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First published online October 5, 2006
Journal of Experimental Biology 209, 4011-4023 (2006)
Published by The Company of Biologists 2006
doi: 10.1242/jeb.02480
Hydrogen sulfide as an oxygen sensor/transducer in vertebrate hypoxic vasoconstriction and hypoxic vasodilation
1 Indiana University School of Medicine-South Bend, 1234 Notre Dame Avenue,
South Bend, IN 46617, USA
2 Department of Biological Sciences, University of Notre Dame, Notre Dame,
IN 46556, USA
3 Department of Neurology, The Medical College of Wisconsin, Milwaukee
53226, WI, USA
4 Research Service, Zablocki Veterans Affairs Medical Center, Milwaukee, WI
53295, USA
* Author for correspondence (e-mail: kolson{at}nd.edu)
Accepted 1 August 2006
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Summary |
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 TOP Summary IntroductionMaterials and methodsResultsDiscussionList of abbreviationsReferences |
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Key words: vascular smooth muscle, hydrogen sulfide metabolism, cysteine metabolism, redox signaling
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Introduction |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionList of abbreviationsReferences |
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). H2S
has been shown to be a neuromodulator and neuroprotectant
(Kimura et al., 2005), to
exert effects in intestinal (Teague et
al., 2002) and genito-urinary
(Sidhu et al., 2001;
Patacchini et al., 2005;
Dombkowski, 2006) systems, and
to have potent cardiovascular actions.
Until now, studies of the vasoactive effects of H2S have been
limited to systemic vessels. H2S has been shown to be a vasodilator
in mammalian vessels such as the rat thoracic aorta and portal vein
(Hosoki et al., 1997;
Zhao et al., 2001;
Zhao and Wang, 2002;
Zhang et al., 2003) and the
perfused mesenteric bed (Cheng et al.,
2004). In non-mammalian vertebrates H2S may produce
vasodilation, vasoconstriction or it may produce multi-phasic responses
(Dombkowski et al., 2004;
Dombkowski et al., 2005;
Olson, 2005).
Information on the involvement of H2S in the pulmonary
vasculature is limited and indirect. H2S toxicity is often
associated with pulmonary edema (Roth,
2004), suggesting that either capillary permeability or pulmonary
blood pressure is increased. In chronically hypoxic rats one of the enzymes
responsible for H2S synthesis is reduced in systemic vessels
(Zhang et al., 2003). Plasma
[H2S] is also lower in these animals, suggesting that overall
H2S production is reduced. These data led the authors to infer that
a hypoxia-induced loss in tonic H2S dilation contributed to chronic
hypoxic pulmonary vasoconstriction, although they did not study the effects of
H2S on pulmonary vessels.
During the course of independent studies on the phylogeny of vascular
responses to hypoxia (Smith et al.,
2001; Olson et al.,
2001; Russell et al.,
2001) (M.J.R., R.A.D. and K.R.O., unpublished observation) and
H2S (Dombkowski et al.,
2004; Dombkowski et al.,
2005; Olson,
2005), we noticed that these two stimuli evoked similar, if not
identical, responses in a variety of vessels, irrespective of whether this
response was contraction, relaxation, or multi-phasic. Because hypoxia and
H2S also produced similar responses in trout urinary bladder
(Dombkowski et al., 2006),
this prompted us to investigate whether the relationship between these two
stimuli in blood vessels was coincidental or if H2S might be
involved in the hypoxic response. In the present study, we compared the
effects of hypoxia and H2S (produced from dissolved NaHS or
Na2S) on mechanical responses of respiratory and systemic vessels
from a variety of vertebrates. We then selected four vessels for further study
based on their individual responses to these two stimuli: lamprey dorsal aorta
(mono-phasic constriction), rat thoracic aorta (mono-phasic relaxation) and
rat and bovine pulmonary arteries (multi-phasic responses). In select vessels,
we examined the interaction between hypoxia and H2S on mechanical
responses of vessel rings, measured H2S production by homogenized
vessels, and evaluated the effects of inhibiting H2S production or
adding cysteine, the precursor for H2S synthesis, on the hypoxic
response. We also examined the effects of hypoxia and H2S on smooth
muscle transmembrane potential in bovine pulmonary arteries.
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Materials and methods |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionList of abbreviationsReferences |
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Sea lamprey (Petromyzon marinus L., 130–450 g) were trapped in streams feeding into the Great Lakes during the spring-summer spawning season and airlifted to the Indiana University School of Medicine-South Bend (IUSM-SB) where they were maintained in 500-liter rectangular tanks with aerated, flowing well water (15°C) and exposed to a 12 h:12 h L:D photoperiod. They were not fed. Lampreys were anesthetized in benzocaine (1:5000, w/v) and the dorsal aortas were dissected out and placed in lamprey buffered saline at 4°C until use.
White Sprague Dawley rats Rattus norvegicus (Berkenhour) (Mammalia) were anesthetized with 50 mg/animal pentobarbital and the viscera was removed and placed in 4°C Krebs–Henseleit mammalian saline. The thoracic aorta and pulmonary (first–third generation) arteries were dissected out and stored at 4°C until use.
Holstein cow Bos taurus L. (Mammalia) lungs were obtained from a nearby abattoir, placed in 4°C Krebs–Henseleit mammalian saline, and transported to IUSM-SB. The pulmonary arteries (fourth–sixth generation) were dissected out and stored at 4°C until use.
