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1 Cardiac Muscle Research Laboratory, Boston University School of Medicine, Boston, Massachusetts 02118; 2 Kardiologie, Universitatsklinik, Inselspital, 3010 Bern, Switzerland; and 3 NMR Laboratory for Physiological Chemistry, Cardiovascular Division, Department of Medicine, Brigham and Women's Hospital and Harvard Medical School, Boston, Massachusetts 02115
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIAL AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Decreasing coronary perfusion causes an
immediate decrease in contractile function via unknown mechanisms. It
has long been suspected that this contractile dysfunction is caused by
ischemia-induced changes in cardiac energetics. Our goal was to
determine whether changes in cardiac energetics necessarily precede the
contractile dysfunction as one would expect if a causal relationship
exists. In 14 isolated rat hearts, we gradually decreased coronary
perfusion using a coronary perfusate with a normal hematocrit and
normal concentrations of the major metabolic substrates. Using
31P NMR spectroscopy to measure
ATP, phosphocreatine (PCr), Pi, and ADP concentrations
([ATP], [PCr],
[Pi],
[ADP]), pH, and amount of free energy released from ATP
hydrolysis
(|
GATP|),
we found that none of these variables changed significantly until
several minutes after systolic pressure had significantly decreased.
Even when developed pressure had decreased by over one-third, only very
slight changes in
[Pi], pH, and
|GATP|
had occurred, with no significant changes in [ATP],
[PCr], or [ADP]. Additionally, the rate of
high-energy phosphate transfer between ATP and PCr did not decrease
enough during hypoperfusion to explain the contractile dysfunction. We
conclude that nonenergetic factors are the dominant cause of the
initial decrease in systolic function when myocardial perfusion is decreased.
hibernation; ischemia; perfusion-contraction matching; metabolism
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
MATERIAL AND METHODS
RESULTS
DISCUSSION
REFERENCES
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A DECREASE in myocardial perfusion causes an immediate decrease in left ventricular pressure generation. This decreased contractile work in response to hypoperfusion has complex clinical ramifications because it has the detrimental effect of decreasing left ventricular function but the beneficial effect of protecting the hypoperfused myocardium by decreasing its oxygen requirement (22, 30). The mechanisms that cause and subsequently maintain decreased systolic function when myocardial perfusion is decreased are poorly understood. One long-standing hypothesis is that coronary hypoperfusion causes a change in the energetic state of the heart, which subsequently inhibits systolic pressure generation (8, 16, 24). Specifically, it has been suggested that decreased systolic function is caused by depletion of high-energy phosphates [ATP and phosphocreatine (PCr)] and/or accumulation of metabolic by-products such as H+, ADP, and Pi (8, 13, 14, 24, 25, 29, 31). Evidence that supports this hypothesis comes largely from studies in which a severe degree of myocardial hypoperfusion was induced in a few seconds in buffer/crystalloid-perfused isolated hearts. These studies have arrived at a variety of conclusions, including that the decreased systolic function during hypoperfusion is caused by 1) a decrease in phosphorylation potential ([ATP]/[ADP] × [Pi ], where brackets indicate concentration) (6), 2) an increase in [Pi] (13), 3) an increase in both [Pi] and [H+] (8), and 4) something other than cardiac energetics (23).
A rapid decrease in oxygen delivery to the heart causes obligatory changes in cardiac energetics that are a function of both the rapidity and severity of the decrease in oxygen delivery. Arai et al. (1) demonstrated that a rapid decrease in coronary perfusion causes a much larger change in cardiac energetics than does gradually lowering flow to the same level. Therefore, studies in which myocardial perfusion is decreased to a low level in a few seconds, particularly those that use a buffer/crystalloid perfusate that has a low oxygen content, maximize both the speed and magnitude of the resulting energetic derangement and may observe temporal relationships between changes in cardiac function and energetics during the early minutes of myocardial hypoperfusion that are unrelated to causality.
