The Contribution of Dendritic Kv3 K+ Channels to Burst Threshold in a Sensory Neuron

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The Journal of Neuroscience, January 1, 2001, 21(1):125-135

The Contribution of Dendritic Kv3 K⁺ Channels to Burst Threshold in a Sensory Neuron
Asim J. Rashid¹, Ezequiel Morales², Ray W. Turner², and Robert J. Dunn¹
¹ Departments of Neurology and Biology, McGill University, and Center for Research in Neuroscience, Montreal General Hospital, Montreal, Quebec, Canada H3G 1A4, and ² Neuroscience Research Group, University of Calgary, Calgary, Alberta, Canada T2N 4N1

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Voltage-gated ion channels localized to dendritic membranes can shape signal processing in central neurons. This study describesthe distribution and functional role of a high voltage-activatingK⁺ channel in the electrosensory lobe (ELL) of an apteronotid weaklyelectric fish. We identify a homolog of the Kv3.3 K⁺ channel, AptKv3.3, that exhibits a high density of mRNA expressionand immunolabel that is distributed over the entire soma-dendriticaxis of ELL pyramidal cells. The kinetics and pharmacology ofnative K⁺ channels recorded in pyramidal cell somata and apical dendritesmatch those of AptKv3.3 channels expressed in a heterologous expressionsystem. The functional role of AptKv3.3 channels was assessedusing focal drug ejections in somatic and dendritic regions ofan in vitro slice preparation. Local blockade of AptKv3.3 channelsslows the repolarization of spikes in pyramidal cell somata aswell as spikes backpropagating into apical dendrites. The resultingincrease in dendritic spike duration lowers the threshold fora $gamma$ -frequency burst discharge that is driven by inward currentassociated with backpropagating dendritic spikes. Thus, dendriticAptKv3.3 K⁺ channels influence the threshold for a form of burst dischargethat has an established role in feature extraction of sensoryinput.

Key words: potassium channel; Kv3; dendritic spike; action potential; backpropagation; oscillatory discharge; repolarization; DAP; electrosensory

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The kinetic properties and distribution of voltage-gated ion channels are important determinants of postsynaptic excitabilityin central neurons. A major influence on dendritic activity arisesin cells that support an active "backpropagation" of Na⁺ spikes from the soma into the dendritic tree (Turner et al.,1991, 1994; Spruston et al., 1995; Magee et al., 1998; Goldinget al., 1999). These spikes can secondarily activate other ionchannels that augment membrane depolarizations or modify synaptictransmission. For example, Ca²⁺ currents activated by backpropagating spikes are important tothe induction of synaptic plasticity, dendritic transmitter release,and coupling distal dendritic inputs to the soma (Chen et al.,1997; Magee and Johnston, 1997; Larkum et al., 1999). The amplitudeof backpropagating spikes can be regulated in turn by dendriticK⁺ channels, as found in hippocampal pyramidal cells that exhibita fivefold increase in the density of A-type K⁺ channels from the soma to distal apical dendrites (Hoffman etal., 1997). Given the wealth of information gained from molecularbiology on a host of K⁺ channel subtypes (Coetzee et al., 1999), an understanding ofdendritic activity will ultimately depend on identification ofthe distribution, kinetic properties, and molecular structuresof the K⁺ channels that exhibit a dendriticdistribution.

We are interested in the control of backpropagating Na⁺ spikes in pyramidal cells of the apteronotid electrosensory lateralline lobe (ELL). This sensory nucleus receives direct primaryafferent input encoding modulations of external electric fieldsused by these animals for electrolocation (Berman and Maler, 1999).Signal processing by ELL pyramidal cells involves the generationof burst discharge for the purpose of feature extraction (Gabbianiet al., 1996). The burst response depends on depolarizing afterpotentials(DAPs) at the soma that arise from the long duration of Na⁺ spikes backpropagating into the dendrites (Turner et al., 1994).The DAP is potentiated during repetitive spike discharge througha frequency-dependent broadening of dendritic spikes that increasescurrent flow to the soma and contributes to driving the burstdepolarization (Lemon and Turner, 2000). The pivotal role of dendriticspike broadening in regulating DAP amplitude suggests that dendriticK⁺ channels could exert direct control over burst discharge by controllingthe rate of dendritic spikerepolarization.

We now report that an apteronotid homolog of the Kv3.3 K⁺ channel subtype is distributed over the entire soma-dendritic axisof ELL pyramidal cells and acts to repolarize Na⁺ spike discharge in both the soma and proximal apical dendrites(<150 µm). The ability of AptKv3.3 K⁺ channels to repolarize dendritic spikes allows them to contributeto the establishment of the threshold for $gamma$ -frequency oscillatoryburstdischarge.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Kv3 amino acid sequences. Amino acid sequences for rat Kv3.1a,b, 3.2a-d, 3.4a,b, mouse Kv3.3a,b and Drosophila Shaw were obtainedfrom the GenBank/European Molecular Biology Laboratory databases.Accession numbers are as follows: rKv3.1a(Y07521), rKv3.1b(M68880), rKv3.2a (A39402), rKv3.2b (M59211), rKv3.2c(M59313), rKv3.2d (S22703), mKv3.3a (Q63959), mKv3.3b(Q63959), rKv3.4a (X62841), hKv3.4b (M64676), Shaw(M32661).

Isolation of AptKv3.3 cDNA. We previously isolated by PCR a 124 bp DNA fragment spanning the pore and S6 domains of an ApteronotusKv3-type K⁺ channel gene, AptKChFr 3A (Rashid and Dunn, 1998). This fragmentwas used to probe an Apteronotus cDNA library (Bottai et al.,1998). Kv3 cDNAs were identified by sequencing both strands usingthe OpenGene Automated DNA Sequencing System (Visible Genetics,Toronto, Ontario, Canada). The sequences of overlapping cloneswere assembled and the open reading frames were determined usingthe LASERGENE software package (DNASTAR, Madison, WI). The translationstart site for AptKv3.3 was designated as the first methioninecodon downstream of an in-frame stop codon. The AptKv3.3 cDNAsequence has been submitted to GenBank (accession number AF308934).

The full coding region for AptKv3.3 was isolated by RT-PCR. PCR was performed on randomly primed brain cDNA using the GeneAmpXL PCR kit (Perkin-Elmer, Foster City, CA) with the followingprimers: Forward 5'(CAC TCG AGG CTC CCT CTA ATG CTC AGT T), Reverse5'(CAT CTA GAC GCT CCA CGC TAC AAA A). The nucleotide sequenceof the PCR product was confirmed by DNA sequence analysis. Forin vitro expression, XhoI and XbaI restriction sites in the primerswere used to directionally clone the cDNA into the vector pEUK-C1(Clontech, Palo Alto,CA).

