Na+ Currents in Vestibular Type I and Type II Hair Cells of  the Embryo and Adult Chicken

In birds, type I and type II hair cells differentiate before birth. Here we describe that chick hair cells, from the semicircular canals, begin expressing a voltage-dependent Na current ( INa) from embryonic day 14 (E14) and continue to express the current up to hatching (E21). During this period, INa was present in most (31/43) type I hair cells irrespective of their position in the crista, in most type II hair cells located far from the planum semilunatum (48/63), but only occasionally in type II hair cells close to the planum semilunatum (2/35). INa activated close to –60 mV, showed fast time- and voltage-dependent activation and inactivation, and was completely, and reversibly, blocked by submicromolar concentrations of tetrodotoxin ( Kd = 17 nM). One peculiar property of INa concerns its steady-state inactivation, which is complete at –60 mV (half-inactivating voltage = –96 mV). INa was found in type I and type II hair cells from the adult chicken as well, where it had similar, although possibly not identical, properties and regional distribution. Current-clamp experiments showed that INa could contribute to the voltage response provided that the cell membrane was depolarized from holding potentials more negative than –80 mV. When recruited, INa produced a significant acceleration of the cell membrane depolarization, which occasionally elicited a large rapid depolarization followed by a rapid repolarization (action-potential-like response). Possible physiological roles for INa in the embryo and adult chicken are discussed.

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Current Response in CaV1.3–/– Mouse Vestibular and Cochlear Hair Cells

Frontiers in Neuroscience ◽

10.3389/fnins.2021.749483 ◽

2021 ◽

Vol 15 ◽

Author(s):

Marco Manca ◽

Piece Yen ◽

Paolo Spaiardi ◽

Giancarlo Russo ◽

Roberta Giunta ◽

...

Keyword(s):

Hair Cells ◽

Signal Transmission ◽

Basolateral Membrane ◽

Semicircular Canals ◽

Type I ◽

Current Response ◽

Type Ii ◽

Current Profile ◽

Cochlear Hair Cells ◽

Vestibular Hair Cells

Signal transmission by sensory auditory and vestibular hair cells relies upon Ca2+-dependent exocytosis of glutamate. The Ca2+ current in mammalian inner ear hair cells is predominantly carried through CaV1.3 voltage-gated Ca2+ channels. Despite this, CaV1.3 deficient mice (CaV1.3–/–) are deaf but do not show any obvious vestibular phenotype. Here, we compared the Ca2+ current (ICa) in auditory and vestibular hair cells from wild-type and CaV1.3–/– mice, to assess whether differences in the size of the residual ICa could explain, at least in part, the two phenotypes. Using 5 mM extracellular Ca2+ and near-body temperature conditions, we investigated the cochlear primary sensory receptors inner hair cells (IHCs) and both type I and type II hair cells of the semicircular canals. We found that the residual ICa in both auditory and vestibular hair cells from CaV1.3–/– mice was less than 20% (12–19%, depending on the hair cell type and age investigated) compared to controls, indicating a comparable expression of CaV1.3 Ca2+ channels in both sensory organs. We also showed that, different from IHCs, type I and type II hair cells from CaV1.3–/– mice were able to acquire the adult-like K+ current profile in their basolateral membrane. Intercellular K+ accumulation was still present in CaV1.3–/– mice during IK,L activation, suggesting that the K+-based, non-exocytotic, afferent transmission is still functional in these mice. This non-vesicular mechanism might contribute to the apparent normal vestibular functions in CaV1.3–/– mice.

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Vestibular Type I and Type II Hair Cells. 2: Morphometric Comparisons of Dissociated Pigeon Hair Cells

Journal of Vestibular Research ◽

10.3233/ves-1997-7504 ◽

1997 ◽

Vol 7 (5) ◽

pp. 407-420

Author(s):

Anthony J. Ricci ◽

Stephen L. Cochran ◽

Katherine J. Rennie ◽

Manning J. Correia

Keyword(s):

