Enhancement of Hippocampal Pyramidal Cell Excitability by the Novel Selective Slow-Afterhyperpolarization Channel Blocker 3-(Triphenylmethylaminomethyl)pyridine (UCL2077)

Mala M. Shah, Mazyar Javadzadeh-Tabatabaie, David C. H. Benton, C. Robin Ganellin, and Dennis G. Haylett

Departments of Pharmacology (M.M.S., D.C.H.B., D.G.H.) and Chemistry (M.J.-T., C.R.G.), University College London, Gower Street, London, United Kingdom

Received May 13, 2006; accepted July 28, 2006

Abstract

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Abstract
Materials and Methods
Results
Discussion
References

The slow afterhyperpolarization (sAHP) in hippocampal neuronshas been implicated in learning and memory. However, its preciserole in cell excitability and central nervous system functionhas not been explicitly tested for 2 reasons: 1) there are,at present, no selective inhibitors that effectively reducethe underlying current in vivo or in intact in vitro tissuepreparations, and 2) although it is known that a small conductanceK⁺ channel that activates after a rise in [Ca²⁺]_i underliesthe sAHP, the exact molecular identity remains unknown. We showthat 3-(triphenylmethylaminomethyl)pyridine (UCL2077), a novelcompound, suppressed the sAHP present in hippocampal neuronsin culture (IC₅₀ = 0.5 µM) and in the slice preparation(IC₅₀ ${approx}$ 10 µM). UCL2077 was selective, having minimal effectson Ca²⁺ channels, action potentials, input resistance and themedium afterhyperpolarization. UCL2077 also had little effecton heterologously expressed small conductance Ca²⁺-activatedK⁺ (SK) channels. Moreover, UCL2077 and apamin, a selectiveSK channel blocker, affected spike firing in hippocampal neuronsin different ways. These results provide further evidence thatSK channels are unlikely to underlie the sAHP. This study alsodemonstrates that UCL2077, the most potent, selective sAHP blockerdescribed so far, is a useful pharmacological tool for exploringthe role of sAHP channels in the regulation of cell excitabilityin intact tissue preparations and, potentially, in vivo.

A train of action potentials in hippocampal neurons is followedby an afterhyperpolarization comprising fast, medium (mAHP),and slow (sAHP) components (Storm, 1990

; Sah and Faber, 2002

).The sAHP has been reported to be important for regulation ofspike frequency accommodation and, therefore, neuronal function(Lancaster and Nicoll, 1987

; Storm, 1990

; Sah and Faber, 2002

;Disterhoft et al., 2004

). Indeed, these channels have been suggestedto have a role in hippocampal memory encoding processes. Inparticular, enhanced sAHP has been observed in older animalsand has been correlated with impairments in learning (Poweret al., 2002

; Tombaugh et al., 2005

). Therefore, sAHP currentblockers can potentially be useful for improving learning andmemory. Although it is known that a small conductance K⁺ channelthat requires Ca²⁺ entry for activation underlies the sAHP (Lancasterand Nicoll, 1987

; Sah and Isaacson, 1995

; Sah and Faber, 2002

),the molecular identity of the channel is still a mystery. Threesmall conductance Ca²⁺-activated K⁺ channels (SK1-3) have beencloned, of which SK1 and SK2 are strongly expressed in the hippocampus(Stocker et al., 1999

). Initial studies suggested that SK1 couldbe a potential molecular candidate for the sAHP (Kohler et al.,1996

; Vergara et al., 1998

). However, several more recent studieshave indicated that it is unlikely to contribute to the sAHPin hippocampal neurons (Shah and Haylett, 2000b

; Strobaek etal., 2000

; Grunnet et al., 2001

; Shah et al., 2001

; Bond etal., 2004

; Villalobos et al., 2004

). Thus, the progress in ourunderstanding of the contribution of the sAHP channels to cellexcitability has been limited by ignorance of the identity ofthese channels.

In addition, until recently, there were no selective blockersof the sAHP. The sAHP can be abolished by neurotransmitterssuch as noradrenaline (Madison and Nicoll, 1982, 1986; Malenkaand Nicoll, 1986; Storm, 1990; Sah and Faber, 2002). In theabsence of specific inhibitors, these have been used to studythe role of the sAHP in cell excitability and behavior. Neurotransmitters,however, have multiple actions, making it difficult to determinewhether the effects observed are due to modulation of the sAHPor other currents. For example, noradrenaline blocks the sAHPby elevating cAMP levels and increasing protein kinase A activity(Madison and Nicoll, 1986; Pedarzani and Storm, 1993). cAMP,however, alters the gating of other ion channels, includingthe hyperpolarization-activated cation channels (Wainger etal., 2001), and can thereby modify cell firing and excitabilityindependently of its effects on the sAHP (Robinson and Siegelbaum,2003). Although the studies using neurotransmitters to reducethe sAHP have provided significant information regarding thephysiological role of the sAHP current, it would be beneficialto revisit the question with more selective blockers to understandthe contribution of the current per se to cell excitability.