In situ hybridization. Apteronotus brain was fixed with 4% paraformaldehyde, and 10 µm cryostat sections were probed (Bottaiet al., 1997) with an ³⁵S-labeled RNA probe from the 3' untranslated region of AptKv3.3(nucleotide 2075-2482). After hybridization and washing, the slideswere air-dried and exposed to x-ray film for 3 d, emulsion-dipped[1:1 dilution of NTB2 gel (Eastman Kodak, Rochester, NY) in 600mM ammonium acetate] and exposed for 18 d at 4°C. After they weredeveloped, the slides were counterstained in neutral red to permitthe use of differential interference contrast (DIC)microscopy.

Immunocytochemistry. A C-terminal fragment of AptKv3.3 cDNA corresponding to amino acids 562-634 was subcloned in the GSTfusion vector pGEX-4T-1 (Pharmacia Biotech, Uppsala, Sweden).The fusion protein was expressed in Escherichia coli strain DH5- $alpha$ and purified from inclusion bodies as described (Frangioni andNeel, 1993). Antibodies were prepared in rabbits, depleted ofGST immunoreactivity by adsorption to GST protein bound to Affigel10 beads (Bio-Rad, Richmond, CA), and then affinity-purified byadsorption to AptKv3.3 fusion protein bound to Affigel 10beads.

For Western blotting, Apteronotus brain proteins were prepared by homogenization of brain tissue in 50 mM Tris/HCl, pH 7.5,0.25 M sucrose, 25 mM KCl, 5 mM MgCl₂, and 1 mM phenylmethylsulfonylfluoride at 4°C. The homogenate was clarified by centrifugation(800 × g, 10 min), and then membranes were purified by centrifugation(100,000 × g, 60 min). Soluble and membrane fractions were fractionatedby electrophoresis on a 7.5% polyacrylamide gel and transferredto polyvinylidene difluoride membranes. Membranes were incubatedwith the antibody (0.45 µg/ml) overnight at 4°C, and the immunoreactiveproteins were detected with horseradish peroxidase-coupled secondaryantibody and chemiluminescence (NEN Life Sciences, Boston,MA).

For immunohistochemistry, fish were perfused transcardially with 5 ml of PBS and 40 ml of cold 4% paraformaldehyde in PBS,and the brains were post-fixed overnight at 4°C. Coronal vibratomesections (40 µm) were cut and transferred to PBS (3 × 10 min)before they were incubated in blocking buffer (10% normal goatserum, 1% bovine serum albumin, and 0.2% Triton X-100 in PBS)for 2 hr at room temperature. Immunolabeling followed standardprocedures using primary antibodies (anti-AptKv3.3; 0.9 µg/mlor mouse monoclonal anti-MAP2a,b; 1.0 µg/ml) and a 1:250 dilutionof Oregon green-conjugated goat anti-rabbit IgG conjugate or rhodamine-conjugatedgoat anti-mouse IgG (Molecular Probes, Eugene,OR).

Heterologous expression of AptKv3.3. Human Embryonic Kidney (HEK) 293-tsA201 cells (Margolskee et al., 1993) were cotransfectedwith 10 µg AptKv3.3 vector DNA and 0.5 µg eGFP-C1 (Invitrogen,Carlsbad, CA) by the CaCl₂ transfection procedure. After 24-48hr, coverslips were transferred to an in vitro recording chamberon the stage of a ZeissAxioskop.

ELL recording preparations. Patch recordings were obtained using a novel "Spread Print" preparation, and a conventional invitro slice preparation was used for intracellular recordings.The procedures for animal maintenance, anesthesia, brain dissection,and preparation of ELL tissue slices have been described previously(Turner et al., 1994, 1996). All chemicals for electrophysiologicalstudies were obtained from Sigma (St. Louis, MO) unless indicatedotherwise. A Tissue Print procedure developed by Kotecha et al.(1997) was modified to generate a Spread Print preparation consistingof a partially dissociated thin tissue slice from adult tissue.Spread Prints were prepared by cutting 100 µm ELL slices on avibratome in oxygenated (95% O₂/5% CO₂) artificial CSF (aCSF)consisting of (in mM): NaCl 124, KCl 2.0, KH₂PO₄ 1.25, CaCl₂ 1.5,MgSO₄ 1.5, NaHCO₃ 24, and D-glucose 10, pH 7.4. Slices were transferredby spatula and floated onto the surface of a HEPES-buffered "print"medium consisting of (in mM): sucrose 218, NaHCO₃ 25, K-gluconate3.25, MgCl₂ 4.5, CaCl₂ 0.1, D-glucose 10, Na pyruvate 1, pH 7.4contained within a 35 mm Petri dish. The surface tension of thismedium provided sufficient force to gradually dissociate the slicein all directions over a 10-15 min period. The extent of dissociationwas monitored under a dissecting microscopic until the ELL pyramidalcell layer had just begun to spread. The dissociation was stoppedwhen required by attaching the slice to a gelatin-coated (1.5%)12-mm-round glass coverslip that was lowered to the medium surfaceon the tip of a spatula. The coverslip was then inverted underthe medium surface and either transferred to the recording chamberor stored in this medium at 4°C for up to 5hr.

The Spread Print procedure provided a rapid and enzymatic-free method to partially dissociate cells from adult tissue slicesthat retained an organotypic distribution to aid in identifyingcells within a specific topographic map. Cell yield was very high,with excellent structural preservation in numerous cell typesthat were directly identified using DIC optics and infrared lighttransmission (DIC-IR). Cells exhibiting good structural definitionhad resting potentials between $-$ 50 and $-$ 70 mV and spontaneousTTX-sensitive spike discharge at $-$ 50 mV, which were comparableto previous recordings (Turner et al., 1994, 1996).

Recordings. Patch electrodes were constructed from borosilicate glass (Garner Instruments) (2.0 mm outer diameter, 1.2 mminner diameter) using a Sutter P-87 microelectrode puller, andpatch recordings were obtained using an Axopatch 200-A amplifierand PClamp 6 software (Axon Instruments, Foster City, CA) andwith an electrolyte consisting of (in mM): KCl 140, HEPES 5, MgCl₂1, EGTA 5, Mg-ATP 1.5, pH 7.2. Electrode resistance ranged between2 and 10 M $Omega$ . Microelectrodes were constructed from fiber-filledborosilicate glass (1.5 mm O.D.; A-M Systems, Carlsborg, WA) usinga Campden puller (Frederick Haer, Bowdoinham, MA). Intrasomaticand dendritic recordings were obtained in an in vitro slice preparationusing an Axoclamp 2-A amplifier and CED software (Cambridge ElectronicDesign, Cambridge, UK). Microelectrodes were filled with 2 M K-acetate(80-110 M $Omega$ ). Average values are expressed as mean ± SD, and exponentialfits were obtained using Microcal Origin software (Northampton,MA).

