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1 Department of Medicine, The issue of whether the acinar microvessel
response to alveolar hypoxia and hypercapnia is impaired in injured
lungs has not been vigorously addressed, despite the importance of
knowing whether it is or not when treating patients with serious lung injury in terms of permissive hypercapnia. Applying a real-time laser
confocal luminescence microscope, we studied hypoxia- and hypercapnia-induced changes in the diameter of the intra-acinar arterioles, venules, and capillaries of isolated rat lungs harvested from animals exposed for 48 h to 21%
O2 (group
N) or 90%
O2 (group H). Measurements were made with and
without inhibition of nitric oxide (NO) synthase (NOS) by
N
confocal microscope; hyperoxic lung injury; acinar
microcirculation; cyclooxygenase; nitric oxide synthase; hypoxia; hypercapnia
IN THE NORMAL LUNG, changes in pulmonary microvessel
tone in response to alveolar hypoxia and hypercapnia regulate the local distribution of pulmonary blood flow (4, 29, 32, 34). To the best of
our knowledge, however, no thorough attempts have ever been made to
determine whether these hypoxia- and hypercapnia-related regulatory
mechanisms of pulmonary microvessel tone are significantly impaired in
the injured lung. Several groups of investigators have attempted to
obtain definite evidence for changes in pulmonary vessel diameter in
response to hypoxia (9, 11, 14, 16, 21, 24) or hypercapnia (5, 6, 8,
16, 17, 23, 27, 28) on the basis of radiological and nonconfocal
microscopic studies. Unfortunately, however, these studies mainly
focused on events in small vessels outside pulmonary acini. We
developed a real-time confocal laser luminescence microscope coupled to a high-speed video camera to precisely distinguish dynamic cell kinetics in the arterioles, venules, and capillaries of a single pulmonary acinus (33). Applying this elaborate confocal system to
microvessel kinetics in rat acini, we studied intra-acinar microvessel
constriction and dilation elicited by hypoxia and hypercapnia in
the injured lung. Exact knowledge of microvessel reactions to oxygen is
indispensable when patients with diseased lungs are treated with
varying modes of artificial ventilation, because pulmonary gas exchange
is not adequately maintained if hypoxic microvessel constriction
deteriorates (4, 32, 34). The importance of clarifying the
hypercapnia-induced microvessel response in diseased lungs has
increased, because hypercapnic conditions are encountered when patients
are treated by controlled ventilation with permissive hypercapnia (1,
13). Because of their clinical significance, we hoped to shed light on
the following issues in injured lungs exposed to a hyperoxic
environment that are generally encountered when patients having serious
hypoxemia are artificially ventilated:
1) whether the hypoxia-induced
vascular response in acinar microvessels is impaired;
2) whether the hypercapnia-induced acinar microvessel response is abnormal;
3) the relative importance of NOS-
and COX-associated pathways for the impaired hypoxic response in acinar
microvessels; and 4) whether the
contribution of NOS- and COX-associated pathways to abnormal
hypercapnic microvessel reactions differs qualitatively from their
contribution to impaired hypoxic microvessel reactions.
Isolated perfused lung preparation. We
prepared isolated perfused lungs from pathogen-free 8-wk-old male
Sprague-Dawley rats weighing 250-300 g
(n = 163). Animals were housed in
either a normoxic (21% O2;
group N,
n = 46) or hyperoxic (90%
O2; group H, n = 117)
environment for 48 h. A detailed description of the isolated perfused
lung preparation is provided elsewhere (31). Briefly, the isolated lung
was fixed supine on a microscopic stage and perfused at a constant
recirculating flow rate of 15 ml/min. Krebs-Henseleit solution with 3%
BSA was used as the perfusate, and the hematocrit (Hct) was adjusted to
6.0 ± 0.5% by adding fresh blood from donor rats and erythrocytes
stained with FITC, as described below. Blood remaining within the lung
was expelled into the perfusion circuit during recirculation and used
as part of the perfusate. To prevent the movement produced by
artificial ventilation, the trachea was ligated in the end-inspiratory
position, and gas exchange was maintained with an extracorporeal
membrane oxygenator (ECMO; Merasilox-S; Senko, Tokyo, Japan). A gas
mixture containing 21% O2 and 5%
CO2 was used as the control gas
flowing into the ECMO, allowing adjustment of perfusate
PO2 to 141 ± 3 mmHg,
PCO2 to 36 ± 2 mmHg, and pH to
7.42 ± 0.02. A warmed, humidified gas mixture containing the same
gas composition as used for the ECMO was supplied to the lung surface
to maintain a temperature of 37 ± 0.5°C and to avoid lung
surface desiccation. Mean pulmonary arterial pressure (Ppa) was
continuously monitored by force displacement of pressure transducers
(TP-400T; Nihon Koden, Tokyo, Japan).
