Differentiation of Mammalian Vestibular Hair Cells from Conditionally Immortal, Postnatal Supporting Cells

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The Journal of Neuroscience, November 1, 1999, 19(21):9445-9458

Differentiation of Mammalian Vestibular Hair Cells from Conditionally Immortal, Postnatal Supporting Cells
Patrick Lawlor, Walter Marcotti, Marcelo N. Rivolta, Corné J. Kros, and Matthew C. Holley
Department of Physiology, School of Medical Sciences, University of Bristol, Bristol, BS8 1TD, United Kingdom

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We provide evidence from a newly established, conditionally immortal cell line (UB/UE-1) that vestibular supporting cellsfrom the mammalian inner ear can differentiate postnatally intomore than one variant of hair cell. A clonal supporting cell linewas established from pure utricular sensory epithelia of H2k^btsA58 transgenic mice 2 d after birth. Cell proliferation wasdependent on conditional expression of the immortalizing gene,the "T" antigen from the SV40 virus. Proliferating cells expressedcytokeratins, and patch-clamp recordings revealed that they allexpressed small membrane currents with little time-dependence.They stopped dividing within 2 d of being transferred to differentiatingconditions, and within a week they formed three defined populationsexpressing membrane currents characteristic of supporting cellsand two kinds of neonatal hair cell. The cells expressed severalcharacteristic features of normal hair cells, including the transcriptionfactor Brn3.1, a functional acetylcholine receptor composed of $alpha$ 9 subunits, and the cytoskeletal proteins myosin VI, myosin VIIa,and fimbrin. Immunofluorescence labeling and electron microscopyshowed that the cells formed complex cytoskeletal arrays on theirupper surfaces with structural features resembling those at theapices of normal hair cells. The cell line UB/UE-1 provides avaluable in vitro preparation in which the expression of numerousstructural and physiological components can be initiated or upregulatedduring early stages of mammalian hair cell commitment anddifferentiation.

Key words: mouse; vestibular; utricle; hair cells; epithelial cells; conditional immortalization; tsA58; differentiation; development; potassium current; inward rectifier

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Most mechanosensory epithelia are composed of sensory hair cells surrounded by nonsensory supporting cells. Hair cells canbe replaced in many vertebrate epithelia, including those fromfish (Presson and Popper, 1990; Presson, 1994), amphibia (Bairdet al., 1996), and birds (Corwin and Cotanche, 1988; Ryals andRubel, 1988) (for review, see Cotanche et al., 1994; Stone etal., 1998). There is little evidence that mammalian auditory haircells can be replaced after birth (Kelley et al., 1993, 1995;Lefebvre et al., 1993; Chardin and Romand, 1995; Forge et al.,1998) but convincing evidence for a low level of hair cell replacementin mammalian vestibular organs (Forge et al., 1993; Warchol etal., 1993). Cell lineage studies in the chick show that hair cellsand supporting cells share a common precursor (Fekete et al.,1998), and selective ablation of hair cells in fish lateral linereveals that supporting cells can replace hair cells during sensoryregeneration (Jones and Corwin, 1996).

The mammalian inner ear possesses just a few thousand sensory cells that are encased in several layers of bone and show littleproliferative activity in vitro. Thus there has been some effortto establish mammalian cell lines that will enable more controlledstudies of the mechanisms of cell differentiation and regeneration(Barald et al., 1997; Holley et al., 1997; Rivolta et al., 1998;Zheng et al., 1998). The utricular macula provides a good modelfor mammalian mechanosensory epithelia because it retains theability to replace hair cells postnatally. It is also convenientlycomposed of a simple layer of hair cells and supporting cellsthat can be separated enzymatically from the underlying connectivetissue (Saffer et al., 1996).

Our hypothesis was that mammalian neonatal utricular supporting cells retain the potential to differentiate into hair cells.To establish conditionally immortal cells as close as possibleto the developmental stage at dissection, we used the H2k^btsA58 transgenic mouse (Immortomouse) as a source of differentiatingcells (Jat et al., 1991; Rivolta et al., 1998). During early stagesof development, utricular epithelial cells normally express cytokeratinsand vimentin (Kuijpers et al., 1992). In differentiated hair cells,both proteins are expressed at lower levels, with cytokeratinalmost absent, but in supporting cells cytokeratin expressionremains high. Specific markers for hair cells include the transcriptionfactor Brn3.1 (Erkman et al., 1996; Xiang et al., 1997), the $alpha$ 9subunit of the acetylcholine receptor (Elgoyhen et al., 1994;Glowatzki et al., 1995), an isoform of the cytoskeletal proteinfimbrin (Lee and Cotanche, 1996; Slepecky, 1996), and the motorproteins myosin VI and VIIa (Hasson et al., 1997). Supportingcells express relatively small basolateral membrane currents (Sugiharaand Furukawa, 1996; Masetto and Correia, 1997), whereas differenttypes of hair cell express large characteristic outward and/orinward rectifier currents (Rüsch et al., 1998). We selected immortalcell lines expressing cytokeratins to confirm their identity assupporting cells and then assessed them under differentiatingconditions using both structural and physiological markers forthe different celltypes.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Isolation and culture of cell lines. Four epithelial sheets from the utricular maculae were dissected from the ears of Immortomousepups at postnatal day 2 (P2). After the nonsensory epitheliumand the outer margins of the sensory epithelium were trimmed away,the sheets were incubated in Minimal Essential Medium with Earle'ssalts and Glutamax I (MEM; Life Technologies, Paisley, Scotland)containing 500 µg/ml thermolysin (Protease type X, Sigma, Poole,England) (Saffer et al., 1996) for 5 min at 37°C. They were thenpeeled from the underlying connective tissue and transferred tofresh MEM with 10% horse serum (MEM/HS; Life Technologies) and20 U/ml dispase (Life Technologies). After 15 min at 37°C, theywere rinsed with fresh medium, dissociated by trituration, andplated in 35-mm-diameter dishes (Falcon range, Becton Dickinson,Oxford, England) precoated with fibronectin (1 µg/cm²; Life Technologies) in a small volume of MEM/HS and 100 U/ml $gamma$ -interferon (MEM/HS/ $gamma$ IFN) at 33°C .

