Protection against Myocardial Dysfunction Induced by Global Ischemia-Reperfusion by Antisense-Oligodeoxynucleotides Directed at beta 1-Adrenoceptor mRNA

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Vol. 294, Issue 2, 722-727, August 2000

Protection against Myocardial Dysfunction Induced by Global Ischemia-Reperfusion by Antisense-Oligodeoxynucleotides Directed at $beta$ ₁-Adrenoceptor mRNA¹

Hongjiang Chen , Yuan Clare Zhang, Dayuan Li , M. Ian Phillips, Paullete Mehta, Min Shi and Jawahar L. Mehta

Departments of Medicine (H.C., D.L., M.S., J.L.M.), Physiology (Y.C.Z., M.I.P.), and Pediatrics (P.M.), University of Florida College of Medicine, and the Veterans Affairs Medical Center (H.C., D.L., M.S., J.L.M.), Gainesville, Florida

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

Plasma catecholamine levels rise, and myocardial $beta$ ₁-adrenoceptor ( $beta$ ₁-AR) sensitivity increases during ischemia. These factorsenhance myocardial injury and cardiac dysfunction. $beta$ ₁-AR blockersare clinically used to protect heart against ischemia and to improvecardiac dysfunction in patients with ischemic heart disease, butthese agents often cause intolerable side effects. To examinethe potential cardioprotective effect of therapy with antisense-oligodeoxynucleotidesdirected at $beta$ ₁-AR mRNA ( $beta$ ₁-AS-ODNs) during myocardial ischemia-reperfusion,Sprague-Dawley rats were treated with $beta$ ₁-AS-ODNs or inverted-oligodeoxynucleotides(IN-ODNs), each 200 µg/rat. Hearts were excised, perfused, andsubjected to global ischemia (30 min) followed by reperfusion(30 min). Other rats were given selective $beta$ ₁-AR blocker atenolol(2 mg/kg) or saline before excising the hearts. Ischemia-reperfusionresulted in cardiac dysfunction, indicated by an increase in coronaryperfusion pressure and left ventricular end-diastolic pressureand a decrease in developed left ventricular pressure, as wellas evidence of lipid peroxidation in saline-treated rats (allP < .05 versus control values). Administration of AS-ODNs or atenolol,but not IN-ODNs, protected hearts against functional deteriorationand lipid peroxidation (P < .05 versus saline or IN-ODNs treatment).AS-ODNs therapy appeared to be equivalent to atenolol in theseeffects. Expression of $beta$ ₁-AR protein as well as mRNA in the myocardiumwere markedly up-regulated after ischemia-reperfusion, and treatmentwith $beta$ ₁-AS-ODNs, but not atenolol, decreased the rise in enhancedexpression of $beta$ ₁-AR. These observations imply that $beta$ ₁-AS-ODNscan ameliorate cardiac dysfunction after ischemia-reperfusionby reducing the expression of $beta$ ₁-AR in the ischemic-reperfusedmyocardium.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

Acute myocardial ischemia causes significant increase in plasma catecholamine levels, which leads to exacerbation of the ischemicmyocardial injury (Waldenstrom et al., 1978; Rona, 1985). Theworsening myocardial ischemia is an important factor in cardiacdysfunction. Acute myocardial ischemia also is characterized byincreased sensitivity of $beta$ -adrenoreceptors ( $beta$ -ARs) to catecholamines(Strassere et al., 1990). $beta$ -ARs form the interface between thesympathetic nervous system and the cardiovascular system (Mukherjeeet al., 1979; Maisel et al., 1985; Strassere et al., 1990). Importantly, $beta$ ₁-AR subtype ( $beta$ ₁-AR) is the predominant subtype in the myocardium(Minneman et al., 1995), and its activity and sensitivity arethought to regulate cardiac function via adenylyl cyclase activity(Mukherjee et al., 1979; Thandroyen et al., 1986; Böhm, 1995).Several experimental studies show that density and mRNA of $beta$ ₁-ARare augmented in the myocardium after acute ischemia (Maisel etal., 1985; Karliner et al., 1989; Ihl-Vahl et al., 1995). Experimentaland clinical studies also have demonstrated that therapy with $beta$ -AR blockers, especially with selective $beta$ ₁-AR blockers, can protectmyocardium against ischemic injury and dysfunction (Ablad et al.,1987; Lu et al., 1990; Schulz et al., 1995), decrease infarctsize (Schulz et al., 1995), and reduce the incidence of suddencardiac death in patients with myocardial infarction (Yusuf etal., 1985).