We have previously described the sAHP inhibitor UCL2027 (Shahet al., 2001). Although this particular blocker suppressed thesAHP in dissociated hippocampal neurons with an IC₅₀ of 1 µM,it is very lipophilic and liable to extensive tissue binding.Because the compound also has an aqueous solubility limit of10 µM, it not ideal for in vitro studies involving slicepreparations or in vivo research. In an attempt to find morepotent sAHP blockers that might be useful for understandingits physiological role, we synthesized and tested many compoundsrelated to UCL2027 (Zunszain et al., 2002). We now report theactions of a related compound, UCL2077, a more powerful sAHPinhibitor in cultured hippocampal neurons. In addition, it reducedthe sAHP in hippocampal neurons present in brain slices. Wetook advantage of the activity of this compound to explore therole of the sAHP in spike frequency adaptation in hippocampalneurons present in the slice preparation and compared the changesin firing produced by sAHP channel inhibition with that causedby SK channel block.

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
References

Hippocampal Cell Culture
Hippocampal pyramidal neurons were cultured as described previously(Shah et al., 2001). In brief, 4- to 7-day-old Sprague-Dawleyrats were decapitated, and hippocampal regions were subdissectedand incubated in Hanks' buffered saline solution containingtrypsin. Individual cells were released by trituration and resuspendedin Neurobasal medium supplemented with 2% B27, 0.5 mM L-glutamine,and 10% fetal calf serum (FCS). The cells were plated onto plasticdishes (previously coated with poly-D-lysine) and maintainedin culture for 15 days using the growth medium without the FCS.

Maintenance and Transfection of HEK293 Cells
HEK293 cells were grown in Dulbecco's modified Eagle's mediumsupplemented with 2 mM L-glutamine, 50 U/ml penicillin, 50 µg/mlstreptomycin, and 10% FCS. Cells were transfected with eitherhSK1 (kind gift from Dr. J. P. Adelman, Vollum Institute, OregonHealth and Science University, Portland, OR) or rSK2 (kind giftfrom Dr. W. Joiner and Prof. L. K. Kaczmarek, Department ofCellular and Molecular Physiology, Yale University School ofMedicine, New Haven, CT) and GFP using a modified calcium phosphatemethod (Shah and Haylett, 2000b).

Hippocampal Slice Preparation
Hippocampal slices were prepared as described previously (Shahet al., 2004). In brief, 5- to 6-week-old Sprague-Dawley ratswere anesthetized, brains were removed, and 400-µm sliceswere cut using a vibratome (Leica, Wetzlar, Germany). The sliceswere maintained at room temperature in a holding chamber containingexternal solution (solution A) composed of 125 mM NaCl, 2.5mM KCl, 1.25 mM NaH₂PO₄, 25 mM NaHCO₃, 2 mM CaCl₂, 2 mM MgCl₂,and 10 mM glucose; pH 7.3 when bubbled continuously with 95%O₂/5% CO₂.

Electrophysiological Studies
Perforated Patch Recordings of sI_AHP from Cultured Neurons.The sI_AHP was recorded from neurons that had been in culturefor at least 8 days as described previously (Shah et al., 2001).In brief, the culture dishes were superfused with solution Aalso containing 5 mM HEPES and 5 µM DNQX. Perforated patcheswere obtained at 32-34°C with 4- to 10-M ${Omega}$ pipettes containing126 mM KMeSO₄, 14 mM KCl, 10 mM HEPES, 3 mM MgCl₂, 2 mM Na₂ATP,0.3 mM Na₂GTP, pH adjusted to 7.3, and 0.12 mg/ml amphotericin.Thirteen action potentials were elicited using 5-ms currentpulses (frequency = 76.5 Hz) under discontinuous current-clamp,and the afterhyperpolarization current (sI_AHP) produced wasrecorded under voltage clamp at -55 mV. Voltage and currentsignals were filtered at 3 and 0.3 kHz, respectively, usingan AxoClamp 2A and acquired using pCLAMP 6 software (MolecularDevices, Sunnyvale, CA).

