Circulation Research. 2001
Published online before print June 7, 2001,
doi: 10.1161/hh1201.092035
A more recent version of this article appeared on June 22, 2001
(Circulation Research. 2001;0:hh1201.092035.)
© 2001 American Heart Association, Inc.
Distinct Pathways of Ca2+ Sensitization in Porcine Coronary Artery
Effects of Rho-Related Kinase and Protein Kinase C Inhibition on Force and Intracellular Ca2+
Koji Nobe
Richard J. Paul
From the Department of Molecular and Cellular Physiology, University of
Cincinnati College of Medicine, Cincinnati, Ohio.
Correspondence to Dr Richard Paul, Department of Molecular and Cellular Physiology, University of Cincinnati College of Medicine, 231 Albert Sabin Way, Cincinnati, OH 45267-0576. E-mail richard.paul{at}uc.edu
Abstract
Abstract—Alterations
of the Ca2+ sensitivity of contraction have
been reported for porcine coronary artery, but the mechanisms
are not clearly understood. We investigated the mechanism(s) of
Ca2+ sensitization in response to the
thromboxane A2 analogue (U46619).
Our hypothesis is that different mechanisms of
Ca2+ sensitization could be distinguished by
their distinct time courses. Therefore, we measured the time course of
[Ca2+]i and
isometric force simultaneously in an intact artery after a
single addition of U46619. The initial transient phase was associated
with Ca2+ release from the sarcoplasmic
reticulum, whereas the maintained phase was associated with
Ca2+ influx. Two distinct types of
Ca2+ sensitization characterized these
phases with either protein kinase C (PKC)-mediated or
Rho-kinase–mediated mechanisms. Their effects were quite distinct on
the basis of the time courses over which the sensitization was
effective. PKC inhibition (1 µmol/L calphostin C) had a much greater
effect in the initial phase, diminishing the size of the transient and
prolonging the rise in force and the decline in
[Ca2+]i. There were
limited effects on the sustained force. Rho-kinase inhibition (10
µmol/L Y27632), in contrast, nearly abolished the sustained force but
had a lesser effect on the transient phase. Neither
inhibitor had any effect on the force versus
[Ca2+]i relations
for KCl contractures. Our evidence suggests that both PKC-mediated and
Rho-kinase–mediated Ca2+ sensitizations are
present in coronary arteries, but the latter is dominant in
thromboxane A2 receptor–mediated
contraction.
Key Words: coronary arteries • Ca2+ sensitization • protein kinase C • Rho-kinase • U46619
Vascular smooth
muscle contractility is dependent not only on
intracellular Ca2+ concentration
([Ca2+]i) but also
on the Ca2+ sensitivity of the contractile
apparatus.1
Agonist-mediated activation is generally associated with a higher
Ca2+ sensitivity (greater maintained
isometric force per unit increase in
[Ca2+]i) than that
observed for activation via
depolarization.2 Further
proof of the existence of Ca2+ sensitivity
in smooth muscle contraction was obtained in studies on
permeabilized smooth muscle, in which
Ca2+ can be maintained at fixed levels. In
the presence of GTP, agonists can enhance force at constant
[Ca2+]i.3 4
Thus, our understanding of the mechanisms of receptor-coupled
activation of smooth muscle contraction now include a significant
component attributable to Ca2+
sensitization.5
The mechanisms proposed for Ca2+
sensitization generally fall into two classes. One class alters the
relation between myosin regulatory light chain
phosphorylation and
[Ca2+]i, involving
the myosin light chain kinase or phosphatase cascades. Myosin
regulatory light chain phosphorylation has long been
recognized as a major factor regulating smooth muscle
force.6 Another pathway of
sensitization involves alteration of the
Ca2+ affinity of other proposed regulatory
proteins, such as caldesmon or calponin. These thin
filament–associated proteins are generally postulated to inhibit the
actin-myosin interaction, and this inhibition is proposed to be
relieved by
Ca2+.7
One of the initial hypotheses proposed for
Ca2+ sensitization involved protein kinase C
(PKC).8 Evidence includes the
observation that direct activation of the PKC by phorbol ester
treatment increases force9
and translocation of
calponin.10 More recently,
much attention has been given to the role of the small G protein Rho in
the Ca2+ sensitivity of smooth muscle
contraction. Activated Rho induces
phosphorylation and inactivation of myosin light chain
phosphatase mediated by Rho-related kinase
(Rho-kinase).11 Inhibition
of phosphatase has long been known to elicit contraction in
permeabilized smooth muscle under conditions in which
Ca2+ is maintained below the contraction
threshold.12
Agonist-induced coronary artery responses have
important implications for cardiac function and
cardiovascular disease. Ca2+
sensitization based on in vivo measurements is particularly striking in
porcine coronary arteries with the thromboxane
A2 (TXA2) analogue
(U46619)2 13 ;
thus, its mechanism is of considerable interest. It is possible that
multiple Ca2+-sensitization mechanisms are
in play in this vessel. Sato et
al14 have reported that
endothelin-1 and carbachol enhance force at constant
[Ca2+]i in
ß-escin–permeabilized porcine coronary
arteries. They reported that the Rho-mediated
Ca2+ sensitization might be involved in the
endothelin-1–induced contraction but, surprisingly, was not involved
in the responses to carbachol.
