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Vol. 282, Issue 3, 1473-1479, 1997
Vascular Biology Center and Department of Pharmacology, Medical College of Georgia, Augusta, Georgia
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Abstract |
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 Top
Abstract
Introduction
Methods
Results
Discussion
References
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Endothelium-derived relaxing factors may differentially modulate
vascular tone and relaxation in arteries from specific vascular beds.
We evaluated the role of nitric oxide (NO), prostacyclin (PGI2) and endothelium-derived hyperpolarizing factor in
determining basal tone and acetylcholine (ACh)-induced relaxation of
coronary (Cor), skeletal muscle (Ske) and mesenteric (Mes) small
arteries (150-250 µm) isolated from male Golden Syrian hamsters
(16-17 weeks). Intraluminal diameter (ID) was recorded in vessels
maintained at a constant pressure of 40 mm Hg. Charybdotoxin (0.1 µM), a blocker of large Ca++-dependent K+
channels (BKCa), decreased base-line ID by 33 ± 4%
and 15 ± 4% in Cor and Mes small arteries, respectively. Neither
the nitric oxide synthase (NOS) inhibitor,
N
-nitro-L-arginine (LNA, 0.1 mM), indomethacin
(10
5 M) nor apamin (0.5 µM), which blocks small
Ca++-dependent K+ channels (SKCa),
affected ID. Maximal relaxation to ACh was significantly reduced by LNA
in Cor arteries preconstricted with the thromboxane A2
analog, U46619. LNA shifted the dose-response curve to the right
without altering maximal relaxation to ACh in Mes arteries and had no
effect on relaxation to ACh in Ske arteries relaxation. A high
extracellular K+ concentration (25-50 mM) largely reduced
relaxation to ACh in Ske and Mes and abolished relaxation in Cor
arteries, whereas indomethacin had no effect on any vessel. Blockade of
both BKCa and SKCa channels with a combination
of charybdotoxin and apamin abolished relaxation to ACh in Cor, but had
no effect in Mes or Ske arteries. Collectively, these results indicate
that ACh-induced relaxation is mediated by both NO and an
endothelium-derived hyperpolarizing factor that opens K+
channels independently of NO or PGI2 in Cor and Mes
arteries. Relaxation of Ske arteries is completely due to a NO and
PGI2-independent opening of K+ channels.
Relaxation to ACh is mediated by KCa channels in Cor arteries, and by other types of K+ channels in Ske and Mes
arteries. Additionally, BKCa channels regulate basal tone
in Cor and Mes, but not Ske arteries. These results indicate that
arteries of similar size use different mechanisms of
endothelium-dependent regulation of vascular tone and relaxation which
are dependent on the vascular bed.
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Introduction |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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The
endothelium is an important regulator of vascular tone due to synthesis
and release of vasodilatory substances including NO,
PGI2 and EDHF (Moncada and Vane, 1979
; Furchgott
and Zawadzki, 1980; Feletou and Vanhoutte, 1988). Acetylcholine is
generally used to induce production of EDRFs and may also stimulate
release of vasoconstrictor cyclooxygenase products from endothelial
cells (Miller and Vanhoutte, 1985; Luscher and Vanhoutte, 1990). After stimulation of muscarinic receptors, endothelial NOS converts L-arginine to NO (Palmer et al., 1988). NO may
produce relaxation by decreasing smooth muscle cell
Ca++ levels through a cGMP-dependent pathway or
through hyperpolarization due to increased conductance of
K+ channels (Gruetter et al., 1981;
Murphy and Brayden, 1995a; Corriu et al., 1996b).
PGI2 is produced by the action of prostacyclin synthase on endoperoxides, which are produced by cyclooxygenase. L-Arginine analogs such as LNA inhibit NOS activity,
whereas Indo inhibits cyclooxygenase. The enzyme responsible for EDHF
production is not known. However, EDHF may be arachidonic acid
metabolites of the cytochrome P450 pathway such
as epoxyeicosatrienoic acids (Campbell et al., 1996).
Relaxation to EDHF has been mediated through increased conductance of
Ca++-dependent K+ channels
and ATP-sensitive K+ channels (Cowan et
al., 1993; Campbell et al., 1996).