Measurement of Ca²⁺ Currents. Cultured hippocampal neurons possessan extensive dendritic tree and are difficult to voltage-clamp.Ca²⁺ currents were therefore recorded from freshly dissociatedcells, which have only a small apical dendrite. Pyramidal cellswere isolated and plated as described above and recordings made3.5 to 8 h after isolation at 32-34°C. The cells were superfusedwith 115 mM NaCl, 2 mM KCl, 2 mM CaCl₂, 0.5 mM MgCl₂, 11 mMglucose, 10 mM HEPES, 25 mM TEA, 0.0003 mM tetrodotoxin, and0.005 mM DNQX, pH adjusted to 7.4. Whole-cell recordings weremade with a List EPC-7 amplifier using 7- to 10-M ${Omega}$ patch pipettesfilled with 135 mM CsCl, 0.5 mM CaCl₂, 2 mM MgCl₂, 10 mM HEPES,3 mM EGTA, 2mMNa₂ATP, and 0.3 mM Na₂GTP, pH adjusted to 7.3.The cells were held at -80 mV and the Ca²⁺ current was elicitedusing a ramp protocol (Fig. 1E). Signals were filtered at 1kHz and digitized at 3.33 kHz using pCLAMP 6.

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Fig. 1. Effects of UCL2077 on the sAHP recorded from dissociated hippocampal neurons. A, The chemical structure of UCL2077. B, the time course of block of the sI_AHP by 3 µM UCL2077 in cultured hippocampal neurons. At -55 mV, there is an outward holding current (in this case, 120 pA), which UCL2077 partially suppressed. The effect on the holding current is variable (between 5 and 40%, as noted in the text). Action potentials have been removed for clarity. The mI_AHP was unaffected in the presence of UCL2077, and this is more clearly shown on an enhanced time scale in C. In addition, sometimes the sI_AHP increased with time; in this particular cell, that seems to be the case in that there is an over-recovery upon washout of UCL2077. C, effects of UCL2077 shown on an enhanced time scale. The traces shown correspond to (i), (ii), and (iii) in B. D, concentration-inhibition curve for UCL2077. The numbers of observations for each concentration are shown above the symbol.

Recordings from Hippocampal Cells in Slices. Slices were placedin a recording chamber containing solution A with 0.05 mM DL-2-amino-5-phosphonopentanoicacid, 0.01 mM 6-cyano-2,3-dihydroxy-7-nitroquinoxaline, 0.01mM bicuculline, and 0.001 mM CGP 55,845 added. The solutionin the recording chamber was maintained at a temperature of33-35°C (Shah et al., 2004

). Whole-cell current-clamp recordingswere obtained using 10-12 M ${Omega}$ pipettes filled with 120 mM KMeSO₄,20 mM KCl, 10 mM HEPES, 2 mM MgCl₂, 0.2 mM EGTA, 4 mM Na₂ATP,and 0.3 mM Tris-GTP, 14 mM Tris-phospho-creatinine, pH adjustedto 7.3. A train of 10 action potentials at a frequency of 66.7Hz was applied at a holding potential of -60 mV, and the resultingsAHP acquired using an AxoClamp 2B amplifier. Signals were filteredat 30 kHz using the Axoclamp 2B and obtained using pCLAMP 8software (digitized at 10 kHz).

Measurements of Expressed SK Currents. Cells transfected witheither hSK1 or rSK2 subunits 24 h previously and identifiedby GFP fluorescence, were superfused with 150 mM NaCl, 5 mMKCl, 2 mM CaCl₂, 1 mM MgCl₂, 10 mM HEPES, and 10 mM glucose,pH adjusted to 7.4 using 1 M NaOH. Whole-cell recordings weremade using 3- to 5-M ${Omega}$ pipettes filled with 130 mM KCl, 5 mM HEDTA,10 mM HEPES, 3 mM MgCl₂, 0.67 mM CaCl₂, and 2 mM Na₂ATP, pHadjusted to 7.2 (free [Ca²⁺] calculated to be 1 µM). Cellswere clamped at -80 mV using a List EPC-7 amplifier and voltagepulses applied to evoke SK currents (Fig. 2A). Signals werefiltered at 5 kHz and acquired using pCLAMP 6.

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Fig. 2. Effects of UCL2077 on action potentials and the Ca²⁺ current. A and B, trains of action potentials in the absence and presence of UCL2077 when applied at concentrations of 1 and 3 µM, respectively. A (iii) and B (iii) are superimposed records of the last action potential in a train of 13 action potentials before (black) and after (red) application of UCL2077. Note that the resting membrane potential is slightly depolarized in the presence of 3 µM UCL2077, as shown in B (i) and B (ii). The scale bars shown in A (ii) and B (ii) apply to A (i) and B (i), respectively. In addition, the vertical scale bars shown in A (ii) and B (ii) also apply to A (iii) and B (iii), respectively. C, the Ca²⁺ current was elicited by a ramp as shown. Note the traces in the absence and presence of 3 µM UCL2077 overlap. Cd²⁺ (100 µM) was applied to determine the amplitude of the HVA Ca²⁺ current.