Although chemical $beta$ -AR blockers are commonly used in the treatment of ischemic heart disease, these agents often cause centralnervous system side effects and the $beta$ ₂-AR antagonistic activityis associated with an increase in peripheral vascular resistance.Development of antisense-oligodeoxynucleotides (AS-ODNs) againstspecific receptor mRNA is a novel approach to decrease the synthesisof receptor proteins (Phillips et al., 1994; Phillips, 1997).This approach has potential to be of therapeutic benefit in diseasestates characterized by up-regulation of these receptors (Phillipset al., 1994; Phillips, 1997; Yang et al., 1998). AS-ODNs directedat $beta$ ₁-AR mRNA ( $beta$ ₁-AS-ODNs) have been reported to reduce bloodpressure in spontaneously hypertensive rats (SHR) for prolongedperiod with a single i.v. injection (Zhang et al., 2000).

We hypothesized that the use of $beta$ ₁-AS-ODNs may protect myocardium against ischemia-reperfusion-induced dysfunction in theisolated rat heart. This study was undertaken to test this hypothesis.We also examined the effect of $beta$ ₁-AS-ODNs on lipid peroxidation,the expression of $beta$ ₁-AR protein, and mRNA in the myocardium afterischemia-reperfusion.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

ODNs and Vector Liposome. $beta$ ₁-AS-ODNs and inverted-oligodeoxynucleotides (IN-ODNs) control were 15-mers and targeted to $-$ 5 to +10 of rat $beta$ ₁-AR mRNA encompassingthe AUG start colon. The sequence of AS-ODNs was 5'-CCGCGCCCATGCCGA-3',and the corresponding IN-ODNs was 5'-AGCCGTACCCGCGCC-3'. TheseODNs were modified by backbone phosphorothioation and synthesizedin the DNA Synthesis Core Laboratory of the University ofFlorida.

Because cationic liposomes enhance the uptake of DNA by the tissues and also protect DNA from degradation and extend its circulationtime (Phillips et al., 1994

), The cationic lipid 1,2-bis(oleoyloxy)-3-(trimethylammonio)propane(DOTAP) mixed with helper lipid L- $alpha$ -dioeoyl phosphatidylethanolamine(DOPE; mole:mole = 1:1) was used in this study as vector for ODNs.The average diameter of liposomes was 200 to 300 nm. ODNs/liposomescomplex was prepared on the day of use by mixing the desired amountof ODNs with DOTAP/DOPE to final DNA concentration of 300 µg/mlin 5% (w/w) dextrose in water and incubating at room temperaturefor 60 min (Yang et al., 1998

; Zhang et al., 2000

Animals. Male Sprague-Dawley rats weighing 200 to 250 g were injected i.v. with either AS-ODNs (n = 7) or IN-ODNs (n = 7) at a doseof 200 µg/rat 4 days before excising the hearts. DOTAP/DOPE liposomes(700 µg/rat) were given along with ODNs. Other groups of ratswere treated with saline (n = 13), or the selective $beta$ ₁-AR blockeratenolol (2 mg/kg; n = 7) 6 h before the hearts were excised.These animal studies were approved by the University of FloridaAnimal CareCommittee.

Isolated Perfused Heart Model. All rats were anesthetized with sodium pentobarbital (40 mg/kg i.p). The hearts were excised rapidly and placed in ice-coldKrebs-Henseleit buffer (118 mM NaCl, 4.7 mM KCl, 1.2 mM KH₂PO₄,1.2 mM MgSO₄, 1.25 mM CaCl₂, 25 mM NaHCO₃, and 11 mM glucose,pH 7.4). Within 1 min, the hearts were transferred to an isolatedperfusion apparatus and perfused via the aorta with oxygen-saturated(95% O₂ + 5% CO₂) Krebs-Henseleit buffer kept at 37°C with theuse of a MasterFlex pump (model 7015-21; Cole-Palmer Instrument,Vernon Hills, IL) according to the modified Langendroff procedure(Neely and Rovetto, 1975; Yang et al., 1998). The heart was placedin a semiclosed circulating water-warmed (37°C) air chamber, pacedatrially with a Medtronic 5320 pacemaker at a rate of 300 beats/min,and perfused at a constant flow (5.5-6.0 ml/min). Coronary perfusionpressure (CPP) was measured via a catheter placed just proximalto the aorta and connected to a Gould Statham P23ID pressure transducer.A latex balloon filled with water and connected to a Gould StathamP23ID pressure transducer was inserted the left ventricle throughthe left atrium to measure left ventricular end-diastolic pressure(LVEDP), left ventricular systolic pressure (LVSP), and developedleft ventricular pressure (dLVP; dLVP = LVSP $-$ LVEDP). LVEDP duringequilibration was set at 5 to 7 mm Hg. All measurements were continuouslyrecorded on a four-channel recorder (Astro-Med, West Warwick,RI).