Hair Cells ◽

Semicircular Canals ◽

Columba Livia ◽

Hair Bundle ◽

Type I ◽

Type Ii ◽

Cell Groups ◽

Hair Bundles

Morphometric properties of solitary hair cells dissociated from the semicircular canals (SCC), utricles (UTR), and lagenas (LAG) of adult white king pigeons, Columba livia, were compared. Measurements were made of the cell body, cuticular plate and hair bundle. Cells were divided into two groups: type 1 (group 1) was predominantly type I hair cells, and type 2 (group 3) was primarily type II hair cells. Comparisons are made initially between end organs for each group. A subpopulation of short otolith hair cells was identified. Quantitative comparisons between isolated type 1 and type 2 hair cells demonstrated that type 1 hair cells were more homogeneous both within and between vestibular end organs; while they had shorter, thinner neck regions, narrower apical surfaces, with longer and thinner bodies than did type 2 hair cells. Generally, for both type 1 and type 2 hair cells, two different hair bundle shapes were present, those (unimodal) with a single sharp taper from longest to shortest stereocilia, and those (bimodal) with an initial steep tape-followed by a less steep taper. An additional subtype of type 1 hair cells with short hair bundles was identified. SCC hair cells have fewer hair bundles with bimodal tapers across all cell groups when compared to UTR or LAG. All cell subtypes identified for dissociated hair cells were corroborated using histologic sections.

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Ionic currents and current-clamp depolarisations of type I and type II hair cells from the developing rat utricle

Pflügers Archiv - European Journal of Physiology ◽

10.1007/s004240050877 ◽

1999 ◽

Vol 438 (1) ◽

pp. 40-46 ◽

Cited By ~ 26

Author(s):

G. W. T. Lennan ◽

A. Steinacker ◽

J. Lehouelleur ◽

A. Sans

Keyword(s):

Hair Cells ◽

Ionic Currents ◽

Type I ◽

Type Ii ◽

Current Clamp ◽

Developing Rat

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A delayed rectifier conductance in type I hair cells of the mouse utricle

Journal of Neurophysiology ◽

10.1152/jn.1996.76.2.995 ◽

1996 ◽

Vol 76 (2) ◽

pp. 995-1004 ◽

Cited By ~ 90

Author(s):

A. Rusch ◽

R. A. Eatock

Keyword(s):

Hair Cells ◽

Time Course ◽

Dissociation Constants ◽

Resting Potential ◽

Delayed Rectifier ◽

Type I ◽

Type Ii ◽

Voltage Range ◽

Average Maximum

1. Membrane currents of hair cells in acutely excised or cultured mouse utricles were recorded with the whole cell voltage-clamp method at temperatures between 23 and 36 degrees C. 2. Type I and II hair cells both had delayed rectifier conductances that activated positive to -55 mV. 3. Type I, but not type II, hair cells had an additional delayed rectifier conductance (gK,L) with an activation range that was unusually negative and variable. At 23-25 degrees C, V(1/2) values ranged from -88 to -62 mV in 57 cells. 4. gK,L was very large. At 23-25 degrees C, the average maximum chord conductance was 75 +/- 65 nS (mean +/- SD, n = 57; measured at -54 mV), or approximately 21 nS/pF of cell capacitance. 5. gK,L was highly selective for K+ over Na+ (permeability ratio PNa+/PK+:0.006), but unlike other delayed rectifiers, gK,L was significantly permeable to Cs+ (PCs+/PK+:0.31). gK,L was independent of extracellular Ca2+. 6. At -64 mV, Ba2+ and 4-aminopyridine blocked gK,L with apparent dissociation constants of 2.0 mM and 43 microM, respectively. Extracellular Cs+ (5 mM) blocked gK,L by 50% at -124 mV. Apamin (100 nM) and dendrotoxin (10 nM) has no effect. 7. The kinetic data of gK,L are consistent with a sequential gating model with at least two closed states and one open state. The slow activation kinetics (principal time constants at 23-25 degrees C:600-200 ms) had a thermal Q10 of 2.1. Inactivation (Q10:2.7) was partial at all temperatures. Deactivation followed a double-exponential time course and had a Q10 of 2.0. 8. At 23-25 degrees C, gK,L was appreciably activated at the mean resting potential of type I hair cells (-77 +/- 3.1 mV, n = 62), so that input conductances were often more than an order of magnitude larger than those of type II cells. If these conditions hold in vivo, type I cells would produce unusually small receptor potentials. Warming the cells to 36 degrees C produced parallel shifts in gK,L's activation range (0.8 +/- 0.3 mV/degrees C, n = 8), and in the resting potential (0.6 +/- 0.3 mV/degrees C, n = 4). Thus the high input conductances were not an artifact of unphysiological temperatures but remained high near body temperature. It remains possible that in vivo gK,L's activation range is less negative and input conductances are lower; the large variance in the voltage range of activation suggests that it may be subject to modulation.

