Molecular Heterogeneity of the Voltage-Gated Fast Transient Outward K+ Current, IAf, in Mammalian Neurons

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The Journal of Neuroscience, October 15, 2001, 21(20):8004-8014

Molecular Heterogeneity of the Voltage-Gated Fast Transient Outward K⁺ Current, I_Af, in Mammalian Neurons
Sacha A. Malin and Jeanne M. Nerbonne
Department of Molecular Biology and Pharmacology, Washington University School of Medicine, St. Louis, Missouri 63110

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Recently, we identified four kinetically distinct voltage-gated K⁺ currents, I_Af, I_As, I_K, and I_SS, in rat superior cervical ganglion(SCG) neurons and demonstrated that I_Af and I_As are differentiallyexpressed in type I (I_Af, I_K, I_SS), type II (I_Af, I_As, I_K, I_SS),and type III (I_K, I_SS) SCG cells. In addition, we reported thatI_Af is eliminated in most (~70%) SCG cells expressing Kv4.2W362F,a Kv4 subfamily-specific dominant negative. The molecular correlate(s)of the residual I_Af, as well as that of I_As, I_K, and I_SS, however,are unknown. The experiments here were undertaken to explore therole of Kv1 $alpha$ -subunits in the generation of voltage-gated K⁺ currents in SCG neurons. Using the Biolistics Gene Gun, cDNAconstructs encoding a Kv1 subfamily-specific dominant negative,Kv1.5W461F, and enhanced green fluorescent protein (EGFP) wereintroduced into SCG neurons. Whole-cell recordings from EGFP-positiveKv1.5W461F-expressing cells revealed a selective decrease in thepercentage of type I cells and an increase in type III cells,indicating that I_Af is gated by Kv1 $alpha$ -subunits in a subset oftype I SCG neurons. I_Af is eliminated in all SCG cells expressingboth Kv1.5W461F and Kv4.2W362F. I_Af $tau$ _decay values in Kv1.5W461F-expressingand Kv4.2W362F-expressing type I cells are significantly different,revealing that Kv1 and Kv4 $alpha$ -subunits encode kinetically distinctI_Af channels. Expression of Kv1.5W461F increases excitabilityby decreasing action potential current thresholds and convertsphasic cells to adapting or tonic firing. Interestingly, the molecularheterogeneity of I_Af channels has functional significance becauseKv1- and Kv4-encoded I_Af play distinct roles in the regulationof neuronalexcitability.

Key words: K⁺ channels; I_A; Kv1 $alpha$ -subunits; Kv4 $alpha$ -subunits; Kv1.5W461F; transgenics; gene gun; neuronal excitability; repetitive firing patterns

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

K⁺ channels are important determinants of membrane excitability, and differences in K⁺ channel expression influence action potential waveforms, repetitivefiring patterns, and synaptic integration (Pongs, 1999; Hausseret al., 2000). Electrophysiological studies have revealed thatmost mammalian neurons express multiple types of voltage-gatedK⁺ current components with distinct time- and voltage-dependentproperties (Rudy, 1988; Storm, 1990). In addition, a number ofvoltage-gated K⁺ (Kv) channel pore-forming ( $alpha$ ) and accessory (Kv $beta$ and KChIP) subunitsthat underlie these channels have been identified (Coetzee etal., 1999; Pongs, 1999; An et al., 2000), and there is presentlyconsiderable interest in identifying the molecular correlatesand defining the functional roles of the various voltage-gatedK⁺ currents in mammalianneurons.

Recently, we reported that sympathetic neurons isolated from the rat superior cervical ganglion (SCG) express multiple, kineticallydistinct, voltage-gated K⁺ current components: two transient A-type currents, I_Af and I_As;a delayed rectifier current, I_K; and a steady-state non-inactivatingcurrent, I_SS (Malin and Nerbonne, 2000). Although I_K and I_SS arepresent in all rat SCG neurons, I_Af and I_As are differentiallydistributed; I_Af is detected in ~90% of cells and, in a subsetof these cells (~20%), I_As is also expressed (Malin and Nerbonne,2000). Based on these expression patterns, three cell types weredistinguished: type I cells (I_Af, I_K, I_SS), type II cells (I_Af,I_As, I_K, I_SS), and type III cells (I_K, I_SS) (Malin and Nerbonne,2000). In addition, we exploited a molecular genetic strategyto assess directly the role of Kv4 $alpha$ -subunits in the generationof voltage-gated K⁺ currents in these cells. These experiments revealed that expressionof Kv4.2W362F, a Kv4 subfamily-specific dominant negative (Barryet al., 1998), results in the elimination of I_Af in most (~70%)SCG cells (Malin and Nerbonne, 2000). The molecular correlate(s)of the residual I_Af, as well as of I_As, I_K, and I_SS, have notbeendefined.

Previous studies have documented the expression of mRNAs encoding several Kv $alpha$ - and $beta$ -subunits in SCG neurons, including severalmembers of the Kv1 subfamily, Kv1.1, Kv1.2, Kv1.4, and Kv1.5 (Dixonand McKinnon, 1996; Pankevych et al., 1999). Interestingly, previousstudies have shown that heterologous expression of Kv1 $alpha$ -subunitsalone or in combination with Kv $beta$ subunits gives rise to voltage-gatedK⁺ currents with a wide range of time- and voltage-dependent properties(Coetzee et al., 1999). In addition, it has recently been demonstratedthat Kv1 $alpha$ -subunits encode distinct types of voltage-gated K⁺ currents in myocardial cells (Feng et al., 1997; Bou-Abboud andNerbonne, 1999; Guo et al., 1999, 2000; London et al., 2001).In mouse ventricular myocytes, for example, Kv1.4 encodes theslow transient K⁺ current, I_to,s (Guo et al., 1999, 2000), and Kv1.5 underliesone component of the slow delayed rectifier current I_K,slow (Londonet al., 2001). These observations led us to hypothesize that Kv1 $alpha$ -subunits might contribute to the formation of one or more voltage-gatedK⁺ currents in rat SCG neurons, and the experiments here were undertakento test this hypothesisdirectly.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

SCG neurons in vitro. Sympathetic neurons were isolated from the SCGs of embryonic day 21 to postnatal day 1 Long-Evans ratpups using a procedure similar to that described by Chang et al.(1990). Briefly, after anesthesia with 5% halothane, animals weredecapitated, and the SCGs were removed. Ganglia were successivelyincubated for 30 min periods in collagenase and trypsin at roomtemperature; isolated SCG neurons were obtained by triturationand subsequent centrifugation. Dissociated SCG cells were resuspendedin growth medium (Earle's Minimum Essential Medium with 10% fetalcalf serum, 0.14 mM L-glutamine, 100 U/ml penicillin-streptomycin,and 0.05 mM NGF) and plated at a density of 2.5 × 10⁴ cells per square centimeter on glial monolayers (prepared asin Raff et al., 1979). Cells were maintained at 37°C in a 95%O₂/5% CO₂ incubator, and the medium was exchanged with fresh growthmedium approximately every 48hr.

