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-adrenoceptor density in pacing-induced heart failure
Cardiology Unit, Department of Medicine, Department of Neurobiology and Anatomy, University of Rochester Medical Center, Rochester, New York 14642
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Congestive heart failure is associated with cardiac
adrenergic nerve terminal changes and 
-adrenoceptor density
downregulation. To study the temporal sequence of these changes, we
performed studies in rabbits at 2, 4, and 8 wk of cardiac pacing (360 beats/min) and at 1, 2, and 4 wk after cessation of pacing. Rapid
pacing produced left ventricular (LV) dysfunction and an increase in plasma norepinephrine (NE) in 1-2 wk. At week 2, NE uptake
activity, NE uptake-1 density, and adenylyl cyclase responses to
isoproterenol, 5'-guanylyl imidodiphosphate
[Gpp(NH)p], and forskolin reduced. However, immunostained
tyrosine hydroxylase profile, -adrenoceptor density, and NE
histofluorescence did not reduce until 4-8 wk of pacing. After
cessation of cardiac pacing, LV function normalized quickly, followed
by return of tyrosine hydroxylase and NE profiles in 1 wk and adenylyl
cyclase responses to agonists and NE uptake activity in 2 wk.
Myocardial -adrenoceptor density returned to normal by 4 wk after
cessation of pacing. Our results suggest that there is no permanent
structural neuronal damage in the myocardium within the first 8 wk of
rapid cardiac pacing. Abnormal myocardial NE reuptake mechanism may
play an important pathophysiological role in heart failure.
norepinephrine; norepinephrine reuptake; adrenergic nerve terminals; pacing-induced cardiomyopathy
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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EVIDENCE HAS ACCUMULATED that sympathetic activation in
heart failure plays an important role in the progression of cardiac dysfunction. Recent studies in humans with congestive heart failure secondary to left ventricular systolic dysfunction have shown that
administration of -receptor blockers not only increases the left
ventricular ejection fraction but also reduces cardiac mortality and
morbidity (5, 27, 31). An increase in cardiac release of norepinephrine
(NE) has been observed in early mild heart failure before any obvious
generalized activation of the sympathetic nervous system (10). There is
also a preferential increase in sympathetic activity of the heart
compared with other organs in severe heart failure (10, 13). The marked
preferential increase in the release of cardiac NE probably contributes
to the eventual depletion of NE in the failing heart (9). The heart is
also thought to be functionally denervated, with reduction of tyrosine
hydroxylase activity to account for the loss of NE (8, 44).
We recently reported that unlike tyrosine hydroxylase, the neurolemmal
marker protein gene product 9.5 (PGP9.5)
content is not reduced in the failing myocardium (44), suggesting that the sympathetic nerves are structurally intact and may recover in
function with therapy. We have further shown that the functional alterations in the sympathetic nerve terminals in heart failure include
loss of NE and tyrosine hydroxylase, decrease of NE uptake activity,
and reduction of NE uptake-1 carrier site density (15). Because
neuronal reuptake of NE is the major mechanism for removal of NE from
the presynaptic cleft and termination of action of NE on the myocardial
-adrenoceptors, this decrease in myocardial NE uptake activity is
expected to increase interstitial NE and decrease myocardial
-adrenoceptor density. Indeed, there is a strong inverse
relationship between myocardial NE uptake activity and -adrenoceptor
density in animals with heart failure (15, 23).
To further determine whether the changes in adrenergic neuronal NE
uptake play a role in the pathophysiology of myocardial -adrenoceptor downregulation, we carried out the present study to
examine the temporal associations of cardiac sympathetic nerve terminal
function and the -adrenoceptor-coupled adenylyl cyclase signal
transduction system during the development of and recovery from
pacing-induced heart failure in rabbits.
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METHODS |
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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Animal preparations. Adult healthy New Zealand White rabbits (2.6-3.8 kg, 4-6 mo old) were chosen. Animals were prepared for experimental heart failure by a modified technique of Spinale et al. (40). The study was approved by the University of Rochester Committee on Animal Resources and conformed to the guiding principles approved by the Council of the American Physiological Society and the National Institutes of Health Guide for the Care and Use of Laboratory Animals (DHHS publication National Institutes of Health 85-23, Revised 1985, Office of Science and Health Reports).