Vessel myography
Vessels were cut into 3–8 mm-long segments, mounted on 280
µm-diameter stainless steel wire hooks and suspended in 5 ml water-jacketed
smooth muscle baths filled with the appropriate buffer at the animal's
physiological temperature (lamprey, 14°C; rat and bovine, 37°C).
Lamprey vessels were aerated with room air, mammalian vessels were aerated
with 95% air, 5% CO2. One hook was stationary; the other was
connected to a Grass model FT03C force-displacement transducer (Grass
Instruments, West Warwick, RI, USA). Tension was measured on a Grass Model 7E
or 7F polygraph (Grass Instruments). Polygraph sensitivity was set to detect
changes as small as 5 mg. Data was archived on a PC computer at 1 Hz using
Labtech Notebook software (Laboratory Technologies Corp., Andover, MA, USA) or
SoftWire (Measurement Computing, Middleboro, MA, USA). The chart recorders and
software were calibrated prior to each experiment.
Length–tension relationships were derived from KCl-contracted vessels
and used to apply an appropriate baseline (resting) tension (approximately
500–1500 mg) for 0.5–1 h prior to experimentation. In a typical
experiment, vessels were contracted twice with 80 mmol l–1
KCl and resting tension was re-established between rinses and prior to
experimentation (
30–45 min each). Hypoxia (PO2
<5 mmHg) was achieved by aeration with 100% N2 (lamprey) or 95%
N2/5% CO2 (mammals). H2S was produced by
dissolving NaHS or Na2S. In a number of experiments vessels were
pre-contracted with KCl (lamprey aorta), norepinephrine (rat thoracic aorta
and pulmonary artery) or the thromboxane A2 mimetic, U-46619
(bovine pulmonary artery) agonist, prior to exposure to hypoxia or
H2S. Previous experience in our laboratory has shown that these
agonists and doses (50–80% of maximal contraction) produce optimal and
sustained force in the different vessels. Enzyme inhibitors were added
20–30 min prior to further treatment.
Hypoxia–H2S interactions
To examine the interactions between hypoxia and H2S, vessels
were exposed to one stimulus while in the presence of the other. Lamprey
aortas were contracted with 80 mmol l–1 KCl, washed, then
exposed to hypoxia (N2). When the hypoxic contraction had
stabilized, H2S was added to produce a final concentration of
3x10–4 mol l–1. A second group of
vessels was first exposed to H2S, then to N2. Rat
thoracic aortas were treated with propranolol (10–5 mol
l–1) to block ß-adrenoceptors then pre-contracted with
norepinephrine (10–6 mol l–1). When tension
had stabilized they were exposed to either N2 then H2S
(3x10–4 mol l–1) after the
N2 relaxation stabilized, or vice versa. Bovine pulmonary
arteries were pre-contracted with U-46619 (10–8 mol
l–1) then N2 followed by
3x10–4 mol l–1 H2S or
vice versa. Both groups of bovine vessels were then re-oxygenated
(air) and the hypoxia was repeated to evaluate recovery.
Transmembrane potential
The effects of hypoxia and H2S on transmembrane potential
(Em) were measured in perfused bovine pulmonary arteries.
Glass cannulae with matching tip diameters were inserted into each end of
approximately 300 µm diameter, 15 mm long, vessels and secured with nylon
suture. The vessels were immersed in Krebs–Henseleit buffer (37°C)
in a water-jacketed chamber during cannulation and throughout the experiment.
Side branches, if any, were tied off. A micrometer connected to the proximal
cannula was used to take slack out of the artery and a pressure transducer
connected close to this cannula allowed measurement of intravascular pressure.
The inflow cannula reservoir was raised to produce an intravascular pressure
of 10 mmHg and the vessels were continuously perfused and superfused with
buffer aerated with 5% CO2-balance air. A color video camera
mounted on a stereomicroscope above the vessel was used to project an image of
the artery on a video monitor and the vessel diameter (±1.5 µm) was
measured on screen using a video scaler. Reference points such as adhering
connective tissue, side branches, etc. located near the site of measurement
insured that the diameter was always measured at the same point on the vessel
wall. Vessel diameters were measured immediately after mounting the artery,
after equilibration, and throughout the experimental protocols.
Membrane potentials were measured with glass microelectrodes filled with 3
mol l–1 KCl and having tip resistances between 50–80
M
. Impalements were made from the adventitial side of the vessel.
Criteria for a successful impalement was an abrupt negative drop in voltage
when the electrode entered the cell, an immediate return to baseline upon
withdrawal of the electrode, and no change in electrode resistance. Because it
was difficult to keep the electrode in the cell during an active response,
Em was measured in a number of cells before and after
exposure to hypoxia or H2S. Hypoxia was produced by perfusing and
superfusing the vessels with buffer aerated with 5% CO2 and 95%
N2. H2S in the form of NaHS (1 mmol
l–1) was added directly to the perfusate and superfusate.