The goal of our study was to determine during myocardial hypoperfusion whether changes in cardiac energetics necessarily precede the contractile dysfunction as one would expect if they cause it. Our approach was to decrease myocardial perfusion and oxygen delivery gradually to minimize energetic derangement. This was accomplished not only by decreasing myocardial perfusion slowly but also (in contrast to most prior studies in isolated hearts) using a coronary perfusate with a normal hematocrit, oxygen content, and normal concentrations of the major metabolic substrates of glucose, lactate, and long-chain fatty acids. 31P NMR spectroscopy was used to measure [ATP], [PCr], [Pi], [ADP], and intracellular pH as coronary perfusion was decreased in these isolated rat hearts.
Recently, other variables related to the energy status of the heart
have been suggested as the cause of hypoperfusion-induced contractile
failure. For example, it has been suggested that rapid "shuttling" of high-energy phosphates is necessary to maintain normal contractile function and that a decreased rate may be the cause
of systolic dysfunction during myocardial hypoperfusion (4, 19, 31).
Likewise, it has been suggested that the decreased systolic function
during hypoperfusion might be caused by a decrease in the amount of
free energy released from ATP hydrolysis
(|GATP|), which is a function of [ATP], [ADP], and
[Pi] (17, 27).
Therefore, in addition to measuring [ATP],
[PCr],
[Pi],
[ADP], and intracellular pH, we also calculated
|GATP|
and measured creatine kinase flux rate
(CKflux) using the magnetization
transfer technique.
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MATERIAL AND METHODS |
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TOP
ABSTRACT
INTRODUCTION
MATERIAL AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Experimental preparation. The isolated isovolumic rat heart preparation, perfused with a red blood cell-containing perfusate at a 40% hematocrit, was used. This methodology has previously been described in detail elsewhere (7). Male Sprague-Dawley rats (n = 14) weighing 400-450 g were deeply anesthetized with 80 mg/kg ip pentobarbital sodium. Hearts were rapidly excised and cannulated by the aorta on a constant-flow perfusion apparatus. Flow was adjusted so that coronary perfusion pressure (CPP) was ~95 mmHg. After equilibration, flow was held constant and CPP was determined by coronary vasomotor tone. A small portion of the left atrium was removed so that a polyethylene (PE-160) drain could be inserted and advanced through the apex of the left ventricle to allow drainage of the Thebesian veins. To measure isovolumic left ventricular pressure, a fluid-filled latex balloon attached to a Statham P23 Db pressure transducer (Gould, Oxnard, CA) was inserted through the mitral valve into the left ventricle. The balloon was filled until a left ventricular end-diastolic pressure (EDP) of ~10 mmHg was achieved, and the balloon volume was then held constant. To pace the heart, salt bridge pacing wires consisting of PE-160 tubing filled with 2% agarose and 4 M KCl and tipped with 4 cm of nonmagnetic wire were positioned to make contact with the heart. Hearts were paced at a rate of 5.8 Hz (350 beats/min). Hearts were then inserted in a 20-mm-diameter glass NMR tube that was inserted into an Oxford Instrument 9.4-tesla magnet connected to a General Electric GN400 spectrometer. CPP was monitored via a sidearm of the aortic cannula connected to a Gould-Statham P23 Db pressure transducer. The perfusate level in the NMR tube was maintained by aspiration just above the left atrium by continuous suction through a polyethylene tube. CPP and isovolumic left ventricular pressure were continuously measured using a commercially available data acquisition system (MacLab). All data were sampled at 200 Hz and stored on a hard disk for analysis.
Perfusion solution. The perfusion solution consisted of packed bovine red blood cells resuspended in a phosphate-free modified Krebs-Henseleit solution at a hematocrit of 40%. The packed red cells were processed as previously described (7). The red cell suspension was essentially white blood cell and platelet free. Packed red blood cells were stored in nominally calcium-free buffer at 4°C and washed daily before use. The modified phosphate-free Krebs-Henseleit buffer contained (in mM) 118 NaCl, 4.7 KCl, 2.0 CaCl2, 1.2 MgSO4, 25.5 NaHCO3, 5.5 glucose, 1.0 lactate, 0.5 NaEDTA, 15 µU/ml insulin, and 0.4 palmitic acid in combination with 4 g% bovine serum albumin (no. A7030; Sigma Chemical, St. Louis, MO). Essentially free fatty acid-free bovine serum albumin was first dissolved in Krebs-Henseleit buffer. Palmitic acid (no. P9767, Sigma Chemical) was then added to this mixture. Gentamicin (0.2 mg/dl) was added to the red blood cell perfusate to retard bacterial growth. The perfusate was equilibrated with 20% O2-3% CO2-balance N2 to achieve a PO2 of ~140 mmHg and a pH of 7.4.
