Evidence for Opening of Hair-Cell Transducer Channels after Tip-Link Loss

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (45)

Citing Articles via Google Scholar

Google Scholar

Articles by Meyer, J.

Articles by Gummer, A. W.

Search for Related Content

PubMed

PubMed Citation

Articles by Meyer, J.

Articles by Gummer, A. W.

Previous Article  |  Next Article

The Journal of Neuroscience, September 1, 1998, 18(17):6748-6756

Evidence for Opening of Hair-Cell Transducer Channels after Tip-Link Loss
Jens Meyer¹, David N. Furness², Hans-Peter Zenner¹, Carole M. Hackney², and Anthony W. Gummer¹
¹ Department of Otolaryngology, Section of Physiological Acoustics and Communication, University of Tübingen, 72076 Tübingen, Germany, and ² Department of Communication and Neuroscience, Keele University, Keele, Staffordshire ST5 5BG, United Kingdom

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The mechanosensitive transducer channels of hair cells have long been proposed to be gated directly by tension in the tiplinks. These are thin, elastic extracellular elements connectingthe tips of adjacent stereocilia located on the apical surfaceof the cell. If this hypothesis is true, the channels should closeafter destruction of tip links. The hypothesis was tested pharmacologicallyusing receptor currents obtained in response to mechanical stimulationof the stereociliary bundle of outer hair cells isolated fromthe adult guinea pig cochlea. Application of elastase (20 U/ml)or 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetra-acetic acid (BAPTA;5 mM), both of which are known to disrupt tip links in other hair-cellpreparations, led to the expected irreversible loss of receptorcurrents. However, the cells then displayed a maintained inwardcurrent, implying that channels were left permanently open. Thiscurrent was similar in magnitude to the receptor current beforetreatment and was reduced reversibly by known blockers of mechanosensitivechannels, namely, dihydrostreptomycin (100 µM), amiloride (300µM), and gadolinium ions (1 mM). These observations suggest thatthe maintained current flows through the mechanosensitive channels.Electron microscopical analysis of isolated hair cells, exposedto the same concentrations of elastase or BAPTA as in the electrophysiologicalexperiments, demonstrated an almost total loss of tip links inhair bundles that showed no evidence of other mechanical damage.It is concluded that although the tip links are required for mechanoelectricaltransduction, the channels are not gated directly by the tip links.

Key words: mechanoelectrical transduction; outer hair cells; tip link; elastase; low calcium; channel gating; tip-link hypothesis; BAPTA

  INTRODUCTION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The hair bundle is the mechanosensitive apparatus of hair cells responsible for sensory transduction in auditory, vestibular,and lateral-line systems (Hudspeth and Jacobs, 1979). In mammals,each hair bundle consists of stereocilia arranged in rows of differentlengths, which are connected by fine extracellular filaments (Pickleset al., 1984) called "tip links" that run between the tips ofthe shorter stereocilia and the sides of the taller ones in thenext row. Channels open when the bundle is deflected in the directionof the tallest stereocilium. It has been estimated that each stereociliumpossesses only one to five mechanosensitive transducer channels(Howard et al., 1988). A range of physiological experiments, includingextracellular focal recording around the hair bundle (Hudspeth,1982) and calcium imaging (Denk et al., 1995; Lumpkin and Hudspeth,1995), have suggested that these channels are likely to be locatedwithin 2-3 µm of the tips of the stereocilia. The directionalsensitivity of the receptor current to mechanical stimulationis consistent with (1) the axis of bilateral symmetry of the hairbundle (Shotwell et al., 1981), (2) elastic expansion of tip links(Howard et al., 1988), and (3) only one tip link connecting adjacentstereocilia. It has been proposed that the tip links gate thechannels like springs and that they are more or less directlyconnected to the mechanosensitive ion channels (Pickles et al.,1984). Direct mechanical gating is supported by the fact thatthe channels open with a delay of ~40 µsec after the mechanicalstimulus, which is much too fast to involve second messenger systems(Corey and Hudspeth, 1979).

In the resting position, the transducer channels are not totally closed but are reported to have an open probability of ~10-20%attributable to the normal resting tension of the gating springs(Corey and Hudspeth, 1983). If the tip links are the gating springs,then their destruction should lead to loss of this resting tensionand consequently to closure of the transducer channels. Tip linkshave been shown to be sensitive to elastase in glutaraldehyde-fixedmammalian organ of Corti (Osborne and Comis, 1990). Elastase treatmentof isolated guinea pig outer hair cells (OHCs) led to an irreversibleloss of mechanoelectrical transduction (Preyer et al., 1995),suggesting that the tip links are indeed essential elements ofthe transduction apparatus.

However, there is only indirect evidence of the tip-link hypothesis. Recently, a region directly below the tip-link regionwas described in which the cell membranes of adjacent stereociliacome into close contact (Hackney and Furness, 1995). Positivestaining with antibodies against the amiloride-binding site ofan epithelial sodium channel led those authors to propose thatthe transducer channels might be located in this position, whichthey called the "contact region." To date, the results of electrophysiologicalexperiments do not contradict a possible localization of the channelin this region. Because of the small distance between the tiplink and the contact region (~100 nm), it is extremely difficultto discriminate between these two locations, even with high-resolutioncalcium-imaging methods (Denk et al., 1995). The experiments presentedin this paper provide the first electrophysiological evidencethat the transducer channels are not directly connected to thetip links. They are in fact more consistent with a more indirectconnection between the links and the channels or with a localizationin the contact region.

Parts of this work have been presented at the 21^st ARO-Midwinter Research Meeting, St. Petersburg Beach, Fl, February 1998.

