The thyroid hormone analog DITPA restores Ito in rats after myocardial infarction

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The thyroid hormone analog DITPA restores I_to in rats after myocardial infarction

Alan D. Wickenden, Roger Kaprielian, Xiao-Mang You, and Peter H. Backx

Departments of Physiology and Medicine and The Center for Cardiovascular Research, University Health Network, University of Toronto, Toronto, Ontario, Canada M5G 2C4

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Previous studies have established that reductions in repolarizing currents occur in heart disease and can contribute to life-threateningarrhythmias in myocardium. In this study, we investigated whetherthe thyroid hormone analog 3,5-diiodothyropropionic acid (DITPA)could restore repolarizing transient outward K⁺ current (I_to) density and gene expression in rat myocardium aftermyocardial infarction (MI). Our findings show that I_to densitywas reduced after MI (14.0 ± 1.0 vs. 10.2 ± 0.9 pA/pF, sham vs.post-MI at +40 mV). mRNA levels of Kv4.2 and Kv4.3 genes weredecreased but Kv1.4 mRNA levels were increased post-MI. Correspondingchanges in Kv4.2 and Kv1.4 protein were also observed. Chronictreatment of post-MI rats with 10 mg/kg DITPA restored I_to density(to 15.2 ± 1.1 pA/pF at +40 mV) as well as Kv4.2 and Kv1.4 expressionto levels observed in sham-operated controls. Other membrane currents(Na⁺, L-type Ca²⁺, sustained, and inward rectifier K⁺ currents) were unaffected by DITPA treatment. Associated withthe changes in I_to expression, action potential durations (current-clamprecordings in isolated single right ventricular myocytes and monophasicaction potential recordings from the right free wall in situ)were prolonged after MI and restored with DITPA treatment. Ourresults demonstrate that DITPA restores I_to density in the settingof MI, which may be useful in preventing complications associatedwith I_todownregulation.

action potential; transient outward current; Kv4.2; Kv4.3; Kv1.4; 3,5-diiodothyropropionic acid

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

VENTRICULAR REMODELING is a well-recognized response to myocyte loss such as occurs after a myocardial infarction (MI) (33).The remodeling process involves concentric myocyte hypertrophyand altered gene expression in surviving myocytes in both leftand right ventricles (1, 7, 37, 48). An important featureof the remodeling process is action potential prolongation secondaryto reductions in the transient outward K⁺ current (I_to) density, which can increase intracellular Ca²⁺ concentration ([Ca²⁺]_i) transient amplitude (21) and thus enhance contractilityof the compromised heart (44). On the other hand, chronic elevationsof [Ca²⁺]_i associated with action potential prolongation may potentiatehypertrophic signaling cascades and lead to maladaptive gene expression,thereby overriding any short-term benefits and perhaps contributingto left ventricular dysfunction and failure (44). Action potentialprolongation can also be arrhythmogenic, and, as such, this compensatorymechanism may predispose the heart to arrhythmias and sudden cardiacdeath (40).

Given the potential contribution of I_to downregulation and action potential prolongation to the pathogenesis of heart failure,normalization of I_to in the hypertrophied heart might be usefulin the treatment of this condition. In this regard, thyroid hormonecan increase the expression of genes encoding for I_to (17, 39,45), alter the biophysical properties of I_to (38, 39, 45),and abbreviate action potential duration (4). The effects ofthyroid hormone, however, are complicated by a plethora of noncardiaceffects that may limit the beneficial effects of this agent (14).In this study, we chose to examine the effects of the thyroidhormone analog 3,5-diiodothyropropionic acid (DITPA) on I_to expressionin the postinfarcted rat heart, because this analog binds to nuclearthyroid hormone receptors and can alter the transcription of triiodothyronine-responsivegenes (31) with apparently only minor effects on heart rateand metabolism compared with thyroid hormone itself (25, 32).Our results show that chronic treatment of infarcted hearts withDITPA restored I_to expression and hastened repolarization to levelsobserved in noninfarcted hearts. A preliminary report of our datahas appeared (43).

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Left anterior descending coronary artery ligation procedure. The left anterior descending (LAD) ligation procedure was performed on male Lewis-Brown Norwegian (LBN-F1 strain, Harlan,Indianapolis, IN) rats (220 g, 10-12 wk of age) as previouslydescribed (30). Briefly, animals were anesthetized with ketaminehydrochloride (45 mg/kg) and xylazine (5 mg/kg) intraperitoneally.Once an adequate depth of anesthesia was achieved, animals wereintubated with a 14-gauge polyethylene (PE) catheter and ventilatedwith room air using a small animal ventilator (model 683, HarvardApparatus, Boston, MA). A left thoracotomy was performed in thefifth intercostal space, and the pericardium was opened. The proximalleft coronary artery under the tip of the left atrial appendagewas encircled and ligated using a 6-0 silk suture. The muscleand skin were closed in layers. For sham-operated animals, theleft coronary artery was identified and encircled but not ligated,and the muscle and skin layers were closed similarly. The experimentaland animal care protocol was approved by the Committee on AnimalResearch at the Toronto General Hospital and was performed inaccordance with the "Position of the American Heart Associationon Research Animal Use." After the surgical procedure was completed,rats were housed in pairs in a climate-controlled environmentat an ambient temperature of 21°C with a 12:12-h light-dark cycleand were given water and standard rat chow adlibitum.

Five weeks after the LAD ligation procedure was completed, animals were treated with either DITPA (3.75 or 10 mg/kg body wt)or NaCl (0.9 g/100 ml). Stock solutions containing 3.75 or 10mg/ml DITPA (Sigma Chemical, St. Louis, MO) were prepared as previouslydescribed (32) and diluted in 0.9 g/100 ml NaCl. The doses ofDITPA used in the present study were previously shown to exertbeneficial effects on contractile performance in animal modelsof cardiac hypertrophy and failure (25, 32). Animals receiveddaily subcutaneous injections for 21 days. Eight weeks after thesham or LAD ligation procedure was completed, the animals werekilled and mRNA levels, protein levels, current densities, andaction potentials were measured using the methods described below.In addition, the left ventricular free wall was carefully dissectedfrom base to apex and along the border edge of the right ventricle.Infarct size was determined by measuring the infarcted area onthe epicardial surface and was expressed as a percentage of thearea of the left ventricular freewall.