To make the red cell perfusate feasible for 31P NMR spectroscopy, KH2PO4 was not included in the Krebs-Henseleit buffer. This was done to avoid contamination of phosphorus spectra with signal from outside of the heart. Furthermore, to reduce the 2,3-diphosphoglycerate signal from the red blood cells in the NMR-sensitive volume, a solution of mannitol (0.2 M) was superfused around the heart at twice the coronary flow rate to provide rapid removal of venous effluent. These measures effectively reduced the contamination of the 31P NMR spectra by noncardiac phosphate and also markedly reduced the 2,3-diphosphoglycerate signal, thus permitting 31P NMR study of the red blood cell-perfused heart.
NMR spectroscopy. Myocardial energetics were studied using 31P NMR spectroscopy. Briefly, spectra were collected with the resonance frequency for 31P of 161.94 MHz in a GE-400, 9.4-tesla spectrometer using a pulse width of 27 µs to give a 60° flip angle. Using an interpulse delay of 2.14 s, we collected 104 scans in each 4-min period. Individual free induction decays were zero filled and weighted with a 20-Hz line-broadening decaying exponential before Fourier transformation.
Magnetization transfer was used to measure the pseudo-first-order rate
constant (kfor)
for the forward CK reaction (PCr + MgADP + H+ 
MgATP + creatine).
Magnetization transfer was performed by applying a low-power
radiofrequency pulse centered at the 
-phosphate of ATP for either
0.0 s (M0) or 4.8 s
(M
). The
kfor for this
reaction was calculated as
kfor = (M0 
M)/(T1 × M), with T1 set to 3.5 s
(10). Flux through the CK reaction (rate of ATP synthesis from PCr) was
calculated as
kfor × [PCr]. We measured
kfor at baseline
and after 30 min of hypoperfusion. The two-point
(M0,
M) method for measuring
kfor was used
because it allowed us to complete a measurement of
kfor in 15 min.
Protocol. Hearts
(n = 14) were initially perfused at a
CPP of 90-100 mmHg for a 28-min baseline period. After this
baseline period, CPP was decreased at a rate of ~30% per minute for
3 min by decreasing coronary flow. Coronary flow was decreased by a total of 69-70% in each heart. This level of hypoperfusion was chosen because pilot data indicated that it caused a decrease in
developed pressure (systolic diastolic pressure) of ~50%. Physiological data were collected at 2-min intervals throughout the
protocol except during the early minutes of hypoperfusion, when they
were recorded at 1-min intervals. Cardiac energetics were assessed
using two types of 31P NMR
spectroscopy. Concentrations of ATP, PCr,
Pi, and
H+ were determined with one-pulse
spectra, and CKflux was measured using magnetization transfer. One magnetization transfer measurement was obtained during the baseline period, and the second was obtained after 30 min of myocardial hypoperfusion. A pair of one-pulse spectra
was collected just before and after each measurement of CKflux. One-pulse spectra were
sequentially collected for determination of cardiac energetics at the
onset of myocardial hypoperfusion. For the one-pulse spectra, the
baseline spectra is plotted at time 0 and all other spectra
are plotted at the midpoint of their 4-min collection time (2, 6, and
10 min after the start of hypoperfusion). After 30 min of
hypoperfusion, when cardiac energetics and contractile function were
relatively stable, CKflux was
again measured.
Data analysis and statistics. The area
under the Pi, PCr, and
-phosphate of ATP peaks of each
31P spectrum was measured using
commercially available software (NMR1). From fully relaxed spectra
(interpulse delay of 10 s), it was determined that the area under the
Pi and PCr peaks needed to be
corrected for partial saturation by being multiplied by 1.15 and 1.2, respectively. Area units were converted to intracellular concentrations
by assuming that the ATP concentration in each heart during the control
period was 10.8 mM (2). Setting the area under the -phosphate peak
of ATP during the control period of each heart equal to 10.8 mM
provided a conversion factor used to convert the PCr and
Pi area units into concentrations.
