Differences Between Stereocilia Numbers on Type I and Type II Vestibular Hair Cells

A major outstanding goal of vestibular neuroscience is to understand the distinctive functional roles of type I and type II hair cells. One important question is whether these two hair cell types differ in bundle structure. To address this, we have developed methods to characterize stereocilia numbers on identified type I and type II hair cells in the utricle of a turtle, Trachemys scripta. Our data indicate that type I hair cells, which occur only in the striola, average 95.9 ±16.73 (SD) stereocilia per bundle. In contrast, striolar type II hair cells have 59.9 ± 8.98 stereocilia, and type II hair cells in the adjacent extrastriola average 44.8 ± 10.82 stereocilia. Thus type I hair cells have the highest stereocilia counts in the utricle. These results provide the first direct evidence that type I hair cells have significantly more stereocilia than type II hair cells, and they suggest that the two hair cell types may differ in bundle mechanics and peak mechanoelectric transduction currents.

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Temporal Bone Studies of the Human Peripheral Vestibular System

Annals of Otology Rhinology & Laryngology ◽

10.1177/00034894001090s504 ◽

2000 ◽

Vol 109 (5_suppl) ◽

pp. 20-25 ◽

Cited By ~ 38

Author(s):

Kojiro Tsuji ◽

Steven D. Rauch ◽

Conrad Wall ◽

Luis Velázquez-Villaseñor ◽

Robert J. Glynn ◽

...

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Ganglion Cells ◽

Significant Loss ◽

Small Sample ◽

Type I ◽

Type Ii ◽

Vestibular Hair Cells ◽

Scarpa's Ganglion ◽

Temporal Bones

Quantitative assessments of vestibular hair cells and Scarpa's ganglion cells were performed on 17 temporal bones from 10 individuals who had well-documented clinical evidence of aminoglycoside ototoxicity (streptomycin, kanamycin, and neomycin). Assessment of vestibular hair cells was performed by Nomarski (differential interference contrast) microscopy. Hair cell counts were expressed as densities (number of cells per 0.01 mm2 surface area of the sensory epithelium). The results were compared with age-matched normal data. Streptomycin caused a significant loss of both type I and type II hair cells in all 5 vestibular sense organs. In comparing the ototoxic effect on type I versus type II hair cells, there was greater type I hair cell loss for all 3 cristae, but not for the maculae. The vestibular ototoxic effects of kanamycin appeared to be similar to those of streptomycin, but the small sample size precluded definitive conclusions from being made. Neomycin did not cause loss of vestibular hair cells. Within the limits of this study (maximum postototoxicity survival time of 12 months), there was no significant loss of Scarpa's ganglion cells for any of the 3 drugs. The findings have implications in several clinical areas, including the correlation of vestibular test results to pathological findings, the rehabilitation of patients with vestibular ototoxicity, the use of aminoglycosides to treat Meniere's disease, and the development of a vestibular prosthesis.

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Vestibular Type I and Type II Hair Cells. 1: Morphometric Identification in the Pigeon and Gerbil

Journal of Vestibular Research ◽

10.3233/ves-1997-7503 ◽

1997 ◽

Vol 7 (5) ◽

pp. 393-406

Author(s):

Anthony J. Ricci ◽

Katherine J. Rennie ◽

Stephen L. Cochran ◽

Golda A. Kevetter ◽

Manning J. Correia

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Cell Types ◽

Type I ◽

Type Ii ◽

Body Width ◽

Fixed Tissue ◽

Neck Width ◽

I Cells ◽

Plate Width

Classically, type I and type II vestibular hair cells have been defined by their afferent innervation patterns. Little quantitative information exists on the intrinsic morphometric differences between hair cell types. Data presented here define a quantitative method for distinguishing hair cell types based on the morphometric properties of the hair cell’s neck region. The method is based initially on fixed histological sections, where hair cell types were identified by innervation pattern, type I cells having an afferent calyx. Cells were viewed using light microscopy, images were digitized, and measurements were made of the cell body width, the cuticular plate width, and the neck width. A plot of the ratio of the neck width to cuticular plate width (NPR) versus the ratio of the neck width to the body width (NBR) established four quadrants based on the best separation of type I and type II hair cells. The combination of the two variables made the accuracy of predicting either type I or type II hair cells greater than 90%. Statistical cluster analysis confirmed the quadrant separation. Similar analysis was performed on dissociated hair cells from semicircular canal, utricle, and lagena, giving results statistically similar to those of the fixed tissue. Additional comparisons were made between fixed tissue and isolated hair cells as well as across species (pigeon and gerbil) and between end organs (semicircular canal, utricle, and lagena). In each case, the same morphometric boundaries could be used to establish four quadrants, where quadrant 1 was predominantly type I cells and quadrant 3 was almost exclusively type II hair cells. The quadrant separations were confirmed statistically by cluster analysis. These data demonstrate that there are intrinsic morphometric differences between type I and type II hair cells and that these differences can be maintained when the hair cells are dissociated from their respective epithelia.