H2S production
Lamprey dorsal aortas were pooled from six fish and bovine pulmonary
arteries and veins were pooled from two cows. The vessels were homogenized on
ice in 50 mmol l–1 phosphate buffer (pH 6.8; 1:9
tissue:buffer w/w). L-Cysteine (1 mmol l–1 bovine,
10 mmol l–1 lamprey) and pyridoxyl 5'-phosphate (2 mmol
l–1) were added (Zhao et
al., 2003) and the mixtures were placed in sealed syringes along
with a glass mixing bead, avoiding air bubbles, and gently agitated on a
rotary mixer for 18–24 h at room temperature. The homogenate was briefly
centrifuged to remove tissue debris and 0.5 ml of supernatant was added to an
equal volume of antioxidant buffer to convert all H2S gas and
HS– anion to sulfide (S2–). Total sulfide
anion was measured in triplicate samples with a sulfide electrode (Lazar
Research Laboratories, Los Angeles, CA, USA) on a Fisher Accumet AR50 pH meter
(Fisher Scientific, Pittsburgh, PA, USA). Inhibitors (see
Hosoki et al., 1997;
Zhao et al., 2003) of
cystathionine ß-synthase (CBS), amino-oxyacetate (AOA; 1 mmol
l–1), cystathionine 
-lyase (CSE),
D,L-propargylglycine (PPG; 10 mmol l–1)
and ß-cyanoalanine (BCA; 5 mmol l–1) and the general
inhibitor of pyridoxyl 5'-phosphate-dependent enzymes, hydroxylamine
(HA; 1 mmol l–1) (Kery et
al., 1999), were added to bovine vessels simultaneously with
L-cysteine and pyridoxyl 5'-phosphate.
Contribution of the H2S precursor, cysteine, to hypoxic responses
Lamprey aortas, bovine pulmonary arteries and rat thoracic aortas were
prepared for myography as above, contracted twice with 80 mmol
l–1 KCl and washed. Bovine pulmonary arteries and rat aortas
were pre-contracted with U-46619 (10–7 mol
l–1) before each hypoxic exposure. The vessels were then
exposed to hypoxia for 15–20 min and returned to air, washed 2 times and
resting tension re-established. Cysteine (1 mmol l–1) was
added and 20 min later the procedure was repeated. As exogenous cysteine did
not appear to be necessary for short-term hypoxic responses of bovine
pulmonary arteries, paired vessels were exposed to hypoxia for over 15 h with
or without cysteine, reoxygenated for 60 min and the U-46619 pre-contraction,
hypoxia protocol repeated.
Physiological salines
Lamprey Hepes-buffered saline (in mmol l–1): 145 NaCl, 3
KCl, 0.57 MgSO4, 2 CaCl2, 5 glucose, 3 Hepes acid, and 7
Hepes Na+ salt, pH 7.8.
Mammalian Krebs–Henseleit bicarbonate-buffered saline (in mmol l–1): 115 NaCl, 2.51 KCl, 2.46 MgSO4, 1.91 CaCl2, 5.56 glucose, 1.38 NaH2PO4, and 25 NaHCO3, pH 7.4.
Chemicals
Stock solutions were prepared as follows: U-46619; 0.01 mol
l–1; and epinephrine, 0.01 mol l–1.
Propanolol (final concentration 10–5 mol
l–1) was added to the baths 15 min prior to epinephrine to
block ß-adrenoreceptor-mediated relaxation
(Olson and Meisheri, 1989).
All drugs were dissolved in distilled H2O except U-46619, which was
dissolved in 95% ethanol. Ethanol was not vasoactive at the concentrations
used in these studies. Anti-oxidant buffer for the total H2S assay
was made of 15.6 mmol l–1 sodium salicylate, 3.7 mmol
l–1 ascorbic acid and 21 mmol l–1 NaOH (pH
>12). Unless otherwise stated all chemicals were purchased from
Sigma-Aldrich Co. (St Louis, MO, USA).
Data analysis
Dose–response curves were fit for individual vessels with Table Curve
software (Jandel, Chicago, IL, USA). Statistical comparisons were made using
Student's t-test or paired t-test where appropriate. One-way
ANOVA followed by Student–Newman–Keul's test was used for multiple
comparisons of means. Values are means ± s.e.m. Significance was
assumed when P
0.05.
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Results |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionList of abbreviationsReferences |
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The responses of lamprey aorta, rat thoracic aorta and bovine pulmonary arteries to H2S during hypoxia and to hypoxia during exposure to H2S are shown in Fig. 3. Individually, hypoxia and H2S produced the same magnitude of contraction in lamprey dorsal aorta (Fig. 3A), whereas H2S applied during hypoxia produced a slight relaxation and a hypoxic contraction was significantly inhibited by prior application of H2S. In rat thoracic aorta, H2S produced a slight contraction when applied during hypoxia and hypoxic relaxation was inhibited by exposure to H2S (Fig. 3B); similar results were obtained from seven other vessels. Hypoxia- and H2S-mediated contractions of bovine pulmonary arteries were reversed to a relaxation when the vessels were previously treated with the other stimulus (Fig. 3C); after approximately 30 min aeration with air (95% air, 5% CO2) both hypoxic and H2S contractions were restored; similar results were obtained from seven other vessels.
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Transmembrane potential
Table 2 shows the effect of
hypoxia and H2S on resting transmembrane potential
(Em) and diameter in bovine pulmonary arteries. Hypoxia
and H2S produced essentially identical depolarization and
constriction.
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H2S production
Homogenates of lamprey aortas and bovine pulmonary arteries and veins
produced H2S (H2S+HS–) when incubated
with cysteine and pyridoxyl 5'-phosphate
(Fig. 4). H2S
production by lamprey vessels was twice that of bovine vessels. H2S
production by bovine pulmonary arteries was not significantly affected by the
cystathionine -lyase (CSE) inhibitor,
D,L-propargylglycine (PPG), whereas it was significantly
reduced by the cystathionine ß-synthase (CBS) inhibitor, amino-oxyacetate
(AOA). A combination of AOA and PPG was no more effective than AOA alone.