Animals were anesthetized with intramuscular ketamine (50 mg/kg) and xylazine (3 mg/kg) followed by supplemental doses if necessary. The animals were intubated and ventilated with respirators (Harvard Apparatus, South Natick, MA). Through a sterile skin incision, subxyphoid thoracotomy and pericardiotomy were performed. A shielded pacing lead (TPW50, Ethicon, Somerville, NJ) was then sutured onto the apical region of the left ventricular free wall and brought out through the diaphragm and abdominal wall. A second pacing lead was sutured onto the left pectoral muscle. These pacing leads were routed subcutaneously and exteriorized to the interscapular region, and the wound was closed. Artificial ventilation was discontinued, and the tracheal tube was removed after spontaneous breathing was assured. One week later, the pacing leads were connected to a model 8086 Prevail VHRP programmable pacemaker (Medtronic, Minneapolis, MN). Animals were assigned randomly to receive rapid ventricular pacing at a rate of 360 beats/min for varying durations. A control group of animals underwent identical surgery but received no cardiac pacing. They were euthanized 9 wk after the thoracotomy, corresponding in time to animals after 8 wk of cardiac pacing. The pacemaker and pacing leads were stored in a pocket of a custom-made rabbit jacket.Experimental protocol.
To study the time course of changes during the progression of and
recovery from heart failure, the animals were euthanized for study
after 2, 4, or 8 wk of rapid cardiac pacing or 1, 2, or 4 wk after
cessation of 8 wk of pacing. An electrocardiogram was recorded once a
week during the pacing protocol to confirm proper cardiac pacing. A
group of animals without rapid pacing was included as control. There
were six to eight animals in each group. Echocardiograms were taken
once a week during rapid pacing and at 3 days, 1 wk, 2 wk, and 4 wk
after cessation of pacing. At the end of the specified time periods,
the animals were anesthetized with intramuscular ketamine (28 mg/kg)
and midazolam (0.8 mg/kg) for measuring resting hemodynamics and plasma
NE. The animals were then given a lethal dose (>100 mg/kg) of
intravenous pentobarbital sodium. The hearts were removed and weighed.
Each ventricular free wall was separated from the septum and rinsed in
ice-cold oxygenated normal saline. The left ventricular weight includes both the septum and the left ventricular free wall. Fresh left ventricular muscle blocks were taken for immediate measurement of NE
uptake activity. Other muscle blocks were either rapidly frozen and
fixed or stored in liquid nitrogen for measurements of left ventricular
noradrenergic nerve terminal profiles, NE uptake-1 carrier site
density, -adrenoceptor density, and adenylyl cyclase activity.
Hemodynamic and echocardiographic measurements.
Cardiac pacing was discontinued before the final hemodynamic study.
Two-dimensional and M-mode echocardiographic studies were performed in
a left lateral decubitus position, using a scanning system heart (SSH)
sonographic system (Toshiba America Medical Systems, Tustin,
CA). A 5-mHz transducer was used to measure the maximum
left ventricular end-diastolic (EDD, measured in mm) and end-systolic
dimensions (ESD, mm). Left ventricular fractional shortening (FS, %)
was calculated as [(EDD 
ESD) × 100]/EDD.
Myocardial NE uptake activity. Myocardial NE uptake activity was measured in quadruplicate by incubating fresh tissue slices at 37°C for 15 min in 50 nmol/l l-[7-3H(N)]NE (13.8 Ci/mmol; New England Nuclear, Boston, MA). Specific 3H-uptake activity, defined as the difference in radioactivity between tissue slices incubated in a [3H]NE-containing solution at 37°C and those at 4°C, is considered to represent NE uptake activity (23).
Myocardial NE uptake-1 carrier site density. Myocardial NE uptake-1 carrier site density was measured by using the radioligand binding technique with [3H]nisoxetine (New England Nuclear) (41). Approximately 80 µg of membrane protein, suspended in 50 mM Tris · HCl buffer (pH 7.4) containing 300 mM NaCl and 5 mM KCl, was incubated in triplicate with 3 nM [3H]nisoxetine and eight concentrations of nonradioactive nisoxetine (0.3125-10 pM) at room temperature for 90 min in a final volume of 0.25 ml. For determination of nonspecific binding, 10 µM nisoxetine was used. The reaction was terminated by addition of ice-cold Tris buffer and filtered immediately through Whatman GF/B filters (Whatman Chemical Separation, Clifton, NJ) on a Brandel cell harvester (Biomedical Research and Development Laboratories, Gaithersburg, MD). The membranes were rapidly washed, dried, and counted for 3H radioactivity by liquid scintillation spectrometry (Tri-Carb 460 CD, Packard Instrument, Downers Grove, IL). The number of receptor binding sites and the dissociation constant were calculated using the EBDA computer software program (Elsevier Science Publisher, Cambridge, UK) (26).
