initiating rapid neurite extension and formation functional neuronal connections

Initiating Rapid Neurite Extension and Formation Functional Neuronal Connections

Remove the medium from the upper wells of the microfluidic devices without emptying the wells. Then, add 20 microliters of the concentrated cell solution into the top right well of the microfluidic device, and check in the microscope how cells flow inside the single population microfluidic device.
To plate cells in the multiple populations&#39; device, add 20 microliters of the concentrated cell solution into each of the top wells. Under the microscope, check if the cells are inside the chambers. Afterward, place the devices in the incubator for 15 to 30 minutes to promote cell attachment to the substrate.
After the cells attach to the substrate, add 40 microliters of NBM to the two top wells of the single population device. This will help remove the air bubbles from the microchannels. Add 20 microliters of NBM to the top wells of the multiple populations device, the same wells where the cells were injected. The media should protrude slightly to form a positive meniscus, and give the wells a muffin-top aspect.
One to two days before the microfluidic devices removal, add 2 milliliters of pre-warmed NBM to each sample dish, and flood the chambers. Then, keep the devices in the incubator. Subsequently, use sterile tweezers and a pipette tip to remove the microfluidic devices from the coverslips, leaving a patterned configuration of neurons.
In this procedure, add 40 to 60 microliters of the prepared PDL-coated beads to the cell culture. Then, return the sample to the incubator for one hour to promote the formation of synaptic contacts. Subsequently, install the sample in an experimental setup such that the cells can be assessed from above by two micropipettes and also be accessed optically. In this configuration, a CCD camera is located on the side port of the microscope for image capture. Connect each pipette filled with saline to a 1-milliliter syringe. Then, perfuse the sample with physiological saline solution.
Next, under the microscope, check the gap between the two isolated neuronal populations to ensure that the two populations are not naturally connected. Select a PDL bead that is not attached to the neuron in the field of view. Align the bead with a micropipette tip by focusing on the bead and then on the micropipette.
Subsequently, bring the tip down as close as possible to the bead by monitoring it through the microscope. Then, apply negative pressure to the pipette to pick up the bead, and maintain the negative pressure throughout the experiment.
Now, select a PDL bead attached to a neuron in the field of view, and attach it to the second micropipette using suction. Pull the PDL bead-neuron complex by slowly moving either the micromanipulator or the sample stage at 0.5 micrometers per minute for 1 micrometer, and pause for five minutes to allow neurite initiation.
Pull the PDL bead-neuron complex by slowly moving it laterally at 0.5 micrometers per minute over 2 micrometers. Then, pause for five minutes to allow neurite elongation. After successful initiation and neurite extension for the first 5 micrometers, continuously pull the neurite at 20 micrometers per minute.
To connect the neurons, select a region rich in neurites. Use other beads to gauge the pipette tip height above the coverslip, and lower the PDL bead-neurite complex so that it physically contacts the neurites. Leave the PDL bead-neurite complex in contact with the target neurite while manipulating the second micropipette. Then, lower the second pipette with the second PDL bead on top of the newly formed neurite about 20 micrometers from the first bead, and use the second PDL bead to push the new neurite filament towards the target cell.
Next, hold both beads in place for at least one hour. Verify the absence of focal swelling, a thickening of the neurites contacting the bead with the microscope. During this time, slowly change the medium of the sample from physiological saline to pre-warmed carbon dioxide-equilibrated NBM.
Release the bead from the second pipette by releasing the suction. If the new neurite remains attached, release the first speed as well. Afterward, carefully place the sample back in the incubator to strengthen the neuronal connection for future experiments.

