Regional contributions of Kv1.4, Kv4.2, and Kv4.3 to transient outward K+ current in rat ventricle

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Regional contributions of Kv1.4, Kv4.2, and Kv4.3 to transient outward K⁺ current in rat ventricle

A. D. Wickenden¹, T. J. Jegla², R. Kaprielian¹, and P. H. Backx¹

¹ Department of Medicine, Centre for Cardiovascular Research, and the Toronto Hospital, University of Toronto, Toronto, Canada M5G 2C4; and ² ICAgen Incorporated, Durham, North Carolina 27703

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

The aim of the present study was to assess differences in transient outward potassium current (I_to) between the right ventricularfree wall and the interventricular septum of the adult rat ventricleand to evaluate the relative contributions of Kv4.2, Kv4.3, andKv1.4 to I_to in these regions. The results show that I_to is composedof both rapidly and slowly recovering components in the rightwall and septum. The fast component had a significantly higherdensity in the right free wall than in the septum, whereas theslow component did not differ between the two sites. Kv4.2 mRNAand protein levels were also highest in the right wall and correlatedwith I_to density, whereas Kv4.3 was expressed uniformly in theseregions. The kinetics of the rapidly recovering component of I_toin myocytes was similar to that recorded in tsa-201 cells expressingKv4.2 and Kv4.3 channels. Kv1.4 mRNA and protein expression correlatedwell with the density of the slowly recovering I_to, whereas therecovery kinetics of the slow component were identical to Kv1.4expressed in tsa-201 cells. In conclusion, expression of Kv1.4,Kv4.2, and Kv4.3 differs between regions in rat hearts. Regionallyspecific differences in the genetic composition of I_to can accountfor the region-specific properties of thiscurrent.

septum; right ventricle; rat heart

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

THE CALCIUM-INDEPENDENT transient outward potassium current (I_to) is an important repolarizing current in rat ventricularmyocytes. The expression of this current is not uniform throughoutthe rat heart, and regional variations in the density, biophysicalproperties, and regulation of I_to exist (3, 8, 22). Forexample, the density of I_to in the left ventricle is higher inthe epicardium compared with the endocardium whereas endocardialcurrents show a greater degree of rate dependence, and endocardialand epicardial currents are differentially regulated by thyroidhormone (3, 22). Consistent with heterogeneity of transientoutward currents in rat heart, three different K⁺-channel genes that encode I_to-like currents (i.e., Kv1.4, Kv4.2,and Kv4.3) are known to be expressed at the mRNA level in therat ventricle (5, 6, 16). In the left ventricle, the expressionof Kv4.2 mRNA correlates with the density of I_to across the leftventricular wall (6). On the other hand, Kv4.3 and Kv1.4 mRNAsshow uniform transmural expression in the left ventricle (5,6). It is possible, therefore, that the molecular compositionof I_to may vary across the left ventricular wall and that differencesin the relative contribution of Kv4.2, Kv4.3, and Kv1.4 to epi-and endocardial I_to may underlie differences in the density, biophysical,and regulatory properties of thiscurrent.

In addition to variations in I_to across the left ventricular wall, differences in the density and regulatory properties ofI_to may also exist between other regions of the rat heart. Thedensity of I_to is lower in septum compared with left ventricularfree wall, for example, and I_to in the free wall but not septumare reduced during the development of myocardial hypertrophy inthe rat (8). The molecular basis of these differences, however,has not been addressed. In the present study, we combined electrophysiologyand molecular biology to characterize I_to in the right ventricularfree wall and the interventricular septum of the adult rat ventricleand to evaluate the relative contributions of Kv4.2, Kv4.3, andKv1.4 to I_to in these regions. In addition, because it has beenreported that the mRNA levels of K⁺ channels are not always predictive of protein levels (1, 28),we also used Western blot analysis to evaluate the potential contributionof K⁺-channel gene products to I_to in the right ventricular free wallandseptum.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Isolation of adult rat ventricular myocytes. Adult rat ventricular myocytes were isolated as previously described (27) with minor modifications. Briefly, rats ( $>=$ 250g, Sprague-Dawley, Charles River) were heparinized and killed(under 75 mg/kg pentobarbital sodium) by cervical dislocation.The heart was removed and retrogradely perfused for 3 min withTyrode solution of the following composition (mM): 132 NaCl, 5.4KCl, 1 CaCl₂, 1.2 MgSO₄, 10 HEPES, and 10 D-glucose, pH 7.4. Thehearts were then perfused with nominally calcium-free Tyrode fora further 5 min, followed by perfusion with Tyrode solution containingcollagenase (type II, 0.6 mg/ml, Boehringer-Mannheim), protease(type XIV, 0.05 mg/ml, Sigma Chemical, St. Louis, MO), and CaCl₂(25 µM). Once digestion was complete (typically 7-9 min), heartswere perfused for an additional 5 min with enzyme-free high-K⁺ solution of the following composition (mM): 120 potassium glutamate,20 KCl, 20 HEPES, 1 MgCl₂, 10 D-glucose, and 0.5 K-EGTA. The entireright ventricular free wall (from 5 hearts) and interventricularseptum (from 4 hearts) were removed under a dissecting microscopeand minced in high-K⁺ solution. Cells were liberated with gentle mechanical agitation,filtered through nylon mesh, and stored in high-K⁺ solution until required. Only calcium-tolerant, quiescent, rod-shapedmyocytes with clear cross striations were selected for electrophysiologicalrecordings. All experimental protocols conform with the Guidefor the Care and Use of Laboratory Animals published by the NationalInstitutes of Health (NIH) [DHHS Pub. no. (NIH) 85-23, revised1996]. The protocols were approved by the Animal Care Committeeof the Research Institute at the TorontoHospital.