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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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Axodendritic versus axosomatic cochlear efferent termination is determined by afferent type in a hierarchical logic of circuit formation

Science Advances ◽

10.1126/sciadv.abd8637 ◽

2021 ◽

Vol 7 (4) ◽

pp. eabd8637

Author(s):

Jemma L. Webber ◽

John C. Clancy ◽

Yingjie Zhou ◽

Natalia Yraola ◽

Kazuaki Homma ◽

...

Keyword(s):

Hair Cells ◽

Fiber Type ◽

Afferent Fiber ◽

Outer Hair Cells ◽

Type I ◽

Type Ii ◽

Efferent Neurons ◽

Distinct Pair ◽

Mechanosensory Hair Cells ◽

Circuit Formation

Hearing involves a stereotyped neural network communicating cochlea and brain. How this sensorineural circuit assembles is largely unknown. The cochlea houses two types of mechanosensory hair cells differing in function (sound transmission versus amplification) and location (inner versus outer compartments). Inner (IHCs) and outer hair cells (OHCs) are each innervated by a distinct pair of afferent and efferent neurons: IHCs are contacted by type I afferents receiving axodendritic efferent contacts; OHCs are contacted by type II afferents and axosomatically terminating efferents. Using an Insm1 mouse mutant with IHCs in the position of OHCs, we discover a hierarchical sequence of instructions in which first IHCs attract, and OHCs repel, type I afferents; second, type II afferents innervate hair cells not contacted by type I afferents; and last, afferent fiber type determines if and how efferents innervate, whether axodendritically on the afferent, axosomatically on the hair cell, or not at all.

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Quantal and Nonquantal Transmission in Calyx-Bearing Fibers of the Turtle Posterior Crista

Journal of Neurophysiology ◽

10.1152/jn.00332.2007 ◽

2007 ◽

Vol 98 (3) ◽

pp. 1083-1101 ◽

Cited By ~ 40

Author(s):

Joseph C. Holt ◽

Shilpa Chatlani ◽

Anna Lysakowski ◽

Jay M. Goldberg

Keyword(s):

Ampa Receptor ◽

Hair Cells ◽

Ultrastructural Study ◽

Nerve Fibers ◽

Type I ◽

Outer Face ◽

Type Ii ◽

Intracellular Recordings ◽

External Concentration ◽

Voltage Gated

Intracellular recordings were made from nerve fibers in the posterior ampullary nerve near the neuroepithelium. Calyx-bearing afferents were identified by their distinctive efferent-mediated responses. Such fibers receive inputs from both type I and type II hair cells. Type II inputs are made by synapses on the outer face of the calyx ending and on the boutons of dimorphic fibers. Quantal activity, consisting of brief mEPSPs, is reduced by lowering the external concentration of Ca2+ and blocked by the AMPA-receptor antagonist CNQX. Poisson statistics govern the timing of mEPSPs, which occur at high rates (250–2,500/s) in the absence of mechanical stimulation. Excitation produced by canal-duct indentation can increase mEPSP rates to nearly 5,000/s. As the rate increases, mEPSPs can change from a monophasic depolarization to a biphasic depolarizing–hyperpolarizing sequence, both of whose components are blocked by CNQX. Blockers of voltage-gated currents affect mEPSP size, which is decreased by TTX and is increased by linopirdine. mEPSP size decreases severalfold after impalement. The size decrease, although it may be triggered by the depolarization occurring during impalement, persists even at hyperpolarized membrane potentials. Nonquantal transmission is indicated by shot-noise calculations and by the presence of voltage modulations after quantal activity is abolished pharmacologically. An ultrastructural study shows that inner-face inputs from type I hair cells outnumber outer-face inputs from type II hair cells by an almost 6:1 ratio.