Studies have demonstrated that arteries exhibit heterogeneity in
endothelial and smooth muscle cell shape and function (Gumkowski et al., 1987; Archer et al., 1996). Heterogeneous
vascular relaxation in vessels of different sizes has also been
demonstrated (Galle et al., 1993; Archer et al.,
1996). An example of functional heterogeneity of vascular
responsiveness is the defense reaction in which renal and mesenteric
vascular beds vasoconstrict, whereas the skeletal vascular bed
vasodilates (Abrahams et al., 1960). Studies examining heterogeneity in isolated vessels have been performed in large arteries
such as the carotid artery, femoral artery and aorta (Nagao et
al., 1992; Cowan et al., 1993; Ferrer et
al., 1995). However, heterogeneity in the mechanisms mediating
endothelium-dependent relaxation in small arteries has not been
determined. Small arteries contribute to vascular resistance and may
exhibit different mechanisms of endothelium-dependent relaxation than
large arteries. The present study was designed to examine the roles of
NO, cyclooxygenase products and EDHF in ACh-induced vascular responses
in Cor, Ske and Mes small arteries (150-250 µm diameter).
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Methods |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Male Golden Syrian hamsters (16-17 weeks old) were obtained from Biobreeders, Fitchburg, MA. Hamsters were anesthetized with sodium pentobarbital (60 mg/kg i.p.) and heparin (100 U) was administered into the left ventricle of the heart. The skin over the abdomen was removed and the abdominal skeletal muscle was removed to isolate second-order branching sections of the superior epigastric artery. A section of the small intestine about 2 cm below the stomach was clamped and removed with the mesentery intact for isolation of a third-order branch of the mesenteric artery. The heart was removed for dissection of a second-order branch of the left main coronary artery. All tissues were placed in chilled, oxygenated (20% O2, 5% CO2, balance N2) Krebs-Ringer bicarbonate solution (mM, composition: NaCl, 118.3; KCl, 4.7; CaCl2, 2.5; MgSO4, 1.2; KH2PO4, 1.2; NaHCO3, 25; dextrose, 11.1).
Ske, Cor and Mes small arteries (150-250 µm diameter) were dissected by use of an Olympus dissection scope. Segments about 1 to 2 mm in length were isolated and mounted in a vessel bath between two glass micropipettes (70 µm diameter tip) with 10-0 silk ophthalmic suture. The lumen of the vessel was filled with Krebs' buffer through the micropipette and maintained at a constant pressure of 40 mm Hg. Vessels were monitored under a Olympus inverted microscope connected to a video monitor. Intraluminal diameter was continually measured by a video dimension analyzer (Living Systems Instrumentation, Burlington, VT) and recorded on a Grass polygraph.
Protocol.
After equilibration at 37°C in oxygenated
Krebs' buffer for at least 30 min, Ske, Cor and Mes small arteries
were preconstricted to 35 to 55% of resting diameter with the
thromboxane A2 analog (U46619) and allowed to
stabilize. Endothelium-dependent relaxation was assessed by performing
a dose-response curve to ACh (109 to
3 × 105 M). To determine the role of
vasoactive prostanoids in the response to ACh, vessels were pretreated
with Indo (105 M), an inhibitor of
cyclooxygenase, for 20 min before performing a dose-response curve to
ACh. To determine the role of NO in the response to ACh, vessels were
pretreated with LNA (0.1 mM), an inhibitor of NOS activity, for 20 min
before performing a dose-response curve to ACh. To determine the role
of K+ channels in mediating relaxation to ACh,
vessels were preconstricted with KCl (25-50 mM) before performing a
dose-response curve to ACh. This concentration of KCl effectively
blocks K+ efflux and prevents relaxation mediated
by opening of K+ channels.
).
When possible, more than one Ske, Cor or Mes artery was obtained from
the same hamster, but a single experiment was performed only once in
the same hamster. Additionally, only one dose-response curve was
performed per vessel.
Chemicals. All chemicals used in this study were obtained from Sigma Chemical Company (St. Louis, MO). U46619 was initially dissolved in 10% ethanol and diluted with Krebs' solution. Indo was dissolved in nanopure water in the presence of 94 mM NaCO3. LNA was dissolved in acidic nanopure water and adjusted to a pH of 7.4 with 0.1 N NaOH and diluted in Krebs' solution. All other agents were dissolved in nanopure water and diluted in Krebs' solution.
Data analysis. Data obtained from Ske, Cor and Mes vessels were expressed as mean ± S.E.M. Responses to vasodilatory agents were expressed as percent relaxation after preconstriction with U46619 or KCl. Statistical comparisons between groups were performed by repeated measures analysis of variance with covariance followed by a Fisher's pairwise least-significant-difference test for multiple comparisons.