Experimental protocols. After
pulmonary hemodynamics stabilized, the gas flowing into the ECMO and
blown onto the lung surface was switched from the control gas to the
following mixtures for 15 min: 1)
hypoxic-normocapnic gas (2% O2
and 5% CO2 in
N2), which reduced
PO2 to 34 ± 2 mmHg without
changing PCO2 and pH levels in the
perfusate; and 2)
normoxic-hypercapnic gas (21% O2
and 15% CO2 in
N2), which increased perfusate
PCO2 to 95 ± 3 mmHg and decreased
pH to 7.1 ± 0.04 without altering perfusate
PO2. Changes in Ppa from the baseline
under given experimental conditions were used to measure overall
vascular resistance changes in pulmonary circulation, including
intra-acinar microvessels and large extra-acinar vessels. Measurements
of pulmonary hemodynamic changes during hypoxia and hypercapnia were
made at high and low basal tones of the pulmonary vasculature. High
basal tone was established by administering synthetic thromboxane
A2 [TXA2; ONO-11113
(9,11-epithio-11,12-methanothromboxane
A2); Ono, Tokyo, Japan]
into the perfusate [TX(+) group]. Low basal tone measurements were made in the absence of
TXA2 [TX( In the TX( In the TX(+) experiments, group N
during hypoxia and hypercapnia was measured agent free, with neither
L-NAME nor indomethacin administered (n = 4 hypoxia and
hypercapnia rats each), whereas group
H was measured under three different
experimental conditions: 1)
condition
C (n = 5 hypoxia and hypercapnia rats each), in which no agents were
administered; 2)
condition
L (n = 5 hypoxia and hypercapnia rats each), which was in the presence of
L-NAME; and 3)
condition
I (n = 5 hypoxia and hypercapnia rats each), in which indomethacin was administered.
Real-time measurement of acinar microvessel
kinetics. Erythrocytes were stained with FITC (Sigma,
St. Louis, MO). Fresh rat blood was centrifuged at 1,000 rpm, and the
buffy coat was discarded. The packed erythrocyte solution was diluted
with PBS, and FITC was added to give a final concentration of 0.1 mg/ml. This solution was then incubated at 37°C for 30 min and
washed three times in PBS. A 1-ml volume of FITC-labeled erythrocyte
solution was added to the perfusate, enabling determination of the
direction of flow in the pulmonary microcirculation. The microvessels
from which FITC-erythrocytes entered the capillary network were defined
as arterioles, and the microvessels into which FITC-erythrocytes flowed
from the capillary network were defined as venules. Microvessel diameter was measured by adding 200 µl of 5% FITC-dextran, which has
a molecular weight of 145,000 (Sigma). These microvessel events in the
acinus were studied precisely by using a recently developed real-time
confocal laser luminescence microscope (33). Fluorescent emission from
the specimen was imaged onto a high-sensitivity charge-coupled-device
camera with an image intensifier (EktaPro Intensified Imager VSG;
Kodak, San Diego, CA). By applying an excitation wavelength of 488 nm
emitted from a low-power argon laser (532-BSA04; Omnichrome, Chino,
CA), confocal units enabled us to obtain apparently instantaneous
images at 1,000 frames/s. The resulting field of view was 210 × 210 µm, corresponding roughly to the diameter of a single pulmonary
microvessel adjacent to the terminal bronchiole (33, 34), yielding
images creditably detecting events in a single acinus. We recorded
confocal images at 250 frames/s with a high-speed video analyzer
(EktaPro 1000 Processor; Kodak). The direction of FITC-erythrocyte flow
in the acinar microcirculation was determined during replays of the
videotapes at the normal video rate. Each replay frame represented
events during a 4-ms interval. We measured the diameter of each
microvessel by processing a confocal video image with a digital image
analyzer (Quadra 840AV/Image 1.58; Apple, Cupertino, CA).