All pyramidal cell recordings were restricted to the centromedial segment (CMS) topographic map of the ELL. Dendritic recordingswere restricted to the proximal 150 µm of apical dendrites toexamine electrophysiological properties in the region over whichNa⁺ spikes actively backpropagate (Turner et al., 1994). Antidromicdischarge in the soma and apical dendrites was evoked by stimulatingthe plexiform layer using a bipolar electrode. In the Spread PrintELL preparation, AptKv3.3 currents were isolated in on-cell oroutside-out recording configuration after washing out Ca²⁺-sensitive K⁺ channels as 5 mM EGTA in the electrolyte dialyzed the patch (<5min).

Tissue slices and Spread Prints were perfused with oxygenated aCSF (see above). Transfected HEK cells were perfused with aCSFor in some cases with a medium consisting of (in mM): NaCl 140,HEPES 10, CaCl₂ 1, MgCl₂ 1, Glucose 10, KCl 5, pH 7.4. No detectabledifference in current kinetics were observed between these twomedia. Drugs were bath-applied in the HEK cell and Spread Printpreparations. All patch recordings of pyramidal cells were madein the presence of 1 µM TTX supplemented in some cases with 200µM Cd²⁺ and 0.1 mM CaCl₂ in which MgCl₂ and KCl were substituted forMgSO₄ and KH₂PO₄, respectively. Drugs were focally ejected byapplying one to five pressure pulses (10-14 psi, 100-200 msec)to the side port of an electrode holder containing a glass electrodewith a tip broken back to ~2 µm diameter (Turner et al., 1994).The carrier medium for pressure-ejected drugs consisted of (inmM): NaCl 148, KCl 3.75, CaCl₂ 1.5, MgCl₂ 1.5, HEPES 10, D-glucose10, pH 7.4.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the gymnotid electrosensory system, sensory input from electroreceptors is initially processed by pyramidal neurons ofthe medullary nucleus, the ELL. Pyramidal cell somata are positionedin a well defined cell layer, and they project extensive apicaldendrites 600-800 µm into an overlying molecular layer (Maler,1979). Outside-out patch recordings of K⁺ channels were obtained from identified pyramidal cell somata(n = 31) and apical dendrites (n = 40) using a novel Spread Printslice preparation. The most frequently encountered K⁺ channel in both somata and apical dendrites up to 150 µm fromthe soma was a 20-25 pS channel (Fig. 1). Given the similarityin these channels in somatic and dendritic membranes, we describetheir general properties without specific reference to recordinglocation.

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Figure 1. AptKv3.3 channels in ELL pyramidal cells. A, B, Outside-out patch recordings of K⁺ channels isolated from a pyramidal cell soma (A) and an apical dendrite 150 µm from the soma (B) in the presence of normal extracellular aCSF. A 7 sec depolarizing step from $-$ 80 to 0 mV produces a fast activation of K⁺ channels that subsequently inactivate over 1-2 sec to reveal a unitary conductance level for channels in the patch. C, An outside-out patch recording obtained from somatic membrane and stepped from a holding potential of $-$ 90 mV to the indicated potentials reveals K⁺ channels with a conductance of 24 pS. D, E, A macropatch K⁺ current in an outside-out recording isolated from a pyramidal cell apical dendrite (100 µm from soma) evoked by a depolarizing step from $-$ 100 to 0 mV for 7 sec. Outward current was blocked by 100 µM TEA (D). Inset shows single-channel recordings from another dendritic outside-out patch recording at 0 mV (100 µm from soma) with a substantial reduction of single-channel conductance by 100 µM TEA. E, After washout of TEA, outward current from the same dendritic patch in D is blocked by perfusion of 1 mM 4-AP. Currents in A, B, D, and E were leak-subtracted, and capacitance artifacts were removed by digital subtraction.

Patch formation isolates either single K⁺ channels (one to seven channels per patch) or macropatch outward currents (more thanseven single channels) of 10-120 pA for steps from $-$ 80 to 0 mV.There is an equal probability of obtaining macropatch currentsfrom either somatic or dendritic membranes, suggesting a highdensity of expression in both soma and proximal apical dendrites(<150 µm). Step commands from $-$ 80 to 0 mV evoke immediate channelopenings followed by inactivation over 1-2 sec to a lower openprobability state (Fig. 1A,B). The rate of inactivation in macropatchrecordings or ensemble averages of single-channel activity over7 sec can be fit with a single exponential to $tau$ = 330 ± 87 msec(n = 16). Significant recovery from inactivation requires a stepcommand to potentials more negative than $-$ 60 mV for at least 2sec, with the degree of recovery increasing with step potentialsdown to $-$ 120 mV. Recordings of single-channel activity at steadystate reveal channel openings at membrane potentials more depolarizedthan $-$ 40 mV (Fig. 1C). Macropatch recordings of current are reducedby perfusion of <100 µM TEA (n = 6) (Fig. 1D), revealing a highsensitivity to this K⁺ channel blocker. Analysis of single-channel amplitude revealsa TEA concentration-dependent decrease in the amplitude of transitionsto the open state, with an IC₅₀ = 78 µM (Fig. 1D) (n = 5). Channelcurrent in macropatches is also blocked by externally applied4-AP at concentrations $>=$ 200 µM (n = 5) (Fig. 1E).

These recordings indicate the presence of K⁺ channels in pyramidal cell somata and proximal apical dendrites that exhibit ahigh threshold for activation, a high sensitivity to TEA and 4-AP,and a conductance of ~25 pS. All of these properties are consistentwith the mammalian Kv3 class of voltage-dependent K⁺ channels (for review, see Rudy et al., 1999).

Molecular characterization of the Apteronotus Kv3.3 potassium channel

The properties of these K⁺ channels suggest the expression of one or more Kv3 channel subtypes in pyramidal cells. In a previousstudy, we amplified fragments specific for each of the four KvK⁺ channel gene families, including Kv3, from Apteronotus genomicDNA (Rashid and Dunn, 1998). To identify the channel proteinsresponsible for the Kv3-like currents in pyramidal cells, Kv3-specificPCR fragments were used as probes to isolate cDNAs from an Apteronotusbrain cDNA library. Five partial cDNAs encoding different Kv3K⁺ channel sequences were recovered, and RNase protection studiesindicated that one of these was expressed at high levels in ELL(data not shown). A full-length coding sequence for this channelpredicts a protein sequence that extends for a length of 652 aminoacids and is shown in Figure 2A.

