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All procedures involving animal models have been reviewed by the local institutional animal care committee and the JoVE veterinary review board.

1. Slice Culture Preparation

<ol>
	<li>Prepare mouse organotypic hippocampal slice cultures using postnatal 6- to 7-day old mice of either sex.
	<ol>
		<li>Prepare dissection media for organotypic slice culture consisting of (in mM): 238 sucrose, 2.5 KCl, 1 CaCl2, 4 MgCl2, 26 NaHCO3, 1 NaH2PO4, and 11 glucose in deionized water, then gas with 5% CO2/95% O2&#160;to a pH of 7.4.</li>
		<li>Prepare organotypic slice culture media consisting of: 78.8% (v/v) Minimum Essential Medium Eagle, 20% (v/v) horse serum, 17.9 mM NaHCO3, 26.6 mM glucose, 2 M CaCl2, 2 M MgSO4, 30 mM HEPES, insulin (1 &#181;g/mL), and 0.06 mM ascorbic acid, pH adjusted to 7.3. Adjust the osmolarity to 310&#8211;330 osmol using an osmometer.</li>
		<li>Dissect hippocampi out from the whole brain by using two spatulas, and slice (400 &#181;m) using a tissue chopper. Separate slices by using two forceps and transfer to 30 mm cell culture inserts in a 6-well plate filled with culture media (950 &#181;L) underneath the inserts.</li>
	</ol>
	</li>
	<li>Store organotypic slice cultures in a tissue culture incubator (35&#176;C, 5% CO2) and change the slice culture media every two days.</li>
</ol>

2. Plasmid Preparation

<ol>
	<li>Prepare the plasmid for the gene of interest.
	<ol>
		<li>Subclone enhanced green fluorescent protein (EGFP) gene into a pCAG vector.</li>
		<li>Purify pCAG-EGFP plasmid with an endotoxin-free purification kit and dissolve in an internal solution that consists of diethyl pyrocarbonate-treated water containing 140 mM K-methanesulfonate, 0.2 mM EGTA, 2 mM MgCl2, and 10 mM HEPES, adjusted to pH 7.3 with KOH (plasmid concentration: 0.1 &#181;g/&#181;L).</li>
	</ol>
	</li>
</ol>

3. Glass Pipette Preparation

<ol>
	<li>Pull borosilicate glass pipettes (4.5&#8211;8 M&#937;) on a micropipette puller (Figure 1A). 
	NOTE: The glass pipettes used for whole-cell patch clamp recordings are ideal for electroporation.</li>
	<li>Bake glass pipettes overnight at 200&#176;C to sterilize.</li>
	<li>Check the size of the pipette tip under a dissection microscope to approximate the electrical resistance.
	<ol>
		<li>Optional: Verify pipette resistance by attaching the pipette to the electroporation electrode and use the micromanipulator to maneuver the pipette tip into filter-sterilized artificial cerebrospinal fluid (aCSF) containing (in mM): 119 NaCl, 2.5 KCl, 0.5 CaCl2, 5 MgCl2, 26 NaHCO3, 1 NaH2PO4&#160;and 11 glucose in deionized water, gassed with 5% CO2/95% O2&#160;to a pH of 7.4. Confirm the actual resistance using the readout on the electroporator. 
		NOTE: The sharper the pipette tip, the larger the electrical resistance. The pipette resistance should be below 10 M&#937;. Glass pipettes with high pipette resistance (Figure 1B) often clog at the tip during repeated electroporation.</li>
	</ol>
	</li>
</ol>

4. Electroporation Rig Setup

<ol>
	<li>Install the electroporator to a standard whole-cell electrophysiology rig, equipped with an upright microscope mounted on a shifting table with a micromanipulator and peristaltic pump.</li>
	<li>Install the headstage of the electroporator onto a micromanipulator and connect a pair of speakers to the electroporator. Connect the electroporator to a foot pedal which can be used to send a pulse when ready. 
	NOTE: The speakers emit a tone when turned on, which is an indicator of the electrical resistance at the electrode. This makes it possible to determine relative changes in resistance without pulling attention away from the procedure.</li>
</ol>