At confluence, cells were dissociated using trypsin (0.25%, Sigma) and replated in MEM/HS/ $gamma$ IFN onto fibronectin-coated wells.They were passaged an additional two times using trypsin untilconfluent in 25 cm² flasks. When cells were seeded onto uncoated tissue culture plasticin horse serum, they did not adhere well to the culture surface,so from passage 3 onward they were cultured in 10% fetal calfserum (FCS, Life Technologies). Passage 3 cells were cloned byseeding trypsin-dissociated cells at 1 cell per well in 96-wellplates in MEM/FCS/ $gamma$ IFN. Clones were selected only from wells containingone colony. When individual clones reached confluence they werepassaged using trypsin into larger vessels. Established cloneswere then cultured at 33°C in MEM + 10% FCS, and the $gamma$ IFN wasreduced to 50 U/ml. Cells were fed every 4-5 d with fresh mediumand passaged approximately once perweek.

To culture cells under differentiating conditions, trypsinized cells were replated in MEM/FCS without $gamma$ IFN at 39°C. Cultureswere fed every 7 d with freshmedium.

To measure cell proliferation, cells were seeded at 1.5 × 10⁵ cells per dish in 35-mm-diameter tissue culture plastic dishesat 39° and 33°C. At set times, they were trypsinized off the dishand counted using ahemocytometer.

PCR. Total RNA was extracted from cells at 33° and 39°C. Primers used for the detection of the different transcripts correspondedto mouse sequences, with the exception of $alpha$ 9, which was from rat.Primers were as follows: GAPDH, positions 248 (5'-AACGGGAAGCCCATCACC-3')and 672 (5'-CAGCCTTGGCAGCACCAG-3'); $alpha$ 9, positions 754 (5'-CCTTACCCAGATGTCACCTTCACTC-3')and 1466 (5'-AACACCATAGCAAAGAAAATCCACA-3'); Brn3.1, positions205 (5'-CCATGCGCCGAGTTTGTCTCC-3') and 639 (5'-CTCCACATCGCTGAGACACGC3'); myosin VI, position 2343 (5'ACTTCCAAGATTGGATCCGAGGT-3') and3576 (5'-GTCGTTTCATGTCAATCTCCTGC-3'); and myosin VIIa, positions468 (5'-GCTGTATTATCAGCGGGGAG-3') and 856 (5'-CTGGTGATGCAGTTACCCATG-3').PCRs were performed under conditions that maintained the amplificationswithin the comparable, exponential phase determined by previouskinetic analysis. The identities of the PCR products were confirmedby sequencing and restriction enzymedigestion.

Immunocytochemical labeling of cells. Cells were characterized with numerous antibodies at 33° and 39°C at approximately thesame cell density. Cells were cultured at 33°C for 2-3 d and at39°C for 2 weeks. Cultures were fixed either for 15 min in 4%paraformaldehyde in PBS or for 10 min in cold 50:50 acetone/methanol(v/v) on ice. Acetone/methanol-fixed cultures were air-dried afterfixation. Cultures fixed with 4% paraformaldehyde were labeledwith antibodies to glial fibrillary acid protein (GFAP, Sigma,G-A-5), OCP-2 (gift of R. Thalmann, Washington University, St.Louis, MO), calretinin (AB149, Chemicon, Harrow, UK), parvalbumin(PA235, Sigma), $beta$ -tubulin [E7, Developmental Studies HybridomaBank (DSHB), University of Iowa], pan-fimbrin (737.4, gift ofP. Matsudaira, Whitehead Institute for Biomedical Research, Cambridge,MA), Brn3.1 (PRB249C Babco, Berkeley, CA), and ZO-1 (R26.4c, DSHB,University of Iowa). Those fixed with a 1:1 mixture of acetone/methanolon ice were labeled with antibodies to occludin (71-1500 Zymed,San Francisco), pan-cytokeratin (C2562, Sigma,), vimentin (Vim13.2,Sigma), neurofilaments (200 kDa, Sigma, N4142; 165 kDa, 2H3, DSHB;68 kDa, E1.9, DSHB), T antigen (Ab419; gift of Dr. P. Jat, LudwigInstitute for Cancer Research, London), and a range of our ownmonoclonal antibodies to hair cells (UB/CP1, UB/SC1, UB/SP1-3)(Nishida et al., 1998). After overnight incubation at 4°C, antibodybinding was visualized using FITC-conjugated goat anti-rabbitIg (Sigma), FITC-conjugated goat anti-mouse IgM (Sigma), and lissaminerhodamine-conjugated goat anti-mouse IgG (Jackson ImmunoresearchLabs, West Grove, PA). For control labeling of cultures, preimmunesera (where available), normal sera, or purified immunoglobulinsof the appropriate species were used at comparable concentrationsto the primary antibodies. Nuclei were visualized by incubatingwith 4',6-diamido-2-phenylindole dihydrochloride (DAPI) (1 µg/mlin PBS) for 5 min at room temperature before mounting in Vectashield(Vector Laboratories, Burlingame, CA). Labeled sections and cultureswere viewed on a Nikon Optiphot II and photographed using KodakTMY400 or AgfaRSX200.

All antibodies were also localized on 8 µm cryostat sections from various prenatal and postnatal mouse inner ears. After dissection,inner ears were either snap-frozen in Tissue Tek (Agar Scientific,Cambridge, UK), sectioned, and post-fixed in acetone or fixedovernight in 4% paraformaldehyde and transferred to 30% sucrosein PBS for 2 hr before embedding andsectioning.

For labeling of polymerized actin, cells were fixed with 4% paraformaldehyde, permeabilized with 0.5% Triton X-100 for 5 min,and labeled `with phalloidin conjugated to tetraethyl rhodamineisothiocyanate (Sigma) or Texas Red (Molecular Probes, Eugene,OR).