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Results |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Base-line ID after equilibration at 40 mm Hg intraluminal pressure and the percent preconstriction produced by U46619 or KCl in Ske, Cor and Mes small arteries are shown in table 1. IDs were within the range of 150 to 250 µm and the level of preconstriction was in the range of 35 to 55%. Base-line ID was unaffected by pretreatment with Indo, LNA or AP. CTX caused a 33 ± 4% and 15 ± 4% contraction from base line in Cor and Mes small arteries, respectively. CTX had no effect on base-line ID in Ske small arteries.
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Response to ACh.
Dose-response curves to ACh in isolated Ske,
Cor and Mes small arteries are shown in figure
1. ACh produced dose-dependent relaxation
with a maximum of approximately 100% in vessels from each vascular
bed. Relaxation to ACh was significantly reduced at a dose of
107 M in Cor compared with Ske or
Mes small arteries.
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Effect of inhibition of NOS on the response to ACh.
Dose-response curves to ACh in the absence and presence of LNA are
demonstrated in figure 2. Relaxation to
ACh was unaffected by the presence of LNA in Ske small arteries.
However, LNA significantly lowered relaxation to ACh in Cor and Mes
small arteries. Additionally, in the presence of LNA, relaxation to ACh
was less in Cor than in Mes small arteries. Maximum relaxation to ACh
was not altered by LNA in Ske or Mes small arteries, but was
significantly reduced from 97 ± 2% to 49 ± 11% in Cor
small arteries.
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Role of K+ channels in ACh-induced
relaxation.
Dose-response curves to ACh in Ske, Cor and Mes small
arteries preconstricted with KCl are demonstrated in figure
3. Blockade of K+
efflux with high extracellular K+ significantly
inhibited relaxation to ACh in Cor, Ske and Mes small arteries.
Additionally, constriction to ACh at concentrations of
106 to 3 × 105 M was observed in Cor small arteries.
In the presence of high extracellular K+,
dose-dependent relaxation to ACh at the concentrations of 3 × 107 to 3 × 105 M was significantly lower in Cor than
in Ske or Mes small arteries, and was similar in Mes and Ske small
arteries.
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Role of vasoconstrictor cyclooxygenase products in relaxation to
ACh.
The role of cyclooxygenase products in masking relaxation to
ACh in Mes and Ske small arteries and in producing contraction of Cor
small arteries in the presence of high extracellular
K+ levels was determined. Pretreatment of
KCl-preconstricted Cor or Ske small arteries with Indo did not
significantly alter relaxation to ACh. However, Indo significantly
enhanced relaxation to ACh in KCl-preconstricted Mes small arteries
(fig. 5). This component of the
ACh-induced relaxation was reversed by pretreatment of vessels with
both Indo and LNA, which indicated that it was mediated by NO. Some
relaxation to ACh remained in the presence of LNA, Indo and a high
extracellular K+ concentration.
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Effect of blockade of BKCa and
SKCa channels on relaxation to ACh.
Dose-response curves to ACh in Ske, Cor and Mes small arteries
pretreated with a combination of CTX and AP in the presence of Indo are
shown in figure 6. The combination of CTX
and AP had no effect on ACh-induced relaxation of Mes small arteries,
caused a moderate decrease in relaxation in Ske small arteries and
completely abolished relaxation in Cor small arteries. The effect of
CTX/AP on the response to ACh in Cor small arteries was very similar to
the effect of increasing the extracellular K+
concentration (fig. 3). In both cases contraction to ACh was observed.
The EC50 value and % maximum relaxation to ACh
in Ske and Mes small arteries were not altered by CTX/AP (fig.
7). In the presence of CTX/AP, relaxation
to ACh was significantly less in Cor than in Ske or Mes small arteries.
Because these vessels were pretreated with Indo, it can be concluded
that cyclooxygenase products do not mediate the ACh-induced
contraction.