Immunohistochemistry. The affinity-purified rabbit polyclonal anti-Kv1.2 antibody used here was raised against residues 468-486in the C terminus of Kv1.2 and has been shown to reliably andspecifically detect Kv1.2 (Barry et al., 1995). The Kv1.4-specificantibody was targeted against residues 13-37 in the N-terminalregion of Kv1.4 and has been shown previously to detect Kv1.4with no detectable cross-reactivity to other Kv1 subfamily members(Barry et al., 1995). The anti-Kv1.5 antibody, purchased fromUBI (Lake Placid, NY; catalog #06-463), was generated againstamino acid residues 542-602 in the C terminus of Kv1.5 and hasbeen demonstrated to be specific for Kv1.5 (Barry et al., 1995).For immunohistochemistry, cells were fixed in 4% paraformaldehydefor 30 min, incubated in blocking buffer (PBS containing 5% normalgoat serum, 0.02% Triton X-100, and 0.1% NaNH₃) for 1 hr, andexposed to one of the Kv1 $alpha$ -subunit-specific primary antibodies(1:100 dilution) at 4°C overnight. After washing with PBS, cultureswere incubated first with a biotinylated goat anti-rabbit antibody(1:200 dilution; Chemicon, Temecula, CA) for 1 hr at room temperature,washed again, and then exposed to an avidin-conjugated horseradishperoxidase for 1 hr at room temperature (ABC kit; Vector Laboratories,Burlingame, CA). The cultures were washed again before incubationwith 0.05% diaminobenzidine in PBS. The progress of the reactionwas monitored under the microscope, and the reactions were quenchedafter ~5 min by washing with PBS. A mouse monoclonal anti-mycantibody (Calbiochem, La Jolla, CA) was used at a 1:100 dilutionto detect Kv1.5W461F-myc protein expression in transfected SCGneurons. Cultures were fixed, blocked, and incubated in primaryantibody as described above. After washing, cultures were incubatedwith a Cy3-conjugated rabbit anti-mouse IgG secondary antibody(Chemicon), and labeled cells were visualized under epifluorescenceillumination.

Transfection of isolated SCG neurons. In control experiments, 1.6 µm gold beads were coated with pCMV-EGFP (Clontech, Cambridge,UK) and propelled (450 psi; 2 mm carrier distance) into SCG neuronsat 4 d in vitro using the Gene Gun (Bio-Rad, Hercules, CA), abiolistic projectile system. After transfections, the culturesappeared healthy, and expression of EGFP was readily detected24 hr later (see Results). In experiments aimed at examining theeffects of Kv1.4, Kv1.5W461F or Kv4.2W362F + Kv1.5W461F expressionin SCG neurons, the gold particles were coated with pBK-CMV-Kv1.4and pCMV-EGFP (4:1 ratio); pBK-CMV-Kv1.5W461F-myc and pCMV-EGFP(4:1 ratio); or pBK-CMV-Kv4.2W362F-FLAG, pBK-CMV-Kv1.5W461F-mycand pCMV-EGFP (4:4:1 ratio). In all cases, a total of 10 µg ofDNA was used in coating the beads. Because EGFP expression wasused to identify transfected neurons for subsequent electrophysiologicalcharacterization, immunohistochemical experiments were performedto determine whether EGFP-expressing cells also expressed theKv1.5W461F-myc construct (seeResults).

Electrophysiological recording. Whole-cell recordings were obtained from isolated SCG neurons at room temperature (22-25°C).Data were collected using an Axopatch-1B patch-clamp amplifier,and experiments were controlled with a P5-120 Gateway 2000 computerthrough a TL-1 DMA interface using the pClamp7 software package(Axon Instruments, Foster City, CA). Electrodes were fabricatedfrom soda-lime glass (Chase 2502) with a two-stage puller, andthe shanks were coated with a silicone elastomer (Sylgard; DowCorning, Midland, MI). Pipette resistances were 1.5-3 M $Omega$ afterfire-polishing. For voltage-clamp recordings, the bath solutionroutinely contained (in mM): 140 NaCl, 4 KCl, 2 CaCl₂, 2 MgCl₂,10 HEPES, 5 glucose, 0.001 TTX, and 0.1 CdCl₂, pH 7.5, 300 mOsm.Recordings were also obtained from SCG neurons in the current-clampmode, and the TTX and CdCl₂ were omitted from the bath for thesestudies. The pipette solution for both current- and voltage-clamprecordings contained (in mM): 135 KCl, 10 HEPES, 5 glucose, 3MgATP, 0.5 NaATP, 2 EGTA, 1.1 CaCl₂, pH 7.5, 300 mOsm. Seriesresistances, estimated from the decays of the uncompensated capacitativetransients, were 2-5 M $Omega$ and were compensated electronically by~80-90%. Because current amplitudes were <10 nA, the voltage errorsresulting from the uncompensated series resistance were always<10 mV and were not corrected. Voltage-gated K⁺ currents were evoked during 125 msec or 6 sec depolarizing voltagesteps to test potentials between $-$ 40 mV and +50 mV from a holdingpotential of $-$ 90 mV. Single action potentials and action potentialtrains were recorded in response to brief (1.5 msec) 200-400 pAand prolonged (500 msec) 20-200 pA depolarizing currentinjections.

Data analysis. Data were compiled and analyzed using pClamp7 and Excel (Microsoft, Seattle, WA) software and are presentedas means ± SEM. The decay phases of the capacitative transientswere analyzed, and only cells in which >90% of the amplitude ofthe capacitative transient decayed with a single exponential timecourse were included in this study. Only data obtained from cellswith input resistances >100 M $Omega$ were analyzed and included here.The mean ± SEM input resistance and capacitance of EGFP-expressingSCG neurons were 0.34 ± 0.03 G $Omega$ and 32 ± 2 pF (n = 43), respectively.Leak currents were <100 pA (at $-$ 70 mV) and were not subtracted.To determine the amplitudes and the decay time constants of theindividual components of the total depolarization-activated outwardK⁺ currents in SCG neurons, the inactivation phases of the currentsrecorded during prolonged (6 sec) depolarizations were analyzedusing the equation: y = A₁e^t/1 + A₂e^t/2 + A₃e^t/3 + C, where A₁, A₂, and A₃ (measured in picoamperes per picoFarad)are the amplitudes of the inactivating current components (I_Af,I_As, and I_K) that decay with time constants $tau$ ₁, $tau$ ₂, and $tau$ ₃ (measuredin milliseconds), respectively, and C is the steady-state current(measured in picoamperes per picoFarad) remaining at the end ofthe 6 sec depolarizations (see Results). Fits were obtained usingCLAMPFIT6, and best fits were determined by eye (in all cases, $sigma$ < 30 pA). All current-clamp recordings were obtained from cellswith overshooting action potentials and stable resting membranepotentials negative to $-$ 40 mV. Action potential durations weremeasured at 50% (APD₅₀) and 90% (APD₉₀) repolarization. Statisticalsignificance was examined with the Student's t test; where appropriate,p values are presented in thetext.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Heterogeneity of outward K⁺ current waveforms in SCG neurons