Anatomic studies of ventricular sympathetic nerves. Fresh left ventricular tissue blocks were rapidly frozen and prepared for glyoxylic acid-induced histofluorescence for catecholamines and immunocytochemistry for tyrosine hydroxylase (15). Histofluorescence specific for catecholamines was performed using a modification (1) of the sucrose-potassium-phosphate-glyoxylic acid condensation method of de la Torre (6). A sheep anti-tyrosine hydroxylase primary antibody was used for the immunocytochemical visualization of tyrosine hydroxylase. Sections for NE histofluorescence were photographed at ×30 magnification, whereas slides for tyrosine hydroxylase immunocytochemistry were photographed at ×20 magnification onto 35-mm slides. The number of stained catecholamine profiles was counted in a 0.221-mm2 (0.003536-mm3) field. The number of immunostained tyrosine hydroxylase profiles was counted in a 0.00885-mm3 field. The results of six fields were averaged for each ventricle.
Myocardial -adrenoceptor density.
Myocardial -adrenoceptor density was measured by using the
radioligand binding technique with
[125I]iodocyanopindolol (ICYP, 2,200 Ci/mmol;
New England Nuclear) (20). Tissue protein was determined using a
bicinchoninic acid protein assay reagent (Pierce, Rockford, IL) with
bovine serum albumin as a standard. Approximately 20 µg
of membrane protein, suspended in 50 mM Tris · HCl
buffer (pH 7.4) containing 120 mM NaCl and 5 mM KCl, was incubated in
triplicate with eight concentrations of
[125I]ICYP (5-250 pM) at 37°C for 60 min in a final volume of 0.25 ml. Nonspecific binding was determined by
parallel incubation of samples containing 100 µM propranolol. The
technical details of the assay were similar to those described above
for the NE uptake-1 carrier site density.
Adenylyl cyclase activity. Adenylyl cyclase activity was assayed in duplicate as described previously (11) with a mixture containing 50 mM Tris · HCl (pH 7.4), 0.4 mM EGTA, 0.5 mM 3-isobutyl-1-methylxanthine, 2 mM MgCl2, 5 mM phosphocreatine, 15 units creatine phosphokinase, and approximately 50 µg of membrane protein in a final volume of 0.45 ml. The mixture was incubated at 37°C for 5 min in the presence and absence of isoproterenol (0.1 mM with 0.1 mM GTP), 5'-guanylyl imidodiphosphate [Gpp(NH)p, 0.1 mM], or forskolin (0.1 mM). Isoproterenol and Gpp(NH)p were dissolved in distilled deionized water, whereas forskolin required 50% dimethylsulfoxide to dissolve completely. The agonist concentrations were chosen to produce maximal adenylyl cyclase stimulation. The samples were assayed for cAMP levels by the competitive protein-binding technique (42) using a cAMP assay system (Amersham Life Science, Little Chalfont, Buckinghamshire, UK).
Statistical analysis. The experimental data were analyzed with the RS/1 Research System (Bolt, Beranek, and Newman Software Products, Cambridge, MA) and SYSTAT software (SPSS, Chicago, IL). Data are expressed as means ± SE. The statistical significance of difference among the experimental groups was determined by one-way ANOVA. If the ANOVA revealed significant difference, pairwise tests of individual group means were compared by Tukey comparisons. For the weekly echocardiographic data, ANOVA for repeated measures was used to determine the significance of changes from baseline. A probability value of <0.05 was considered significant.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Body and heart weights.
Figure 1 shows that right and left
ventricular weights, normalized by body weight, were increased by
4-8 wk after commencement of rapid cardiac pacing. The heart
weight remained elevated and showed no regression in 4 wk after
cessation of rapid pacing. There were no significant differences in
body weight during the development and recovery from rapid ventricular
pacing (F = 1.77).
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Resting hemodynamics and cardiac function.
Table 1 shows that resting heart rate and
mean blood pressure did not differ significantly among the various
groups of animals after rapid cardiac pacing or cessation of pacing.