Measurements of NO-related metabolites in the
perfusate. A 2-ml perfusate sample was centrifuged and
frozen at Measurements of prostacyclin metabolite in the
perfusate. A 2-ml perfusate sample collected in a tube
containing indomethacin and EDTA was centrifuged and frozen at
Statistical evaluation. The
statistical significance of differences was generally judged by one-way
ANOVA followed by multiple comparison Scheffés analysis. Ppa
increments, microvessel diameter changes, and perfusate concentrations
of NO and PGI2 metabolites on
hypoxia and hypercapnia during exposure to the same agent were compared
by applying an unpaired t-test. The
effects of TXA2 on the indexes,
including baseline Ppa, microvessel diameter, and concentrations of
vasoactive substances, were estimated by an unpaired
t-test. Changes in Ppa, microvessel
diameter, and NO and PGI2
metabolites after a given stimulation were assessed by a paired
t-test. Values are means ± SD,
with P < 0.05 statistically significant.
Pulmonary hemodynamics before hypoxic and hypercapnic
stimulation in the absence of
TXA2. Because many different
experimental conditions were employed, we defined "agent free" as
a condition in which neither
L-NAME nor indomethacin was
added to the perfusate, irrespective of the presence or absence of
TXA2. "Baseline" is used to
indicate conditions before hypoxic or hypercapnic stimulation.
Before exposure to hypoxia and hypercapnia, Ppa did not differ in
groups N and
H, and the values averaged 12.3 ± 2.5 mmHg. The baseline diameter of precapillary arterioles and
postcapillary venules before hypoxia or hypercapnia did not differ
between the groups, and ranged between 20 and 40 µm. Baseline
capillary diameter was 6-7 µm, with no difference between the
groups. Administration of L-NAME
or indomethacin did not alter baseline Ppa or microvessel diameter.
Hypoxia- and hypercapnia-induced microvessel diameter
changes in agent-free groups N and H in the absence of
TXA2. Hypoxia enhanced Ppa in
association with a reduction in arteriole diameter in
group N (Table
1; Figs. 1 and
2). Hypoxia-induced Ppa increments in
group
H, however, were conspicuously smaller
than in group N (Table 1). Although arteriole
diameter in group
H before hypoxic stimulation did not
differ from the diameter in group
N, hyperoxia-injured arterioles did
not constrict during hypoxia (Fig. 2).
Neither venule nor capillary diameter in
group
N or
H was altered by hypoxic stimulation
(Fig. 2).
ABSTRACT
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
-nitro-L-arginine methyl ester or
of cyclooxygenase (COX) by indomethacin at different basal vascular
tones evoked by thromboxane A2
(TXA2) analog. Hypoxia in the
absence of TXA2 contracted
arterioles in group
N but not in
group
H. Attenuated hypoxia-induced
arteriole constriction was restored almost fully by inhibiting NOS and
partially by inhibiting COX. Hypercapnia induced venule dilation in
group N, but did not dilate venules in
group
H, irrespective of
TXA2. NOS inhibition in
hypercapnia unexpectedly enhanced venule and arteriole dilation in
group
H. These responses no longer occurred when NOS and COX were inhibited simultaneously. In conclusion, microvessel reactions to hypoxia and hypercapnia are abnormal in
hyperoxia-injured acini, in which NO directly attenuates
hypoxia-induced arteriole constriction, whereas COX inhibited by
excessive NO impedes hypercapnia-induced microvessel dilation.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
MATERIALS AND METHODS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
)
group]. In the TX(+) experiments, 3.5 ml of
TXA2 solution prepared at 0.1 µg/ml was slowly added to the perfusate over 5 min to obtain a stable
Ppa transition throughout observations. The final concentration of
TXA2 in the perfusate was adjusted
to 5 ng/ml.
