oxidant activity was decreased in the presence
of the NAD(P)H oxidase inhibitor diphenyleneiodonium chloride (DPI;
Sigma; St. Louis, MO) and/or the xanthine oxidase inhibitor oxypurinol
(Oxy; Sigma). Oxidant activity was identified by the reduction of
tetranitroblue tetrazolium (TNBT), which forms dark insoluble formazan
deposits when reduced by ROS (50, 51). The exteriorized
muscle was continuously superfused with either a normal superfusate
containing 2% TNBT for 60 min or a superfusate containing DPI (2 × 10
5 M), Oxy (3 × 104 M), or
DPI + Oxy for 90 min, with 2% TNBT added for the final 60 min.
The muscle was then fixed in situ and excised. To determine whether
these inhibitors were reaching the microvascular endothelium in
sufficient concentrations to exert a maximal effect, another group of
experiments was performed in which DPI (0.1 mg/kg), Oxy (40 mg/kg), or
DPI + Oxy were infused as a bolus intraarterially. After inhibitor
infusion and a 15-min equilibration period, the exteriorized muscle was
exposed to TNBT for 60 min, as described above.
ln (It/Io), where It is the
vessel wall gray value and Io is the gray value for the
paired avascular region. Control studies have verified that the amount
of formazan formed from TNBT is directly proportional to the level of
oxidant activity and that there is also a similar linear relationship
between tissue TNBT levels and light absorption (2, 29).
Protocol 3: Effect of oxidant enzyme inhibition on
endothelium-dependent responses.
In these experiments, we first evaluated the in vivo responsiveness of
arcade arterioles to iontophoretically applied ACh (Sigma) under the
normal superfusate. For ACh application, a micropipette (2-3 µm
outer tip diameter) was filled with 0.025 M ACh in distilled water and
placed in light contact with the arteriolar wall. Ejection currents of
5, 20, and 40 nA (delivered in random order) were used to apply ACh.
For each current dose of ACh, the vessel was continuously observed
during a 2-min control period, a 2-min application period, and a 2-min
recovery period. The series of ACh applications was then repeated after
30 min of exposure to a superfusate containing DPI, Oxy, or DPI + Oxy, or 15 min after arterial infusion of DPI + Oxy as described
above. Passive arteriolar diameters were then measured after addition
of adenosine (Sigma, 104 M) to the superfusate.
Data and Statistical Analysis
For protocol 1, the effect of high salt intake on microvessel protein expression was evaluated by comparing protein band optical densities between the two dietary groups. Each gel contained two lanes of protein from HS rats and two lanes of protein from NS rats. The optical densities for the two bands representing each diet were averaged, and the ratio of HS to NS density was calculated for each gel to control for any gel-to-gel variation. These individual ratios for a given enzyme were then combined and averaged.For protocol 3, arteriolar diameter and arterial pressure
measurements were digitized, stored, and analyzed using Polyview Lab
Manager (Grass Instrument Division/Astro-Med; West Warwick, RI). Data
were collected at 100 samples/s during control, ACh application, and
recovery periods. Resting vascular tone (T) was calculated as T = [(Dpass Dc)/Dpass] × 100, where
Dpass is the passive vessel diameter in the
presence of 104 M adenosine and Dc
is the average resting diameter measured during the 2-min control
period. A tone value of 0% represents a vessel that is completely
passive, whereas a value of 100% represents a vessel that is
constricted to the point of closure. Arteriolar responses to vasoactive
agents were determined by comparing the steady-state diameter reached
during the application period to the immediately preceding control diameter.