tsa-201 cell culture and transfection. tsa-201 cells were maintained in MEM supplemented with 10% fetal bovine serum and gentamicin (50 µg/ml) in an incubator at37°C with a humidified atmosphere of 5% CO₂. Medium was replacedevery 48-72 h. Twenty-four hours before transfection, tsa-201cells were harvested by brief trypsinization (0.5 mg/ml in phosphate-bufferedsaline) and replated at a density of 3 × 10⁵ cells per 35-mm culture dish. Cells were transfected using Lipofectaminereagent (GIBCO BRL) according to the manufacturer's instructions.Cells were incubated for a period of 5 h with a mixture of 10µl Lipofectamine, 1 µg green fluorescent protein (GFP), and 0.5-1µg pRcCMVKv4.2, 1 µg pcDNA3Kv4.3, 0.03-1 µg pGW1HKv1.4, or a similaramount of vector alone in OPTI-MEM serum-free media. Twenty-fourto forty-eight hours posttransfection, cells were prepared forelectrophysiological evaluation. Cells were removed from the culturedish by brief trypsinization (as described in Isolation of adultrat ventricular myocytes), collected by centrifugation (1,000rpm, 5 min), and replated in growth medium at low density. Allreagents for cell culture were purchased from GIBCOBRL.

Electrophysiological recording. Adult right ventricular myocytes were placed in a bath and perfused (~1 ml/min) with extracellular Tyrode solution of thefollowing composition (mM): 140 NaCl, 2 CaCl₂, 4 KCl, 1 MgCl₂· 6H₂O, 10 glucose, 10 HEPES, and 0.5 CdCl₂ (for myocyte recordingsonly), pH 7.4 with NaOH. Electrophysiological recordings fromtsa-201 cells were made with the cells adhered to the 35-mm culturedishes in which they were plated. Culture medium was replacedwith extracellular solution immediately before recordings. Pipettetips were heat polished to a resistance of 1-3 M $Omega$ when filledwith an intracellular solution of the following composition (mM):140 KCl, 1 MgCl₂ · 6H₂O, 10 EGTA, 10 HEPES, and 5 MgATP, pH 7.2-7.3with KOH. In some experiments with cultured cells a KF-based pipettesolution was used to improve seal stability. The composition (mM)of the modified Tyrode (KF) solution was 100 KF, 40 KCl, 5 NaCl,2 MgCl₂, 10 HEPES, 5 EGTA, and 5 glucose, pH 7.2-7.3 with KOH.Recovery kinetics were similar with KCl- and KF-based intracellularsolutions. All recordings were made at room temperature (22-24°C)within 12 h of cell isolation (myocytes) or replating (tsa-201cells). Successfully transfected tsa-201 cells were identifiedby their green fluorescence under appropriateconditions.

After membrane rupture, the capacitance transient was integrated on-line to estimate cell capacitance as a measure of cellsize. Uncompensated series resistance was 4.0 ± 0.3 M $Omega$ (n = 20)for recordings from right ventricular myocytes and 3.8 ± 0.4 M $Omega$ (n = 19) for recordings from septal myocytes. Series resistancecompensation was 81.0 ± 2.4% (n = 20) for recordings from rightventricular myocytes and 73.0 ± 2.6% (n = 19) for recordings fromseptal myocytes. Outward currents were induced with 500-ms depolarizingpulses to 60 mV from a holding potential of $-$ 80 (myocytes) or $-$ 100 (tsa-201 cells) mV. In myocyte recordings, a brief prepulse( $-$ 40 mV for 30 ms) was used to inactivate Na⁺ current. In all studies, I_to was defined as peak current elicitedby the depolarizing voltage step minus the steady-state currentremaining at the end of a 500-ms voltage step. Current-voltagerelationships were constructed by eliciting a series of depolarizingsteps ( $-$ 60 to +60 mV) in 20-mV increments from the holding potential.Recovery from inactivation was measured using a double-pulse protocol.From the holding potential, cells were depolarized for 500 ms.Cells were returned to the holding potential for 10 ms to 20 s,and then a second 500-ms depolarizing pulse was applied. The magnitudeof I_to induced by the second pulse is expressed as a percentageof I_to induced by the first pulse. Monoexponential or biexponentialfunctions were used to fit recovery from inactivation data. Forbiexponential fits

<IT>I</IT>/<IT>I</IT><SUB>0</SUB> = <IT>A</IT><SUB>fast</SUB> ⋅ [1 − exp (−<IT>t</IT>/&tgr;<SUB>fast</SUB>)] + <IT>A</IT><SUB>slow</SUB> ⋅ [1 − exp (−<IT>t</IT>/&tgr;<SUB>slow</SUB>)]

where A_fast and A_slow are the amplitudes of the fast and slow components for recovery, t is the time spent at the recoverypotential, and $tau$ _fast and $tau$ _slow are the time constants for recoveryof the fast and slow components, respectively. When the recoverydata was fit to a monoexponential, A_fast = A_slow = A and $tau$ _fast= $tau$ .

