eoe sub articles

EoE Sub Articles

1. Two-photon Injury and Confocal Imaging
<ol>
	<li>Microscope setup 
	NOTE: A confocal laser scanning microscope with a two-photon laser was used for this experiment, but other systems with an equivalent setup will also suffice. The two-photon laser (930 nm) was used for delivering injury and an Argon laser (488 nm) was used for confocal imaging of GFP.
	<ol>
		<li>At the beginning of each session, turn on the two-photon laser and/or the confocal laser(s) and the microscope. Then, open the imaging software.</li>
		<li>For two-photon injury, set up the following parameters for imaging GFP with the two-photon laser at 930 nm (1,950 mW).
		<ol>
			<li>Select line scan mode. Open up the pinhole all the way. Increase laser intensity to ~20% (390 mW).</li>
			<li>Select 512 x 512 as the frame scan. Use maximal scanning speed (typically with the pixel dwell time at 0.77 &#181;s). Ensure that the average number is 1 and bit depth is 8 bits.</li>
			<li>Set gain to ~750 and the offset to 0.</li>
			<li>Save this pre-set experimental protocol as 2P GFP 930 Ablation, allowing for easy reuse in future experiments.</li>
		</ol>
		</li>
		<li>For confocal imaging, set up the following parameters for imaging GFP with the Argon laser at 488 nm:
		<ol>
			<li>Select the Acquisition tab and then Z-stack.</li>
			<li>Under &#34;Laser&#34;, turn on the power for the 488 nm Argon laser.</li>
			<li>Go to Channels, select the 488 mm laser, and increase the laser power to 5-10%. For the pinhole, use the 1-2 airy unit (AU). Adjust the gain to 650.</li>
			<li>In Acquisition Mode, select 1024 x 1024 as the frame scan, use the maximum scan speed, an average number of 2, and bit depth of 8 Bit.</li>
			<li>Save this pre-set experimental protocol as GFP(green fluorescent protein) Imaging.</li>
		</ol>
		</li>
	</ol>
	</li>
	<li>Larvae anesthesia with diethyl ether and mounting
	<ol>
		<li>In a fume hood, place a 60-mm glass dish in a 15-cm plastic Petri dish. Fold and lay a piece of tissue paper at the bottom of the glass dish, then place a grape juice agar plate on the tissue. Add diethyl ether into the glass dish, to the point where the tissue paper is soaked and there is a layer of liquid ether remaining in the dish. Keep the lid on at all times.</li>
		<li>Prepare a glass slide with one drop of halocarbon 27 oil in the center. Add 4 spots of vacuum grease onto the four corners of the slide, to later support the coverslip.</li>
		<li>Use forceps to pick up a cleaned larva and place it on the agar plate in the 60-mm glass dish. Cover the glass dish with its lid and wait until the larva stops moving. For PNS injury/imaging, take out the larva as soon as its tail stops twitching. For the CNS, wait until the entire larva becomes motionless, especially the head segments. 
		NOTE: The timing of ether exposure is critical. See Discussion.</li>
		<li>Carefully pick up the anesthetized larva and place it head-upright into the drop of halocarbon oil on the slide. Add a coverslip on top of the slide. Use gentle pressure to push down on the coverslip, until it touches the larva (Figure 1A).</li>
		<li>Adjust the larva&#39;s position by gently pushing the coverslip towards the left or right to roll the larva, so that the neuron/axon/dendrite of interest is on the top and closest to the microscope lens.</li>
		<li>For PNS injury, mount the larva dorsal side up, so that both the tracheas are visible. Then roll the larva ~30 degrees to the left for injuring class III da neuron axons (Figure 1B and 1C), 90 degrees for injuring class IV da neuron axons (Figure 1B and 1E), or ~30 degrees for injuring class IV da neuron dendrites.</li>
		<li>For CNS injury, position the larva to be perfectly ventral side up, so that the region of interest is closest to the microscope lens in the z-plane.</li>
	</ol>
	</li>
	<li>Injury by two-photon laser
	<ol>
		<li>Place the slide with the larva under the microscope and secure it in place with the slide holder on the stage. Use the 10X (0.3 NA) objective to find the larva.</li>
		<li>Add 1 drop of objective oil onto the coverslip, switch to the 40X (1.3 NA) objective and adjust the focus.</li>
		<li>Switch to the scanning mode and reuse the experimental protocol 2P GFP 930 Ablation. Make sure the pinhole is opened all the way. 
		NOTE: The configuration needs to be optimized based on individual systems.</li>