5. Electroporation Preparation

<ol>
	<li>Transfer slice culture inserts from 6-well plates to 3 cm Petri dishes loaded with 900 &#181;L of culture media and store in a tabletop CO2&#160;incubator until ready to perform electroporation.
	<ol>
		<li>Preincubate fresh culture inserts with slice culture media (1 mL) for at least 30 min in a 3.5 cm Petri dish to culture slices after electroporation.</li>
	</ol>
	</li>
	<li>Clean and prepare the rig for electroporation.
	<ol>
		<li>Perfuse the lines with 10% bleach for 5 min to sterilize the tubing and chamber prior to beginning the experiment for the day.</li>
		<li>Perfuse the lines with deionized autoclaved water for at least 30 min to rinse completely.</li>
		<li>Perfuse the lines with filter-sterilized aCSF containing 0.001 mM tetrodotoxin (TTX). 
		NOTE: TTX minimizes cellular toxicity and death due to overexcitation of interneurons.</li>
	</ol>
	</li>
	<li>Set the electroporator&#8217;s pulse parameters: amplitude of &#8211;5 V, square pulse, train of 500 ms, frequency of 50 Hz, and a pulse width of 500 &#181;s.</li>
	<li>Fill glass pipette with 5 &#181;L of plasmid-containing internal solution.
	<ol>
		<li>Remove any trapped air bubbles from the pipette tip by flicking and gently tapping the tip multiple times.</li>
		<li>Check the tip for damage by visualizing it under a dissection microscope or by repeating step 3.3.1 to check the pipette resistance. 
		NOTE: If the tip is damaged, the glass pipette must be discarded, and this step must be repeated with a new glass pipette previously prepared in step 3.</li>
	</ol>
	</li>
	<li>Securely attach the pipette tip to the electrode and turn the speakers on. Record the readout (the pipette&#8217;s resistance) of the electroporator when the tip has made contact with&#160;the aCSF medium.</li>
	<li>Cut the culture insert membrane using a sharp blade and isolate one slice culture. Carefully transfer the slice culture to the electroporation chamber by using sharp angled forceps and fix its position with a slice anchor.
	<ol>
		<li>Do not keep the slice culture outside of the incubator for more than 30 min at a time to prevent side effects such as changes in neuronal health or function.</li>
	</ol>
	</li>
</ol>

6. Electroporate Cells of Interest

<ol>
	<li>Apply positive pressure to the pipette with mouth or by using a 1 mL syringe (0.2&#8211;0.5 mL pressure) attached to the tubing.</li>
	<li>Use the micromanipulator&#8217;s 3-dimensional knob controls to maneuver the pipette tip near the surface of the slice culture.</li>
	<li>Choose a target cell and approach it, keeping the positive pressure applied until a dimple forms on the cell surface, visible on the microscope.</li>
	<li>Perform pressure cycles.
	<ol>
		<li>Quickly apply mild negative pressure by mouth so that a loose seal forms between the pipette tip and the plasma membrane, indicated visually by the membrane going up into the pipette tip somewhat. Observe an increase (~2.5x the initial resistance) in pipette resistance by listening for an increase in tone coming from the speakers. Quickly re-apply positive pressure so that the dimple re-forms.</li>
		<li>Immediately complete at least two more pressure cycles without pausing, then hold negative pressure for 1 s. 
		NOTE: Pausing between cycles, applying too much pressure, or holding the negative pressure for too long can cause significant cell damage and possibly cause the cell to die during electroporation.</li>
	</ol>
	</li>
	<li>Quickly pulse the electroporator once using the foot pedal when the tone from the speakers reaches a stable apex in pitch, indicating peak electrical resistance. Do not wait at the peak resistance for more than 1 s before sending the pulse. 
	NOTE: We have observed no off-target electroporation when using this protocol. Only the cells in contact with the glass pipette during pressure cycles were transfected. Positioning the pipette near other neurons does not result in gene transfection.</li>
	<li>Gently retract the pipette approximately 100 &#181;m from the cell without applying pressure.</li>
	<li>Re-apply positive pressure, verifying that the resistance is similar to the recorded readout in step 5.5, then approach the next cell.
	<ol>
		<li>Remove potential clogs, indicated visually or by a significantly increased (&#62;15% higher) pipette resistance after electroporation, by applying positive pressure. 
		NOTE: If there is no visible clog and the resistance is still significantly higher, discard the pipette and use a new one. On an average, a pipette can be used for up to 20 electroporation events if the user is careful.</li>
	</ol>
	</li>
</ol>
After electroporation, transfer the slice culture onto a fresh culture insert, and incubate at 35&#176;C in the incubator for up to 3 days.