All data are expressed as means ± SE, and statistical analysis
was carried out using commercially available software (SigmaStat, SPSS;
Chicago, IL). Comparisons between groups were made using two-way
analysis of variance (ANOVA) in combination with Student-Newman-Keuls post hoc analysis to isolate pairwise differences. One-way ANOVA was
used to determine differences within a group subjected to repeated
measures. P values 
0.05 were considered significant for all tests.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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General characteristics of the rats used to assess enzyme
activities and endothelium-dependent responses in vivo (protocols 2 and 3) and the characteristics of the arterioles
studied in vivo (protocol 3) are shown in Table
1. The HS rats were slightly older than
the NS rats, but there was no significant difference in either body
weight or mean arterial pressure between the two groups. The high-salt
diet did not affect resting or passive arteriolar diameters, and
therefore the calculated resting tone of the vessels was unchanged.
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Representative Western blots for p67phox and xanthine
oxidase from microvessels of NS and HS rats are shown in Fig.
1. High salt intake had no effect on the
expression of NAD(P)H oxidase or xanthine oxidase, as judged by
comparing protein band optical densities between the two dietary
groups. The HS-to-NS optical density ratios averaged 1.07 ± 0.02 for p67phox and 0.96 ± 0.03 for xanthine oxidase, and
these values were not significantly different from 1.0.
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Figure 2 shows some representative images
of arterioles and venules exposed to 2% TNBT in NS rats
(left) and HS rats (right). The microvessels in
HS rats typically had a darker appearance due to deposition of the TNBT
reduction product formazan in the microvascular walls.
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Figure 3 shows the average level of
oxidant activity under control conditions in microvessels of
TNBT-exposed NS and HS rats, as assessed by the effect of formazan on
vascular wall light absorption. The mean absorption value for
arterioles was significantly greater in HS rats (0.100 ± 0.004)
than in NS rats (0.066 ± 0.004). A similar difference was found
in the venules, with the value in HS rats (0.129 ± 0.004)
significantly greater than that in NS rats (0.090 ± 0.004). These
findings, which are consistent with a previous report by this
laboratory (30), indicate that arteriolar and venular ROS
activity is greater in HS rats than in NS rats. This interpretation is
supported by our recent finding that ROS scavengers abolish these
differences in microvascular wall light absorption between HS and NS
rats (30).
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As shown in Fig. 4, exposure to Oxy, DPI,
or Oxy + DPI via either the superfusate (left) or
intraarterial infusion (right) had no effect on arterioles
in NS rats. In contrast, these inhibitors significantly reduced
arteriolar oxidant activity in HS rats (respective decreases in
absorption to 0.0835 ± 0.005, 0.079 ± 0.006, and 0.077 ± 0.005 with superfusion of Oxy, DPI, and Oxy + DPI, and to
0.071 ± 0.004, 0.072 ± 0.004 and 0.062 ± 0.003 with
infusion of Oxy, DPI, and Oxy + DPI). In the presence of Oxy
and/or DPI, arteriolar values in HS rats were not significantly
different from those in NS rats.
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The effects of these inhibitors on venules in each group are shown in
Fig. 5. In the NS rats, superfusion of
Oxy, DPI, or Oxy + DPI had no effect on the venules
(left), but infusion of these inhibitors significantly
decreased absorption values from 0.0898 ± 0.004 to 0.063 ± 0.003, 0.069 ± 0.003 and 0.071 ± 0.004, respectively
(right). In the HS rats, venular oxidant activity was
significantly decreased after either superfusion or infusion of the
inhibitors (from 0.129 ± 0.004 to 0.115 ± 0.006, 0.103 ± 0.006, and 0.083 ± 0.005 with superfusion and to 0.107 ± 0.004, 0.097 ± 0.005, and 0.085 ± 0.004 with infusion).
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Figure 6 shows the mean arteriolar
responses to ACh under the normal superfusate for all vessels studied
in protocol 3. Arterioles in NS rats dilated in a
dose-dependent manner to ACh applied at currents of 5, 20, and 40 nA
(dilations of 2.7 ± 0.2, 4.8 ± 0.3, and 7.1 ± 0.4 µm, respectively). At all three doses, arteriolar dilation in HS rats
was significantly less than that in NS rats (0.8 ± 0.1, 1.7 ± 0.2, and 2.6 ± 0.2 µm, respectively). There was no
difference between groups in maximal arteriolar dilation in response to
adenosine (NS: 26.1 ± 1.4 µm; HS: 23.4 ± 1.1 µm).