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Figure 2. Molecular characterization of AptKv3.3. A, Alignment of predicted amino acid sequence of AptKv3.3 with that of the murine splice isoform mKv3.3b. The six transmembrane domains (S1-S6) and the pore domain (P) are indicated above the sequence. Also indicated are consensus sites for N-linked glycosylation (asterisks) and phosphorylation by protein kinase C (open squares), protein kinase A (filled square), and calcium/calmodulin-dependent protein kinase (filled ovals). Amino acid identities are shaded. B, Phylogenetic comparison of AptKv3.3 to members of the mammalian Kv3 family. The sequences used for comparison included splice isoforms of each Kv3 subtype and, with the exception of murine Kv3.3a and Kv3.3b, were from rat (see Materials and Methods). The phylogenetic tree demonstrates that AptKv3.3 is most related to mammalian Kv3.3. Analysis by the parsimony method was performed using the PROTPARS program in the Phylogeny Inference Package (PHYLIP) (Felsenstein, 1989). In this algorithm, the Drosophila Shaw K⁺ channel was used as the outgroup.

A phylogenetic comparison (Fig. 2B) and amino acid comparisons (Table 1) to the rodent Kv3 family members and their spliceisoforms indicate that the Apteronotus channel is most closelyrelated to the Kv3.3 subtype. We therefore refer to the channelas AptKv3.3. The rodent Kv3.3 genes are subject to alternativeRNA splicing in the gene segments encoding the intracellular C-terminaltail regions, giving rise to a series of alternatively splicedisoforms (mouse: mKv3.3a, mKv3.3b; rat: rKv3.3a, rKv3.3b, rKv3.3c).Sequence comparisons indicate that the C-terminal segment of AptKv3.3is most similar to the carboxyl segment of mKv3.3b (Fig. 2A).The functional implications of this similarity to the carboxylsegment of mKv3.3b are unknown but may involve targeting of Kv3.3channels to specific subcellular domains (Ponce et al., 1997).


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Table 1. AptKv3.3 amino acid sequence identities with mammalian Kv3 channels

Within the central core of the channel sequence, each of the six transmembrane domains (S1-S6) and the pore domain are wellconserved between Apteronotus and mammalian Kv3.3 (Fig. 2A). Thehigh sequence conservation of the S4, the S5, the pore, and theS6 domains suggests that the voltage dependencies and conductanceproperties of the fish channel should be similar to those reportedfor the rodent homologs. Outside of the transmembrane domainsthere is significantly less homology, one notable exception beingthe NAB domain (N-terminal A and B domains, AptKv3.3 amino acids36-152), a segment of channel protein that determines Kv family-specificsubunit assembly (Xu et al., 1995; Yu et al., 1996).

Two of the mammalian Kv3 subtypes, Kv3.3 and Kv3.4, contain N-terminal inactivation motifs and demonstrate fast channel inactivationwhen expressed in oocytes or cultured cells (Rudy et al., 1999).The amino-terminal sequence of AptKv3.3 fits closely with criteriaestablished for fast N-type inactivation, including a string of11 hydrophobic or uncharged residues followed by 8 hydrophilicamino acids containing four highly charged residues (K12, R14,K15, K19). These two regions together form the "ball" of the ball-and-chainmodel of inactivation (Hoshi et al., 1990). Although the N-terminalinactivation segment is conserved in AptKv3.3, the linker segmentbetween the inactivation peptide and the NAB domain in AptKv3.3(residues 20-35) is much shorter than the equivalent segment inrodent Kv3.3.

The primary sequence of AptKv3.3 suggests that it may be subject to regulation by protein phosphorylation. The AptKv3.3 sequencehas consensus target sites for various protein kinases, includingCa²⁺-dependent phospholipid-sensitive protein kinase (PKC), cAMP-dependentprotein kinase (PKA), and Ca²⁺/calmodulin-dependent protein kinase II (CamKII) (Fig. 2A). Sevenof the nine consensus sequences for phosphorylation by PKC areconserved between Apteronotus and mKv3.3b, including a site betweenS4 and S5, which is common to vertebrate K⁺ channels (Chandy and Gutman, 1995).

High levels of AptKv3.3 mRNA expression in electrosensory neurons

Preliminary RNase protection studies indicated that AptKv3.3 mRNA is present in brain but not in liver or skeletal muscleRNA samples (data not shown). To determine the specific cellularexpression of AptKv3.3, we performed in situ hybridization analysisusing a probe derived from the 3' UTR of AptKv3.3 cDNA. The ELLhas a well defined laminar organization, with the two principalclasses of neurons distributed as a layer of pyramidal cells anda more ventral layer of granule cell interneurons. Figure 3A-Eillustrates that AptKv3.3 mRNA is expressed at high levels inboth of these cell types. By comparison, mRNA is expressed atlow levels in the overlying cerebellar structure, the eminentiagranularis posterior (EGp). The levels of AptKv3.3 mRNA expressionare similar for pyramidal and granule cells across each of fourtopographic maps (segments) of electroreceptor distribution inthe ELL: the medial, centromedial, centrolateral, and lateralsegments (Maler et al., 1991). The high levels of gene expressionin ELL pyramidal cells identify AptKv3.3 as a probable candidatefor the Kv3-like currents that dominate the patch-clamp recordingsfrom pyramidal cell soma and dendrites (Fig. 1).

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Figure 3. The expression of AptKv3.3 mRNA in the hindbrain. Tissue sections from hindbrain were hybridized with AptKv3.3 RNA probe. The distribution of silver grains over pyramidal and granule cell layers is indicated in A. B and C show that AptKv3.3 is expressed in all of the pyramidal cells. D and E illustrate localization of silver grains over the pyramidal cell somata. A, In situ hybridization of AptKv3.3 mRNA in the hindbrain at low power demonstrates prominent expression in the ELL and lighter expression in the adjacent caudal lobe of the cerebellum (eminentia granularis posterior; EGp) and the corpus cerebelli (CCb). The four topographic maps of the ELL are indicated: MS, medial segment; CMS, centromedial segment; CLS, centrolateral segment; LS, lateral segment. Label is dense over the entire extent of the ELL pyramidal cell (PCL) and granule cell (GCL) layers. Scale bar, 200 µm. B, A section of the pyramidal cell layer showing a cluster of pyramidal cell somata viewed under DIC optics. Scale bar, 25 µm. C, The position of silver grains in the micrograph shown in B when viewed at the plane of emulsion illustrates dense labeling positioned over individual pyramidal cell somata. D, A pyramidal cell viewed under DIC optics at higher magnification. Scale bar, 10 µm. E, Corresponding image as that shown in D viewed at the plane of emulsion illustrates the restriction of grains to the somatic region of a pyramidal cell.

It should be noted that we have evidence for the additional expression of an AptKv3.1 mRNA in pyramidal cells (data not shown),providing the possibility for heteromeric channel formation betweenAptKv3.3 and AptKv3.1 proteins. However, AptKv3.1 mRNA is at alevel ~2% that of AptKv3.3 mRNA in the centromedial segment pyramidalcells examined here. Furthermore, we found no labeling in theELL for two other Kv3 probes corresponding to putative analogsof mammalian Kv3.2 and 3.4. We can thus expect these pyramidalcell Kv3 channels to be composed predominantly of AptKv3.3 protein,an interpretation supported by the close match between the propertiesof native and expressed AptKv3.3 channels (Figs. 1, 5).