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Discussion |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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Several endothelium-derived vasoactive substances can modulate
vascular tone of small arteries. The present study has shown that
inhibition of NOS or cyclooxygenase activity, or blockade of
SKCa channels, has no significant effect on tone
of isolated Ske, Cor or Mes arteries. Conversely,
BKCa channels appear to be open under similar
conditions and modulate basal tone of Cor and Mes, but not Ske,
isolated small arteries. In other studies, CTX was found to produce a
moderate contraction of isolated porcine coronary arteries and a
dose-dependent contraction of carotid, femoral and superior mesenteric
arteries of Wistar Kyoto and spontaneously hypertensive rats (Asano
et al., 1993; O'Rourke, 1996). Mesenteric veins of
Sprague-Dawley rats were found to contract in response to CTX, but not
AP (Winquist et al., 1989). CTX had no effect on basal tone
of the rabbit superior mesenteric artery (Khan et al.,
1993). Therefore, the role of KCa channels in
determining basal tone appears to depend on both the species and the
vascular bed and size.
ACh induced similar quantitative relaxation of isolated Mes and Ske
small arteries, and relaxation of Cor small arteries was slightly less
than Mes or Ske small arteries. Additionally, heterogeneity existed in
the mechanisms mediating ACh-induced relaxation among arteries of
similar size from different vascular beds. It has been well documented
that ACh stimulates NO production and release in large arteries such as
aorta, in which inhibitors of NOS activity nearly abolish relaxation.
(Nagao et al., 1992; Wu et al., 1993). In
contrast, heterogenous responses based on arterial diameter within the
rat pulmonary vascular bed have been observed where the role of NO in
endothelium-dependent relaxation was found to be enhanced in conduit
compared with resistance rat pulmonary artery rings (Archer et
al., 1996). Others have observed that NO-mediated relaxation is
enhanced with increases in vessel size (Hwa et al., 1994).
Our study indicates that ACh-induced release of NO does not contribute
to Ske small artery relaxation, plays a moderate role in relaxing Mes
small arteries and significantly contributes to relaxation of Cor small
arteries. Cyclooxygenase products were not found to contribute to
ACh-induced relaxation in any vascular bed in this study.
Both EDHF and NO are capable of opening vascular smooth muscle
K+ channels (Murphy and Brayden, 1995a; Campbell
et al., 1996; Corriu et al., 1996b).
Endothelium-dependent vascular relaxation which remains in the presence
of NOS inhibitors can be blocked by a high
[K+]o (Cowan et
al., 1993; Corriu et al., 1996b). In the present study,
relaxation to ACh was largely inhibited in all vascular beds by a high
[K+]o, and contraction to
ACh was observed in Cor small arteries. Because LNA and Indo had little
effect on relaxation in Mes and no effect in Ske vessels, these results
indicate that opening of K+ channels, mediated by
an EDHF that is independent of NO or PGI2, is
required for relaxation to ACh in Ske and Mes small arteries. Conversely, Cor small arteries appear to depend on both NO and a
hyperpolarizing factor other than NO or PGI2,
because Indo had no effect, LNA significantly impaired relaxation and a
high [K+]o nearly
abolished relaxation.
A bioassay study showed that an EDHF is a product of the vascular
endothelium, independent of PGI2 and NO, which
acts to produce hyperpolarization and relaxation of smooth muscle cells
(Mombouli et al., 1996). Unlike NO, the role of EDHF in
mediating relaxation has been shown to be enhanced with decreasing
vessel size (Hwa et al., 1994). This hypothesis is supported
by our finding that ACh-induced relaxation in Mes small arteries was
largely mediated by K+ channels, and the finding
of others that ACh-induced relaxation of the rat main superior
mesenteric artery was not prevented by a high
[K+]o (Chen and Cheung,
1996). Some studies indicate that EDHF is a product of the cytochrome
P450 pathway derived from arachidonic acid
(Bauersachs et al., 1994; Campbell et al., 1996;
Chen and Cheung, 1996). However, studies on endothelium-dependent
relaxation to bradykinin in porcine coronary arteries suggest that EDHF
is produced by a pathway independent of cytochrome
P450, but reliant on arachidonic acid (Weintraub
et al., 1995), whereas ACh-induced relaxation of guinea pig
carotid artery is not mediated by lipoxygenase or cytochrome P450
(Corriu et al., 1996a). Studies in bovine coronary arteries
suggest that epoxyeicosatrienoic acids are EDHF (Campbell et
al., 1996), whereas a study in the rat hepatic artery refutes this
result (Zygmunt et al., 1996).
Relaxation to EDHF has been shown to be mediated primarily through
opening of KCa and KATP
channels of vascular smooth muscle cells (Cowan et al.,
1993; Bauersachs et al., 1994; Campbell et al.,
1996). In the present study, heterogeneity in the type of K+ channels mediating relaxation to ACh was
observed. KCa channels do not mediate
endothelium-dependent relaxation to ACh in Mes, minimally contribute to
relaxation in Ske and largely mediate relaxation in Cor small arteries.