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Architecture of the Mouse Utricle: Macular Organization and Hair Bundle Heights

Journal of Neurophysiology ◽

10.1152/jn.00831.2007 ◽

2008 ◽

Vol 99 (2) ◽

pp. 718-733 ◽

Cited By ~ 60

Author(s):

A. Li ◽

J. Xue ◽

E. H. Peterson

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Quantitative Data ◽

Posterior Margin ◽

Adult Mouse ◽

Type I ◽

Type Ii ◽

Cell Type ◽

Vestibular Hair Cells ◽

Utricular Macula

Hair bundles are critical to mechanotransduction by vestibular hair cells, but quantitative data are lacking on vestibular bundles in mice or other mammals. Here we quantify bundle heights and their variation with macular locus and hair cell type in adult mouse utricular macula. We also determined that macular organization differs from previous reports. The utricle has ∼3,600 hair cells, half on each side of the line of polarity reversal (LPR). A band of low hair cell density corresponds to a band of calretinin-positive calyces, i.e., the striola. The relation between the LPR and the striola differs from previous reports in two ways. First, the LPR lies lateral to the striola instead of bisecting it. Second, the LPR follows the striolar trajectory anteriorly, but posteriorly it veers from the edge of the striola to reach the posterior margin of the macula. Consequently, more utricular bundles are oriented mediolaterally than previously supposed. Three hair cell classes are distinguished in calretinin-stained material: type II hair cells, type ID hair cells contacting calretinin-negative (dimorphic) afferents, and type IC hair cells contacting calretinin-positive (calyceal) afferents. They differ significantly on most bundle measures. Type II bundles have short stereocilia. Type IC bundles have kinocilia and stereocilia of similar heights, i.e., KS ratios (ratio of kinocilium to stereocilia heights) ∼1, unlike other receptor classes. In contrast to these class-specific differences, bundles show little regional variation except that KS ratios are lowest in the striola. These low KS ratios suggest that bundle stiffness is greater in the striola than in the extrastriola.

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Autocorrelation Analysis of Hair Bundle Structure in the Utricle

Journal of Neurophysiology ◽

10.1152/jn.00565.2006 ◽

2006 ◽

Vol 96 (5) ◽

pp. 2653-2669 ◽

Cited By ~ 18

Author(s):

M. H. Rowe ◽

E. H. Peterson

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Cell Types ◽

Head Movements ◽

Type I ◽

Autocorrelation Analysis ◽

Response Dynamics ◽

Hair Bundles ◽

Vestibular Organs ◽

Bundle Structure

The ability of hair bundles to signal head movements and sounds depends significantly on their structure, but a quantitative picture of bundle structure has proved elusive. The problem is acute for vestibular organs because their hair bundles exhibit complex morphologies that vary with endorgan, hair cell type, and epithelial locus. Here we use autocorrelation analysis to quantify stereociliary arrays (the number, spacing, and distribution of stereocilia) on hair cells of the turtle utricle. Our first goal was to characterize zonal variation across the macula, from medial extrastriola, through striola, to lateral extrastriola. This is important because it may help explain zonal variation in response dynamics of utricular hair cells and afferents. We also use known differences in type I and II bundles to estimate array characteristics of these two hair cell types. Our second goal was to quantify variation in array orientation at single macular loci and use this to estimate directional tuning in utricular afferents. Our major findings are that, of the features measured, array width is the most distinctive feature of striolar bundles, and within the striola there are significant, negatively correlated gradients in stereocilia number and spacing that parallel gradients in bundle heights. Together with previous results on stereocilia number and bundle heights, our results support the hypothesis that striolar hair cells are specialized to signal high-frequency/acceleration head movements. Finally, there is substantial variation in bundle orientation at single macular loci that may help explain why utricular afferents respond to stimuli orthogonal to their preferred directions.

