evaluation of ribbon synapses at specific frequency regions of mouse cochlea

Evaluation of Ribbon Synapses at Specific Frequency Regions of Mouse Cochlea

After dissection, place each cochlear turn into individual 2.5-milliliter centrifuge tubes. Block any nonspecific binding with 10% goat serum in PBS in 0.1% Triton X-100 for 1 hour at room temperature on a rotator.
At the end of the incubation, use a 200-microliter pipette tip to remove the solution under a dissection microscope. Incubate the specimens with the primary antibodies of interest diluted in 5% goat serum in PBS and 0.1% Triton X-100 overnight at 4 degrees Celsius on a rotator.
The next morning, rinse the tissue samples three times for 5 minutes with cold 0.1 molar PBS per wash to remove any residual primary antibody. Then, label the specimens with the appropriate secondary antibodies diluted in 5% goat serum in PBS and 0.1% Triton X-100 for two to three hours at room temperature on the rotator, protected from light.
At the end of the incubation, wash the samples three times with 0.1 molar PBS as demonstrated, and transfer the specimens into individual 35-millimeter plates containing 0.1 molar PBS. Place a drop of DAPI-supplemented mounting medium onto the slide, and transfer the specimens from PBS to the mounting medium. Place one edge of a coverslip onto each slide and release to let the coverslips fall gently. Then, dry the slides in a slide box at 4 degrees Celsius overnight.
To image the specimens, use a confocal microscope with the appropriate lasers and a 63x high-resolution oil immersion lens. To acquire 8-micrometer confocal z-stacks from each cochlea turn. For synaptic punctum counts, set the z-stacks with the 0.3-micrometer step size to span the entire length of inner hair cells, ensuring that all of the synaptic puncta can be imaged, and merge the puncta-containing images in a stack to obtain the z-axis projection.
Import the merged images to an appropriate image processing software program. Divide the synaptic total counts in each z-stack at specific frequency regions by the number of DAPI-positive inner hair cells to calculate the number of synaptic puncta for each cell. At each specific frequency region, average all of the synaptic puncta in 3 images of different microscopic fields containing 9 to 11 inner hair cells.
To better visualize the cytoskeletal architecture and synaptic localization, use the brush tool to visually assess the synaptic structure and distribution of the individual inner hair cells. To inspect the juxtaposition of presynaptic ribbons and postsynaptic receptor patches, use the rectangular marquee tool to extract the voxel space around the ribbons, and use image cutting to isolate the individual ribbons. Then, click Image and Image Size to acquire a thumbnail array of these miniature projections that can be used to identify paired synapses versus orphan ribbons.

