Calcium-dependent inactivation of calcium channels in cochlear hair cells of the chicken

doi:10.1113/jphysiol.2007.135582

CELLULAR

Calcium-dependent inactivation of calcium channels in cochlear hair cells of the chicken

Seunghwan Lee², Olga Briklin¹, Hakim Hiel¹ and Paul Fuchs¹

¹ Center for Hearing and Balance, Department of Otolaryngology, Head and Neck Surgery, and Center for Sensory Biology, Johns Hopkins University School of Medicine, Baltimore, MD 21205, USA
² Department of Otolaryngology – Head & Neck Surgery, Hanyang University, Seoul, Korea

Abstract

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Abstract
Introduction
Methods
Results
Discussion
References

Voltage-gated calcium channels support both spontaneous andsound-evoked neurotransmitter release from ribbon synapses ofcochlear hair cells. A variety of regulatory mechanisms mustcooperate to ensure the appropriate level of activity in therestricted pool of synaptic calcium channels ( $~$ 100) availableto each synaptic ribbon. One potential feedback mechanism, calcium-dependentinactivation (CDI) of voltage-gated, L-type calcium channels,can be modulated by calmodulin-like calcium-binding proteins.CDI of voltage-gated calcium current was studied in hair cellsof the chicken's basilar papilla (analogous to the mammaliancochlea) after blocking the predominant potassium conductances.For inactivating currents produced by 2.5 s steps to the peakof the current–voltage relation (1 mM EGTA internal calciumbuffer), single exponential fits yielded an average decay timeconstant of 1.92 ± 0.18 s (mean ± S.E.M.,n = 12) at 20–22°C, while recovery occurred witha half-time of $~$ 10 s. Inactivation produced no change in reversalpotential, arguing that the observed relaxation did not resultfrom alternative processes such as calcium accumulation or activationof residual potassium currents. Substitution of external calciumwith barium greatly reduced inactivation, while inhibition ofendoplasmic calcium pumps with t-benzohydroquinone (BHQ) orthapsigargin made inactivation occur faster and to a greaterextent. Raising external calcium 10-fold (from 2 to 20 mM) increasedpeak current 3-fold, but did not alter the extent or time courseof CDI. However, increasing levels of internal calcium bufferconsistently reduced the rate and extent of inactivation. With1 mM EGTA buffering and in 2 mM external calcium, the availablepool of calcium channels was half-inactivated near the restingmembrane potential (–50 mV). CDI may be further regulatedby calmodulin-like calcium-binding proteins (CaBPs). mRNAs forseveral CaBPs are expressed in chicken cochlear tissue, andantibodies to CaBP4 label hair cells, but not supporting cells,equivalent to the pattern seen in mammalian cochlea. Thus, molecularmechanisms that underlie CDI appeared to be conserved acrossvertebrate species, may provide a means to adjust calcium channelopen probability, and could serve to maintain the set-pointfor spontaneous release from the ribbon synapse.

(Received 1 May 2007; accepted after revision 24 July 2007; first published online 26 July 2007)
Corresponding author P. Fuchs: The Johns Hopkins University School of Medicine, 818 Ross Building, 720 Rutland Avenue, Baltimore, MD 21205, USA. Email: pfuchs{at}jhmi.edu

Introduction

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Abstract
Introduction
Methods
Results
Discussion
References

Voltage-gated calcium channels (VGCCs) in hair cells providethe trigger for both spontaneous and sound-evoked activity ofcochlear afferent neurons (Robertson & Paki, 2002). In amphibia(Lewis & Hudspeth, 1983; Roberts et al. 1990; Prigioni et al. 1992;Rodriguez-Contreras & Yamoah, 2001), reptiles (Art & Fettiplace, 1987;Art et al. 1993; Schnee & Ricci, 2003), birds (Fuchs et al. 1990;Zidanic & Fuchs, 1995) and mammals (Nakagawa et al. 1991;Beutner & Moser, 2001; Engel et al. 2002; Bao et al. 2003;Marcotti et al. 2003; Michna et al. 2003), evidence consistentlyshows that the majority of hair cell calcium channels are ‘L-type’.That is, they are dihydropyridine sensitive, and preferentiallypermeant to barium over calcium. Some studies, particularlyin vestibular hair cells, have identified a distinctive minorityof channels that are dihydropyridine insensitive (Su et al. 1995;Rodriguez-Contreras & Yamoah, 2001). The L-type calciumchannel of hair cells is encoded by the ${alpha}$ 1D or Ca_V1.3 gene (Green et al. 1996;Kollmar et al. 1997b; Platzer et al. 2000; Ramakrishnan et al. 2002;Brandt et al. 2003; Michna et al. 2003; Dou et al. 2004; Hafidi & Dulon, 2004).VGCCs in most hair cells activate and deactivate rapidly (withinless than 1 ms) and remain open during 100–200 ms commandsto membrane potentials positive to –40 mV, showing littleor no inactivation. This has long been viewed as consistentwith the role of these channels in spontaneous, as well as sound-evoked,transmitter release from hair cells. More recently however,evidence has been found for slow, seconds-long inactivationof voltage-gated calcium currents in hair cells of amphibia(Rispoli et al. 2000; Martini et al. 2004), reptiles (Schnee & Ricci, 2003),and the inner (Marcotti et al. 2003) and outer (Michna et al. 2003)hair cells of the mammalian cochlea. Does this inactivationhave functional relevance and if so, how is it reconciled withthe requirement for steady-state gating? The implication isthat additional processes must exist to modulate inactivation.That is, such modulation would serve to ensure spontaneous activity,and at the same time, an adequate dynamic range for sound-evokedgating of the limited number of calcium channels ( $~$ 100) thoughtto operate at each ribbon synapse (Roberts et al. 1990; Martinez-Dunst et al. 1997;Brandt et al. 2005; Fuchs, 2005), emphasized by the fact thateach ribbon is the sole input for a single auditory neuron inmammals. Also, such a mechanism could contribute to differencesin spontaneous rate among cochlear afferent neurons (Merchan-Perez & Liberman, 1996).

