eoe sub articles

EoE Sub Articles

All procedures involving sample collection have been performed in accordance with the institute&#39;s IRB guidelines.
1. Electrophysiological Recording Setup&#160;
<ol>
	<li>Pin the mouse external ear (pinna) skin to the PDMS-lined base of a recording chamber with fine insect pins around the edges (~6-8 per ear), placing the cleaned nerves at the base of the ear near two suction electrodes&#160;&#8211; one for recording (to take the nerve) and the other an indifferent electrode (to provide the neutral signal to a differential amplifier).</li>
	<li>For the recording electrode, carefully match the aperture and internal diameter of the opening to the combined thickness of the two nerves, so they fit as snugly as possible and for as great a length as possible.</li>
	<li>Draw the nerves into the electrode by gentle suction from a 2 ml&#160;syringe attached to the other end with silicone rubber tubing. Ensure the nerves are straight, not folded or doubled up.</li>
	<li>Develop a high electrical resistance/impedance fit by using stronger suction to draw connective tissue or adipose tissue to form a plug that tightly seals the aperture around the nerve.</li>
	<li>Fill the other (indifferent) electrode with saline by suction if necessary (it may be filled by capillary action).</li>
	<li>Place identical recording wires (silver or platinum) into the internal bore of the recording electrodes to contact the saline and the nerve (recording) or narrowed, fire-polished end (indifferent) of the electrode. Each electrode is soldered individually to different cores of two-core screened cable. Place the bath (ground) electrode (Ag/AgCl pellet) into the bath and ground it to the screen of the two-core cable connected to the recording electrodes.</li>
	<li>Feed the electrical activity from the two electrodes into the separate channels of a differential amplifier, filter (band-passed 0.2-2 kHz), and view on an oscilloscope screen. Check that channel A (recording) and channel B (indifferent) electrical noise levels look similar. At this stage it may not be possible to see the normal spontaneous action potentials in channel A before the two electrodes are balanced.</li>
	<li>Redress any differences in background noise between electrodes by increasing the impedance of the recording (channel A) or indifferent (channel B) electrodes. Do this by sucking areolar (adipose) connective tissue further into either electrode and/or applying greater suction force on the 50 ml&#160;syringe.
	<ol>
		<li>Once &#39;balanced&#39; in this way, switch back to differential (A-B) recording and look for spontaneous action potentials (APs) in the trace or when stroking hairs at the margin of the pinna. If no activity (spiking) is seen, re-check the tight fit of the nerve in the recording electrode and the areolar connective tissue in the indifferent electrode&#160;&#8211; usually, the tighter (higher resistance) the seal and the more equal the impedance in the two electrodes, the better. With practice, this will achieve a good quality (&#62;2:1) signal:noise ratio.</li>
	</ol>
	</li>
	<li>Record the electroneurogram via a lab interface and electrophysiology software running on a computer. An audio output of spiking is very useful and can be achieved by feeding the neurogram through an audio amplifier and associated audio speaker. Adjust the threshold to be just above the baseline noise (identified by the absence of white-noise &#39;hiss&#39;).</li>