		<li>Start the Live mode to locate the region of interest (ROI), and fine-tune the settings to achieve good image quality with the appropriate zoom. 
		NOTE: The purpose of this step is to find the neuron/axon/dendrite to injure, rather than taking the best quality image. Therefore, use the minimal settings sufficient to visualize the target area, in order to avoid overexposure or photobleaching.</li>
		<li>Stop Live scan, so that the Crop button will become available. Let the still image serve as the roadmap. Select the Crop function and adjust the scan window to focus on the target to be injured.</li>
		<li>Reduce the ROI to be the size of the prospective site of injury. For example, just cover the width of an axon or a dendrite, to ensure the precision of the injury and reduce damage to neighboring tissues. If desired, zoom in on the ROI before cropping, allowing for more precise injury.</li>
		<li>Open a new imaging window. Reduce the scan speed and increase laser intensity. Determine the increase in laser intensity based on the tissue fluorescence signal scanned in Live mode.</li>
		<li>Typically, set the two-photon laser intensity starting from 25% for PNS injury and 50-100% for VNC injury. For PNS axon injury, ensure that the laser intensity is ~480 mW and pixel dwell time is 8.19 &#956;s. For the VNC axon injury, ensure that the laser intensity and pixel dwell time are usually 965-1930 mW and 8.19-32.77 &#956;s, respectively.</li>
		<li>Start Continuous scan. Leave the cursor hovering over the Continuous button. Keep a close eye on the image and stop the scan as soon as a drastic increase in fluorescence is observed. 
		NOTE: The appearance of the fluorescence spike is due to auto-fluorescence at the injury site.</li>
		<li>Switch back to the Live mode by reusing the settings. Find the region of interest that was just targeted by adjusting the focus. 
		NOTE: A good indication of successful injury is the appearance of a small crater, ring-like structure, or localized debris right at the injury site.</li>
		<li>Move to the next neuron and repeat from Step 1.3.5, to injure multiple neurons in a single animal. Or repeat Step 3.3.5 while gradually increasing the power and/or reducing scan speed if the initial injury was insufficient. 
		NOTE: In the case that the laser power is too high, a large damaged area will be visible in the post-injury live scan image. Too much injury may cause the death of the larva.</li>
		<li>Recover the larva by carefully removing the coverslip and transferring the injured larva onto a new plate with yeast paste. Ditch several caves on the agar plate with forceps; alternatively, make an island of agar in the plate instead of using the whole plate, to reduce the possibility of the larva crawling out of the plate.</li>
		<li>Put the plate in a 60-mm Petri dish with wet tissue (soaked with 0.5% propionic acid solution) and culture at room temperature or 25&#176;C. 
		NOTE: The larva will remain in the larval stage for approximately an extra day at room temperature (22&#176;C) compared to at 25&#176;C.</li>
	</ol>
	</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>Diethyl ether, ACS reagent, anhydrous</td>
			<td>Acros Organics</td>
			<td>AC615080010</td>
			<td></td>
		</tr>
		<tr>
			<td>Halocarbon 27 Oil</td>
			<td>Genesee Scientific</td>
			<td>59-133</td>
			<td></td>
		</tr>
		<tr>
			<td>Phosphate buffered saline (PBS), 20x Concentrate, pH 7.5, supplier # E703-1L</td>
			<td>VWR</td>
			<td>97062-948</td>
			<td></td>
		</tr>
		<tr>
			<td>Agar powder, Alfa Aesar, 500GM</td>
			<td>VWR</td>
			<td>AAA10752-36</td>
			<td></td>
		</tr>
		<tr>
			<td>Grape juice</td>
			<td>Welch&#39;s</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Ethanol 95% (Reagent Alcohol 95%)</td>
			<td>VWR</td>
			<td>64-17-5</td>
			<td></td>
		</tr>
		<tr>
			<td>Acetic acid</td>
			<td>Sigma-Aldrich</td>
			<td>A6283</td>
			<td></td>
		</tr>
		<tr>
			<td>Propionic Acid</td>
			<td>J.T.Baker</td>
			<td>U33007</td>
			<td></td>
		</tr>
		<tr>
			<td>Cover Glasses: Rectangles</td>
			<td>Fisher Scientific</td>
			<td>12-544-D</td>
			<td>50 mm X 22 mm</td>
		</tr>
		<tr>
			<td>Zeiss LSM 880 laser scanning microscope</td>
			<td>Zeiss</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Zen software</td>
			<td>Zeiss</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Chameleon Ultra II</td>
			<td>Coherent</td>
			<td></td>
			<td></td>
		</tr>
	</tbody>
</table>