H2S production by pulmonary arteries and veins was inhibited by a
mixture of AOA, PPG and the pyridoxyl 5'-phosphate-dependent enzyme
inhibitor, hydroxylamine (HA). The three inhibitors combined were no more
effective in pulmonary arteries than AOA alone.
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60%) blocked by
AOA, converted to slight relaxation by HA and a strong relaxation by a
combination of the three inhibitors (Fig.
5D). In U-46619 contracted bovine pulmonary arteries, the initial
application of AOA produced a brief (<5 min) contraction that was only
3.5±1% (N=8) of a KCl (80 mmol l–1)
contraction (not shown). HA had no effect on un-stimulated bovine pulmonary
arteries, but it completely relaxed U-46619 (10–7 mol
l–1) contracted arteries (not shown). Between
10–7 mol l–1 and
3x10–5 mol l–1, HA produced a
dose-dependent relaxation of KCl-contracted bovine pulmonary arteries that was
equivalent to a 13±3% (N=8) reduction of a KCl contraction. HA
between 3x10–5 mol l–1 and
3x10–3 mol l–1 produced a
dose-dependent contraction of the same vessels (not shown). At
10–3 mol l–1, the HA contraction was
equivalent to 6±5% of a 80 mmol l–1 KCl
contraction.
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Contribution of the H2S precursor, cysteine, to hypoxic responses
The contribution of cysteine to hypoxic vasoconstriction and dilation is
shown in Fig. 6. Addition of 1
mmol l–1 cysteine to lamprey aortas produced a slight
contraction, doubled the strength of the hypoxic contraction, but did not
affect the strength of the KCl contraction
(Fig. 6A). Glycine (1 mmol
l–1) also produced a slight contraction of lamprey aortas,
but did not affect the strength of either hypoxic or KCl contractions
(Fig. 6A). Exogenous cysteine
did not appear to affect either the magnitude or rate of hypoxic relaxation of
rat thoracic aortas (not shown). However, rat aortas incubated with cysteine
contracted immediately upon re-oxygenation, whereas control vessels exhibited
a transient further relaxation before contracting (not shown). The effects of
cysteine incubation during long-term (15 h) hypoxia on subsequent hypoxic
responses of rat aortas is shown in Fig.
6B. The magnitude of a U-46619 pre-contraction was increased by
50% after 15 h hypoxia (P0.05, N=16) and this was
unaffected by the presence or absence of cysteine. Cysteine treatment
significantly decreased the magnitude of the hypoxic relaxation (from
42±2% to 32±2% relaxation of the U-46619 contraction; control
vs cysteine, respectively). Cysteine treatment did not affect the
magnitude of the initial force recovered during reoxygenation (262±138
mg vs 259±63 mg, control vs cysteine), but enabled
the vessels to maintain tension during a 25 min recovery, whereas control
vessels relaxed to baseline. A transient relaxation preceding re-oxygenation
recovery was observed in control, but not cysteine-treated vessels; these
responses were similar to those described above in vessels that were not
exposed to 15 h hypoxia. Control vessels did not respond to a second hypoxic
exposure, whereas hypoxic relaxation could be repeated in cysteine-treated
vessels (Fig. 6B).
Cysteine-treated vessels also relaxed when washed with U-46619-free buffer;
control vessels did not (Fig.
6B). The apparent inability of control vessels to respond at the
end of this experiment was not due to damage to the vessel as this protocol
(U-46619 contraction, two consecutive hypoxia treatments and wash) could be
repeated on both groups of vessels with identical results (not shown).
Addition of cysteine to bovine pulmonary arteries did not affect the magnitude
of a subsequent hypoxic contraction (not shown). However, after 15 h of
hypoxia (Fig. 6C), hypoxic
contraction of pulmonary arteries incubated with 1 mmol l–1
cysteine for 15 h was twice that of control vessels. Both cysteine-treated and
control vessels relaxed upon re-oxygenation. Force developed during a second
hypoxic exposure was not significantly different between the two groups, but
the control vessels could not sustain the contraction (by 30 min they were
completely relaxed) whereas cysteine-treated vessels were able to sustain the
hypoxic vasoconstriction (at 30 min they retained 55% of their contractile
force; Fig. 6C).
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Discussion |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionList of abbreviationsReferences |
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) in a variety of
vertebrate blood vessels. Although considerable work remains to be done, our
experiments also suggest that H2S, or more likely the metabolism of
H2S, is an important component in the O2 sensing/signal
transduction cascade involved in the hypoxic response.
Vessel responses to hypoxia and H2S are virtually identical
Vertebrate vessels from various species and from various vascular beds
within the same species exhibit their own unique response to hypoxia,
mono-phasic relaxations and mono or multi-phasic contraction. In every vessel
we have examined thus far (Table
1, Fig. 1), as well
as in studies by others (Olson et al.,
2001; Zhao et al.,
2001; Zhao and Wang,
2002; Dombkowski et al.,
2005), the responses to H2S are essentially identical
to those produced by hypoxia. In lamprey dorsal aortas both hypoxia and
H2S produce a mono-phasic contraction
(Fig. 1A) and both are
dose-dependent (Olson et al.,
2001; Dombkowski et al.,
2005). In rat thoracic aorta these stimuli produce a mono-phasic,
dose-dependent relaxation (Fig.