The right ventricle was chosen for these studies because myocyte hypertrophy and the altered gene expression that occurs inthe right ventricle after left-sided infarctions (1, 3,37, 48) may be important prognostic determinants in heartdisease (49). Furthermore, isolation of myocytes from the rightventricle avoids potential problems associated the presence ofa large scar in the infarcted left ventricle. We chose to makeour recordings 8 wk post-MI because previous characterizationof this model established that this time point represents a phaseof compensated hypertrophy, rather than failure (15), and wouldencompass the period during which there is an increased incidenceof arrhythmias (35). Therefore, 8 wk postinfarction is a relevanttime point at which to study mechanisms with potential relevanceto hypertrophy andarrhythmogenesis.

Monophasic action potential and hemodynamic studies. For monophasic action potential recordings, isolated hearts were retrogradely perfused with a solution containing (in mM)140 NaCl, 5.4 KCl, 10 HEPES, 1 MgCl₂, and 10 D-glucose, with pHbalanced to 7.4 with NaOH at 37°C. Ca²⁺ was excluded from this solution to eliminate possible artifactsassociated with wall motion. A custom-made contact probe was usedto record monophasic action potentials as previously described(12). The monophasic action potential probe consisted of a bipolarelectrode (0.8 mm in diameter) of sintered Ag-AgCl pellet (E255,In Vivo Metric, Healdsburg, CA) encased in PE tubing (with a totalouter diameter of 1.3 mm). The monophasic action potential probewas gently pressed against the centrolateral surface of the rightventricular wall with constant pressure to eliminate electricalartifacts associated with slippage or uneven contact (13). Monophasicaction potentials were filtered at 1 kHz and recorded at 10kHz.

For hemodynamic assessment, animals were anesthetized with ketamine hydrochloride (45 mg/kg) and xylazine (5 mg/kg) injectedintraperitoneally. The right carotid artery was cannulated withPE-200 tubing that was drawn to a diameter of ~100-200 µm. Thetubing was attached to a pressure transducer to record hydrostaticpressure. The catheter was advanced into the aorta and then intothe left ventricle. From the pressure traces, left ventricularend-diastolic (LVEDP) and end-systolic pressure (LVESP) as wellas the maximal derivatives of pressure (i.e., +dP/dt and $-$ dP/dt)weremeasured.

Isolation of right ventricular myocytes. The procedure used for isolation of rat ventricular myocytes was described in detail previously (21). Heparinized (500 Uip) rats were anesthetized with pentobarbital sodium (75 mg/kgip). Once an adequate depth of anesthesia was achieved, the heartswere quickly removed and retrogradely perfused for ~3 min witha Ca²⁺-containing Tyrode solution of the following composition (in mM):140 NaCl, 5.4 KCl, 10 HEPES, 1 MgCl₂, 1 CaCl₂, and 10 D-glucose,with pH balanced to 7.4 with NaOH at 37°C. The heart was thenperfused with Ca²⁺-free Tyrode solution for 5 min before the heart was digestedwith the same solution containing collagenase (type II, 0.55 mg/ml,Boehringer-Mannheim) and protease (type XIV, 0.05 mg/ml, SigmaChemical) for 8-9 min. The enzyme solution was subsequently removedby perfusion with a Kraftbrühe (high K⁺) solution containing (in mM) 120 K-glutamate, 20 KCl, 20 HEPES,1 MgCl₂, 0.3 K-EGTA, and 10 D-glucose for 5 min. All solutionswere prebubbled with 100% O₂ for 5 min. After the enzyme washoutperiod, the atria and blood vessels were removed and the ventricleswere separated. The right ventricular free wall was dissectedfree from the remainder of the ventricle. Myocytes were mincedand mechanically agitated in a high-K⁺ solution containing BSA (0.02% wt/vol). Myocytes were then filteredthrough a nylon mesh and resuspended in a Kraftbrühe solutionwith 50 mg/ml gentamicin. Ca²⁺-tolerant, quiescent rod-shaped cells with clear, regular cross-striationswere selected for electrophysiological recordings. Cells weretransferred into a perfusion bath situated on the stage of aninverted microscope and perfused with recording solution at arate of 1-2 ml/min.

Electrophysiological measurements in right ventricular myocytes. Current densities [I_to, inward rectifier K⁺ current (I_K1), sustained current (I_sus), Na⁺ current (I_Na), L-type Ca²⁺ current (I_Ca,L)] and action potentials were measured using thewhole cell patch-clamp recording method (18) under voltage-and current-clamp conditions with an Axopatch 200A amplifier (AxonInstruments, Foster City, CA) as described in detail previously(21). When pipettes were filled with intracellular solution,pipette tip resistances were typically 2-3 M $Omega$ . Series resistancecompensation ranged between 60 and 90%. After membrane rupture,we estimated the cell capacitance by integrating the area of thecapacitance transients after a 5-mV step from a holding potentialof $-$ 80mV.

For K⁺ currents, myocytes were superfused with a standard Tyrode solution containing (in mM) 140 NaCl, 1 MgCl₂, 10 HEPES, 4KCl, 1 CaCl₂, and 10 D-glucose, with pH adjusted to 7.4 with NaOH.Intracellular solutions for K⁺ currents and action potentials contained (in mM) 130 K-aspartate,20 KCl, 5 EGTA, 5 NaCl, 10 HEPES, and 5 MgATP, with pH adjustedto 7.2 with Trizma base. Action potentials were also recordedwith an intracellular solution containing 30 mM 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraaceticacid (BAPTA) and a modified Tyrode solution containing 0.1 mMCaCl₂. Recordings were not corrected for a liquid junction potentialof approximately $-$ 8mV.

To isolate I_to, we used prepulses to $-$ 40 mV for 30 ms to inactivate I_Na, and 0.3 mM CdCl₂ was added to block I_Ca,L. AlthoughCdCl₂ has been reported to shift I_to channel gating (2, 46),it was the preferred choice to block I_Ca,L because organic Ca²⁺ channel blockers have been shown to affect I_to amplitude andkinetics (22). I_to was defined as the peak current (I_peak) elicitedby 500-ms voltage steps in the range from $-$ 30 to +70 mV minusthe steady-state current (I_sus) remaining at the end of the 500-msvoltagestep.