initiating-rapid-neurite-extension-formation-functional-neuronal

Universidad de Cartagena UDEC

Research

JoVE Encyclopedia of Experiments

Neuroscience

Neuronal Culture Techniques

Advanced Neuronal Models

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1.&#160;Standardization of Neuronal Cultures Using Microfluidic Devices: Device Assembly
<ol>
	<li>Select a suitable microfluidic device for the desired experiment. To connect neurons within the same population, use the Neuro Devices (Figure 1), and to connect neurons in different populations, use the Co-Culture Devices (Figure 2).</li>
	<li>Clean and prepare the desired number of sterile coverslips or glass bottom dishes. For best results on plastic surfaces, use 35 mm dishes, on glass, use 25 mm coverslips or 35 mm glass bottom dishes. Select glass thickness based on the imaging system, for instance, 0.15 mm.</li>
	<li>Coat the dishes or coverslips with 0.5-1 mL of 100 &#181;g/mL PDL for 2 h or overnight at room temperature. 
	NOTE: Protocol can be paused here and resumed the following day if desired. Furthemore, dishes can be coated with borate buffer-diluted PDL, Poly-L-Lysine (PLL), laminin or any other cell adhesion molecule.</li>
	<li>Wash the dishes twice with water (do not use phosphate-buffered saline (PBS) as salt crystals may block the channels), remove all the liquid and let it dry in a sterile environment such as a biosafety cabinet for 5-10 min or until the surface is completely dry. 
	NOTE: Be careful to ensure that the coverslips are absolutely dry, as any remaining liquid will interfere with the adherence of the microfluidic systems.</li>
	<li>Place microfluidic devices with patterns facing up under UV light in a sterile environment (biosafety cabinet) for 10 min. Be sure to follow sterile procedures when working in the biosafety cabinet10.</li>
	<li>Using tweezers, place a microfluidic device with a pattern facing down in contact with the clean coverslip/dish. Use the tweezers to softly press the device so that it adheres to the glass. 
	NOTE: The transparency of the adhered region will be visible when looking against the light. Make sure all corners are in contact with the glass. Do this to all microfluidic devices. See Figure 1a.</li>
	<li>To fill the single population device with medium, point the pipette towards the channels and add 50 &#181;L of complete cell medium supplemented with serum-free B-27 (volume ratio 1:50) and 500 &#181;g/mL penicillin/streptomycin/glutamine (collectively called NBM) to the right upper well, and then add another 50 &#181;L to the well lying diagonally to it. Do this for all devices, making sure that the medium flows between wells. Next, add 50 &#181;L of medium to the remaining two wells. See Figure 3a.
	<ol>
		<li>To fill the multiple population device with medium, point the pipette towards the channels and add 30 &#181;L of complete NBM to the right wells, refer to Figure 2a. Do this for all devices, making sure that the medium flows between wells. Next, add 50 &#181;L of medium to the remaining four wells.</li>
	</ol>
	</li>
	<li>Place the devices in a bigger plate with an open dish with autoclaved water (wet chamber) and place in the incubator (37 &#176;C, 5% CO2, and 95% humidity) for 1-2 h while preparing the cell culture. See Figure 3b.</li>
</ol>
2. Plating Neurons in Microfluidic Systems
<ol>
	<li>Following a protocol, obtain dissociated hippocampal or cortical neurons from Sprague Dawley rat embryos (either gender).</li>
	<li>Resuspend embryonic neurons in NBM at a concentration of 1-2 million neurons/mL. Verify cell concentrations in the microscope using a hemocytometer and following reference8. Adjust the cell concentration according to the desired cell density. To increase the chances of obtaining single hippocampal axons per channel, plate 10,000 neurons per device. To have multiple axons in the same channel, plate 60,000 neurons per device. 
	Note: These numbers vary according to the neuronal type used.</li>
	<li>Remove the medium from the microfluidic devices without emptying the wells. Leave approximately 5 &#181;L in each.</li>
	<li>To plate cells in the single population device, add 50 &#181;L of NBM to the lower right well. At this point, the medium flows by itself to fill the other lower well. Add 20 &#181;L of the concentrate cell solution into the top right well of the microfluidic device, as indicated in Figure 1b.
	<ol>
		<li>To plate cells in the multiple population device add 20 &#181;L of the concentrate cell solution into each of the right wells in Figure 2a.</li>
	</ol>
	</li>
	<li>Check in the microscope if cells are inside the chambers and place the devices in the incubator for 15-30 min to promote cell attachment to the substrate.</li>
	<li>Check in the microscope if there are enough cells in the chambers. If more are needed, repeat steps 2.4 and 2.5.</li>
	<li>Add 50 &#181;L of NBM to the 2 top wells of the single population device and 20 &#181;L of NBM into the same well as the cells were injected in the multiple population device. The media protrudes slightly to form a positive meniscus giving the wells a muffin top aspect. Again, see Figure 3a.</li>