The existence of multiple mechanisms of
Ca2+ sensitization may be differentiated in
view of differences in their time courses. It has long been postulated
that the mechanisms underlying the initial phase of tension development
may be different from that of tension
maintenance.15 16
The aim of the present study was to investigate the
mechanism(s) of Ca2+ sensitization in
U46619-induced contraction in porcine coronary artery. Our
hypothesis is that different mechanisms of
Ca2+ sensitization could be distinguished by
their potentially distinct time courses. The evidence for the operation
of these pathways of Ca2+ sensitization in
vivo and for their clinical significance has been inferred largely from
studies based on contractility
alone.17 18
Therefore, we measured the time course of
[Ca2+]i and
isometric force simultaneously in an intact artery in
response to a single addition of U46619. We report that U46619-induced
contraction is characterized by two distinct phases of
Ca2+ sensitization, having either
PKC-mediated or Rho-kinase–mediated mechanisms, with the latter
dominant in the steady state. This is the first direct evidence in
intact coronary arteries for an increase in
Ca2+ sensitivity associated with
Rho-kinase.
Materials and Methods
Materials
Y27632 was a gift from the Welfide Corp (Osaka,
Japan). Fura 2 was purchased from Molecular
Probes. All other reagents were of the highest purity and
were purchased from Sigma Chemical Co. U46619
was dissolved in ethanol, and calphostin C, phorbol
12-myristate 13-acetate (PMA), calyculin A, and SQ29548 were
dissolved in dimethyl sulfoxide; no effects of vehicle were noted if
total vehicle was 
0.03%. Physiological salt
solution (PSS) contained 122 mmol/L NaCl, 4.73 mmol/L KCl,
15.0 mmol/L NaHCO3, 1.19 mmol/L
MgCl2, 0.02 mmol/L EDTA, 1.19 mmol/L
KH2PO4, 2.5 mmol/L
CaCl2, and 11.1 mmol/L glucose aerated with
95% O2/5% CO2 for a pH
of 7.4 at 37°C. MOPS-buffered PSS (MOPS-PSS) contained 140
mmol/L NaCl, 4.70 mmol/L KCl, 1.20 mmol/L
NaH2PO4, 20.0 mmol/L
MOPS, 0.02 mmol/L EDTA, 1.2 mmol/L
MgSO4, 2.5 mmol/L
CaCl2, and 11.1 mmol/L glucose with a pH of
7.4 by NaOH at 37°C.
Preparation of Coronary Artery
Smooth Muscle Rings
Porcine hearts obtained shortly after slaughter were
rinsed of blood and placed in cold (4°C) PSS. The distal portions of
the left anterior descending coronary artery were dissected and
placed in ice-cold PSS. Arteries were then cleaned of fat and
connective tissue and cut into 5-mm segments. The arterial
wall thickness was between 300 and 500 µmol/L. The segments were
everted to expose the luminal side for fluorescence
measurements and deendothelialized by rolling
gently on filter paper.
Measurement of
[Ca2+]i and
Isometric Force
[Ca2+]i
was measured with the fluorescent dye fura 2-AM as previously
described.13 The
arterial rings were mounted isometrically on a
stainless-steel bracket. Arteries were then incubated for 3 hours
at 20°C in a well-stirred MOPS-PSS containing 12.5 µmol/L fura
2-AM, 0.005% pluronic F-127, and 2 mg/mL BSA. After incubation, the
tissues were rinsed in PSS for 20 minutes to remove any residual dye.