To measure I_K1, we elicited a series of 500-ms steps from $-$ 130 to 0 mV (in 10-mV increments) in the presence and absence of0.3 mM BaCl₂. I_K1 was defined as the Ba²⁺-sensitive current component. To measure I_Ca,L, we replaced theKCl in the Tyrode solution with equimolar CsCl while intracellularsolutions contained (in mM) 150 CsCl, 10 HEPES, 1 MgCl₂, 5 EGTAand 5 MgATP, with pH adjusted to 7.2 with CsOH. A brief prepulseto $-$ 40 mV for 100 ms was used to inactivate I_Na. I_Ca,L was estimatedas peak Cd²⁺-sensitive current in response to 500-ms voltage steps from $-$ 60to +70 mV. To measure I_Na, we superfused myocytes with a solutioncontaining (in mM) 5 NaCl, 125 triethylamine hydrochloride (TEA-Cl),1 MgCl₂, 20 HEPES, 5 CsCl, 1 MnCl₂, and 10 D-glucose, with pHadjusted to 7.4 with CsOH. Intracellular solution contained (inmM) 125 CsCl, 20 TEA-Cl, 10 HEPES, 10 EGTA, and 5 MgATP, withpH adjusted to 7.2 with CsOH. A series of 50-ms voltage stepswas applied between $-$ 80 and +10 mV in 5-mV increments from a holdingpotential of $-$ 100 mV. A P/4 protocol was used for leak and capacitancesubtraction in the I_Na experiments. All experiments were performedat room temperature (19-21°C).

Preparation of total RNA from the right ventricle and RNase protection assays. Rat right ventricles and brains were isolated, rinsed briefly in a standard Tyrode solution, and snap-frozen in liquid N₂.Ventricular tissue was powdered and RNA extracted by the one-stepacid guanidinium-phenol method (8). The concentration of RNAwas measured spectrophotometrically and confirmed by agarose gelelectrophoresis. Gels were loaded with 10 µg of total RNA obtainedfrom three hearts per group. RNase protection assays were performedusing an RPAII Ribonuclease Protection Assay Kit (Ambion, Austin,TX) as previously described (21, 42, 45). The Kvx probesfor RNase protection assays were kindly provided by Dr. DavidMcKinnon (State University of New York at Stony Brook, Stony Brook,NY) and have been described previously (10, 11, 42). Thecyclophilin probe was purchased from Ambion. The myosin heavychain (MHC) probe was kindly supplied by Drs. J. N. Tsoporis andT. G Parker (University of Toronto, Toronto, ON, Canada) and wasalso described previously (41). Abundance of mRNA transcriptswas quantified by densitometry (Bio-Rad GS670 Imaging densitometer).Signals were normalized to a cyclophilin internal standard toensure that findings were not influenced by minor variations inloading.

Isolation of protein from the right ventricle. Rat right ventricles or brains from three rats per group were quickly rinsed, frozen in liquid N₂, and stored at $-$ 70°C beforeisolation of membrane proteins. Frozen tissue was homogenizedin 10 volumes of 0.3 M sucrose and 30 mM histidine, and the resultinghomogenate was then centrifuged at 3,000 g for 15 min. The supernatantwas collected and recentrifuged at 45,000 g for 1 h to precipitatemembrane protein. The membrane pellet was resuspended in 1% TritonX-100 and 50 mM Tris (pH 6.8), left on ice for 1 h, and then centrifugedat 14,000 g for 15 min. The final supernatant was saved for proteinassay by the Lowry method, and Western blot analysis was performed.All solutions in this procedure were chilled on ice and containedprotease inhibitors (0.1 mM phenylmethylsulfonyl fluoride and5 µg/ml each of aprotinin, leupeptin, antipain, andpepstatin).

Preparation of anti-Kv1.4 and anti-Kv4.2 antibodies. Anti-Kv1.4 and anti-Kv4.2 antibodies were kindly supplied by Dr. O. T. Jones (Department of Pharmacology, University of Toronto).The procedure by which the anti-Kv1.4 and anti-Kv4.2 antibodieswere produced was described in detail previously (42, 45).

Western blot analysis. For Western blot analysis, 50-100 µg of total heart protein and 10-20 µg of total brain protein were resolved on a 10% SDS-PAGEgel and transferred to a polyvinylidene fluoride membrane. Afterthe transfer, the membrane was rinsed with Tris-buffered saline(TBS; 150 mM NaCl and 20 mM Tris, pH 7.5). Blots were blockedwith 10% Carnation Instant milk powder in TBS for 1 h and probedwith anti-Kv antibodies diluted in 3% milk-TBS overnight at 4°C.After being washed with TBS to remove excess primary antibody,the blots were incubated with secondary antibody (donkey anti-rabbitIgG conjugated to horseradish peroxidase, Amersham) in blockingbuffer for 1 h. The membrane was washed again with TBS containing0.05% Tween 20 and 1% Triton X-100 and developed by enhanced chemiluminescence(ECL reagent, Amersham). Gel loading was checked by staining totalproteins with Ponceau S, and molecular weights were determinedusing prestained markers (Kaleidoscope, Bio-Rad). Western blotswere repeated two to three times per sample. Protein abundancewas quantified by densitometry (Bio-Rad GS670 Imagingdensitometer).

Statistical analysis. All data are expressed as means ± SE. Data were collected from right ventricles and single right ventricular myocytes isolatedfrom three to eight hearts per group. For RNase protection assays,the arbitrary densitometric units were normalized to the valueof the cyclophilin gene. Statistical analysis was done using one-wayANOVA from the SPSS software program (version 7.0 for Windows).When ANOVA showed statistical significance by F test, intergroupcomparisons were made using the Student-Newman-Keuls procedure.P < 0.05 was consideredsignificant.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Effect of DITPA after MI. In our study, we analyzed rats with infarct sizes >30% (range 30-60%). Table 1 shows some of the general characteristicsand hemodynamic parameters after MI and DITPA treatment. Infarctsizes were comparable among vehicle-treated post-MI and DITPA-treatedpost-MI animals [49.9 ± 4.1% (n = 13), 52.7 ± 3.9% (n = 4), and53.2 ± 3.8% (n = 13) for groups treated with vehicle, 3.75 mg/kgDITPA, and 10 mg/kg DITPA, respectively]. Daily subcutaneous injectionswith DITPA had no effect on body weight. After 21 days of DITPAtreatment, body weight increased by 5.6 ± 0.8% (n = 14) in vehicle-treatedpost-MI animals, by 7.1 ± 1.6% (n = 8) in 3.75 mg/kg DITPA-treatedpost-MI animals, and by 4.2 ± 1.5% (n = 14) in 10 mg/kg DITPA-treatedpost-MI animals. Lung wet weight-to-dry weight ratios were slightlyincreased in vehicle-treated post-MI animals compared with sham-operatedanimals, but this did not reach statistical significance [4.4± 0.2 (n = 11) vs. 3.9 ± 0.2 (n = 7); P = 0.1] and were unchangedin DITPA-treated post-MI animals [3.75 mg/kg DITPA: 3.8 ± 0.4(n = 4); 10 mg/kg DITPA, 4.2 ± 0.2 (n = 7); P > 0.05].