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The effect of inhibiting NAD(P)H oxidase and/or xanthine oxidase on
arteriolar responsiveness to ACh in NS and HS rats is shown in Fig.
7. Inhibiting NAD(P)H oxidase with DPI
had no effect on the arteriolar dilation to any level of ACh in either
group (Fig. 7A). Inhibition of xanthine oxidase with Oxy
also did not affect the responsiveness to ACh in either group (Fig.
7B). Finally, exposure to DPI + Oxy either via the
superfusate (Fig. 7C) or infusion (Fig.
8) also did not affect arteriolar
responses to ACh in either group.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Consumption of a diet high in salt leads to functional changes in the microcirculation that may compromise the ability of these vessels to respond to various physiological stimuli (5, 17, 18, 31, 32). Therefore, in addition to its potential importance for blood pressure control in hypertensive patients, lowering salt intake may have benefits for normotensive individuals as well. In the spinotrapezius muscle of normotensive rats fed a high-salt diet, this laboratory has consistently found reduced arteriolar responsiveness to endothelium-dependent stimuli (shear stress and exogenous ACh) due to an apparent loss of NO activity in these vessels (4, 5, 30). A salt-induced decrease in endothelium-dependent responses has also been observed in rat cremaster muscle and cerebral arterioles (17, 18, 32) and in rat gracilis muscle feed arteries (31). Consistent with our previous findings (29), the current findings indicate that under resting conditions, there is increased arteriolar and venular oxidant activity in the spinotrapezius muscle of normotensive rats fed a high-salt diet (Figs. 2 and 3). We have previously reported that exposure of the muscle to ROS scavengers abolishes this oxidative stress and restores normal arteriolar responsiveness to ACh, suggesting that the presence of vascular ROS is either directly or indirectly responsible for the depressed endothelium-dependent responses (30).
ROS may influence vascular tone by reducing the bioavailability of NO.
The half-life of NO is decreased when O
In this study, a high-salt diet did not alter the expression of NAD(P)H oxidase or xanthine oxidase in spinotrapezius muscle microvessels (Fig. 1). However, our findings do suggest that the tonic in vivo activity of these enzymes is increased in the HS rats. Exposing the unstimulated vascular bed of HS rats to the NAD(P)H oxidase inhibitor DPI and/or the xanthine oxidase inhibitor Oxy reduced arteriolar and venular light absorption to levels not different from those in NS rats (Figs. 4 and 5), suggesting that under resting conditions, the increased ROS present in these vessels is at least partially due to increased activity of oxidant enzymes. Although DPI reduced arteriolar wall light absorption by the same amount as Oxy, we were surprised to find no additive effect of these two inhibitors when they were applied together (Fig. 4). There is evidence to suggest that under some conditions, DPI can inhibit xanthine oxidase as well as NAD(P)H oxidase (13), and such a lack of specificity could explain our findings in the arterioles. However, we did observe the expected additive effect of DPI and Oxy in the venules (Fig. 5), raising the possibility that DPI may have a more specific effect on NAD(P)H oxidase in the venules than in the arterioles.
The finding of increased oxidant activity in the venules as well as the arterioles of HS rats is in itself an important aspect of this study. Increased arteriolar and venular oxidant activity has also been documented in the mesentery of SHR (47) and hypertensive Dahl rats (50, 51). In those studies, increased levels of ROS in the postcapillary vessels indicated that the development of this oxidant stress is unrelated to increased vascular pressure. Instead, increased microvascular oxidant activity in these models of hypertension may be related to elevated circulating glucocorticoid levels (47) and/or the interaction of activated neutrophils with the endothelium (51). In the normotensive salt-fed rats studied here, the mechanism leading to increased ROS in both the arterioles and venules is open to speculation (see below).