Estimates of numbers of cells labeled, particularly with antibodies to cytokeratin and vimentin, were made from cells culturedin 35 mm Petri dishes. In each dish four sites were selected randomly,and 50 cells were counted within grid squares defined with aneye-piecegraticule.

Immunoblotting. Whole-cell extracts were prepared from cells at 33°C after 2-3 d in culture and at 39°C after 14 d in culture.Cells (1.5 × 10⁶) were extracted on ice in 750 µl of buffer (150 mM NaCl, 1% NP40,0.1% SDS, 50 mM Tris, pH 7.4). The extract was centrifuged at10,000 × g for 10 min at 4°C. After discarding the pellet thesupernatant was assayed for protein concentration using a BCAassay (Pierce, Chester, England). The sample was then dilutedwith 2× sample buffer (10% 2-mercaptoethanol, 4% SDS, 20% glycerol,0.125 M Tris, pH 6.8) and boiled for 2-3 min before aliquotingat $-$ 80°C.

Samples were separated on either 4-15 or 10% SDS-PAGE gels (5 µg of protein per lane) under reducing conditions (Laemmli,1970). After SDS-PAGE, proteins were transferred to nitrocellulosemembranes (Sartorius, Göttingen, Germany), using a semi-dry blottingsystem, in 25 mM Tris, 192 mM glycine, 20% methanol, and 0.1%SDS for 2 hr at 40 mA. Nonspecific binding sites were blockedin PBS containing 2.5% BSA and 2.5% nonfat dried milk. Blots wereprobed for 2 hr with antisera against fimbrin (1:2000 dilution),Brn3.1 (1:400), and myosin VIIa (1:1000; kindly supplied by Dr.Aziz El-Amraoui, Institut Pasteur, Paris, France) followed bydetection with HRP-conjugated mouse anti-rabbit monoclonal antibody(RG-96 1:5000, Sigma) and Supersignal chemiluminescence substrate(Pierce, Rockford,IL).

Electron microscopy. Cells were cultured in 35-mm-diameter Petri dishes. The culture medium was removed and replaced with2% glutaraldehyde in 0.1 M sodium cacodylate buffer, pH 7.2, for60 min. After three 10 min washes in fresh buffer, the cells werepost-fixed with 1% osmium tetroxide in buffer (60 min), washedwith fresh buffer (three 10 min washes) and then distilled water(10 min), dehydrated with an ethanol series, and embedded in Eponthat was polymerized at 60°C for 48 hr. Thin sections were cuton a Reichert OMU2 ultramicrotome, mounted on pioloform filmson slotted grids, and stained with uranyl acetate and leadcitrate.

Electrophysiology. Whole-cell patch clamp was used to record membrane currents of single UB/UE-1 cells at room temperature(20-25°C). The extracellular solution contained (in mM): 135 NaCl,5.8 KCl, 1.3 CaCl₂, 0.9 MgCl₂, 0.7 NaH₂PO₄, 5.6 D-glucose, 10HEPES-NaOH. Amino acids and vitamins for Eagle's MEM were addedfrom concentrates (Life Technologies). The pH was adjusted to7.5, and the osmolality was ~302 mOsm/kg. In some experimentsa nominally Ca²⁺-free solution was used in which MgCl₂ was increased to 4.8 mMto keep membrane charge screening approximately constant. Measuredfree Ca²⁺ was 18 µM. In this solution and in a solution containing 10 mM4-aminopyridine (4-AP), NaCl was reduced to keep osmolality constant.In some experiments 100 µM acetylcholine was simply added. Patchpipettes were pulled from soda glass capillaries (Clark ElectromedicalInstruments). To reduce the electrode capacitance, the shank ofthe electrode was coated with wax. The pipette filling solutioncontained (in mM): 145 KCl, 3 MgCl₂, 1 EGTA-KOH, 5 Na₂ATP, 5 HEPES-KOH,pH 7.3 (288 mOsm/kg). The recording electrode had a resistancein the bath of 2-3 M $Omega$ . An EPC-8 (Heka) patch-clamp amplifier wasused for recordings. Data acquisition was performed using pClampsoftware (Axon Instruments, Foster City, CA) connected to a LabMasterDMA Interface. Data were filtered at 2.5 or 5 kHz, sampled at5 or 20 kHz, and stored on computer for off-line analysis. Residualseries resistance after compensation (40-50%) was 2-6 M $Omega$ . Recordingsand reported currents and conductances were corrected off-linefor linear leakage and residual capacitative transients. Membranepotentials were corrected for series resistance, and a liquidjunction potential of $-$ 4 mV was measured between pipette and bathsolutions. Statistical comparisons of means were made by one-wayANOVA followed by Tukey's post test; differences were deemed statisticallysignificant if p < 0.05. Values are shown as mean ±SD.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Isolation of utricular epithelial cells

Pure sheets of hair cells and supporting cells from the utriculi of 2-d-old Immortomouse pups were obtained after treatmentwith thermolysin. The epithelium was dissociated from the underlyingconnective tissue along the plane of the basal lamina. In similartissue fixed for electron microscopy, only epithelial cells wereobserved (Fig. 1a). In the light microscope the sensory epitheliumwas clearly visible, and trimming the edges ensured that all nonsensoryepithelial cells were removed. This was confirmed by labelingdissected epithelia with rhodamine-phalloidin to show the presenceof hair cells. In early experiments, the isolated maculae wereplated as intact epithelial sheets, but outgrowth was limitedto the edge of the explant, raising the possibility that we wereselecting a subpopulation of supporting cells from the edge. Bydissociating the epithelial sheet, it was possible to obtain cellclumps from throughout the whole epithelium (Fig. 1b). Cell outgrowthwas evident from most epithelial clumps, confirming that viable,dividing cells were present throughout the dissected epithelium.In these clumps, all cells expressed cytokeratins except for theremaining hair cells (Fig. 1c,d). These results showed that theprimary cultures were composed exclusively of utricular sensoryepithelial cells.