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Table 1. General characteristics and hemodynamic parameters after myocardial infarction and DITPA treatment

The effects of MI and DITPA treatment on hemodynamic properties of the hearts are summarized in Table 1. The most notablechange was in LVEDP, which was elevated after MI with or withoutDITPA treatment. Changes in the rate of contraction (+dP/dt) wereunaffected after MI or DITPA treatment. The rate of relaxation( $-$ dP/dt) was significantly (P < 0.05) decreased after MI and wasmodestly restored after DITPA treatment. The lack of significancein these parameters might be explained by the variations in infarctsizes (33).

Effect of DITPA on Ito. From this point, right ventricular myocytes derived from sham-operated animals, vehicle-treated post-MI animals, 3.75 mg/kgDITPA-treated post-MI animals, and 10 mg/kg DITPA-treated post-MIanimals are referred to as sham myocytes, post-MI myocytes, 3.75mg/kg DITPA post-MI myocytes, and 10 mg/kg DITPA post-MI myocytes,respectively. Figure 1 shows representative normalized whole cellvoltage-clamp records measured from sham (Fig. 1A), post-MI (Fig.1B), 3.75 mg/kg DITPA post-MI (Fig. 1C), and 10 mg/kg DITPA post-MImyocytes (Fig. 1D). Comparison of Fig. 1, A and B, shows thatpeak current density (I_peak) was reduced in post-MI myocytes comparedwith that in sham myocytes. Treatment with 3.75 mg/kg DITPA modestlyincreased I_peak (Fig. 1C), whereas 10 mg/kg DITPA restored I_peakto levels observed in sham-operated controls (Fig. 1D). I_to density-voltagerelationships are summarized in Fig. 1E. I_to density at +40 mVwas significantly reduced from 14.0 ± 1.0 pA/pF (n = 21) in shammyocytes to 10.2 ± 0.9 pA/pF (n = 41, P = 0.001) in post-MI myocytes.To assess whether the observed changes in I_to densities resultedfrom alterations in the channel gating or in maximal conductance,we also calculated conductance-voltage curves (see MATERIALS ANDMETHODS) from the data in Fig. 1. The estimated maximal wholecell transient outward channel conductance (G_max) was significantlyreduced from 127.9 ± 9.8 pS/pF (n = 21) in sham myocytes to 84.6± 7.8 pS/pF (n = 41; P = 0.002) in post-MI myocytes. As summarizedin Table 2, the midpoint of the conductance-voltage relationship(V_1/2 act) was shifted slightly in a hyperpolarizingdirection in post-MI myocytes compared with that of sham myocyteswithout differences in the slope factors for activation (k).

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Fig. 1. Effect of 3,5-diiodothyropropionic acid (DITPA) on transient outward (I_to) and sustained currents (I_sus) in right ventricular myocytes after myocardial infarction (post-MI). Normalized traces of I_to and I_sus elicited by 500-ms voltage steps from $-$ 40 to +60 mV (in 20-mV steps) from a holding potential of $-$ 80 mV were derived from sham (A), post-MI (B), 3.75 mg/kg DITPA post-MI (C), and 10 mg/kg DITPA post-MI myocytes (D). Horizontal bars indicate 0 pA/pF. Current-voltage (I-V) plots are shown for I_to (E) and I_sus (F) for sham, post-MI, 3.75 mg/kg DITPA post-MI, and 10 mg/kg DITPA post-MI myocytes. Myocytes were depolarized every 10 s. * P < 0.05, sham vs. post-MI myocytes; $Dagger$ P < 0.05, post-MI vs. 10 mg/kg DITPA post-MI myocytes.

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Table 2. Characteristics of the transient outward current after myocardial infarction and DITPA treatment

Treatment of post-MI animals with 3.75 mg/kg DITPA increased I_to density to 11.2 ± 0.8 pA/pF (+40 mV, n = 45; P = 0.56), whereas10 mg/kg DITPA treatment produced a marked increase in I_to densityto 15.2 ± 1.1 pA/pF (+40 mV, n = 45; P = 0.001) compared withpost-MI myocytes. Changes in G_max mirrored changes in I_to density.Compared with vehicle-treated post-MI animals, treatment with3.75 mg/kg DITPA increased G_max to 107.2 ± 8.3 pS/pF (n = 45)without reaching statistical significance (P > 0.05), whereas10 mg/kg DITPA significantly increased G_max to 133.0 ± 10.7 pS/pF(n = 45). Despite the changes in G_max, DITPA treatment had noeffect on V_{1/2 act} or k compared with vehicle treatment.Steady-state inactivation properties of I_to were not affectedafter MI or DITPA treatment, as summarized in Table 2.

Effect of DITPA on Kv4.2, Kv4.3, and Kv1.4 expression. To investigate the molecular basis for the effects of DITPA on I_to, we employed RNase protection assays to measure mRNA levelsof the "transient-outward like" K⁺ channel genes Kv1.4, Kv4.2, and Kv4.3 (10, 11). Because I_towas only marginally affected by 3.75 mg/kg DITPA, we only examinedthe effects of 10 mg/kg DITPA. To confirm that 10 mg/kg DITPAhad the expected effects on gene expression under our experimentalconditions, we examined the mRNA levels of $alpha$ -MHC and $beta$ -MHC becausethese genes are strongly regulated by hypertrophy and thyroidhormone (19). As shown in Fig. 2A, the ratio of $beta$ -MHC to $alpha$ -MHCincreased significantly after MI [sham: 0.48 ± 0.01 (n = 3) vs.post-MI: 1.79 ± 0.07 (n = 3); P < 0.01]. Consistent with previousresults (19), DITPA treatment reduced the ratio of $beta$ -MHC to $alpha$ -MHC [0.59 ± 0.02 (n = 3)] to levels similar to those measuredin sham-operated hearts (P > 0.05). Figure 2 also shows the resultsof RNase protection assays for cyclophilin as well as Kv4.2 (Fig.2B), Kv4.3 (Fig. 2C), and Kv1.4 (Fig. 2D) mRNA levels in rightventricle. Mean Kv4.2-to-cyclophilin mRNA ratios were reducedfrom 0.73 ± 0.03 (n = 3) in sham samples to 0.51 ± 0.02 (n = 3)in post-MI samples (P < 0.01). After DITPA treatment, Kv4.2 mRNAlevels were significantly (P < 0.01) greater than those in untreatedhearts [0.63 ± 0.01 (n = 3)], indicating that DITPA partiallyrestored Kv4.2 mRNA levels. Kv4.3-to-cyclophilin mRNA ratios werealso significantly decreased in vehicle-treated post-MI hearts[1.00 ± 0.06 (n = 3)] compared with sham samples [1.19 ± 0.05(n = 3); P < 0.05], but DITPA treatment did not reverse thesechanges [0.889 ± 0.002 (n = 3); P > 0.05]. As shown in Fig. 2D,Kv1.4 mRNA ratios were significantly (P < 0.01) increased in post-MIsamples [0.55 ± 0.03 (n = 3)] compared with sham samples [0.36± 0.04 (n = 3)]. DITPA treatment normalized Kv1.4 mRNA ratiosto levels observed in sham-operated hearts [0.37 ± 0.02 (n = 3);P > 0.05].