ApKv3.3 protein localizes to dendrites and somata of ELL pyramidal cells

To investigate the subcellular distribution of AptKv3.3, a polyclonal antibody ( $alpha$ -AptKv3.3) was generated against the C-terminalregion of AptKv3.3 (amino acids 562-634). In Western blot experiments, $alpha$ -AptKv3.3 recognizes a single protein band of ~87 kDa in brainmembrane fractions with no signal in the corresponding solubleprotein fraction (Fig. 4E). Comparison of this value with thepredicted molecular weight of 72.8 kDa suggests that the channelis glycosylated at the three consensus sites for N-linked glycosylationlocated between transmembrane segments S1 and S2 (Fig. 2A).

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Figure 4. AptKv3.3 protein is localized to somata and dendrites of ELL pyramidal cells. Tissue sections of hindbrain were stained with $alpha$ -AptKv3.3 antibody (A-D) or double-labeled with MAP-2 monoclonal antibody (D). The specificity of the $alpha$ -AptKv3.3 antibody is indicated in a Western blot (E) and tissue section (C). A and B show that AptKv3.3 protein is distributed throughout the pyramidal cell somatic and dendritic domains. Colocalization of AptKv3.3 with MAP2 in apical dendrites is shown for pyramidal cells from the medial segment (D). A, Low-power micrograph of $alpha$ -AptKv3.3-immunolabeled hindbrain. Intense label is seen throughout the ELL, particularly the pyramidal cell layer (PCL), granule cell layer (GCL), and deep neuropil layer (DNL). Note also the dense label in the ventral (VML) and dorsal (DML) molecular layers that overlie the PCL and contain pyramidal cell apical dendritic projections. Scale bar, 400 µm. B, Higher-magnification confocal image of the ELL pyramidal cell layer in the centrolateral segment illustrating immunolabeling of pyramidal cell somata and apical dendrites. Labeling of apical dendrites remains constant in intensity past primary and secondary branchpoints (indicated with arrows). Note the lack of immunolabel in the tractus stratus fibrosum (tSF) and plexiform (PLX) layers, which both contain dense axonal fascicles. Scale bar, 100 µm. C, A control section from centrolateral segment viewed at the magnification used for B. This section was treated with $alpha$ -AptKv3.3 that had been preadsorbed with the AptKv3.3 fusion protein. Only a diffuse background signal is detected. D, High-magnification image of two medial segment apical dendrites colabeled with $alpha$ -AptKv3.3 (D1) and MAP-2a,b (D2) antibodies. AptKv3.3 protein appears to be localized exclusively to MAP-2-containing dendritic structures. Scale bar, 10 µm. E, Western blot analysis demonstrates that $alpha$ -AptKv3.3 recognizes a single protein of ~87 kDa in the brain membrane fraction (P) but not the corresponding soluble protein fraction (S).

Immunohistochemical analysis reveals a striking distribution of AptKv3.3 protein in the ELL pyramidal and granule cell bodylayers, as well as throughout the entire extent of the molecularlayer, where pyramidal and granule cells project extensive apicaldendrites (Fig. 4A,B). Control sections with the secondary antibodyalone or $alpha$ -AptKv3.3 preadsorbed with a 100-fold excess of fusionprotein show only low levels of nonspecific background staining(Fig. 4C). Because our electrophysiological recordings focus onpyramidal cells (Fig. 1), we will restrict our cytochemical analysisprimarily to pyramidal cellimmunolabel.

Higher magnification reveals AptKv3.3 protein on pyramidal cell bodies (Fig. 4B), apical dendrites in the molecular layer(Fig. 4B,D1), and basilar dendrites that extend ventrally throughthe deep neuropil layer (Fig. 4B). The high density of antigenicsites presents a continuous image of labeled structures, suchthat individual apical dendrites can be tracked from the soma,through the proximal dendritic shaft, and beyond secondary andtertiary dendritic branch points (Fig. 4D1). In these sections,costaining with an antibody to the microtubule-associated proteinMAP2 confirms the presence of AptKv3.3 out to the most distalaspects of the pyramidal cell apical dendrites (Fig. 4D2). Similarly, $alpha$ -AptKv3.3 immunofluorescence labels individual basilar dendritesfrom the soma to the final extension of a basilar bush that receivesprimary afferent input 300-400 µm from the cell layer (Fig. 4A,B).

Pyramidal cells extend axons that course medially in a plexiform layer immediately beneath the pyramidal cell layer. As apparentin Figure 4B, AptKv3.3 immunoreactivity is absent in the axonfascicles of the plexiform layer, providing a stark contrast tothe pyramidal cell basilar dendrites projecting through this region.Although the apparent lack of immunolabel of these structuresis suggestive, further distinctions on axonal or presynaptic distributionsneed to be made at the ultrastructurallevel.

AptKv3.3 channels expressed in HEK cells resemble K⁺ channels in native pyramidal cells

To determine whether AptKv3.3 channel properties match those found in ELL pyramidal cells, we transfected HEK tsA201 cellswith an expression vector for AptKv3.3 cDNA. Whole-cell recordingsof transfected cells reveal an outward rectifying K⁺ current of 5-10 nA with a characteristic early peak that subsequentlyrelaxed to a steady-state current within ~5 msec (Fig. 5A). AptKv3.3whole-cell current was initially detected at a relatively highvoltage ( $-$ 20 to $-$ 10 mV) with a voltage for half-activation ofV_0.5 = 15.6 ± 5.05 (Fig. 5A) (n = 13). Activation and deactivationare fast, reaching the early peak of the outward current in 2.0± 0.64 msec for a command step from $-$ 90 to 50 mV (n = 27) anddeactivating with $tau$ = 0.6 ± 0.19 msec (n = 22) for voltage stepsfrom 50 to $-$ 60 mV (Fig. 5A). AptKv3.3 currents are highly sensitiveto both TEA and 4-AP, with substantial block obtained at concentrations>50 µM (Fig. 5B). Whole-cell currents exhibit little inactivationover 50-100 msec for voltage commands up to 70 mV (Fig. 5A). Commandpulses of 1-7 sec invoked a voltage-dependent steady-state inactivation,although the voltage and time required to initiate this processwere variable (data not shown).