Previously, we have shown that the waveforms of the Ca²⁺-independent, depolarization-activated K⁺ currents in isolated rat SCG neurons are highly stereotyped (Malinand Nerbonne, 2000). The records presented in Figure 1, left panel,are representative of the three distinct phenotypes observed;they are referred to as types I, II, and III. Most (>90%) wild-typeSCG cells express a prominent rapid component of current decay,consistent with the presence of the fast transient "A-type" current,referred to as I_Af (Malin and Nerbonne, 2000). The exception istype III cells, which express only a slowly decaying outward K⁺ current, I_K, and a non-inactivating current, I_SS (Fig. 1, leftpanel; Table 1). In type I SCG cells (Fig. 1, left panel), thedecay phases of the currents are well fitted by the sum of twoexponentials, reflecting the presence of I_Af (mean ± SEM $tau$ _decay= 121 ± 14 msec), I_K (mean ± SEM $tau$ _decay = 2560 ± 187 msec), andthe non-inactivating current I_SS (Table 1). In addition to I_Af,I_K, and I_SS, a more slowly inactivating, transient outward K⁺ current, referred to as I_As, (mean ± SEM $tau$ _decay 480 ± 21 msec)is present in type II SCG cells (Fig. 1, left panel; Table 1).The decay properties of the individual current components aresimilar in types I, II, and III SCG cells, although there aremarked differences in current densities (Table 1).

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Figure 1. Distinct effects of expression of Kv4.2W362F or Kv1.5W461F on voltage-gated outward K⁺ currents in SCG neurons. Whole-cell voltage-gated outward K⁺ currents were recorded from isolated SCG neurons in response to 6 sec depolarizing voltage steps to test potentials between $-$ 10 and +50 mV from a holding potential of $-$ 90 mV. Experiments were conducted as described in Materials and Methods with 1 µM TTX and 100 µM CdCl₂ in the bath solution to block voltage-gated inward Na⁺ and Ca²⁺ currents, respectively. The records in the left, middle, and right panels were recorded from wild-type, Kv4.2W362F-expressing, and Kv1.5W461F-expressing cells, respectively. There are distinct and stereotyped differences in the waveforms of the currents in wild-type I, II, and III SCG cells (see Results). There is, for example, a prominent rapid component of current decay, I_Af, in type I and II cells that is not evident in type III cells. The numbers given above the records in each column reflect the percentages of cells studied under each experimental condition that display the type I, II, or III phenotype. Expression of either Kv4.2W362F (middle) or Kv1.5W461F (right) decreases the percentage of type I cells and increases the percentage of type III cells. Kv4.2W362F expression also eliminates I_Af in type II cells (see Results) (Malin and Nerbonne, 2000).


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Table 1. Outward K⁺ currents in wild-type SCG neurons expressing Kv4.2W362F and/or Kv1.5W461F^{^a}

In previous studies, we also demonstrated that expression of a pore mutant of Kv4.2, Kv4.2W362F, which functions as a Kv4-specificdominant negative (Barry et al., 1998), eliminates I_Af in most(~70%) SCG neurons (Malin and Nerbonne, 2000). The expressionof Kv4.2W362F (Fig. 1, middle panel) results in a marked increasein type III cells, which express only I_K and I_SS, and revealsa novel phenotype (i.e., one not seen in wild-type SCG cells)in which only I_As, I_K, and I_SS are present (Malin and Nerbonne,2000). In a subset (~20%) of type I SCG cells expressing Kv4.2W362F(Fig. 1, middle panel, top), however, I_Af is evident (Table 1).These observations suggested either that Kv4.2W362F expressionwas insufficient to eliminate I_Af in some cells or, alternatively,that the fast transient outward K⁺ current in a subset of type I SCG neurons is not encoded by $alpha$ -subunitsof the Kv4 subfamily. The mean density of I_Af (64 ± 20 pA/pF)in type I cells expressing Kv4.2W362F is not significantly differentfrom the mean I_Af density (81 ± 11 pA/pF) in wild-type I cells(Table 1). Analysis of the decay phases of the currents, however,revealed that the mean ± SEM inactivation time constant (190 ±18 msec) of the residual I_Af is significantly larger than in wild-type(I or II) SCG cells (Table 1) (Malin and Nerbonne, 2000). Inaddition, examination of the distribution of I_Af inactivationtime constants (Fig. 2) in wild-type I SCG cells suggested thepresence of two distinct I_Af components: one with $tau$ _decay valuesbetween 50 and 130 msec, and another with $tau$ _decay values between131 and 210 msec (Fig. 2). Interestingly, expression of Kv4.2W362Fdramatically shifts the distribution of $tau$ _decay values in the remainingtype I cells; the range of $tau$ _decay values in Kv4.2W362F-expressingtype I cells is 138-249 msec, with a mean of 190 ± 18 msec (Fig.2) (Malin and Nerbonne, 2000). These observations were interpretedas suggesting that, in a subset of type I SCG cells, I_Af is notencoded by $alpha$ -subunits of the Kv4 subfamily (Malin and Nerbonne,2000).

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Figure 2. Distinct components of I_Af inactivation in SCG neurons. The time constants of inactivation of the rapid component of current decay, I_Af, were determined in wild-type, Kv4.2W362F-expressing, and Kv1.5W461F-expressing SCG cells as described in Materials and Methods. The $tau$ _decay values were binned in 40 msec increments for comparison purposes and, as is evident, the distributions of $tau$ _decay values in wild-type, Kv4.2W362F-expressing, and Kv1.5W461F-expressing SCG cells are distinct.