inducing targeted neuronal injury using a high-power laser in a drosophila larva

Source: Li, D., Li, F., et al. <a href="https://app.jove.com/v/57557">A Drosophila in vivo injury model for studying neuroregeneration in the peripheral and central nervous system.</a> J. Vis. Exp. (2018)
This video demonstrates a method for inducing targeted neuronal injury in Drosophila larvae using a high-power laser. After positioning the larva under a microscope, a low-power laser scans for fluorescent neurons, and then the laser power is increased to induce localized damage. The injury is confirmed by increased fluorescence and a crater at the injury site.

<img alt="Figure 1" src="/files/ftp_upload/23117/23117_Figure1v2.jpg" /> 
Figure 1: Da neuron axon regeneration in the periphery displays class specificity. (A and B) Schematic drawing showing the position of the larvae. (C) Schematic drawing of class III da neurons. (D) Axons of the class III da neurons ddaF, labeled with 19-12-Gal4, UAS-CD4-tdGFP, repo-Gal80/+, fail to regrow. (E) Schematic drawing of class IV da neurons. (F) Axons of the class IV da neurons v&#39;...

Inducing Targeted Neuronal Injury Using a High-Power Laser in a Drosophila Larva

Source: Li, D., Li, F., et al. A Drosophila in vivo injury model for studying neuroregeneration in the peripheral and central nervous system. J. Vis. Exp. ...

Place an anesthetized Drosophila larva with its head-up on an oil drop on a glass slide containing vacuum grease spots.
Position a coverslip and gently press it to make contact with the larva.
Adjust the larva to expose the region containing the target neurons expressing fluorescent proteins.
Secure the slide on a two-photon microscope.
Use a low-power laser to minimize damage and scan the larva to locate the region with the fluorescent target neurons.
Next, adjust the scan window to focus on the target region containing axons, a type of neuronal projections.
Now, reduce the scan rate and increase the laser power.
The high-power laser will strike the targeted axons, generating localized heat that damages them and enhances fluorescence around the injury site.
Finally, switch back to low-power laser mode. The presence of small crater, ring-like structures at the injury site confirms successful neuronal injury.

inducing-targeted-neuronal-injury-using-high-power-laser-drosophila

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JoVE Encyclopedia of Experiments

Neuroscience

Neuropathology

Trauma

25 Görüntüleme. Source: Li, D., Li, F., et al. A Drosophila in vivo injury model for studying neuroregeneration in the peripheral and central nervous system. J. Vis. Exp. (2018) This video demonstrates a method for inducing targeted neuronal injury in Drosophila larvae using a high-power laser. After positioning the larva under a microscope, a low-power laser scans for fluorescent neurons, and then the laser power is increased to induce localized damage. The injury is confirmed by increased fluorescence and a ...

Video: Inducing Targeted Neuronal Injury Using a High-Power Laser in a Drosophila Larva - Kavram

Facial Nerve Surgery in the Rat Model to Study Axonal Inhibition and Regeneration

This protocol describes consistent and reproducible methods to study axonal regeneration and inhibition in a rat facial nerve injury model. The facial nerve can be manipulated along its entire length, from its intracranial segment to its extratemporal course. There are three primary types of nerve injury used for the experimental study of regenerative properties: nerve crush, transection, and nerve gap. The range of possible interventions is vast, including surgical manipulation of the nerve, delivery of neuroactive reagents or cells, and either central or end-organ manipulations. Advantages of this model for studying nerve regeneration include simplicity, reproducibility, interspecies consistency, reliable survival rates of the rat, and an increased anatomic size relative to murine models. Its limitations involve a more limited genetic manipulation versus the mouse model and the superlative regenerative capability of the rat, such that the facial nerve scientist must carefully assess time points for recovery and whether to translate results to higher animals and human studies. The rat model for facial nerve injury allows for functional, electrophysiological, and histomorphometric parameters for the interpretation and comparison of nerve regeneration. It thereby boasts tremendous potential toward furthering the understanding and treatment of the devastating consequences of facial nerve injury in human patients.