) experiments, hypoxia- or hypercapnia-induced changes
in Ppa and intra-acinar microvessel diameters in normoxia-exposed lungs
(group N) were estimated in the absence of
addition of any exogenous agents (n = 18 and 20 hypoxia and hypercapnia rats, respectively), whereas the
changes in hyperoxia-injured lungs (group
H) were analyzed under four
different experimental conditions: 1)
condition
C (n = 14 and 15 hypoxia and hypercapnia rats, respectively), in which no
agents were administered; 2)
condition
L (n = 10 and 12 hypoxia and hypercapnia rats, respectively), in which a
constitutive form of NO synthase (ecNOS) and an inducible form of NO
synthase (iNOS) were concomitantly inhibited with
N-nitro-L-arginine methyl ester
(L-NAME; 100 µmol/l);
3)
condition I (n = 9 and 11 hypoxia and hypercapnia rats, respectively), in which
indomethacin (20 µmol/l) was used to inhibit both constitutive and
inducible cyclooxygenase (COX-1 and COX-2); and
4)
condition LI (n = 7 and 9 hypoxia and hypercapnia rats, respectively), in which
measurements were made in the presence of both
L-NAME and indomethacin.
80°C immediately after collection. To measure NO
production in the lung, we studied the total concentration of end
products of NO metabolism, NO
2 and
NO3, by the modified method of Green
et al. (10). To deproteinize the perfusate sample, a 500-µl sample was mixed with 100 µl of 35% sulfosalicylic acid. The sample was then centrifuged, and 300 µl of 5%
NH4Cl and 60 µl of 5% NaOH were
added to 300 µl of the supernatant. The prepared sample was passed
through a high-pressure Teflon column packed with copper-plated cadmium
metal allowing reduction of NO3 to
NO2. The effluent was mixed with the
reagent containing sulfanilamide and
N-(1-naphthyl)ethylenediamine in
phosphoric acid, and the color of the product yielded by the
diazotization reaction was examined at 0°C with a spectrophotometer
(US 501; Unisoku, Osaka, Japan) at an absorbance wavelength of 546 nm.
80°C until extraction. Measurements were made by extracting
1 ml of the sample into medium containing 4 ml of ethyl acetate. The
ethyl acetate layer was transferred to a second tube and evaporated to
dryness with pure N2 gas. The
dried extract was reconstituted in the assay buffer, and the
concentration of immunoreactive 6-ketoprostaglandin
F1
(6-keto-PGF1), the stable
metabolite of prostacyclin
(PGI2), was measured by ELISA
(EIA kit; Cayman Chemical, Ann Arbor, MI).
RESULTS
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
Table 1.
Ppa increments from baseline in groups N and H during exposure to
hypoxia and hypercapnia in the absence of TXA2
View larger version (145K):
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Fig. 1.
Confocal views of hypoxia-induced arteriole constriction and
hypercapnia-induced venule dilation in an intact acinus without
addition of any agents, including thromboxane
A2
(TXA2; 20× objective).
Top: arteriole before
(A) and after
(B) hypoxia.
Bottom: venule before
(C) and after
(D) hypercapnia.
View larger version (19K):
[in a new window]
Fig. 2.
Arteriole (A) and venule
(B) responses to hypoxia and
hypercapnia in rats exposed for 48 h to 21%
(group N) or
90% O2 (group
H) in the absence of
TXA2. Data are absolute diameter
changes expressed in µm. C, agent free; L,
N -nitro-L-arginine methyl ester
(L-NAME) administration;
I: indomethacin administration. LI: concurrent
administration of L-NAME and
indomethacin. * Active vasoconstriction or vasodilation;
# significantly different
from group
N under
condition
C;
+ significantly different
from group
H under
condition
C;
$ significantly different
from group
H under
condition
L;
& significantly different
from group
H under
conditions
L and
LI.
Exposure to hypercapnia increased Ppa in both groups, but the degree of the Ppa increment was significantly greater in group H (Table 1). Hypercapnia elicited distinct venule dilation in group N but no change in arteriole or capillary diameter (Figs. 1 and 2). This hypercapnia-induced venule dilation was not seen in group H (Fig. 2). Arteriole and capillary diameter did not change in group H during hypercapnia (Fig. 2).
Effects of NOS inhibition on hypoxia- and hypercapnia-induced microvessel diameter changes in group H in the absence of TXA2. L-NAME administration yielded a significant Ppa increment during hypoxia, comparable to the increment in group N (Table 1). L-NAME concomitantly restored hypoxic arteriole constriction without any change in venule or capillary diameter (Fig. 2).