Arterial segments were attached to a movable post connected
to a Kent force transducer. Resting tension was adjusted to 30 to 40
mN. This value was chosen on the basis of prior experiments to set a
tissue length in the optimal range for maximum tension development.
Isometric force was expressed as mN/mm2;
cross-sectional area was approximated as 2xwet
weight/circumference.
The mounted artery was placed into a cuvette, and this
assembly was placed a water-jacketed holder maintained at 37°C in a
PTI Delta Scan-1 (Photon Technology
International) spectrofluorometer. The cuvette was aligned
such that the artery was configured for front face measurements.
Fluorescence was excited at 340 and 380 nm, and emission was
measured at 510 nm. The fluorescence intensity at 340-nm
excitation was divided by that measured at 380 nm, and this ratio
(R340/380) was used in calibration of absolute
[Ca2+]i, according
to Grynkiewicz et al.19
Ca2+ calibrations are dependent on a number
of assumptions, including the value for the
Kd (224
nmol/L). Although this is always a factor in interpretation of fura 2
data, the relative values (eg, when
[Ca2+]i is
expressed in terms of the maximum) are valid. Details of various
Ca2+ calibrations and assumptions in intact
porcine coronary artery have been
reported.13
Analysis of Data
Values given are mean±SEM; n values are the number
of hearts from which arteries were taken. Significance was determined
by standard ANOVA with the Bonferroni method used for multiple
comparisons.
Results
U46619-Induced
[Ca2+]i and
Isometric Force Responses in Coronary Artery
Resting
[Ca2+]i and force
averaged 121.0±5.5 nmol/L and 2.00±0.12
mN/mm2, respectively (n=29). U46619 (100
nmol/L) increased both
[Ca2+]i and force
(Figure 1A
).
[Ca2+]i increased
rapidly, and maximal values were attained within 1 minute, averaging
1115.7±10.3 nmol/L (n=7).
[Ca2+]i then
decreased, almost as rapidly, to a low but suprabasal steady-state
level, averaging 201.6±13.5 nmol/L (n=7). Force developed with a much
slower time course. The maximal response (14.93±0.48
mN/mm2, n=7) occurred within 5 minutes of
stimulation, and >90% of the maximal response was maintained for at
least 15 minutes. When
[Ca2+]i reached its
peak level, force was only 19.7% (4.86±0.55
mN/mm2, n=7) of maximum. The relation
between the peak responses of
[Ca2+]i and force
for U46619 (1 to 300 nmol/L) is shown in
Figure 1B. Values of EC50 for
[Ca2+]i and force
were 15.48 and 19.99 nmol/L, respectively. The
TXA2 receptor antagonist SQ29548 (1
µmol/L, 10-minute pretreatment) abolished the responses to U46619
without affecting baseline
(Figure 1B, inset).
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Figure 1. U46619-induced changes in [Ca2+]i and isometric force. Fura 2–loaded tissue was stimulated with U46619 at 37°C for 3 minutes. Fluorescence was excited at 340 and 380 nm, and emission intensities at 510 nm were recorded. A, Typical recording of simultaneous measurements of isometric force ( ) and [Ca2+]i (•), calculated as described in Materials and Methods. B, Concentration-maximal response relations. Inset, Tissues were preincubated in the presence or absence of the TXA2 receptor antagonist (1 µmol/L SQ29548 [SQ]) for 10 minutes, and then 100 nmol/L U46619 (U4) was added. [Ca2+]i (dark bars) and isometric force (light bars) are presented as a percentage of the U46619-induced responses (% of max responses). *P<0.05 vs U46619 responses. C, Data from panel B replotted as isometric force vs [Ca2+]i relations. In the transient phase of the U46619-induced responses, the relation between the maximal [Ca2+]i value (a) and the isometric force developed at that time (b) as shown in panel A is denoted as the a-b relation (diamonds). The relation between the maximal sustained force (c) and its corresponding [Ca2+]i value (d) is designated the c-d relation (squares). The relation between the maximal isometric force (c) and the max [Ca2+]i value (a) is designated as the a-c relation (circles).