Myocardial Ischemia and Reperfusion. Six hearts from saline-treated rats were continuously perfused with Krebs-Henseleit buffer for 80 min and served as sham control.Hearts from other rats, after 20 min of equilibration, were subjectedto 30 min of ischemia followed by 30 min of reperfusion. Aftercompletion of the experiment, hearts were frozen in liquid nitrogenfor $beta$ ₁-AR density analysis (by radioligand binding assay), $beta$ ₁-ARprotein analysis (by Western blot), $beta$ ₁-AR mRNA analysis by reversetranscription-polymerase chain reaction (RT-PCR), and measurementof malondialdehyde (MDA).

Quantification of $beta$ ₁-AR Protein Expression in Myocardium. Myocardial tissues were homogenized and lysed in boiling lysis buffer (1% SDS, 0.1% Triton X-100, and 10 mM Tris-HCl, pH 7.4)and centrifuged at 10,000 rpm for 30 min at 4°C. The lysate proteinfrom myocardial tissues (20 µg/lane) was separated by 8% SDS-polyacrylamidegel electrophoresis with a Bio-Rad Mini-Protean cell, transferredto nitrocellulose membrane (Amersham, Arlington Heights, IL).After incubation in blocking solution (4% nonfat milk; Sigma,St. Louis, MO), membranes were incubated with 1:1000 dilationprimary antibody (polycolonal antibody to $beta$ ₁-AR; Santa Cruz Biotechnology,Santa Cruz, CA) overnight at 4°C. Membranes were washed and incubatedwith 1:2000 dilution second antibody (Amersham) for 1 h. The membraneswere detected with the enhanced chemiluminescence system, andrelative intensity of bands of interest was analyzed by NSF-300GScanner (Microtek, San Clemente, CA), as described previously(Yang et al., 1998; Li et al., 1999).

Determination of $beta$ ₁-AR mRNA. Total RNA was isolated from rat myocardium with the single step acid-guanidinum thiocyanate-phenol-chloroform method and quantified(Chomczynski and Sacchi, 1987). One microgram of total RNA wasreverse transcripted with oligo-dT (Promega, Madison, WI) andM-MLV reverse transcriptase (Promega) at 37°C for 1 h. RT material(1.5 µl) was amplified with Taq DNA polymerase (Promega) witha primer pair specific to $beta$ ₁-AR (forward primer: 5'-CTCCGAAGCTCGGCATGG-3';and reverse primer: 5'-GCACGTCTACCGAAGTCCAGA-3'). PCR productwas 432 base pairs. For PCR, 35 cycles were used at 95°C for 1min, 60°C for 1 min, and 72°C for 1 min. The RT-PCR amplifiedsamples were visualized on 1.8% agarose gels with ethidium bromide.A primer pair rat GAPDH was used as control (forward primer: 5'-ATCAAATGGGGTGCTGGTGCTG-3', and reverse primer: 5'-CAGGTTTCTCCAGGCGGCATGTCA-3'). ForPCR, 35 cycles were used at 95°C for 1 min, 60°C for 1 min, and72°C for 1 min. PCR product was 504 base pairs. The amount ofPCR product of $beta$ ₁-AR mRNA was determined by comparison of signaldensity with simultaneously amplified cDNA for GAPDHmRNA.