1B) (Zhao et al.,
2001; Zhao and Wang,
2002). When hypoxia produces a multi-phasic response, so does
H2S. This similarity between hypoxic and H2S responses
is quite striking in rat pulmonary arteries where both stimuli produce an
identical complex tri-phasic contraction–relaxation–contraction
(Fig. 1C). To our knowledge
only hypoxia and H2S produce this characteristic tri-phasic
response in rat pulmonary vessels. In bovine pulmonary arteries, hypoxia and
H2S (Fig. 1D and
Fig. 3C, respectively) often
produce a slight, transient dilation that precedes the sustained
contraction.
The similarity between the effects of H2S and hypoxia in both pulmonary and systemic vessels suggests that H2S and hypoxia may share common activation pathways. Furthermore, because we have observed identical effects of hypoxia and H2S in vessels from at least one species in each vertebrate class (Table 1), we propose that H2S mediation of a hypoxic response is common throughout vertebrate phylogeny and that it was a primordial feature of the earliest vertebrate vessels.
Vessel responses to hypoxia and H2S are competitive
In addition to the similarity in the form of the response, in our
experience in a variety of vessels, hypoxia and H2S have been the
only two stimuli whose effects are eliminated or reversed by pre-existing
exposure to the other stimulus, whereas their response to other agonists is
generally not affected (Fig.
3). These studies suggest that hypoxia and H2S share a
common and unique pathway in the excitation–contraction process that,
when activated by one stimulus, cannot be further activated by the other.
In lamprey aorta (Fig. 3A),
hypoxic and H2S contractions are 76 and 60%, respectively, of an 80
mmol l–1 KCl contraction. Exposing the vessel to
H2S during a hypoxic contraction results in a small relaxation.
Exposing the vessel to hypoxia during an H2S contraction results in
a contraction whose magnitude is less than 25% of the KCl contraction. By
comparison, when lamprey aortas are pre-contracted with either 80 mmol
l–1 KCl, or 10–6 mol l–1
epinephrine, the contractions produced by hypoxia
(Olson et al., 2001) and
H2S (Dombkowski,
2006) are not diminished. In norepinephrine pre-contracted rat
thoracic aortas, where initial exposure to either hypoxia or H2S
produces a characteristic relaxation, subsequent treatment with the other
stimulus (H2S or hypoxia, respectively) fails to relax, and in fact
elicits a slight contraction (Fig.
3B). The inability of the second stimulus to produce additional
relaxation is not due to a mechanical property of the vessel because the
vessel is not completely relaxed by the first stimulus. In bovine pulmonary
arteries, both hypoxia and H2S produce a monophasic contraction
that is additive to a pre-existing U-46619 contraction
(Fig. 3C). However, secondary
application of H2S during hypoxia relaxes the hypoxic constriction
and hypoxia relaxes the H2S contraction
(Fig. 3C). Thus the effects of
hypoxia and H2S appear to be uniquely competitive in both systemic
and pulmonary vessels.
What is not yet clear is why in some instances the second stimulus not only inhibited, but reversed the effects of the first, i.e. H2S reversed hypoxic contraction in the lamprey aorta (Fig. 3A) and bovine pulmonary artery (Fig. 3C) and hypoxic relaxation in the rat thoracic aorta (Fig. 3B) and hypoxia reversed the H2S contraction in bovine pulmonary arteries (Fig. 3C). This effect may be due to different conditions produced by endogenous (hypoxia-mediated) and exogenous H2S (NaHS or Na2S), which could affect the magnitude and direction of the relative fluxes of H2S gas and HS– across the cell membrane. Similarly, when vessels are made hypoxic during H2S treatment, actual [H2S] may be greater than exogenous [H2S] alone. This question may not be resolved until it is understood how exogenous and endogenous H2S interact and how H2S gas and HS– move across cell membranes and mediate cellular responses.
Hypoxia and H2S have similar effects on Em
Hypoxia and H2S have similar effects on vascular smooth muscle
transmembrane potential (Em); both hyperpolarize systemic
vessels (Lombard et al., 1999;
Frisbee et al., 2001;
Zhao et al., 2001) and
depolarize respiratory (bovine pulmonary) arteries
(Table 2). Whether this means
that both stimuli act through a common pathway is not known. While it is
tempting to associate a change in Em with intracellular
[Ca2+] ([Ca2+]i) and relaxation or
contraction, it is not clear if this is always the case. In a number of
systemic vessels a substantial portion of hypoxic vasodilation is independent
of [Ca2+]i (Thorne
et al., 2002) and vessels contracted with high (
80 mmol
l–1) KCl can still relax to hypoxia
(Pearce et al., 1989;
Shimizu et al., 2000).
Similarly, the relaxant effect of H2S in rat aortas has been shown
to be only partially mediated by K+ (KATP) channels and
it requires extracellular Ca2+
(Zhao et al., 2001;
Zhao and Wang, 2002). In rat
pulmonary arteries cell depolarization can be uncoupled from the rise in
[Ca2+]i (Gelband and
Gelband, 1997) and Ca2+ may enter the cell via
voltage-independent (capacitative Ca2+) pathways
(Robertson et al., 2000). Both
hypoxic pulmonary vasoconstriction in the rat
(Robertson et al., 2000) and
hypoxic vasoconstriction in the lamprey aorta
(Olson et al., 2001) can occur
in the presence of elevated extracellular [K+]. Thus, the
mechanism(s) responsible for the change in Em during
H2S exposure remain to be elucidated.
Vessels produce H2S enzymatically
H2S production has now been demonstrated in vessels from lamprey
(Fig. 4), rainbow trout
(Dombkowski, 2006), rat
(Hosoki et al., 1997;
Zhao et al., 2001;
Zhao et al., 2003;
Wang et al., 2004) and cow
(Fig. 4). This suggests that
H2S synthesis is a general property of vertebrate vascular smooth
muscle.