Intracellular pH was measured by comparing the chemical shift between
Pi and PCr resonances to a
standard curve.
ADP was calculated from the CK equilibrium equation using
Keq = [ATP][free
creatine]/[ADP][PCr][H+],
where Keq was set
equal to 1.66 × 109 at pH 7 (26, 34). A total creatine concentration of 33 mM was used in all
calculations.
|GATP|
was calculated from the equation
|GATP| = |G° RTln[ATP]/[ADP][Pi]|,
where G° (30.5 kJ/mol)
is the value of ATP hydrolysis under standard conditions of molarity,
temperature, pH, and
[Mg2+];
R is the gas constant (8.314 J · mol
1 · °K1);
and T is temperature in Kelvin (20).
Values for physiological data and energetics are expressed as means ± SE. Data were analyzed statistically using ANOVA with repeated measures and a Fisher post hoc test. Differences were considered statistically significant at P < 0.05.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
MATERIAL AND METHODS
RESULTS
DISCUSSION
REFERENCES
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During the baseline period there were no significant changes in any
measure of cardiac energetics or contractile function, as shown in
Table 1, where values at the start and end
of the baseline magnetization transfer were not different.
After the 28-min baseline period, CPP was gradually lowered from 95 ± 2 mmHg at baseline to 63 ± 2 mmHg after 1 min (34% decrease) to 43 ± 2 mmHg after 2 min (27% decrease) to 34 ± 1 mmHg after 3 min
(26% decrease) (Fig. 1). Coronary flow was
2.43 ± 0.25 ml/min at baseline and 0.72 ± 0.07 ml/min after 10 min
of hypoperfusion. The lowering of CPP caused systolic pressure to
decrease from its baseline value of 80 ± 3 mmHg to 72 ± 3 mmHg
after 1 min, 67 ± 2 mmHg after 2 min, and 59 ± 3 mmHg after 3 min
(each significantly less than baseline). During this time, heart rate
was maintained constant at 350 beats/min with epicardial pacing and EDP
did not change from its baseline value of 8 ± 1 mmHg.
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Figure 2 is a representative example of
contractile function and 31P
spectra measured at baseline and after 10 min of hypoperfusion. In this
example, the heart responded to hypoperfusion by decreasing left
ventricular systolic pressure from 96 mmHg at baseline to 52 mmHg. This
reduction in systolic pressure was accompanied by only small changes in
cardiac energetics, because [ATP] was 10.7 mM at both time
points, [PCr] decreased from 24.5 to 21.8 mM, [Pi] increased from
7.0 to 9.5 mM, and pH decreased from 7.23 to 7.16. This example
highlights the fact that large hypoperfusion-induced decreases in
systolic pressure occur in the presence of very small changes in
cardiac energetics.
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Effect of hypoperfusion on cardiac
energetics. The effect of gradually lowering CPP on
cardiac energetics is shown in Figs. 3 and
4. During the first 2 min of hypoperfusion,
when systolic pressure fell significantly, there were no changes in
[ATP], [PCr], [Pi],
[ADP],
|GATP|,
or pH.
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After 6 min of hypoperfusion, [ATP], [PCr],
[ADP], and
|GATP|
had not changed significantly from baseline (Figs. 3 and 4). In
contrast, [Pi]
increased from 6.1 ± 0.8 to 8.6 ± 0.4 mM, and pH decreased from
7.15 ± 0.01 to 7.09 ± 0.02 (each P < 0.05). After 10 min of hypoperfusion, [ATP] and
[ADP] were still not significantly different from baseline
but [PCr],
[Pi], pH, and |GATP|
were each significantly different from their baseline values. The total
amount of NMR-observable phosphate ([ATP] × 3 + [PCr] + [Pi]) did not
significantly change during myocardial hypoperfusion (61.5 ± 0.8 mM
at baseline, 62.2 ± 1.2 mM after 2 min, 64.7 ± 1.7 mM after 6 min,
and 63.2 ± 1.7 mM after 10 min of hypoperfusion).