Determination of MDA Levels in Myocardium. MDA levels in the myocardium were measured in duplicate by a modification of the method of Ohkawa et al. (1979). Briefly,the ventricular tissues were homogenized. The assay mixture consistedof 0.1 ml of the tissue homogenate, 0.4 ml of 0.9% NaCl, 0.5 mlof 3% SDS, and 3 ml of TBA (thiobarbituric acid reagent, containingequal parts of 0.8% aqueous thiobarbituric acid and acetic acid),and was heated for 75 min at 95°C. Thereafter, 1 ml of cold 0.9%NaCl was added to the mixture, which was cooled and extractedwith 5 ml of n-butanol. After centrifugation at 3000 rpm for 15min, the butanol phase was assayed spectrophotometrically at 532nm. Tetramethoxypropane (in amounts of 0, 0.1, 0.2, 0.4, 0.8,and 1.0 nmol) served as external standard. MDA levels in myocardiumwere expressed as micromoles per gram oftissue.

Data Analysis. Data are presented as mean ± S.E. Statistical significance was determined in multiple comparisons among independent groupsof data in which ANOVA and the Student-Newman-Keuls test indicatedthe presence of significant differences. A P value of $<=$ .05 wasconsidered statisticallysignificant.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Cardiac Dysfunction during Ischemia-Reperfusion. The basal values of CPP, LVEDP, and dLVP were similar in all groups of rat hearts. In the control continuously buffer-perfusedhearts observed for 80 min (n = 6), there were only minimal (~5%)changes in the indices of cardiac function. In the hearts fromsaline-treated rats (n = 7), 30 min of ischemia followed by 30min of reperfusion resulted in marked cardiac dysfunction, indicatingby a significant increase in CPP and LVEDP, and a decrease indLVP (all P < .01 versus preischemiavalues).

Treatment of rats with $beta$ ₁-AS-ODNs (n = 7) markedly attenuated the ischemia-reperfusion-induced myocardial dysfunction, indicatedby preservation of dLVP and minimization of increase in LVEDPand CPP (all P < .05 versus saline group). Treatment of rats withatenolol (n = 7) also reduced the increase in CPP and LVEDP inducedby ischemia-reperfusion (all P < .05 versus saline group), andmodestly attenuated the ischemia-reperfusion-induced change indLVP (P < .05 versus saline group). Overall, AS-ODN treatmentappeared to be equivalent to atenolol treatment in these effects.Treatment with IN-ODNs showed no effect on ischemia-reperfusion-inducedmyocardial dysfunction. Data on cardiac function parameters frommultiple experiments are summarized in Fig. 1.

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Fig. 1. Summary of data on ischemia-reperfusion-induced changes in CPP, LVEDP, and dLVP in hearts from different group of rats. Note the marked increase in LVEDP and CPP and a decrease in dLVP in the saline-treated rat hearts exposed to a brief period of ischemia-reperfusion. Administration of AS-ODNs, but not IN-ODNs, showed a markedly beneficial effect on cardiac function, indicated by smaller increases in CPP and LVEDP and preservation of dLVP. Treatment with atenolol also showed a modest protective effect. Data from seven rat hearts in each group are expressed as mean ± S.E. (*P < .05 versus saline, P < .05 versus atenolol).

MDA Levels in Myocardium. As shown in Fig. 2, MDA levels in myocardium increased significantly after ischemia-reperfusion (P < .05 versus sham controlhearts; n = 6). Pretreatment of rats with AS-ODNs and atenololattenuated the increase in MDA levels in the myocardium (bothP < .05 versus saline pretreatment; n = 7 each group). As expected,IN-ODNs did not affect MDA levels in myocardium.

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Fig. 2. MDA levels in the myocardium in each group rats. MDA levels increased markedly after ischemia-reperfusion in the saline-treated rat hearts. Treatment with AS-ODNs and atenolol, but not with IN-ODNs, attenuated the increase in MDA levels. Data from seven rat hearts in each group are shown as mean ± S.E. (*P < .05 versus sham control, P < .05 versus saline).

, sham control; $black-square$ , saline + I/R;

, AS-ODNs + I/R;

, IN-ODNs + I/R;

, atenolol + I/R.

Expression of $beta$ ₁-AR Protein and mRNA in Myocardium. Western analysis of the control continuously perfused hearts showed a distinct $beta$ ₁-AR protein band of 65 kDa. A similar molecularmass band was observed in hearts from saline-, AS-ODNs-, IN-ODNs-,and atenolol-treated rat hearts. The $beta$ ₁-AR protein band was verydense in the saline-treated rat hearts, indicating up-regulationof the protein during ischemia-reperfusion. Treatment of ratswith AS-ODNs abolished the ischemia-reperfusion-mediated increasein $beta$ ₁-AR protein expression. Notably, treatment of rats with IN-ODNsor atenolol had no effect on the level of $beta$ ₁-AR protein. Resultsof a representative experiment and summary of data from threeseparate experiments are presented in Fig. 3.