evaluation-ribbon-synapses-at-specific-frequency-regions-mouse

Research

JoVE Encyclopedia of Experiments

Neuroscience

Neurophysiology

Electrophysiology Techniques

EoE Sub Articles

eoe sub articles

All procedures involving animal handling have been performed in accordance with the institute&#39;s IRB guidelines.
1. Animal Selection
<ol>
	<li>For all experiments, use adult C57BL/6J male mice (8 weeks old) as the animal model. 
	&#160;NOTE: C57BL/6J mice carrying a splice variant of the Cdh23 exhibit accelerated senescence in the auditory system, reflected as a 40% loss of ribbon synapses at the basal turn of the cochlea and a 10% loss at the middle turn by 6 months of age, followed by a rapid increase of this loss in the whole cochlea with age. Thus, we advise caution when using C57BL/6J mice older than 6 months for auditory research. Other strains of mice can be used depending on specific experimental aims.</li>
	<li>Inspect the mice using a professional diagnostic pocket otoscope to rule out outer or middle ear pathologies prior to hearing assessments. Potential signs may include fluid or pus in the external auditory canal, redness and swelling in local tissue, and tympanic membrane perforation. 
	&#160;NOTE: Although this is rarely encountered, once identified, mice with outer or middle ear diseases should be excluded.</li>
</ol>
2. Hearing Assessment
<ol>
	<li>Anesthetize mice using an intraperitoneal injection of a mixture of ketamine hydrochloride (100 mg/kg) and xylazine hydrochloride (10 mg/kg). Judge the depth of anesthesia via painful stimuli (e.g., toe-pinch reflex). 
	&#160;NOTE: When the toe-pinch reflex is completely absent, the animal has reached an adequate depth of anesthesia for auditory testing. If more time is required for bilateral ABR (auditory brainstem response) recordings, administer a lower dosage (one-fifth the original dosage) of anesthetics to restore the original anesthetic plane. Take care to avoid anesthetic overdose, as this may lead to death in mice.</li>
	<li>Maintain the anesthetized animal&#39;s body temperature at 37.5 &#176;C using a thermoregulating heating pad. Place the anesthetized animal in an electrically and acoustically shielded room to avoid interference throughout the hearing test. 
	&#160;NOTE: Maintain the physiological temperature during the entire procedure until the animal is totally awake in order to prevent death caused by post-anesthesia hypothermia.</li>
	<li>Place subdermal needle electrodes (20 mm, 28 G) at the vertex of the skull (recording electrode), in the ipsilateral parotid region below the pinna of the measured ear (reference electrode), and in the contralateral parotid region (ground electrode), with a depth of 3 mm under the skin of the mouse head, respectively.</li>
	<li>Use a closed-field speaker to perform acoustic stimulation via a 2 cm plastic tube with a cone-shaped tip. Fit the tip into the external ear canal. 
	&#160;NOTE: Ensure that the electrical impedance in the recording and reference electrodes is less than 3 kOhm (usually 1 kOhm). If the impedance is high, change the insertion site of the electrode, clean the electrode with alcohol, or replace the electrode to avoid alterations in ABR wave amplitude.</li>
	<li>For ABR recording, generate tone pips (3 ms duration, 1 ms rise/fall times, at a rate of 21.1/s, frequency: 4&#8211;48 kHz) and present them at decreasing sound pressure levels (SPLs) from 90 to 10 dB in 5&#8210;10 dB SPL steps. During this step, the responses are amplified (10,000 times), filtered (0.1&#8211;3 kHz), and averaged (1,024 samples/stimulus level). 
	&#160;NOTE: ABRs are collected for each stimulus level in 10 dB steps, with an additional 5 dB steps near the threshold.</li>
	<li>At each frequency, determine the ABR threshold, which refers to the minimal SPL resulting in a reliable ABR recording with one or more distinguishable waves that can be clearly identified by visual inspection. 
	&#160;NOTE: It is usually necessary to repeat the process for low SPLs around the threshold to ensure the consistency of the waveforms. The response threshold is the lowest stimulus level at which the waveform can be observed when a decrease of 5 dB would lead to the disappearance of the waveform.</li>