The hypercapnia-induced increase in Ppa in the presence of L-NAME was smaller than in its absence (Table 1). Contrary to our expectation, L-NAME augmented venule and arteriole dilation during hypercapnia (Fig. 2).
Effect of COX inhibition on hypoxia- and hypercapnia-induced microvessel diameter changes in group H in the absence of TXA2. Although indomethacin restored arteriole constriction with hypoxia, its extent was smaller than that of L-NAME (Fig. 2). Indomethacin did not improve hypoxia-induced Ppa changes (Table 1), nor did it alter venule and capillary diameter after hypoxia (Fig. 2).
Compared with the agent-free results, administration of indomethacin alone did not alter the hypercapnia-induced Ppa increment in association with no change in arteriole, venule, or capillary diameter (Table 1; Fig. 2).
Effect of simultaneous inhibition of NOS and COX on hypoxia- and hypercapnia-induced microvessel diameter changes in group H in the absence of TXA2. Compared with the results with L-NAME alone, no additional improvement in microvessel constriction or overall Ppa increment on hypoxia was seen in response to concurrent L-NAME and indomethacin administration (Table 1; Fig. 2).
The augmentation of hypercapnia-induced venule and arteriole dilation observed in group H in the presence of L-NAME alone was inhibited in the concomitant presence of L-NAME and indomethacin (Fig. 2). Furthermore, simultaneous administration of both agents enhanced the Ppa increment to a level equal to that under agent-free conditions (Table 1).
Effects of TXA2 on microcirculatory hemodynamics in groups N and H during hypoxic and hypercapnic gas breathing. TXA2 analog increased baseline Ppa by a comparable amount in groups N and H under agent-free conditions (increment in group N, 3.6 ± 3.2 mmHg; in group H, 2.2 ± 0.9 mmHg). Group H baseline Ppa was enhanced by 4.2 ± 4.7 mmHg by TXA2 concomitant with L-NAME and by 2.2 ± 1.4 mmHg in the presence of TXA2 and indomethacin. These increments were not different from the values observed under agent-free conditions.
TXA2 distinctly augmented
hypoxia-induced Ppa changes under all experimental conditions studied
for group
H, decreasing differences in the
hypoxia-induced overall pressor response observed in the absence of
TXA2 (Table
2). The extent of arteriole constriction on
hypoxia in the presence of TXA2
did not differ among the experimental conditions in
group
H (Fig.
3). The hypoxia-induced arteriole constriction in group
H was not different from that obtained
in group
N (Fig. 3). Neither venule nor
capillary diameter was modified by hypoxia under
TXA2 conditions in
group
H.
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The hypercapnia-induced Ppa increments in groups N and H were larger in the presence of TXA2 than in the absence of TXA2 (Tables 1 and 2). The Ppa increase in response to hypercapnia with TXA2 in group H was even larger than in group N (Table 2). The Ppa increase in the presence of L-NAME in combination with TXA2 in group H was much smaller than obtained under agent-free conditions or in the presence of indomethacin (Table 2). The extent of hypercapnia-induced venule dilation in group N with TXA2 did not differ from that obtained without TXA2, whereas arteriole constriction was observed during hypercapnia in group N when TXA2 was administered (Fig. 3). Hypercapnia-induced venule dilation was not seen in group H with TXA2, but group H arterioles showed constriction in response to hypercapnia when TXA2 was present (Fig. 3). Hypercapnic stimulation in the presence of TXA2 evoked venule and arteriole dilation in group H when L-NAME was added (Fig. 3). In the presence of TXA2, the hypercapnia-induced microvessel diameter changes with indomethacin were quantitatively the same as those observed when agent free (Fig. 3).
Perfusate concentrations of NO and
PGI2 in groups N and H in the
absence of TXA2. In the agent's
absence, the baseline perfusate NO concentration in
group
H was 1.7× that in
group
N (Table
3). Hypoxia augmented NO production in both
groups, but hypercapnia did not.
L-NAME suppressed baseline NO
production and the increase after hypoxia in
group
H.