Cysteine is the major source of H2S production in mammals
(Maclean and Kraus, 2004) and
cysteine was added to our tissue homogenates to produce optimal enzymatic
activity (S.K.H., N.L.W. and K.R.O., unpublished observation). A number of
enzymes desulfurate cysteine. These include cystathionine ß-synthase
(CBS; EC 4.2.1.22), cystathionine (-lyase (CSE; EC 4.4.1.1), cysteine
aminotransferase (EC 2.6.1.3), mercaptopyruvate sulfurtransferase (MST; EC
2.8.1.2), rhodanase (thiosulfate cyanide sulfurtransferase; EC 2.8.1.1) and
cysteine lyase (EC 4.2.1.10) (Maclean and
Kraus, 2004; Stipanuk,
2004). Most vascular studies have focused on CSE and CBS as the
potential H2S-generating enzymes, although other enzymes may also
be involved (Maclean and Kraus,
2004).
CSE is thought to be the primary enzyme for H2S synthesis in
mammalian vessels. CSE mRNA has been identified in human systemic vessels and
rat pulmonary arteries; in rat systemic vessels, both CSE mRNA and the 43 kDA
CSE protein have been identified (Hosoki
et al., 1997; Zhao et al.,
2003; Cheng et al.,
2004; Wang et al.,
2004). We have also found CSE mRNA in systemic arteries, veins and
respiratory vessels of trout (R. Wang, R.A.D. and K.R.O., unpublished
observation). Unlike nitric oxide synthase and hemeoxygenase, CSE mRNA in rat
vessels is confined to vascular smooth muscle and is absent from the
endothelium (Wang et al.,
2004). The CSE inhibitor, propargyl glycine (PPG), inhibits
H2S production in rat vessels
(Hosoki et al., 1997;
Zhao et al., 2003), but in
bovine pulmonary arteries PPG did not significantly affect either
H2S production (Fig.
4), or hypoxic contraction
(Fig. 5). This suggests that
enzymes other than CSE also contribute to vascular H2S
production.
Previous studies have indicated that CBS is not involved in H2S
synthesis in mammalian vessels. CBS mRNA has not been detected in mammalian
(rat and human) vessels and the CBS inhibitor, aminooxyacetic acid (AOA) did
not block H2S production by rat vessel homogenates
(Hosoki et al., 1997;
Zhao et al., 2001;
Zhao et al., 2003;
Wang et al., 2004). However,
our findings suggest that in a number of vertebrates, CBS and perhaps other
enzymes are important in vascular H2S production. AOA partially
inhibits H2S production in homogenized bovine pulmonary arteries
and veins (Fig. 4), and trout
arteries and veins (Dombkowski,
2006), and it partially inhibits the hypoxic contraction of bovine
pulmonary arteries (Fig. 5). We
have also found that CBS mRNA is ubiquitously expressed in trout systemic
arteries, veins and respiratory vessels (R. Wang, R.A.D. and K.R.O.,
unpublished observation). Collectively, these studies suggest that CBS is also
involved in vascular H2S production.
Although we did not systematically examine all enzyme inhibitors in all
vessels, hydroxylamine appeared to have the greatest inhibitory effect on
H2S production and hypoxic responses. CBS, CSE and cysteine lyase
all depend on the co-factor, pyridoxal 5'-phosphate (PLP) for enzymatic
activity (Maclean and Kraus,
2004, and as hydroxylamine is a general inhibitor of PLP-dependent
enzymes (Kery et al., 1999),
it is possible that multiple enzymes contribute to H2S production
in some vessels.
Inhibition of H2S production inhibits hypoxic vasoconstriction and hypoxic vasodilation
The inhibition of both hypoxic vasoconstriction and hypoxic vasodilation by
inhibitors of H2S synthesis
(Fig. 5) further supports the
hypothesis that the vascular response to hypoxia and H2S are
interrelated. These studies also suggest that H2S synthesis may
depend on different, even vessel-specific, enzymes and that other enzymes, in
addition to CBS and CSE, may be involved in H2S production. PPG,
which inhibits CSE and H2S production by rat aorta
(Zhao et al., 2003),
essentially abolished hypoxic vasodilation in rat thoracic aortas
(Fig. 5B) and the CSE inhibitor
ß-cyano-L-alanine (BCA), partially inhibited hypoxic phase 1
contraction and phase 2 relaxation in rat pulmonary arteries and was no less
effective than AOA, BCA and PPG combined. However, CBS appears to account for
at least part of the hypoxic generation of H2S by bovine pulmonary
arteries as the CBS inhibitor, AOA, reduced hypoxic vasoconstriction by 50%,
whereas the CSE inhibitor, PPG, was ineffective
(Fig. 5D). This is consistent
with the predominance of CBS in H2S synthesis by these vessels
(Fig. 4). Although CBS mRNA has
not been identified in mammalian vessels, we have found it in trout vessels
(R. Wang, R.A.D. and K.R.O., unpublished observation) suggesting a potential
function.
The inhibitors used in our, and essentially all other studies on blood
vessels, are somewhat non-specific, e.g. AOA inhibits the
malate–aspartate shuttle (Bunger et
al., 1980), PPG inhibits L-alanine transaminase
(Burnett et al., 1980), BCA
interacts with NMDA receptors (Roy et al.,
1996) and hydroxylamine is a NO donor in rat aorta
(Beranova et al., 2005). Thus
it is possible that some of the effects of these inhibitors on hypoxic
vasodilation and hypoxic vasoconstriction may not involve H2S.