Data Analysis
Data were analyzed using pCLAMP software. The average amplitudeof three successive records of sI_AHP and sAHP traces in thepresence of the drug was expressed as a percentage of that inthe absence of the compound. The sI_AHP and sAHP decay time constants,as well as the amplitude of the mI_AHP recorded in cultured hippocampalneurons, were estimated by fitting a multicomponent exponentialequation as described previously (Shah et al., 2001). With thecurrent-clamp experiments done using the slice preparation,the mAHP peak could be easily distinguished by eye in both theabsence and the presence of UCL2077 or apamin (Fig. 4).

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Fig. 4. Effect of UCL2077 on the sAHP in hippocampal neurons present in the slice preparation. A, representative illustrations of the sAHP produced by an action potential train at -60 mV in hippocampal CA1 pyramidal neurons present in the slice preparation before and after application of 10 µM UCL2077. As explained in the text, concentrations of UCL2077 lower than 3 µM were ineffective in the slice preparation; presumably, as is known to occur with many compounds, it is sequestered by tissue. Note that UCL2077 had little effect on the mAHP (shown on an enhanced time scale in the inset). B, time course of the effects of 10 µM UCL2077 on the sAHP shown in A. C, bar graph to show the relative inhibition by 10 µM UCL2077 of the sAHP and mAHP recorded from hippocampal neurons present in the slice preparation. D, records of trains of action potentials in the absence and presence of 10 µM UCL2077. Superimposed traces of the last action potential under control conditions (black) and with UCL2077 present (red) are shown on an enhanced time scale.

The input resistance was measured using 1-s hyperpolarizingcurrent pulses of -100 pA from a potential of -70 mV in theabsence and presence of the drugs. One-second, depolarizingpulses were applied to study the effects of UCL2077 on the numberand frequency of action potentials (see Fig. 5). The minimumcurrent required to evoke a single action potential was usedto measure spike threshold. The width and amplitude of the lastaction potential in the train that was used to evoke the sAHPwas also measured in the absence and presence of UCL2077. Theaction potential width was measured at -20 mV, and the amplitudewas measured from the threshold to the tip of the spike.

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Fig. 5. Comparison of effects of UCL2077 and apamin on spike frequency adaptation in hippocampal neurons. A and B, typical effects of 10 µM UCL2077 and 100 nM apamin on spike-firing when a 250-pA depolarizing pulse is applied from -70 mV. The scale bars shown in A apply to B. C, graph depicting action potential (AP) number produced by current pulses in the absence (open symbols) and presence (closed symbols) of 10 µM UCL2077 or 100 nM apamin. D, E, and F, graphs show the effects of 10 µM UCL2077 and 100 nM apamin on input resistance (IR) and spike frequency within the first 250 ms (E) or the last 250 ms (F) of a 1-s step. ^*, significance at p < 0.05.

To investigate effects on the high-voltage-activated (HVA) Ca²⁺current, the peak average of two successive traces in the presenceof the drug were expressed as a percentage of the average peakof the traces acquired immediately before application and afterwashout of UCL2077. This allowed for alterations in the peakCa²⁺ current that may occur because of rundown.

SK current steady-state amplitudes in HEK293 cells were measuredat -40 mV to minimize the contribution of series resistanceerrors and the small endogenous delayed rectifier current. TheSK current amplitude in the presence of the drug was expressedas a percentage of the average current before addition and afterwashout of the compound.

All results are expressed as mean ± S.E. Statisticalanalysis was carried out using the appropriate Student's t test.Concentration-inhibition curves were fitted with a modifiedHill equation (Shah et al., 2001).

Materials
All tissue culture reagents were purchased from Invitrogen (UK).All other materials were acquired from Sigma-Aldrich (UK) apartfrom apamin and KMeSO₄, which were bought from Alamone Labs(Jerusalem, Israel) and Pfaltz and Bauer Ltd. (Waterbury, CT),respectively. UCL2077 (Fig. 1A) was synthesized by authors M.J.-Tand C.R.G. Stocks of 100 mM UCL2077 were prepared in dimethylsulfoxide and kept refrigerated. For experimental purposes,the solutions were diluted at least 10,000-fold in the externalsolution (final dimethyl sulfoxide concentration <0.01%)because it was found to be insoluble at concentrations >10µM in our external solution.