For myocyte studies, the repetition interval was >20 s to allow complete repriming of slowly recovering currents. In tsa-201studies, the repetition interval was set at 15 s for Kv4.2 andKv4.3 and >20 s for Kv1.4.

Preparation of total RNA. Hearts were removed rapidly, and the right ventricle and septum were isolated, rinsed briefly in 0.9% NaCl (wt/vol), and snapfrozen in liquid nitrogen. Ventricular tissue was homogenizedin Trizol reagent (GIBCO) and RNA precipitated with isopropylalcohol. The integrity of RNA samples was confirmed by the presenceof sharp bands after brief electrophoresis through a 1% agarosegel. The concentration of RNA was measured spectrophotometricallyand confirmed by agarose gel electrophoresis. RNA was isolatedindependently from four adult rathearts.

RNase protection assays. RNase protection assays were performed using an RPAII Ribonuclease Protection Assay Kit (Ambion, Austin, TX) as previouslydescribed (27). The Kv4.2 and Kv4.3 probes were kindly providedby Dr. David McKinnon (State University of New York at Stony Brook)and have been described previously (5). A 429-bp fragment ofrat Kv1.4 (kindly provided by Dr. David McKinnon) was subclonedinto pGEM11 (Hind III-Nsi I) to make a Kv1.4 probe capable ofprotecting a 331-bp fragment of Kv1.4 mRNA. The cyclophilin probewas purchased from Ambion. Abundance of mRNA transcripts was quantifiedby densitometry (Bio-Rad GS670 Imaging densitometer). Signalswere normalized to a cyclophilin internal standard to ensure thatfindings were not influenced by minor variations in loading. Absolutecyclophilin levels (densitometric units) were not significantlydifferent between right ventricle and septum in the present study(right ventricular cyclophilin levels were 129 ± 20% of septallevels; n = 24; P > 0.05, two-tailed, paired t-test), indicatingthat this gene was expressed uniformly between these regions.Right ventricular wall mRNA levels for each rat were normalizedto mRNA levels in the septum of the sameanimal.

Isolation of protein from right ventricular wall and septum. Hearts were removed rapidly, and the right ventricle and septum were isolated as described in Isolation of adult rat ventricularmyocytes, rinsed briefly, and homogenized in buffer A [0.32 Msucrose, 5 mM Tris (pH 7.4) containing protease inhibitors phenylmethylsulfonylfluoride (100 µM), o-phenanthroline (1 mM), iodoacetamide (1 mM),and benzamidine (1 mM)]. Homogenate was centrifuged to removeparticulate matter. Membranes were collected from the supernatantby centrifugation at 27,000 g for 45 min and resuspended in bufferC (0.32 M sucrose, 5 mM HEPES solution containing protease inhibitorsas described above). Membrane protein was isolated independentlyfrom three to five adult rat hearts. Protein concentration wasdetermined by the Lowry method with minor modifications (11),and the membranes were aliquoted and stored at $-$ 70°C until furtheruse. Rat brain membranes were prepared as described previously(9). After protein determination, rat brain membranes werealiquoted and frozen in liquidnitrogen.

Western blot analysis. For Western blot analysis, 10- to 50-µg (heart) or 3.5- to 10-µg (brain) aliquots of freshly thawed membrane protein weretritrated in 2× SDS sample buffer containing $beta$ -mercaptoethanol,heated for 5 min at 95°C, and centrifuged to pellet any insolubledebris. Supernatant proteins were then resolved by electrophoresison 7.5% SDS-polyacrylamide gels and transferred electrophoreticallyto nitrocellulose (0.45 µm Kv1.4) or polyvinylidene difluoride(Kv4.2). The blots were then blocked in Tris-buffered saline (TBS)containing 5% nonfat dried milk, washed with TBS, and probed withanti-Kv antibody raised in rabbit (Dr. O. T. Jones, Departmentof Pharmacology, University of Toronto) at a 1:1,000 dilutionin blocking solution. After consecutive washes with TBS containing0.05% Tween-20 and TBS alone, the blots were incubated for 2 hwith secondary antibody [horseradish peroxidase-conjugated donkeyanti-rabbit (Amersham), 1:4,000 in blocking solution], rewashed,and developed by enhanced chemiluminescence (ECL, Amersham). Gelloading was checked by staining total proteins with Ponceau S,and molecular masses were determined using prestained markers(Kaleidoscope, Bio-Rad). Densitometric analysis of films was donewith a Bio-Rad model GS-670 imagingdensitometer.