  MATERIALS AND METHODS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Cell isolation. OHCs were mechanically isolated from all turns of the adult guinea pig cochlea, with most cells derived fromthe apical one-half of the cochlea. The procedure is describedin detail elsewhere (Preyer et al., 1996). After separation, thecells were allowed to adhere to a poly-L-lysine- (0.1%; Sigma,Deisenhofen, Germany) coated coverslip in a droplet (200 µl) ofHBSS (300 mOsm/l; pH 7.25; Seromed, Berlin, Germany) at room temperature(20-22°C). The extracellular Ca²⁺ concentration in these experiments was 1.25 mM. For experimentsin which gadolinium ions were applied to the stereociliary bundle,a phosphate-free extracellular solution was used (in mM, 135 NaCl,5.4 KCl, 1.25 CaCl₂, 1 MgCl₂, 10 HEPES, and 300 mOsm/l, pH 7.25).All experiments were conducted under continuous video control(Hamamatsu 2400) using an inverted microscope (Labovert; Leitz,Wetzlar, Germany); total magnification was 800×.

Whole-cell recording. Electrophysiological recordings were made in current or voltage clamp at a holding potential of $-$ 60mV, using an EPC-7 patch-clamp amplifier (List-Electronic, Darmrstadt,Germany). Soda glass pipettes filled with K⁺ solution (in mM, 140 KCl, 2 MgCl₂, 11 EGTA, 0.1 CaCl₂, and 10HEPES) were used for whole-cell patch-clamp recordings (Hamillet al., 1981). The electrode resistance in extracellular fluidwas 2-5 M $Omega$ . Only cells with a resting potential less than $-$ 50mV and intact hair bundles, as assessed by light microscopy, wereused. In some experiments, KCl was replaced by 140 mM CsCl toblock most of the basolateral channels.

Drug application. Unless otherwise stated, all chemicals used were obtained from Sigma. Drugs were pressure-applied (Eppendorf5242) locally to the hair-bundle region from a distance of ~10µm, using double-barreled glass capillaries with a tip diameterof ~5 µm. Care was taken not to elicit stereocilia movement duringdrug application. With a double photodiode system (BPX48; SiemensAG, Erlangen, Germany) mounted on the microscope, it was possibleto ensure that there were no mechanical artifacts attributableto pressure application of the drugs. The aminoglycoside dihydrostreptomycin(DHSM; 100 µM) (Kroese et al., 1989; Kimitsuki and Ohmori, 1993),amiloride (300 µM) (Rüsch et al., 1994), or gadolinium ions (1mM) (Kimitsuki et al., 1996) were used to test for transductionchannels. For destruction of tip links, either the enzyme elastase(20 U/ml) (Osborne and Comis, 1990) or 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetra-aceticacid (BAPTA; 5 mM; for lowering the Ca²⁺ concentration) (Assad et al., 1991) was used. For blocking purinoreceptorslocated in the stereocilia (Mockett et al., 1994), suramin (300µM; Bayer, Wuppertal, Germany) was applied to the hair bundle.

Mechanically induced hair-bundle movement. A fluid jet composed of extracellular solution (HBSS) and driven by a piezoelectriccrystal was used to deflect the hair bundle (Saunders and Szymko,1989). The tip of the micropipette, which served as a nozzle forthe fluid jet, had a diameter of 5-8 µm and was placed at a distanceof ~10 µm from the hair bundle. The piezoelectric crystal wasdriven sinusoidally with a frequency of 8 Hz (Hewlett-Packard8904A multifunction synthesizer). The stimulus amplitude was setto produce saturated receptor currents. Data were stored on DATtape or were analog-to-digital-converted by a 14-bit PCM processorand stored on hard disk for later analysis by appropriate software(TIDA, Batelle, Germany).

Scanning electron microscopy. The effects of elastase and BAPTA application on hair-bundle morphology were assessed in isolatedhair cells. A total of six guinea pigs were used, and the cochleaewere partitioned between treatments as follows: BAPTA (n = 4),elastase (n = 4), and HBSS alone (n = 4). The cells were isolatedonto coverslips, using the same preparation techniques describedfor electrophysiological recordings. Cells were incubated in either5 mM BAPTA in HBSS for 10 min (n = 2) or 10 sec (n = 2), 20 U/mlelastase for 10 min, or HBSS for 10 min. The coverslips were thencarefully washed with HBSS and flooded with 2.5% glutaraldehydein 0.1 M sodium cacodylate buffer containing 2 mM CaCl₂. After1 hr in this fixative, they were post-fixed with 1% OsO₄ in thesame buffer for 1 hr, washed thoroughly, and then incubated alternatelyin saturated aqueous sodium thiocarbohydrazide solution for 20min and 1% OsO₄ in buffer twice more, with washing between eachstep. The preparations were then dehydrated in 70, 90, and twodry 100% ethanol steps (10 min each) before critical-point dryingfrom liquid CO₂, attached to stubs using sticky carbon pads, andexamined in a field-emission scanning electron microscope (HitachiS-4500) at 2-3 kV. All isolated cells with intact hair bundlesat appropriate orientations were examined, the number of possibletip-link sites were counted, and each site was assigned to oneof three categories: (1) "obscured" (in which the tip of the stereociliumwas covered by material and no assessment could be made), (2)"fused" (in which the stereocilium was fused to a neighbor ina way that precluded the presence of a link), and (3) "visible"(in which the region between two stereocilia was sufficientlyvisible to make a decision about the state of the tip links).If classified as visible, a site was assigned to one of five categories:(1) "intact" (tip links present), (2) "broken" (tip links severed),(3) "remnant" (stump of a tip link evident on the membrane ofa stereocilium), (4) "absent" (no evidence of any tip-link material),and (5) "uncertain" (some evidence of a link present but not capableof being readily categorized). In some cases, small portions ofthe organ of Corti containing several cells were left intact;in these cases, a small number of randomly selected bundles wasincluded in the assessment.