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Figure 1. The origin of the utricular cell line. a, Thin section of a dissected utricular epithelium treated with thermolysin. The arrowheads indicate the base of the epithelium. Immediately above this level are the supporting cells with their relatively dark nuclei. The lighter stained nuclei belong to hair cells. The epithelium has been separated from the underlying connective tissue so that hair cells and supporting cells are the only cells present. Scale bar, 10 µm. b, Dissociated clumps of epithelium such as that shown in a cultured under conditions for expression of the immortalizing gene. Scale bar, 100 µm. c, A recently isolated clump of utricular epithelium labeled by immunofluorescence for cytokeratin. The arrowheads indicate spaces occupied by hair cells. Scale bar, 50 µm. d, The same image as shown in c but labeled with DAPI to show the cell nuclei. The arrowheads indicate hair cell nuclei corresponding to the arrowheads in c. Scale bar, 100 µm. e, The cell line UB/UE-1 after 6 months at 33°C with $gamma$ -interferon. The cells proliferated rapidly under these conditions. Scale bar, 50 µm. f, UB/UE-1 at 39°C without $gamma$ -interferon. The cells ceased dividing and assumed more symmetrical, flattened shapes like epithelial cells. The arrowhead indicates the junctions between neighboring cells. Scale bar, 50 µm.

Epithelial cell proliferation was dependent on the expression of T antigen, because wild-type cultures maintained in the samemedium showed little or no outgrowth compared with the immortalizedcells. At confluence, primary cultures were passaged into freshdishes. The cells expressed cytokeratin and vimentin but not GFAPor neurofilaments at 33°C. After a number of additional passages,some lost their cytokeratin expression. Stable cytokeratin-positivecell lines were established from these cultures by limiting dilutioncloning, and one of these lines, UB/UE-1 (Fig. 1e,f), was usedfor these studies. Expression of cytokeratin was used as confirmationthat selected clones were derived from supporting cells and notfrom existing haircells.

At 33°C in the presence of $gamma$ IFN, 90% of the cells were labeled with antibody against the T antigen, the label being restrictedto the nucleus. After plating out at 39°C without $gamma$ IFN, the numberof labeled cells dropped to <10% in 2 d, and by 3-4 d none werelabeled (Fig. 2A). This reduction in T antigen expression wasrelated to a decrease in cell division (Fig. 2B). Proliferationcontinued past confluence at 33°C, and the cells became very tightlypacked. At 39°C, however, the cells stopped proliferating andrapidly adopted a flattened "fried-egg" morphology and formedsome cell-cell contacts (Fig. 1f).

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Figure 2. The relationship between cell proliferation and expression of the T antigen. A, Graph showing the percentage of the total number of cell nuclei (n = 200 at each point) labeled with an antibody to the T antigen after subculture from 33°C with $gamma$ IFN to 39°C without $gamma$ IFN. The result suggests that the immortalizing gene was downregulated within 2-3 d. b, Graph showing the number of cells counted in cultures placed under the same conditions as those in a. The proliferation rate was much higher at 33°C with $gamma$ IFN.

Expression of supporting and hair cell markers

Cytokeratin was expressed in >90% of cells at 33°C (Fig. 3a), and this level of expression was stable over a large numberof population doublings. At 39°C the proportion of positive cellsdecreased to ~40%, and the intensity of labeling in those cellsstill expressing cytokeratin (Fig. 3b) was reduced. Objectiveassessment of cytokeratin expression was not clear-cut becausea few labeled strands were often observed in cells that otherwiseappeared to be unlabeled. In contrast, vimentin continued to beexpressed in >95% of cells at both 33° and 39°C (Fig. 3c,d). Labelingwith pan-cadherin antibodies showed little evidence for cell-celljunctions at 33°C but clear evidence of adherens-type junctionsat 39°C (data not shown).

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Figure 3. Expression of cytoskeletal proteins in cells under proliferating and differentiating conditions. Cells were cultured at 33°C with $gamma$ IFN (a, c, e, g) or for 14 d at 39°C without $gamma$ IFN (b, d, f, h). They were then labeled with antibodies to cytokeratin (a, b), vimentin (c, d), or tubulin (e, f), or with rhodamine-phalloidin to label actin (g, h). Most cells expressed vimentin, so the antibody to this protein was used to identify cells that did not express cytokeratin. Thus a and c (33°C) and b and d (39°C) show the same cells double-labeled for cytokeratin and vimentin. Up to 10% of cells were unlabeled for cytokeratin at 33°C (arrowheads in a and c), but up to 60% were unlabeled at 39°C (arrowheads in b and d). Although vimentin was expressed in most cells at both temperatures, the labeling was less intense at 39°C. The changes in cell morphology under differentiating conditions were clearly illustrated in cells labeled for microtubules and actin filaments. The distribution of microtubules was more even and symmetrical in cells at 39°C (e, f). The more intensely labeled filaments may be flagellar axonemes (arrowhead in f). At 39°C cells possessed strong, punctate labeling for actin (arrowhead in h) and numerous well developed structures resembling stress fibers (arrow in h). Scale bar (shown in b for a-h), 100 µm.

The immunolabeling for microtubules clearly revealed the change in general cell morphology at the two temperatures (Fig. 3e,f).The dense labeling at 39°C made it difficult to discern individualstructures, but despite the appearance of more intensely labeledfilaments (Fig. 3f) and the identification of flagellar axonemesby electron microscopy (see below), there did not appear to beany evidence for organized kinocilia. The label for actin showedtwo relevant differences in morphology (Fig. 3g,h). Cells at 39°Cpossessed many more actin filament bundles, or "stress fibers,"and in most cases a very bright, punctate structure formed closeto the center (Fig. 3h). Although well ordered hair bundles werenot observed, some of these stress fibers labeled for fimbrin,an actin bundling protein that has previously been localized tostereocilia of mouse vestibular hair cells. Immunolabeling ofprimary cultures of vestibular epithelia from normal mice showedthat fimbrin localized only to stereocilia within hair cells butwas absent from supporting cells (Fig. 4a). In cells from UB/UE-1,fimbrin was also expressed in focal contact-like, actin-labeledstructures at the free edges of cells (Fig. 4b,c). It did notappear to coincide with the punctate label observed with phalloidin.