	<li>Maintain the cells at 37 &#176;C, 5%CO2, and 95% humidity.</li>
</ol>
3. Maintaining the Neuronal Cultures
<ol>
	<li>Remove NBM (roughly 30 &#181;L with a pipette) from the cells and apply new pre-warmed NBM the day following their introduction to the devices (that is 1 d after step 2).</li>
	<li>Check every 2 days if there is enough medium in each channel. If the muffin top is low just add more medium to the top wells.</li>
	<li>Culture cells for at least 7 d before removal of the microfluidic devices. The cells can survive in these devices for several weeks. Remove the devices 1-2 days before experiments are performed on samples.</li>
</ol>
4.&#160;Removal of Microfluidic Devices
<ol>
	<li>1 - 2 d before removal of microfluidic devices, add 2 mL of NBM prewarmed to 37 &#176;C to each sample dish, flooding the chambers, and maintain the devices in the incubator.</li>
	<li>Use sterile tweezers and one tip to remove the microfluidic devices from the coverslips leaving a patterned configuration of neurons. Use the tip to hold the coverslip in place and the tweezers to clasp the edge of the device at the bottom left corner of the well. Delicately apply torsion, raising the device up with the tweezers so that it peels off the coverslip. See Figure 3c-3d.</li>
	<li>Every 2-3 days, replace half the NBM until the sample is used for experiments.</li>
	<li>Before performing rewiring experiments on the sample, verify that neurites in the single population device channels and the neuronal populations in the multiple population device are isolated by examining the gaps between them in the microscope to ensure there are no filaments linking neuronal populations.</li>
</ol>
5.&#160;Preparing PDL-coated Beads
<ol>
	<li>Add 2 x 50 &#181;L drops of either 4, 10 or 20 &#181;m polystyrene beads diluted in water (1:500) to 1 mL of PDL (100 &#181;g/mL). Leave for at least 2 h at room temperature. 
	NOTE: Protocol can be paused here and resumed the following day.</li>
	<li>Centrifuge the solution at 8,820 x g for 1 min. Carefully remove the supernatant without disturbing the beads accumulated at the bottom of the container.</li>
	<li>Wash the beads twice with 1 mL of sterile 10 mM HEPES pH 8.4 solution.</li>
	<li>Resuspend the PDL-coated beads in 200 mL of 10 mM HEPES pH 8.4 solution.</li>
</ol>
6.&#160;Preparing Micropipettes
<ol>
	<li>Prepare pipettes from glass capillary tubes (1 mm inner diameter, 1.5 mm outer diameter) using a horizontal electrode puller. Adjust settings so the outer tip of the pulled micropipette is ~ 2-5 &#181;m. Before pulling, ensure the glass tubes are clean.</li>
	<li>Fix pipettes to glass slides for storage, and ensure that the tip does not contact the surface of the slide as the tip is fragile. Store at room temperature in a covered container to protect from dust. Use pipettes the same day they are pulled.</li>
</ol>
7.&#160;PDL-bead Adhesion to Neurons
<ol>
	<li>Add 40-60 &#181;L of PDL-coated beads prepared in step 5 to a cell culture prepared in step 4. Center the pipette tip over the neurons, which are faintly visible on the coverslip, and add the beads (See Figure 4).</li>
	<li>Return the sample to the incubator for 1 h to promote the formation of synaptic contacts.</li>
	<li>After the incubation, remove any unadhered beads by gently washing the culture with pre-warmed NBM.</li>
</ol>
8.&#160;Preparing Physiological Saline Solution (for Room Temperature Experiments)
<ol>
	<li>Prepare a physiological saline solution. This is to regulate the cell environment outside the incubator.</li>
	<li>Verify osmolarity and pH levels.</li>
	<li>Continuously infuse solution with O2 to minimize pH fluctuations while conducting experiments.</li>
	<li>Heat to room temperature.</li>
	<li>Set up the perfusion system by inserting one end of a plastic tube (optional dimensions) in an O2-infused physiological solution and fixing the other end to a needle inserted in the sample holder. Place the tubing and solution higher than the sample (See Figure 5).
	<ol>
		<li>Disconnect the tube from the needle and connect it to a syringe. Use the syringe to exert pressure and draw liquid, filling the tube. Seal with a roller clamp and reconnect the needle.</li>
	</ol>
	</li>
</ol>
9.&#160;Bead Micromanipulation
<ol>
	<li>Install the sample in an experimental set-up such that cells can be accessed from above by two micropipettes mounted in micromanipulators and accessed optically below, for instance, with the 40X-phase objective (numerical aperture of 0.6) of an inverted optical microscope. In this configuration, mount a CCD camera for image capture on the side port of the microscope. Connect each pipette to 1 mL syringes via plastic tubing. At this step, replace NBM with a physiological saline solution (1-2 mL) (See Figure 5).</li>
	<li>During experiments, continuously perfused cells with the physiological saline solution prepared in step 8 at a rate of 0.5-1 mL/min.</li>