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Fig. 2. Effect of DITPA on genes encoding I_to and myosin heavy chain (MHC) in right ventricle. Left: representative comparison of mRNA levels are from sham (S1, S2, S3), post-MI (V1, V2, V3), and 10 mg/kg DITPA post-MI hearts (D1, D2, D3). Expression of $alpha$ - (top) and $beta$ -MHC (bottom) isoforms is shown in A. Expression of Kv (top) and cyclophilin-protected mRNA fragments (bottom) is shown in B-D. Right: mean changes in Kv mRNA and $beta$ -MHC-to- $alpha$ -MHC ratio normalized to cyclophilin mRNA levels in sham (open bars), post-MI (shaded bars), and 10 mg/kg DITPA post-MI. hearts (filled bars), respectively. * P < 0.05, sham vs. post-MI hearts; $dagger$ P < 0.05, sham vs. 10 mg/kg DITPA post-MI hearts; $Dagger$ P < 0.05, post-MI vs. 10 mg/kg DITPA post-MI hearts.

Because the level of RNA expression may not always be indicative of protein expression levels, we also measured protein levelsof Kv1.4 and Kv4.2 subunits. Kv4.3 protein was also measured butwas not reported because of rapid degradation of this proteinunder our experimental conditions. Figure 3A shows a representativeWestern blot of protein from adult rat brain (10 µg) and rightventricles probed with anti-Kv4.2 antibody. The antibody labeleda single band in all samples, with an approximate molecular massof 77 kDa. As summarized in Fig. 3B, the level of Kv4.2 proteinwas markedly reduced (P = 0.03) in the post-MI hearts comparedwith that in sham-operated hearts [sham: 0.53 ± 0.09 arbitraryunits (n = 3) vs. post-MI: 0.21 ± 0.04 arbitrary units (n = 3)].Figure 3B also shows that DITPA treatment of post-MI animals restoresKv4.2 protein [0.50 ± 0.04 arbitrary units (n = 3)] to levelsobserved in sham-operated animals, correlating well with electrophysiologicaland Kv4.2 mRNA studies. Figure 3C depicts a Western blot of thesame protein samples as shown in Fig. 3A, probed with anti-Kv1.4antibody, and shows two distinct bands, in both brain and myocyteprotein, as shown previously in adult and cultured neonatal ratventricular myocytes (42, 45). Consistent with the Kv1.4 mRNAmeasurements, Kv1.4 immunoreactivity increased significantly from0.43 ± 0.04 arbitrary units (P < 0.05) in sham-operated animals(n = 3) to 0.68 ± 0.15 arbitrary units in post-MI animals (n =3). After DITPA treatment, Kv1.4 protein levels were significantlyreduced below levels observed in sham-operated samples [0.224± 0.007 arbitrary units (n = 3); P < 0.001].

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Fig. 3. Effect of DITPA on Kv channel subunit immunoreactive proteins encoding I_to in right ventricle after MI. Blots show levels of Kv4.2 (A) and Kv1.4 proteins (C) from brain (Br), sham (S1, S2, S3), post-MI (V1, V2, V3), and 10 mg/kg DITPA post-MI hearts (D1, D2, D3). Bar graphs show mean changes in Kv4.2 (B) and Kv1.4 (D) in sham (open bars), post-MI (shaded bars), and 10 mg/kg DITPA post-MI hearts (filled bars). * P < 0.05, sham vs. post-MI hearts; $dagger$ P < 0.05, sham vs. 10 mg/kg DITPA post-MI hearts; $Dagger$ P < 0.05, post-MI vs. 10 mg/kg DITPA post-MI hearts.

Effect of DITPA on other ion currents. Given the effect of DITPA on I_to, we wanted to examine whether this agent could exert similar effects on other ionic currents.Figure 1F shows the current-voltage relationships for I_sus evaluatedat the end of a 500-ms depolarizing voltage step. At +40 mV, I_susdensity was not significantly different in post-MI myocytes [5.6± 0.3 pA/pF (n = 41)] from that in sham myocytes [6.4 ± 0.4 pA/pF(n = 21); P = 0.07]. Treatment with 3.75 mg/kg DITPA [6.0 ± 0.3pA/pF (n = 45); P = 0.06] and 10 mg/kg DITPA [7.0 ± 0.4 pA/pF(n = 45); P = 0.06] produced no changes in I_sus density comparedwith vehicle-treated controls. Figure 4 shows representative normalizedI_K1 currents recorded from sham (Fig. 4A), post-MI (Fig. 4B),3.75 mg/kg DITPA post-MI (Fig. 4C), and 10 mg/kg DITPA post-MImyocytes (Fig. 4D). Comparison of these figures demonstrates thatI_K1 was lower in all post-MI myocytes than in sham myocytes. I_K1density evaluated at $-$ 130 mV was decreased significantly (P =0.006) in post-MI myocytes [ $-$ 12.1 ± 0.8 pA/pF (n = 25)] comparedwith that in sham myocytes [ $-$ 15.7 ± 0.9 pA/pF (n = 25)]. Treatmentwith DITPA did not restore (P > 0.05) I_K1 density (Fig. 4E) tothat observed in sham myocytes [ $-$ 11.3 ± 1.0 pA/pF (n = 14) for3.75 mg/kg DITPA and $-$ 10.8 ± 1.0 pA/pF (n = 10) for 10 mg/kg DITPAevaluated at $-$ 130 mV]. Figure 5 shows representative normalizedCd²⁺-subtracted I_Ca,L traces recorded in sham (Fig. 5A), post-MI (Fig.5B), and 10 mg/kg DITPA post-MI (Fig. 5C) myocytes, with the current-voltagerelationship depicted in Fig. 5D. I_Ca,L density was unchangedafter MI [I_Ca,Ldensities evaluated at 0 mV were $-$ 6.1 ± 0.5 pA/pF(n = 17) and $-$ 5.4 ± 0.3 pA/pF (n = 26) in myocytes from sham andpost-MI myocytes, respectively; P > 0.05]. DITPA treatment didnot change I_Ca,L compared with vehicle-treated controls [I_Ca,Ldensity evaluated at 0 mV was $-$ 6.6 ± 0.4 pA/pF (n = 20); P > 0.05].I_Na density and the midpoints for steady-state inactivation (V_1/2 inact)were also unchanged (P > 0.05) after MI and 10 mg/kg DITPA treatment.I_Na density at $-$ 35 mV was $-$ 17.6 ± 1.1 (n = 21), $-$ 16.5 ± 1.5 (n= 15), and $-$ 15.0 ± 1.0 pA/pF (n = 11), and V_1/2 inactwas $-$ 94.7 ± 3.2 (n = 4), $-$ 93.9 ± 1.1 (n = 4), and $-$ 91.8 ± 4.8mV (n = 3), in sham, post-MI, and 10 mg/kg DITPA post-MI myocytes,respectively.