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Figure 4. Fimbrin was expressed in stereocilia and in some actin bundles of cultured cells. a, An antibody to fimbrin specifically labeled hair bundles on utricular hair cells in organotypic cultures. b, A cell from UB/UE-1 at 39°C labeled for actin with rhodamine-phalloidin. Labeling was observed on intracellular structures resembling stress fibers (arrowheads). c, The same cell as shown in b labeled for fimbrin. Note that all the fibers labeled for fimbrin also contained actin (arrowheads). Scale bar, 100 µm.

RT-PCR and immunoblotting revealed the expression of several genes normally expressed selectively by hair cells (Fig. 5).mRNA for Brn3.1 was detected at low levels under both conditionsbut was apparently expressed at lower levels at 39°C. Immunoblottingfor the Brn3.1 protein confirmed this result. mRNA for the $alpha$ 9AChRwas not detected at 33°C but was clearly present at 39°C, suggestingthat the gene was only expressed under differentiating conditions.Lack of a suitable antibody for the $alpha$ 9AChR meant that we wereunable to verify the level of protein expression. Trace levelsof mRNA for myosin VIIa were detected at 33°C, with higher levelsat 39°C. By immunoblotting, no myosin VIIa protein was detectedat 33°C, but a band of 220 kDa was detected at 39°C showing thatprotein expression also increased. mRNA for myosin VI was expressedunder both conditions and also appeared to be more abundant at39°C.

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Figure 5. Expression of hair cell markers under proliferating and differentiating conditions. a, RT-PCR showing the relative levels of expression of different hair cell markers between cells at 33°C and cells at 39°C. GAPDH was used as a normalizing control. b, Immunoblots of UB/UE-1 using anti-Brn3.1, fimbrin, and myosin VIIa antibodies. The protein samples probed for Brn3.1 and fimbrin were fractionated through a 10% SDS-PAGE, whereas the ones for myosin VIIa were run in a 6% SDS-PAGE. Each lane was loaded with 5 µg of protein. A slight decrease in both mRNA and protein was observed for Brn3.1 at 39°C. Myosin VIIa and fimbrin were upregulated at 39°C. In general terms, the results for the immunoblots and RT-PCR correlated well except for myosin VIIa, where mRNA but not protein was detectable at 33°C.

The antibodies to fimbrin recognized a 68 kDa band by immunoblotting, and this labeling suggested that expression was higherat 39°C than at 33°C (Fig. 5b). These results confirmed the specificityof the label and correlated with the higher number of stress fibersthat formed at 39°C. The cell line did not express calretinin,OCP-2, UB/CP1, UB/SC1, UB/SP1-3, ZO-1, or occludin at either temperatureas judged by either immunofluorescence-labeling or immunoblotting.

Ionic currents in cells grown at 33°C

Cells grown at 33°C, hereafter referred to as proliferating cells, were visibly variable in size, an observation confirmedby the large SD of the membrane capacitance (Table 1; Fig. 6).All cells investigated exhibited a small negative resting membranepotential of $-$ 10 to $-$ 30 mV. Typical examples of membrane responses,during application of depolarizing and hyperpolarizing voltagesteps, are shown in Figure 7a,b. In all cells investigated, depolarizingsteps from a holding potential of $-$ 64 mV elicited small, seeminglyinstantaneous outward currents from potentials positive to about $-$ 20 mV. Only small inward currents could usually be detected duringapplication of hyperpolarizing voltage steps from the same holdingpotential. A typical steady-state current-voltage (I-V) relationshipis shown in Figure 7c. No electrical responses were observed afterapplication of 100 µM acetylcholine to cells whose membrane potentialwas held at $-$ 54 mV (n = 13).


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Table 1. Physiological properties of different cell populations

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Figure 6. Histograms showing the distribution of membrane capacitance (C_m) in the different groups of cells. a, Cells grown at 33°C (n = 40); b, supporting-type cells grown at 39°C (n = 18); c, Sensory-type cells grown at 39°C (n = 25). Bin width is 20 pF.

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Figure 7. Membrane currents under voltage clamp in a UB/UE-1 cell grown at 33°C. a, Outward currents from a holding potential of $-$ 64 mV elicited by depolarizing voltage steps in nominal increments of 10 mV (actual membrane potentials shown by some of the traces). b, Responses to hyperpolarizing steps in nominal 10 mV increments from $-$ 64 mV. Note the absence of inward currents. c, Steady-state current-voltage (I-V) curve of currents shown in a and b. The steady-state currents in Figures 7-11 were measured near the end of the voltage steps (t = 170 msec for depolarizing steps and t = 40 msec for hyperpolarizing steps). All records are single traces in this and all subsequent figures. V_m = $-$ 12 mV; C_m = 21 pF; residual R_s = 4.3 M $Omega$ ; 22°C. Linear leak subtracted: 3.7 nS.

Ionic currents in cells grown at 39°C

At 39°C the membrane currents were more heterogeneous than at 33°C. On the basis of differences in current responses, cellswere grouped in three categories: two with currents similar tothose in normal vestibular hair cells, and one with currents similarto those of normal supporting cells. These categories of cellswill be referred to as "sensory-type cells" and "supporting-typecells." Sensory-type cells were first encountered after 6 d at39°C, and all three groups were still present after 45 d, thelongest time tested. The resting membrane potentials of sensory-typecells (range $-$ 15 to $-$ 40 mV; n = 25) were significantly differentfrom those of both supporting-type cells ( $-$ 10 to $-$ 25 mV, n = 16;p < 0.001) and proliferating cells ( $-$ 10 to $-$ 30 mV, n = 33; p <0.001) (Table 1). Although all cell types had a wide range ofmembrane capacitance, the mean capacitance of the sensory-typecells was larger than both the supporting-type (p < 0.01) andproliferating cells (p < 0.05) (Fig. 6). No significant differencesin membrane potential or capacitance were found between supporting-typeand proliferatingcells.