To further examine the relationship between
[Pi] and systolic
function during hypoperfusion, we plotted these two variables at each
time point (baseline, 2, 6, and 10 min after the start of
hypoperfusion) for each of the 14 hearts (Fig.
5). There was not a significant correlation
between systolic pressure and
[Pi]. When data from
all hearts were averaged at each of the four time points, however,
there was a strong linear correlation between systolic pressure and
[Pi] (Fig. 5,
inset). This suggests that the
length of time of hypoperfusion is a key determinant of both the fall
in systolic pressure and increase in
[Pi]. If
[Pi] was an important
determinant of systolic function during the early minutes of
hypoperfusion, hearts with the largest increases in [Pi] would be expected
to have the largest decreases in systolic pressure. This was not the
case, because no correlation existed between the change in
[Pi] and the change in
systolic pressure during the first 2 min of hypoperfusion (Fig.
6).
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CKflux. The rate
of high-energy phosphate transfer between ATP and PCr
(CKflux) is determined by
measuring the rate of disappearance of the PCr resonance area when the
-ATP resonance is selectively saturated, as shown in Fig.
7. The difference in the PCr resonance areas between M0 and
M is proportional to
CKflux. In this example, we see
that during myocardial hypoperfusion [PCr] is somewhat
decreased but that the decrease in PCr resonance area during
M is very similar at baseline
and during hypoperfusion. In this example, systolic pressure decreased
from 96 mmHg at baseline to 50 mmHg during
M while
CKflux decreased from 8.8 to 7.0 mM/s. On average, there was a 27% decrease in
CKflux during myocardial
hypoperfusion (P < 0.05), an amount
that would not be expected to cause any significant change in systolic
function (11, 32) (Table 1).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
MATERIAL AND METHODS
RESULTS
DISCUSSION
REFERENCES
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The mechanisms that link myocardial perfusion level with contractile
state are of great clinical importance but are poorly understood.
Several studies have demonstrated that when myocardial perfusion is
rapidly decreased, changes in cardiac energetics can occur before the
decrease in systolic function (6, 13). This temporal relationship has
led investigators to suggest that the early changes in cardiac
energetics may be the cause of the decreased systolic function. To test
this, we determined whether the temporal relationships are obligatory
as one would expect them to be if they are causal. We found that when
myocardial perfusion was decreased gradually, significant changes in
cardiac energetics, including
|GATP|,
occurred only after systolic pressure had decreased. The rate of
high-energy phosphate transfer between ATP and PCr (CKflux) decreased only modestly
during hypoperfusion, making it unlikely to have caused the
hypoperfusion-induced systolic dysfunction. We conclude that
nonenergetic factors are the dominant cause of the initial decrease in
systolic function when myocardial perfusion is decreased slowly.
Relationship between systolic function and cardiac energetics during myocardial hypoperfusion. One approach to studying the mechanism by which myocardial hypoperfusion causes decreased systolic function has been to measure cardiac energetics using 31P NMR spectroscopy in isolated, buffer-perfused hearts as coronary perfusion is rapidly decreased, the goal being to determine what variable(s) change fast enough when perfusion is decreased to potentially explain the rapid decrease in systolic function. Although these studies use similar methodologies, they come to a variety of conclusions. Clarke et al. (6) concluded that phosphorylation potential ([ATP]/[ADP] × [Pi]) controls contractile function during myocardial hypoperfusion. Elliott et al. (8) concluded that changes in [Pi] and [H+] are the major determinants of contractile failure secondary to myocardial hypoperfusion. He et al. (13) measured cardiac energetics with unprecedented time resolution during repeated 33-s bouts of rapidly induced hypoperfusion in buffer-perfused rat hearts. They found that [Pi] increased significantly during the first second of hypoperfusion, before a change in systolic function, and concluded that [Pi] may play an important role in inhibiting contractile function during myocardial hypoperfusion. Our results were similar to those of He et al. (13) in many important respects, considering the differences in methodology such as the degree of hypoperfusion and its speed of induction (very rapid induction of zero-flow ischemia compared with gradual induction of low-flow ischemia) and the composition of the perfusate (buffer compared with reconstituted blood). Most notably, data at our 10-min time point were very similar to their 10-s time point because in both cases developed pressure was decreased by ~40-45%, [Pi] was increased ~3 mM, [PCr] was decreased 2-4 mM, and [ATP] was unchanged from baseline (13). Our different methodologies did, however, cause one critical difference in results. In the study of He et al. (13), the hypoperfusion-induced increase in [Pi] preceded the decrease in systolic function, whereas a significant increase in [Pi] did not occur until several minutes after the decrease in systolic function when our methodology, designed to minimize ischemia-induced energetic changes, was employed.