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Figure 5. Expression of AptKv3.3 currents in HEK tsA201 cells. A, Whole-cell recording of currents expressed 1 d after AptKv3.3 cDNA transfection reveals an outward rectifying K⁺ current for command steps from $-$ 90 to 70 mV (10 mV steps after a 10 msec prepulse to $-$ 90 mV). AptKv3.3 K⁺ current exhibits a fast activation that reaches a characteristic early peak of ~5 msec duration that subsequently relaxes to a steady-state current and fast deactivation on stepping back to $-$ 60 mV. Little steady-state inactivation is apparent after 60 msec. The current-voltage relationship indicates outward rectification, a high threshold for initial activation of $-$ 10 mV, and little saturation for steps up to 70 mV. B, Whole-cell AptKv3.3 currents are highly sensitive to micromole concentrations of externally applied TEA and 4-AP. C, An outside-out patch recording of AptKv3.3 single channels stepped to different steady-state potentials reveals a single channel slope conductance of 23 pS. D, An outside-out macropatch recording of AptKv3.3 current reveals a very similar response as found for whole-cell currents >100 msec (compare with A). E, An outside-out patch recording of AptKv3.3 single channels indicates a fast and maximal activation of channels over the initial 200 msec followed by inactivation during a 7 sec depolarizing command step from $-$ 100 to 0 mV. Capacitance artifacts in D and E were digitally subtracted.

Outside-out recordings reveal outward rectifying K⁺ channels with transitions to the open state detectable between $-$ 40 and50 mV under steady-state conditions. The single-channel conductancecalculated in either on-cell or outside-out recordings is 22.9± 0.53 pS (Fig. 5C) (n = 16). As found for whole-cell currents,AptKv3.3 single-channel conductance is reduced by low concentrationsof TEA, with an IC₅₀ = 40 µM (n = 4). Outside-out macropatch currentsresemble whole-cell currents in exhibiting an early peak followedby a relaxation to a lower steady state with little subsequentinactivation during 50-100 msec step commands (Fig. 5D). Steady-stateinactivation with longer duration pulses was more pronounced andmore consistent in outside-out recordings than for whole-cellcurrents. An example is shown in Figure 5E, where inactivationis prominent over a 7 sec time frame for a step from $-$ 100 to 0mV. Inactivation in macropatch recordings with depolarizing stepsfrom $-$ 90 or $-$ 100 mV to 0 mV is fit by a single exponential of $tau$ = 366 ± 84 msec (n = 9). Significant recovery from inactivationrequires a return to holding potentials of at least $-$ 60mV.

The voltage ranges for activation, single-channel conductance, and high TEA and 4-AP sensitivity of AptKv3.3 channels arein agreement with those reported for mammalian Kv3 channels (Vega-Saenzde Miera et al., 1992; Critz et al., 1993; Kanemasa et al., 1995;Rudy et al., 1999). Most importantly, these properties match theK⁺ channel recordings that we obtained in native ELL pyramidal cellsomata and apical dendrites when recorded under the same ionicconditions (Fig. 1). Together with the cytochemical localizationof AptKv3.3 (Fig. 4), our results provide compelling evidencethat the AptKv3.3 channel subtype contributes prominently to theK⁺ channel activity recorded in pyramidal cell somata and apicaldendrites.

AptKv3.3 channels are involved in spike repolarization and establishment of burst threshold in pyramidal cells

The functional significance of AptKv3.3 channels to spike discharge was assessed by focally ejecting TEA or 4-AP in the immediatevicinity of dendritic or somatic recordings in a conventionalin vitro slice preparation, an approach that restricts drug ejectionsto a limited region of the cell axis (Turner et al., 1994). Focalejections of either 1 mM TEA or 4-AP rapidly decreased the rateof spike repolarization in both somatic and dendritic locations(Fig. 6). This change in repolarization increases the half-widthof somatic spikes by 46.5 ± 33% (n = 8) (Fig. 6A) and the half-widthof dendritic spikes by 20.3 ± 9.8% (n = 6) (Fig. 6B), with a slightincrease in spike amplitude in somatic recordings. It is importantto note that diffusion and dilution of ejected drugs in the extracellularmedium will result in effective concentrations that are substantiallylower than the initial ejected medium. The immediate results obtainedwith 1 mM concentrations of these blockers thus indicate thatK⁺ channels underlying spike repolarization are highly sensitiveto TEA and 4-AP, as found for Kv3 K⁺ channels (Rudy et al., 1999). However, low concentrations ofTEA and 4-AP can also affect large conductance (BK) Ca²⁺-activated K⁺ channels (Coetzee et al., 1999). Although BK K⁺ channels are present in both somatic and dendritic membranesof pyramidal cells, we have determined that BK channel conductanceis reduced by bath-applied TEA only at concentrations >1 mM (E.Morales and R. W. Turner, unpublished observations). In addition,somatic and dendritic spikes proved insensitive to Cd²⁺ ejections (200-400 µM; n = 10), suggesting that BK K⁺ channels do not contribute to spike repolarization in pyramidalcells (data not shown). The Kv1 (Shaker) class of K⁺ channels is also sensitive to low concentrations of TEA (Coetzeeet al., 1999). However, no effects are observed with focal ejectionof 2 µM dendrotoxin in either somatic or dendritic regions (n= 5), suggesting that spike repolarization does not involve thisclass of K⁺ channels. These data strongly suggest that AptKv3.3 current contributesto the repolarization of both somatic and dendritic spikes inpyramidal cells. Nevertheless, it is important to note that spikehalf-widths could be increased in a dose-dependent manner by TEAor 4-AP concentrations of up to 5 mM, suggesting that additionalK⁺ channel subtypes may contribute to spike repolarization.

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Figure 6. Somatic and dendritic spike repolarization is highly sensitive to TEA and 4-AP. A, B, Schematic diagrams of pyramidal cells are shown to indicate the placement of a stimulating electrode in the plexiform layer for antidromic activation (double wires), intracellular recording electrodes (white fill), and pressure electrodes for focal drug ejections (shaded fill) in an in vitro ELL slice preparation. Focal pressure ejection of either TEA or 4-AP (1 mM) in the immediate region of separate (A) somatic or (B) dendritic recordings slows the rate of repolarization and increases the duration of antidromic spikes. Control and test responses are shown superimposed, with test responses identified as thick gray traces.

It has been established that ELL pyramidal cells discharge bursts of action potentials in vivo to encode specific featuresof electrosensory input, revealing a direct role in feature extraction(Gabbiani et al., 1996). These bursts arise through a processof "conditional spike backpropagation," a newly recognized aspectof spike conduction that generates burst discharge in the $gamma$ -frequencyrange (20-80 Hz) (Lemon and Turner, 2000). Burst discharge isinitiated when the long duration of a backpropagating dendriticNa⁺ spike generates a DAP at the soma (Turner et al., 1994). Duringrepetitive discharge, dendritic spikes exhibit a frequency-dependentbroadening that increases current flow back to the soma to potentiatethe DAP. The increase in somatic depolarization eventually triggersa high-frequency spike doublet at the soma that exceeds the dendriticspike refractory period. As a result, spike backpropagation intodendrites abruptly fails, removing the dendritic depolarizationdriving the burst from one spike to the next, allowing a burstafterhyperpolarization (AHP) to terminate the burst (Lemon andTurner, 2000). A change in the rate of dendritic spike repolarizationduring repetitive discharge is thus a critical aspect of K⁺ channel function in pyramidal cells. Given the role for AptKv3.3K⁺ channels in repolarizing dendritic spikes, one would predictthat a reduction in dendritic AptKv3.3 conductance could directlymodulate burst discharge by augmenting the current flow underlyingthe somaticDAP.