Ionic currents in supporting-type cells
Figure 8a,b shows a representative set of traces. In almost all cells, depolarizing steps from $-$ 64 mV evoked tiny, almostinstantaneous outward currents. Hyperpolarizing steps from thesame potential elicited small and sustained inward currents. Thesteady-state I-V relationship (Fig. 8c) indicated small amountsof outward and inward rectification positive to $-$ 20 and negativeto $-$ 90 mV, respectively. When acetylcholine was applied, no responseswere recorded from seven of eight cells held at $-$ 54 mV. One cellproduced a very small inward current.

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Figure 8. Membrane currents in a UB/UE-1 supporting-type cell grown at 39°C. a, Outward currents from $-$ 64 mV. b, Inward currents from $-$ 64 mV. c, Steady-state I-V curve of currents shows in a and b. V_m = $-$ 14 mV; C_m = 13 pF; residual R_s = 3.6 M $Omega$ ; 23°C. Linear leak subtracted: 1.5 nS.

Ionic currents in sensory-type cells
Typical examples of voltage-dependent potassium currents recorded from a holding potential of $-$ 64 mV for the two differentgroups of sensory-type cells are shown in Figures 9, 10. In thesecells, depolarizing voltage steps caused slowly activating voltage-dependentoutward currents that were much larger than those in the othercell types. A small inward current, probably carried by calciumions, preceded the outward current in some cells. The time ofhalf-maximal activation of the outward currents decreased as afunction of increasing test potential and in both groups was ~13msec around 0 mV and 6 msec around +40 mV. The steady-state valuesof the outward currents were measured near the end of the testpulse to generate I-V curves. Outward current started to activateat potentials close to $-$ 40 mV. The size of the current, measuredat +40 mV, ranged from 400 to 1300 pA. Superfusion with nominallyCa²⁺-free solution had no effect on this current (n = 5). Superfusionwith 10 mM 4-AP reversibly reduced the outward currents (measurednear +50 mV) by ~65% (n = 5).

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Figure 9. Membrane currents under voltage clamp in UB/UE-1 sensory-type cells with inward rectifier grown at 39°C. a, Outward currents in response to depolarizing voltage steps from $-$ 64 mV to the various test potentials shown by some of the traces. b, Inward currents of the same cell to hyperpolarizing steps from $-$ 64 mV. Note the decay of the currents for potentials negative to $-$ 130 mV. c, Steady-state I-V curves of currents shown in a and b () and peak I-V ( $open circle$ ) of currents shown in b. V_m = $-$ 29 mV; C_m = 48 pF; residual R_s = 6 M $Omega$ ; 23°C. Linear leak subtracted: 1.0 nS. d, Steady-state activation curve of the outward currents in another cell. The inset shows the tail currents on returning to a test potential of $-$ 24 mV after 170 msec steps to a range of potentials between $-$ 64 mV and + 33 mV in nominal increments of 10 mV. The curve is the best fit to the Boltzmann equation (see Results), with I_max = 209 pA, V_1/2 = $-$ 16.6 mV, and S = 6.7 mV. V_m = $-$ 39 mV; C_m = 52 pF; residual R_s = 4 M $Omega$ ; 23°C. Linear leak subtracted: 0.9 nS.

Hyperpolarizing voltage steps elicited inward currents only in 40% of sensory-type cells. A typical example of the inwardrectifier current is shown in Figure 9b. The current rapidly reacheda plateau that was maintained throughout the voltage steps downto approximately $-$ 130 mV. At more negative potentials, the currentsdecayed in a voltage-dependent manner. The I-V relationship (Fig.9c) shows that the inward current activated negative to $-$ 80 mVand that peak and late currents started to diverge negative to $-$ 130 mV. In other sensory-type cells, hyperpolarizing steps didnot elicit any time- or voltage-dependent current (Fig. 10b). Long(500 msec) hyperpolarizing voltage steps elicited no evidenceof the slowly activating weak inward rectifier I_h (Holt and Eatock,1995).

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Figure 10. Membrane currents in a UB/UE-1 sensory-type cell without inward rectification, grown at 39°C, under voltage-clamp conditions. a, Outward currents from $-$ 64 mV. b, Lack of inward currents from $-$ 64 mV (12 nominal 10 mV steps down to $-$ 174 mV). c, Steady-state I-V curve of currents shown in a and b. d, Steady-state activation curve of the outward currents. The inset shows the tail currents on returning to a test potential of $-$ 24 mV. Boltzmann fit: I_max =227 pA, V_1/2 = $-$ 14.1 mV, and S = 7.5 mV. V_m = $-$ 24 mV; C_m = 41 pF; residual R_s = 6 M $Omega$ ; 23°C. Linear leak subtracted: 0.6 nS.

The activation curves of the outward currents recorded in the two groups of sensory-type cells were generated by analyzingtail currents at a fixed test membrane potential (Figs. 9d, 10d).The outward current activated at potentials close to $-$ 40 mV andwas almost completely recruited close to 0 mV. Data were fittedby the first-order Boltzmann equation: I = I_max/{1 + exp[(V_1/2 $-$ V_m)/S]}, in which I is the tail current measured 1 msec afterthe step to the test potential, I_max is the maximal tail current,V_1/2 is the potential at which the half-maximal activation occurred,V_m is the membrane potential of the voltage step preceding thetest potential, and S describes the voltage sensitivity of activation.No significant differences were found in V_1/2 and S between thetwo groups of cells. V_1/2 and S in sensory-type cells that showinward rectification were $-$ 14.9 ± 1.5 mV (n = 3) and 7.7 ± 1.1mV (n = 3), respectively. V_1/2 and S values in sensory-type cellswithout inward rectification were $-$ 13.6 ± 1.4 mV (n = 3) and 8.0± 1.6 mV (n = 3). Application of acetylcholine elicited an inwardcurrent of up to 200 pA in four of five sensory-type cells culturedat 39°C when held at a holding potential of $-$ 54 mV, thus confirmingthe expression of functional receptors as suggested by the resultsfrom the RT-PCR.