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Block of transducer channels by dihydrostreptomycin

Aminoglycosides, such as DHSM, cause a voltage-dependent block of mechanoelectrical transduction channels (Kroese et al.,1989; Kimitsuki and Ohmori, 1993). In the present series of experiments,DHSM was used as a control for the presence of open mechanoelectricaltransducer channels. The series of experiments in this sectiondescribe the effect of DHSM on mechanoelectrical transducer channelsof untreated OHCs.

Figure 1 shows the effect of DHSM (100 µM) on the receptor current of an isolated hair cell; sinusoidal deflection of thehair bundle with an amplitude of ~180 nm leads to a saturatedreceptor current of ~45 pA (Fig. 1a). Application of DHSM producesa reduction of the receptor current (Fig. 1b). The receptor currentfully recovers after terminating the application and washing outthe drug.

View larger version (25K):
[in this window]
[in a new window]
Figure 1. Effect of DHSM on the receptor current of an isolated outer hair cell. a, Sinusoidal mechanical stimulation of the hair bundle with an amplitude of 180 nm (top) leads to a saturated receptor response of 45 pA peak-to-peak (bottom). The holding potential is $-$ 60 mV. b, Application of 100 µM DHSM leads to reversible loss of the receptor current. The dashed lines in this and the following figures represent the resting current without mechanical stimulation. Inward currents are directed downward.

That DHSM actually blocks mechanoelectrical transducer channels in our experimental conditions was examined by applicationof DHSM during static deflection of the intact hair bundle, eitherin the direction of the tallest row of stereocilia (positive deflection)or in the opposite direction (negative deflection). Static deflectionof ~250 nm in the positive direction resulted in a maintained,saturated inward current, whereas static deflection of the sameamplitude in the negative direction resulted in a maintained zerocurrent (Fig. 2). That is, these static deflections caused thetransducer channels to be permanently opened or closed. Underthese conditions, DHSM had no effect during static deflectionin the negative direction but caused reversible reduction of thereceptor current during static deflection in the positive direction.This experiment indicates that the reduction of receptor currentby DHSM is indeed caused by blocking the mechanoelectrical transducerchannels.

View larger version (22K):
[in this window]
[in a new window]
Figure 2. DHSM blocks only the mechanoelectrical transducer channels of the outer hair cell. To examine whether it is really the transducer channel that is blocked by DHSM (100 µM), we statically deflected the hair bundle by ~250 nm in the positive or negative direction (top), so that all transducer channels were either open or closed, respectively (bottom). The receptor current is unaltered by the presence of DHSM during static negative deflection, whereas it is reduced by DHSM during static positive deflection. This indicates that under these experimental conditions, DHSM blocks only the mechanoelectrical transducer channels. Horizontal bars indicate application of 100 µM DHSM.

Abolition of transduction by elastase

If the tip links are indeed connected directly to the transducer channels, then their destruction by elastase should causesimilar effects to those caused by channel block with DHSM. Therefore,the responses of cells (n = 6) to application of DHSM (100 µM)followed by elastase treatment (20 U/ml) were examined. No obviouschange of shape of the hair bundle because of elastase treatment(such as splaying of the stereocilia) was seen by light microscopy.Exposure to DHSM during mechanical stimulation (Fig. 3a) led toreversible loss of the receptor current (Fig. 3b), similar tothat for the cell illustrated in Figure 1b. Then, elastase wasapplied after recovery (25 sec) of the receptor current from theDHSM treatment (Fig. 3c). Elastase caused an irreversible lossof the phasic component of the receptor current (8 Hz). But incontrast to DHSM, the current was not totally abolished. Instead,a sustained inward current was recorded (tonic current) with similaramplitude (50 pA) to the peak-to-peak value of the receptor (phasic)current before elastase treatment. This tonic component persistedin the absence of stereocilia deflection. The amplitude and tonicform of this stimulus-independent, inward current suggest thattransducer channels are in a permanently opened state after lossof tip links.

View larger version (38K):
[in this window]
[in a new window]
Figure 3. Elastase and DHSM have different effects on mechanoelectrical transduction. a-c, Whereas 100 µM DHSM causes reversible loss of the receptor current (b), subsequent application (25 sec later) of elastase (20 U/ml) to the same cell causes an irreversible loss of the phasic component of the current but a steady (tonic) inward current (c), which persisted in the absence of stereocilia deflection. d, The current flow after previous elastase treatment (in a cell different from that in b and c) is reversibly blocked with DHSM. e, The amplitude of the current suppressed by DHSM after elastase treatment is correlated (r = 0.95) with the receptor current before drug application. This indicates that the tonic current flows through permanently opened transducer channels after loss of tip links.

Evidence that the sustained current after elastase treatment originated from permanently opened transducer channels was obtainedby applying 100 µM DHSM after previous elastase treatment (ina different set of cells). Cells did not react to sinusoidal mechanicalstimulation (8 Hz) after elastase treatment. However, a totaland reversible block of the sustained inward current was causedby application of DHSM (Fig. 3d). The amplitude of this suppressedcurrent was similar to the amplitude of the receptor current beforeelastase treatment. This effect is summarized in Figure 3e fordifferent cells (n = 6). A strong positive correlation is seenbetween the amplitude of the DHSM-suppressed tonic current andthe amplitude of the receptor current before elastase treatment.This strongly suggests that the sustained current flows throughpermanently opened transducer channels.