Calcium-dependent inactivation (CDI) of L-type calcium channelsis mediated by calmodulin (Liang et al. 2003), raising the possibilitythat the extent of CDI could be regulated by calmodulin-likecalcium-binding proteins (CaBPs). Indeed, recent work has shownthat calmodulin-dependent CDI of Ca_V1.3 is diminished by heterologouscoexpression with CaPBs (Yang et al. 2006). One of these, CaBP4,is preferentially expressed in retinal photoreceptors (Haeseleer et al. 2004)and cochlear inner hair cells (Yang et al. 2006), both employingribbon synapses. Still further heterogeneity of CDI may resultfrom alternative splicing of the Ca_V1.3 ${alpha}$ subunit to eliminateportions of the calmodulin-binding ‘IQ’ domain (Shen et al. 2006).

The present work seeks to characterize CDI and to nominate potentialmolecular mechanisms in chicken auditory hair cells. The chickenbasilar papilla (‘cochlea’) is a tonotopically organizedsensory epithelium (Chen et al. 1994) containing some 10, 000hair cells differentially innervated by afferent and efferentnerve fibres (Fischer, 1992). Avian (chicken) hair cells sharefeatures in common with those of cold-blooded vertebrates, aswell as with those of mammals. Spontaneous afferent activityhas preferred intervals (Salvi et al. 1992), presumably reflectingthe electrical resonance in chicken auditory hair cells (Fuchs et al. 1988)like that shown previously in turtles (Crawford & Fettiplace, 1981).As in mammals, a subset of hair cells of chickens, ‘tallhair cells’, are preferentially innervated by afferentnerve fibres, possess numerous presynaptic structures (ribbons)and have relatively large voltage-gated calcium currents (Martinez-Dunst et al. 1997).Corresponding tonotopic gradients occur in the expression ofcalcium-buffering proteins such as calbindin (Hiel et al. 2002).Finally, developmental changes in ion channel expression bychicken hair cells (Fuchs & Sokolowski, 1990) parallel thoseobserved in the mammalian cochlea (Kros et al. 1998). The chickenotocyst and basilar papilla provide a useful model system forin vitro developmental studies (Sokolowski et al. 1993), andan important source of comparative information. We have examinedthe slow inactivation of calcium currents in tall hair cellsof the chicken's basilar papilla, analogous to inner hair cellsof the mammalian cochlea. The expectation is that basic molecularmechanisms of calcium channel modulation that are conservedthroughout vertebrates should be evident here.

Methods

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Abstract
Introduction
Methods
Results
Discussion
References

The basilar papilla (auditory sensory epithelium) was dissectedfrom the temporal bone of chickens (Gallus gallus, 1–21days old), after they had been deeply anaesthetized (intramuscularpentobarbitol) and decapitated, according to a protocol (no.AV04M160) approved by the Institutional Animal Care and UseCommittee of Johns Hopkins University. Procedures for innerear microdissection and isolation of hair cells essentiallyfollowed those published previously (Fuchs et al. 1988). Theexcised basilar papilla (auditory epithelium) was treated brieflywith protease (0.1 mg ml^–1 protease type XXIV, Sigma-Aldrich)to facilitate the removal of the overlying tectorial membrane.‘Tall’ hair cells (analogous to inner hair cellsin the mammalian cochlea) were aspirated from a region 1.0–1.2mm from the apical tip of the papilla, and then dispersed intoa recording chamber.

Whole-cell, gigohm-seal voltage clamp

Whole-cell, patch-clamp recordings were made from the isolatedhair cells as previously described (Fuchs & Evans, 1990;Fuchs et al. 1990) using commercially available equipment andsoftware (Axon Instruments 200B, pCLAMP). Patch pipettes (5–10M ${Omega}$ resistance) were coated with Sylgard or ski wax to reducecapacitance. The seal resistance before breaking into the whole-cellrecording mode was always > 2 G ${Omega}$ . In the standard ‘inactivationprotocol’, the membrane was clamped to the potential atwhich calcium current was maximal (between –20 and 0 mV)for 2 s. The extent of inactivation was determined as the fractionaldrop in current amplitude during that step. For example, a reductionfrom 100 pA to 30 pA would constitute 70% inactivation. Thetime constant of inactivation was taken from a single exponentialfit to the entire 2 s-long inward current. The cell was allowedto recover for 60 s between successive inactivation protocols.In other experiments a 100 mV, 100 ms-long voltage ramp wasused to assess calcium current magnitude, voltage dependenceand reversal potential before and following an inactivatingvoltage step. The same voltage ramp was also used to assessthe calcium current I–V relation from different holdingpotentials, ranging from $~$ –90 to –50 mV. Inthese latter experiments the extent of inactivation was takenas the ratio of peak currents obtained during I–V rampsfrom different holding potentials.

Both internal and external saline solutions were designed toblock predominant potassium currents that normally overlie andobscure the smaller voltage-gated calcium currents of hair cells.The internal (pipette) solution contained (mM): 140 CsMeSO₄,10 Hepes, 3 Mg₂ATP, 5 phosphocreatine, 5.6 glucose, and pH to7.3; 290 mosmol l^–1. This was modified to provide a rangeof calcium buffer concentrations as noted in Results. The standardexternal saline contained (mM): 90 NaCl, 6 KCl, 1 MgCl₂, 10Hepes, 30 tetraethyl-ammonium chloride (TEA), 5.6 glucose, 2pyruvate, 3,4-aminopyridine, and 500 nM apamin, pH 7.3, 310mosmol l^–1. The measured junction potential was $~$ –10mV and this has been added to the reported values. Divalentcations (calcium or barium) were added as 2 or 20 mM of thechloride salt. Compounds designed to alter calcium-dependentinactivation were dissolved into external saline and perfusedinto the bath after initial recordings in control conditions.All tissue preparation, cell isolation and recordings were conductedat room temperature (20–22°C).