Expression of Kv1 $alpha$ -subunits in SCG neurons

Although the previous studies clearly documented a role for Kv4 $alpha$ -subunits in the generation of I_Af in the majority of SCGneurons (Malin and Nerbonne, 2000), the molecular correlate(s)of the residual I_Af, as well as I_As, I_K, and I_SS, remain to beidentified. Previous molecular studies have demonstrated thatseveral Kv $alpha$ -subunits, in addition to Kv4.2 and Kv4.3, as wellas several Kv $beta$ -subunits are expressed in rat SCG neurons (Dixonand McKinnon, 1996; Pankevych et al., 1999). In heterologous systems,expression of Kv1 $alpha$ -subunits, alone or in combination with accessory $beta$ -subunits, gives rise to voltage-gated K⁺ currents with diverse kinetic and voltage-dependent properties,suggesting that Kv1 subfamily members may contribute to one ormore outward K⁺ currents in rat SCG (and other) neurons. Importantly, previousstudies have shown that several Kv1 $alpha$ -subunits, including Kv1.1,Kv1.2, Kv1.4, and Kv1.5, and Kv $beta$ -subunits are expressed at themessage level in SCG neurons (Dixon and McKinnon, 1996; Pankevychet al., 1999), suggesting that Kv1 $alpha$ -subunits likely play a rolein the generation of voltage-gated K⁺ currents in these cells. To examine Kv1 $alpha$ -subunit protein expressionin SCG cells, therefore, immunohistochemical experiments withanti-Kv1 $alpha$ -subunit-specific antibodies were undertaken. Theseexperiments revealed that Kv1 $alpha$ -subunits are readily detectedin isolated SCG neurons at the protein level (Fig. 3). As is illustratedin Figure 3B, for example, Kv1.4 expression is readily detectedin the cell bodies of isolated SCG neurons. The expression patternfor Kv1.2 is distinct (from that of Kv1.4) in that Kv1.2 stainingis seen throughout the processes of isolated SCG neurons, whereasKv1.4 is only detected in cell bodies and proximal processes (Fig.3A,B). In addition, all SCG cells are labeled with the anti-Kv1.2antibody (Fig. 3A), whereas only a subset of cells express Kv1.4(Fig. 3B). In contrast, Kv1.5 protein expression was not detectedin SCG neurons (Fig. 3C).

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Figure 3. Expression of Kv1 $alpha$ -subunits in SCG neurons. Isolated wild-type SCG neurons were fixed and probed with polyclonal antibodies generated against Kv1.2 (A), Kv1.4 (B), or Kv1.5 (C) 48 hr after plating, as described in Materials and Methods. As is evident, the Kv1.2 and Kv1.4 $alpha$ -subunits are readily detected in SCG neurons, although the staining patterns of these subunits are distinct. Scale bars, 50 µm.

Expression of Kv1.5W461F eliminates I_Af in a subset of SCG neurons

To explore directly the role of Kv1 $alpha$ -subunits, the Kv1 subfamily-specific dominant negative construct, Kv1.5W461F-myc (Liet al., 1999), was used. Previous studies have shown that heterologousco-expression [in human embryonic kidney (HEK)-293 cells] of Kv1.5W461F-mycwith either Kv1.5 or Kv1.4 attenuates current amplitudes relativeto cells expressing (wild-type) Kv1.5 or Kv1.4 alone (Li et al.,1999). To examine the effects of Kv1.5W461F expression on theoutward K⁺ currents in SCG neurons, beads were coated with cDNA constructsencoding Kv1.5W461F-myc and EGFP, and SCG cells were transfectedusing the Biolistic Gene Gun (see Materials and Methods). Within~24 hr of transfection, EGFP was readily detected under epifluorescenceillumination (Fig. 4); ~10% of the cells in these cultures wereEGFP-positive. To determine whether EGFP-positive SCG cells alsoexpress the Kv1.5W461F transgene, the cultures were fixed ~48hr after transfection and probed with an anti-myc antibody. Theseexperiments revealed that all EGFP-positive cells (n = 100) alsoexpress Kv1.5W461F-myc. An example of an EGFP-positive, Kv1.5W461F-myc-positiveSCG cell is shown in Figure 4, (bottom panels). The myc stainingappears to be predominantly on the cell surface (arrowheads),whereas EGFP expression is detected in the cytosol (Fig. 4, bottom).

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Figure 4. Expression of Kv1.5W461F-myc in transfected SCG neurons. Isolated SCG neurons, transfected with EGFP alone (top) or with Kv1.5W461F-myc and EGFP (bottom) using the gene gun, were fixed and stained 24 hr later (see Materials and Methods). The top and bottom panels show EGFP fluorescence (left) and Cy3 fluorescence (right) images of the same field. Anti-myc staining is only evident in cultures transfected with Kv1.5W461F-myc (compare right panels, top and bottom). In addition, EGFP expression correlates with Kv1.5W461F (bottom, compare left and right panels). Scale bar, 50 µm.

Representative whole-cell voltage-gated outward K⁺ current waveforms recorded from Kv1.5W461F-expressing SCG cells are presentedin Figure 1 (right panel). In Kv1.5W461F-expressing type I cells(Fig. 1, right panel), I_Af is evident, and the mean ± SEM currentdensity (57 ± 6 pA/pF) is similar to that seen in wild-type Icells (Table 1). Mean ± SEM I_K (90 ± 13 pA/pF) and I_SS (52 ±8 pA/pF) densities in Kv1.5W461F-expressing type I cells are alsosimilar to the densities in wild-type I cells (Table 1). Thepercentage (44%; 15 of 34) of type I SCG neurons, however, issubstantially lower than seen in recordings from wild-type cells,in which 70% of cells are classified as type I (Fig. 1, left panel).In parallel with the decrease in the percentage of type I cells,there is a marked increase in the percentage of type III cells(Fig. 1, compare left and right panels), which express only I_Kand I_SS. In contrast, the percentage of Kv1.5W461F-expressingcells classified as type II is similar to the percentage of wild-typecells displaying this phenotype (Fig. 1, compare left and rightpanels). The densities of the currents and mean ± SEM $tau$ _decay valuesfor I_Af (72 ± 8 msec), I_As (585 ± 47 msec), and I_K (3125 ± 438msec) in Kv1.5W461F-expressing type II cells are not significantlydifferent from those in wild-type II cells (Table 1). These observationssuggest that Kv1 $alpha$ -subunits do not contribute measurably to thevoltage-gated outward K⁺ currents in wild-type II SCG cells (seeDiscussion).

The concomitant decrease in type I cells and the increase in type III cells with the expression of Kv1.5W461F suggests thatthe functional removal of channels encoded by Kv1 $alpha$ -subunits converts~25% of type I cells to type III by specific elimination of I_Af.The expression of Kv1.5W461F also results in a shift in the distributionof $tau$ _decay values for I_Af (Fig. 2). In cells expressing Kv1.5W461F, $tau$ _decay values range from 54 to 150 msec, with a mean ± SEM valueof 88 ± 8 msec (Table 1). This value is significantly (p < 0.001)smaller than the mean ± SEM $tau$ _decay (190 ± 18 msec) for I_Af remainingin Kv4.2W362F-expressing cells (Table 1, Fig. 2), consistentwith the hypothesis that there are two molecularly distinct componentsof I_Af.

I_Af is eliminated in all SCG cells co-expressing Kv4.2W362F and Kv1.5W461F

To test the hypothesis that there are two populations of I_Af channels encoded by distinct Kv subfamilies, SCG cells were cotransfectedwith Kv1.5W461F and Kv4.2W362F (and EGFP). Representative outwardK⁺ currents recorded from EGFP-positive cells are presented in Figure5. As is evident, the rapidly inactivating I_Af, prominent in wild-typeSCG cells (Fig. 1, left panels), is not evident in cells expressingKv4.2W362F and Kv1.5W461F (Fig. 5). The majority (~75%) of Kv4.2W362F-Kv1.5W461F-expressingcells are classified as type III (Fig. 5). This is a significantincrease in type III cells, compared with wild-type, Kv4.2W362F-expressing,or Kv1.5W461F-expressing cells (Fig. 1). The mean ± SEM densitiesof I_K (135 ± 60 pA/pF) and I_SS (86 ± 12 pA/pF) in the Kv1.5W461F-Kv4.2W362F-expressingtype III cells are not significantly different from the densitiesof these currents determined in wild-type III cells (Table 1).Analysis of the outward K⁺ currents in the remaining (~25%) cells reveals the presence ofI_As, I_K, and I_SS, suggesting that these are type II cells lackingI_Af (Table 1).