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Fig. 3. Representative Western blot analysis of $beta$ ₁-AR protein expression in myocardium from each group of rats (top). Please note that $beta$ ₁-AR protein in the saline-treated rat hearts increased (P < .01) after ischemia-reperfusion. Treatment with AS-ODNs decreased (P < .01) the enhanced $beta$ ₁-AR protein in the myocardium after ischemia-reperfusion, whereas treatment with IN-ODNs or atenolol had no effect. Summary of data (mean ± S.E.) from three separate rats in each group (bottom). See text for details of the methodology.

Ischemia-reperfusion also resulted in an increase of mRNA for $beta$ ₁-AR signal (adjusted for GAPDH signal) in the myocardium ofsaline-treated rats, as determined by RT-PCR. Pretreatment ofrats with AS-ODNs attenuated the increase of mRNA for $beta$ ₁-AR inmyocardium, but mRNA level for $beta$ ₁-AR in the myocardium was notsignificantly affected by treatment of rats with IN-ODNs or atenolol(Fig. 4).

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Fig. 4. Expression of $beta$ ₁-AR mRNA in myocardial tissue from each group of rat hearts. GAPDH was amplified as a reference for quantitation of $beta$ ₁-AR mRNA. Please note that $beta$ ₁-AR mRNA expression markedly increased in the myocardium after ischemia-reperfusion in the saline-treated rat hearts. Administration of AS-ODNs inhibited the increased expression of $beta$ ₁-AR mRNA after ischemia-reperfusion. IN-ODNs and atenolol had no effect. The RT-PCR analysis (top) is representative of each group. Summary of data (mean ± S.E.) from three separate rats in each group (bottom). See text for details of the methodology.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

This study was designed to examine the protective role of AS-ODNs directed at $beta$ ₁-AR mRNA against cardiac dysfunction aftera brief period of ischemia-reperfusion. We also compared the effectsof pretreatment with AS-ODNs with a selective $beta$ ₁-AR blocker atenololin this process. This study showed that ischemia for 30 min followedby reperfusion for 30 min resulted in significant cardiac dysfunctionand lipid peroxidation in the saline-treated rat hearts. Furthermore,ischemia-reperfusion was associated with a marked up-regulationof $beta$ ₁-AR expression in the hearts. Pretreatment of rats with atenololdecreased cardiac dysfunction after ischemia-reperfusion, butdid not affect the expression of $beta$ ₁-AR protein or mRNA in myocardium.However, pretreatment of rats with $beta$ ₁-AS-ODNs not only preservedcardiac function and decreased lipid peroxidation after ischemia-reperfusionbut also prevented the up-regulation of $beta$ ₁-AR protein and mRNAexpression in the ischemic-reperfused myocardium. The effectsof AS-ODNs on cardiac function appeared to be equivalent to thoseof the commonly used $beta$ ₁-AR blocker atenolol, but AS-ODNs weresuperior to atenolol in inhibiting the enhanced expression of $beta$ ₁-AR induced by ischemia-reperfusion.

There is a generalized stimulation of the sympathetic nervous system during ischemia, perhaps a compensatory response in anattempt to preserve cardiac function. Accordingly, catecholaminelevels increase in both plasma and myocardium after myocardialischemia (Abrahamsson et al., 1983; Rona, 1985; Richard et al.,1994), but the increased catecholamine concentrations have thepotential to contribute to increased excitability of myocardium,resulting in arrhythmia (Mukherjee et al., 1979; Maisel et al.,1985, 1987; Ohyanahi et al., 1988; Strassere et al., 1990). Thereis also an increase in the sensitivity of $beta$ ₁-ARs during myocardialischemia (Strassere et al., 1990). This coupled with increasedcirculating and myocardial catecholamine concentrations can exacerbatecardiac injury anddysfunction.