In NS rats, inhibiting NAD(P)H oxidase and/or xanthine oxidase had no effect on resting arteriolar light absorption (Fig. 4). Therefore, in the normal state, the scavenging activities of antioxidant enzymes such as SOD and catalase are apparently sufficient to prevent the accumulation of ROS generated by more modest NAD(P)H oxidase or xanthine oxidase activity (54). Consequently, inhibition of NAD(P)H oxidase and xanthine oxidase would not be expected to have any effect on arteriolar wall redox state, and light absorption would not change. In contrast, we found that oxidant enzyme inhibitors did reduce resting venular light absorption in NS rats, but only when delivered by intraarterial infusion (Fig. 5). This method of administration presumably produced higher inhibitor levels in the vicinity of the venular endothelium than could be attained by superfusate delivery. This finding suggests that there is a prevailing and detectable level of oxidant activity in the venular walls of NS rats and is consistent with our earlier findings (30). The normal presence of ROS in the venular walls may reflect a physiological role for these molecules in various cell signaling pathways, as has been documented in other vascular beds (48, 54).
Although our findings suggest that inhibition of NAD(P)H oxidase and/or
xanthine oxidase abolishes the oxidant stress in unstimulated arterioles of HS rats, normal endothelium-dependent responses to
exogenous ACh were not restored by this inhibition (Figs. 7 and 8).
Because exposure to ROS scavengers does restore the normal endothelium-dependent dilation of these vessels in HS rats
(30), we speculate that there may be another source of
microvascular ROS in these animals that is only triggered when the
endothelium is stimulated. A plausible candidate for this source is
endothelial NO synthase (eNOS), which can generate O
The current findings suggest that increased dietary salt affects the redox state of the resting microvascular wall by increasing the activity of NAD(P)H oxidase and xanthine oxidase. The mechanistic link between high salt intake and these changes in enzyme activity has yet to be identified. Angiotensin II is known to stimulate NAD(P)H oxidase (19), but circulating angiotensin II levels are decreased in rats fed a high-salt diet (24). Other changes in the vascular microenvironment, such as increased sodium accumulation within the vessel wall (3), could alter endothelial cell membrane potential or glycocalyx proteins and lead to enzymatic changes on the surface of or within the endothelium.
Although the amount of ROS generated by NAD(P)H oxidase and/or xanthine oxidase may be insufficient to limit at least some forms of endothelium-dependent dilation in HS rats (Figs. 7 and 8), the oxidative stress that is attributable to these enzymes under resting conditions could influence other NO-dependent processes at the microvascular level. For example, the venules have been shown to release NO under resting conditions (6, 37), and this NO can have a profound influence on the tone of nearby arterioles (6, 8, 14, 15). Continuous NO release from the venular endothelium also contributes to the low venular resistance that helps to shield capillaries from high hydrostatic pressures (6, 8, 37), and the presence of postcapillary NO is also necessary for the regulation of venular wall permeability (1) and for the inhibition of leukocyte adhesion and aggregation in a low-shear environment (12). The increased venular oxidative stress in rats fed a high-salt diet (Fig. 3) may reduce the availability of venular NO and therefore affect one or more of these processes. It is therefore important to further investigate the mechanisms and functional consequences of elevated NAD(P)H oxidase and xanthine oxidase activity associated with high salt intake.
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ACKNOWLEDGEMENTS |
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The authors gratefully acknowledge the expert technical assistance of Kimberley Wix in this study.
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FOOTNOTES |
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This work was supported by National Heart, Lung, and Blood Institute Grants HL-44012 and HL-52019.
Address for reprint requests and other correspondence: M. A. Boegehold, Dept. of Physiology, West Virginia Univ. School of Medicine, PO Box 9229, Robert C. Byrd Health Sciences Center, Morgantown, WV 26506-9229 (E-mail: mboegehold{at}hsc.wvu.edu).
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.0354.2001
Received 30 April 2001; accepted in final form 15 October 2001.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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