Aminoglycosides such as DHSM are also known to affect other channels, such as P_2X receptors in the stereocilia (Lin et al.,1993). Binding of extracellular ATP to the P_2X receptors leadsto the opening of a cation channel and to a strong inward current(Nakagawa et al., 1990) and Ca²⁺ influx (Ashmore and Ohmori, 1990). To exclude the possibilitythat DHSM blocked P_2X receptors, we performed a second seriesof experiments (n = 3 cells). After treatment with elastase, apotent P_2X-receptor blocker, suramin (250 µM), was applied tothe hair bundle. Whereas DHSM led to block of the elastase-inducedtonic current, suramin had no detectable effect (data not shown).This indicates that P_2X receptors are not activated in the experimentswith elastase. In another series of experiments (Meyer et al.,1997), application of ATP (300 µM) to an intact hair bundle wasfound to produce a large inward current of several hundred picoamperes,much larger than the transduction current. The ATP-induced inwardcurrent was partially (50-70%) blocked by 250 µM suramin withoutaffecting mechanoelectrical transduction. The large differencebetween the amplitudes of the currents flowing through P_2X receptorsand transducer channels is additional evidence that the sustainedcurrent after elastase treatment is not attributable to activationof P_2X receptors. That suramin still blocks the purinergic channelsafter elastase treatment was not tested in these experiments.

Abolition of transduction by BAPTA

Because lowering the extracellular Ca²⁺ concentration to sufficiently low levels (<1 µM) has been shown to abolish transductionand destroy the tip links (Assad et al., 1991), the effects ofBAPTA, a potent Ca²⁺ chelator, on the receptor current were investigated (n = 8 cells).Application of 5 mM BAPTA immediately and irreversibly abolishedmechanoelectrical transduction (Fig. 4). Similar to the effectof elastase, a sustained inward current resulted from BAPTA application,which was maintained after mechanical stimulation was terminated.This finding suggests that the loss of mechanoelectrical transductioncaused by the destruction of tip links by BAPTA leads to openingof the transducer channels. In analogy to the elastase experiments,the application of DHSM (100 µM; n = 8) after BAPTA treatmentled to a total and reversible block of the tonic inward current(Fig. 5a), again indicating that the transducer channels werein an open state after BAPTA treatment. Two other known transducer-channelblockers, amiloride (300 µM; n = 3) and gadolinium ions (1 mM;n = 3), were also tested; both led to a total and reversible blockof the sustained inward current after BAPTA treatment (Fig. 5b,c).Both DHSM (100 µM; n = 3; Fig. 5d) and gadolinium ions (1 mM;n = 3; data not shown) blocked this sustained inward current atnegative holding potentials in a voltage-dependent manner. Thedependence of the amiloride block on voltage was not tested. Forthese experiments, CsCl was added to the internal solution toblock most of the basolateral K⁺ channels. Again, these results strongly suggest that the toniccurrent flows through transduction channels.

View larger version (46K):
[in this window]
[in a new window]
Figure 4. Effect of a reduction of extracellular Ca²⁺ on mechanoelectrical transduction. Application of 5 mM BAPTA, to reduce the extracellular Ca²⁺ concentration, results in an immediate and irreversible loss of the receptor current together with a sustained inward current approximately equal in magnitude to the receptor current before treatment.

View larger version (17K):
[in this window]
[in a new window]
Figure 5. Pharmacological block of the sustained current induced by BAPTA treatment. a-c, Application of 100 µM DHSM (a), 300 µM amiloride (b), or 1 mM gadolinium ions (c) leads to a total and reversible block of the tonic current induced by the treatment with 5 mM BAPTA. Horizontal bars indicate application of DHSM, amiloride, and Gd³⁺, respectively. d, DHSM blocks the tonic current at negative holding potentials in a voltage-dependent manner. These experiments indicate that the tonic current flows through permanently opened transduction channels after loss of tip links.

DC shift in response to DHSM application

The experiments presented above provide evidence for the opening of transducer channels after pharmacologically induced lossof tip links. Accordingly, channels could also open after mechanicaldisruption of tip links, as might occur because of the mechanicalisolation procedure. In this context it is important that in responseto DHSM application, approximately one-third of the cells notonly showed a block of the 8 Hz receptor current but showed aDC shift in the inhibitory direction (Fig. 6b,c, arrows). Theamplitude of this DC shift varied in different cells from hardlydetectable values (Fig. 6a) to amplitudes larger than the receptorcurrent (Fig. 6c). The size of the DC shift was not correlatedwith the amplitude of the receptor current. This kind of DC shiftwas also observed during application of amiloride (300 µM; datanot shown). A similar experiment with gadolinium ions was notconducted. Together with the finding that DHSM only blocks mechanoelectricaltransducer channels in our experimental configuration, these DCshifts provide additional evidence of permanently opened transducerchannels that do not respond to mechanical stimulation but thatcan be still blocked pharmacologically. The different amplitudeof the DC shift for different cells may reflect different degreesof hair-bundle damage during the isolation procedure.

View larger version (43K):
[in this window]
[in a new window]
Figure 6. In addition to blocking mechanotransduction, dihydrostreptomycin leads to a DC shift in the inhibitory direction in some cells. The amplitude of the DC shift varies from hardly detectable (a) to larger (b) values that could be much greater than the receptor current (c). This DC shift indicates a block of opened, mechanically insensitive ion channels.

Effect of elastase and BAPTA on hair-bundle morphology

Stereociliary bundles were examined electron microscopically to establish that the concentrations of elastase and BAPTA specificallycaused destruction of the tip links. In addition, the proportionof tip links that might have been damaged by the isolation procedurewas investigated. Drugs were applied before glutaraldehyde fixation.

Qualitative morphological assessment of single cells (Fig. 7A) and of small clumps of cells in the control solution (HBSSalone) showed that many hair bundles were intact and that tiplinks were present (Fig. 7B). By contrast, after treatment ofisolated cells with either 20 U/ml elastase (Fig. 7C) or 5 mMBAPTA (Fig. 7D), tip links were almost completely absent.