Results

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Abstract
Materials and Methods
Results
Discussion
References

Effects of UCL2077 on the sI_AHP Recorded in Cultured HippocampalNeurons. The chemistry program produced a number of compoundsrelated to UCL2027, which were tested for sAHP blocking actionusing cultured hippocampal neurons (Zunszain et al., 2002).We chose this particular system for two reasons: 1) althoughit would be more straightforward to test the activity of compoundson expressed channels, the channel underlying the sAHP is unknown,and 2) the sI_AHP could be recorded very stably for 1 h, andtest compounds could be applied and washed off very rapidly(< 1 min). We identified UCL2077 (Fig. 1A) as a potent sI_AHPblocker. In contrast to UCL2027, 3 µM UCL2077 abolishedthe current (Fig. 1, B and C). Maximum effects of the compoundwere achieved within 2 min and recovery within 5 min (Fig. 1B).The IC₅₀ for block of the sI_AHP was 0.5 ± 0.1 µM(Fig. 1D), approximately 2-fold more potent than UCL2027 (Shahet al., 2001). Unlike neurotransmitters (e.g., see Malenka andNicoll, 1986; Krause and Pedarzani, 2000), UCL2077 also hadlittle effect on the decay time constant ( ${tau}$ ) or time to peakof the sI_AHP (see Table 1). Furthermore, the mI_AHP [due to apamin-sensitiveSK channels in cultured hippocampal neurons (Shah et al., 2001)]was unaffected [percentage inhibition =-18.9 ± 10.0%(n = 3)] by 1 µM UCL2077 (Fig. 1). In addition, at concentrations<1 µM, UCL2077 had no effect on resting membrane potential(RMP) under current clamp or the outward holding current undervoltage clamp. At 3 µM, UCL2077 reversibly reduced theoutward holding current present at -55 mV. The decrease of theoutward holding current, however, was very variable, rangingfrom 5 to 40% (n = 3). Alterations in the outward holding currentcan be equivalent to neuronal depolarization in unclamped cell(Fig. 1B). Indeed, the resting membrane potential depolarizedfrom -62.7 ± 1.2 mV (n = 3) under control conditionsto -59.3 ± 0.3 mV (n = 3, p = 0.15) in the presence of3 µM UCL2077.

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TABLE 1 Effects of UCL2077 on action potential shapes and sAHP kinetics in cultured hippocampal pyramidal neurons

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Fig. 3. Effects of UCL2077 on SK currents. Example traces of hSK1 (A) and rSK2 (B) currents in the absence, presence, and washout of 3 µM UCL2077. The currents were elicited by 100- to 200-ms steps from -120/-140 mV to +40 mV from a holding potential of -80 mV. C, summary of effects of 3 µM UCL2077 and 10 nM UCL1848 on SK currents. The numbers of observations for each treatment are shown above the bar.

It is noteworthy that in two thirds of cells, a slow inwardcurrent (an "afterdepolarization") after the action potentialtrain was revealed in the presence of 3 µM UCL2077 (Fig. 1, B and C).A similar current is observed when the sAHP is abolished inCA1 pyramidal neurons (see, for example, Wu et al., 2004

). Thisafterdepolarization may be due to a residual Ca²⁺ current orother channels activated by Ca²⁺ (Caeser et al., 1993

; Mageeand Carruth, 1999

; Wu et al., 2004

; Yue and Yaari, 2004

UCL2077 Effects on Ca²⁺ Influx. Inhibition of the sI_AHP mightalso result from reductions in Ca²⁺ entry caused by either Ca²⁺channel block or narrowing of action potentials (which are necessaryto elicit the sI_AHP). We thus measured the effects of UCL2077directly on the HVA Ca²⁺ current, because Ca²⁺ entry throughthese channels is likely to be involved in the generation ofthe sI_AHP in hippocampal neurons (Shah and Haylett, 2000a).UCL2077 (3 µM) had no effect on the HVA Ca²⁺ current [inhibition= 1.1 ± 1.2% (n = 7); Fig. 2]. In many cases, it wasdifficult to distinguish between the low-voltage-activated Ca²⁺current and the HVA Ca²⁺ current (see Fig. 2C). However, becauseUCL2077 had little effect on the kinetics of the Ca²⁺ currentor the amplitude of the current, it is assumed that it did notaffect the low-voltage-activated component either. In addition,at concentrations $≤$ 1 µM, it had little effect on actionpotential width or amplitude (Fig. 2, Table 1). In this respect,UCL2077 is more selective than UCL2027 because UCL2027 causeswidening of action potentials at concentrations that block thesAHP by 80% or less (see Shah et al., 2001). Action potentialbroadening, however, did occur in the presence of 3 µMUCL2077 (Fig. 2, Table 1). Wider action potentials, however,would be expected to increase the Ca²⁺ influx into the cell,leading to sI_AHP enhancement, not reduction. These results indicatethat UCL2077 does not alter Ca²⁺ influx into neurons.