Ionic basis of the outward current
The ionic basis of the outward current in sensory-type cells was established by analyzing the tail currents at different potentialsafter a step potential to near 0 mV for 170 msec, from a holdingpotential of $-$ 84 mV. A family of tail currents elicited in a solutioncontaining a normal concentration of K⁺ (5.8 mM) is shown in Figure 11a. The tail currents at the peakand at the steady state were plotted against potential to generateI-V curves (Fig. 11b). The reversal potential was taken as theintersection of the two curves (Ritchie, 1987). Tail currentsreversed at $-$ 62 ± 9 mV (n = 3), near the K⁺ equilibrium potential ( $-$ 83 mV) calculated for our experimentalconditions using the Nernst equation. These results indicate thatthe outward current was mainly carried by potassium ions.

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Figure 11. Reversal potential of I_K of a sensory-type cell without inward rectifier. a, Tail currents in response to voltage steps to potentials between $-$ 114 and $-$ 4 mV after a 170 msec conditioning step to $-$ 4 mV (protocol shown schematically below). b, Tail currents 1 msec after the voltage step ( $open circle$ ) and at the steady state () plotted against voltage. Reversal potential ( $-$ 70 mV) taken as the intersection of the two curves. V_m = $-$ 29 mV; C_m = 47 pF; residual R_s = 2.3 M $Omega$ ; 23°C. Linear leak subtracted: 0.7 nS.

Electron microscopy

Cultured cells were ~50-60 µm in diameter and 1-3 µm thick (Fig. 12a). In the central, nuclear region the thickness increasedto ~5 µm. Electron-dense, punctate structures were observed aroundthe cell margins, but there was no evidence for continuous intercellularjunctions. The most notable feature of some cells at 39°C wasa thickened cytoskeletal meshwork underlying the entire apicalsurface penetrated by focal cytoskeletal structures resemblingmicrovillar rootlets (Fig. 12b). These rootlets almost certainlyrepresented at least a subset of the stress fibers labeled withphalloidin and viewed in the light microscope (Fig. 3h). Fromsome cells microvillar projections emerged from the cell surface,but only a few structures like this were observed in thin section(Fig. 12c). The mesh, rootlets, and projections were all composedof microfilaments 4-6 nm thick. Ciliary axonemes lay across thesurfaces of cells and were visible both in transverse section(Fig. 12d) and in scanning images at low power (data not shown).

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Figure 12. Cytoskeletal structures beneath the upper surfaces of cells from UB/UE-1 at 39°C. a, Electron micrograph of an oblique section through a cell from UE-1 under differentiating conditions. Beneath the upper plasma membrane there is a thick cytoskeletal mesh composed of microfilaments (arrowheads). The arrow indicates the nucleus. Scale bar, 20 µm. b, The microfilament mesh was penetrated by numerous microfilament bundles (arrowheads). Scale bar, 1 µm. c, This image shows a single structure, containing a parallel bundle of microfilaments, projecting from the cell surface. Scale bar as in b. d, This image shows the microfilament mesh (arrow) and cross sections through two flagellar axonemes (arrowheads). Scale bar as in b.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have established a clonal, conditionally immortal cell line from a postnatal, mammalian vestibular sensory epithelium.The cells differentiate into three discrete types that can bedistinguished unambiguously by the ionic channels that they expressin the plasma membrane. The two sensory-type cells resemble variantsof normal, neonatal, vestibular hair cells, and the supporting-typeresembles normal vestibular supporting cells. The identity ofthe cells under proliferating conditions is based on the initialpreparation of pure sensory epithelia and on selection for cellsthat express cytokeratins. Pure epithelia are composed of haircells and supporting cells, but although differentiated hair cellssurvive for some weeks in our cultures, they never express cytokeratinsor mitotic figures. The electrophysiology of membrane currentsprovides an objective, functional assay for the identity of differentcell types, and it is this evidence that forms the basis of ourconclusions.

Many different types of hair cell express a characteristic, delayed rectifier potassium current (I_K) (Fuchs, 1992). The sensory-typecells from UB/UE-1 express a slow-activating, outward potassiumcurrent recruited at potentials positive to $-$ 40 mV with a timecourse characterized by a relatively slow half-maximal activation(~13 msec at 0 mV) and by the lack of any fast inactivation during170 msec test pulses. These properties, together with the sensitivityto block by 4-AP and the insensitivity to extracellular calciumlevels, suggest that they express a typical I_Kcurrent.

Delayed rectifiers represent the principal potassium current in type II hair cells of several vestibular organs (Lang andCorreia, 1989; Griguer et al., 1993; Masetto et al., 1994; Masettoand Correia, 1997), where they contribute to shaping the receptorpotential. Type I vestibular hair cells are dominated by a muchlarger potassium conductance, I_K,L, which is activated at verynegative potentials (Rennie and Correia, 1994; Rüsch and Eatock,1996). This conductance is so large that it normally masks anyother outward potassium conductances in type I cells. Residualpotassium conductances are revealed on blocking I_K,L pharmacologically.In guinea pigs, such a conductance has been identified as a calcium-activatedpotassium current (Rennie and Correia, 1994), whereas in micethe residual conductance has been classified as a classic delayedrectifier (Rüsch et al., 1998). Too little is known about thedevelopment, pharmacology, or molecular basis of delayed rectifierpotassium currents in vestibular hair cells to judge whether thecurrent in UB/UE-1 resembles that in neonatal, mature type IIor mature type I hair cells (Rüsch et al., 1998). However, theabsence of I_h, a weak inward rectifier normally expressed fromP3 or P4 (Rüsch et al., 1998), suggests that they are more likeneonatal hair cells that may retain the competence to differentiateinto either type I or type II haircells.