The fact that changes in cardiac energetics can occur before decreased systolic pressure is of interest, but from a mechanistic point of view the more important question is, must they? In our study, all of the variables related to cardiac energetics that we measured changed only after systolic pressure had significantly decreased. We interpret this to mean that temporal correlations between changes in cardiac function and energetics that may occur in some protocols do not describe an obligatory, i.e., causal, relationship. Our findings are similar to those of Koretsune et al. (23), who demonstrated in four buffer-perfused ferret hearts that the start of contractile failure secondary to zero-flow ischemia occurred 15 s before significant changes in any measure of cardiac energetics, including Pi. Koretsune et al. (23) proceeded to demonstrate that loss of coronary turgor, not cardiac energetics, was the main cause of the systolic dysfunction during the first minutes of rapidly induced ischemia. He et al. (13) also noted that CPP decreased more rapidly than systolic pressure and suggested that the loss of coronary vasculature turgor may play some role in the rapid decrease in systolic pressure when coronary flow is decreased. More recent work from this group, however, demonstrates that, during a rapid decrease in coronary flow, the timing of the decrease in CPP correlates poorly with the timing of the decrease in contractile function (12).
One likely reason for the differences in findings among investigators
who have measured cardiac energetics while rapidly decreasing myocardial perfusion is that the timing and size of the resulting changes in cardiac energetics are strongly influenced by the speed at
which coronary perfusion is decreased. Contractile function and ATP
consumption do not downregulate as fast as coronary flow and oxygen
supply can be experimentally decreased. To minimize any decrease in the
concentration of ATP, two metabolic pathways are activated. First, ATP
is synthesized from PCr and ADP via the CK reaction (PCr + ADP ATP + creatine). This reaction is closely coupled to ATP hydrolysis so
that the net reaction of the two coupled reactions is PCr
creatine + Pi.
Second, ATP synthesis via anaerobic glycolysis is increased, which
causes production of lactic acid and a fall in myocardial pH.
Therefore, the first observable changes in energetics when coronary
flow is decreased are decreased [PCr], a reciprocal
increase in [Pi], and
a fall in pH (13). The faster coronary flow is decreased, the greater
is the imbalance between ATP supply and demand and the resultant
changes in [PCr],
[Pi], and pH, as
demonstrated by Arai et al. (1), who found that rapidly decreasing
coronary flow causes larger changes in cardiac energetics compared with decreasing flow to the same level gradually.
To avoid issues of timing, several studies have examined the subacute steady-state relationship between cardiac energetics and systolic function during graded myocardial hypoperfusion (9, 33). These studies have reported that progressive decreases in myocardial perfusion cause both progressive decreases in systolic function and progressive changes in cardiac energetics. Schaefer et al. (33) found that, during graded myocardial hypoperfusion, the magnitude of the decrease in systolic function closely correlated with the magnitude of the decrease in the [PCr]-to-[Pi] ratio, increases in [Pi], and decreases in pH. They suggest that [Pi] and [H+] may play important roles in inhibiting systolic function during ischemia. Subsequent work from this group showed a strong linear correlation between increased [Pi] and decreased developed pressure during graded hypoperfusion (9).
Our data (where myocardial perfusion was decreased gradually) are very similar to these steady-state data of Figueredo et al. (9) in several important respects. First, at 2 min after myocardial hypoperfusion was initiated, and at their mildest level of hypoperfusion, contractile function is significantly decreased, whereas [Pi] is not different from baseline. We interpret this to indicate that contractile failure secondary to myocardial hypoperfusion can occur without a significant increase in [Pi]. Second, in their study, and in our study when data were grouped by time points (Fig. 5, inset), there is a strong linear correlation between [Pi] and systolic pressure. The slope of this relationship in both studies is such that an ~50% decrease in systolic pressure occurs coincident with an ~4 mM increase in [Pi]. Although a causal relationship might be inferred from this correlation, at least in our study, a plot of [Pi] and systolic pressure at each time point in each heart demonstrates that there is no relationship between these two variables (Fig. 5). Additionally, there was no correlation between the change in [Pi] during the first 2 min of hypoperfusion and the change in systolic pressure (Fig. 6). We therefore conclude that the correlation seen in Fig. 5, inset, is due not to a causal relationship but instead to the fact that [Pi] and systolic pressure are both functions of the degree of hypoperfusion and therefore correlate with each other.