The procedure by which the anti-Kv1.4 antibody was produced has been described in detail previously (27). Peptide Kv4.2N,corresponding to a region of Kv4.2 that shares little identitywith Kv4.3 (amino acid residues 23-42 of Kv4.2, ASGPMPAPPRQERKRTQDALare distinct from the analogous sequence in Kv4.3, i.e., ANCPMPLAPADKNKRQDEL)was synthesized by solid-phase fluorenymethoxy carbonyl chemistry(Vetrogen, London, ON, Canada) and coupled to keyhole limpet hemocyanin(KLH) using the heterobifunctional crosslinker N-[ $gamma$ -maleimidobutyryloxy]sulfosuccinimideester (Pierce). After being dialyzed against PBS, the KLH conjugatewas injected into New Zealand White rabbits at multiple subcutaneoussites by Berkeley Antibody (Richmond, CA). Antisera were collectedand tested by ELISA using microtiter plates coated with Kv4.2Npeptide, and the IgG was enriched by affinity chromatography onprotein A agarose (MAPS kits, Bio-Rad). The specificity of theserum was determined by immunoblots with rat brain membranes exactlyas previously described (21).

Plasmid constructs. The long splice variant of human Kv4.3 (10) was amplified from a hippocampus cDNA library (Clontech) using overlap extension.First, three overlapping pieces covering the entire Kv4.3 codingsequence were amplified using three primer pairs: 5'-TCTCAAGCTTCCACCATGGCGGCCGGAGTTGCGGCCTGGCT-3'and 5'-CGAGGGCATCGATTCCTGGTTGTTCTCCGAGTCGTTG-3'; 5'-CACCAGGAATCGATGCCCTCGCTCAGCTTCCGCCAGAC-3'and 5'-GCAGATGGAGCCGAAGATCTTCCCTGC-3'; and 5'-GCAGGGAAGATCTTCGGCTCCATCTGC-3'and 5'-TAGCTCTAGATTACAAGACAGAGAGACCTTGACAACATTGC-3'. Overlap extensionwas performed using 20 ng of each amplified fragment, using thefirst and last primers. The overlap product was subcloned intopcDNA3 (Invitrogen), and the insert was confirmed bysequencing.

Plasmid pRc/CMVKv4.2, containing the entire coding region of rat Kv4.2 was obtained from Dr. J. Nerbonne (Washington University,St. Louis) with kind permission from Dr. L. Jan (University ofCalifornia, San Francisco). Full-length rat Kv1.4 was kindly providedby Dr. M. M. Tamkun (Vanderbilt Medical Center, Nashville, TN).A BamHI/SalI fragment containing the entire coding region of Kv1.4was subcloned into BglII/SalI pGW1H (British Biolabs). A plasmidencoding jellyfish GFP was kindly provided by Dr. Jeremy Nathan(Johns HopkinsUniversity).

Statistics. All data are expressed as means ± SE. Statistical significance was determined using a suitable (hetero- or homoscedastic)unpaired two-tailed t-test. For RNase protection assays and Westernblot analysis, the null hypothesis (i.e, that mRNA/protein levelswere not different in septum and right wall) was tested usingpaired two-tailed t-tests. A P < 0.05 was consideredsignificant.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

I_to in right ventricular free wall and septum. I_to density (at 60 mV) was 29.5 ± 3.0 (n = 20 cells from 5 hearts) and 15.9 ± 3.0 (n = 19 cells from 4 hearts) pA/pF in myocytesisolated from the right ventricular free wall (cell capacitance139.3 ± 8.0 pF) and the interventricular septum (cell capacitance167.0 ± 7.2 pF), respectively. When comparing the biophysicalproperties of these currents, we focused exclusively on the kineticsof recovery from inactivation because the rate of recovery frominactivation has previously been shown to vary between differentregions of the left ventricle and at different developmental stages(22, 27). Furthermore, dramatically different rates of recoveryfrom inactivation have been observed between Kv1.4 and the Shal-relatedK⁺ channels Kv4.2 and Kv4.3 in Xenopus oocytes (6, 14, 19,20, 25), thereby potentially providing an electrophysiologicalfingerprint for the different channel types. Recovery from inactivationwas measured using the double-pulse protocol shown in the insetto Fig. 1C and described in METHODS. In these studies we useda very low stimulation frequency (0.05 Hz) to ensure sufficienttime for all currents to completely recover (see below). In boththe right ventricular free wall and interventricular septum therecovery from inactivation of I_to was dominated by a rapid component.Complete recovery from inactivation, however, frequently requiredvery long interpulse intervals, resulting in a biphasic time courseof recovery. The slowly recovering component of I_to was observedin less than one-half of the cells isolated from the right ventricularfree wall (7/20) and in virtually all cells isolated from theseptum (17/19). The biphasic nature of recovery from inactivationfor I_to is clearly visible from the voltage-clamp recordings displayedin Fig. 1 for myocytes from the right wall (Fig. 1A) and septum(Fig. 1B). For both cells I_to recovered rapidly to ~80% of thecontrol level, but complete recovery required prolonged interpulseintervals. The plots of normalized current against interpulseinterval for the same cells are shown in Fig. 1, C (right wall)and D (septum). These figures show that the rapid phase of recoverywas complete within 200 ms but that full recovery required aninterpulse interval of 20 s. Consistent with the presence of aslowly recovering component of I_to, the amplitude of I_to was decreasedin some cells during repetitive, high-frequency stimulation. Thisis shown in Fig. 2, C and D, in which voltage-clamp recordingsfrom a septal cell show that the amplitude of I_to was reducedby 20% during repetitive stimulation with 500-ms depolarizingpulses at a rate of 1 Hz.