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The baseline concentration of perfusate
6-keto-PGF1 under agent-free
conditions was higher in group H than
in group N (Table 4). Agent-free
6-keto-PGF1 production was
enhanced during hypoxia and hypercapnia in both groups. Indomethacin
reduced the baseline 6-keto-PGF1 concentration in
group H to a level comparable to that
in group N (Table 4). Indomethacin
inhibited the 6-keto-PGF1 increase after hypoxia and hypercapnia in group
H. The influence of
L-NAME on
6-keto-PGF1 production in
group
H differed depending on whether the
conditions were hypoxic or hypercapnic, i.e., hypoxia augmented
6-keto-PGF1 production in the
presence of L-NAME, but hypercapnia did not (Table 4).
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Perfusate concentrations of NO and PGI2 in groups N and H in the presence of TXA2. Perfusate concentrations of NO metabolites before and after hypoxia obtained in the presence of TXA2 did not differ from those in the absence of TXA2 in groups N and H. Qualitatively the same trend was observed in hypercapnic experiments. L-NAME reduced NO concentrations in both groups.
Concentrations of 6-keto-PGF1
under baseline conditions were higher in the presence of
TXA2 than in the absence of
TXA2 in groups
N and
H (Table
5). Both hypoxia and hypercapnia in the presence of TXA2 enhanced
6-keto-PGF1 production under
agent-free conditions in group
H, but the enhancement was inhibited
by indomethacin (Table 5). In the concomitant presence of
TXA2 and
L-NAME, hypoxic stimulation
augmented 6-keto-PGF1
production in group
H, but hypercapnic stimulation did not
(Table 5).
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Critique of methods. We perfused the
isolated lung with buffer containing a small quantity of fresh blood,
just enough to delineate the outlines of intra-acinar microvessels on
confocal observation. This is because we wanted to preclude
constriction and dilation elicited by vasoactive substances released
from leukocytes and platelets in the blood. As shown by Barnard et al.
(3) and Wilson et al. (30), however, the extent of NO and prostaglandin (PG) production in the lung may be closely related to vascular wall
shear force, which depends on perfusate viscosity, and in turn is
mainly governed by the Hct. They (3, 30) examined the vascular response
to NOS inhibitors and perfusate concentrations of COX-associated
products and reported that NO and PG production in the intact lung is
enhanced in parallel with increasing perfusate viscosity. Their
findings (3, 30) suggest that our experiments were substantially flawed
in assessing the important roles of vasoactive compounds in pulmonary
microvessels because of the significantly lower Hct than in vivo. To
overcome these obstacles, we estimated microvessel kinetics in both the
presence and absence of the stable
TXA2 analog, allowing shear force
along the microvessel wall to change. In fact,
TXA2 augmented baseline Ppa, the
increments in Ppa after hypoxic or hypercapnic stimulation, and
perfusate concentrations of
6-keto-PGF1 in
group
N compared with the values obtained in
the absence of TXA2 (Tables 2 and
5). Although the overall perfusate concentrations of NO were not
increased by addition of TXA2 in
group H, the
L-NAME-associated Ppa increments
in group H during hypoxia were much
larger in the presence of TXA2
than in the absence of TXA2
(Tables 1 and 2). These results suggest that addition of
TXA2 increases NO production
locally in the lung, but this is not always reflected in the overall
circulating medium. These findings appear to be consistent with those
reported by Barnard et al. (3) and Wilson et al. (30).
The direction of the microvessel diameter changes in response to hypercapnia under various experimental conditions in groups N and H did not differ qualitatively according to whether TXA2 was present or absent. Meanwhile, fine differences in hypoxia-induced microvessel diameter changes between agent-free conditions and conditions in which L-NAME and/or indomethacin were present but TXA2 was absent were not observed in the presence of TXA2 (Figs. 2 and 3). These findings seem to indicate that vasodilator production in the lung is actually augmented by TXA2 but that its effect on microcirculatory kinetics is masked by the constrictive effect of TXA2, especially during hypoxic stimulation. This suggests that the lung preparation perfused with low-Hct medium in the absence of TXA2 is superior to the preparation in the presence of TXA2 when attempting to detect subtle roles of vasodilators in modifying the vascular reactivity of acinar microvessels. Further study, however, is necessary to determine whether our experimental results regarding microvessel kinetics can actually be applied in vivo, where the Hct is much higher than in the present experiments. Unless otherwise specified, the discussions below focus on the acinar microvessel response to hypoxia and hypercapnia without TXA2.