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Force versus
[Ca2+]i relations
were analyzed
(Figure 1C
) by using the 4 parameters indicated
in
Figure 1A. Point a is the maximal
[Ca2+]i response
corresponding to a particular concentration of U46619. Point b is the
value of force attained at the time of the peak
[Ca2+]i. Point c is
the maximal force, and point d is the
[Ca2+]i level
occurring at that time. The transient phase of the force versus
[Ca2+]i relation is
delineated by the a-b relation; the sustained phase, by the c-d
relation; and the relation between maximal increase in force and that
in [Ca2+]i, by the
a-c relation. Strong significant correlations between force and
[Ca2+]i were
observed for the a-b, c-d, and a-c relations;
r2
values were 0.908, 0.726, and 0.998, respectively. The
Ca2+ sensitivity of the sustained phase (the
slope of the c-d relation) was markedly greater than that of the
transient phase (the slope of the a-b relation). The slope of the
relation between the maximal force and
[Ca2+]i responses
(a-c) was intermediate.
Source of Ca2+
Induced by U46619 Stimulation
To elucidate the source of the
[Ca2+]i increase
for U46619-induced responses, we used a pharmacological approach
inhibiting the sarcoplasmic reticulum
Ca2+-ATPase with cyclopiazonic
acid (CPA) and the plasmalemmal L-type
Ca2+ channels with nifedipine
(Figure 2). CPA (10 µmol/L) induced transient increases in
[Ca2+]i and force.
The peak levels were 371.0±44.1 nmol/L and 3.72±0.74
mN/mm2, respectively (n=5). These transients
returned to baseline within 10 minutes. In the continued presence of
CPA, the [Ca2+]i
transient to U46619 was significantly inhibited to 36.4±1.8% of
control (n=5). The force transient was also slightly but not
significantly reduced (15.1±1.8% to 6.4±5.9%, n=5). The responses
in the sustained phase were not significantly inhibited; >75% of
control responses remained in the presence of CPA.
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Figure 2. Characterization of the Ca2+ sources in U46619-induced responses: effects of CPA (A) or nifedipine (B) on the U46619-induced [Ca2+]i and force responses. Coronary arteries were preincubated in the presence or absence of the sarcoplasmic reticulum Ca2+-ATPase inhibitor (10 µmol/L CPA) (A) or a Ca2+ channel blocker (10 µmol/L nifedipine) (B) for 10 minutes, and then 100 nmol/L U46619 was added. [Ca2+]i (darkly hatched bars) and isometric force (lightly hatched bars) were measured simultaneously as described in Materials and Methods. Values are expressed in terms of the maximal [Ca2+]i response, which occurred in the transient phases (Trans), and in terms of the maximal force, which occurred in the sustained phases (Sust). Maximal responses for CPA or nifedipine alone are designated (Max). Data, as a percentage of each maximal response, are given as mean±SEM (n 5). *P<0.05 vs U46619 responses.
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In contrast
(Figure 2B), preincubation with nifedipine (10
µmol/L) for 10 minutes reduced the sustained force (53.1±6.3% of
control, n=6). Nifedipine caused a small decrease in the
transient [Ca2+]i
(100% to 91.1%, P<0.02). The
sustained [Ca2+]i
was substantially reduced (19.6% to 5.6%), but the precision at these
low levels of
[Ca2+]i was such
that statistical significance was not achieved
(P=0.12). Our results are
consistent with the classic picture for smooth muscle in which
intracellular Ca2+ stores underlie the
transient responses and in which transmembrane
Ca2+ influx underlies the sustained
component of force.
PKC and U46619 Responses
Activation of PKC is associated with
receptor-mediated stimulation in many cell types mediated by
diacylglycerol formation. We investigated the role of PKC in
U46619-induced responses by using the PKC inhibitor
calphostin C.
Figure 3 shows typical
[Ca2+]i and force
responses
(Figure 3A) and summarized data
(Figure 3B). Calphostin C (1 µmol/L) had no effects on
either resting
[Ca2+]i or force.