View larger version (147K):
[in this window]
[in a new window]
Figure 7. Effect of elastase and BAPTA on hair-bundle morphology. A, An example of a single hair cell after the isolation procedure. Note the intact hair bundle at the apex of the cell (arrow). Scale bar, 10 µm. B, Detail of a stereociliary bundle from an isolated hair cell after incubation in HBSS alone. Note the presence of tip links on many of the stereocilia (arrows). C, A stereociliary bundle after elastase treatment (20 U/ml). Note the complete absence of tip links. D, A stereociliary bundle after 10 min of BAPTA treatment (5 mM). Tip links are completely absent. Scale bars: B-D, 750 nm.

The degree of tip-link survival in each of these different treatments was quantified by counting the number of possible tip-linksites in the hair bundles of a random sample of cells and thenby assessing the condition of the tip link at each site (Table1). These counts showed that in controls, 30% of visible siteshad intact tip links, whereas broken links and remnants were visiblein a further 20 and 7%, respectively. After BAPTA treatment for10 sec, 8% of links were still intact, and the numbers of brokenlinks (0.7%) and remnants (3%) were reduced, although not proportionalto the degree of tip-link loss. After longer BAPTA treatment (10min), only 1.4% of links were intact, whereas more remnants werepresent (6.5%). After elastase treatment, the number of intactlinks was reduced to 2.5%, and neither remnants nor broken linkswere detected. However, side links appeared to be present afterboth elastase and BAPTA treatment. There was no morphologicalevidence of other effects on the hair bundle.


View this table:
[in this window]
[in a new window]
Table 1. Quantitative analysis of tip links after treatment with BAPTA or elastase

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Hair-bundle morphology after mechanical isolation

The morphological observations with scanning electron microscopy demonstrate that at least 30% of tip links survive the isolationprocedure. They also show that the concentrations of elastaseand BAPTA chosen for the electrophysiological investigations resultin almost complete loss of tip links. Although other isolatedcells appeared to have damaged stereocilia, only cells with intacthair bundles determined by light microscopy were chosen for theelectrophysiological experiments. The percentage of intact tiplinks found in the control group of isolated OHCs after preparationfor scanning electron microscopy (30%) is only slightly lowerthan that for bullfrog saccular hair cells (39%) in the intactepithelium reported by Assad et al. (1991). However, because itis not possible to determine whether the broken links or remnantsobserved are the result of the isolation procedure or the shrinkagethat occurs during the subsequent preparation for scanning electronmicroscopy, the data suggest that the average proportion of linkssurviving after isolation lies between 30 and 57%. Thus, the numberof intact tip links was more than an order of magnitude higherin the control cells than in the elastase- or BAPTA-treated cells.In this context, it is important to note that the hair cells forboth the electrophysiological and the morphological investigationswere isolated using identical procedures performed by the sameperson (J.M.).

Receptor currents of isolated OHCs

Isolated OHCs from the adult guinea pig cochlea are reported to be metabolically viable for at least 2 hr, as ascertainedby measuring the intracellular ATP concentration (Puschner andSchacht, 1997). Although many hair bundles seem to be morphologicallyintact after mechanical isolation (Fig. 7), the mechanically elicitedreceptor currents (10-112 pA; mean, 40 pA) appear to be smallcompared with other hair-cell systems; the amplitudes of receptorcurrents also show a wide range in different studies. For bullfrog,turtle, or neonatal mouse hair cells, receptor currents up toseveral hundred picoamperes have been reported (e.g., Corey andHudspeth, 1983; Crawford et al., 1991; Kros et al., 1992; Rüschet al., 1994), particularly when intact epithelia have been used.However, it must be remembered that the hair-bundle morphologyis different in other systems. Whereas nonmammalian hair cellscontain up to 300 stereocilia arranged in several rows (Hudspeth,1989), stereocilia of adult OHCs are arranged only in two to threerows, and the total number is lower, decreasing from the baseto the apical half of the cochlea and from the first to the thirdrow of OHCs (Lim, 1986). Most of the cells used in this studyfor patch-clamp recordings originated from the apical part ofthe cochlea, where the number of stereocilia can be extremelysmall, as few as 20 (D. N. Furness, personal observation). Theresults from neonatal cultured mouse hair cells are also not directlycomparable with those from OHCs from the adult guinea pig cochleabecause they have a different morphology. Unlike adult hair cells,neonatal hair cells have a kinocilium and show a variety of additionallinks between stereocilia (Furness et al., 1989). Moreover, thestereocilia are much smaller and presumably stiffer, and thereare several more rows in the hair bundle (Furness et al., 1989).Nevertheless, the transduction currents reported in our studyare comparable with those reported for chick hair cells (<100pA) (e.g., Kimitsuki and Ohmori, 1993; Kimitsuki et al., 1996;Zhao et al., 1996). Although not specifically investigated here,other studies from our laboratory have shown that the size ofthe saturated receptor potentials of adult, isolated hair cells(Preyer et al., 1996) is comparable with those of intracellularpotentials in vivo. Taken together with the quantitative electronmicroscopical investigations reported here, we conclude that althoughthe receptor currents are smaller than in other species, the isolatedhair cells appear to possess between 30 and 60% of their normalcomplement of tip links and that the size of the currents areconsistent with the number of stereocilia in the hair bundle.