However, plasma NE increased quickly after the beginning of cardiac
pacing, and remained elevated throughout the pacing. Plasma NE
decreased promptly after cardiac pacing.
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Myocardial NE uptake.
Figure 4 shows that myocardial NE uptake
activity and NE uptake-1 carrier site density were decreased shortly
(within 2 wk) after onset of rapid cardiac pacing. By 8 wk of pacing,
myocardial NE uptake activity and NE uptake-1 carrier site density
decreased to 40-50% of the control. Also shown in Fig. 4 is the
return of myocardial NE uptake function after cessation of pacing.
However, the return was not as prompt as the left ventricular
hemodynamic and echocardiographic parameters (Figs. 2 and 3). The NE
uptake-1 carrier site density did not return to control until 2-4
wk after cessation of pacing.
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Cardiac sympathetic nerve terminal profiles.
Figure 5 shows representative NE
histofluorescence profiles at different stages of rapid cardiac pacing
and 1 and 4 wk after cessation of pacing. In addition, we have
summarized the group data of NE histofluorescence and immunostained
tyrosine hydroxylase profiles in Fig. 6.
Figure 5 shows that neither catecholaminergic histofluorescence
profiles nor immunostained tyrosine hydroxylase profiles decreased
immediately after commencement of rapid ventricular pacing. No
significant changes occurred in animals after 2 wk of pacing. However,
both neurotransmitter profiles decreased significantly by 4-8 wk
of rapid cardiac pacing. Figure 5 also shows that both neuronal NE and
tyrosine hydroxylase profiles returned to control within 1 wk after
cessation of rapid pacing and remained unchanged thereafter.
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Myocardial -adrenoceptor function.
Figure 7 shows that left ventricular
-adrenoceptor density did not change from the control values 2 wk
after the start of rapid cardiac pacing but decreased significantly at
4 and 8 wk of rapid pacing. Myocardial -adrenoceptor density also
did not change immediately after discontinuation of rapid ventricular pacing. It remained reduced below control values at 2 wk and did not
return to control until 4 wk after cessation of rapid pacing.
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-adrenoceptor density. Significant improvements already
occurred within 1 wk after cessation of pacing. The responsiveness of
adenylyl cyclase to isoproterenol, Gpp(NH)p, and forskolin returned to
baseline within 1-2 wk after discontinuation of rapid pacing.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Rapid ventricular pacing has been used extensively to study the
hemodynamics, neurohormonal alterations, pathogenesis, and efficacy of
therapeutic interventions in heart failure (39, 40). Studies have shown
that hemodynamic changes occur as early as 24 h after rapid pacing
(18), with continuing deterioration of ventricular function (29),
myocardial muscle depression (12), and eventual development of clinical
heart failure after 3-4 wk of pacing (18). Acute rapid ventricular
pacing also causes an increase in plasma NE and reductions
of fraction of myocardial -receptor binding agonist with high
affinity as well as adenylyl cyclase activity within 24 h (18), but
changes in myocardial -receptor density, regulatory guanosine
nucleotide binding proteins (G proteins), and myocardial NE do not
occur until 3-4 wk after cessation of rapid cardiac pacing (18,
25). Furthermore, it has been demonstrated that left ventricular
systolic function and myocardial -adrenoceptor density return to
normal within 4 wk after discontinuation of pacing (22, 28).
Our present study is the first longitudinal investigation linking the
hemodynamic changes produced by rapid cardiac pacing to the myocardial
-adrenoceptor-coupled adenylyl cyclase system and sympathetic nerve
terminal abnormalities in a time-dependent fashion. The study not only
confirmed the hemodynamic and myocardial -adrenoceptor changes
mentioned previously in pacing-induced cardiomyopathy but also showed
that as in dogs with heart failure (15, 23), sympathetic nerve terminal
function was abnormal in the rabbits with pacing-induced heart failure.
Left ventricular NE uptake activity and NE uptake-1 carrier site
density decreased significantly within 2 wk after the start of rapid
cardiac pacing, followed by the reductions of NE histofluorescence and
tyrosine hydroxylase profiles and myocardial -receptor density at
4-8 wk of rapid pacing. The findings suggest that the reduction of the cardiac NE uptake function is an earlier alteration in the process
of cardiac sympathetic nerve terminal abnormalities in heart failure.
Decreases in NE uptake activity and NE uptake sites have also been
shown to occur in the failing human heart (2, 9, 19).
There is a positive correlation between cardiac NE uptake and left
ventricular ejection fraction (19).