<table><tbody><tr><td>&lt;strong&gt;Plasmid preparation&lt;/strong&gt;</td><td></td><td></td><td></td></tr><tr><td>Plasmid Purification Kit</td><td>Qiagen</td><td>12362</td><td></td></tr><tr><td>&lt;strong&gt;Organotypic slice culture preparation&lt;/strong&gt;</td><td></td><td></td><td></td></tr><tr><td>6-well plates</td><td>GREINER BIO-ONE</td><td>657160</td><td></td></tr><tr><td>Dumont #5/45 Forceps</td><td>FST</td><td>#5/45</td><td>Angled dissection forceps for organotypic slice culture preparation</td></tr><tr><td>Flask Filter Unit</td><td>Millipore</td><td>SCHVU02RE</td><td>Filtration and storage of culture media</td></tr><tr><td>Incubator</td><td>Binder</td><td>BD C150-UL</td><td></td></tr><tr><td>McIlwain Tissue Chopper</td><td>TED PELLA, INC.</td><td>10180</td><td>Tissue chopper for organotypic slice culture preparation</td></tr><tr><td>Millicell Cell Culture Insert, 30 mm</td><td>Millipore</td><td>PIHP03050</td><td>Organotypic slice culture inserts</td></tr><tr><td>Osmometer</td><td>Precision Systems</td><td>OSMETTE II</td><td></td></tr><tr><td>PTFE coated spatulas</td><td>Cole-Parmer</td><td>SK-06369-11</td><td></td></tr><tr><td>Scissors</td><td>FST</td><td>14958-09</td><td></td></tr><tr><td>Stereo Microscope</td><td>Olympus</td><td>SZ61</td><td></td></tr><tr><td>Sterile Vacuum Filtration System</td><td>Millipore</td><td>SCGPT01RE</td><td>Filtration and storage of aCSF</td></tr><tr><td>&lt;strong&gt;Electrode preparation&lt;/strong&gt;</td><td></td><td></td><td></td></tr><tr><td>Capillary Glasses</td><td>Warner Instruments</td><td>640796</td><td></td></tr><tr><td>Micropipetter Puller</td><td>Sutter Instrument</td><td>P-1000</td><td>Puller</td></tr><tr><td>Oven</td><td>Binder</td><td>BD (E2)</td><td></td></tr><tr><td>Puller Filament</td><td>Sutter Instrument</td><td>FB330B</td><td>Puller</td></tr><tr><td>3.5 mm Falcon Petri Dishes</td><td>BD Falcon</td><td>353001</td><td></td></tr><tr><td>Airtable</td><td>TMC</td><td>63-7512E</td><td></td></tr><tr><td>CCD camera</td><td>Q Imaging</td><td>Retiga-2000DC</td><td>Camera</td></tr><tr><td>Electroporation System</td><td>Molecular Devices</td><td>Axoporator 800A</td><td>Electroporator</td></tr><tr><td>Fluorescence Illumination System</td><td>Prior</td><td>Lumen 200</td><td></td></tr><tr><td>Manipulator</td><td>Sutter Instrument</td><td>MPC-385</td><td>Manipulator</td></tr><tr><td>Metamorph software</td><td>Molecular Devices</td><td></td><td>Image acquisition</td></tr><tr><td>Peristaltic Pump</td><td>Rainin</td><td>Dynamax, RP-2</td><td>Perfusion pump</td></tr><tr><td>Shifting Table</td><td>Luigs &amp;amp; Neuman</td><td>240 XY</td><td></td></tr><tr><td>Speaker</td><td>Unknown</td><td></td><td>Speakers connected to the electroporator</td></tr><tr><td>Stereo Microscope</td><td>Olympus</td><td>SZ30</td><td></td></tr><tr><td>Table Top Incubator</td><td>Thermo Scientific</td><td>MIDI 40</td><td></td></tr><tr><td>Upright Microscope</td><td>Olympus</td><td>BX61WI</td><td></td></tr></tbody></table>

single cell electroporation in organotypic brain slice cultures: an in vitro technique to deliver plasmids inside targeted neurons in brain hippocampal slices

Source: Keener, D. G. et al. <a href="https://www.jove.com/video/61662" target="_blank">Single-Cell Electroporation Across Different Organotypic Slice Culture of Mouse Hippocampal Excitatory and Class-Specific Inhibitory Neurons.</a> J. Vis. Exp. (2020)
This video demonstrates the protocol for single-cell electroporation of genes in both excitatory and inhibitory neurons across a range of in vitro hippocampal slice cultures. The technique is useful to examine specific molecular and physiological functions of neurons, including cell autonomous mechanisms and transsynaptic protein interactions.