Block of mechanoelectrical transduction by dihydrostreptomycin

Aminoglycoside antibiotics are known to reduce the receptor current of mechanoelectrical transduction channels in a dose-and voltage-dependent manner (Kroese et al., 1989; Denk et al.,1992; Kimitsuki and Ohmori, 1993). Because of its large molecularsize (>1 nm) compared with the estimated diameter of the channelpore (~0.7 nm), DHSM appears to block the pore physically (Kroeseet al., 1989). In our experiments, the application of DHSM toa hair bundle statically deflected to close the channels alsohad no effect, strongly suggesting that DHSM blocks only the transductionchannels. Thus, an effect of DHSM on the basolateral channelsin these experiments can be safely excluded. Control experimentswith the purinoreceptor antagonist suramin showed that the reducedcurrent was not caused by the action of DHSM on the P_2X receptors,prevalent in hair-cell stereocilia (Mockett et al., 1994). Therefore,DHSM served as a potent means of specifically blocking mechanoelectricaltransduction channels to study the action of the proteolytic enzymeelastase as well as BAPTA on the transduction apparatus.

Loss of mechanoelectrical transduction by elastase and BAPTA

The enzyme elastase is known to destroy tip links, as shown electron microscopically for frog vestibular hair cells (Takumidaet al., 1993) or fixed hair cells from the guinea pig cochlea(Osborne and Comis, 1990). These authors reported an almost completeabsence of tip links after elastase incubation for 10 min withthe same concentration used in this study (20 U/ml). Side linkswere less damaged (Osborne and Comis, 1990). Comparable resultswere obtained in this study using unfixed isolated OHCs. Elastaseproduced almost total loss of tip links without leaving any remnantor broken links. This is consistent with enzymatic degradationand implies a direct effect by elastase on the link itself oron both of its anchoring structures. However, it cannot be concludedthat the tip links consist of elastin; (1) elastase is known todigest other extracellular matrix proteins (Gronski et al., 1997),and (2) antibodies raised against elastin fail to label any partof the organ of Corti (Katori et al., 1996).

Preyer et al. (1995) showed that elastase led to an irreversible loss of the receptor potential of isolated OHCs after a fewseconds of application. They interpreted their results as a verificationof the tip-link hypothesis. Indeed, from their experiments itseems clear that tip links are essential elements for the transductionapparatus of cochlear hair cells. The suggested gating-springmodel for mechanoelectrical transduction assumes the tip link-thegating spring-to be connected directly to the channel protein(Gillespie, 1995). If true, then destruction of tip links shouldlead to closure of the transducer channels because of the absenceof an elastic restoring force. The closure of the mechanoelectricalchannels should be observed as a reduction of current flow intothe cell, comparable with the situation during block of the transducerchannels with DHSM. The experiments presented here have clearlyshown that the cells are no longer sensitive to mechanical stimulationafter elastase treatment. But instead of a loss of current, apermanent inward current was observed that could be totally andreversibly blocked with DHSM. This effect can be explained bythe transduction channels remaining in the open state after lossof tip links. This result is not consistent with the tip-linkhypothesis.

Low extracellular calcium levels (<1 µM), achieved by application of Ca²⁺ chelators such as BAPTA, are known to lead to destruction oftip links and to loss of mechanoelectrical transduction (Assadet al., 1991; Crawford et al., 1991). BAPTA treatment had a rapideffect, the number of intact tip links being substantially reducedwithin 10 sec (8% remaining). However, a 10 min treatment withBAPTA resulted in an almost total loss of tip links (1.4% remaining),whereas the proportion that remained as remnants was greater (6.5%).This suggests that as well as destroying most links, BAPTA mayweaken the remaining links, making them more susceptible to damageduring preparation for electron microscopy. This is consistentwith a chemical alteration of the links during BAPTA treatmentand accords with the suggestion that the link consists of twocomponents held together at a Ca²⁺-dependent site that becomes uncoupled after reduction of theCa²⁺ concentration (Assad et al., 1991). This appears to differ fromthe effects of elastase in that the former removes all evidenceof the link, whereas the latter occasionally leaves some remnantsat the anchoring points (Table 1).

The BAPTA experiments presented here resulted in effects similar to that of the elastase experiments, again suggesting thatthe transduction channels of treated hair bundles were in an openconfiguration. That both enzymatic and nonenzymatic means of destroyingtip links caused similar effects on transduction provides strongevidence that transducer channels open after tip-link loss, withoutbeing damaged. Assad et al. (1991) also reported an increase oftotal membrane current after treatment with BAPTA. They suggestedthat a shift in the activation of basolaterally situated voltage-dependentCa²⁺ channels caused the current increase. However, two lines of evidenceare provided here for the increased current being attributableto permanently opened transduction channels; (1) the tonic currentresulting from BAPTA treatment in our experiments had about thesame magnitude as the receptor current, and (2) the tonic currentcould be totally and reversibly blocked by DHSM, amiloride, andgadolinium ions.

Experiments with turtle hair cells have also shown a loss of mechanoelectrical transduction after exposure to low calcium(Crawford et al., 1991). The authors observed a strong inwardcurrent immediately after treatment with low-calcium saline. Thisstrong inward current is reported to return to near the controllevel. However, it must be pointed out that in contrast to ourprocedure, the experiments by Crawford et al. (1991) were performedby bathing whole cells in saline of different calcium concentrations.Therefore, an effect on the basolateral membrane or the hair bundlecannot be excluded in their experiments. Control experiments witha fluorescent dye (Lucifer yellow) suggested that in the presentelectrophysiological experiments, diffusion of the applied chemicalswas localized to the stereocilia bundle (Preyer et al., 1995).This could explain the difference between the present resultsand those of Crawford et al. (1991). It should be noted that whencells are exposed to low-calcium saline, fusion of adjacent stereociliamay occur (Hackney et al., 1997). In the present study, applicationof low-calcium saline to the hair bundles also produced a degreeof fusion, but the majority of stereocilia remained unfused, sothat this cannot fully explain the effects on transduction observedhere.