Effects of UCL2077 on the Cloned SK Channels. Noise analysisstudies have indicated that the sAHP channel has a small conductance(2-5 pS; Sah and Isaacson, 1995). Because Ca²⁺ entry is requiredfor the initiation of the sAHP, it has been assumed that a smallconductance K⁺ channel activated by Ca²⁺ generates the current.SK channels are therefore likely candidates. However, many recentstudies, (including ours) have indicated that the SK channelscloned so far are unlikely to underlie the sI_AHP (Shah and Haylett,2000b; Shah et al., 2001; Bond et al., 2004; Villalobos et al.,2004). Nonetheless, we tested the effects of UCL2077 on thecloned SK1 and SK2 channels because these are highly expressedin hippocampal neurons (Stocker et al., 1999). Because rat hippocampalneurons were used, it would be ideal to use the rat homologsof SK channels. However, rSK1 subunits when expressed on theirown in heterologous systems do not form functional channels(Bowden et al., 2001; Benton et al., 2003; D'Hoedt et al., 2004).We have thus examined the effects of UCL2077 on channels formedby expression of hSK1 or rSK2 subunits in HEK293 cells. UCL2077(3 µM) reduced hSK1 and rSK2 current by only 27.2 ±3.8% (n = 4) and 16.2 ± 8.9% (n = 4), respectively (Fig. 3).As expected, 10 nM UCL1848, a selective SK channel blocker (Shahand Haylett, 2000b; Hosseini et al., 2001; Benton et al., 2003),reduced the SK1 and SK2 currents by 61.5 ± 4.3% (n =7) and 90.1 ± 0.4% (n = 3, Fig. 3), respectively. Theseresults show that concentrations of UCL 2077 that affect thesI_AHP have much smaller effects on SK channels.

Effects of UCL2077 on sAHP in Hippocampal Neurones in Slices.As noted earlier, it is important to examine the activity ofthis compound on sAHP block in a more intact preparation. BecauseUCL2077 is 2-fold more potent than UCL2027 (Shah et al., 2001),it seemed worthwhile to test the effects of suppressing thesAHP recorded from visually identified hippocampal neurons presentin slices obtained from adult rats. A train of 10 action potentialsat -60 mV resulted in a fast afterdepolarization followed bya mAHP and a sAHP in all cells tested (see Fig. 4). The averagesAHP amplitude and decay time constant ( ${tau}$ ) were 4.79 ±0.5 mV (n = 19) and 2.05 ± 0.1 s (n = 19), respectively.There was also no significant rundown of the AHPs over a periodof approximately 1 h (decrease = 0.32 ± 3.7%; n = 9).Unlike the cultured neuron system, concentrations of UCL2077less than 3 µM had little effect on neurons present inthe slice preparation. This may be due to tissue sequestrationof the compound. In addition, because of limitations in solubilityof the compound, concentrations greater than 10 µM cannotbe used. We therefore explored the effects of 10 µM UCL2077on the sAHP. Bath application of this concentration of the compoundreduced the sAHP by 60.2 ± 5.9% (n = 8, Fig. 4, A and C),without having a significant effect on the neuronal RMP (theRMP at -60 mV depolarized by 2.3 ± 1.0 mV (n = 7, p >0.05). The onset of the effects of the compound was slow (approximately5 min; Fig. 4B) and may be due in part to the slow perfusionrate of 1 ml/min. Maximal block of the sAHP was achieved within20 min of application and was irreversible up to 20 min afterwashout in six cells. Partial reversal was obtained in the remainingtwo neurons. UCL2077 (10 µM) had little effect on actionpotential width or threshold or the sAHP ${tau}$ (see Table 2; Fig. 4D).The mAHP was also unaffected (decrease = 7.0 ± 17%, n= 6; Fig. 4, A and C). UCL2077 is thus the first synthetic compoundto block the sAHP in more intact tissue preparations and representsa significant step forward in the pharmacology of the sAHP.

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TABLE 2 Effects of UCL2077 on action potential and sAHP kinetics measured from hippocampal neurons present in the slice preparation.