	<li>To increase drug or fluorescent styryl dye access to the lanceolate endings, carefully peel away the sub-dermal adipose layer near the pinna margin, opening a window of ~5 mm x 5 mm, exposing the dermis and base of the follicles (Figure 1A,&#160;B).</li>
	<li>Pin back a fold of ~1 mm of adipose-cleared ear skin at the leading margin (at the level of the window just produced, if applicable), leaving a clear saline-filled gap between the apposed skin layers. Gently stroke the hairs protruding along the folded edge with a pin or grounded fine forceps, without touching the skin, to locate the area of maximal AP output on the oscilloscope and the distinctive &#39;clicks&#39; and &#39;pops&#39; in the audio output.</li>
</ol>
2. Recording Stimulus-evoked Action Potentials
<ol>
	<li>Position the mechanical stimulation probe&#160;&#8211; a fire-polished 10 cm borosilicate microelectrode glass attached to a ceramic piezo-electric actuator&#160;&#8211; so movement is parallel with the skin fold. Place the tip about 0.5-1 mm from the skin fold, so it touches the hairs but not the skin. Verify effective stimulation by slowly moving the probe tip manually to deflect the hairs and observe/listen to the spiking.</li>
	<li>Use the software to drive mechanical stimulation of 1-3 hairs (e.g.&#160;3 sec at 5 Hz sinusoids, every 10 sec. Probe displacement 200-500 &#181;m), and record the stimulation-evoked responses in the nerves.</li>
	<li>Give several identical mechanical stimulation trains at 10 sec intervals. Optimize the probe position for repeatability, then reduce frequency of stimulation according to experimental protocol (e.g.&#160;drop repeat rate from 10 sec to 30 sec).</li>
	<li>Use the software to discriminate AP-like activity,&#160;e.g.,&#160;using a simple threshold set to ~2x the high-frequency noise amplitude and ~25% of the largest APs.</li>
	<li>Count the APs crossing the threshold as &#39;events&#39;, quantifying the frequency and characteristics of the APs produced.</li>
</ol>
3. Recording Stimulus-evoked Firing Combined with N-(3-triethylammoniumpropyl)-4-(4-(dibutylamino) styryl) Pyridinium Dibromide Labeling
<ol>
	<li>To examine the effects of styryl dyes on stimulus-evoked afferent firing and terminal labeling, add the appropriate concentration of a styryl dye of choice to the bathing solution and continue with the electrical recording.</li>
	<li>After the required exposure time (usually at least 30 min), prepare the preparation for viewing the follicles. Unfold the skin flap by removing the retaining pins, and expose the cleared dermal area to reveal the terminal labeling.</li>
	<li>Wash away external dye with dye-free saline, making 3 complete changes of saline.</li>
	<li>Incubate in the final change of gassed dye-free saline for 10-15 min to allow the most persistent dye contamination to leach from exposed/external membranes.</li>
	<li>Remove non-internalized dye remaining on membranes with a sequestering agent (sulfobutylated beta-cyclodextrin, 1 mM, 5 min) in saline.</li>
	<li>Transfer the recording chamber to the stage of an upright epifluorescence microscope and engage the chamber with the stage/slide movement mechanism.</li>
	<li>Illuminate the preparation with excitation light appropriate for the styryl dye. Use a 10X or 25X fluorescence microscope objective to observe the follicle labeling (Figure 1).</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>PDMS - Sylgard 184</td>
			<td>Dow Corning</td>