<img alt="Figure 1" src="/files/ftp_upload/20697/20697_Figure1.jpg" /> 
Figure 1: Two representative glass pipette images. (A) Display lower resistance (6.5 M&#937;) pipettes, used in this protocol, and (B) higher resistance (10.4 M&#937;) pipettes typical for electroporation protocols.
<img alt="Figure 1" src="/files/ftp_upload/20697/20697_Figure2.jpg" /> 
Fig...

Single Cell Electroporation in Organotypic Brain Slice Cultures: An In Vitro Technique to Deliver Plasmids Inside Targeted Neurons in Brain Hippocampal Slices

Source: Keener, D. G. et al. Single-Cell Electroporation Across Different Organotypic Slice Culture of Mouse Hippocampal Excitatory and Class-Specific ...

Begin electroporation by taking a glass pipette containing the desired plasmid solution. Attach it to a micropipette holder fitted with a silver wire electrode, ensuring that the electrode is inserted into the micropipette. Take an electroporation chamber containing an ultrathin hippocampal section submerged in artificial cerebrospinal fluid.
Dip the ground electrode into the fluid present in the chamber for subsequent electroporation. Lower the pipette tip into the electroporation chamber and record the baseline resistance. Use a microscope to position the pipette tip near the target cell. Once the pipette is in contact with the neuronal membrane, its resistance increases sharply.
Apply positive air pressure to create a small invagination in the neuronal membrane. Rapidly apply mild suction to push the membrane up, creating a loose seal between the pipette tip and the membrane. Repeat this process a few more times to condition the membrane and avoid cell lysis.
After conditioning, apply strong suction to form a tight seal with a membrane called gigaohm seal. Use electric pulses to form transient pores in the sealed area of the membrane. These openings facilitate the entry of plasmids inside the targeted neuron. Post electroporation, the pores reseal, entrapping plasmids inside the neuron.

single-cell-electroporation-organotypic-brain-slice-cultures-an-vitro

Research

JoVE Encyclopedia of Experiments

Cancer Research

Cancers of the Nervous System

In vitro studies

1.2K Views. Źródło: Keener, D. G. et al. Elektroporacja jednokomórkowa w różnych organotypowych kulturach warstwowych mysich neuronów pobudzających hipokampa i specyficznych dla klasy neuronów hamujących. J. Vis. Exp. (2020) Ten film demonstruje protokół elektroporacji pojedynczych komórek genów zarówno w neuronach pobudzających, jak i hamujących w różnych kulturach in vitro w warstwach hipokampa. Technika ta jest przydatna do badania specyficznych funkcji molekularnych i fizjologicznych...

Video: Elektroporacja pojedynczych komórek w organotypowych kulturach wycinków mózgu: technika in vitro dostarczania plazmidów do docelowych neuronów w wycinkach hipokampa mózgu - Concept

Organotypic Hippocampal Slice Cultures

The hippocampus, a component of the limbic system, plays important roles in long-term memory and spatial navigation 1. Hippocampal neurons can modify the strength of their connections after brief periods of strong activation. This phenomenon, known as long-term potentiation (LTP) can last for hours or days and has become the best candidate mechanism for learning and memory 2. In addition, the well defined anatomy and connectivity of the hippocampus 3 has made it a classical model system to study synaptic transmission and synaptic plasticity4.
As our understanding of the physiology of hippocampal synapses grew and molecular players became identified, a need to manipulate synaptic proteins became imperative. Organotypic hippocampal cultures offer the possibility for easy gene manipulation and precise pharmacological intervention but maintain synaptic organization that is critical to understanding synapse function in a more naturalistic context than routine culture dissociated neurons methods.
Here we present a method to prepare and culture hippocampal slices that can be easily adapted to other brain regions. This method allows easy access to the slices for genetic manipulation using different approaches like viral infection 5,6 or biolistics 7. In addition, slices can be easily recovered for biochemical assays 8, or transferred to microscopes for imaging 9 or electrophysiological experiments 10.