Neither the [Ca2+]i
transient (1089.0±21.3 nmol/L, n=6) nor the sustained levels
(216.8±56.2 nmol/L, n=6) in response to U46619 (100 nmol/L) were
altered by calphostin C. In contrast, force development differed from
control. The response was biphasic with a small peak (2.39±0.17
mN/mm2, n=6) shortly after stimulation in
most cases. This initial peak in force coincided with the
[Ca2+]i peak. After
the small peak, force again increased to a sustained maximal level
(14.95±0.18 mN/mm2, n=6). This maximal
level was not different from control, but the half-time for force
development was significantly greater than control (97.8±3.2 versus
39.2±7.3 seconds, respectively; n=4). Calphostin C also prolonged the
relaxation from the peak
[Ca2+]i; the
half-time was increased to 61.8 seconds compared with a control value
of 25.8 seconds. Calphostin C affected the relation between force and
[Ca2+]i during the
transient phase (a-b), but the relations in both the sustained phase
(c-d relation) and maximal responses (a-c relation) were unaffected
(Figure 3C).
To further investigate the role of PKC, we used the PKC
activator PMA. PMA (3 µmol/L) induced a transient
increase in isometric force
(Figure 4). The maximal value (10.56±0.95
mN/mm2, n=8) was detected within 2 minutes.
After attaining the peak, force slowly decreased.
[Ca2+]i was not
significantly changed from baseline, averaging <1.5% of the U46619
response. Based on standard ANOVA for n=8, changes in
[Ca2+]i of 5.0
nmol/L, or 0.6% of the U46619 peak, would be detectable. In control
experiments, after a similar preincubation with calphostin C, the
responses to PMA were measured. As shown in
Figure 4B, the isometric force responses were blocked by
calphostin C, with no change in
[Ca2+]i.
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Figure 4. PMA-induced changes in [Ca2+]i and isometric force in coronary arteries. A, Typical responses of [Ca2+]i (•), calculated as described in Materials and Methods, and force () to 100 nmol/L U46619 or 3 µmol/L PMA. B, Average (n=5) values for [Ca2+]i (darkly hatched bars) and force (lightly hatched bars) after treatment with 100 nmol/L U46619, 3 µmol/L PMA, or 1 µmol/L calphostin C, with subsequent addition of 3 µmol/L PMA from experiments as shown in panel A. Values are expressed in terms of the maximal [Ca2+]i and force responses.
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Rho-Kinase and U46619 Responses
We investigated the role of Rho-kinase by using the
inhibitor Y27632. Y27632 (1 µmol/L) decreased the force
baseline; typical responses are shown in
Figure 5A, and the summarized data are in the inset. After
10 minutes, the resting force decreased from 4.41±0.65 to 0.47±0.14
mN/mm2 (n=5). No effects on
[Ca2+]i were
observed.
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Figure 5. Effects of Y27632 on U46619-induced [Ca2+]i and isometric force responses in porcine coronary artery. Arteries were preincubated in the presence or absence of the Rho-kinase inhibitor (10 µmol/L Y27632) for 10 minutes, and then U46619 was added. A, Typical responses of [Ca2+]i (•) and force (). Inset, Averaged data (mean±SEM, n=5) for [Ca2+]i (darkly hatched bars) and force (lightly hatched bars). Values are expressed in terms of the maximal [Ca2+]i or force responses. Maximal responses to Y27632 alone are indicated (Max). Sus indicates sustained; Trns, transient. *P<0.05 and #P<0.05 vs U46619 responses and nontreated resting levels, respectively. B, U46619 (1 to 300 nmol/L) response data plotted as force vs [Ca2+]i relations in the presence (closed symbols, solid lines) or absence (open symbols, broken lines) of 10 µmol/L Y27632 (Y). The transient (a-b), maximum (a-c), and sustained (c-d) relations are as defined in Figure 1. C, Expansion of panel B to highlight relations at low [Ca2+]i levels. Data showing the effects of 10 µmol/L Y27632 at high concentrations of U46619 (1 and 3 µmol/L) are also plotted.
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Rho-kinase inhibition nearly abolished the contraction.
U46619 (100 nmol/L) elicited only small transient (15.6%) and
sustained (12.6%) increases in force in the presence of Y27632
(Figure 5A, inset).