</ol>
3.&#160;Cochlear Tissue Processing
<ol>
	<li>After ABR recording, euthanize the anesthetized mice via cervical dislocation, decapitate them, expose the bulla from the ventral side, and open them with sharp scissors to gain access to the cochlea.</li>
	<li>Using fine forceps, remove the temporal bones, sever the stapes artery, remove the stapes from the oval window, and rupture the round window membrane. Make a small hole at the apex of the cochlea by gently rotating the tip of a needle (13 mm, 27 G).</li>
	<li>Fix the isolated bones with 4% (wt/vol) paraformaldehyde in 0.1 M phosphate-buffered saline (PBS, pH 7.4) overnight at 4 &#176;C. Using a fine-tipped pipette, gently flush fixative through the perilymphatic spaces via application to the oval or round windows (as an inlet) and the opening at the apex (as an outlet). 
	&#160;NOTE: Some proteins require a short duration of fixation to avoid destruction of their epitopes for immunolabeling. In such cases, incubate bones in 4% paraformaldehyde at room temperature (RT) for 2 h, depending on the manufacturer&#8217;s instructions for immunohistochemistry. Fixation can also be performed via cardiac perfusion to remove the cochlear blood, avoiding background noise due to non-specific staining at later stages, particularly in mouse models of cochlear synaptopathy.</li>
	<li>Rinse the bones three times for 5 min with 0.1 M cold PBS to remove residual paraformaldehyde. Decalcify the bones with 10% ethylenediaminetetraacetic acid (EDTA) either at RT for 4 h or at 4 &#176;C for 24 h via gentle shaking in a horizontal shaker at 20 rpm. EDTA can be refreshed midway. 
	&#160;NOTE: Decalcification times are subject to the concentration of EDTA and users&#8217; preferences. Decalcified tissue should maintain a certain degree of toughness, which facilitates the manipulation of isolating cochlear whole mounts at later steps. Temporal bones can be decalcified in 10% EDTA with rotation, allowing researchers to leave the laboratory following ABR tests and fixation experiments. The decalcification time is flexible within the range of 20 to 30 h at 4 &#176;C.</li>
	<li>Transfer one decalcified temporal bone from EDTA to 0.1 M PBS. Use #3 and #5 Dumont forceps and the 27 G needle to dissect the apical, middle, and basal cochlear regions in turn and then dissect the cochlea out of the bone under a stereo dissection microscope. Make a series of small cuts along the spiral ligament using a razor blade, and remove the tectorial membrane and Reissner&#8217;s membrane (Figure 1). 
	&#160;NOTE: As long as the dissected cochlea is intact, this process can be modified according to the individual operator&#39;s usual protocol.</li>
	<li>Further dissect the remaining auditory epithelium including the spiral limbus into individual cochlear turns (apex, middle, and base with hook region) for whole-mount preparations.</li>
	<li>Under a 40x oil objective of a light microscope, measure the basilar membrane length with a 250 &#956;m scale placed in the eyepiece, which can be adjusted along the stereocilia of the IHCs.</li>
	<li>Calculate the length of each cochlear turn by adding all segment lengths (250 &#956;m per segment), and concomitantly obtain the total length of the basilar membrane by summing the lengths of each turn.</li>
	<li>Convert the total length of the basilar membrane, including the hook region, into a percentage based on distance from the cochlear apex (0% refers to the cochlear apex, 100% to the cochlear base).</li>
	<li>Convert this distance into the cochlear characteristic frequency using a logarithmic function (d(%) = 1 - 156.5 + 82.5 &#215; log(f), with a slope of 1.25 mm/octave of frequency, where d is the normalized distance from the cochlear apex in percent, f is the frequency in kHz), as previously described. Thus frequency range in a corresponding area of the basilar membrane on each cochlear turn can be acquired.</li>
</ol>
4.&#160;Immunofluorescence Staining
<ol>