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Fig. 1. Biphasic recovery from inactivation of transient outward potassium current (I_to) in myocytes isolated from adult rat heart. Recovery from inactivation was measured using double-pulse protocol shown in inset in C. Typical voltage-clamp recordings showing recovery from inactivation of I_to in a right ventricular free cell (A) and a septal cell (B), with increasing interpulse intervals (10, 20, 40, 100, 200, and 600 ms, 1 , 2, and 20 s), are shown. Note that although recovery is dominated by a rapid component, complete recovery required prolonged interpulse intervals in both cells. I_to (peak current $-$ current remaining at end of 500-ms pulse) elicited by second pulse was normalized to that elicited by first pulse and plotted against interpulse interval in C (right wall) and D (septum). Recoveries were best fit with a biexponential function, with fast components accounting for 80.2% of the recovery in right wall and 85.4% in septum [time constant for recovery of fast component ( $tau$ _fast) = 26.7 and 49 ms for right wall and septal cells, respectively], with a slow component [time constant for recovery of slow component ( $tau$ _slow) = 3,478 and 12,772 ms for right wall and septal cells, respectively] accounting for the remainder.

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Fig. 2. Reduction of I_to amplitude during 1-Hz stimulation in a myocyte isolated from interventricular septum. Superimposed voltage-clamp recordings shown in A are first 5 sweeps recorded from a septal cell stimulated at a frequency of 1 Hz after a rest period of 30 s (sweep 1 is top trace). I_to amplitude (peak $-$ sustained) was normalized to I_to amplitude on sweep 1 and plotted against sweep number in B. This figure shows that I_to amplitude was abruptly reduced between sweep 1 and sweep 2.

On average, the rapidly recovering component of I_to accounted for 92.9 ± 2.5% (n = 15) of I_to in the right ventricular cellsand 81.6 ± 3.1% (n = 19) of I_to in the septal cells. The densityof the fast component was significantly larger in the right ventricularcells (27.6 ± 3.2 pA/pF, n = 15) compared with the septum (13.6± 2.9 pA/pF, n = 19; P = 0.003). The $tau$ _fast were also significantlydifferent between the right ventricular free wall (24.2 ± 1.4ms, n = 15) and the septum (33.3 ± 3.1 ms, n = 19; P = 0.012).The density of the slow component, on the other hand, was notdifferent between regions (2.4 ± 0.98 pA/pF in right wall comparedwith 2.2 ± 0.6 pA/pF in septum; P = 0.85). The $tau$ _slow were 3,527± 983 ms (n = 7) in right ventricular free wall cells and 4,561± 1,090 ms (n = 17) in cells from the septum. These values werenot significantly different (P = 0.58).

Recovery from inactivation of Kv4.2-, Kv4.3-, and Kv1.4-based currents in a mammalian cell line. To understand the molecular basis of the rapidly and slowly recovering components of I_to in the right wall and septum, wemeasured the recovery kinetics of candidate K⁺-channel gene products (Kv4.2, Kv4.3, and Kv1.4) after transienttransfection of mammalian tsa-201 cells. Cells transfected withKv4.2 (Fig. 3B), Kv4.3 (Fig. 3C), or Kv1.4 (Fig. 3D) expressedrobust, transient outward-like currents. Similar currents werenever recorded from nontransfected cells or cells transfectedwith vector DNA only (although these cells do express a smallendogenous delayed rectifier-like current; Fig. 3A). Figure 3,E and G, shows typical voltage-clamp recordings of recovery frominactivation of Kv4.3- and Kv4.2-based currents, respectively.As shown, recovery from inactivation for both these gene productswas relatively rapid, with the normalized current versus interpulseinterval being fit with monoexponential functions with time constantsof 84 (Kv4.3, Fig. 3F) and 51.4 (Kv4.2, Fig. 3H) ms. Similar observationswere made in a total of six cells per group. On average, recoveryfrom inactivation was slower for Kv4.3 (mean ± SE $tau$ value was141 ± 23 ms) compared with Kv4.2 ( $tau$ value was 73.1 ± 9.5 ms; P= 0.02). The recovery kinetics of Kv4.3 and Kv4.2 based currentsexpressed in tsa-201 cells resembled the rapid component of I_tomeasured in myocytes. These findings suggest that Kv4.3 and/orKv4.2 may underlie the rapidly recovering component of I_to inthese regions.