	<li>Select a PDL bead NOT attached to a neuron in the field of view. Align the bead with a micropipette tip by focusing on the bead and then up to the micropipette. Bring the tip down as close as possible to the bead by monitoring it through the microscope.</li>
	<li>Apply negative pressure with the 1 mL syringe connected to the pipette to pick up the bead. Maintain negative pressure throughout the experiment.</li>
</ol>
10.&#160;Pulling Neurites
<ol>
	<li>Select a PDL bead attached to a neuron in the field of view and attach it to the second micropipette using suction as described in steps 9.3-9.4.</li>
	<li>Pull the PDL-bead-neuron complex slowly (~0.5 &#181;m/min), moving either the micromanipulator or the sample stage by 1 &#181;m and pausing for 5 min to allow neurite initiation.</li>
	<li>Repeat step 10.2 twice. 
	Note: The first 3 &#181;m have to be pulled very slowly to guarantee experimental success, which occurs over 95% of the time.</li>
	<li>Pull the PDL-bead-neuron complex by slowly (~0.5 &#181;m/min) moving either the micromanipulator or the sample stage by 2 &#181;m and pause for 5 min to allow neurite elongation.</li>
	<li>After successful initiation and neurite extension for the first 5 &#181;m, pull the neurite at 20 &#181;m/min over millimeter-scale distances. 
	Note: Pulling can be performed continuously or in steps and at varying rates. See Figure 6b-6c.</li>
</ol>
11. Connecting Neurons
<ol>
	<li>Select a region rich in neurites and lower the PDL-bead-neurite complex so that it physically contacts it. Use other beads to gauge tip height above the coverslip surface. See Figure 6d.</li>
	<li>Leave the PDL-bead-neurite complex in contact with the target neurite while manipulating the second micropipette. Lower the second pipette with the second PDL-bead on top of the newly formed neurite about 20 &#181;m from the first bead. Use the second PDL-bead to push the new neurite filament toward the target cell.</li>
	<li>Hold both beads in place for at least 1 h. Verify the absence of focal swelling, a thickening of the neurites contacting the bead, with the microscope16.</li>
	<li>During this time, use perfusion to slowly change the medium of the sample from physiological saline to pre-warmed, CO2-equilibrated NBM.</li>
	<li>Release the bead from the second pipette by releasing suction. If the new neurite remains attached, release the first bead as well. See Figure 6e .</li>
	<li>Gently remove saline solution and replace with NBM (~2 mL).</li>
	<li>Carefully place the sample back in the incubator to strengthen the neuronal connection for future experiments. This connection is stable for &#62;24</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>Neuro devices&#160;&#160;</td>
			<td>Ananda Devices</td>
			<td></td>
			<td>Commercially available at http:// www.anandadevices.com</td>
		</tr>
		<tr>
			<td>No. 1 Glass Coverslip 25 mm Round&#160;&#160;</td>
			<td>Warner Instruments</td>
			<td>64-0705</td>
			<td></td>
		</tr>
		<tr>
			<td>35 mm cell culture dish, NonPyrogenic, Sterile&#160;&#160;</td>
			<td>Corning Inc</td>
			<td>430165</td>
			<td></td>
		</tr>
		<tr>
			<td>95 mm x 15 mm Petri Dish, Slippable Lid, Sterile Polystyrene&#160;&#160;</td>
			<td>Fisherbrand</td>
			<td>FB0875714G</td>
			<td></td>
		</tr>
		<tr>
			<td>Neurobasal Medium&#160;&#160;</td>
			<td>Life Technologies</td>
			<td>21103-049</td>
			<td>Extracellular solution</td>
		</tr>
		<tr>
			<td>B-27 Supplement (50X), serum free&#160;</td>
			<td>Thermo Fisher Scientific</td>
			<td>17504044</td>
			<td>Extracellular solution</td>
		</tr>
		<tr>
			<td>Pennicilin, Streptomyocin, Glutamine&#160;&#160;</td>
			<td>Thermo Fisher Scientific</td>
			<td>11995-065</td>
			<td>Extracellular solution</td>
		</tr>
		<tr>
			<td>2 - 20 &#956;L Pipettors Aerosol Resistant Tips</td>
			<td>Thermo Fisher Scientific</td>
			<td>2149P</td>
			<td></td>
		</tr>
		<tr>
			<td>Dumont Dumostar Tweezers 11 cm&#160;&#160;</td>
			<td>World Precision Instruments</td>
			<td>500233</td>
			<td></td>
		</tr>
		<tr>
			<td>Dissection tools&#160;</td>
			<td>Braun, Aesculap</td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>Poly-D-lysine Hydrobromide&#160;</td>
			<td>Sigma-Aldrich</td>
			<td>P6407</td>
			<td></td>
		</tr>
		<tr>
			<td>Micro particles based on polystyrene, 10 &#956;m&#160;</td>
			<td>Sigma-Aldrich</td>
			<td>72986</td>
			<td></td>
		</tr>
		<tr>
			<td>Horizontal Pipette Puller&#160;</td>
			<td>Sutter Instruments</td>
			<td>Brown-Flaming P-97</td>
			<td></td>
		</tr>
		<tr>
			<td>Micromanipulators, PCS-5000 Series&#160; MC7600R</td>
			<td>SD Instruments</td>
			<td>MC7600R</td>
			<td></td>
		</tr>
		<tr>
			<td>1 mL Syringe&#160;</td>
			<td>BD Luer-Lok</td>
			<td>309628</td>
			<td></td>
		</tr>
		<tr>
			<td>Inverted Microscope&#160;</td>
			<td>Olympus</td>
			<td>IX71</td>
			<td></td>
		</tr>
		<tr>
			<td>Objective UIS2</td>
			<td>Olympus</td>
			<td>LUCPLFLN 40X</td>
			<td></td>
		</tr>
		<tr>
			<td>CCD Camera&#160;&#160;</td>
			<td>Photometrics</td>
			<td>Cascade II: 512</td>
			<td></td>
		</tr>
	</tbody>
</table>