Rohrer et al. (1996, 1998) found that inhibition of $beta$ ₁-AR expression, based on studies in $beta$ ₁-AR knockout mouse, significantlylimits the heart rate and blood pressure response during gradetreadmill exercise. This observation clearly demonstrates that $beta$ ₁-AR is important in $beta$ ₁-AR functional regulation in heart. Itis generally accepted that activation of $beta$ -AR is the first elementin the signal transduction chain mediating sympathetic stimulationof the heart (Gudermann et al., 1995). $beta$ ₁-AR, the dominant $beta$ -ARsubtype in the heart (Ungerer et al., 1993; Minneman et al., 1995),up-regulates cardiac function by mediating adenylyl cyclase activity(Thandroyen et al., 1986; Böhm, 1995). Several experimental studieshave shown an up-regulation in $beta$ ₁-ARs, but not $beta$ ₂-ARs, duringacute ischemia-reperfusion (Maisel et al., 1985; Karliner et al.,1989; Persad et al., 1998). Ihl-Vahl et al. (1995) conclusivelydemonstrated a rapid up-regulation of $beta$ -AR mRNA during acute myocardialischemia; this up-regulation is subtype selective with a specificincrease in mRNA level for $beta$ ₁-ARs, but not for $beta$ ₂-ARs. They alsoshowed that the increase of $beta$ ₁-AR mRNA is ischemia time-dependent.Notably, the regulation of $beta$ ₁-ARs is different in chronic heartfailure from that in myocardial ischemia. The number of $beta$ ₁-ARsis diminished in heart failure and is increased in acute myocardialischemia.

Pretreatment of animals with $beta$ -AR blockers does not affect ischemia-reperfusion-induced increase in $beta$ ₁-AR mRNA level. Thispretreatment effect became evident in this study wherein treatmentwith atenolol did not affect $beta$ ₁-AR protein (Western analysis)and mRNA (RT-PCR) levels. Other studies also have shown that $beta$ ₁-ARblockers do not block the expression of $beta$ ₁-AR expression (Aaronset al., 1980; Aarons and Molinoff, 1982; Heilbrunn et al., 1989).However, our study clearly demonstrates that $beta$ ₁-AS-ODN blocksthe up-regulation of $beta$ ₁-ARs. We also observed that therapy witha single dose of AS-ODNs prevented the increase in $beta$ ₁-AR protein.AS-ODNs were given 4 days before excising the heart to permitincorporation of the AS into the $beta$ ₁-AR mRNA and inhibition of $beta$ ₁-AR at transcriptional level. Atenolol was given 6 h beforeexcising the heart because of short half-life of this chemical $beta$ ₁-AR blocker. A previous study in the SHR from our laboratoryindeed demonstrated that the $beta$ ₁-AS-ODNs used in this study decreases $beta$ ₁-AR mRNA translation in the hearts for up to 20 days (Zhanget al., 2000). The reduction in mRNA could result from inhibitionof transcription or induction of RNaseH.

Although chemical $beta$ -AR blockers are effective in the therapy of ischemic heart disease and are widely used in the short- andlong-term management of patients with myocardial ischemia (Yusufet al., 1985), these agents have several undesirable side effectsrelated to their effects on central nervous system, peripheralvascular resistance, and tracheobronchial tree. Even the selective $beta$ ₁-AR blockers, such as atenolol, lose their cardioselectivityat moderate doses. In addition, these agents need to be takenfrequently, at least once daily, due to their short half-life.Furthermore, chemical $beta$ -AR blockers do not influence $beta$ -ARs atgenomic level. Gene therapy, such as AS-ODNs directed at $beta$ ₁-ARmRNA, have unique effects. A previous study from our group (Zhanget al., 2000) showed that a single i.v. injection of $beta$ ₁-AS-ODNsdelivered with cationic liposomes markedly decreased blood pressurefor 20 days with maximum drop of 38 mm Hg and without significantbradycardia in SHR. However, $beta$ ₁-AR density in SHR hearts was significantlydecreased for 18 days with maximum reduction of 47% on day 4,33% on day 10, and 29% on day 18, but there was no effect on $beta$ ₂-ARdensity. Quantitative autoradiography indicated that the administrationof $beta$ ₁-AS-ODNs decreased $beta$ ₁-AR density in cardiac ventricles andrenal cortex without any effect on distribution of $beta$ -ARs in brain.The demonstration in this study of preservation of cardiac functionand protection of myocardium from lipid peroxidation during ischemia-reperfusionwith a single dose of $beta$ ₁-AS-ODNs with highly selective effectson the expression of $beta$ ₁-AR in the myocardium complements the observationsin SHR. Importantly, IN-ODNs, used as control for $beta$ ₁-AS-ODNs,did not show any of these effects. These observations in a ratmodel are consistent with our hypothesis that up-regulation of $beta$ ₁-AR expression is pathogenetically involved in cardiac dysfunctionduring ischemia-reperfusion. We suggest that the results of thisstudy set the stage for conduct of similar studies in other modelsof myocardial ischemia and eventually inhumans.