Although the increase in [Pi] from 6.1 ± 0.8 mM at baseline to 7.2 ± 0.5 mM after 2 min of hypoperfusion was not statistically significant by repeated-measures ANOVA, the question remains as to whether it is biologically significant. In preparations where [Pi] can be independently manipulated, it is clear that elevating [Pi] can inhibit systolic tension development but that the degree of any inhibition is a function of the background concentrations of many molecules, including ATP and PCr (28). In the experiments that most closely model our metabolic conditions, Mekhfi and Ventura-Clapier (28) demonstrated in skinned ventricular muscle fibers that increasing [Pi] from 0 to 12 mM caused no inhibition of tension when the increase in [Pi] was accompanied by a reciprocal decrease in PCr and a constant [ATP]. In light of these data, it is unlikely that even the statistically significant 3.0 mM increase in [Pi] that we observed after 10 min of hypoperfusion would contribute to the concomitant 30-mmHg decrease in systolic pressure given that [ATP] was constant and there was a reciprocal decrease in [PCr] of 2.4 mM.
Effect of coronary hypoperfusion on
|GATP| and
CKflux. In recent reviews, Heusch
(15) and Heusch and Schulz (17) raised the possibility that
ischemia-induced downregulation of contractile function may be
caused not by decreases in [ATP] or [PCr], or by accumulation of ADP, Pi, or
H+, but by changes in other
measures of cardiac energetics such as
|GATP|
or an inadequate rate of ATP synthesis from PCr
(CKflux).
To address this, we calculated
|GATP|,
which is not constant but is determined in vivo by the concentrations
of ATP, ADP, and Pi (20). In our
study, the calculated values for
|GATP| did not significantly decrease until 6 min after hypoperfusion had
begun, at least 4 min after systolic pressure had significantly decreased. From this we conclude that the change in
|GATP|
is unlikely to have caused the systolic dysfunction. We cannot rule out
the possibility that small changes in
|GATP|
can cause a decrease in systolic pressure, but this is very unlikely
because Balschi et al. (3) demonstrated that, to impair baseline
cardiac function,
|GATP|
must be lowered well below 54 kJ/mol, and in our study
|GATP|
did not fall below 57 kJ/mol. Similarly, it has been estimated that the
|GATP|
required for the major ATPases in cardiac muscle (myosin-ATPase,
Ca2+-ATPase,
Na+-K+-ATPase)
are all <57 kJ/mol (20).
Another major aspect of cardiac energetics that has been suggested to link perfusion level with contractile state is the rate at which ATP is synthesized from PCr, also called CKflux. In the healthy, well-oxygenated heart, the rate of ATP synthesis from PCr is 5-10 times that of ATP synthesis from oxidative phosphorylation and glycolysis combined, indicating that each molecule of ATP synthesized via these pathways is chemically "shuttled" between ATP and PCr many times before it is hydrolyzed to ADP and Pi. The idea that decreased "shuttling rate" of high-energy phosphates would impair systolic function is conceptually similar to the idea that depressed CKflux during heart failure contributes to the contractile dysfunction (18). Likewise, Rauch et al. (31) conclude that disturbance of PCr shuttle might be of importance in early contractile failure. To directly test this possibility, we measured CKflux at baseline and after 30 min of myocardial hypoperfusion, a time when cardiac function and energetics were relatively stable. Hypoperfusion caused CKflux to decrease from 9.2 to 7.2 mM/s, a 27% decrease. This modest decrease in CKflux would not be expected to cause a significant inhibition of systolic function because acute inhibition of CK by >90% caused no change in left ventricular developed pressure (11). Similarly, a chronic decrease in CK activity to <5% of normal in mice did not cause impaired systolic function in isolated hearts (32). As Bittl and Ingwall (5) showed, CKflux varies with cardiac workload such that when workload is low, CKflux is decreased. Therefore, it is likely that the decrease in CKflux we observe during hypoperfusion is caused by the decreased myocardial oxygen consumption and cardiac work, as opposed to the decrease in CKflux causing the decrease in cardiac work.