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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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Efferent Synaptic Transmission at the Vestibular Type II Hair Cell Synapse

10.1101/2020.03.14.992180 ◽

2020 ◽

Author(s):

Zhou Yu ◽

J. Michael McIntosh ◽

Soroush Sadeghi ◽

Elisabeth Glowatzki

Keyword(s):

Hair Cells ◽

Nerve Fibers ◽

Repetitive Stimulation ◽

Vestibular Nerve ◽

Type I ◽

Type Ii ◽

Optogenetic Stimulation ◽

Vestibular Afferents ◽

Stimulation Of

ABSTRACTIn the vestibular peripheral organs, type I and type II hair cells (HCs) transmit incoming signals via glutamatergic quantal transmission onto afferent nerve fibers. Additionally, type I HCs transmit via ‘non-quantal’ transmission to calyx afferent fibers, by accumulation of glutamate and potassium in the synaptic cleft. Vestibular efferent inputs originating in the brainstem contact type II HCs and vestibular afferents. Here, we aimed at characterizing the synaptic efferent inputs to type II HCs using electrical and optogenetic stimulation of efferent fibers combined with in vitro whole-cell patch clamp recording from type II HCs in the rodent vestibular crista. Properties of efferent synaptic currents in type II HCs were similar to those found in cochlear hair cells and mediated by activation of α9/α10 nicotinic acetylcholine receptors (AChRs) and SK potassium channels. While efferents showed a low probability of release at low frequencies of stimulation, repetitive stimulation resulted in facilitation and increased probability of release. Notably, the membrane potential of type II HCs measured during optogenetic stimulation of efferents showed a strong hyperpolarization even in response to single pulses and was further enhanced by repetitive stimulation. Such efferent-mediated inhibition of type II HCs can provide a mechanism to adjust the contribution of signals from type I and type II HCs to vestibular nerve fibers. As a result, the relative input of type I hair cells to vestibular afferents will be strengthened, emphasizing the phasic properties of the incoming signal that are transmitted via fast non-quantal transmission.New and NoteworthyType II vestibular hair cells (HCs) receive inputs from efferent fibers originating in the brainstem. We used in vitro optogenetic and electrical stimulation of efferent fibers to study their synaptic inputs to type II HCs. Efferent inputs inhibited type II HCs, similar to cochlear efferent effects. We propose that efferent inputs adjust the contribution of signals from type I and type II HCs that report different components of the incoming signal to vestibular nerve fibers.

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Membrane Properties of Chick Semicircular Canal Hair Cells In Situ During Embryonic Development

Journal of Neurophysiology ◽

10.1152/jn.2000.83.5.2740 ◽

2000 ◽

Vol 83 (5) ◽

pp. 2740-2756 ◽

Cited By ~ 31

Author(s):

S. Masetto ◽

P. Perin ◽

A. Malusà ◽

G. Zucca ◽

P. Valli

Keyword(s):

Hair Cell ◽

Hair Cells ◽

Central Zone ◽

Cell Voltage ◽

Peripheral Zone ◽

Membrane Properties ◽

Voltage Response ◽

Type I ◽

Electrophysiological Properties ◽

Different Types

The electrophysiological properties of developing vestibular hair cells have been investigated in a chick crista slice preparation, from embryonic day 10 ( E10) to E21 (when hatching would occur). Patch-clamp whole-cell experiments showed that different types of ion channels are sequentially expressed during development. An inward Ca2+ current and a slow outward rectifying K+current ( I K(V)) are acquired first, at or before E10, followed by a rapid transient K+current ( I K(A)) at E12, and by a small Ca-dependent K+ current ( I KCa) at E14. Hair cell maturation then proceeds with the expression of hyperpolarization-activated currents: a slow I h appears first, around E16, followed by the fast inward rectifier I K1around E19. From the time of its first appearance, I K(A) is preferentially expressed in peripheral ( zone 1) hair cells, whereas inward rectifying currents are preferentially expressed in intermediate ( zone 2) and central ( zone 3) hair cells. Each conductance conferred distinctive properties on hair cell voltage response. Starting from E15, some hair cells, preferentially located at the intermediate region, showed the amphora shape typical of type I hair cells. From E17 (a time when the afferent calyx is completed) these cells expressed I K, L, the signature current of mature type I hair cells. Close to hatching, hair cell complements and regional organization of ion currents appeared similar to those reported for the mature avian crista. By the progressive acquisition of different types of inward and outward rectifying currents, hair cell repolarization after both positive- and negative-current injections is greatly strengthened and speeded up.

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