Reverse-transcriptase polymerase chain reaction from chicken basilar papilla

Basilar papillae were quickly removed from the severed headand stored on dry ice. RNA was extracted with TRIzol reagent,chloroform, isopropyl alcohol and RNase free water, and subjectedto reverse transcription with oligo(dT)12–18 primers.Polymerase chain reactions (30 cycles) were run with primersspecific for each of the three chicken CaBP orthologues identifiedfrom a homology search of the chicken genome (NCBI http://www.ncbi.nlm.nih.gov/genome/guide/chicken/).Amplified cDNAs were separated on gels, and bands of the predictedsize cut out, subcloned into bacteria, excised, purified andsequenced (Johns Hopkins Sequencing Center).

Immunohistology

The inner ear was fixed in situ for 1 h by perfusion with 2%paraformaldehyde. The otic capsule was dissected free and immersedin fixative for 2–3 h more. The entire capsule was thenprepared for cryosectioning at 10–14 µm thickness.Mounted sections were exposed to goat anti-ChAT (Chemicon) andrabbit anti-CaBP4, or rabbit anti-CaBP1 (both CaBP antibodiesfrom F. Haeseleer, University of Washington, Seattle, WA). Secondaryantibodies were conjugated to Alexa 488 or Alexa 555. Labelledsections were viewed and photographed on an upright Nikon fluorescencemicroscope.

Results

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Abstract
Introduction
Methods
Results
Discussion
References

Potassium blockers isolate hair cell calcium current

Hair cells were isolated from a region approximately 1 mm fromthe apical tip of the basilar papilla, corresponding to approximately1 kHz along the tonotopic axis (Chen et al. 1994). As in mammals,auditory hair cells in birds can be subdivided based on thepattern of innervation and cross-cochlear position. ‘Tall’hair cells in chickens are analogous to inner hair cells ofmammals, having the majority of afferent synaptic contacts andlittle if any efferent innervation (Fischer, 1992). In contrast,chicken short hair cells have efferent, rather than afferentinnervation (Zidanic, 2002). Consistent with this differentialsynaptic function, tall hair cells consistently have largervoltage-gated calcium currents than do short hair cells (Martinez-Dunst et al. 1997).

The membrane conductance of chicken hair cells is dominatedby voltage-gated potassium channels (Fig. 1A, 5 mM externalcalcium, holding voltage –64 mV). Thus, recording conditionswere designed to eliminate the predominant potassium currentsand reveal the smaller, usually covert, voltage-gated calciumcurrents. This involved a panel of potassium channel blockers,and elevating external calcium to enlarge usually small currentsthrough these channels (Fuchs et al. 1990; Martinez-Dunst et al. 1997).The standard protocol used 20 mM external calcium, and holdingvoltages of –70 mV (Fig. 1B, C and D), negative to theactivation range of the calcium channels (Zidanic & Fuchs, 1996).Internal caesium completely eliminated the rapidly activatingcalcium-sensitive (BK) potassium current of these hair cells.However, especially in the ‘tallest’ hair cells,whole-cell recordings still showed substantial outward currentsat positive membrane potentials, as well as large, slow inwardtail currents (Fig. 1B). These residual currents probably resultfrom the significant numbers of slowly gating delayed rectifierand inward rectifier channels found in this cell type (Murrow, 1994).These voltage-gated currents are particularly problematic becausethey are blocked by the external barium that was used for differentiatingcalcium-dependent inactivation of inward currents. Thus, 30mM TEA and 3 mM 4-aminopyridine (4-AP) were added to the externalsaline. This combination eliminated slow tail currents and effectivelyisolated inward calcium currents (Fig. 1C). The peak leak-correctedmembrane current was inward up to +60 mV on average (+59.5 ±1.0 mV, mean ± S.E.M., n = 28), and did notvary as a function of calcium buffer (see later).

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Figure 1. Isolation of calcium current
A, selected membrane currents produced by 60 ms-long voltage commands (–100 to +30 in 10 mV steps) in a chicken cochlear hair cell (holding potential –64 mV). The external solution contained 5.6 mM calcium and the internal saline was buffered with 10 mM EGTA. No potassium channel blockers were used. The observed currents include those through large-conductance (BK) potassium channels, delayed rectifier and inward rectifier K⁺ channels (inward currents produced during negative voltage steps). B, selected membrane currents produced by indicated voltage commands with internal caesium and 20 mM external calcium (holding voltage –70 mV). Residual unblocked delayed rectifier channels carry the outward currents positive to –40 mV, and inward rectifier channels may contribute to the slow tail currents. C, hair cell membrane currents produced by indicated voltage commands as in B, but with addition of external TEA and 4-AP. Purely inward currents are visible up to +20 mV and no slow tail currents are seen. D, inward currents produced by a 2 s step to 0 mV with TEA and 4-AP in the external saline (holding voltage –70 mV). Addition of 1 µM apamin caused no additional change, arguing that little or no SK current was present. External calcium 20 mM in C and D.

Under these conditions, prolonged depolarizing voltage stepsthen produced inward currents that decayed gradually (Fig. 1D).The mean time constant of decay obtained for maximal inwardcurrents was 1.92 ± 0.17 s, ± S.E.M., n =12) at room temperature. This slow inactivation is the focusof this work and subsequent experiments will demonstrate thatit results largely from calcium-dependent inactivation (CDI)of the hair cell's L-type calcium channels. Before doing so,however, one further control experiment was required: a testfor possible contributions from calcium-dependent potassiumcurrents through small-conductance (SK) channels (Matthews etal. 2004). These are ordinarily activated through the releaseof acetylcholine at the efferent synapses (Yuhas & Fuchs, 1999)that are found on short hair cells. If also present in thesetall hair cells, SK channels could be activated during prolongedvoltage-gated calcium influx, as has been shown in reptilian(Tucker & Fettiplace, 1996) and mammalian hair cells (Marcotti et al. 2004)and their contribution might then be mistaken for calcium-dependentinactivation of calcium current. However, exposure to the SKchannel blocker apamin at concentrations 10 times those thatblock hair cell channels (Yuhas & Fuchs, 1999) producedno change in decay of the inward current (or amplitude of thesubsequent tail current) produced by a long depolarization (Fig. 1D),suggesting that few if any SK channels are available in thesetall hair cells. Nevertheless, 500 nM apamin was added to theexternal saline throughout these studies to assure that allSK activity was eliminated.