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Figure 5. Coexpression of both Kv1.5W461F and Kv4.2W362F eliminates I_Af. Isolated SCG neurons were transfected with Kv1.5W461F, Kv4.2W362F, and EGFP using the Biolistic Gene Gun (as described in Materials and Methods), and outward K⁺ currents were recorded from EGFP-positive cells as described in the legend to Figure 1. Two distinct current waveforms were evident in these recordings: the vast majority (76%) of cells were found to express only I_K and I_SS and were classified as type III (B); the remaining cells (24%) express I_As, I_K, and I_SS, and, therefore, are type II cells lacking I_Af (A). The fast transient current I_Af was not detected in any of these cells (n = 15). Analysis of the decay phases of the currents revealed that the densities of I_As, I_K, and I_SS in Kv1.5W461F + Kv4.2W362F-expressing type II and III cells are indistinguishable from the currents in wild-type II and III cells (Table 1).

Expression of Kv1.5W461F increases excitability of SCG cells

Subsequent experiments were aimed at determining the effects of eliminating the Kv1-mediated I_Af on the waveforms of individualaction potentials and the repetitive firing properties of SCGneurons. As reported previously, current-clamp recordings fromwild-type SCG cells reveal that ~45% of the cells are "phasic,"firing one or two action potentials in response to a prolonged(500 msec) depolarizing current injection (Malin and Nerbonne,2000). Increasing the amplitude of the injected current does notmarkedly influence the number of action potentials recorded (Malinand Nerbonne, 2000). Approximately 30% of wild-type SCG cellsdisplay the "adapting" phenotype. In these cells, low-amplitudecurrent injections produce repetitive firing, and the firing frequencydecreases over time. At higher amplitude current injections, adaptingcells cease firing and are refractory (Malin and Nerbonne, 2000).Adapting cells are further distinguished from phasic cells byincreased input resistances and decreased current thresholds foraction potential generation (Table 2). The remaining (~25%) wild-typeSCG neurons are "tonic," regular-spiking cells that fire at afixed frequency during prolonged current injections up to 300pA (Malin and Nerbonne, 2000). In addition, individual actionpotentials in tonic cells are brief (Table 2), and the firingfrequency increases with the amplitude of the injected current(Malin and Nerbonne, 2000). Briefer action potential durationsand the lack of adaptation (Table 2) clearly distinguish tonicfrom phasic and adapting SCG neurons.


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Table 2. Effects of Kv1.5W461F and Kv4.2W362F expression on SCG neuron firing properties^{^a}

The phasic, adapting, and tonic firing patterns are also seen in recordings obtained from Kv1.5W461F-expressing SCG cells(Fig. 6). The distribution of SCG cell firing patterns, however,is markedly affected by Kv1.5W461F expression. Functional eliminationof Kv1-encoded I_Af channels reduces the number of phasic cells(Fig. 6A) from 43% of wild-type to 24% of Kv1.5W461F-expressingcells (Table 2). In contrast, the percentage of adapting cells(Fig. 6B) increases from 32% of wild-type to 44% of Kv1.5W461F-expressingcells (Table 2). The percentage of tonic cells (Fig. 6C) is alsoincreased slightly (from 25 to 32%) with Kv1.5W461F expression(Table 2). Thus, the selective removal of the Kv1-mediated I_Afconverts many (~40%) phasic cells to the adapting or tonic firingpatterns (Fig. 6, Table 2). Interestingly, the percentage oftype I cells with Kv1-encoded I_Af channels (~25%) is very similarto the percentage of cells (~20%) converted from phasic firingwith Kv1.5W461F expression, suggesting that type I cells withKv1-encoded I_Af channels are phasic (see Discussion). In contrastto the findings with Kv4.2W362F, however, expression of Kv1.5W461Fdoes not affect the input resistances of phasic or tonic cells(Table 2). Thus, the properties of Kv1- and Kv4-encoded I_Af channelsare distinct, in that Kv1-encoded I_Af channels are not open atrest and, therefore, do not contribute to the resting input resistancesof SCG neurons.

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Figure 6. Expression of Kv1.5W461F increases the percentage of adapting cells. Isolated SCG neurons were transfected with Kv1.5W461F (and EGFP), and action potentials and repetitive firing patterns were recorded in response to brief or prolonged depolarizing current injections, as described in Materials and Methods. Current-clamp recordings from (3) representative Kv1.5W461F-expressing cells are shown in A, B, and C. In each cell, single action potentials were elicited by 1.5 msec current injections (left), and repetitive firing patterns were recorded in response to 100 pA (middle) or 200 pA (right) 500 msec current injections. On the basis of the response(s) to the 500 msec current injections, cells were classified as phasic (A), adapting (B), or tonic (C) (Table 2). With Kv1.5W461F expression, the percentages of adapting and tonic cells are increased, and the percentage of phasic cells is decreased relative to the firing pattern distribution seen in wild-type cells (Table 2).

Analysis of the properties of the phasic firing cells remaining with Kv1.5W461F expression revealed that the mean ± SEM currentthreshold for action potential generation in the phasic cellslacking Kv1-encoded I_Af (i.e., the remaining phasic cells) issignificantly (p < 0.005) lower than the mean determined in wild-typephasic cells (Table 2). In addition, the mean ± SEM action potentialamplitude in the remaining phasic cells is significantly (p <0.03) larger than in wild-type phasic cells (Table 2). Theseobservations are consistent with the suggestion that there aretwo distinct populations of phasic SCG cells and, further, thatthe current thresholds for action potential generation are lowerand action potential amplitudes are higher in the subset of phasiccells lacking Kv1-encoded I_Af channels. Action potential durationsin the remaining phasic cells are also decreased significantly(p < 0.005) compared with wild-type phasic cells (Table 2). Thisunexpected observation suggests that there are additional repolarizingcurrents activated in phasic cells lacking Kv1-encoded I_Af channels,perhaps because of the increased action potential amplitudes inthese cells (Table 2). The mean ± SEM current threshold valuesfor action potential generation, as well as action potential amplitudesand durations, in adapting and tonic SCG cells, in contrast, arenot affected by Kv1.5W461F expression (Table 2), consistent withthe suggestion that Kv1-encoded I_Af channels specifically tuneexcitability in phasic cells (seeDiscussion).