Implications for the localization of the transducer channels

The precise location of the transducer channels remains unknown (Gillespie, 1995; Hackney and Furness, 1995). It seems relativelyclear that one or two functional channels are located in the upperregion of each stereocilium (Jaramillo and Hudspeth, 1991; Denket al., 1995; Lumpkin and Hudspeth, 1995), a finding that wasconsistent with the hypothesis that the transducer channels aredirectly gated by the tip links. However, the opening of the transducerchannels after loss of tip links reported here suggests an indirectinteraction between the tip links and the channels.

  FOOTNOTES

Received June 5, 1998; accepted June 22, 1998.

This work was supported by the Deutsche Forschungsgemeinschaft, Klinische Forschergruppe "Hörforschung," Projekt A and theWellcome Trust. We thank V. Lesiuk for technical assistance.
Correspondence should be addressed to Dr. Jens Meyer, University of Tübingen, Department of Otolaryngology, Section of PhysiologicalAcoustics and Communication, Silcherstrasse 5, 72076 Tübingen,Germany.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Ashmore JF, Ohmori H (1990) Control of intracellular calcium by ATP in isolated outer hair cells of the guinea-pig cochlea. J Physiol (Lond) 428:109-131[Abstract/Free Full Text].
Assad JA, Shepherd GMG, Corey DP (1991) Tip-link integrity and mechanical transduction in vertebrate hair cells. Neuron 7:985-994[Web of Science][Medline].
Corey DP, Hudspeth AJ (1979) Response latency of vertebrate hair cells. Biophys J 26:499-506[Web of Science][Medline].
Corey DP, Hudspeth AJ (1983) Kinetics of the receptor current in bullfrog saccular hair cells. J Neurosci 3:962-976[Abstract].
Crawford AC, Evans MG, Fettiplace R (1991) The actions of calcium on the mechano-electrical transducer currents of turtle hair cells. J Physiol (Lond) 434:369-398[Abstract/Free Full Text].
Denk W, Keolian RM, Webb WW (1992) Mechanical response of frog saccular hair bundles to the aminoglycoside block of mechanoelectrical transduction. J Neurophysiol 68:927-932[Abstract/Free Full Text].
Denk W, Holt JR, Shepherd MG, Corey DP (1995) Calcium imaging of single stereocilia in hair cells: localization of transduction channels at both ends of tip links. Neuron 15:1311-1321[Web of Science][Medline].
Furness DN, Richardson GP, Russell IJ (1989) Stereociliary bundle morphology in organotypic cultures of the mouse cochlea. Hear Res 38:95-110[Web of Science][Medline].
Gillespie PG (1995) Molecular machinery of auditory and vestibular transduction. Curr Opin Neurobiol 5:449-455[Web of Science][Medline].
Gronski Jr TJ, Martin RL, Kobayashi DK, Walsh BC, Holman MC, Huber M, Van Wart HE, Shapiro SD (1997) Hydrolysis of a broad spectrum of extracellular matrix proteins by human macrophage elastase. J Biol Chem 272:12189-12194[Abstract/Free Full Text].
Hackney CM, Furness DN (1995) Mechanotransduction in vertebrate hair cells: structure and function of the stereociliary bundle. Am J Physiol 268:C1-C13[Abstract/Free Full Text].
Hackney CM, Furness DN, Mahendrasingam S, Macnamara M (1997) Ultrastructural and immunocytochemical investigations of the mechanotransducing apparatus of vertebrate hair cells. Proc Sendai Ear Symp 7:83-86.
Hamill OP, Marty A, Neher A, Sakmann B, Sigworth FJ (1981) Improved patch-clamp technique for high-resolution current recording from cells and cell-free membrane patches. Pflügers Arch 391:85-100[Web of Science][Medline].
Howard J, Roberts WM, Hudspeth AJ (1988) Mechanoelectrical transduction by hair cells. Annu Rev Biophys Biophys Chem 17:99-124[Web of Science][Medline].
Hudspeth AJ (1982) Extracellular current flow and the site of transduction by vertebrate hair cells. J Neurosci 2:1-10[Abstract].
Hudspeth AJ (1989) How the ear`s works work. Nature 341:397-404[Medline].
Hudspeth AJ, Jacobs R (1979) Stereocilia mediate transduction in vertebrate hair cells. Proc Natl Acad Sci USA 76:1506-1509[Abstract/Free Full Text].
Jaramillo F, Hudspeth AJ (1991) Localization of the hair cell's transduction channels at the hair bundle's top by iontophoretic application of a channel blocker. Neuron 7:409-420[Web of Science][Medline].
Katori Y, Hackney CM, Furness DN (1996) Immunoreactivity of sensory hair bundles of the guinea-pig cochlea to antibodies against elastin and keratan sulphate. Cell Tissue Res 284:473-479[Web of Science][Medline].
Kimitsuki T, Ohmori H (1993) Dihydrostreptomycin modifies adaptation and blocks the mechano-electric transducer in chick cochlear hair cells. Brain Res 624:143-150[Web of Science][Medline].
Kimitsuki T, Nakagawa T, Hisashi K, Komune S, Komiyama S (1996) Gadolinium blocks mechano-electric transducer current in chick cochlear hair cells. Hear Res 101:75-80[Web of Science][Medline].
Kroese ABA, Das A, Hudspeth AJ (1989) Blockage of the transduction channels of hair cells in the bullfrog's sacculus by aminoglycoside antibiotics. Hear Res 37:203-218[Web of Science][Medline].
Kros CJ, Rüsch A, Richardson GP (1992) Mechano-electrical transducer currents in hair cells of the cultured neonatal mouse cochlea. Proc R Soc Lond [Biol] 249:185-193[Medline].
Lim DJ (1986) Functional structure of the organ of Corti: a review. Hear Res 22:117-146[Web of Science][Medline].
Lin X, Hume RI, Nuttall AL (1993) Voltage-dependent block by neomycin of the ATP-induced whole cell current of guinea-pig outer hair cells. J Neurophysiol 70:1593-1605[Abstract/Free Full Text].
Lumpkin EA, Hudspeth AJ (1995) Detection of Ca²⁺ entry through mechanosensitive channels localizes the site of mechanoelectrical transduction in hair cells. Proc Natl Acad Sci USA 92:10297-10301[Abstract/Free Full Text].
Meyer J, Preyer S, Zenner H-P, Gummer AW (1997) The effect of static hair-bundle displacement on the mechanoelectric transduction in isolated cochlear hair cells. In: Diversity in auditory mechanics (Lewis ER, Long GR, Lyon RF, Narins PM, Steele CR, Hecht-Poinar E, eds), pp 538-541. London: World Scientific.
Mockett BG, Housley GD, Thorne PR (1994) Fluorescence imaging of extracellular purinergic receptor sites and putative ecto-ATPase sites on isolated cochlear hair cells. J Neurosci 14:6992-7007[Abstract].
Nakagawa T, Akaike N, Kimitsuki T, Komune S, Arima T (1990) ATP-induced current in isolated outer hair cells of guinea pig cochlea. J Neurophysiol 63:1068-1074[Abstract/Free Full Text].
Osborne MP, Comis SD (1990) Action of elastase, collagenase and other enzymes upon linkages between stereocilia in the guinea-pig cochlea. Acta Otolaryngol 110:37-45[Medline].
Pickles JO, Comis SD, Osborne MP (1984) Cross-links between stereocilia in the guinea-pig organ of Corti and their possible relation to sensory transduction. Hear Res 15:103-112[Web of Science][Medline].
Preyer S, Hemmert W, Zenner HP, Gummer AW (1995) Abolition of the receptor potential response of isolated mammalian outer hair cells by hair-bundle treatment with elastase: a test of the tip-link hypothesis. Hear Res 89:187-193[Web of Science][Medline].
Preyer S, Renz S, Hemmert W, Zenner HP, Gummer AW (1996) Receptor potential of outer hair cells isolated from base to apex of the adult guinea-pig cochlea: implications for cochlear tuning mechanisms. Aud Neurosci 2:145-157.
Puschner B, Schacht J (1997) Energy metabolism in cochlear outer hair cells in vitro. Hear Res 114:102-106[Web of Science][Medline].
Rüsch A, Kros CJ, Richardson GP (1994) Block by amiloride and its derivatives of mechano-electrical transduction in outer hair cells of mouse cochlear cultures. J Physiol (Lond) 474:75-86[Abstract/Free Full Text].
Saunders JC, Szymko YM (1989) The design, calibration, and use of a water microjet for stimulating hair cell sensory hair bundles. J Acoust Soc Am 86:1797-1804[Web of Science][Medline].
Shotwell SL, Jacobs R, Hudspeth AJ (1981) Directional sensitivity of individual vertebrate hair cells to controlled deflection of hair bundles. Ann NY Acad Sci 374:1-10.
Takumida M, Harada Y, Kanemi Y (1993) Influence of elastase and hyaluronidase on the ciliary interconnecting systems in frog vestibular sensory cells. ORL J Otorhinolaryngol Relat Spec 55:77-83[Medline].
Zhao YD, Yamoah EN, Gillespie PG (1996) Regeneration of broken tip links and restoration of mechanical transduction in hair cells. Proc Natl Acad Sci USA 94:15469-15474.