[Ca2+]i increased
transiently, but the maximal level (771.5±31.3 nmol/L, n=5) was
decreased compared with control (1169.7±16.8 nmol/L, n=5). The
sustained phase of the
[Ca2+]i increase
was not different from control. Y27632 did not have a major effect on
the relation between force and
[Ca2+]i for the
transients (a-b), but the sustained phase (c-d) and maximal responses
(a-c relation) were markedly depressed, largely reflecting the
inhibition of force
(Figure 5B). This can be better seen in the expanded axes
(Figure 5C). To further delineate the effects of Y27632 on
force and [Ca2+]i,
we added data points at high concentrations of U46619 (1 to 3
µmol/L). These concentrations induce larger
[Ca2+]i increases,
but high doses are difficult to reverse on washout. The sustained
phases of the contraction in response to 1 µmol/L and 3 µmol/L
U46619 were inhibited by 10 µmol/L Y27632, and these points fitted
well within the c-d relation, derived from lower concentrations (1 to
300 nmol/L). Our major point is that Y27632 inhibits the steady-state
force with little change in
[Ca2+]i.
We also investigated the phosphatase inhibitor
calyculin A. Calyculin A (1 µmol/L) increased force with no change in
[Ca2+]i (data not
shown). This force developed slowly, and the maximal value was detected
within 2.5 minutes after treatment (7.91±0.98
mN/mm2, n=5). Over 90% of the maximal
response was maintained after 10 minutes of the
stimulation.
KCl-Induced
[Ca2+]i and
Isometric Force
To compare with receptor-mediated activation,
activation by depolarization with KCl, attributed to
Ca2+ influx through L-type
Ca2+ channels, was also investigated. KCl
(80 mmol/L) quickly increased both
[Ca2+]i and force
(Figure 6A). Maximal
[Ca2+]i values
(1129.4±15.0 nmol/L, n=7) were detected within 1 minute. After a peak
was attained,
[Ca2+]i slightly
decreased but was still maintained at >75% of the maximum after 5
minutes. Similarly, the maximal increase in force was detected within 2
minutes (15.04±0.27 mN/mm2, n=7), and
>90% of the maximal response was maintained at 5 minutes. At the peak
[Ca2+]i, the
corresponding force was 82.2±4.6% of the maximal force (12.97±0.61
mN/mm2, n=7). Moreover, when force attained
its maximum,
[Ca2+]i was
88.6±3.1% (1018.4±34.2 nmol/L, n=7) of its peak value. The maximal
responses of
[Ca2+]i and force
were a function of the KCl concentration
(Figure 6B). Significant increases were detected at 30
mmol/L KCl, and the maximal responses were attained at 80 mmol/L.
EC50 values of
[Ca2+]i and force
were 31.7 and 39.7 mmol/L, respectively. The relations between
force and [Ca2+]i
were analyzed
(Figure 7C) by using the 4 parameters previously
described for U46619 contractions in
Figure 1A. They showed strong correlations between force and
[Ca2+]i; for a-b,
c-d, and a-c relations,
r2
values were 0.992, 0.997, and 0.986, respectively. Moreover, there were
no differences in the relations among these
phases.
Effects of PKC and Rho-Kinase
Inhibitors on KCl-Induced Responses
Pretreatment with calphostin C (1 µmol/L) for 10
minutes did not affect either resting or KCl-induced
[Ca2+]i and force
responses
(Figure 6C). Similarly, little effects of the Rho-kinase
inhibitor Y27632 were observed. Baseline values were
slightly decreased, and the KCl-induced increases of
[Ca2+]i and force
were not affected;
[Ca2+]i versus
isometric force relations were unchanged
(Figure 6D).
Figure 7 shows a graphic comparison of the effects of PKC or
Rho-kinase inhibition on the relations between force and
[Ca2+]i for U46619
(Figure 7A) and KCl stimulation
(Figure 7B) in the sustained phase (c-d). Inhibition of
Rho-kinase can be seen as the major player for receptor-mediated but
not for KCl stimulation.
Discussion
U46619 increases coronary artery
[Ca2+]i and force
(Figure 1A) largely via activation of
TXA2 receptors, inasmuch as its effects were
blocked by the antagonist SQ29548
(Figure 1B). In general, the Ca2+
sensitization–associated U46619 is often greater than other agonists
in other vascular tissues. Our results indicate that the responses to
U46619 involve both PKC-mediated and Rho-kinase–mediated changes in
Ca2+ sensitivity. However, their effects,
based on the time courses over which the sensitization was effective,
were quite distinct. PKC inhibition had a much greater effect on the
initial phase of contraction. Its major effects were to diminish the
size of the initial transient and to prolong the duration of force
development and the decline in
[Ca2+]i. However,
there were limited effects on the magnitude of the sustained force.