We describe a method to prepare organotypic hippocampal slices that can be easily adapted to other brain regions. Brain slices are laid on porous membranes and culture media is allowed to form an interface. This method preserves the gross architecture of the hippocampus for up to 2 weeks in culture.

The hippocampus, a component of the limbic system, plays important roles in long-term memory and spatial navigation 1. Hippocampal neurons can modify the ...

JoVE Journal

Neuroscience

Organotypic Hippocampal Slice Cultures As a Model to Study Neuroprotection and Invasiveness of Tumor Cells

In organotypic hippocampal slice cultures (OHSC), the morphological and functional characteristics of both neurons and glial cells are well preserved. This model is suitable for addressing different research questions that involve studies on neuroprotection, electrophysiological experiments on neurons, neuronal networks or tumor invasion. The hippocampal architecture and neuronal activity in multisynaptic circuits are well conserved in OHSC, even though the slicing procedure itself initially lesions and leads to formation of a glial scar. The scar formation alters presumably the mechanical properties and diffusive behavior of small molecules, etc. Slices allow the monitoring of time dependent processes after brain injury without animal surgery, and studies on interactions between various brain-derived cell types, namely astrocytes, microglia and neurons under both physiological and pathological conditions. An ambivalent aspect of this model is the absence of blood flow and immune blood cells. During the progression of the neuronal injury, migrating immune cells from the blood play an important role. As those cells are missing in slices, the intrinsic processes in the culture may be observed without external interference. Moreover, in OHSC the composition of the medium-external environment is precisely controlled. A further advantage of this method is the lower number of sacrificed animals compared to standard preparations. Several OHSC can be obtained from one animal making simultaneous studies with multiple treatments in one animal possible. For these reasons, OHSC are well suited to analyze the effects of new protective therapeutics after tissue damage or during tumor invasion. 
The protocol presented here describes a preparation method of OHSC that allows generating highly reproducible, well preserved slices that can be used for a variety of experimental research, like neuroprotection or tumor invasion studies.

Organotypic hippocampal slice cultures (OHSC) represent an in vitro model that simulates the in vivo situation very well. Here we describe a vibratome-based improved slicing protocol to obtain high quality slices for use in assessing the neuroprotective potential of novel substances or the biological behavior of tumor cells.

In organotypic hippocampal slice cultures (OHSC), the morphological and functional characteristics of both neurons and glial cells are well preserved. ...

Single-Cell Electroporation across Different Organotypic Slice Culture of Mouse Hippocampal Excitatory and Class-Specific Inhibitory Neurons

Electroporation has established itself as a critical method for transferring specific genes into cells to understand their function. Here, we describe a single-cell electroporation technique that maximizes the efficiency (~80%) of in vitro gene transfection in excitatory and class-specific inhibitory neurons in mouse organotypic hippocampal slice culture. Using large glass electrodes, tetrodotoxin-containing artificial cerebrospinal fluid and mild electrical pulses, we delivered a gene of interest into cultured hippocampal CA1 pyramidal neurons and inhibitory interneurons. Moreover, electroporation could be carried out in cultured hippocampal slices up to 21 days in vitro with no reduction in transfection efficiency, allowing for the study of varying slice culture developmental stages. With interest growing in examining the molecular functions of genes across a diverse range of cell types, our method demonstrates a reliable and straightforward approach to in vitro gene transfection in mouse brain tissue that can be performed with existing electrophysiology equipment and techniques.

Presented here is a protocol for single-cell electroporation that can deliver genes in both excitatory and inhibitory neurons across a range of in vitro hippocampal slice culture ages. Our approach provides precise and efficient expression of genes in individual cells, which can be used to examine cell-autonomous and intercellular functions.

Electroporation has established itself as a critical method for transferring specific genes into cells to understand their function. Here, we describe a ...

Single Cell Electroporation in Organotypic Brain Slice Cultures: An In Vitro Technique to Deliver Plasmids Inside Targeted Neurons in Brain Hippocampal Slices

Transkrypcja

Single Cell Electroporation in Organotypic Brain Slice Cultures: An In Vitro Technique to Deliver Plasmids Inside Targeted Neurons in Brain Hippocampal Slices