Complete removal of I_Af markedly increases excitability and further reduces the percentage of phasic cells

In SCG neurons transfected with both the Kv1.5W461F and the Kv4.2W362F dominant negative constructs, the distribution of repetitivefiring patterns is altered markedly (Fig. 7D) compared with wild-typecells (Fig. 7A), as well as with cells expressing Kv4.2W362F (Fig.7B) or Kv1.5W461F (Fig. 7C) alone. After the complete removalof I_Af, few phasic cells remain (13%) (Fig. 7D), and the percentagesof adapting and tonic cells are increased. These effects appearto be the sum of the Kv1- and Kv4-mediated changes; removal ofeither the Kv1- or the Kv4-encoded I_Af channels alone increasesthe percentage of adapting cells at the expense of phasic cells,and removal of Kv1 channels also increases tonic cell number (Fig.7). As seen with the expression of Kv4.2W362F alone, the mean± SEM input resistance of SCG cells expressing Kv1.5W461F andKv4.2W362F is significantly (p < 0.005) increased compared withwild-type cells (Table 2). These findings are expected becauseexpression of Kv4.2W362F alone significantly affects the mean± SEM input resistance (Table 2). Expression of Kv1.5W461F andKv4.2W362F, like expression of either Kv1.5W461F or Kv4.2W362Falone, also decreases the current thresholds for action potentialgeneration (Table 2).

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Figure 7. Elimination of the Kv1- and Kv4-encoded I_Af increases the percentage of adapting SCG neurons. Action potentials and repetitive firing patterns were recorded from isolated SCG neurons 24 hr after transfection with EGFP alone (A), EGFP and Kv4.2W362F (B), EGFP and Kv1.5W461F (C), or EGFP, Kv1.5W461F and Kv4.2W362F (D), as described in the legend to Figure 6. The phasic (left), adapting (middle), and tonic (right) firing patterns were evident in recordings obtained under all of these experimental conditions. In recordings from cells with reduced I_Af density, the percentages of phasic cells are lower, and the percentages of adapting and tonic cells are higher than seen in recordings from wild-type cells (Tables 2, 4, 5).

Increasing Kv1-mediated I_Af converts adapting cells to phasic firing

The experiments described above demonstrate a role for Kv1 $alpha$ -subunits in the generation of I_Af in a subset of type I phasic-firingSCG neurons. Of the Kv1 $alpha$ -subunits, only Kv1.4 produces rapidlyinactivating outward K⁺ currents when expressed alone in heterologous expression systems(Coetzee et al., 1999). In addition, Kv1.4 has recently been shownto underlie the slow transient outward K⁺ current in mammalian cardiac cells (Guo et al., 1999, 2000),and Kv1.4 is expressed at the protein level in SCG neurons (Fig.3). Subsequent experiments, therefore, were aimed at examiningthe effects of "over-expression" of Kv1.4 on the outward K⁺ currents and the firing properties of SCG neurons. Representativecurrent-clamp recordings from Kv1.4-expressing cells are shownin Figure 8. The percentage of phasic cells (Fig. 8A) is increasedmarkedly (to 67%) with Kv1.4 expression, relative to the percentage(43%) of wild-type phasic SCG cells (Table 3). The fraction ofadapting cells is decreased (Fig. 8B), whereas the percentageof tonic cells is unchanged (Fig. 8C, Table 3). Indeed, of the18 cells examined, only two adapting cells were detected, suggestingthat Kv1.4 expression converts most adapting cells to phasic firing.Consistent with the increase in phasic cells and the decreasein adapting cells, the mean ± SEM current threshold for actionpotential generation is increased significantly (p < 0.005) inall Kv1.4-expressing SCG cells (Table 3). These data supportour hypothesis that the current threshold for action potentialgeneration is determined largely by I_Af density and is linkedto firing pattern. Expression of Kv1.4 also significantly (p <0.04) decreases mean ± SEM APD₅₀ values in phasic cells, whereasaction potential durations in Kv1.4-expressing tonic and adaptingcells are not significantly different from those in wild-typetonic and adapting cells (Table 3).

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Figure 8. Expression of Kv1.4 increases the percentage of phasic firing SCG cells. Action potentials and repetitive firing patterns, recorded as described in the legend to Figure 6, were obtained from isolated SCG neurons 24 hr after transfection with wild-type Kv1.4 and EGFP. As in wild-type cells, the phasic (A), adapting (B), and tonic (C) firing patterns were seen in recordings from cells transfected with Kv1.4. The percentage of adapting cells, however, is lower and the percentage of phasic cells is higher in Kv1.4-expressing cells than seen in recordings from wild-type or Kv1.5W461F-expressing SCG cells (Figs. 6, 7, Tables 2, 4).


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Table 3. Expression of Kv1.4 decreases the excitability of SCG neurons^{^a}

Representative voltage-clamp recordings obtained from SCG neurons expressing Kv1.4 (and EGFP) are shown in Figure 9. Analysisof the decay phases of the currents revealed that I_Af densityis increased significantly (p < 0.02) to a mean ± SEM value of141 ± 9 pA/pF in Kv1.4-expressing type I cells. In addition, themean ± SEM $tau$ _decay value for I_Af (169 ± 10 msec) in Kv1.4-expressingtype I cells is significantly larger than the mean time constantfor I_Af (121 ± 14 msec) in wild-type I cells (Table 1). Interestingly,over-expression of Kv4.2 reduces the mean ± SEM $tau$ _decay for I_Af(Table 3), revealing that Kv1.4 and Kv4.2 encode kineticallydistinct K⁺ currents when expressed in sympathetic neurons. These differencesare also reflected in the ranges of I_Af $tau$ _decay values seen. Inwild-type I cells, for example, I_Af $tau$ _decay values range from 40to 209 msec (Fig. 9D), whereas in SCG cells expressing Kv1.4,I_Af $tau$ _decay values range from 142 to 205 msec. This change is distinctfrom that seen in SCG cells expressing Kv4.2, in which $tau$ _decayvalues range from 50 to 128 msec (Fig. 9D, Table 4). Thus, exogenousKv1.4 encodes a fast transient current in SCG neurons with inactivationkinetics similar to the component eliminated with Kv1.5W461F expression(Fig. 1, Tables 1, 4). Furthermore, this component is kineticallydistinct from that encoded by Kv4.2 (Fig. 9D, Table 4).

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Figure 9. Expression of Kv1.4 increases I_Af only in type I SCG neurons. Isolated SCG neurons were transfected with Kv1.4 and EGFP using the Biolistic Gene Gun (as described in Materials and Methods), and outward K⁺ currents were recorded from EGFP-expressing cells as described in the legend to Figure 1. Analysis of the decay phases of the currents provided the mean ± SEM densities of I_Af, I_As, I_K, and I_SS (Table 1) and allowed classification of Kv1.4-expressing cells as type I (A), type II (B), or type III (C). The distribution of (type I, type II, and type III) cells is unaffected by Kv1.4 expression, and the mean ± SEM I_Af density is increased significantly (p < 0.001) in type I SCG cells, as compared with wild-type I cells (Table 1). Interestingly, type II and type III cells are unaffected by expression of Kv1.4. The distributions of I_Af $tau$ _decay values in wild-type, Kv4.2-expressing, and Kv1.4-expressing type I cells are distinct, consistent with the hypothesis that Kv4.2 and Kv1.4 encode kinetically distinct fast transient currents in SCG cells (D).