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Fig. 4. Effect of DITPA on inward (I_K1) rectifier current in right ventricular myocytes after MI. Normalized I_K1 traces were derived from sham (A), post-MI (B), 3.75 mg/kg DITPA post-MI (C), and 10 mg/kg DITPA post-MI myocytes (D). I_K1 traces were elicited by 500-ms voltage steps from $-$ 130 to $-$ 60 mV from a holding potential of $-$ 80 mV. Horizontal bars indicate 0 pA/pF. E: I_K1were normalized to membrane capacitance and plotted against voltage for sham, post-MI, 3.75 mg/kg DITPA post-MI, and 10 mg/kg DITPA post-MI myocytes. Steady-state current measured at end of test pulse in presence of Ba²⁺ (0.3 mM) was subtracted from current evoked at same voltage step in absence of Ba²⁺. Myocytes were depolarized every 10 s. * P < 0.05, sham vs. post-MI myocytes.

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Fig. 5. Effect of DITPA on L-type Ca²⁺ current (I_Ca,L) in right ventricular myocytes after MI. Representative normalized I_Ca,L were derived from sham (A), post-MI (B), and 10 mg/kg DITPA post-MI myocytes (C). Current traces show Cd²⁺-sensitive difference currents (0.3 mM CdCl₂) elicited by 500-ms voltage steps to $-$ 40, 0,+10, and +30 mV from a holding potential of $-$ 80 mV. Horizontal bars indicate 0 pA/pF. D: I_Ca,L density was plotted against voltage for sham, post-MI, and 10 mg/kg DITPA post-MI myocytes. Myocytes were depolarized every 5 s.

Effect of DITPA on action potential. Because DITPA treatment was able to normalize I_to density without affecting other current densities, we examined whether theincrease in I_to density in post-MI myocytes was associated withaction potential shortening. As shown in Fig. 6, action potentialsin sham myocytes typically had a spikelike appearance, whereasthe rate of repolarization in post-MI myocytes was slowed, resultingin a significant prolongation of action potential duration (APD)at both the 50% (APD₅₀) and 90% (APD₉₀) repolarization level [APD₅₀was 5.0 ± 0.8 (n = 21) and 12.6 ± 1.3 ms (n = 15), P < 0.05, whereasAPD₉₀ was 30.8 ± 3.5 (n = 21) and 55.7 ± 5.7 ms (n = 15), P <0.05, for sham and post-MI myocytes, respectively]. Both 3.75and 10 mg/kg DITPA treatment accelerated repolarization and shortenedAPD compared with vehicle-treated controls. The effect of 3.75mg/kg DITPA was most apparent for APD₅₀ [8.2 ± 0.7 ms (n = 16);P < 0.01], whereas 10 mg/kg DITPA significantly (P < 0.01) shortenedboth the APD₅₀ [8.0 ± 0.6 ms (n = 18)] and APD₉₀ [35.3 ± 3.2 ms(n = 16] compared with vehicle-treated controls. Resting membranepotentials in post-MI myocytes were significantly (P < 0.001)depolarized [ $-$ 71.1 ± 1.0 mV (n = 18)] compared with sham myocytes[ $-$ 76.0 ± 1.3 mV (n = 20)]. DITPA treatment had no effect on theresting membrane potential [ $-$ 69.2 ± 1.2 mV (n = 16) for 3.75 mg/kgDITPA post-MI and $-$ 71.1 ± 1.0 mV (n = 18) for 10 mg/kg DITPA post-MI;P > 0.05].

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Fig. 6. Effect of DITPA on action potentials in right ventricular myocytes after MI. Representative action potential traces were recorded from sham (A), post-MI (B), 3.75 mg/kg DITPA post-MI (C), and 10 mg/kg DITPA post-MI myocytes (D). Horizontal bars indicate 0 mV. Bar graphs show mean changes in action potential duration at 50% (APD₅₀; E) and 90% repolarization (APD₉₀; F) in sham, post-MI, 3.75 mg/kg DITPA post-MI, and 10 mg/kg DITPA post-MI myocytes. Action potentials were elicited by a brief (5 ms) suprathreshold injection of depolarizing current (2× threshold) applied at 0.1 Hz. * P < 0.05, sham vs. post-MI myocytes; $dagger$ P < 0.05, sham vs. 10 mg/kg DITPA post-MI myocytes; $Dagger$ P < 0.05, post-MI vs. 10 mg/kg DITPA post-MI myocytes; * P < 0.05, sham vs. 3.75 mg/kg DITPA post-MI myocytes.