Parameters of inactivation

As an additional assessment of the ionic basis of slow inactivation,the voltage dependence and reversal potential of calcium currentwas measured with a 100 mV, 100 ms-long voltage ramp just before,and immediately after a 2 s inactivating step. If ‘inactivation’results from calcium accumulation or contamination by residualunblocked potassium channels, rather than a simple closure ofcalcium channels, the reversal potential should undergo a negativeshift as a function of ‘inactivation’. In particular,SK channels in chicken hair cells are permeant to Cs⁺ as wellas K⁺ (Yuhas & Fuchs, 1999), yielding a negative equilibriumpotential under these recording conditions. Although the calciumcurrent fell by more than 50% in the illustrated cell, the leak-correctedI–V relation showed no significant change in shape orin the location of the reversal potential, $~$ +70 mV inthis cell (Fig. 2A).

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Figure 2. Characterization of inactivation
A, current produced in 20 mM external calcium (1.0 mM EGTA internal buffering) during 100 mV/100 ms voltage ramp 100 ms before, and 100 ms after, a 2 s depolarization to 0 mV that produced 60% inactivation (holding voltage –70 mV). Each I–V relation was corrected for the linear leak calculated between –70 and –60 mV. After leak correction the reversal potential was +74 mV before and +82 mV after inactivation. B, recovery from inactivation (peak current as percentage of control, from voltage ramps as in A, measured at successive times after a 2 s inactivating step to 0 mV (20 mM external calcium, 1.0 mM EGTA internal buffering). Calculated doubling time (single exponential fit) was 10.5 s with r² only 0.59; 95% confidence interval from 5.9 to 47.9 s. C, percentage inactivation (during 2 s depolarization) as a function of peak calcium current in each cell (20 mM external calcium). Different concentrations of EGTA are indicated by the symbols ( $bullet$ = 0.1 mM, ${blacktriangledown}$ = 1.0 mM, ${blacksquare}$ = 10 mM). Linear fits through each buffer condition have slopes not statistically different from zero. The relation between buffer concentration and percentage inactivation is shown in detail in Fig. 5.

Given the seconds-long onset of inactivation, it was necessaryalso to determine the rate of recovery so that repeated measurescould be made on a single cell without risking accumulationof inactivation. The rate of recovery from inactivation wasdelineated by applying voltage ramps at various times afteran inactivating voltage step to a maximally activating voltage(1 mM EGTA internal, 20 mM calcium external). Under these conditions,a test ramp 100 ms after a 2 second-long inactivating step produceda peak inward current that was $~$ 50% smaller than one immediatelybefore the inactivating step. Over the course of approximately10 s, the peak inward current recovered nearly completely (Fig. 2B).The recovery half-time derived from a single exponential fitwas 10.5 s. However, there was considerable variability betweencells, and this value ranged from 5.9 to 47.9 s (95% confidencelimits). To avoid residual inactivation, standard protocolswere spaced at least 60 s apart throughout these experiments.

We also sought to determine whether there was significant intercellularvariability in the extent of inactivation. Calcium current magnitude(but not cell volume) varies significantly among chicken auditoryhair cells (Martinez-Dunst et al. 1997). Thus it was of interestto determine whether inactivation varied as a function of calciumcurrent amplitude among different hair cells, perhaps offeringinsights into underlying mechanisms. Maximal current amplitudein 20 mM calcium (obtained from the I–V relation) wascompared to the percentage inactivation (the percentage changein current amplitude during a 2 s inactivating voltage step)among the population of cells buffered with different concentrationsof EGTA. However, no correlation was found. Lines fitted throughpoints for each group of cells with a given buffer concentrationhad slopes not different from zero (Fig. 2C). Nor was any correlationfound in cells buffered with BAPTA (not shown). This lack ofcorrelation argues that current magnitude, i.e. calcium accumulationper se, did not determine the extent of inactivation. In particular,buffer saturation is unlikely to play a significant role, sinceeven with minimal internal buffering (0.1 mM), calcium currentsize did not predict the extent of inactivation between cells.However, as is evident from the vertical displacement of thefit for each group of cells, the extent of inactivation appearedto vary with the concentration of calcium buffer. This is shownfurther in Fig. 5.

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Figure 5. Effects of internal calcium buffering
A, membrane currents in 20 mM external calcium during a 2 s step to 0 mV (from holding voltage –70 mV) from two hair cells with different concentrations of internal EGTA. Peak currents in 0.1 EGTA normalized (by 0.77) to match those in 10 mM EGTA. Single exponentials (continuous white lines) fitted to the current decay yielded time constants of 1.4 s in 0.1 mM EGTA and 2.2 s in 10 mM EGTA. B, time constant of inactivation calculated as in A for cells in 20 mM external calcium, under different conditions of buffering indicated below each set of two bars (black for EGTA, grey for BAPTA). Time constants in 0.1 mM EGTA and 0.1 mM BAPTA were significantly shorter (P < 0.03, ANOVA) than those in the other conditions, which otherwise were not statistically different. C, black bars indicate the percentage inactivation of current carried by 20 mM calcium into hair cells buffered with 0.1 mM (66 ± 3.1%, mean ± S.E.M., n = 14), 1.0 mM (48 ± 2.2%, n = 13) and 10.0 mM (37 ± 2.2%, n = 12) EGTA. All means in calcium differ significantly from neighbouring values (P < 0.03, ANOVA). Grey bars indicate measurements from the same cells with calcium substituted by 20 mM barium. D, black bars indicate percentage inactivation of current carried by 20 mM calcium into hair cells buffered with 0.1 mM (56 ± 1.9%, mean ± S.E.M., n = 13), 1.0 mM (42 ± 2.4%, n = 13) and 10.0 mM (28 ± 1.6%, n = 12) BAPTA. All means in calcium differ significantly from neighbouring values (P < 0.03, ANOVA). With barium as charge carrier (grey bars) the percentage inactivation ranged between 14 and 19% with no significant differences between neighbours.