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Table 4. SCG neurons transfected with wild-type Kv4.2 or Kv1.4^{^a}

In contrast, mean I_K and I_SS densities, as well as the kinetics of I_K decay, are not significantly different in Kv1.4-expressingand wild-type I cells (compare Tables 1, 4). Interestingly,Kv1.4 expression has no effect on I_Af density (83 ± 8 pA/pF) intype II cells (Fig. 9B, Table 4). The other currents, I_As, I_K,and I_SS, in type II cells are also unaffected by Kv1.4 expression(Table 4). Similarly, the densities and properties of I_K andI_SS in type III cells expressing Kv1.4 are indistinguishable fromthose seen in wild-type III cells (Tables 1, 4). Together, theseresults suggest that functional Kv1-encoded I_Af channels are notexpressed in type II or type III cells even when the (wild-type)Kv1.4 $alpha$ -subunit is exogenously introduced (seeDiscussion).

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Kv1 $alpha$ -subunits underlie I_Af in a subset of type I SCG neurons

The results of the experiments reported here demonstrate that expression of Kv1.5W461F results in the elimination of I_Af ina subset of type I SCG cells and a corresponding increase in thepercentage of type III cells (Fig. 1, Table 1). The propertiesand the densities of the currents in Kv1.5W461F-expressing typeII and type III cells are indistinguishable from the currentsin wild-type II and III cells, suggesting that Kv1 $alpha$ -subunitsdo not make a significant contribution to I_Af in type II cellsor to I_K and I_SS in type II and III cells. Importantly, the experimentshere also demonstrate that the residual I_Af present in Kv4.2W362F-expressingtype I SCG cells (Malin and Nerbonne, 2000) does not reflect incompletesuppression of Kv4-encoded I_Af channels. Rather, the residualI_Af in the Kv4.2W362F-expressing SCG cells reflects Kv1-encodedI_Af channels. In addition, the mean ± SEM I_Af $tau$ _decay values determinedin Kv1.5W461F- and Kv4.2W362F-expressing cells are significantly(p < 0.001) different (Fig. 2), consistent with the hypothesisthat there are two types of I_Af channels in wild-type SCG neuronsthat reflect the expression of distinct gene products. Becauseco-expression of Kv1.5W461F and Kv4.2W362F eliminates I_Af in allSCG cells (Fig. 5, Table 1), it is also possible to concludethat Kv1 and Kv4 $alpha$ -subunits must encode all of the fast transientcurrent (I_Af) in thesecells.

Previous studies have demonstrated the presence of distinct types of transient outward K⁺ currents in neurons and muscle cells and shown that these areencoded by Kv1 and Kv4 $alpha$ -subunits (Solc et al., 1987; Tsunodaand Salkoff, 1995; Guo et al., 1999, 2000). In contrast to thefindings here, however, the transient outward K⁺ currents in Drosophila neurons and myocytes (Solc et al., 1987;Tsunoda and Salkoff, 1995), as well as those in mammalian cardiacmyocytes (Guo et al., 1999, 2000), display markedly differenttime- and voltage-dependent properties and are readily distinguishedelectrophysiologically. Interestingly, however, the identificationof two molecularly distinct components of a "single" electrophysiologicallydefined current has been reported previously for I_Kr in Xenopusspinal neurons (Ribera, 1996) and for I_K,
slow in mouse ventricularmyocytes (Xu et al., 1999). These findings corroborate the powerof the molecular pharmacological approach exploited here and inthese previous studies (Ribera, 1996; Xu et al., 1999). The Kv $alpha$ -subunit-specific dominant negative strategy selectively eliminatesindividual current components, allowing the characterization ofdetailed properties of the currents remaining (as well as of thecurrents eliminated). In the case of I_Af in SCG neurons, experimentscompleted on cells expressing Kv1.5W461F or Kv4.2W362F revealedthe presence of two current components that had not previouslybeen distinguished using conventional electrophysiological and/orpharmacological methods. The molecular pharmacological approachexploited here also allowed determination of the functional rolesof the individual Kv1- and Kv4-encoded components of I_Af in shapingthe waveforms of individual action potentials and repetitive firingpatterns in SCGneurons.

Functional roles of I_Af in SCG neurons

The experiments completed here reveal that the functional consequences of eliminating the Kv1- or the Kv4-encoded I_Af channelsin SCG cells are distinct, suggesting that the molecular heterogeneityin I_Af has physiological significance. Elimination of Kv1-encodedI_Af increases excitability by decreasing the current thresholdfor action potential generation (Table 5), without measurablyaffecting cell input resistances. Removal of Kv4-encoded I_Af channelsalso increases excitability by lowering current thresholds, although,in this case, input resistances are also increased (Table 5)(Malin and Nerbonne, 2000). In addition, the Kv1- and Kv4-encodedI_Af channels play different roles in controlling repetitive firingin SCG neurons. Although elimination of either Kv1- or Kv4-encodedI_Af reduces (by ~50%) the number of phasic cells (Table 5), removalof the Kv4-encoded I_Af converts phasic cells to adapting firing,whereas removal of the Kv1-encoded I_Af converts some phasic cellsto adapting and others to tonic firing (Fig. 7, Table 2). Interestingly,co-expression of Kv1.5W461F and Kv4.2W362F dramatically reduces,but does not eliminate, the number (percentage) of phasic cells.This finding suggests that, although I_Af is an important contributor,it is not the sole determinant of phasic firing. In addition,expression of Kv4.2W362F significantly (p < 0.02) increases themean (±SEM) firing rates in tonic cells (in response to 200 pAcurrent injections) to 29 ± 2 Hz from the wild-type value of 15± 1 Hz. There is also an increase in the mean ± SEM tonic firingrate in Kv1.5W461F-expressing cells, although, in this case, theincrease (to 20 ± 6 Hz) is modest (~30%) and most Kv1.5W461F-expressingtonic cells fire at frequencies well within the wild-type range(Fig. 7).


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Table 5. Phenotypic consequences of eliminating the Kv1- or Kv4-encoded components of I_Af

As noted above, the experiments here revealed that the voltage-clamp effects of Kv1.5W461F expression are specific to typeI cells; expression of Kv1.5W461F removes I_Af in ~25% of SCG cells,all of which are type I (Fig. 1, Table 1). In addition, expressionof Kv1.5W461F converts ~50% of phasic firing rat SCG cells tothe adapting or tonic firing patterns (Fig. 7, Table 5). Thus,we can conclude that ~50% of the phasic cells are type I. Theexperiments here also revealed that the mean (±SEM) active andpassive membrane properties of the phasic cells remaining withKv1.5W461F expression are distinct from those of wild-type phasiccells (Table 3). Specifically, action potential amplitudes aregreater, and action potential durations are shorter in the phasiccells lacking Kv1-encoded I_Af channels (i.e., the phasic cellsremaining with Kv1.5W461F expression). In contrast, action potentialamplitudes and durations in Kv4.2W362F-expressing and wild-typephasic cells are indistinguishable (Table 5). These observationssuggest that in the phasic cells expressing Kv1-encoded I_Af channels,action potential amplitudes are lower, and action potential durationsare longer than in phasic cells expressing Kv4-encoded I_Afchannels.