Copyright © 1998 Society for Neuroscience 0270-6474/98/18176748-09$05.00/0

This article has been cited by other articles:

D. Gothelf, N. Farber, E. Raveh, A. Apter, and J. Attias
Hyperacusis in Williams syndrome: Characteristics and associated neuroaudiologic abnormalities
Neurology, February 14, 2006; 66(3): 390 - 395.
[Abstract] [Full Text] [PDF]

A. Brandt, J. Striessnig, and T. Moser
CaV1.3 Channels Are Essential for Development and Presynaptic Activity of Cochlear Inner Hair Cells
J. Neurosci., November 26, 2003; 23(34): 10832 - 10840.
[Abstract] [Full Text] [PDF]

J. Gartzke and K. Lange
Cellular target of weak magnetic fields: ionic conduction along actin filaments of microvilli
Am J Physiol Cell Physiol, November 1, 2002; 283(5): C1333 - C1346.
[Abstract] [Full Text] [PDF]

J. E. Gale, W. Marcotti, H. J. Kennedy, C. J. Kros, and G. P. Richardson
FM1-43 Dye Behaves as a Permeant Blocker of the Hair-Cell Mechanotransducer Channel
J. Neurosci., September 15, 2001; 21(18): 7013 - 7025.
[Abstract] [Full Text] [PDF]

C. Boyer, J. J. Art, C. J. Dechesne, J. Lehouelleur, J. Vautrin, and A. Sans
Contribution of the Plasmalemma to Ca2+ Homeostasis in Hair Cells
J. Neurosci., April 15, 2001; 21(8): 2640 - 2650.
[Abstract] [Full Text] [PDF]

O. P. Hamill and B. Martinac
Molecular Basis of Mechanotransduction in Living Cells
Physiol Rev, April 1, 2001; 81(2): 685 - 740.
[Abstract] [Full Text] [PDF]

B. Kachar, M. Parakkal, M. Kurc, Y.-d. Zhao, and P. G. Gillespie
High-resolution structure of hair-cell tip links
PNAS, November 21, 2000; 97(24): 13336 - 13341.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Web of Science (45)

Citing Articles via Google Scholar

Google Scholar

Articles by Meyer, J.

Articles by Gummer, A. W.

Search for Related Content

PubMed

PubMed Citation

Articles by Meyer, J.

Articles by Gummer, A. W.