Source: M. H. Magdesian et al., <a href="https://appjove.unicartagenaproxy.elogim.com/v/55697">Rewiring Neuronal Circuits: A New Method for Fast Neurite Extension and Functional Neuronal Connection,</a> J. Vis. Exp. (2017)
This video demonstrates a technique for the rapid initiation and extension of a neuron and creation of new connections with a target neuron using a microfluidic device and micromanipulation. This could be used for therapies that aim to reconnect neuronal circuits after trauma or in neurodegenerative diseases.

<img alt="Figure 1" src="/files/ftp_upload/22413/22413_Figure1.jpg" /> 
Figure 1: Standardization of Neuronal Cultures using Microfluidic Devices7. (a) Device assembly: when the microfluidic devices are properly assembled on a dry surface all chambers are visible. (b) Cell plating: plate the cells on the top right well and cells should move towards the left well. (c) Cell density: just after plating, check in the mic...

1.&#160;Standardization of Neuronal Cultures Using Microfluidic Devices: Device Assembly

	Select a suitable microfluidic device for the desired ...

Begin by assembling a microfluidic device containing microchannels within a dish coated with lysine.
Seed embryonic neurons with a growth medium into the microfluidic wells, allowing them to flow through the microchannels.
Incubate to facilitate neuronal attachment and growth, forming physically isolated neuronal populations.
Disassemble the setup and place the dish in a micromanipulator chamber with a saline flow to maintain cell viability.
Introduce lysine-coated beads near the neurons, enabling the neurites or cell projections to attach and form bead-neurite complexes.
Using a micromanipulator, apply suction to engage a bead-neurite complex from one channel.
Pull this complex to induce mechanical tension, leading to rapid neurite extension.
Guide this toward another bead-neuron complex and hold it with a second micromanipulator.
Keep both beads in place to facilitate the formation of a neuritic connection.
Release the suction and replace the saline with a culture medium.
Incubate to establish functional connections between neurons, promoting communication through neurotransmitters.

11 次观看. 启动快速神经突延伸和形成功能性神经元连接

视频: 启动快速神经突延伸和形成功能性神经元连接 - 实验

Rapid Neuronal Differentiation of Induced Pluripotent Stem Cells for Measuring Network Activity on Micro-electrode Arrays