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Molecular characterization of an inward rectifier channel (IKir) found in avian vestibular hair cells: cloning and expression of pKir2.1

Physiological Genomics ◽

10.1152/physiolgenomics.00096.2004 ◽

2004 ◽

Vol 19 (2) ◽

pp. 155-169 ◽

Cited By ~ 11

Author(s):

Manning J. Correia ◽

Thomas G. Wood ◽

Deborah Prusak ◽

Tianxiang Weng ◽

Katherine J. Rennie ◽

...

Keyword(s):

Hair Cells ◽

Cho Cells ◽

Dwell Time ◽

Single Channel ◽

Cloning And Expression ◽

Single Type ◽

Type I ◽

Type Ii ◽

Vestibular Hair Cells ◽

Inwardly Rectifying

A fast inwardly rectifying current has been observed in some of the sensory cells (hair cells) of the inner ear of several species. While the current was presumed to be an IKir current, contradictory evidence existed as to whether the cloned channel actually belonged to the Kir2.0 subfamily of potassium inward rectifiers. In this paper, we report for the first time converging evidence from electrophysiological, biochemical, immunohistochemical, and genetic studies that show that the Kir2.1 channel carries the fast inwardly rectifying currents found in pigeon vestibular hair cells. Following cytoplasm extraction from single type II and multiple pigeon vestibular hair cells, mRNA was reverse transcribed, amplified, and sequenced. The open reading frame (ORF), consisting of a 1,284-bp nucleotide sequence, showed 94, 85, and 83% identity with Kir2.1 subunit sequences from chick lens, Kir2 sequences from human heart, and a mouse macrophage cell line, respectively. Phylogenetic analyses revealed that pKir2.1 formed an immediate node with hKir2.1 but not with hKir2.2–2.4. Hair cells (type I and type II) and supporting cells in the sensory epithelium reacted positively with a Kir2.1 antibody. The whole cell current recorded in oocytes and CHO cells, transfected with pigeon hair cell Kir2.1 (pKir2.1), demonstrated blockage by Ba2+ and sensitivity to changing K+ concentration. The mean single-channel linear slope conductance in transfected CHO cells was 29 pS. The open dwell time was long (∼300 ms at −100 mV), and the closed dwell time was short (∼34 ms at −100 mV). Multistates ranging from 3–6 were noted in some single-channel responses. All of the above features have been described for other Kir2.1 channels. Current clamp studies of native pigeon vestibular hair cells illustrated possible physiological roles of the channel and showed that blockage of the channel by Ba2+ depolarized the resting membrane potential by ∼30 mV. Negative currents hyperpolarized the membrane ∼20 mV before block but ∼60 mV following block. RT-PCR studies revealed that the pKir2.1 channels found in pigeon vestibular hair cells were also present in pigeon vestibular nerve, vestibular ganglion, lens, neck muscle, brain (brain stem, cerebellum and optic tectum), liver, and heart.

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Effects of KCNQ channel blockers on K+ currents in vestibular hair cells

AJP Cell Physiology ◽

10.1152/ajpcell.2001.280.3.c473 ◽

2001 ◽

Vol 280 (3) ◽

pp. C473-C480 ◽

Cited By ~ 29

Author(s):

Katherine J. Rennie ◽

Tianxiang Weng ◽

Manning J. Correia

Keyword(s):

Steady State ◽

Hair Cells ◽

Low Voltage ◽

Dissociation Constants ◽

Channel Blockers ◽

Type I ◽

Type Ii ◽

Kcnq Channels ◽

Vestibular Hair Cells ◽

Inward Currents

Linopirdine and XE991, selective blockers of K+ channels belonging to the KCNQ family, were applied to hair cells isolated from gerbil vestibular system and to hair cells in slices of pigeon crista. In type II hair cells, both compounds inhibited a slowly activating, slowly inactivating component of the macroscopic current recruited at potentials above −60 mV. The dissociation constants for linopirdine and XE991 block were <5 μM. A similar component of the current was also blocked by 50 μM capsaicin in gerbil type II hair cells. All three drugs blocked a current component that showed steady-state inactivation and a biexponential inactivation with time constants of ∼300 ms and 4 s. Linopirdine (10 μM) reduced inward currents through the low-voltage-activated K+ current in type I hair cells, but concentrations up to 200 μM had little effect on steady-state outward K+ current in these cells. These results suggest that KCNQ channels may be present in amniote vestibular hair cells.