Limitations. Several limitations of our study merit mention. First, because we were unable to completely prevent cardiac energetics from changing during hypoperfusion, we cannot definitively conclude that changes in cardiac energetics do not contribute to the systolic dysfunction. Instead, we demonstrated that significant decreases in systolic pressure can occur before significant changes in cardiac energetics, and we interpret this to mean that changes in cardiac energetics are not the dominant cause of the systolic dysfunction. We have no direct evidence of the mechanism responsible for the almost immediate decrease in systolic pressure during hypoperfusion, only evidence against a large role for changes in cardiac energetics.
A second limitation is that we did not measure cardiac energetics with the 0.5-s time resolution of He et al. (13). Therefore, we cannot be certain that some variable did not exhibit a large but temporary change before our first measurement of cardiac energetics 2 min after the start of myocardial hypoperfusion. Such a pattern is extremely unlikely because He et al. show that all energetic variables show only steady, not biphasic, changes during the first 30 s of myocardial hypoperfusion. Similarly, Clarke et al. (6) demonstrated with a 10-s time resolution that pH, Pi, and high-energy phosphates all change in a simple, steady direction during the early minutes of myocardial hypoperfusion and not in a complex biphasic way.
Finally, our technique for measuring CKflux requires the heart to be in a near-energetic steady state, a condition not met during the early minutes of myocardial hypoperfusion. To minimize the duration of steady state needed, we used a simplified technique for measuring CKflux that only required 15 min. Even so, relatively steady-state conditions were not met until 30 min into myocardial hypoperfusion. For this reason, we cannot say how CKflux changed before that time, and our data only demonstrate that CKflux contributes little if any to the sustained decrease in contractile function during myocardial hypoperfusion. It seems reasonable to suspect that large changes in CKflux do not occur during the early seconds of myocardial hypoperfusion because we know of no reports that describe rapid changes under any circumstances.
In summary, we report that, when CPP is gradually lowered, systolic
function decreases before changes in [ATP],
[PCr], [ADP], [Pi],
[H+], or
|GATP|.
Even after 6 min of hypoperfusion, when developed pressure had
decreased by over one-third, only very slight changes in
[Pi] and pH had
occurred, with no significant changes in [ATP], [PCr], [ADP], or
|GATP|.
The decrease in high-energy phosphate transfer rate during
hypoperfusion, CKflux, was not of
sufficient magnitude to explain the decrease in systolic function
observed after 30 min of hypoperfusion. We interpret these data to mean that the hypoperfusion-induced decrease in systolic pressure is not
causally linked to changes in any of these measures of cardiac energetics. Although there are undoubtedly other possible energetic explanations for the decrease in systolic function secondary to hypoperfusion not studied in the present paper, it seems likely that
nonenergetics mechanisms are of primary importance (13, 21, 23, 35).
Particularly intriguing are recent studies demonstrating that the
endocardial and coronary vascular epithelial cells produce substances
that modulate contractile function in a manner that is dependent on
coronary flow, shear stress, and the partial pressure of oxygen (35).
The role of these substances in causing the rapid downregulation of
contractile function during hypoperfusion remains to be determined in
the intact heart.
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ACKNOWLEDGEMENTS |
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This research was supported by National Heart, Lung, and Blood Institute Grants HL-48715 and HL-50594 and by a Grant-in-Aid from the American Heart Association, Massachusetts Affiliate. K. W. Saupe was supported by a National Research Service Award Fellowship.
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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. W. Saupe, 700 Albany St., W611, Boston, MA 02118.
Received 23 October 1998; accepted in final form 28 January 1999.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIAL AND METHODS
RESULTS
DISCUSSION
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) during myocardial hypoperfusion. [ADP] (
)
did not change during protocol, and pH (