An inward rectifier current was found only in a subpopulation (40%) of cells from UB/UE-1 that expressed the delayed rectifier.Its rapid activation negative to the potassium equilibrium potentialidentifies the current as the classic inward rectifier I_K1. Themarked decay observed at potentials negative to $-$ 130 mV has beendescribed for I_K1 in vestibular neonatal and type II hair cellsof various classes of vertebrates (Ohmori, 1984; Masetto et al.,1994; Holt and Eatock, 1995; Sugihara and Furukawa, 1996; Rüschet al., 1998) and indeed in many other cell types and cloned channels(Kubo et al., 1993). In agreement with our findings in the culturedcells, I_K1 is not found in all neonatal and type II hair cellsin the developing mouse utricle (Rüsch et al., 1998). A possibleexplanation for this is regional variation across the epitheliumin the expression of I_K1 that has been reported in type II haircells of the frog semicircular canal (Marcotti et al., 1999).Such regional variations have thus far not been studied in mammalianvestibular epithelia. Both I_K and I_K1 are likely to contributeto the resting potential, which was somewhat more negative (butnot significantly so) in the cells expressing I_K1 (Table 1).

The membrane currents of the supporting-type cells were similar to those of normal vestibular supporting cells (Sugihara andFurukawa, 1996; Masetto and Correia, 1997). They were electricallysimilar to the cells grown at 33°C and showed little or no voltage-dependentionic currents except for a weak inward and outward rectificationfor very negative and positive voltages,respectively.

The electrophysiology of the cell line remained remarkably consistent throughout many different experimental transitions from33° to 39°C and for different populations of cells thawed fromfrozen stocks at different times. At 33°C the population was clearlyhomogeneous, and at 39°C there was virtually no ambiguity in definingthe three different phenotypes. With the exception of a smallresponse in one cell, acetylcholine receptor currents were onlyrecorded from cells that also expressed the delayed rectifierpotassium current. There was also a direct correlation betweenthis rectifier and cell size as estimated by membrane capacitance.Thus the transition to differentiating conditions activates thecoherent, functional expression of a number of key hair cellgenes.

The decrease in cytokeratin expression from 90 to 40% is consistent with the differentiation of approximately half the cellsas hair cells. The observed increase in expression of myosin VIIaand the $alpha$ 9AChR is also consistent with the differentiation ofhair cells. However, we did not expect to see either Brn3.1 expressedat 33°C or downregulation at 39°C. Brn3.1 is expressed as earlyas embryonic day 14 in the utricle, but new cells continue tobe born until P6 (Sans and Chat, 1982). Although Brn3.1 is essentialfor continued hair cell differentiation (Erkman et al., 1996;Xiang et al., 1997), myosin VIIa is expressed transiently in theBrn3.1 null mutant, suggesting that hair cells begin to differentiatebut then die (Xiang et al., 1998). In current models of cell patternformation by lateral inhibition, differentiating hair cells arethought to inhibit adjacent cells from adopting the same fate(Adam et al., 1998; Haddon et al., 1998; Lewis et al., 1998; Lanfordet al., 1999). If hair cells are lost then the inhibition maydecrease, allowing new or existing neighbors to become hair cells(Stone and Rubel, 1999). Thus we might expect supporting celllines to initiate hair cell differentiation simply as a functionof dilution cloning. Proliferating cells did not reform tightintercellular junctions at 33°C, and if the mechanism of lateralinhibition was thus blocked, then the cells may effectively havebeen immortalized at an early stage of hair cell differentiation.When differentiated, however, the cells formed closer contacts,and lateral inhibition may have been at least partially restored.Thus if Brn3.1 was expressed in all cells at 33°C but subsequentlysuppressed in 50% of them at 39°C, this might explain the observeddecrease in expression of Brn3.1. The implication is that cellsexpressing Brn3.1 are not irreversibly committed to becoming haircells, suggesting some plasticity in the mechanism of lateralinhibition. We were unable to detect Brn3.1 in individual cellsby immunofluorescence, so expression appeared to be low comparedwith that in our cochlear cell lines (Rivolta et al., 1998).

The cell line UB/UE-1 offers significant experimental potential toward understanding the molecular mechanisms that governhair cell differentiation. It conditionally expresses at leastthree functional ion channels and several cytoskeletal proteinsthat characterize an early, critical stage in hair cell differentiation.These features are unlikely to be an artifact of the T antigenfor several reasons. Not all cells at 39°C express the same markers,and different cell lines from the cochlea express different structuraland physiological markers under the influence of the T antigenat 33°C (Rivolta et al., 1998; Jagger et al., 1999). Few celllines differentiate fully in vitro. In previous experiments withmixed utricular cultures derived from the Immortomouse, markersfor much later stages of hair cell differentiation were expressed(Holley et al., 1997). Thus it is more likely to be the cultureconditions that limit hair cell differentiation in UB/UE-1 ratherthan an inhibitory effect of the Tantigen.

Cell lines lend themselves to studies of low-abundance, cell-specific molecules. This is particularly important in the mammalianinner ear because the number of sensory cells is so small. Moreimportantly, the conditional expression of a number of importanthair cell genes in UB/UE-1 reflects the likely activation of keytranscriptional processes. With an abundance of cells, the associatedgenes can be identified by screening with oligonucleotide (Alonet al., 1999) or cDNA arrays (Vishwanath et al., 1999). The samecells provide the means to explore the function of those genesexperimentally. Such applications should make a substantial contributionto our understanding of development and potential mechanisms oftherapeutic regeneration in the mammalian innerear.

  FOOTNOTES

Received June 8, 1999; revised Aug. 4, 1999; accepted Aug. 13, 1999.

This work was supported by The Wellcome Trust. M.C.H. is a Royal Society University ResearchFellow.
P.L. and W.M. contributed equally to thiswork.

Correspondence should be addressed to Matthew C. Holley or Corné J. Kros, Department of Physiology, School of Medical Sciences,University of Bristol, University Walk, Bristol BS8 1TD, UK. E-mail:m.c.holley{at}bristol.ac.uk or c.j.kros{at}bristol.ac.uk.

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ABSTRACT
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MATERIALS AND METHODS
RESULTS
DISCUSSION
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