To test whether such a mechanism could affect burst generation, we examined the effects of focally ejecting TEA or 4-AP indendritic regions on the pattern of spike output. In the firstset of experiments, we recorded the antidromic somatic spike andDAP and current-evoked spike discharge when set below thresholdfor burst output (Fig. 7B). Focal ejections of 1 mM TEA or 4-APin the dendritic region selectively increases the amplitude ofthe somatic DAP on average 116 ± 108% (n = 5; range, 41-274%)and immediately converts cell output from one of tonic to burstdischarge (Fig. 7C). The lack of any change in somatic spike repolarizationin these experiments confirms that drug actions were restrictedto the dendritic region. We then examined the effects of thesedrugs on dendritic spike discharge by focally ejecting TEA (n= 6) or 4-AP (n = 5) in the immediate region of dendritic recordings.This slows dendritic spike repolarization and shifts current-evokedspike output from tonic discharge to an oscillatory series ofspike bursts (Fig. 7D-F). These studies reveal that reducing theability of AptKv3.3 K⁺ channels to repolarize dendritic spikes immediately potentiatesthe somatic DAP and lowers the threshold for generating burstdischarge.

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Figure 7. Dendritic spike repolarization controls burst threshold. A-C, The effects of dendritic 4-AP ejection on somatic spike discharge. A, Schematic diagram of a pyramidal cell to indicate the placement of a stimulating electrode for antidromic activation (double wires), an intrasomatic recording electrode (white fill), and a pressure electrode for focal drug ejection of 2 mM 4-AP (shaded fill) in an in vitro ELL slice preparation. B, C, The effects of dendritic 4-AP ejection on somatic spike discharge. B, Control intrasomatic recordings of antidromic spike discharge and associated DAP (open arrow) and current-evoked spike discharge when set below threshold for generating oscillatory spike bursts. C, Focal ejection of 4-AP to apical dendrites selectively enhances the somatic DAP (open arrow), as shown by superimposition of the control and test antidromic response (test response shown by gray trace). The lack of any change in somatic spike repolarization confirms that the drug was restricted to the dendritic region. This is sufficient to convert cell output from a tonic to bursting pattern, as indicated by a repeating series of spike bursts. Burst period is indicated by solid arrows designating the occurrence of burst afterhyperpolarizations (burst AHPs). D, Schematic diagram of a pyramidal cell indicates an intradendritic recording in another pyramidal cell (white filled electrode) and pressure electrode for focal ejection of 2 mM 4-AP (shaded fill). E, F, The effects of dendritic 4-AP ejection on dendritic spike discharge. E, Control intradendritic recordings showing current-evoked spike discharge set below threshold for generating spike bursts. Insets to the left in E and F show expanded views of the first current-evoked spikes in control and test recordings (asterisks). F, Focal ejection of 4-AP in the dendritic region broadens the dendritic spike by slowing spike repolarization and shifts cell output from a tonic to bursting pattern. Solid arrows indicate the occurrence of burst AHPs that terminate each spike burst. Inset shows the control and test responses superimposed (test response shown by gray trace). Excitation after dendritic 4-AP results in burst discharge composed of a repeating series of spike doublets.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This study describes the distribution and functional roles of a Kv3 K⁺ channel subtype, AptKv3.3, in a principal sensory neuron. AptKv3.3proves to be unique among the Kv3 K⁺ channel family in exhibiting an extensive localization to dendriticmembranes. In dendrites, these channels act to repolarize spikesbackpropagating from the somatic region, and in so doing, regulatethe threshold for a type of burst discharge that has an establishedrole in sensory processing in vivo.

Functional role of dendritic AptKv3.3 channels

K⁺ currents localized to dendritic membranes are increasingly recognized for their ability to shape signal processing (Hoffmanet al., 1997). In only a few cases have specific channel subtypesbeen associated with dendritic K⁺ currents that have an identified role in modulating cell output(Magee et al., 1998). We have now shown that AptKv3.3 K⁺ channels are localized to both somata and apical dendrites ofELL pyramidal cells, a conclusion supported by both patch recordingsand dense immunolabel over the entire soma-dendritic axis. Ourdata suggest that AptKv3.3 channels are distributed with essentiallyequivalent densities over the soma and proximal apical dendritesout to at least 150 µm, although further mapping will be requiredto rigorously establish channel densities. It is important toemphasize that the extensive dendritic distribution of AptKv3.3channels reported here is entirely novel among the Kv3 class,because all previous immunolocalization studies have identifiedonly somatic, axonal, and a limited extent of dendritic membranes( $approx$ 20 µm) as the distribution target for Kv3.1, 3.2, and 3.4 K⁺ channels (Weiser et al., 1995; Du et al., 1996; Perney and Kaczmarek,1997; Sekirnjak et al., 1997). The distribution of Kv3.3 K⁺ channel proteins has not been examinedpreviously.

In other cells, Kv3 channels contribute to spike repolarization and facilitate recovery from Na⁺ channel inactivation, helping to maintain high frequencies ofspike discharge (Rudy et al., 1999). A similar role in spike repolarizationis served by AptKv3.3 channels in ELL pyramidal cells at boththe somatic and dendritic levels in ELL pyramidal cells. The mostsignificant consequence of dendritic localization of AptKv3.3channels is the control over a form of burst discharge known tobe involved in feature extraction in vivo (Gabbiani et al., 1996).Through their ability to control dendritic spike repolarization,AptKv3.3 channels have a pronounced effect on burst discharge.Thus, focal dendritic ejections of TEA or 4-AP that block AptKv3.3channels immediately increased DAP amplitude at the soma and shiftedcell output from tonic to burst discharge. This demonstrates thatthe contribution by AptKv3.3 channels to repolarizing dendriticspikes establishes a specific threshold for $gamma$ -frequency burstdischarge in pyramidalcells.

A characteristic of the burst response in ELL pyramidal cells is a progressive increase in the DAP resulting from a frequency-dependentbroadening of dendritic spikes during repetitive discharge (Lemonand Turner, 2000). Although the mechanism underlying the changein dendritic spike duration remains to be determined, our dataindicate that a decrease in dendritic AptKv3.3 currents wouldeffectively broaden dendritic spikes. In this regard, it is interestingthat Kv3.4 channel kinetics can be controlled by the degree ofphosphorylation (Covarrubias et al., 1994) such that dephosphorylationis predicted to increase the rate of inactivation. If a similaraction is found for AptKv3.3 channels, it would produce a stateconducive to cumulative inactivation during repetitive discharge:decreasing the ability of AptKv3.3 channels to repolarize dendriticspikes.