			<td></td>
			<td>Flexible, inert, translucent solid silicone polymer.</td>
		</tr>
		<tr>
			<td>No. 3 Dumont forceps</td>
			<td>Fine Science Tools</td>
			<td>11231-20</td>
			<td></td>
		</tr>
		<tr>
			<td>Austerlitz Insect pins</td>
			<td>Fine Science Tools</td>
			<td>26002-10</td>
			<td>Very fine pins to attach pinna preparation securely to the PDMS with minimal damage.</td>
		</tr>
		<tr>
			<td>AC Differential Preamplifier</td>
			<td>Digitimer</td>
			<td>Neurolog NL104A</td>
			<td>Amplifying the size of the incoming afferent electroneurogram. Differential recording minimises the extraneous electrical noise and baseline drift.&#160;</td>
		</tr>
		<tr>
			<td>High/Low-pass Filter</td>
			<td>Digitimer</td>
			<td>Neurolog NL125</td>
			<td>Signal conditioning, by reducing extraneous electrical noise to ensure best signal to noise ratio.</td>
		</tr>
		<tr>
			<td>Spike Trigger</td>
			<td>Digitimer</td>
			<td>Neurolog NL201</td>
			<td>Sets the event detector threshold and displays it on the oscilloscope. This shows the action potential detection efficacy.&#160;</td>
		</tr>
		<tr>
			<td>Audio Amplifier &#38; speakers</td>
			<td>Digitimer</td>
			<td>Neurolog NL120S</td>
			<td>Useful audio monitoring for the presencec of electrical firing of the sensory endings while adjusting the mechanical stimulation preparation down the microscope&#160;</td>
		</tr>
		<tr>
			<td>Oscilloscope</td>
			<td>Digitimer</td>
			<td>PM3380A</td>
			<td>We use this old model but any standard oscilloscope will suffice.</td>
		</tr>
		<tr>
			<td>Piezo electroceramic&#160; wafer</td>
			<td>Morgan Electroceramics, Southampton UK</td>
			<td>PZT507</td>
			<td>Electrophysiology/computer interface</td>
		</tr>
		<tr>
			<td>Piezo electroceramic&#160; powersupply</td>
			<td>Home made</td>
			<td></td>
			<td>0-200V DC output to drive the ceramic wafer displacement, with variable electronic control of output via recording/stimulation software and computer interface. We use Spike2 software and 1401micro computer interface.</td>
		</tr>
		<tr>
			<td>Electrophysiology Software</td>
			<td>Cambridge Electronic Design (CED)</td>
			<td>Spike2 v7</td>
			<td>Electrophysiology recording, stimulation and data analysis software</td>
		</tr>
		<tr>
			<td>Laboratory interface</td>
			<td>Cambridge Electronic Design (CED)</td>
			<td>1401 micro</td>
			<td>Electrophysiology interface, between the amplifier/filters and the computer. It inputs the electroneurogram and also drives the electroceramic movement.</td>
		</tr>
		<tr>
			<td>FM1-43/Synaptogreen C4</td>
			<td>Biotium/Cambridge Bioscience</td>
			<td>BT70020</td>
			<td>Fluorescent membrane probe that reversibly partitions into the outer leaflet of cell membranes. Used predominantly for monitoring vesicle membrane endo-/exocytosis.</td>
		</tr>
		<tr>
			<td>Advasep 7</td>
			<td>Biotium/Cambridge Bioscience</td>
			<td>BT70029</td>
			<td>A sulfonated b-cyclodextrin derivative that chelates FM1-43 (&#38; other styryl pyridinium dyes) out of the exposed membranes, leaving internalised dye to be seen more clearly by lowering the background labelling/fluorescence.</td>
		</tr>
		<tr>
			<td>Retiga Exi Fast 1394</td>
			<td>Qimaging</td>
			<td></td>
			<td>Monochrome, cooled CCD camera - basic model</td>
		</tr>
		<tr>
			<td>Volocity 3D Image Analysis Software</td>
			<td>Perkin Elmer</td>
			<td>Volocity 6.3</td>
			<td>Image capture and analysis software.</td>
		</tr>
	</tbody>
</table>