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Fig. 3. Recovery from inactivation of Kv4.3, Kv4.2, and Kv1.4 expressed in tsa-201 cells. Current recordings showing families of outward currents recorded from tsa-201 cells transfected with green fluorescent protein alone, Kv4.2, Kv4.3, or Kv1.4 are shown in A-D, respectively (for clarity only currents elicited after steps to $-$ 40, $-$ 20, 0, 20, 40, and 60 mV are shown). Recovery from inactivation was measured using double-pulse protocol shown in insets in F, H, and J. Typical voltage-clamp recordings showing recovery of a Kv4.3- or Kv4.2-based current with increasing interpulse interval (20-ms steps starting at 20 ms) are shown in E and G, respectively. Kv4.2/Kv4.3 currents (defined as peak current $-$ current remaining at end of 500-ms pulse) elicited by second pulse were normalized to those elicited by first pulse and plotted against interpulse interval (Kv4.2, F; Kv4.3, H). In both cases, recovery was well fit with a single exponential function with $tau$ of 84 (Kv4.3) and 51.4 (Kv4.2) ms. Typical voltage-clamp recordings showing recovery of a Kv1.4-based current with increasing interpulse interval (from 200 ms to 5 s) are shown in C. Recovery of this Kv1.4-based current was well fit with a single exponential with a $tau$ of 1,784 ms (D).

Recovery from inactivation of Kv1.4-based currents was relatively slow in tsa-201 cells, as illustrated in Fig. 3, I and J.Kv1.4-based currents typically required interpulse intervals of $>=$ 20 s to fully recover from inactivation. The plot of normalizedKv1.4 current against interpulse interval shown in Fig. 3J waswell fit with a monoexponential function with a $tau$ equal to 1,784ms. Similar observations were made in a total of six cells ( $tau$ = 3,307 ± 902 ms). Clearly, the recovery kinetics of Kv1.4 expressedin tsa-201 cells was similar to the recovery kinetics of the slowcomponent of I_to, supporting the notion that Kv1.4 contributesto I_to in right ventricular and septalcells.

Kv4.2, Kv4.3, and Kv1.4 mRNA levels in right ventricular free wall and interventricular septum. To gain further insight into the molecular basis of I_to in the right ventricular free wall and septum, we measured mRNA levelsof Kv4.2, Kv4.3, and Kv1.4 in these regions. Figure 4, A, C, andE, shows representative gels from RNase protection assays showingKv4.2, Kv4.3, and Kv1.4 mRNA levels in the right ventricular freewall, the interventricular septum, and brain. Robust transcriptionalexpression of Kv4.2, Kv4.3, and Kv1.4 was observed in both theright ventricular free wall and septum. Transcript levels (normalizedto the levels of cyclophilin mRNA and to respective mRNA levelsin the septum) are plotted in Fig. 4, B, D, and F. The mRNA levelsof Kv4.2, Kv4.3, and Kv1.4 tended to be higher in the right ventricularfree wall compared with the septum (right ventricular mRNA levelswere 248 ± 46, 113 ± 9, and 133 ± 26% of those in the septum forKv4.2, Kv4.3, and Kv1.4, respectively; n = 4/group). However,only the Kv4.2 levels were significantly different between rightventricle and septum (P = 0.049). The higher level of expressionof Kv4.2 mRNA in the right wall compared with the septum correlatedwell with the twofold higher density of the rapidly recoveringcomponent of I_to in the right wall compared with the septum. Furthermore,the observation that Kv1.4 mRNA was readily detected supportsthe suggestion that the product of this gene may underlie theslowly recovering component of I_to.

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Fig. 4. Kv4.2, Kv4.3, and Kv1.4 mRNA levels in right ventricular free wall and septum measured using an RNase protection assay. Gels show Kv4.2 (A)-, Kv4.3 (C)-, and Kv1.4 (E)-protected mRNA fragments, along with control cyclophilin mRNA levels for samples containing 10 µg of total RNA isolated from rat brain (Br), 4 right ventricular free walls (RV1-4), and 4 septums (S1-4). mRNA levels were quantified by densitometry and normalized to cyclophilin mRNA levels in same sample. mRNA level in right ventricle was further normalized to septum level in same heart, and mean values are plotted in bar graphs for Kv4.2 (B), Kv4.3 (D), and Kv1.4 (F) in right ventricular wall (solid bars) and septum (open bars). Bars represent means of 4 determinations, and vertical lines represent SE.