Rho-kinase inhibition on the other hand, nearly abolished the sustained
force but had a lesser effect on the transient phase. Although
Ca2+ sensitization due to activation of the
Rho-kinase pathway has been implicated by use of
permeabilized
preparations14 or
contractility
measurements,18 it is
possible that Rho-kinase inhibition also modifies
[Ca2+]i. Our data
provide the first evidence that Rho-kinase indeed changes
Ca2+ sensitivity in vivo in the intact
coronary artery.
These phases differed not only in their sensitivity to
kinase inhibitors but also in their source of
Ca2+ for the increase in
[Ca2+]i. Because
the transient increase in
[Ca2+]i to U46619
was reduced by CPA to <40% of control, it appears that
Ca2+ was provided largely by the
sarcoplasmic reticulum stores
(Figure 2A). The sustained phases of the
[Ca2+]i increase
and isometric force were reduced by the Ca2+
channel inhibitor nifedipine
(Figure 2B) or Ca2+-free PSS (data
not shown), indicating a dependence of the sustained phase on
extracellular Ca2+ influx. These results
suggested the possibility of different isometric force versus
[Ca2+]i relations
in each phase of the U46619 stimulation.
In fact, whether
[Ca2+]i is elevated
in the steady state has important ramifications. In 
10% of
responses, [Ca2+]i
appeared to return to baseline. But in the majority of cases,
[Ca2+]i remained
elevated. We analyzed the 17 controls for the experiments shown
in
Figures 2A, 2B, and 3C. When expressed as a percentage of
baseline, [Ca2+]i
in the sustained phase averaged 242.8±38.8%. When expressed as a
percentage of the maximum
[Ca2+]i response to
100 nmol/L U46619, the increase above baseline was 12.6±3.4%. Both
were highly statistically significant. A total of 40 control U46619
responses yielded a sustained
[Ca2+]i of
202.5±22.2% of baseline and 10.2±2.3% of maximal response. Thus, an
elevated [Ca2+]i is
associated with the sustained force.
Receptor-mediated activation is associated with the
production of inositol triphosphate from phosphatidylinositol
biphosphate and with the hydrolysis of phosphatidylinositol biphosphate
by phospholipase C, with the important second messenger diacylglycerol.
Inhibition of PKC by calphostin C pretreatment caused a significant
delay in the force response to U46619
(Figure 3). Because the
[Ca2+]i transient
was largely unaffected, the suppression of force development suggests
the loss of a PKC-mediated Ca2+
sensitization. Because the maximal force and increase in
[Ca2+]i were not
affected in the steady state, either force is saturated or calphostin C
inhibition is effective only in the transient phase. The decrease in
the slope of the
force-[Ca2+]i
relation in the presence of calphostin C
(Figure 3C) suggests that the latter may be the case. This is
further supported by evidence from the experiments in which PKC was
directly activated by PMA. A transient increase in isometric
force was observed without a statistically significant increase in
[Ca2+]i
(Figure 4). We cannot rule out changes in
[Ca2+]i of <10%,
but our point is that with or without a small change in
[Ca2+]i, the
increase in force in response to PMA is characterized by a very high
Ca2+ sensitivity.
The sustained phase of the U46619-induced contraction was
significantly reduced by nifedipine
(Figure 2B). Similarly, pretreatment with 5 mmol/L EGTA
and Ca2+-free PSS reduced the maintained
force to <20% of control (data not shown). Thus, extracellular
Ca2+ and transmembrane influx are necessary
for the maintenance of force. The relation between isometric
force and [Ca2+]i
indicates a much higher Ca2+ sensitivity
than in the transient phase of the U46619 response. Because our data
suggested that PKC sensitization was not likely a major player in the
sustained phase, we investigated the potential role of Rho-kinase,
postulated to be involved in Ca2+
sensitization.11
The Rho-kinase inhibitor Y27632 was an
impressive inhibitor of contractility,
nearly completely suppressing the sustained phase of contraction. It
also partially reduced the resting levels and the U46619-induced
transient phases of both force and
[Ca2+]i. The
mechanism for the reduction of the transient increase in
[Ca2+]i is not
known. However, the sustained phase of the increase in
[Ca2+]i was not
statistically different from that of the control. These effects of
Y27632 are consistent with the loss of Rho-kinase–mediated
Ca2+ sensitivity. Calyculin A, an
inhibitor of myosin light chain phosphatase, also induces
an increase in force with minimal changes in
[Ca2+]i, similar to
that previously reported for okadaic
acid.20 That phosphatase
inhibition can lead to an increase in force without increasing
[Ca2+]i supports a
mechanism consistent with the hypothesis of Rho-kinase
modulation of phosphatase activity and, consequently,
contractility.