	<li>After dissection, place each cochlear turn in a separate 2.5 mL centrifuge tube and incubate cochlear turns in 10% goat serum/PBS/0.1% Triton X-100 for 1 h at RT on a rotator.</li>
	<li>Remove the above blocking/permeabilization solution from each tube using a 200 &#956;L pipette tip under a dissection microscope and incubate the specimens with primary antibodies diluted in 5% goat serum/PBS/0.1% Triton X-100 overnight at&#160; 4 &#176;C on a rotator. 
	&#160;NOTE: For immunolabeling of cochlear synaptic ribbons, use the presynaptic marker mouse anti-carboxyl-terminal binding protein 2 IgG1 (CtBP2, labeling the B domain of the RIBEYE scaffolding protein, 1:400) and the postsynaptic marker mouse anti-glutamate receptor 2 IgG2a (GluR2, labeling a subunit of the &#945;-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid or AMPA receptor, 1:200).</li>
	<li>Rinse three times for 5 min with 0.1 M cold PBS to remove residual primary antibodies and incubate the specimens with secondary antibodies diluted in 5% goat serum/PBS/0.1% Triton X-100 at RT for 2&#8210;3 h in darkness on a rotator. 
	&#160;NOTE: Prepare appropriate secondary antibody mixtures using goat anti-mouse Alexa Fluor 568 (IgG1, 1:500) and goat anti-mouse Alexa Fluor 488 (IgG2a, 1:500), which are complementary to the primary antibodies used in step 4.2. To improve labeling efficiency for synaptic ribbons, we recommend selecting specific secondary antibodies. Some labs extend incubation with secondary antibodies to increase GluR2 immunolabeling.</li>
	<li>Rinse three times for 5 min with 0.1 M PBS to remove residual secondary antibodies and transfer the specimens from 2.5 mL centrifuge tubes to 35 mm plates containing 0.1 M PBS.</li>
	<li>Place a drop of mounting medium containing 4&#8217;,6-diamidino-2-phenylindole (DAPI) onto the slide and transfer the specimens from PBS to the mounting medium. Place one edge of a coverslip on the slide and release to let the coverslip fall gently. 
	&#160;NOTE: To ensure that the hair cells face upward and that no folding or twisting of cochlear specimens occurs during the procedure, mount cochlear specimens under a stereo dissection microscope.</li>
	<li>Place the slides in a slide box at 4 &#176;C overnight to let slides dry and then image under a laser confocal microscope.</li>
</ol>
5. Morphological Evaluation of Cochlear Ribbon Synapses
<ol>
	<li>Image slides using a confocal microscope with three lasers&#8212;a 405 nm UV diode, a 488 nm argon laser, and a 561 nm diode-pumped solid-state (DPSS) laser to excite DAPI (Excitation spectrum 409&#8211;464 nm), Alexa Fluor 488 (Excitation spectrum 496&#8211;549 nm) and Alexa Fluor 568 (Excitation spectrum 573&#8211;631 nm), respectively.</li>
	<li>Acquire confocal z-stacks over a distance of 8 &#956;m from each cochlear turn using a 63x high-resolution oil immersion lens. 
	&#160;&#8203;NOTE: Once defined, all parameters for digitizing photomicrographs should be saved and applied uniformly to all slides.</li>
	<li>For synaptic punctum counts, set the z-stacks (0.3 &#956;m step size) to span the entire length of inner hair cells (IHCs), thereby ensuring that all synaptic puncta can be imaged.</li>
	<li>Merge the images containing puncta in a z-stack to obtain the z-axis projection, and import to the image-processing software.</li>
	<li>Divide synaptic total counts in each z-stack at specific frequency regions by the number of IHCs (equal to the DAPI nuclear manual counts) to calculate the number of synaptic puncta for each IHC. At each specific frequency region, average all synaptic puncta in three images of different microscopic fields containing 9&#8211;11 IHCs.
	<ol>
		<li>Outline the region of interests (ROIs) including the basolateral regions of each IHC using freehand selections button. Use the measure function for automatic quantification of puncta, and the watershed function to distinguish between closely adjacent spots.</li>
		<li>After each automated counting, perform visual inspections with manual corrections to ensure puncta counting is reliable. 
		&#160;NOTE: Experimenters should remain blinded as to whether the slide is from the apex, middle, or basal turn of the cochlea.</li>