While it was beyond the scope of this study to characterize the non-specific
effects of these inhibitors on the mechanical properties of blood vessels,
several points are worth noting. First, we
(Fig. 4) and others
(Hosoki et al., 1997;
Zhao et al., 2003) have
clearly demonstrated that H2S synthesis by blood vessels is
sensitive to specific enzyme inhibitors. Second, inhibition of hypoxic
vasodilation and hypoxic vasoconstriction also appears somewhat dependent on
specific enzyme inhibitors, i.e. PPG is a better inhibitor of hypoxic
relaxation of the rat aorta than AOA, whereas AOA is more effective than PPG
in inhibiting hypoxic vasoconstriction in the bovine pulmonary artery. Third,
the direct effects of inhibitors on vessel tension do not necessarily mimic
their effect on hypoxic vasodilation and hypoxic vasoconstriction; HA
contracts lamprey aortas, but inhibits hypoxic vasoconstriction, and AOA has
essentially no effect on U-46619 pre-contracted bovine pulmonary arteries, but
also inhibits hypoxic vasoconstriction. The effects of HA on bovine pulmonary
arteries, however, could be non-specific through the release of NO
(Beranova et al., 2005). To our
knowledge, there are no specific inhibitors of H2S synthesis and
clearly they are needed to resolve this issue.
Addition of H2S precursor cysteine affects hypoxic responses
Cysteine, which is the precursor for H2S production, doubled the
force of a hypoxic contraction in both lamprey aortas and bovine pulmonary
arteries (Fig. 6A,B),
suggesting that under these circumstances H2S production was also
increased. The cysteine effect was not apparent in bovine pulmonary arteries
unless they had been exposed to prolonged hypoxia whereas pre-hypoxic exposure
was not needed in the lamprey. The difference between lamprey and bovine
vessels may be due to the amount of endogenous cysteine stored in the vessel
or to differences in metabolism. Incubation with cysteine also changed the
hypoxic responses of rat aortas, but it unexpectedly augmented the recovery
during re-oxygenation rather than the hypoxic relaxation. It is not clear how
this occurred.
H2S as a mediator of the hypoxic response
Collectively, the above experiments indicate that H2S
participates in vascular responses to hypoxia. We propose that it is the
metabolism of H2S that serves as the `O2
sensor/transducer' in vascular smooth muscle. In this model the concentration
of vasoactive H2S is regulated by the simple balance between
endogenous vascular H2S production and its oxidation by available
O2. As described below, the stoichiometric relationship between
[O2] and [H2S] in vascular smooth muscle and the
primordial precedent for H2S production in the cytosol and
oxidation in the mitochondria add anecdotal support to our model.
Recent studies have shown that PO2 in the walls of
systemic arterioles in many vascular beds is around 50 mmHg, partly because
they supply much of the O2 to tissues, and partly because the rate
of O2 consumption by the vessel wall is very high, up to 500 times
that of resting skeletal muscle (Tsai et
al., 2002; Shibata et al.,
2005). With an oxygen solubility around 10–6 mol
l–1 mmHg–1 (see
Shibata et al., 2005), the
O2 concentration in arteriolar smooth muscle would be
5–6x10–5 mol l–1. This is
strikingly similar to most reports showing plasma [H2S] in rats at
around 4–6x10–5 mol l–1
(Zhao et al., 2001;
Geng et al., 2004;
Yan et al., 2004;
Yusuf et al., 2005).
Unfortunately, intracellular [H2S] is unknown. It may equal or
exceed plasma [H2S], but it may also be lower due to
compartmentalization within the cell; it is well known that
10–6 mol l–1 H2S is toxic to
isolated mitochondrial cytochrome c oxidase, but not to intact cells
(see Dombkowski et al., 2005).
Thus if there is excess dissolved O2 relative to H2S, as
would be expected in normoxia, continual oxidation, and therefore
inactivation, of H2S would be expected. However, even moderate
hypoxia would lower arteriolar [O2], which would then decrease the
rate of H2S oxidation and allow intracellular [H2S] to
increase. This scenario is feasible. A 1 min reduction in inspired
PO2 in rats, which is similar to that experienced in
humans during sleep apnea, lowers PO2 in cremaster muscle
arterioles to 15.8 mmHg (Johnson et al.,
2005). This is essentially half that of plasma [H2S].
Furthermore, Doeller et al. observed
(Doeller et al., 2005) that
intact segments of rat aortas produced significant amounts of H2S
when the incubation medium [O2] was 4 µmol l–1,
but they could not detect H2S production when the medium
[O2] was raised to 200 µmol l–1, i.e. normoxia.
We predict that the resultant rise in [H2S] due to decreased
oxidation during hypoxia will then initiate the appropriate vascular
responses. The continual oxidation of H2S during normoxia may also
contribute to the high O2 demand of vascular smooth muscle.
Intracellular compartmentalization of H2S production and
oxidation appears to be a common property of all eucaryotic cells and we
propose that smooth muscle cells employ this to regulate [H2S].