Studies have linked the reduction of cardiac neuronal uptake of NE to the increased release of NE from the heart and depletion of NE in the failing heart (19). The sympathetic nervous system is activated early after initiation of rapid ventricular pacing (16, 18). This early activation of cardiac sympathetic activity could potentially increase the cardiac synaptic NE concentration to a level sufficient to cause downregulation of NE uptake-1 carrier sites and decreased NE uptake activity within 2 wk. Direct support of a pivotal role of NE on cardiac sympathetic nerve function was provided using an exogenous NE infusion (15). The dose of NE used was subhypertensive but was sufficient to increase cardiac interstitial NE to a level similar to that found in heart failure (7, 21). This dose of NE was sufficient to decrease NE uptake activity and reduce neuronal profiles of NE histofluorescence and tyrosine hydroxylase (15). We have also shown that the effects of excess NE on sympathetic nerve terminal function could be prevented by antioxidant vitamins (23a), suggesting that this action of NE probably is mediated via the formation of NE-derived metabolites of oxygen free radicals.
We found a decrease of cardiac adenylyl cyclase response to
isoproterenol stimulation in rabbits 2 wk after rapid cardiac pacing,
followed by a reduction of myocardial -adrenoceptors at week
4 of pacing. Because the increase in plasma NE precedes the onset
of changes in regulatory G proteins and -adrenoceptor density in the
development of heart failure, it has been postulated that the changes
in the -adrenoceptor-coupled G protein adenylyl cyclase system are a
result of generalized adrenergic stimulation. However, our prior
studies in an animal model with right-sided heart failure have shown
that myocardial -adrenoceptor density is reduced only in the failing
right ventricle (23). The left ventricle shows no changes in myocardial
-adrenoceptor density despite exposure to the same levels of
elevated circulating NE as the right ventricle. Thus the
-adrenoceptor changes would have to be explained by increased local
cardiac-derived NE (4), produced by either the preferential sympathetic
stimulation to the failing heart, or a defect in the neuronal NE uptake
mechanism, or both. A recent study (38) indicates that intact
ventricular innervation is essential for the expression of myocardial
-adrenergic subsensitivity during the development of pacing-induced
heart failure. We have shown previously that myocardial
-adrenoceptor density correlated inversely with cardiac interstitial
NE (7), suggesting localized chamber-specific agonist-induced
homologous desensitization in heart failure (14).
Unlike -adrenoceptor density, the decreases of adenylyl cyclase
activity in response to isoproterenol, Gpp(NH)p, and forskolin were
diminished in early heart failure, occurring within 2 wk of rapid
cardiac pacing. The decrease in the response to isoproterenol may be
related, at least in part, to the uncoupling of the -receptors to G
proteins, which is known to occur after NE infusion (43). The coupling
of -receptors to G proteins probably is mediated by G protein
receptor kinase (33). In addition, rapid cardiac pacing has been shown
to reduce Gs protein expression in the left ventricle (33,
34). Changes in Gi proteins, however, have been
conflicting. Kiuchi et al. (18) showed an increase in
Gi
2 protein in heart failure, but other
investigators (34, 36) have demonstrated a decrease in
Gi2. Roth et al. (36) found that
cardiac Gi content did not correlate with adrenergic
responsiveness and that the decreased Gs was caused by
increased degradation rather than decreased synthesis.
Rabbits are fragile and do not tolerate acute manipulations (such as catheterization) well unless they are adequately anesthetized. Ketamine, midazolam, and xylazine are the preferred parenteral anesthetics compared with pentobarbital (3). We employed ketamine and midazolam to facilitate insertion of a Millar catheter into the left ventricle. Although this anesthetic combination produces minimal cardiorespiratory effects, it increases heart rate in normal animals and humans (17, 24). The increase in heart rate produced by anesthetics might have minimized the difference in heart rate between control and heart failure rabbits and thus obscured the tachycardia known to occur in heart failure.