	</ol>
	</li>
	<li>Visually assess synaptic structure and distribution to manually isolate individual IHCs from their neighbors by the Pencil Tool (M) to better visualize the cytoskeletal architecture and synaptic localization.</li>
	<li>To inspect the juxtaposition of presynaptic ribbons (CtBP2) and postsynaptic receptor patches (GluR2), extract the voxel space around the ribbon with the Rectangular Marquee Tool and isolate the individual ribbon by Crop. Through clicking Image &#62; Image Size, acquire a thumbnail array of these miniature projections, which can then be used to identify paired synapses (appeared as closely juxtaposed pairs of CtBP2-positive and GluR2-positive puncta) versus orphan ribbons (lacking postsynaptic glutamate receptor patches) (Figure 2). 
	&#160;NOTE: Normal cochlear synapses appear as combined immunolabeling of the presynaptic ribbon within the hair cell (anti-CtBP2) and the postsynaptic glutamate receptor patch on the auditory nerve terminal (anti-GluR2). Some labs use confocal projections in conjunction with 3D modeling to quantify synaptic patch size or volume. Prior to significant loss of ribbon synapses, ribbons exhibiting changes in size or without paired glutamate receptor patches are likely indicative of synaptic dysfunction.</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>Ketamine hydrochloride</td>
			<td>Gutian Pharmaceutical Co., Ltd., Fujian, China</td>
			<td>H35020148</td>
			<td>100 mg/kg</td>
		</tr>
		<tr>
			<td>Xylazine hydrochloride</td>
			<td>Sigma-Aldrich, St. Louis, MO, USA</td>
			<td>X-1251</td>
			<td>10 mg/kg</td>
		</tr>
		<tr>
			<td>TDT physiology apparatus</td>
			<td>Tucker-Davis Technologies, Alachua, FL, USA</td>
			<td>Auditory Physiology System III</td>
			<td></td>
		</tr>
		<tr>
			<td>SigGen/BioSig software</td>
			<td>Tucker-Davis Technologies, Alachua, FL, USA</td>
			<td>Auditory Physiology System III</td>
			<td></td>
		</tr>
		<tr>
			<td>Electric Pad</td>
			<td>Pet Fun</td>
			<td>11072931136</td>
			<td></td>
		</tr>
		<tr>
			<td>Dumont forceps 3#</td>
			<td>Fine Science Tools, North Vancouver, B.C., Canada</td>
			<td>0203-3-PO</td>
			<td></td>
		</tr>
		<tr>
			<td>Dumont forceps 5#</td>
			<td>Fine Science Tools, North Vancouver, B.C., Canada</td>
			<td>0209-5-PO</td>
			<td></td>
		</tr>
		<tr>
			<td>Stereo dissection microscope</td>
			<td>Nikon Corp., Tokyo, Japan</td>
			<td>SMZ1270</td>
			<td></td>
		</tr>
		<tr>
			<td>Goat serum</td>
			<td>ZSGB-BIO, Beijing,China</td>
			<td>ZLI-9021</td>
			<td></td>
		</tr>
		<tr>
			<td>Anti-glutamate receptor 2, extracellular, clone 6C4</td>
			<td>Millipore Corp., Billerica, MA, USA</td>
			<td>MAB397</td>
			<td>mouse</td>
		</tr>
		<tr>
			<td>Purified Mouse Anti-CtBP2</td>
			<td>BD Biosciences, Billerica, MA, USA</td>
			<td>612044</td>
			<td>mouse</td>
		</tr>
		<tr>
			<td>Alexa Fluor 568 goat anti-mouse IgG1antibody</td>
			<td>Thermo Fisher Scientific Inc., Waltham, MA, USA</td>
			<td>A21124</td>
			<td>goat</td>
		</tr>
		<tr>
			<td>Alexa Fluor 488 goat anti-mouse IgG2a antibody</td>
			<td>Thermo Fisher Scientific Inc., Waltham, MA, USA</td>
			<td>A21131</td>
			<td>goat</td>
		</tr>
		<tr>
			<td>Mounting medium containing DAPI</td>
			<td>ZSGB-BIO, Beijing,China</td>
			<td>ZLI-9557</td>
			<td></td>
		</tr>
		<tr>
			<td>Confocal fluorescent microscopy</td>
			<td>Leica Microsystems, Wetzlar, Germany</td>
			<td>TCS SP8 II</td>
			<td></td>
		</tr>
		<tr>
			<td>Image Pro Plus software</td>
			<td>Media Cybernetics, Bethesda, MD, USA</td>
			<td>version 6.0</td>
			<td></td>
		</tr>
		<tr>
			<td>Professional diagnostic pocket otoscope</td>
			<td>Lude Medical Apparatus and Instruments Trade Co., Ltd., Shanghai,China</td>
			<td>HS-OT10</td>
			<td></td>
		</tr>
		<tr>
			<td>Needle electrode</td>
			<td>Friendship Medical Electronics Co., Ltd., Xi&#39;an,China</td>
			<td>1029</td>
			<td>20 mm, 28 G</td>
		</tr>
		<tr>
			<td>Closed-field speaker</td>
			<td>Tucker-Davis Technologies, Alachua, FL, USA</td>
			<td>CF1</td>
			<td></td>
		</tr>
	</tbody>
</table>