Abnormal response of hyperoxia-injured microvessels to hypoxia. Attenuated hypoxia-induced arteriole constriction in hyperoxia-injured acini was caused independently by increased production of vasodilating NO and PGs, because inhibition of either NOS or COX allowed arterioles to regain contractility during hypoxic stimulation (Fig. 2). The importance of NOS and COX was supported by the increased concentrations of NO and PGI2 in the perfusate excreted from the hyperoxia-injured lung (Tables 3 and 4). The vasodilating substances yielded by NOS, however, appear to be more significant in blunting hypoxia-induced arteriole constriction than those yielded by COX (Fig. 2). Hypoxia-induced overall Ppa changes differed quantitatively between L-NAME and indomethacin; i.e., L-NAME markedly improved Ppa changes after hypoxia in hyperoxia-injured lungs, whereas indomethacin did not (Table 1). Because the overall Ppa increment reflects the sum of the pressor response imposed by all intra-acinar and extra-acinar vasculature (34), microvascular analysis, together with Ppa measurements, indicates that NOS upregulation in hyperoxia-injured lungs occurs along both intra-acinar and extra-acinar arterioles, whereas COX upregulation is confined to intra-acinar regions. Our findings are qualitatively consistent with in vitro studies reported by Liao et al. (20) and Lee et al. (19). Liao et al. (20) demonstrated an increase in ecNOS mRNA in bovine pulmonary artery endothelial cells exposed to hyperoxia, and Lee et al. (19) reported that exposure to hyperoxia upregulated COX in perinatal rat lung cells.
Abnormal response of hyperoxia-injured microvessels to
hypercapnia. In intact acini, the hypercapnia-induced
vasodilation was restricted to venules (Figs. 1 and 2) in association
with an increase in perfusate
6-keto-PGF1 but not in NO
metabolites (Tables 3 and 4). We recently demonstrated
that vasodilating PGs are the main substances mediating
hypercapnia-induced venule dilation in intact rat acini, whereas NO has
little impact on it (34). In the present study, we found that
hypercapnia-induced venule dilation in hyperoxia-injured lungs was
largely attenuated under agent-free conditions but that it was
unexpectedly restored by NOS inhibition, irrespective of the presence
or absence of TXA2 (Figs. 2 and
3). These phenomena were no longer observed when NOS and COX were
inhibited concurrently (Fig. 2). Taken together, our findings strongly
suggest that COX activity causing hypercapnia-induced venule dilation
is distinctly concealed, probably by COX inhibition by NO. This concept
may explain the functional equivalence between the agent-free
conditions and conditions in which COX is inhibited by indomethacin,
neither of which caused constriction or dilation in hyperoxia-injured
venules on hypercapnia (Fig. 2). Because COX is a hemoprotein
containing iron, NO is expected to alter COX activity by interacting
with iron at the active site. Several groups that used purified COX-1
and COX-2 enzymes have reported dual effects of NO on COX activity in
vitro (7, 15, 18, 22, 25, 26), i.e., inhibition and excitation of COX
by NO. COX-1 activity is maintained by ferric irons, and COX-2 activity is maintained by ferrous irons (15, 26). Tsai et al. (26) demonstrated
that NO is a strong ligand for ferrous irons and that COX-2 (ferrous
form) activity is almost completely inhibited by the presence of NO
under anaerobic conditions. Kanner et al. (15) found that ferric COX-1
activity is largely inhibited by NO because of its ability to reduce
the ferric enzyme to the ferrous form and because of competition for
iron sites available for exogenous ligands. These studies indicate that
NO inhibits the activity of the respective COX isoform. Landino et al.
(18) reported that NO significantly enhances the activity of purified
COX-1 and COX-2 when both NO and superoxide production is augmented. This is because peroxynitrite, a coupling product of NO and superoxide, specifically modulates both COX isoforms, indicating that NO-exciting COX activity must be taken into account in oxidative states. Given our
experimental conditions, hyperoxia exposure is expected to enhance the
generation of reactive oxygen species (2, 12, 31) and NO in the lung
(Table 3), suggesting that both inhibitory and excitatory effects of NO
on COX isoforms must be taken into account under our experimental
conditions. Our findings of restoration in hypercapnia-induced venule
dilation by NOS inhibition (Fig. 2) are consistent with the notion that
the inhibitory effect of NO on COX activity exceeds its excitatory
effect, at least in hyperoxia-injured venules under hypercapnia.