It is conceivable that the changes in APD after DITPA treatment could result from changes in a number of currents during anaction potential. However, as shown above, the changes in APDwith DITPA treatment are not due to alterations in I_sus, I_K1,I_Ca,L, or I_Na. The APD measurements (Fig. 6) were performed underconditions in which [Ca²⁺]_i transients might not be entirely eliminated when 5 mM EGTAwas included in the pipette. Therefore, the changes in APD withDITPA could conceivably have resulted from differences in Na⁺/Ca²⁺ exchange currents (I_Na/Ca) secondary to alterations in [Ca²⁺]_i transients. Therefore, we also measured action potentials inthe presence of 30 mM BAPTA in the pipette and 0.1 mM externalCa²⁺to eliminate [Ca²⁺]_i transients (R. Kaprielian and P. H. Backx, unpublished observations).Under these conditions, the APD₅₀ [4.4 ± 0.8 (n = 6) and 10.5± 3.6 ms (n = 5) for sham and post-MI myocytes, respectively;P < 0.01] and APD₉₀ (27.7 ± 4.6 and 49.1 ± 7.8 ms for sham andpost-MI myocytes, respectively; P < 0.01) were prolonged afterMI. DITPA treatment (at 10 mg/kg) restored APD₅₀ [4.9 ± 0.7 ms(n = 6)] and APD₉₀ [31.2 ± 3.5 ms (n = 6)] to levels observedin shammyocytes.

To determine whether the changes in APD recorded in single cells under relatively nonphysiological conditions might be predictiveof changes occurring in the whole heart, we recorded monophasicaction potentials from the right ventricular wall in Langendorff-perfusedhearts at 37°C. Typical examples of monophasic action potentialsare shown in Fig. 7. Consistent with the single-cell electrophysiology,monophasic APD₅₀ [17.9 ± 1.2 (n = 13) and 24.8 ± 1.9 ms (n = 9);P < 0.01] and APD₉₀ [42.9 ± 2.1 (n = 13) and 52.5 ± 5.4 ms (n= 9); P < 0.01] were significantly prolonged after MI. DITPA treatment(at 10 mg/kg) normalized the monophasic APD in hearts from post-MIanimals to values similar to those observed in hearts from sham-operatedanimals [monophasic APD₅₀: 14.2 ± 0.8 ms (n = 9); monophasic APD₉₀:37.6 ± 1.1 ms (n = 9)].

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Fig. 7. Effect of DITPA on monophasic action potentials in right ventricular free wall after MI. Recordings were obtained from sham (A), post-MI (B), and 10 mg/kg DITPA post-MI hearts (C). Bar graphs show mean changes in APD₅₀ (D) and APD₉₀ (E) in sham, post-MI, and 10 mg/kg DITPA post-MI hearts. * P < 0.05, sham vs. post-MI hearts; $dagger$ P < 0.05, sham vs. 10 mg/kg DITPA post-MI hearts; $Dagger$ P < 0.05, post-MI vs. 10 mg/kg DITPA post-MI hearts.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Most previous studies of heart disease following left ventricular infarction have reported cellular, electrical, and mechanicalchanges in the right and left ventricles (1, 3, 21, 24,30, 35, 37). In our studies we examined the changes in I_toand APDs that occur in the right ventricle after MI of the leftventricle. The right ventricle was chosen for these studies becausechanges in the right ventricle are important determinants of theprognosis in heart disease (49) and isolation of myocytes fromthe right ventricle avoids potential problems associated the presenceof a large scar in the infarcted left ventricle. In addition,hypertrophic remodeling in the right ventricle exceeds that occurringin the noninfarcted left ventricle (data not shown). Alterationsin the right ventricle following loss of left ventricular myocytesas a result of infarction are not unexpected for a number of reasons.For example, reductions in left ventricular contractility willdirectly increase the load on the right ventricle. Left ventricularchanges can also affect right ventricular properties as a consequenceof direct mechanical coupling between the two ventricular chambers.Furthermore, neurohumoral activation following infarction willproduce circulating local factors that may affect both ventricles(1, 36, 37).

Effect of DITPA on I_to. Downregulation of I_to is consistently observed in human patients (27, 28) and in a variety of heart disease models (20,21, 24, 35). Consistent with previous observations (21,35), I_to density was reduced in myocytes from post-MI hearts,but this reduction only reached statistical significance at voltagesabove +30 mV. Our inability to detect significant changes in I_todensity at potentials below +30 mV is unclear but might resultfrom the relatively small current magnitude at these voltagescoupled with biological and experimental variability of the wholecell current measurements in myocytes. Alternatively, the lackof significant reduction in I_to at less positive potentials mightoriginate from the positive shift (about +5 mV) in the V_1/2of I_to activation observed in the post-MIgroup.

G_max and I_to were significantly reduced in post-MI myocytes. This decrease in G_max could result from either reductions inthe number of channels or changes in the maximum probability ofchannel opening, or both. However, the reductions in Kv4.2 andKv4.3 expression were very similar to those for G_max, suggestingthat reductions in channel density were primarily responsiblefor the decline in I_to density and G_max. These results are consistentwith previous studies showing that Kv4.2 and Kv4.3 are the majorcontributors to I_to in the adult rodent (11, 15, 21, 39,47). In contrast, the expression of the "fetal" K⁺ channel gene Kv1.4 was increased after MI, as reported previously(21, 45, 47), and similar to that observed in hypertensiverats (26). The significance of increases in Kv1.4 expressionremains unclear, but it is interesting to note that the directionalshifts in V_1/2 matched those expected from shifts in theexpression of Kv4.2-based currents to Kv1.4-based currents (46).

Because thyroid hormone can increase the expression of genes encoding for I_to (17, 39, 45) and alter the biophysicalproperties of I_to (38, 39, 45), we were interested in examiningwhether agents with thyroid hormone-like activity could reversesome of the right ventricular electrical remodeling that occurredin our model. The effects of thyroid hormone itself, however,may be complicated by noncardiac effects (14). We chose, instead,to examine the effects of the thyroid hormone analog DITPA, becausethis agent reportedly exerts only minor effects on heart rateand metabolism compared with thyroid hormone itself (25, 32)and might, therefore, have clinical value. DITPA treatment restoredI_to density and G_max in post-MI myocytes to levels observed insham cells but did not affect the V_1/2 of activation. Theseincreases in G_max after DITPA treatment were accompanied by elevationsin Kv4.2 expression and decreases in Kv1.4 expression, reversingthe pattern of changes observed after MI. The effects of DITPAon K⁺ channel expression appear to be mediated at the transcriptionallevel, consistent with the known effects of thyroid hormone onKv4.2 and Kv1.4 transcription in cardiac myocytes (17, 29,39, 45). In contrast, Kv4.3 RNA levels were unchanged afterDITPA treatment, consistent with previous studies using thyroidhormones in adult rats (29, 39). These differential effectsof DITPA treatment on Kv4.2, Kv4.3, and Kv1.4 might explain theinability of this drug to reverse the shift in V_1/2 of activationobserved in post-MImyocytes.