Calcium current inactivation was measured during 2 s steps tovoltages ranging up to +20 mV (Fig. 3A). Inactivation, thatis the percentage loss of current during the voltage step, wasminimal negative to –30 mV and maximal positive to 0 mV(Fig. 3B), and in some cases fell again at more positive voltages(Fig. 3A) corresponding roughly with the peak of the I–Vcurve for calcium. The mean percentage inactivation for eightcells as a function of membrane potential shows that this behaviourwas consistent, essentially saturating positive to 0 mV. Significantlyreduced inactivation was not always seen at +20 mV (Fig. 3B)and still stronger depolarization usually damaged the cells.This form of voltage dependence also argues against substantialcontamination by voltage-activated delayed rectifier-type potassiumcurrents, since these should rise steeply at more positive membranepotentials (Fig. 1B).

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Figure 3. Voltage dependence of calcium-dependent inactivation
A, currents recorded in 20 mM external calcium during a family of 2 s voltage commands to the indicated membrane potentials (holding voltage –70 mV). At –40 and –30 mV little or no inactivation occurred. Maximal inactivation occurred at 0 and +10 mV, while inactivation decreased at +20 mV. Internal calcium buffered with 10 mM BAPTA. B, the percentage inactivation in 20 mM calcium at different membrane potentials averaged (± S.E.M.) from 7 cells (4 with 10 mM BAPTA, 2 with 1 mM EGTA, 1 with 0.1 mM EGTA). Inactivation rose as the membrane was depolarized between –40 and 0 mV, then reached a plateau with no significant differences between means at positive membrane potentials (by ANOVA).

Calcium dependence of CDI

Substitution of external calcium (20 mM) with barium (20 mM)enlarged the inward currents (Fig. 4A). However, inactivationwas considerably reduced and slowed with barium as charge carrier(Fig. 4B). In the illustrated records (peak currents normalized)inactivation reached 75% in calcium and 15% in barium, whilethe time constant of inactivation was 1.2 s in calcium and 5.0s in barium (group averages are given in Fig. 5). In additionto showing a requirement for calcium influx, the identical (essentiallyzero) slow tail currents in calcium and barium confirmed thatlittle contamination by slow inward rectifier channels remainedin these recording conditions (compare to Fig. 1B), since inwardrectifier channels in chicken hair cells are blocked by externalbarium (Fuchs et al. 1990). Note also that the illustrated cellwas weakly buffered with 0.1 mM EGTA, associated with strongerinactivation than seen with 1 or 10 mM EGTA (see Fig. 5).

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Figure 4. The effects of calcium influx and internal stores
A, current–voltage relation obtained with 20 mM calcium or barium in the external saline (holding voltage –70 mV). Barium current was on average twice the amplitude of calcium current in all cells tested. B, a 2 s step to 0 mV from a holding voltage of –70 mV produced a slowly decaying inward current ( ${tau}$ = 0.8 s, from single exponential fit, continuous white line) carried by 20 mM calcium (0.1 mM EGTA buffering). Substitution with barium yielded a larger current (scaled by 0.63) that decayed much more slowly ( ${tau}$ = 6.5 s, from single exponential fit, continuous white line). C, membrane current during a 2 s step to 0 mV before (‘control’) and 4 min after the addition of 50 µM SERCA blocker benzo-hydroquinone (‘50 µM BHQ’) (20 mM calcium external, 1.0 mM EGTA internal buffer, holding voltage –70 mV). Inactivation was more extensive in the SERCA blocker. Peak control current was scaled by 0.8. Continuous white line indicates double exponential fit to each record. D, the percentage inactivation in control (46.2 ± 2.9%, mean ± S.E.M., n = 5), 50 µM BHQ (88.9 ± 3.5%, n = 5), control (40 ± 11%, n = 3) and 10 µM thapsigargin (72 ± 10%, n = 4). Each treatment condition differed significantly (P < 0.03) from its independent control (Student's two-tailed t test).

Substitution with barium demonstrated a requirement for calciuminflux for inactivation to occur. The seconds-long time coursefurther implies that relatively slow mechanisms such as endoplasmiccalcium pumping could modulate the underlying cytoplasmic calciumsignal. This possibility was examined using compounds that inhibitthe activity of endoplasmic calcium (SERCA) pumps (e.g. tert-benzo-hydroquinone(BHQ) and thapsigargin). In cells buffered with 1 mM EGTA, inactivationbecame faster after treatment with 50 µM BHQ (Fig. 4C).During exposure to SERCA blockers the time course of inactivationwas better fitted with a double, rather than single exponential,due to the appearance of a faster ( ${tau}$ $~$ 100 ms) initial rateof decay. The origin of this process was not determined, butit did require that control records also be fitted with doubleexponentials. Nonetheless, in five cells, the second, slowertime constant of decay (over the last 1.8 s) was faster in thepresence of BHQ, 1.18 s (± 0.7 s, S.E.M.), than in controlconditions for those same cells, 1.71 s (±0.3 s, S.E.M.).Correspondingly, the extent of inactivation was approximatelydoubled after SERCA block (Fig. 4D). Thapsigargin (10 µM)had a nearly equivalent effect, producing a 1.8-fold increasein the extent of inactivation in four cells (Fig. 4D). The effectsof the SERCA blockers were not reversible during the time courseof these recordings.

The effect of cytoplasmic buffering on CDI

To explore further the calcium dependence of inactivation, thestandard recording protocols were repeated using
internal (pipette)solution containing EGTA or BAPTA at concentrations rangingfrom 0.1 to 10 mM. In keeping with its hypothesized calciumdependence, the degree of inactivation varied with buffer concentration.Lower concentrations of buffer resulted in faster, more extensiveinactivation (Fig. 5A). Averaged time constants obtained fromeach group suggested a progressive slowing with higher bufferconcentrations, as well as generally slower time constants inBAPTA than in EGTA (Fig. 5B). However, statistical tests (ANOVA)showed significance (P < 0.05) only between the lowest bufferconcentration (EGTA or BAPTA) and any other groups with 20 mMexternal calcium. The loss of significance arose primarily fromincreased variance in higher buffer conditions, presumably reflectingthe difficulty of extrapolating fits beyond the 2 s time courseof the conditioning voltage step.