Negative modulation of COX pathways by NO may not, however, completely
explain the hypercapnia-induced changes in perfusate
6-keto-PGF1 concentrations during NOS inhibition in hyperoxia-injured lungs. Hypercapnia did not
increase perfusate 6-keto-PGF1
concentrations when NOS was inhibited (Table 4). This requires
NO-dependent COX excitation, suggesting that the inhibitory effect of
NO on COX is confined to intra-acinar regions where venules are
located, whereas the excitatory effect of NO on COX may dominate in
other lung regions.
Although we previously demonstrated that intact arterioles are not sensitive to hypercapnia (34), the present study showed that hyperoxia-injured arterioles dilated on exposure to hypercapnia when NOS was inhibited but that this arteriolar dilation was lost when NOS and COX were simultaneously inhibited (Fig. 2). These findings suggest that hyperoxia-injured arterioles basically become more reactive to vasodilating PGs, but this is generally masked by the negative effect of excessive NO on the COX pathway. The unexpected reduction in overall Ppa increment during hypercapnia with L-NAME in hyperoxia-injured lungs may be attributable to enhanced venule and arteriole dilation under L-NAME conditions (Fig. 2; Table 1). Interestingly, negative crosstalk between NOS and COX pathways does not appear evident during hypoxic stimulation (Fig. 2; Table 1), indicating that hypercapnia per se and/or hypercapnia-induced acidosis is indispensable for eliciting NO-dependent reduction in COX activity in acinar microcirculation. To the best of our knowledge, this is the first study demonstrating that negative modulation of COX pathway by NO plays an important role in distorting microvascular response to hypercapnia in acinar regions injured by hyperoxia exposure.
Our findings have valuable clinical implications, i.e., NOS inhibitors administered while treating patients with injured lungs by permissive hypercapnia improves gas exchange by reducing alveolar edema via relieving venule constriction. Meanwhile, the improvement in hypoxia-induced arteriole constriction by NOS inhibitors is counteracted by enhanced hypercapnia-induced arteriole dilation. COX inhibitors may not be as effective as NOS inhibitors, because COX inhibition is latently achieved by enhanced NO production in injured acinar microvessels.
In conclusion, although the diameter of intact intra-acinar arterioles varies with changes in ambient PO2, this is blunted in the microcirculation of lungs injured by exposure to hyperoxia. The blunted arteriole responsiveness to O2 is caused by enhanced production of both NO and PGs along microvessel walls, with NO seeming to be more potent than PGs. Although the hypercapnia-induced vasodilator response of hyperoxia-injured venules is basically the same as that of normal venules, this is apparently masked by the inhibitory effect of excessive NO on COX activity. Injured arterioles show a greater vasodilator response to hypercapnia than normal arterioles, but this is also masked by the negative interaction between NOS- and COX-dependent pathways. Crosstalk between these two pathways is important in hypercapnia with both NOS and COX upregulated, whereas this mechanism has little influence in hypoxia.
Perspectives
We found that hypoxia- and hypercapnia-induced microvessel responses in hyperoxia-injured acini were distinctly impaired by NOS and COX upregulation. However, the issue of which isoform of each enzyme is more significant in causing these abnormal responses has never been determined with certainty. In our next step, we plan to partition abnormal microvessel reactions to physiological stimuli into those evoked by constitutive enzymes (ecNOS and COX-1) and those by inducible forms (iNOS and COX-2). This is absolutely important when attempting to minutely describe hypercapnic augmentation of crosstalk between NOS and COX pathways in hyperoxia-injured acini, because both constitutive and inducible forms of NOS and COX are expected to be upregulated by exposure to hyperoxia. Clinically, it is also valuable to determine the importance of crosstalk between NOS and COX pathways for acinar microvessel responses to hypoxia and hypercapnia in other forms of injured lungs.| |
FOOTNOTES |
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The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. §1734 solely to indicate this fact.
Address for reprint requests and other correspondence: K. Yamaguchi, Dept. of Medicine, School of Medicine, Keio Univ., 35 Shinanomachi, Shinjuku-ku, Tokyo 160-8582, Japan (E-mail: yamaguc{at}cpnet.med.keio.ac.jp).
Received 29 July 1998; accepted in final form 30 March 1999.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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