The majority of NE in the tissue is stored in the adrenergic neuronal terminal vesicles. The cardiac NE content is determined by the rates of NE release, turnover, and synthesis. NE release and turnover are influenced by cardiac sympathetic tone and NE uptake capacity, whereas the rate of NE synthesis is affected largely by tyrosine hydroxylation, which is the rate-limiting step involved in the catecholamine biosynthesis (30). Results of our present study indicate that despite apparent increased sympathetic discharges, cardiac NE content was preserved in an early phase of heart failure, probably because the tyrosine hydroxylation and NE reuptake were relatively intact to compensate for the increased NE discharge. However, as heart failure advanced, both tyrosine hydroxylase and NE uptake-1 carrier site density decreased. As a result, cardiac NE content, as judged by the NE histofluorescence, decreased at 8 wk of rapid cardiac pacing. The relative contributions of the various factors to cardiac NE depletion in heart failure, however, may vary depending on the experimental conditions. An early study in animals showed reduced tyrosine hydroxylase activity played a role in the depletion of cardiac NE stores in heart failure (35). On the other hand, Eisenhofer et al. (9) showed that the decreased cardiac NE stores in patients with heart failure was caused by chronically increased NE turnover and reduced efficiency of NE reuptake and storage rather than by insufficient tyrosine hydroxylation.
In conclusion, our present study is the first systematic longitudinal
investigation of the temporal alterations in cardiac sympathetic nerve
terminal function and its associations with myocardial -adrenoceptor
density in pacing-induced cardiomyopathy. Such a study is important not
only because it illustrates that both qualitative and quantitative
changes may occur at different stages of heart failure but also because
it provides a temporal sequence of events that may allow us to
speculate on the mechanisms of changes in early heart failure.
Discrepancies in results in the heart failure literature may be related
in part by the differences in duration of heart failure studied by the
various investigators. Figure 9 summarizes
the changes observed in this study, and a hypothesis that we have
developed regarding the initial changes in heart failure. It is
believed that rapid ventricular pacing causes immediate left
ventricular dysfunction and sympathetic nervous system stimulation.
There is an early and preferential activation of the cardiac
sympathetic nerves. This results in an increase in cardiac interstitial
NE concentration. Early in the course of development of heart failure
(within the first 2 wk), adenylyl cyclase responses to isoproterenol,
Gpp(NH)p, and forskolin are reduced, suggesting a defect in the
-receptor coupling mechanism and its associated regulatory G
proteins. Myocardial NE uptake activity is also reduced. This impairs
the ability of the heart to remove NE in the synaptic cleft, leading to
a higher interstitial NE concentration and greater spillover of NE from the heart. By 4 wk of pacing, we found reductions of immunostained tyrosine hydroxylase profiles and myocardial -adrenoceptor density. At 8 wk of pacing, NE histofluorescence decreased. Cardiac NE depletion
probably is caused by both the increased release and turnover of NE and
the decreased synthesis of NE because of reduced tyrosine
hydroxylation. However, NE depletion probably is not responsible for
left ventricular systolic dysfunction, because left ventricular
systolic function improved promptly after cessation of rapid
ventricular pacing, with no changes in tissue NE stores. The high
interstitial NE probably is responsible for reductions of NE uptake-1
carrier site density, tyrosine hydroxylase, and -adrenoceptor
density. The rapid recovery of function indicates that cardiac
sympathetic nerve terminal abnormalities in heart failure probably are
caused by reversible functional alterations rather than by permanent
structural damage. NE is a trophic hormone and may play a role in the
development of cardiac hypertrophy and left ventricular remodeling in
the pacing-induced cardiomyopathy. Myocardial -adrenergic
sensitivity is reduced in established heart failure, because of both
-adrenoceptor downregulation and other postreceptor abnormalities in
the receptor-coupled G protein adenylyl cyclase signal transduction
pathway. The temporal relationships between changes of NE uptake
activity and myocardial -adrenoceptor function suggest an important,
pivotal role of NE uptake activity in myocardial -adrenoceptor
downregulation in pacing-induced cardiomyopathy. Additional
investigations are needed to fully establish the cause-and-effect
relationships and the biochemical or cellular mechanisms that lead to
these changes.
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ACKNOWLEDGEMENTS |
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The authors thank Dr. William B. Hood, Jr., for constructive comments and suggestions during the conduct of study and in the preparation of the manuscript.
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FOOTNOTES |
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The study was supported in part by an American Heart Associate grant and a Paul N. Yu Fellowship.
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: C.-s. Liang, Univ. of Rochester Medical Center, Cardiology Unit, Box 679, 601 Elmwood Ave., Rochester, NY 14642 (E-mail: chang-seng_liang{at}URMC.Rochester.edu).
Received 21 June 1999; accepted in final form 15 November 1999.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Values
that differed from week 8 of pacing at P < 0.05.