Given the uncertainty of extrapolated time constant measureswith strong buffering, it proved useful alternatively to measurethe extent of inactivation that also varied systematically withthe internal buffer concentration (cf. Fig. 2C). Inactivation(the fraction of current lost) reached an average value of 66± 3.1% (± S.E.M., n = 14) in 0.1 mMEGTA, 48 ± 2.1% (n = 14) in 1 mM EGTA, and 37 ±2.2% (n = 12) in 10 mM EGTA (Fig. 5C). All these meanswere significantly different (P < 0.05 by ANOVA). Inactivationaveraged approximately 17% when barium was substituted for calciumand this residual level had no significant correlation withbuffer concentration. Although it did not reach statisticalsignificance, the average peak current was largest in the highestbuffer concentration ( $~$ 120 pA in 10 mM EGTA compared to $~$ 100 pAin 0.1 mM EGTA). Finally, there were no significant differencesin the reversal potential measured during voltage ramps in thedifferent buffering conditions.

A second series of experiments was undertaken with BAPTA ratherthan EGTA as the internal calcium buffer. Here a similar relationshipwas obtained, with stronger inactivation for lower concentrationsof buffer, with mean values significantly different at the 0.05level (ANOVA) (Fig. 5D). Also as in EGTA, the largest initialcurrents were found with the strongest buffering, but againshort of a significant difference. There appeared to be a trendtoward less inactivation for equivalent concentrations of BAPTAcompared to EGTA (e.g. 28% in 10 mM BAPTA, versus 37% in 10mM EGTA); however, those differences were not statisticallysignificant. As with EGTA buffering, modest residual inactivationremained when barium served as charge carrier, but again thisdid not vary with buffer concentration.

Inactivation in 2 mM calcium

The foregoing experiments were carried out by eliciting maximalcurrents (at voltages corresponding to the peak of the I–Vrelation), with 20 mM calcium in the external saline. This calciumconcentration was chosen for consistency with earlier work (Martinez-Dunst et al. 1997)and to optimize signal-to-noise of the relatively small currentsin these cells. The question arises then whether CDI occurswith more physiological calcium loads. Total calcium in chickenserum is $~$ 5 mmol l^–1 (Prosser & Brown, 1961) whileionized calcium levels range from 1.4 to 1.6 mmol l^–1,(e.g. Peltonen et al. 2006), and vary significantly during theegg-laying cycle, as well as between males and females. To approximatenormal conditions then, calcium-dependent inactivation was alsoexamined with 2 mM external calcium, and compared to 20 mM calciumon a cell-by-cell basis. For seven cells the peak inward currentin 2 mM calcium was on average only one-third that in 20 mMcalcium (Fig. 6A). Nonetheless, the extent and time course ofinactivation after a 2 s conditioning voltage step (to the peakof the I–V relation) was not significantly different underthese two conditions (assessed by voltage ramps). This findingimplies that the inactivation process was saturated by prolongedinflux from either 20 or 2 mM calcium.

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Figure 6. Inactivation in ‘physiological’ external calcium
A, inward currents were measured in 13 cells exposed successively to 2 and 20 mM external calcium (1.0 mM EGTA internal buffer). Peak inward currents and percentage inactivation were determined from voltage ramps executed before and after a 2 s depolarization to the peak of the I–V relation from –70 mV holding voltage. The time constant of inactivation was taken from a single exponential fit to the current during the inactivating step. Only peak currents were significantly different (105 ± 8.8 pA, mean ± S.E.M., n = 13 in 20 mM calcium; 32 ± 2.4 pA, in 2 mM calcium, n = 13). The percentage inactivation in 20 mM calcium (48 ± 2.1%, mean ± S.E.M.) and in 2 mM calcium (44 ± 4.3%) was not different (nor did it differ from the independent measurements averaged in Fig. 5, 48 ± 2.2%), nor was the time constant of decay significantly different (1.9 ± 0.2 and 1.7 ± 0.3 s, mean ± S.E.M., in 20 and 2 mM calcium, respectively). B, voltage ramps evoked inward currents in 2 mM external calcium from a holding potential of –90 mV (grey traces) before and after an I–V collected at –50 mV holding potential (black trace). In 7 such experiments, the ratio of peak inward currents obtained at –50 mV to those from –90 mV was 0.50 ± 0.20 (mean ± S.E.M.). The average recovery value (comparing the I–V peak from –90 mV before and 1 min after inactivation) was 0.82 ± 0.08.

A second question is to what extent CDI occurs at lower levelsof calcium channel gating, in particular, near the resting membranepotential at which spontaneous transmitter release occurs. Thisquestion was addressed in 2 mM external calcium by alternatelyholding the membrane potential at –90 or –50 mVfor 1 min, then probing calcium channel availability with avoltage ramp. For seven cells the ratio of peak inward currentsmeasured at –50 and –90 mV was 0.50 ± 0.07(± S.E.M.). The inactivation occurring at –50mV could be completely reversed by holding again at a negativemembrane potential for 1 min (Fig. 6B). After correction forleak conductance there was no consistent change in reversalpotential or overall position of the I–V curve.