Our hypothesis for two different pathways modulating
Ca2+ sensitivity is specific to
receptor-mediated activation, inasmuch as it requires G-protein
activation of Rho-kinase and diacylglycerol activation of PKC.
Moreover, our demonstration of their presence is dependent on a
pharmacological approach and limitations of the specificity of agents.
To confirm that these sensitization mechanisms are specifically coupled
to receptor-mediated stimulation and to control for specificity, we
performed similar measurements on KCl-induced responses.
For KCl contractures, the relations between isometric force
and [Ca2+]i did not
differ between transient and sustained phases
(Figure 6). Importantly, the increases in
[Ca2+]i and force
were not inhibited either by calphostin C or Y27632, nor were any
changes in Ca2+ sensitivity observed
(Figure 6). The Ca2+ sensitivity
measured for KCl contractures is also of interest compared with that
observed for the different phases in receptor-mediated contractions.
The Ca2+ sensitivity for the sustained phase
for U46619 was 10-fold greater than that observed for the responses
to KCl. On the other hand, that of the transient PKC-modulated phase
was 5-fold less. This largely reflects the much more rapid increase in
[Ca2+]i than in
force. Some caution must be exerted in interpreting the slope of force
versus Ca2+ in the transient phase as a
Ca2+ sensitivity that can be readily
compared with that in the steady state. Force development lags that of
actomyosin activation because of the presence of any series elasticity.
In smooth muscle, the series elastic component and slow contraction
velocities can exacerbate the differences between the measured force
and the level of activation of the smooth muscle. The latter is what is
generally inferred from isometric force measurements in terms of
Ca2+ sensitivity. However, this inference is
valid in the steady state. Another potential caveat to interpretation
of transient data are that although isometric force represents
a tissue average,
[Ca2+]i is
dependent on the depth of light penetration and reflected for the
fluorometric measurements. Our simultaneous measurements of
force and [Ca2+]i
for the KCl measurements set limits on these potential artifacts. The
Ca2+ sensitivity of the steady state was
<22% greater than that of the transient phase.
Independent of the exact meaning of
Ca2+ sensitivity in transient phases, the
important point is that the effects of PKC inhibition were prominent
only during this initial transient. The transient phase is effective
over the first 30 seconds, so there may be sufficient time for its
effects on force to be of physiological relevance.
Force is not necessarily the only outcome of activation of the PKC
pathway; eg, contractile speed may also be affected. Although the
physiological significance of the PKC sensitization
is not clear, our data show unambiguously that it is present in
porcine coronary artery.
In conclusion, our data show that
Ca2+ sensitivity of smooth muscle
demonstrated in permeabilized
fibers11 is a major factor
in receptor-mediated responses to U46619 in vivo. Moreover, two
distinct types of Ca2+ sensitization were
observed. The transient phase of contraction to U46619 was associated
with Ca2+ release from the sarcoplasmic
reticulum and PKC-mediated Ca2+
sensitization. In the sustained phase, Ca2+
influx from extracellular space is central and involves
Rho-kinase–mediated Ca2+ sensitization.
Although both pathways have been postulated to play a role in
coronary
vasospasm,17 18
our data indicate that Rho-kinase is the dominant factor in
thromboxane receptor–mediated
contraction.
Acknowledgments
This study was supported in part by
National Institutes of Health Grants HL-54829 and HL-61974. We
appreciate the generous gift of the Rho-kinase inhibitor
Y27632 from the Welfide
Corporation.
Footnotes
Original received January 16, 2001; revision received April 24, 2001; accepted April 24, 2001.
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