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Recovery of the Vestibulocolic Reflex After Aminoglycoside Ototoxicity in Domestic Chickens

Journal of Neurophysiology ◽

10.1152/jn.1999.81.3.1025 ◽

1999 ◽

Vol 81 (3) ◽

pp. 1025-1035 ◽

Cited By ~ 15

Author(s):

Christopher T. Goode ◽

John P. Carey ◽

Albert F. Fuchs ◽

Edwin W Rubel

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Afferent Input ◽

Open Loop ◽

Cell Regeneration ◽

Type I ◽

Neural Pathways ◽

Hair Cell Regeneration ◽

Vestibular Hair Cells ◽

Aminoglycoside Ototoxicity

Recovery of the vestibulocolic reflex after aminoglycoside ototoxicity in domestic chickens. Avian auditory and vestibular hair cells regenerate after damage by ototoxic drugs, but until recently there was little evidence that regenerated vestibular hair cells function normally. In an earlier study we showed that the vestibuloocular reflex (VOR) is eliminated with aminoglycoside antibiotic treatment and recovers as hair cells regenerate. The VOR, which stabilizes the eye in the head, is an open-loop system that is thought to depend largely on regularly firing afferents. Recovery of the VOR is highly correlated with the regeneration of type I hair cells. In contrast, the vestibulocolic reflex (VCR), which stabilizes the head in space, is a closed-loop, negative-feedback system that seems to depend more on irregularly firing afferent input and is thought to be subserved by different circuitry than the VOR. We examined whether this different reflex also of vestibular origin would show similar recovery after hair cell regeneration. Lesions of the vestibular hair cells of 10-day-old chicks were created by a 5-day course of streptomycin sulfate. One day after completion of streptomycin treatment there was no measurable VCR gain, and total hair cell density was ∼35% of that in untreated, age-matched controls. At 2 wk postlesion there was significant recovery of the VCR; at this time two subjects showed VCR gains within the range of control chicks. At 3 wk postlesion all subjects showed VCR gains and phase shifts within the normal range. These data show that the VCR recovers before the VOR. Unlike VOR gain, recovering VCR gain correlates equally well with the density of regenerating type I and type II vestibular hair cells, except at high frequencies. Several factors other than hair cell regeneration, such as length of stereocilia, reafferentation of hair cells, and compensation involving central neural pathways, may be involved in behavioral recovery. Our data suggest that one or more of these factors differentially affect the recovery of these two vestibular reflexes.

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Temporal Bone Studies of the Human Peripheral Vestibular System

Annals of Otology Rhinology & Laryngology ◽

10.1177/00034894001090s502 ◽

2000 ◽

Vol 109 (5_suppl) ◽

pp. 3-13 ◽

Cited By ~ 110

Author(s):

Saumil N. Merchant ◽

Kojiro Tsuji ◽

Conrad Wall ◽

Luis Velázquez-Villaseñor ◽

Robert J. Glynn ◽

...

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Type I ◽

Type Ii ◽

Sense Organs ◽

Age Related ◽

The Mean ◽

Cell Densities ◽

Temporal Bones ◽

Total Type

Quantitative studies of the vestibular system with serially sectioned human temporal bones have been limited because of difficulty in distinguishing hair cells from supporting cells and type I from type II hair cells. In addition, there is only a limited amount of normative data available regarding vestibular hair cell counts in humans. In this study, archival temporal bone sections were examined by Nomarski (differential interference contrast) microscopy, which permitted visualization of the cuticular plate and stereociliary bundle so as to allow unambiguous identification of hair cells. The density of type I, type II, and total numbers of vestibular hair cells in each of the 5 sense organs was determined in a set of 67 normal temporal bones that ranged from birth through 100 years of age. The mean total densities at birth were 76 to 79 cells per 0.01 mm2 in the cristae, 68 cells per 0.01 mm2 in the utricle, and 61 cells per 0.01 mm2 in the saccule. The ratio of type I to type II hair cells at birth was 2.4:1 in the cristae and 1.3:1 in the maculae. There was a highly significant age-related decline in all sense organs for total, type I, and type II hair cell densities that was best fit by a linear regression model. The cristae lost type I cells with advancing age at a significantly greater rate than the maculae, whereas age-related losses for type II cells occurred at the same rate for all 5 sense organs. Hair cell densities in the cristae were significantly higher at the periphery than at the center. There were no significant sex or interaural differences for any of the counts. Mathematical models were developed to calculate the mean and 95% prediction intervals for the total, type I, and type II hair cell densities in each sense organ on the basis of age. There was overall good agreement between the hair cell densities determined in this study and those reported by others using surface preparation techniques. Our data and related models will serve as a normative database that will be useful for comparison to counts made from subjects with known vestibular disorders.