Calcium-binding proteins in chicken basilar papilla

Calcium-binding proteins (CaBPs) constitute a family of sevencalmodulin-like proteins that are thought to modulate the interactionsof calmodulin (CaM) with target binding sites (Haeseleer et al. 2002).Nucleotide sequences for mammalian CaBPs were used to scan thechicken genome (NCBI), and three partial coding sequences homologouswith mouse and human CaBPs 1, 4 and 7 were identified. MessengerRNA was reverse-transcribed from microdissected lagenar ducts(containing the basilar papilla and lagena). All three orthologousCaBPs could be amplified using specific primers. Nucleotideidentities of the RT-PCR products were 77% for CaBP4, 82% forCaBP1, and 89% for CaBP7. The RT-PCR products were translatedto the equivalent amino acid sequences and compared to thosefor mice. Only three conservative amino acid substitutions were
predicted by the chicken CaBP1 and CaBP7 cDNAs (Fig. 7A and C).However, the CaBP4 cDNA from chicken yielded a substantiallymore variant amino acid sequence, with only $~$ 70% identical aminoacids, although the majority of those changed were for aminoacids in the same functional groups (Fig. 7B).

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Figure 7. CaBPs in chicken basilar papilla
RT-PCR using specific chicken CaBP sequences (derived by homology search of the chicken genome with mouse CaBPs) amplified products corresponding to mammalian orthologues of CaBPs 1, 4 and 7. The derived sequences were translated to amino acids and compared to their mouse orthologues, with variant amino acids indicated by grey background. A, an RT-PCR product corresponding to 97 amino acids of mouse CaBP1 differed by only 3 conserved substitutions. B, the CaBP4 RT-PCR product encoded 103 amino acids, of which 72 were identical and 20 were conserved substitutions compared to the mouse CaBP4 sequence, the remainder being changes to dissimilar amino acids. C, the RT-PCR product encoding 71 amino acids corresponding to mouse CaBP7 had only 3 conservative amino acid substitutions.

Further confirmation of the expression of CaBPs was achievedusing antibodies against the mammalian proteins, although theseare available only for CaBP1 and CaBP4. When applied to cross-sectionsfrom the basilar papilla, antibodies to CaBP1 bound relativelywell to the stereociliary bundle and cuticular plate regionof hair cells (Fig. 8A and B) in addition to labelling the tectorialmembrane and various cell types in the tegmentum vasculosum.On the other hand, hair cell cytoplasm, and in particular, thesynaptic pole of tall (inner-like) hair cells, were not welllabelled. Although cholinergic efferent neurons preferentiallylabel short, outer-like hair cells in chicken (Zidanic & Fuchs, 1996;Zidanic, 2002), a few efferent endings labelled red with antibodiesagainst choline acetyl-transferase (ChAT) demarcate the synapticpole of tall hair cells in Fig. 8. When antibodies to CaBP4were employed, tectorial membrane and tegmentum vasculosum wereessentially unlabelled, but more robust labelling of hair cellsomata was achieved (Fig. 8B). Stereociliary bundles, however,were not labelled. In contrast to the pattern seen with antibodiesto CaBP1, CaBP4 antibodies labelled the synaptic pole of thehair cells as strongly as the cuticular plates. These same patternsof labelling were achieved in four separate preparations.

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Figure 8. CaBP antibody labelling in chicken basilar papilla
Antibodies available for CaBP1 and CaBP4 were used to label cryosections (across the long axis) of the chicken basilar papilla. Tegmentum vasculosum (collapsed onto basilar papilla) is labelled ‘TV’. Tectorial membrane (visible only in A) is labelled ‘TM’. A single hair cell is shaded white in each image for reference. A, antiserum to CaBP1 (green) bound to hair cells and supporting cells in the basilar papilla, to the tectorial membrane, and to cells in the tegmentum vasculosum. Immunolabelling of hair cells was concentrated in the cuticular plate and hair bundle. Antibody to choline acetyl-transferase (ChAT, red) indicates the position of efferent cholinergic endings located on the synaptic pole of hair cells. B, antiserum to CaBP4 (green) strongly labelled hair cells in the basilar papilla, and TV very faintly. Hair cell cytoplasm labelled as strongly as cuticular plate (hair bundles did not label). Each image has been optimized for brightness and contrast, so relative intensities cannot be compared between panels. ChAT antibody label (in red) indicates efferent boutons at synaptic pole of hair cells.

	Discussion

Top Abstract Introduction Methods Results Discussion References

The present work was designed to establish the extent of calcium-dependentinactivation of hair cells in the chicken basilar papilla (analogousto the mammalian cochlea). This model was chosen as a representativevertebrate whose auditory epithelium shares features of structureand function with those of both cold-blooded reptiles and mammals(Fuchs et al. 1988; Fischer, 1992; Fuchs & Murrow, 1992),and for which substantial auditory nerve data also exist (e.g.Saunders et al. 2002). Prolonged (2 s) maximal calcium currentsproduced significant inactivation that was itself calcium dependent.The extent of inactivation in any one hair cell depended onthe magnitude of calcium influx (i.e. as adjusted by changingmembrane potential and so driving force on influx). Higher concentrationsof internal calcium buffer (10 mM) reduced the extent of inactivation,while lower levels of buffer (0.1 mM) were associated with morerapid, more extensive inactivation.

Several observations suggest that CDI depended on the relativelygradual accumulation of calcium into an as-yet undefined ‘activationvolume’. First, the time constant of CDI was slow, nearly2 s for maximal currents with 1 mM EGTA internal buffering,with a recovery half-time of 10 s. Secondly, the extent of inactivationwas not significantly different whether EGTA or BAPTA was usedas the internal calcium buffer, arguing that the more rapidbinding kinetic of BAPTA was irrelevant to this gradual process.Finally, reduced activity of endoplasmic calcium pumps increasedthe extent and hastened the time course of CDI, as though acausal cytoplasmic calcium pool was enhanced. One possible interpretationof these observations is that CDI involves a process such asa phosphorylation cascade in which calcium-dependent kinasesare involved. Activity in
this cascade would vary in proportionto free calcium in the cytoplasm, itself a product of influx,buffering and pumping.