Kv1.4 and Kv4.2 protein levels in right ventricular free wall and interventricular septum. Because mRNA levels may not always be predictive of expression at the protein level (28), we also conducted Western blotanalyses using specific anti-Kv4.2 and anti-Kv1.4 antibodies.Figure 5A shows that Kv1.4 was detectable in samples isolatedfrom the right ventricular free wall and septum, albeit at considerablylower levels than in brain. In the present study, the anti-Kv1.4antibody labeled two distinct bands, in both brain (seen withreduced exposures; Fig. 5A, inset) and myocyte protein. The molecularmasses of these two bands were ~91.5 and 100.5 kDa, which arevery similar to those previously identified in protein extractedfrom cos-1 cells transfected with Kv1.4 (18) and cultured neonatalrat ventricular myocytes (27). The basis for the presence oftwo bands is unclear, but studies have established that Shaker,Kv1.3, and Kv1.1 channels have glycosylated and nonglycosylatedfractions leading to two distinct bands (4, 18, 23). Bothbands could be eliminated by preincubation of the antibody withthe peptide against which the antibody was raised (Kv1.4N 12 µg/µl;Fig. 5B). Taken together, these results suggest that both bandslikely represent Kv1.4-related proteins. Total Kv1.4 immunoreactivityin the right ventricular free wall, although somewhat greater,was not statistically (P = 0.06) different from the septum infive hearts studied.

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Fig. 5. Kv1.4 and Kv4.2 protein levels in right ventricular free wall and septum. Representative gels from Western blots showing Kv1.4 (A) and Kv4.2 (D) levels in protein samples (see METHODS) obtained from adult rat brain (Br, 10 µg), adult rat right ventricular wall (R1-R3, 50 µg), and adult rat interventricular septum (S1-S3, 50 µg). Anti-Kv1.4 antibody labeled 2 distinct bands in myocyte protein with molecular masses of ~91.5 and 100.5 kDa. As shown in inset in A, 2 bands were also seen in rat brain samples. Because of higher expression of Kv1.4 in brain samples, it was difficult to resolve these 2 bands under conditions required to visualize cardiac proteins (right lane of inset). However, two bands were evident with reduced exposure of film (left lane of inset). Blots of protein from rat heart probed with anti-Kv1.4 or anti-Kv4.2 antibodies after preincubation with peptide are shown in B and E, respectively. Absence of bands in these blots, despite prolonged exposures, indicates that bands seen in A and D were specific. Protein levels were quantified by densitometry and normalized to levels in septum of same heart. Relative expression levels are plotted as bar charts for Kv1.4 (C) and Kv4.2 (F). Solid bars represent relative expression in right ventricular free wall; open bars show relative expression in septum. Each bar is mean ± SE from 3-5 hearts.

Kv4.2 immunoreactivity was also readily detectable in protein samples from the right wall and septum. The anti-Kv4.2 antibodylabeled a single band with an estimated molecular mass of 72 kDa(Fig. 5D), similar to that reported previously (1, 28). Thislabeling appeared to be specific because the band disappearedwhen the blot was probed with antibody that had been preincubatedwith the Kv4.2N peptide (20 µg/µl, Fig. 5E). It is unlikely thatthe detected band contained contributions from Kv4.3 channelsbecause the NH₂-terminal Kv4.2 peptide sequence used to generatethe antibodies had only roughly 50% sequence identity with Kv4.3.Furthermore, the predominant (long) isoform of Kv4.3, expressedin the heart, has a predicted molecular mass that is 20% largerthen Kv4.2, yet only a single band was detected (13, 24).Nevertheless, we found that Kv4.2-like immunoreactivity in theright ventricular free wall was significantly higher (361 ± 54%,n = 3 hearts; P = 0.008) than in the septum, which coincided closelywith the mRNA expression of Kv4.2 and correlated with the densityof the rapidly recovering component of I_to in both the septumand right freewall.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Differences in the density and regulatory properties of I_to exist between anatomically distinct regions of the rat heart (3,8, 22). The purpose of the present study was to characterizeand compare I_to in the right ventricular free wall and the interventricularseptum of the adult rat ventricle and to evaluate the possiblerelative contributions of Kv4.2, Kv4.3, and Kv1.4 to I_to in theseregions. In the present study, we found that the density of I_towas significantly greater in the right ventricular free wall comparedwith the septum. Recovery from inactivation (using slow stimulationfrequencies) revealed two kinetically distinct components to I_toin both regions. Recovery from inactivation of I_to was dominatedby a rapidly recovering component in both the right ventricularfree wall and the interventricular septum. The kinetics of thisrapid component were similar to the kinetics of recovery of Kv4.2expressed in mammalian cells (Refs. 7 and 29 and presentstudy) and to Kv4.3 expressed in mammalian cells (present study)and in Xenopus oocytes (6, 20), suggesting that these Shal-relatedK⁺-channel genes, either as homo- or heterotetramers, contributeimportantly to the rapidly recovering component of I_to in theright wall and septum. Consistent with this, we found that Kv4.2and Kv4.3 mRNAs and Kv4.2 protein were robustly expressed in boththe right ventricle and the septum. The finding that Kv4.2 mRNAand protein levels were significantly higher in the right wallcompared with the septum suggests that differences in Kv4.2 expressionaccount for the difference in the density of the rapidly recoveringcomponent of I_to between these regions. The observation that Kv4.3mRNA levels were similar in these regions suggests that Kv4.3may be proportionately more important in the septum compared withthe right wall. Because we found that recovery from inactivationfor Kv4.3 is marginally slower than that for Kv4.2, it is possiblethat differences in the quantities of Kv4.2 and Kv4.3 in differentregions of the adult rat heart could explain the finding thatthe recovery kinetics of the fast component differed between theright wall and the septum, as suggested previously for differencesobserved between the endo- and epicardium (6).