There is accumulating evidence that mitochondria originated from sulfide
(H2S)-oxidizing bacteria and the nucleocytoplasm from
sulfide-reducing (H2S generating) Archaea
(Searcy, 2003). Where ancient
(and some modern) eucaryotic cells shuttled sulfur to generate ATP, we propose
that smooth muscle uses this mechanism to regulate the level of
H2S-mediated vasoactivity. In fact, H2S oxidation has
been demonstrated in chicken liver mitochondria
(Yong and Searcy, 2001) and
H2S production has been observed in cells lacking mitochondria such
as human erythrocytes (Searcy and Lee,
1998). The observations that H2S production is
essentially the same in normoxic and hypoxic erythrocytes
(Searcy and Lee, 1998),
whereas pieces of rat thoracic aorta produce H2S when hypoxic, but
consume H2S when normoxic
(Doeller et al., 2005), are
also consistent with our model.
It is also possible that vascular H2S production is actively
regulated as CBS appears to have a number of O2-sensitive
regulatory sites (Maclean and Kraus,
2004; Stipanuk,
2004; Banerjee and Zou,
2005). This needs further investigation. Even if the short-term
H2S response to hypoxia is not enzymatically regulated in vascular
smooth muscle, tonic regulation of H2S production could contribute
to resting (normoxic) tone and bias the pattern and magnitude of the hypoxic
response.
Function of multi-phasic H2S effects
The distinct phases of the H2S response in respiratory vessels
(Table 1) may have specific
physiological functions at different PO2 values. As shown
in Fig. 2, low [H2S]
relaxes bovine pulmonary arteries and higher [H2S] contracts them.
According to our hypothesis, much of the H2S produced by the
vascular smooth muscle cells during normoxia will be oxidized and the
resultant low [H2S] will dilate the vessels and minimize pulmonary
vascular resistance. However, during hypoxia, [H2S] will increase
and result in the characteristic constriction. Although H2S levels
have not been measured in bovine plasma or in smooth muscle intracellular
fluid, [H2S] in (putatively normoxic) rat plasma is usually around
4x10–5 mol l–1
(Zhao et al., 2001;
Geng et al., 2004;
Yan et al., 2004;
Yusuf et al., 2005). In fact,
it has been estimated that vascular H2S may approach
10–4 mol l–1 in some vessels
(Zhao and Wang, 2002),
although intracellular [H2S] may be somewhat lower due to
compartmentalization. As shown in Fig.
2, maximum dilation to H2S in bovine pulmonary artery
occurs around 10–5 mol l–1 H2S
and this is also the threshold for constriction. A tenfold increase in
[H2S] to 10–4 mol l–1 will shift
the vessel from nearly complete relaxation to 40% of a maximal H2S
contraction.
Distinct dose-dependent dilatory and constrictory effects of H2S
are not unique to bovine pulmonary arteries; we have also characterized them
in rainbow trout efferent branchial (systemic) arteries where they overlap
with plasma titers (Dombkowski et al.,
2004), and in Pekin duck pulmonary arteries
(Dombkowski et al., 2005). This
suggests that the PO2–H2S system is a
versatile bipolar effector of vascular responses to ambient O2 in
many vertebrates.
Acute vs chronic hypoxia
Previous investigators (Zhang et al.,
2003; Zhang et al.,
2004) have suggested that H2S is inversely related to
hypoxic pulmonary hypertension. They
(Zhang et al., 2003;
Zhang et al., 2004) reported
that hypoxia decreased H2S production in rat pulmonary arteries and
they concluded that the resultant loss in H2S-mediated vasodilation
contributed to the observed increase in pulmonary vascular resistance. While
this conclusion appears to contradict ours, it likely represents a
fundamentally different mechanism. First, they
(Zhang et al., 2003;
Zhang et al., 2004) examined
the effects of chronic (3 weeks, 6 h per day, 10% O2) hypoxia
in vivo, whereas our study focuses on the immediate effects of acute
hypoxia in isolated vessels. Second, they found that hypoxia produced vascular
hypertrophy, but because they did not directly examine the response of
pulmonary vessels to H2S, they could only assume that it would be a
relaxation similar to that observed in the aorta
(Zhao et al., 2001;
Zhao and Wang, 2002). Our
present and prior studies (Dombkowski et
al., 2004) show that H2S constricts many respiratory
vessels. Although it is likely that many of the effects of chronic hypoxia are
mediated by genomic factors (as shown by vascular remodeling), it is doubtful
that these would contribute to the acute hypoxic responses we observed.
Overview
Hypoxic vasoconstriction and dilation have been observed in blood vessels
from all classes of vertebrates and although numerous factors, endothelial and
otherwise, can modify these responses, it would seem that the basic mechanisms
intrinsic to vascular smooth muscle have a conservative evolutionary history.
Perhaps this is best exemplified in cyclostomes where the mono-phasic hypoxic
vasoconstriction is unencumbered by endothelial and other evolutionary
embellishments. H2S production and vasoactivity have a similar
phylogenetic profile and, based on the present study, H2S appears
to be interwoven with the hypoxic responses. To date, little is known
regarding the mechanism(s) of H2S vasoactivity other than its
demonstrated ability to open KATP channels and initiate
vasodilation. However, H2S may prove to be the most versatile
gasotransmitter because of its unique ability to participate in redox
reactions, form S-nitrosothiols, buffer at physiological pH, and exert
biological effects either as a gas or anion. Undoubtedly this versatility is
appropriately utilized by vascular smooth muscle.
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List of abbreviations |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionList of abbreviationsReferences |
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-lyase)
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Acknowledgments |
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Footnotes |
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Present address: Dept of Biology, Saint Mary's College, Notre Dame, IN
46556, USA 
Present address: Dept of Basic Medical Sciences, Mercer School of Medicine,
1550 College St Macon, GA 31207, USA
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionList of abbreviationsReferences |
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