Given this hypothesis, it is of interest that the extent ofinactivation did not vary with peak calcium current among thepopulation of cells studied. The implication is that the cell-to-cellvariation in calcium channel number (peak current) is accompaniedby equivalent variation in associated mechanisms of calciumhomeostasis. This is consistent with the supposition that calciumchannels are clustered specifically at ribbon synapses in chicken(Martinez-Dunst et al. 1997) as in other species (Roberts et al. 1990;Issa & Hudspeth, 1994; Ricci et al. 2000; Khimich et al. 2005).That is, each cluster of calcium channels generates its ownlocal calcium load, regulated by local calcium stores and otherhomeostatic mechanisms. Variations in the extent of inactivationbetween cells could result from the relative positioning ofribbons (density), such that local calcium loads could overlap,or that fixed buffer efficacy (endoplasmic stores) varied betweencells. The other related observation is that CDI was equivalentwhether external calcium was 2 or 20 mM. Apparently then, thecytoplasmic ‘activation volume’ for calcium wassaturated by prolonged influx from either of these conditions.This is not entirely surprising since the total change in drivingforce was theoretically less than 20% (26 mV out of $~$ 150 mV).However, this supposition will depend on total buffer concentration.Finally, CDI was substantial even for moderate levels of calciuminflux. The peak calcium current was reduced by 50% when haircells were simply held at –50 mV, near the presumptivein vivo membrane potential and near the foot of the calciumactivation curve.

Studies of auditory hair cells of reptiles (Schnee & Ricci, 2003)and mice (Marcotti et al. 2003; Michna et al. 2003) also haveshown that voltage-gated calcium currents inactivate. In turtlehair cells, for example, inactivation was sensitive to substitutionof calcium with barium, and the extent of inactivation fellapproximately 30% when internal BAPTA was raised from 1 to 30mM. A virtually identical degree of inactivation of calciumcurrents ( $~$ 50%) was obtained in turtle and chicken hair cellsby a 40 mV change in holding potential. In contrast, inactivationin turtle hair cells was relatively insensitive to calcium bufferingwhen compared to that in chicken, and barium preserved inactivationto a larger extent in turtle than in chicken hair cells. Itis not known yet whether the L-type calcium channels of turtlepossess calmodulin-binding sites, so the molecular basis forthese distinctions remains to be explored. Inactivation hasbeen reported in both inner (Marcotti et al. 2003) and outer(Michna et al. 2003) hair cells of the neonatal mammalian cochlea.In both cell types inactivation was dependent on external calciumand the calcium driving force as expected for CDI. It was notdetermined whether CDI varied with internal calcium bufferingor alterations in calcium store function.

CDI has been described at other ‘tonic’ (ribbon-dependent)synapses. In bipolar cell terminals from goldfish retina (von Gersdorff & Matthews, 1996)the extent and time course of CDI were strikingly similar tothat reported here in chicken hair cells and, as in the presentreport, lower concentrations of internal calcium buffer wereassociated with more extensive CDI. The similarities betweenthese two systems may not be accidental. Both goldfish bipolarcells (Logiudice et al. 2006) and chicken cochlear hair cells(Kollmar et al. 1997b) express Ca_V1.3 ( ${alpha}$ 1D), a member of thedihydropyridine-sensitive L-type family of voltage-gated calciumchannels. This also is the predominant gene encoding voltage-gatedcalcium channels in mammalian cochlear hair cells (Platzer et al. 2000).Recent studies have raised the possibility that CDI of thesechannels can be modulated by calmodulin-like calcium-bindingproteins (CaBPs) (Yang et al. 2006). These proteins may alterthe action of calmodulin bound to IQ domains on the carboxytail of Ca_V1.3, thereby disrupting CDI that depends on calmodulin.CaBPs were first identified in mammalian retina (Haeseleer et al. 2000).CaBP4 was found to be expressed specifically in photoreceptorterminals (Haeseleer et al. 2004) and subsequently in innerhair cells of the rat cochlea (Yang et al. 2006). However, unlikehair cells the photoreceptors express a different L-type calciumchannel, Ca_V1.4, that does not inactivate when expressed inheterologous cells (McRory et al. 2004). Thus, coexpressionwith CaBP4 had no impact on inactivation, but did cause a negativeshift in the voltage activation range of Ca_V1.4 (Haeseleer et al. 2004).Functional interactions are likely, then, to depend on boththe specific channel type, including splice variants (Kollmar et al. 1997a;Ramakrishnan et al. 2002; Shen et al. 2006), and which of thefamily of calmodulin-like proteins are present in each celltype. In this context it is interesting that the partial sequencefor CaBP4 found here was more variant from mouse than that foreither CaBP1 or CaBP7. One might speculate that greater functionalspecialization has occurred for this ‘synaptic’calcium-binding protein.

What functional role might CDI play in chicken cochlear haircells? The slow time course argues against participation inadaptation of afferent nerve firing that occurs within $~$ 20 ms(Crumling & Saunders, 2007), and has a temperature Q₁₀ ofonly 1.2 (Crumling & Saunders, 2005). Afferent nerve adaptationin chicken may reflect exhaustion of presynaptic vesicular pools(Spassova et al. 2004). Rather, CDI as observed in the presentwork could be important as a negative feedback mechanism thatadjusts the ‘steady-state’ number of available calciumchannels. This becomes particularly critical considering thelimited number of calcium channels available to each ribbon.The relation between ribbon size and calcium current amplitude(Martinez-Dunst et al. 1997) implies that hair cells largelyrestrict channel expression to release sites, thereby minimizingtotal calcium flux. Indeed various studies report that onlya small number of channels, 100 or fewer, will be found at eachsynaptic ribbon (Roberts et al. 1990; Martinez-Dunst et al. 1997;Brandt et al. 2005; Fuchs, 2005) and modelling studies suggestthat small, dense channel clusters will provide the best temporalresolution for synaptic release (Wu et al. 1996). With sucha limited pool of channels to draw upon, the hair cell mustensure that some level of release continues even at rest, whilesimultaneously preserving the widest possible dynamic range.A negative feedback process such as steady-state CDI observedin the present work is able to make such adjustments, providingthat CDI itself can be fine-tuned to each cell's specific needs.We propose that calmodulin-like calcium-binding proteins couldserve this role in avian, as in mammalian hair cells.

References

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Abstract
Introduction
Methods
Results
Discussion
References

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