We found that AptKv3.3 channels are distributed over the entire extent of the apical dendritic axis. This was somewhat unexpectedfor a K⁺ channel activated by high voltage because Na⁺ spike backpropagation is believed to occur only over the proximalthird of the dendritic tree (Turner et al., 1994). The high thresholdfor activation of AptKv3.3 channels would appear to preclude adirect modulation of synaptic potentials. However, it is possiblethat under some conditions active membrane depolarizations maybe triggered in more distal dendritic regions and be shaped byAptKv3.3 channels in a manner similar to dendritic K⁺ channels in other cells (Golding et al., 1999; Magee and Carruth,1999). The functional role for AptKv3.3 channels in these distaldendritic regions will be an important area for futureinvestigation.

Properties of AptKv3.3 channels

AptKv3.3 is the first member of the teleost Kv3 family of K⁺ channel $alpha$ -subunits for which a complete amino acid sequence isknown. There is remarkable sequence similarity with mammalianKv3 channels, particularly within the six transmembrane domainsand the pore domain. The fact that the Xenopus Kv3.1 channel alsoshows high sequence similarity to mammalian Kv3.1 (Gurantz etal., 2000) confirms that the Kv3 amino acid sequences have beenwell maintained through vertebrate evolution. Phylogenetic analysisindicates that the apteronotid channel is most similar to themammalian subtype Kv3.3, and moreover, the C terminus of AptKv3.3is most similar to the mouse splice isoform mKv3.3b (Fig. 2A).Interestingly, the C-terminal sequence of AptKv3.3 (-SIL) resemblesthe consensus sequences that bind to the PSD-95, Dlg-1, Zho-1(PDZ) protein-protein interaction domains that are found on familiesof subcellular localizing proteins (Kim et al., 1995; Kim andSheng, 1996; Songyang et al., 1997). It is possible that interactionswith one of these PDZ domain proteins is responsible for the extensivedendritic targeting of AptKv3.3channels.

A unique feature of mammalian Kv3 channels is their requirement for membrane voltages exceeding $-$ 20 mV for activation. Thishigh-voltage dependence restricts Kv3 channel activation to depolarizedpotentials where they can mediate the repolarization of the actionpotentials without limiting the voltage-dependent conductancesnear resting potential (Kanemasa et al., 1995; Weiser et al.,1995; Du et al., 1996; Wang et al., 1998; Erisir et al., 1999).This role in spike repolarization is further assisted by the characteristicallyrapid activation and deactivation kinetics of Kv3 channels. AptKv3.3channels expressed in heterologous cells display each of thesekey properties, with a high voltage for activation (approximately $-$ 20 mV) and fast activation-deactivation kinetics. Importantly,these properties were shared by the AptKv3.3 currents recordedin ELL pyramidal cell somata and apical dendrites, a comparisonfacilitated by recording under the same ionicconditions.

The primary distinction between mammalian Kv3 subtypes is the rate of steady-state inactivation, with the degree of Kv3.3inactivation falling between the noninactivating Kv3.1 and 3.2isoforms and the fast inactivating Kv3.4 channel (Rudy et al.,1999). The rate of AptKv3.3 inactivation during short step commandsunder whole-cell recording conditions in HEK cells (50 mV, 100msec) was comparable to reported values for mammalian Kv3.3 (Vega-Saenzde Miera et al., 1994; Rae and Shepard, 2000). However, duringlonger step commands (1-7 sec) in whole-cell recording mode, thevoltage dependence and rate of inactivation of AptKv3.3 was highlyvariable. In contrast, with outside-out patch recordings the rateof AptKv3.3 inactivation in response to similar steady-state commandswas more consistent and also substantially increased. This mayrelate to the degree of washout of cytoplasmic constituents inthe outside-out recording mode, reducing the ability of solublesecond messengers to modulate the AptKv3.3 channel. Indeed, therate of steady-state inactivation of AptKv3.3 channels isolatedfrom HEK cells or pyramidal cells in outside-out recordings wasessentially equivalent (Figs. 1A,B, 4E).

N-type inactivation of K⁺ channels depends on the presence of an inactivation motif at the amino terminus of the protein (Hoshiet al., 1990). This motif is conserved between AptKv3.3 and thetwo mammalian Kv3 channel subtypes that exhibit inactivation,Kv3.3 and Kv3.4. Specifically, the amino terminus of AptKv3.3consists of a string of 11 hydrophobic or uncharged residues followedby a segment of 8 amino acids containing 4 highly charged residues,consistent with the proposed requirements for N-type inactivation(Hoshi et al., 1990; Zagotta et al., 1990). AptKv3.3 also containsa critical cysteine in the amino terminus (Fig. 2A, position 6)that has been shown to be important for inactivation in rodentKv3.3 and Kv3.4 (Ruppersberg et al., 1991; Rudy et al., 1999).However, the portion of AptKv3.3 that links the inactivation motifto the rest of the channel, the so-called "chain" in the ball-and-chainmodel of inactivation, is much shorter than that found in mammalianKv3.3. Although this would predict a faster rate of inactivation(Hoshi et al., 1990), our measured rate of AptKv3.3 inactivationis somewhat slower than mammalian channels when compared underequivalent recording conditions. The reason for this is unknown,but it indicates that the length of the linker peptide is notthe limiting factor for N-type inactivation in AptKv3.3 channelsand may well signify intracellular regulation of the inactivationmechanism.

We have established that dendritic AptKv3.3 channels contribute to determining the threshold for generating $gamma$ -frequency burstdischarge in ELL pyramidal cells. Spike bursts are recorded inpyramidal cells in vivo, and discharge is recorded in direct relationto relevant features of external sensory input (Gabbiani et al.,1996; Metzner et al., 1998). The known regulation of Kv3 K⁺ channels by second messengers provides a potential route by whichmodulation of AptKv3.3 channels could shape burst characteristicsand contribute to feature detection during electrolocatory behaviorin the liveanimal.

  FOOTNOTES

Received July 21, 2000; revised Oct. 16, 2000; accepted Oct. 17, 2000.

This research was supported by grants from the Medical Research Council to R.J.D. and R.W.T. and the National Engineeringand Science Research Council to R.J.D. R.W.T. is an AHFMR SeniorScholar. We thank B. Ellis and S. Sinclair for technical assistance,E. Harvey-Girard and C. Doering for assistance with DNA transfections,and Rejean Munger and Len Maler for assistance with confocalmicroscopy.
Correspondence should be addressed to Dr. Robert J. Dunn, Department of Neurology, Montreal General Hospital, 1650 Cedar Avenue,Montreal, Quebec, Canada, H3G 1A4. E-mail: mc81{at}musica.mcgill.ca.

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MATERIALS AND METHODS
RESULTS
DISCUSSION
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