Effects of UCL2077 and Apamin on Hippocampal Cell Excitability.As explained in the Introduction, it would be beneficial toevaluate the effects of specifically suppressing the sAHP oncell excitability. Because UCL2077 is the most potent, selectivesAHP blocker so far and the only one that is effective in densetissue preparations such as the slice preparation, we used itto study the effects of a reduced sAHP on spike frequency adaptationusing the hippocampal slice preparation. Its actions were comparedwith those of apamin (an SK channel blocker), because an SK-likechannel could underlie the sAHP (Sah and Isaacson, 1995; Vergaraet al., 1998).

Application of 10 µM UCL2077 significantly increased theaction potential number produced at small current pulses (Fig. 5, A and C)In contrast, treatment with 100 nM apamin [a supramaximal concentration(Stocker et al., 1999)] had no significant effect on actionpotential number at low current pulses of less than 250 pA inmagnitude (Fig. 5C). At higher current pulses ( $≥$ 250 pA), apamindid substantially increase the number of action potentials,but its effect was significantly less than that of UCL2077 (Fig. 5, B and C).The effects of apamin were irreversible up to 20 min after washoutas reported in earlier studies (Stocker et al., 1999). In thesesame cells, apamin was found to reduce the mAHP evoked by atrain of 10 action potentials by 18.5 ± 0.2% (n = 5).Apamin had no effect on action potential shape (data not shown)or the sAHP (inhibition = -2.9 ± 4.5%, n = 5). Alterationsin action potential number could result from changes in a cell'sinput resistance. Therefore, the input resistance was monitoredthroughout the recordings and was not significantly alteredin the presence of either UCL2077 or apamin (Fig. 5D). Theseresults suggest that sAHP channels are more powerful regulatorsof spike frequency adaptation than SK channels.

Because the mAHP is short in duration (<500 ms), SK channelblock may affect the interval between the first few action potentialsand thereby modulate the initial firing frequency. We thereforestudied the effects of apamin on action potential frequencyin the first 250 ms of a 1-s step. Only steps that in the absenceof the peptide produced two to four action potentials were used.We found that the spike frequency and thus the interspike intervalin the first 250 ms was indeed altered in the presence of apamin(Fig. 5E). As expected, the firing frequency for the last 250ms was less affected (Fig. 5F). Thus, SK channels are importantfor controlling early spike frequency adaptation.

It can be hypothesized that, because of its slow onset and timecourse, the sAHP would affect firing frequency in the last 250ms more than in the first 250 ms. Indeed, UCL2077 significantlyincreased the number of spikes occurring in the last 250 ms(Fig. 5F). It had a nonsignificant but more variable effectduring the first 250 ms (Fig. 5E). These results show that thesAHP per se is an influential controller of action potentialfiring and plays a particularly significant role in affectingspike frequency adaptation.

Discussion

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References

In this study, we report the most potent, direct sAHP blockerproduced so far. This particular compound, UCL2077, is alsothe first of its kind to effectively reduce the sAHP in a slicepreparation and thus may be beneficial for in vivo and in vitrostudies involving intact tissue preparations. This is a significantstep forward in the pharmacology of sAHP suppressors becausethe only effective blockers described so far are neurotransmitterssuch as noradrenaline, which are not ideal probes; they affectmultiple intracellular processes with effects on multiple channels.Note, however, that 10-fold higher concentrations of UCL2077were required to block the sAHP in slices than in cultured cells,indicating that the compound might be sequestered by tissue.Hence, even more potent compounds are required for abolitionof the sAHP in intact tissue preparations. Nonetheless, we haveshown that UCL2077 can be useful for further evaluating thephysiological role of the sAHP in in vitro studies and, possibly,by extension in in vivo studies.

UCL2077 had no effect on the Ca²⁺ current or the time courseof the sAHP/sI_AHP recorded from both cultured hippocampal neuronsand hippocampal neurons present in the slice preparation. Partialblock of the sAHP by neurotransmitters alters its decay timeconstant ( ${tau}$ ; e.g., see Malenka and Nicoll, 1986; Krause and Pedarzani,2000). Because ${tau}$ was unaffected by UCL2077, it indicates thatits mechanism of action differs from that of neurotransmitters.It is thus possible that UCL2077 may block the sAHP by directlyinhibiting the underlying K⁺ channel. Indeed, UCL2077 is a derivativeof clotrimazole, which is a known inhibitor of the intermediateconductance Ca²⁺-activated K⁺ (IK) channel (Alvarez et al.,1992; Brugnara et al., 1993; Logsdon et al., 1997; Rittenhouseet al., 1997; Jensen et al., 1998; Hoffman et al., 2003). However,because the molecular identity of the K⁺ channel that generatesthe sAHP is unknown, this hypothesis cannot be directly tested.UCL2077 may, in fact, prove useful in identifying the molecularcorrelate of the sAHP.