The distinct functional roles of Kv1- and Kv4-encoded I_Af likely reflect differences in the voltage dependences of activationof the currents. The results of experiments completed here suggest,for example, that the Kv4-encoded I_Af channels are open at morehyperpolarized potentials (than the Kv1-encoded channels) andaffect neuronal excitability by decreasing resting SCG cell inputresistance (Malin and Nerbonne, 2000). The Kv1-encoded I_Af channels,in contrast, likely are only activated at more depolarized potentialsand influence excitability, therefore, by opposing the actionpotential upstroke; Kv1-encoded I_Af channels do not contributeto resting input resistance in SCG cells. In addition to thisfunctional diversity, the expression of molecularly distinct I_Afchannels encoded by Kv1 and Kv4 $alpha$ -subunits also provides a meansfor differential modulation of channel, and therefore, cellular,functioning through interactions with distinct transmitters and/orintracellular messenger pathways (Roeper et al., 1997; Wang etal., 1997; Pan et al., 2000). Clearly, experiments aimed at exploringthe molecular mechanisms involved in the regulation and modulationof Kv1- and Kv4-encoded neuronal I_Af channels will be of considerableinterest.

  FOOTNOTES

Received May 21, 2001; revised July 9, 2001; accepted July 11, 2001.

This work was supported by a National Science Foundation predoctoral fellowship to S.A.M. and the National Institutes of HealthGrant NS-30676.
Correspondence should be addressed to Dr. Jeanne M. Nerbonne, Washington University Medical School, 660 South Euclid Avenue,Box 8130, St. Louis, MO 63110. E-mail: jnerbonn{at}pcg.wustl.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

An WF, Bowlby MR, Betty M, Cao J, Ling H-P, Mendoza G, Hinson JW, Mattson KI, Strassle BW, Trimmer JS, Rhodes KJ (2000) Modulation of A-type potassium channels by a family of calcium sensors. Nature 403:553-556[Medline].
Barry DM, Trimmer JS, Merlie JP, Nerbonne JM (1995) Differential expression of voltage-gated K⁺ channel subunits in adult rat heart. Relation to functional K⁺ channels? Circ Res 77:361-369[Abstract/Free Full Text].
Barry DM, Xu H, Schuessler RB, Nerbonne JM (1998) Functional knock-out of the transient outward current, long-QT syndrome, and cardiac remodeling in mice expressing a dominant-negative Kv4 $alpha$ -subunit. Circ Res 83:560-567[Abstract/Free Full Text].
Bou-Abboud E, Nerbonne JM (1999) Molecular correlates of the calcium-independent depolarization-activated K⁺ currents in rat atrial myocytes. J Physiol (Lond) 517:407-420[Abstract/Free Full Text].
Chang JY, Martin DP, Johnson Jr EM (1990) Interferon suppresses sympathetic neuronal cell death caused by nerve growth factor deprivation. J Neurochem 55:436-445[ISI][Medline].
Coetzee WA, Amarillo Y, Chiu J, Chow A, Lau D, McCormack T, Moreno H, Nadal MS, Ozaita A, Pountney D, Saganich M, Vega-Saenz de Meira E, Rudy B (1999) Molecular diversity of K⁺ channels. Ann NY Acad Sci 868:233-285[Abstract/Free Full Text].
Dixon JE, McKinnon D (1996) Potassium channel mRNA expression in prevertebral and paravertebral sympathetic neurons. Eur J Neurosci 8:183-191[ISI][Medline].
Feng J, Wible B, Li G-R, Wang Z, Nattel S (1997) Antisense oligodeoxynucleotides directed against Kv1.5 mRNA specifically inhibit ultrarapid delayed rectifier K⁺ current in cultured adult human atrial myocytes. Circ Res 80:572-579[Abstract/Free Full Text].
Guo W, Xu H, London B, Nerbonne JM (1999) Molecular basis of transient outward K⁺ current diversity in mouse ventricular myocytes. J Physiol (Lond) 521:587-599[Abstract/Free Full Text].
Guo W, Li H, London B, Nerbonne JM (2000) Functional consequences of elimination of I_to,f and I_to,s: early afterdepolarizations, atrioventricular block, and ventricular arrhythmias in mice lacking Kv1.4 and expressing a dominant-negative Kv4 $alpha$ -subunit. Circ Res 87:73-79[Abstract/Free Full Text].
Hausser M, Spruston N, Stuart GJ (2000) Diversity and dynamics of dendritic signaling. Science 290:739-744[Abstract/Free Full Text].
Li H, Guo W, Nerbonne JM (1999) Functional consequences of cardiac-specific expression of wild-type or mutant (dominant negative) Kv1.5 $alpha$ -subunits in mouse ventricular myocytes. Circulation 102:II-261.
London B, Guo W, Pan X-H, Lee JS, Shusterman V, Rocco CJ, Logothetis DA, Nerbonne JM, Hill JA (2001) Targeted replacement of Kv1.5 in the mouse leads to loss of the 4-aminopyridine-sensitive component of I_K,slow and resistance to drug-induced QT prolongation. Circ Res 88:940-946[Abstract/Free Full Text].
Malin SA, Nerbonne JM (2000) Elimination of the fast transient in superior cervical ganglion neurons with expression of Kv4.2W362F: molecular dissection of I_A. J Neurosci 20:5191-5199[Abstract/Free Full Text].
Pan S-J, Sumners C, Gelband CH (2000) Kv1.4 underlies angiotensin II-mediated inhibition of neuronal A-type K⁺ current. Biophys J 78:450A.
Pankevych H, Kristufek D, Huck S (1999) Perinatal and postnatal regulation of Shaker-related genes in rat superior cervical ganglion. Soc Neurosci Abstr 25:739.1.
Pongs O (1999) Voltage-gated potassium channels: from hyperexcitability to excitement. FEBS Lett 452:31-35[ISI][Medline].
Raff MC, Fields KL, Hakomori S-I, Mirsky R, Pruss RM, Winter J (1979) Cell-type-specific markers for distinguishing and studying neurons and the major classes of glial cells in culture. Brain Res 174:283-308[ISI][Medline].
Ribera AB (1996) Homogeneous development of electrical excitability via heterogeneous ion channel expression. J Neurosci 16:1123-1130[Abstract/Free Full Text].
Roeper J, Lorra C, Pongs O (1997) Frequency-depen