Source: Yu, S., et al. <a href="https://app.jove.com/v/59189">Morphological and Functional Evaluation of Ribbon Synapses at Specific Frequency Regions of the Mouse Cochlea.</a> J. Vis. Exp. (2019).
This video demonstrates a method for evaluating ribbon synapses in specific regions of the mouse cochlea. It utilizes immunostaining and confocal imaging techniques to identify functional synapses across different frequency regions in each cochlear turn.

<img alt="Figure 1" src="/files/ftp_upload/22945/22945_Figure1.jpg" /> 
Figure 1: Cochlear frequency localization in mice. (A) A representative image of the full explanted cochlea, which has been dissected out of the temporal bone under a stereo dissection microscope. (B) The mouse cochlea is divided into apical, middle, and basal turns, where the cochlear lateral wall is removed. Red circles on the fragments of the ...

All procedures involving animal handling have been performed in accordance with the institute&#39;s IRB guidelines.
1. Animal Selection

	For all ...

Begin with tubes containing pre-treated mouse cochlear turns with a permeabilizing agent and a blocking agent that prevent non-specific interactions.
Each turn detects different sound frequencies and contains hair cells that convert sound into electrical signals. These signals are transmitted via neurotransmitters in ribbon synapses to the auditory nerve.
Remove the solution and add primary antibodies that interact with proteins in hair and nerve cells at the ribbon synapses, then wash.
Incubate with secondary antibodies tagged with red and green fluorophores, which bind to their primary antibodies.
Wash to remove unbound secondary antibodies.
Place the specimen on a glass slide with a mounting medium containing nuclear dye to stain nuclei blue.
Mount the coverslip. Dry it, then use a confocal microscope to image each segment at various depths.
Ribbon synapses appear as closely positioned red and green puncta.
Count these functional puncta in each turn to correlate their response to sound frequency.

16 次观看. 小鼠耳蜗特定频率区域的带状突触评估

视频: 小鼠耳蜗特定频率区域的带状突触评估 - 实验

Whole Mount Dissection and Immunofluorescence of the Adult Mouse Cochlea

The organ of Corti, housed in the cochlea of the inner ear, contains mechanosensory hair cells and surrounding supporting cells which are organized in a spiral shape and have a tonotopic gradient for sound detection. The mouse cochlea is approximately 6 mm long and often divided into three turns (apex, middle, and base) for analysis. To investigate cell loss, cell division, or mosaic gene expression, the whole mount or surface preparation of the cochlea is useful. This dissection method allows visualization of all cells within the organ of Corti when combined with immunostaining and confocal microscopy to image cells at different planes in the z-axis. Multiple optical cross-sections can also be obtained from these z-stack images. In addition, the whole mount dissection method can be used for scanning electron microscopy, although a different fixation method is needed. Here, we present a method to isolate the organ of Corti as three intact cochlear turns (apex, middle, and base). This method can be used for mice ranging from one week of age through adulthood and differs from the technique used for neonatal samples where calcification of the cochlea is incomplete. A slightly modified version can be used for dissection of the rat cochlea. We also demonstrate a procedure for immunostaining with fluorescently tagged antibodies.

We present a method to isolate the adult organ of Corti as three intact cochlear turns (apex, middle, and base). We also demonstrate a procedure for immunostaining with fluorescently tagged antibodies. Together these techniques allow the study of hair cells, supporting cells, and other cell types found in the cochlea.

全山解剖和成年小鼠耳蜗的免疫

The organ of Corti, housed in the cochlea of the inner ear, contains mechanosensory hair cells and surrounding supporting cells which are organized in a ...