Neurons derived from human induced Pluripotent Stem Cells (hiPSCs) provide a promising new tool for studying neurological disorders. In the past decade, many protocols for differentiating hiPSCs into neurons have been developed. However, these protocols are often slow with high variability, low reproducibility, and low efficiency. In addition, the neurons obtained with these protocols are often immature and lack adequate functional activity both at the single-cell and network levels unless the neurons are cultured for several months. Partially due to these limitations, the functional properties of hiPSC-derived neuronal networks are still not well characterized. Here, we adapt a recently published protocol that describes production of human neurons from hiPSCs by forced expression of the transcription factor neurogenin-212. This protocol is rapid (yielding mature neurons within 3 weeks) and efficient, with nearly 100% conversion efficiency of transduced cells (&#62;95% of DAPI-positive cells are MAP2 positive). Furthermore, the protocol yields a homogeneous population of excitatory neurons that would allow the investigation of cell-type specific contributions to neurological disorders. We modified the original protocol by generating stably transduced hiPSC cells, giving us explicit control over the total number of neurons. These cells are then used to generate hiPSC-derived neuronal networks on micro-electrode arrays. In this way, the spontaneous electrophysiological activity of hiPSC-derived neuronal networks can be measured and characterized, while retaining interexperimental consistency in terms of cell density. The presented protocol is broadly applicable, especially for mechanistic and pharmacological studies on human neuronal networks.

We modify and implement a previously published protocol describing the rapid, reproducible, and efficient differentiation of human&#160;induced&#160;Pluripotent Stem Cells (hiPSCs) into excitatory cortical neurons12. Specifically, our modification allows for control of neuronal cell density and use on micro-electrode arrays to measure electrophysiological properties at the network level.

诱导多能干细胞的快速神经元分化有关微电极阵列测量网络活动

Neurons derived from human induced Pluripotent Stem Cells (hiPSCs) provide a promising new tool for studying neurological disorders. In the past decade, ...

科研

JoVE Journal

发育生物学

Mouse Hindbrain Ex Vivo Culture to Study Facial Branchiomotor Neuron Migration

Embryonic neurons are born in the ventricular zone of the brain, but subsequently migrate to new destinations to reach appropriate targets. Deciphering the molecular signals that cooperatively guide neuronal migration in the embryonic brain is therefore important to understand how the complex neural networks form which later support postnatal life. Facial branchiomotor (FBM) neurons in the mouse embryo hindbrain migrate from rhombomere (r) 4 caudally to form the paired facial nuclei in the r6-derived region of the hindbrain. Here we provide a detailed protocol for wholemount ex vivo culture of mouse embryo hindbrains suitable to investigate the signaling pathways that regulate FBM migration. In this method, hindbrains of E11.5 mouse embryos are dissected and cultured in an open book preparation on cell culture inserts for 24 hr. During this time, FBM neurons migrate caudally towards r6 and can be exposed to function-blocking antibodies and small molecules in the culture media or heparin beads loaded with recombinant proteins to examine roles for signaling pathways implicated in guiding neuronal migration.

Mouse Hindbrain Ex Vivo Culture to Study Facial Branchiomotor Neuron Migration

Embryonic neurons are born in the ventricular zone of the neural tube, but migrate to reach appropriate targets. Facial branchiomotor (FBM) neurons are a useful model to study neuronal migration. This protocol describes the wholemount ex vivo culture of mouse embryo hindbrains to investigate mechanisms that regulate FBM migration.

鼠标后脑<em&gt;前体内</em&gt;企业文化来研究面部Branchiomotor神经元迁移

Embryonic neurons are born in the ventricular zone of the brain, but subsequently migrate to new destinations to reach appropriate targets. Deciphering ...

神经科学

The Indirect Neuron-astrocyte Coculture Assay: An In Vitro Set-up for the Detailed Investigation of Neuron-glia Interactions

Proper neuronal development and function is the prerequisite of the developing and the adult brain. However, the mechanisms underlying the highly controlled formation and maintenance of complex neuronal networks are not completely understood thus far. The open questions concerning neurons in health and disease are diverse and reaching from understanding the basic development to investigating human related pathologies, e.g.,&#160;Alzheimer&#39;s disease and&#160;Schizophrenia. The most detailed analysis of neurons can be performed in vitro. However, neurons are demanding cells and need the additional support of astrocytes for their long-term survival. This cellular heterogeneity is in conflict with the aim to dissect the analysis of neurons and astrocytes. We present here a cell-culture assay that allows for the long-term cocultivation of pure primary neurons and astrocytes, which share the same chemically defined medium, while being physically separated. In this setup, the cultures survive for up to four weeks and the assay is suitable for a diversity of investigations concerning neuron-glia interaction.

The Indirect Neuron-astrocyte Coculture Assay: An In Vitro Set-up for the Detailed Investigation of Neuron-glia Interactions

This protocol describes the indirect neuron-astrocyte coculture for compartmentalized analysis of neuron-glia interactions.

Initiating Rapid Neurite Extension and Formation Functional Neuronal Connections

成績單

Initiating Rapid Neurite Extension and Formation Functional Neuronal Connections