combined recording of mechanically stimulated afferent output and nerve terminal labelling in mouse hair follicles

Source: Bewick, G. et al., <a href="https://appjove.unicartagenaproxy.elogim.com/v/53854">Combined Recording of Mechanically Stimulated Afferent Output and Nerve Terminal Labelling in Mouse Hair Follicle Lanceolate Endings.</a> J. Vis. Exp. (2016).
This video demonstrates the combined recording of mechanically stimulated afferent output and nerve terminal labeling in the hair follicles of a mouse pinna. It outlines the steps involved in the mechanical stimulation of hair follicle nerve terminals before and after exposure to a fluorescent membrane dye, electrophysiology recording of the generated action potentials, and visualization of the nerve terminal labeling in the hair follicles.

<img alt="Figure 1" src="/files/ftp_upload/22758/22758_Figure1.jpg" /> 
Figure 1: Electrophysiological Recording Arrangement and N-(3-triethylammoniumpropyl)-4-(4-(dibutylamino) styryl) Pyridinium Dibromide Labeling of Hair Follicle Afferent Lanceolate endings.&#160;(A) A pinna preparation set up for an electrophysiological experiment showing the pinna orientation, the location of the nerves, the recording electrodes and the exposed area of follicle ...

Combined Recording of Mechanically Stimulated Afferent Output and Nerve Terminal Labelling in Mouse Hair Follicles

All procedures involving sample collection have been performed in accordance with the institute&#39;s IRB guidelines.
1. Electrophysiological Recording ...

Begin with a dissected mouse pinna, or outer ear, with its connected nerves exposed.
Insert the nerve intended for recording into the recording electrode.
Remove the fat layer near the pinna margin to expose the hair follicle base, then fold the skin to expose the hairs for stimulation.
Position a mechanical stimulation probe to touch and deflect the hairs.
This stimulation activates sensory nerve endings, opens mechanically-gated ion channels, allows positive ion influx, and generates action potentials.
The action potentials propagate through these endings to the nerve being recorded. Visualize the signal.
Next, add a fluorescent dye and continue hair stimulation.
The dye binds to the stimulated neuronal membranes and is internalized via endocytosis without affecting neuronal activity.
Post-stimulation, wash to remove unbound dye.
Add a sequestering agent to remove the non-internalized membrane-bound dye.
Using fluorescence microscopy, visualize the staining in the hair follicles to identify mechanically stimulated nerve endings.

combined-recording-mechanically-stimulated-afferent-output-nerve

Universidad de Cartagena UDEC

Research

JoVE Encyclopedia of Experiments

Neuroscience

Neurophysiology

Stimulation and Modulation Techniques

23 ビュー. 出典:Bewick, G. et al., Combined Recording of Mechanically Stimulated Afferent Output and Nerve Terminal Labelling in Mouse Hair Follicle Lanceolate Endings. J. Vis. Exp. (2016). このビデオは、マウスの耳介の毛包における機械的に刺激された求心性出力と神経終末標識の複合記録を示しています。蛍光膜色素への曝露前後の毛包神経終末の機械的刺激、生成された活動電位の電気生理学的記録、および毛包の神経...

ビデオ: マウス毛包における機械的に刺激された求心性出力と神経終末標識の複合記録 - 概念

Electrophysiology on Isolated Brainstem-spinal Cord Preparations from Newborn Rodents Allows Neural Respiratory Network Output Recording

While it is well known that the central respiratory drive is located in the brainstem, several aspects of its basic function, development, and response to stimuli remain to be fully understood. To overcome the difficulty of accessing the brainstem in the whole animal, isolation of the brainstem and part of the spinal cord is performed. This preparation is maintained in artificial cerebro-spinal fluid where gases, concentrations, and temperature are controlled and monitored. The output signal from the respiratory network is recorded by a suction electrode placed on the fourth ventral root. In this manner, stimuli can be directly applied onto the brainstem, and the effect can be recorded directly. The signal recorded is linked to the inspiratory signal sent to the diaphragm via the phrenic nerve, and can be described as bursts (around 8 bursts per minute). Analysis of these bursts (frequency, amplitude, length, and area under the curve) allows precise characterization of the stimulus effect on the respiratory network. The main limitation of this method is the viability of the preparation beyond the early post-natal stages. Thus, this method greatly focuses on the study of the whole network without the peripheral inputs in the newborn rat.

The central respiratory drive is located in the brainstem. Spontaneous respiratory motor output from an isolated brainstem-spinal cord is recorded by placing an electrode on the fourth ventral root. This experimental approach is valuable for pharmacological investigations or the assessment of respiratory challenges and genetic manipulations on rhythmic motor behavior.

新生児げっ歯類から単離された脳幹・脊髄調製物の電気生理学は、ニューラルネットワーク呼吸器の出力の記録を可能にします

While it is well known that the central respiratory drive is located in the brainstem, several aspects of its basic function, development, and response to ...