A small conductance K⁺ channel activated by Ca²⁺ is believedto underlie the sAHP (Sah and Isaacson, 1995) and thus SK channelscan potentially underlie the current (Vergara et al., 1998).We therefore tested the effects of UCL2077 on channels formedby expression of SK1 and SK2 subunits in cultured HEK293 cells.At concentrations that abolished the sI_AHP in cultured hippocampalneurons, UCL2077 had little effect on SK current (Fig. 3). Furthermore,SK channels are known to underlie the mAHP in hippocampal neurons(Stocker et al., 1999; Bond et al., 2004; Villalobos et al.,2004; Gu et al., 2005), and UCL2077 had little effect on themI_AHP in cultured hippocampal neurons (Fig. 1) or the mAHP inhippocampal neurons present in the slice preparation (Fig. 4).Thus, these results provide further evidence that SK channelsare unlikely to contribute to the generation of the sAHP inhippocampal neurons, although it cannot be ruled out that thepresence of as-yet-unidentified accessory subunits may resultin alterations of the pharmacological and biophysical propertiesof SK channels such that the consequential channel complex generatesthe sAHP.

We also used the slice preparation and UCL2077 to further evaluatethe effects of specifically suppressing the sAHP on hippocampalcell excitability. Consistent with the time course of the sAHP,the number of spikes at the end of a long (>500 ms) depolarizingpulse was substantially increased in the presence of UCL2077(Fig. 5F). This is in agreement with results from previous studiesusing neurotransmitters to suppress the sAHP (Storm, 1990; Sahand Faber, 2002). It is noteworthy that there was also a nonsignificant,variable increase in the number of spikes during the beginningof a current pulse in the presence of UCL2077 (Fig. 5E), whichmight be explained by the suggestion that the sAHP, in additionto the fast afterhyperpolarization and mAHP, can also be activatedby a single action potential (Storm, 1990). The effects of UCL2077were independent of alterations in resting membrane potential,spike threshold (Table 2), input resistance (Fig. 5D), and themAHP (Fig. 4, A and C), indicating that the compound has littleeffect on M or h channels, modulation of which can also substantiallyalter spike frequency adaptation (Aiken et al., 1995; Robinsonand Siegelbaum, 2003; Gu et al., 2005). This is an advantageof using UCL2077 over neurotransmitters such as acetylcholineor noradrenaline for studying the physiological role of thesAHP.

Because SK channels have previously been suggested to underliethe sAHP (Vergara et al., 1998), we compared the actions ofa specific SK channel blocker with those of UCL2077 on spikefrequency adaptation. Unlike UCL2077, the SK channel blockerapamin had a much smaller effect on action potential number(Fig. 5) and only significantly altered early spike frequencyadaptation (Fig. 5E). This result indicates that sAHP suppressionis likely to generate significantly more somatic action potentialsin response to a strong synaptic input and so increase neuronaloutput. Therefore, more action potentials would back-propagateinto dendrites and facilitate opening of NMDA receptor channelsby removing the Mg²⁺ block, enhancing further incoming excitatorysynaptic inputs and, perhaps, synaptic integration (Johnstonet al., 1999). SK channel inhibition may also affect NMDA receptoractivation. However, because it is possible that they are locatedin dendrites and spines near the NMDA receptor, this effectis more likely to be mediated by local dendritic and spine depolarization(Cai et al., 2004; Faber et al., 2005; Ngo-Anh et al., 2005).Thus, SK and sAHP channel blockers affect hippocampal cellularinformation processing by different mechanisms and may therebyinfluence learning and memory processes distinctly.

Acknowledgements

We thank Dr. P. Pedarzani (University College London, UnitedKingdom) for help with spike frequency train analysis.

Footnotes

This work was supported by the Wellcome Trust and the MedicalResearch Council.

ABBREVIATIONS: mAHP, medium afterhyperpolarization; sAHP, slowafterhyperpolarization; UCL2027, 2-tritylaminothiazole; FCS,fetal calf serum; HEK, human embryonic kidney; sI_AHP, slow afterhyperpolarizationcurrent; CGP 55,845, (2S)-3-[[(1S)-1-(3,4-dichlorophenyl)ethyl]amino-2-hydroxypropyl] (phenylmethyl) phosphinic acid; UCL2077,3-(triphenylmethylaminomethyl)pyridine; HVA, high-voltage-activated;NMDA, N-methyl-D-aspartate.

Address correspondence to: Mala M. Shah, Department of Pharmacology, University College London, Gower Street, London WC1E 6BT UK. E-mail: mala.shah{at}ucl.ac.uk

References

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Abstract
Materials and Methods
Results
Discussion
References

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