科研

JoVE Journal

神经科学

Neonatal Murine Cochlear Explant Technique as an In Vitro Screening Tool in Hearing Research

While there have been remarkable advances in hearing research over the past few decades, there is still no cure for Sensorineural Hearing Loss (SNHL), a condition that typically involves damage to or loss of the delicate mechanosensory structures of the inner ear. Sophisticated in vitro and ex vivo assays have emerged in recent years, enabling the screening of an increasing number of potentially therapeutic compounds while minimizing resources and accelerating efforts to develop cures for SNHL. Though homogenous cultures of certain cell types continue to play an important role in current research, many scientists now rely on more complex organotypic cultures of murine inner ears, also known as cochlear explants. The preservation of organized cellular structures within the inner ear facilitates the in situ evaluation of various components of the cochlear infrastructure, including inner and outer hair cells, spiral ganglion neurons, neurites, and supporting cells. Here we present the preparation, culture, treatment, and immunostaining of neonatal murine cochlear explants. The careful preparation of these explants facilitates the identification of mechanisms that contribute to SNHL and constitutes a valuable tool for the hearing research community.

Neonatal Murine Cochlear Explant Technique as an In Vitro Screening Tool in Hearing Research

The goal of this protocol is to demonstrate the preparation, culture, treatment, and immunostaining of neonatal murine cochlear explants. The technique can be utilized as an in vitro screening tool in hearing research.

新生儿鼠耳蜗外科手术技术<em&gt;体外</em&gt;听力研究筛选工具

While there have been remarkable advances in hearing research over the past few decades, there is still no cure for Sensorineural Hearing Loss (SNHL), a ...

医学

Cochlear Surface Preparation in the Adult Mouse

Auditory processing in the cochlea depends on the integrity of the mechanosensory hair cells. Over a lifetime, hearing loss can be acquired from numerous etiologies such as exposure to excessive noise, the use of ototoxic medications, bacterial or viral ear infections, head injuries, and the aging process. Loss of sensory hair cells is a common pathological feature of the varieties of acquired hearing loss. Additionally, the inner hair cell synapse can be damaged by mild insults. Therefore, surface preparations of cochlear epithelia, in combination with immunolabeling techniques and confocal imagery, are a very useful tool for the investigation of cochlear pathologies, including losses of ribbon synapses and sensory hair cells, changes in protein levels in hair cells and supporting cells, hair cell regeneration, and determination of report gene expression (i.e., GFP) for verification of successful transduction and identification of transduced cell types. The cochlea, a bony spiral-shaped structure in the inner ear, holds the auditory sensory end organ, the organ of Corti (OC). Sensory hair cells and surrounding supporting cells in the OC are contained in the cochlear duct and rest on the basilar membrane, organized in a tonotopic fashion with high-frequency detection occurring in the base and low-frequency in the apex. With the availability of molecular and genetic information and the ability to manipulate genes by knockout and knock-in techniques, mice have been widely used in biological research, including in hearing science. However, the adult mouse cochlea is miniscule, and the cochlear epithelium is encapsulated in a bony labyrinth, making microdissection difficult. Although dissection techniques have been developed and used in many laboratories, this modified microdissection method using cell and tissue adhesive is easier and more convenient. It can be used in all types of adult mouse cochleae following decalcification.

This article presents a modified cochlear surface preparation method that requires decalcification and use of a cell and tissue adhesive to adhere the pieces of cochlear epithelia to 10 mm round cover slips for immunohistochemistry in adult mouse cochleae.

成年小鼠中的科利耳表面制备

Auditory processing in the cochlea depends on the integrity of the mechanosensory hair cells. Over a lifetime, hearing loss can be acquired from numerous ...

Evaluation of Ribbon Synapses at Specific Frequency Regions of Mouse Cochlea

成績單

Evaluation of Ribbon Synapses at Specific Frequency Regions of Mouse Cochlea