This protocol describes a reproducible approach to facial nerve surgery in the rat model, including descriptions of various inducible patterns of injury.

Aksonal İnhibisyon ve Rejenerasyon Çalışması için Sıçan Modelinde Yüz Sinir Cerrahisi

This protocol describes consistent and reproducible methods to study axonal regeneration and inhibition in a rat facial nerve injury model. The facial ...

JoVE Journal

Nörobilim

Laser-Induced Brain Injury in the Motor Cortex of Rats

A common technique for inducing stroke in experimental rodent models involves the transient (often denoted as MCAO-t) or permanent (designated as MCAO-p) occlusion of the middle cerebral artery (MCA) using a catheter. This generally accepted technique, however, has some limitations, thereby limiting its extensive use. Stroke induction by this method is often characterized by high variability in the localization and size of the ischemic area, periodical occurrences of hemorrhage, and high death rates. Also, the successful completion of any of the transient or permanent procedures requires expertise and often lasts for about 30 minutes. In this protocol, a laser irradiation technique is presented that can serve as an alternative method for inducing and studying brain injury in rodent models.
When compared to rats in the control and MCAO groups, the brain injury by laser induction showed reduced variability in body temperature, infarct volume, brain edema, intracranial hemorrhage, and mortality. Furthermore, the use of a laser-induced injury caused damage to the brain tissues only in the motor cortex unlike in the MCAO experiments where destruction of both the motor cortex and striatal tissues is observed.
Findings from this investigation suggest that laser irradiation could serve as an alternative and effective technique for inducing brain injury in the motor cortex. The method also shortens the time for completing the procedure and does not require expert handlers.

The protocol presented here shows a technique to create a rodent model of brain injury. The method described here uses laser irradiation and targets motor cortex.

Farelerin Motor Korteksinde LazerE Bağlı Beyin Hasarı

A common technique for inducing stroke in experimental rodent models involves the transient (often denoted as MCAO-t) or permanent (designated as MCAO-p) ...

Modified Spared Nerve Injury Surgery Model of Neuropathic Pain in Mice

Spared nerve injury (SNI) is an animal model that mimics the cardinal symptoms of peripheral nerve injury for studying the molecular and cellular mechanism of neuropathic pain in mice and rats. Currently, there are two types of SNI model, one to cut and ligate the common peroneal and the tibial nerves with intact sural nerve, which is defined as SNIs in this study, and another to cut and ligate the common peroneal and the sural nerves with intact tibial nerve, which is defined as SNIt in this study. Because the sural nerve is purely sensory whereas the tibial nerve contains both motor and sensory fibers, the SNIt model has much less motor deficit than the SNIs model. In the traditional SNIt mouse model, the common peroneal and the sural nerves are cut and ligated separately. Here a modified SNIt surgery method is described to damage both common peroneal and sural nerves with only one ligation and one cut with a shorter procedure time, which is easier to perform and reduces the potential risk of stretching the sciatic or tibial nerves, and produces similar mechanical hypersensitivity as the traditional SNIt model.

<meta charset="utf8"></head><body>Farelerde Nöropatik Ağrının Modifiye Edilmiş Korunmuş Sinir Yaralanması Cerrahisi Modeli

The modified surgery is a simplified method for mouse or rat spared nerve injury model that requires only one ligation and one cut to injure both common peroneal and sural nerves.

Inducing Targeted Neuronal Injury Using a High-Power Laser in a Drosophila Larva

TRANSKRIPT

Inducing Targeted Neuronal Injury Using a High-Power Laser in a Drosophila Larva

Aksonal İnhibisyon ve Rejenerasyon Çalışması için Sıçan Modelinde Yüz Sinir Cerrahisi

Farelerin Motor Korteksinde LazerE Bağlı Beyin Hasarı

Farelerde Nöropatik Ağrının Modifiye Edilmiş Korunmuş Sinir Yaralanması Cerrahisi Modeli

Farelerde Nöropatik Ağrının Modifiye Edilmiş Korunmuş Sinir Yaralanması Cerrahisi Modeli