In this study, ischemia-reperfusion-induced cardiac dysfunction was evaluated by the measurement of CPP, LVEDP, and dLVP.These indices of myocardial dysfunction have been used in severalstudies in the isolated heart model of global ischemia-reperfusion(Yang et al., 1993, 1997, 1998; Kokita et al., 1998; Ozden etal., 1998). Isolated rat, rabbit, or guinea pig heart models providean inexpensive and reproducible method to evaluate cardiac functionand myocardial metabolic alterations during ischemia-reperfusion.We and others have used this model extensively to study regulationof variety of receptors and modulation of cardiac function byagents acting on different receptors (Neely and Rovetto, 1975;Lu et al., 1990; Yang et al., 1993, 1997, 1998; Kokita et al.,1998). In the isolated beating heart, cardiac function can beassessed independent of the influence of circulating blood cellsand hormones, which may be considered an important advantage ofthismodel.

MDA, a lipid peroxidation product, has been used as an index of tissue injury after ischemia-reperfusion by several investigators(Kokita et al., 1998; Ozden et al., 1998). Increase in myocardialMDA was attenuated by the use of AS-ODNs in this study. One ofthe limitations of this study is absence of clear demonstrationof AS-ODNs taken up by the heart. Nonetheless, several studieshave shown substantial uptake and relatively good stability ofphosphorothioate deoxynucleotides in cardiac tissues (Agrawalet al., 1991; Raynaud et al., 1997). Our previous study (Zhanget al., 2000) with the AS-ODNs used in this study showed a dramaticreduction in $beta$ ₁-AR density in the myocardium. Furthermore, wenow show that AS-ODNs decrease the up-regulation of $beta$ ₁-AR mRNAand protein in the heart during ischemia-reperfusion; thus stronglysuggesting that the AS-ODNs were taken up by the myocardium. Becausethis study was carried out in an isolated heart preparation, theperipheral effects of AS-ODNs were not taken into account. Assuch, the role of peripheral factors in the preservation of cardiacfunction cannot be ascertained from thisstudy.

In summary, this study is the first report on the amelioration of cardiac dysfunction and myocardial injury induced by ischemia-reperfusionin the isolated rat heart with a single i.v. injection of AS-ODNsdirected at $beta$ ₁-AR mRNA. This study also provides evidence thatthe AS-ODNs can block the augmented expression of $beta$ ₁-AR in theischemic myocardium. The cardiac dynamic effects of AS-ODNs appearto be equivalent to those of atenolol in the isolated rat heartmodel of ischemia-reperfusion.

	Footnotes

Accepted for publication April 4, 2000.

Received for publication February 8, 2000.

¹ This study was supported in part by a Merit Review Award from the Department of Veterans Affairs and a National Institutesof Health MERITAward.

Send reprint requests to: J. L. Mehta, M.D., Ph.D., Professor of Medicine and Physiology, University of Florida, Department of Medicine, Box 100277, JHMHC, Gainesville, FL 32610. E-mail: mehta{at}medmac.ufl.edu

	Abbreviations

$beta$ -AR, $beta$ -adrenoreceptor; AS-ODN, antisense-oligodeoxynucleotide; $beta$ ₁-AS-ODN, antisense-oligodeoxynucleotide directed at $beta$ ₁-AR mRNA; SHR, spontaneously hypertensive rats; IN-ODN, inverted-oligodeoxynucleotide; DOTAP, 1,2-bis(oleoyloxy)-3-(trimethylammonio)propane; DOPE, L- $alpha$ -dioeoyl phosphatidylethanolamine; CPP, coronary perfusion pressure; LVEDP, left ventricular end diastolic pressure; LVSP, left ventricular systolic pressure; dLVP, developed left ventricular pressure; RT-PCR, reverse transcription-polymerase chain reaction; MDA, malondialdehyde.

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