Additionally, a contraction in response to ACh was observed after
inhibition of KCa channels with CTX and AP,
similar to that observed in the presence of high [K+]o. In other studies,
the ACh-induced hyperpolarization of vascular smooth muscle cells which
remained after inhibition of NOS and cyclooxygenase was inhibited by AP
in rabbit mesenteric arteries and by a combination of AP and CTX in
guinea pig carotid arteries (Murphy and Brayden, 1995b; Corriu et
al., 1996b).
Although vasodilatory cyclooxygenase products do not appear to contribute to ACh-induced relaxation of small arteries from the three vascular beds studied, release of a vasoconstrictor cyclooxygenase product masked relaxation to ACh in Mes, but not Ske or Cor small arteries, which indicates heterogeneity among vascular beds. The component of relaxation masked by vasoconstrictor cyclooxygenase products was mediated by NO as indicated by its reversal by LNA. Because a high [K+]o was present in this experiment, relaxation to NO could not have been mediated through an increase in K+ channel efflux, and was most likely caused by a decrease in smooth muscle cell intracellular Ca++ mediated by cGMP. The mechanism mediating contraction to ACh in Cor small arteries cannot be identified from the results of this study. However, it can be concluded that contraction is not mediated by a cyclooxygenase product. Other possibilities include ACh-induced release of endothelin or direct stimulation of smooth muscle cell muscarinic receptors.
Although the causes of the differential vascular responses cannot be
determined from the results of this study, they may be related to a
heterogeneity in the types and numbers of K+
channels present in vascular tissue. Archer et al. (1996)
demonstrated a higher number of KCa channels in
sheep pulmonary conduit than in resistance arteries, whereas a higher
number of delayed rectifier K+ channels where
observed in resistance than in conduit arteries (Archer et
al., 1996). An altered sensitivity to NO could also contribute to
heterogeneity and has been observed in a comparison of smooth muscle of
rabbit aorta, mesenteric and femoral arteries (Galle et al.,
1993).
Heterogeneity of vascular reactivity is important for physiological
responses such as the defense reaction. Additionally, adequate
perfusion of individual vascular beds depends on heterogeneity in the
responsiveness of vessels of different size. However, it is important
to note that heterogeneity in the mechanisms mediating relaxation in
arteries from different vascular beds may contribute to the vascular
patterns associated with development of diseases such as
atherosclerosis (Verbeuren et al., 1986). Several studies have demonstrated that responsiveness is altered in selective vascular
beds in diseases such as hypertension and congestive heart failure
(Wright and Fozard, 1990; Galle et al., 1991; O'Murchu et al., 1994; Fuchs, 1996). O'Murchu et al.
(1994) suggested that the selective increase in endothelium-dependent
relaxation in coronary arteries of dogs with congestive heart failure
may contribute to preserving coronary blood flow. The results of this
study clearly indicate that the role of NO and
Ca++-dependent K+ channels
in regulation of basal tone and mechanisms mediating ACh-induced
relaxation of isolated Cor small arteries are different from those of
Ske or Mes arteries.
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Footnotes |
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Accepted for publication May 19, 1997.
Received for publication March 21, 1997.
1 This work was supported by the American Heart Association, Georgia Affiliate.
Send reprint requests to: Leslie C. Fuchs, Ph.D., Vascular Biology Center, Medical College of Georgia, Augusta, GA 30912.
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Abbreviations |
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ACh, acetylcholine;
AP, apamin;
BKCa, large Ca++-dependent K+
channel;
CTX, charybdotoxin;
Cor, coronary;
EDHF, endothelium-derived
hyperpolarizing factor;
EDRF, endothelium-derived relaxing factor;
ID, intraluminal diameter;
Indo, indomethacin;
LNA, N-nitro-L-arginine;
Mes, mesenteric;
NO, nitric oxide;
NOS, nitric oxide synthase;
PGI2, prostacyclin;
SKCa, small
Ca++-dependent K+ channel;
Ske, skeletal
muscle.
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References |
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Top
Abstract
Introduction
Methods
Results
Discussion
References
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:5-monophosphate formation and relaxation of coronary arterial smooth muscle by glyceryl trinitrate, nitroprusside, nitrite and nitric oxide: Effects of methylene blue and methemoglobin.
J. Pharmacol. Exp. Ther.
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