Effect of DITPA on APD and membrane potentials. Consistent with previous observations, we observed action potential prolongation in noninfarcted right ventricular myocytesafter MI (21, 35). Our study further shows that DITPA treatmentin post-MI hearts accelerated action potential repolarizationback to control values. The modulation of APD in isolated myocytesby MI and DITPA treatment coincided closely with changes in I_to,suggesting that the alterations in I_to density were responsiblefor the differences in APD among the groups. It should be recognized,however, that the divalent cation Cd²⁺ was present when I_to was recorded but was absent when actionpotentials were recorded. This could help explain the observationthat I_to densities were only significantly reduced at the morepositive potentials in the post-MI group despite significant reductionsin G_max, because Cd²⁺ potently shifts the V_1/2 for I_to activation to more depolarizedvoltages (2, 46).

The observed changes in APD among the different groups could also conceivably involve alterations in a number of depolarizingand/or hyperpolarizing currents. Our studies establish that I_sus,I_Ca,L, or I_Na densities and their gating properties were not affectedby MI or DITPA treatment. However, changes in other currents besidesI_to might contribute to the observed alterations in action potentialprofile among the groups. Previous studies reported that I_Na/Cawere either increased (24) or decreased (50) after MI andthat the exchanger activity was either decreased (5) or unchanged(6) after daily thyroid hormone treatment. In some of our studiesany contribution of I_Na/Ca to the action potential were minimizedeither by including 5 mM EGTA in the pipette or by reducing extracellularCa²⁺ to 0.1 mM and including 30 mM BAPTA in the pipette. Therefore,the changes in APD under these experimental conditions, at leastin the single-cell recordings, are unlikely to result from differencesin I_Na/Ca among thegroups.

Monophasic action potential recordings from whole hearts showed similar APD differences among groups to those observed inisolated myocyte experiments, suggesting that the isolated myocytestudies are representative of global changes in the intact heart.However, the isolated myocyte studies were performed under relativelynonphysiological conditions (with respect to temperature, frequency,and cellular dialysis) compared with the isolated heart measurements,making it possible that one or more other mechanisms might alsocontribute to the pattern of changes in APD. Extrapolation, therefore,from isolated cells to the whole heart should be done withcaution.

I_K1 was significantly reduced at hyperpolarized potentials but not at depolarized potentials (positive to $-$ 90 mV) after MI.As mentioned previously for I_to, the lack of detectable changesin I_K1 at depolarized potentials might result from the relativelysmall magnitude (34) of the current at these potentials coupledwith the inherent biological and experimental variability in thesewhole cell voltage-clamp recordings. Alternatively, MI could haveconceivably altered the properties of I_K1 differently as a functionof membrane potential. Regardless, depolarization of resting membranepotentials after MI is consistent with decreased I_K1 densities,although changes in other background currents (i.e., Cl and ATP-sensitive K⁺ currents) might also contribute to these alterations. Nevertheless,the inability of DITPA treatment to reverse changes in eitherI_K1 or resting membrane potential are consistent with a connectionbetween the alterations of these parameters afterMI.

Limitations of the present study. Our studies show that APD in myocytes was prolonged after MI. DITPA treatment shortened the duration of myocytes from infarctedhearts back to control levels. The APD in the different groupscoincided with I_to density but not with I_Na, I_Ca,L, I_sus, or I_K1density, suggesting that changes in I_to density are responsiblefor the observed alterations in APD. However, it is certainlypossible that other currents, not measured in this study, mayalso change after infarction and DITPA treatment and thereby contributeto the observed changes in APD. Because the primary aim of ourstudy was to determine the effects of infarction and DITPA onI_to, the investigation of these other currents is beyond the scopeof the presentstudy.

Similar changes in APD after MI and DITPA treatment were seen in both single-myocyte studies and in whole heart monophasicaction potential recordings. These data tend to suggest that thefindings of the single-myocyte studies, under rather nonphysiologicalconditions, are predictive of global properties of the heart undermore physiological conditions. Nevertheless, it is clearly possiblethat the mechanism(s) underlying the changes in APD in these twoconditions isdifferent.

The duration of the cardiac action potential is not uniform throughout the mammalian heart. Regional heterogeneity of APDexists in the normal myocardium (9, 23, 28) and is modulatedby hypertrophy (16). Nonuniform alterations in repolarizationwithin the myocardium may create conditions favorable for theinitiation and/or propagation of reentrant arrhythmias. In thepresent study we made no attempt to determine whether the effectsof MI and DITPA treatment varied among different regions of theheart. We also did not investigate transmural variations of APDwithin the right ventricular free wall because of technical difficultiesassociated with separation of the epicardial and endocardial layers.The question as to how MI and DITPA treatment affect transmuralheterogeneity in the right ventricular free wall may be best studiedin a largerspecies.

In conclusion, we show that DITPA treatment in post-MI rats can restore I_to density and increase Kv4.2 expression to levelsobserved in sham-operated controls. DITPA treatment did not affectI_sus, I_K1, I_Ca,L, or I_Na. Consistent with the increase in expressionof I_to, a shortening of the APD was observed after DITPA treatment.These data suggest that thyroid hormones and analogs might beuseful in the reversal of electrical remodeling observed afterMI.

	ACKNOWLEDGEMENTS

A. D. Wickenden and R. Kaprielian contributed equally to thiswork.

	FOOTNOTES

We thank Dr. Fayez Dawood for performing the surgeries. We also extend special thanks to Tin Nguyen for performing RNase protectionand Western blot assays. We are grateful to the Tiffen Trust Fundand the Center for Cardiovascular Research at the University ofToronto for equipmentgrants.

This study was supported by a grant from the Heart and Stroke Foundation of Ontario (HSFO). P. H. Backx received a MedicalResearch Council (MRC) scholarship and is a career investigatorof the HSFO. R. Kaprielian holds an MRC Doctoral Researchaward.

Present address of A. D. Wickenden: ICAgen Inc., 4222 Emperor Blvd., Ste. 460, Durham, NC27703.

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate thisfact.

Address for reprint requests and other correspondence: P. H. Backx, Univ. Health Network, Center for Cardiovascular Research, 101 College St., CCRW 3-802, Toronto, Ontario, Canada M5G 2C4 (E-mail: p.backx{at}utoronto.ca).

Received 25 January 1999; accepted in final form 21 September 1999.

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