JoVE Journal

神経科学

Optical Monitoring of Living Nerve Terminal Labeling in Hair Follicle Lanceolate Endings of the Ex Vivo Mouse Ear Skin

A novel dissection and recording technique is described for optical monitoring staining and de-staining of lanceolate terminals surrounding hair follicles in the skin of the mouse pinna. The preparation is simple and relatively fast, reliably yielding extensive regions of multiple labeled units of living nerve terminals to study uptake and release of styryl pyridinium dyes extensively used in studies of vesicle recycling. Subdividing the preparations before labeling allows test vs. control comparisons in the same ear from a single individual. Helpful tips are given for improving the quality of the preparation, the labeling and the imaging parameters. This new system is suitable for assaying pharmacologically and mechanically-induced uptake and release of these vital dyes in lanceolate terminals in both wild-type and genetically modified animals. Examples of modulatory influences on labeling intensity are given.

Optical Monitoring of Living Nerve Terminal Labeling in Hair Follicle Lanceolate Endings of the Ex Vivo Mouse Ear Skin

Here we describe a novel preparation for imaging live lanceolate sensory terminals of palisade endings that innervate mouse ear skin hair follicles during staining and destaining with styryl pyridinium dyes.

の毛包披針形語尾に神経末端標識リビングの光監視<em&gt; ex vivoで</em&gt;マウスの耳皮膚

A novel dissection and recording technique is described for optical monitoring staining and de-staining of lanceolate terminals surrounding hair follicles ...

In Vitro Recording of Mesenteric Afferent Nerve Activity in Mouse Jejunal and Colonic Segments

Afferent nerves not only convey information concerning normal physiology, but also signal disturbed homeostasis and pathophysiological processes of the different organ systems from the periphery towards the central nervous system. As such, the increased activity or &#39;sensitization&#39; of mesenteric afferent nerves has been allocated an important role in the pathophysiology of visceral hypersensitivity and abdominal pain syndromes.
Mesenteric afferent nerve activity can be measured in vitro in an isolated intestinal segment that is mounted in a purpose-built organ bath and from which the splanchnic nerve is isolated, allowing researchers to directly assess nerve activity adjacent to the gastrointestinal segment. Activity can be recorded at baseline in standardized conditions, during distension of the segment or following the addition of pharmacological compounds delivered intraluminally or serosally. This technique allows the researcher to easily study the effect of drugs targeting the peripheral nervous system in control specimens; besides, it provides crucial information on how neuronal activity is altered during disease. It should be noted however that measuring afferent neuronal firing activity only constitutes one relay station in the complex neuronal signaling cascade, and researchers should bear in mind not to overlook neuronal activity at other levels (e.g., dorsal root ganglia, spinal cord or central nervous system) in order to fully elucidate the complex neuronal physiology in health and disease.
Commonly used applications include the study of neuronal activity in response to the administration of lipopolysaccharide, and the study of afferent nerve activity in animal models of irritable bowel syndrome. In a more translational approach, the isolated mouse intestinal segment can be exposed to colonic supernatants from IBS patients. Furthermore, a modification of this technique has been recently shown to be applicable in human colonic specimens.

In Vitro Recording of Mesenteric Afferent Nerve Activity in Mouse Jejunal and Colonic Segments

Mesenteric afferent nerves convey information from the gastrointestinal tract towards the brain regarding normal homeostasis as well as pathophysiology. Gastrointestinal afferent nerve activity can be assessed by mounting isolated intestinal segments with attached afferent nerves into an organ bath, isolating the nerve, and assessing basal as well as stimulated activity.

マウス空腸および結腸セグメントにおける腸間膜求心性神経活動のin vitro記録で

Afferent nerves not only convey information concerning normal physiology, but also signal disturbed homeostasis and pathophysiological processes of the ...