In addition to the dominant, rapidly recovering component of I_to, a smaller, slowly recovering component of I_to was also evidentin a portion of right wall cells and the septum in the presentstudy. This current appeared proportionately more important inthe septum, in which on average it accounted for ~20% of I_to.The kinetics of recovery of this current was remarkably similarto that recorded from Kv1.4 expressed in the mammalian cell line.Moreover, the absolute current density of the slow component wassimilar between regions, which coincided with the absence of significantdifferences in the Kv1.4 protein and mRNA levels. Although itremains possible that the slowly recovering component of I_to mayrepresent some other (i.e., non-Kv1.4) channel and that the sourceof the Kv1.4-like protein may be nerve or vascular smooth muscle(i.e., noncardiac), the simplest interpretation of our findingsis that Kv1.4 underlies the slowly recovering component of I_toin the right wall and septum of the adult rat heart, as has beenpreviously suggested for the slowly recovering I_to recorded inrabbit ventricle (26). These findings are also consistent withprevious studies in human and rat myocardium showing that a slowlyrecovering I_to is expressed predominantly in cells from the endocardiallayer of the left ventricular free wall (12, 22) and thatKv1.4 protein is preferentially expressed in the endocardial layerof the ferret left ventricle (2). In addition, the slowly recoveringcomponent of I_to was only detected in a portion of right wallcells. It is possible that the right wall cells displaying theslow component originate from the endocardium portion of the rightwall. Further studies are required to address this possibility.Our findings differed from previous studies that failed to detectKv1.4 protein in adult rat heart (1, 28). It is possiblethat this discrepancy may be explained by the use of differentstrains of rats, differences in the methods of protein isolation,and/or by the use of different anti-Kv1.4antibodies.

Although Kv1.4-based currents seem to contribute to I_to under the conditions of the present study (i.e., long interpulse intervals),the functional contribution of such slowly recovering channelsunder more physiological conditions is unclear. Indeed, it hasbeen suggested that at normal heart rates these currents wouldbe permanently inactivated (15). In fact, however, the behaviorof these currents under physiological conditions is very difficultto predict. Temperature, action potential amplitude and/or duration,extracellular K⁺, redox, and posttranslational modification could all impact onthe degree of inactivation and/or recovery from inactivation andpotentially render these currents available at physiological heartrates. Interestingly in this regard, one recent report has shownthat Ca/calmodulin-dependent protein kinase II-mediated phosphorylationof the NH₂-terminus of Kv1.4 slows the rate of inactivation andaccelerates the recovery kinetics of Kv1.4-based currents (17).

In the present study we have sought to correlate gene expression (mRNA and protein) with function (electrophysiology) to identifythe molecular correlates of I_to in the right wall and the septumof the rat heart. The RNase protection assay is a powerful techniquefor the identification of rare messages such as ion channels.However, this technique can only provide information on the relativeexpression of a given transcript between regions and does notallow for the measurement and comparison of absolute copy numberof multiple molecular species within a region. Further studiesusing alternative molecular techniques (such as quantitative PCR)would be helpful in this regard. Correlations between gene expressionand function, although persuasive, also require support usingalternative techniques. We are currently examining the possibilityof using recombinant adenoviruses to deliver dominant negativeconstructs into cardiac muscle before cell isolation as an alternativestrategy for determining the molecular nature of native currentsin the ratheart.

In summary, the results of the present study show that I_to is composed of both rapidly and slowly recovering components inthe right wall and septum of the rat ventricle. Both Kv4.2 andKv4.3 probably contribute to the rapid component, and Kv1.4 appearsto underlie the slow component of I_to. Kv4.2 expression predominatesin the right wall, whereas Kv4.3 and Kv1.4 may be proportionatelymore important in the septum. Such regional differences in thecontribution of Kv4.2, Kv4.3, and Kv1.4 may account for regionaldifferences in the properties and regulation of I_to.

	ACKNOWLEDGEMENTS

The authors gratefully acknowledge T. Nguyen for help with the RNase protection assays and Westernblotting.

	FOOTNOTES

This work was supported by a grant from the Heart and Stroke Foundation of Ontario (to P. H. Backx) and a University of TorontoDepartment of Medicine Post-Doctoral Fellowship (to A. D. Wickenden).Funding from the Alan Tiffin Trust and the Centre for CardiovascularResearch for equipment is also gratefully acknowledged. The anti-Kv1.4and anti-Kv4.2 antibodies and rat brain protein were kindly providedby Dr. O. T. Jones, Department of Pharmacology, University ofToronto and the Playfair Neuroscience Unit, the TorontoHospital.

Present address of A. D. Wickenden: ICAgen Inc., 4222 Emperor Blvd., Suite 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, CCRW 3-802, the Toronto Hospital (General Division), 101 College St., Toronto, Ontario, Canada M5G 2C4 (E-mail: p.backx{at}utoronto.ca).

Received 27 January 1998; accepted in final form 3 February 1999.

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