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Unmyelinated type II afferent neurons report cochlear damage

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1515228112 ◽

2015 ◽

Vol 112 (47) ◽

pp. 14723-14727 ◽

Cited By ~ 54

Author(s):

Chang Liu ◽

Elisabeth Glowatzki ◽

Paul Albert Fuchs

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Outer Hair Cell ◽

Cell Damage ◽

Large Diameter ◽

Outer Hair Cells ◽

Type I ◽

Type Ii ◽

Inner Hair Cell ◽

Hair Cell Damage

In the mammalian cochlea, acoustic information is carried to the brain by the predominant (95%) large-diameter, myelinated type I afferents, each of which is postsynaptic to a single inner hair cell. The remaining thin, unmyelinated type II afferents extend hundreds of microns along the cochlear duct to contact many outer hair cells. Despite this extensive arbor, type II afferents are weakly activated by outer hair cell transmitter release and are insensitive to sound. Intriguingly, type II afferents remain intact in damaged regions of the cochlea. Here, we show that type II afferents are activated when outer hair cells are damaged. This response depends on both ionotropic (P2X) and metabotropic (P2Y) purinergic receptors, binding ATP released from nearby supporting cells in response to hair cell damage. Selective activation of P2Y receptors increased type II afferent excitability by the closure of KCNQ-type potassium channels, a potential mechanism for the painful hypersensitivity (that we term “noxacusis” to distinguish from hyperacusis without pain) that can accompany hearing loss. Exposure to the KCNQ channel activator retigabine suppressed the type II fiber’s response to hair cell damage. Type II afferents may be the cochlea’s nociceptors, prompting avoidance of further damage to the irreparable inner ear.

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Evidence for an Na+-K+-Cl−cotransporter in mammalian type I vestibular hair cells

AJP Cell Physiology ◽

10.1152/ajpcell.1997.273.6.c1972 ◽

1997 ◽

Vol 273 (6) ◽

pp. C1972-C1980 ◽

Cited By ~ 16

Author(s):

K. J. Rennie ◽

J. F. Ashmore ◽

M. J. Correia

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Cell Swelling ◽

Type I ◽

Vestibular Hair Cells ◽

Type I Cells ◽

High K ◽

I Cells ◽

Shape Changes ◽

External K

In amniotes, there are two types of hair cells, designated I and II, that differ in their morphology, innervation pattern, and ionic membrane properties. Type I cells are unique among hair cells in that their basolateral surfaces are almost completely enclosed by an afferent calyceal nerve terminal. Recently, several lines of evidence have ascribed a motile function to type I hair cells. To investigate this, elevated external K+, which had been used previously to induce hair cell shortening, was used to induce shape changes in dissociated mammalian type I vestibular hair cells. Morphologically identified type I cells shortened and widened when the external K+ concentration was raised isotonically from 2 to 125 mM. The shortening did not require external Ca2+ but was abolished when external Cl− was replaced with gluconate or sulfate and when external Na+ was replaced with N-methyl-d-glucamine. Bumetanide (10–100 μM), a specific blocker of the Na+-K+-Cl− cotransporter, significantly reduced K+-induced shortening. Hyposmotic solution resulted in type I cell shape changes similar to those seen with high K+, i.e., shortening and widening. Type I cells became more spherical in hyposmotic solution, presumably as a result of a volume increase due to water influx. In hypertonic solution, cells became narrower and increased in length. These results suggest that shape changes in type I hair cells induced by high K+ are due, at least in part, to ion and solute entry via an Na+-K+-Cl− cotransporter, which results in cell swelling. A scheme is proposed whereby the type I hair cell depolarizes and K+ leaves the cell via voltage-dependent K+channels and accumulates in the synaptic space between the type I hair cell and calyx. Excess K+ could then be removed from the intercellular space by uptake via the cotransporter.

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