testing monosynaptic connections using tetrodotoxin and tetrodotoxin-resistant sodium channels

Testing Monosynaptic Connections Using Tetrodotoxin and Tetrodotoxin-Resistant Sodium Channels

At the rig, immediately start perfusing the preparation with recording saline bubbled with carbogen. Use a gravity-fed saline solution reservoir placed above the microscope stage. To collect the waste saline, use a vacuum line in a two-liter flask.
Next, load the patch pipette with four microliters of internal recording solution, and attach the pipette to a micromanipulator. Then, zero the amplifier&#39;s offset and set the amplifier to deliver test pulses. Then, adjust IR oblique illumination in order to obtain a clear view of the brain.
Now, while applying positive pressure to the pipette, approach the cell with the pipette. When contact with the cell is made, release the positive pressure to seal the pipette to the membrane. Then, set the holding potential of the membrane to -60 millivolts, and the pipette should form a gigaohm seal with the cell membrane. The holding current should drop to a low sub-picoamp level.
To obtain constant gigaohm seals, make sure to keep your pipette clean by keeping positive pressure, and avoid hitting tissue when approaching your cells.
To proceed, set the amplifier to deliver test pulses from -50 to -60 millivolts. The test pulses will reveal a large capacitative transient representing the current necessary to charge the patch pipette. To remove capacitative transients, adjust the capacity compensation knobs on the amplifier.
Now, apply brief pulses of negative pressure to rupture the cell membrane and obtain the whole-cell configuration. A large increase in the capacitative transients indicates success. A small increase in the holding current should also be observed. Then, set the amplifier to current clamp mode and adjust the cell&#39;s potential to between -50 and -60 millivolts.
The holding potential may be adjusted to emphasize the excitatory or inhibitory connections accordingly. Once a connection is verified, set up the saline perfusion for recirculation of the saline. Set the pumps so the saline level in the bath stays stable.
Then, add enough tetrodotoxin to the system for a final concentration of one micromolar. This should stop the spiking activity of the patched neuron. If not, add more tetrodotoxin to the system. Now, apply brief pulses of red light to activate what is likely to be a monosynaptic connection.

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1. Prepare Flies and Identify GAL4 promoter Lines
<ol>
	<li>Select a GAL4 promoter line and cross it with flies carrying both the UAS-NaChBac transgene and an optogenetic transgene for activation. 
	NOTE: UAS-CsChrimson&#160;is selected due to its high conductance and the ease with which it activates tetrodotoxin (TTX)-resistant sodium channel (NaChBac)-mediated action potentials. Both UAS-NaChBac and UAS-CsChrimson are available from the Bloomington Stocks Repository.</li>
	<li>Prepare all-trans retinal as a stock solution in ethanol (35 mM) and store the solution in freezer at -20 &#176;C.</li>
	<li>Mix 28 &#181;L of this stock into approximately 5 mL of rehydrated potato flake food and add this mixture to the top of a vial of conventional&#160;Drosophila&#160;medium.</li>
	<li>Raise adult flies expressing csChrimson on food containing 0.2 mM all-trans-retinal for 1&#8211;3 days.</li>
</ol>
2. Prepare TTX Stock
<ol>
	<li>Create a stock solution of 1 mM TTX in distilled or deionized water. Store this solution in a lab refrigerator for several months. Check the institution&#39;s policies regarding the storage of TTX, as many institutions classify TTX as a hazardous or controlled substance.</li>
</ol>
3. Prepare Flies for Electrophysiology
<ol>
	<li>Collect 1&#8211;3 day old adult flies that are raised on the food with all-trans-retinal.</li>
	<li>Put the flies in a glass scintillation vial. Place the vial onto ice for 1 min to immobilize the flies.</li>
	<li>Use coarse forceps to insert a fly into a custom-made recording chamber. The chamber consists of a 3 &#189;&#34; circle laser cut from 1/16&#34; acrylic. Cut a &#190;&#34; hole into the center, where a custom foil is attached with 2-part epoxy. The foil contains a triangular-shaped hope that the fly is inserted into.</li>
	<li>Apply wax or ultraviolet (UV) curable epoxy around the animal to firmly secure it within the recording chamber.</li>
	<li>Illuminate the preparation with a gooseneck optical fiber for visualization under a stereomicroscope. Set the gooseneck fibers for oblique illumination by adjusting them so that they illuminate the fly directly from the side.</li>
	<li>Adjust the light level to lowest possible setting that still allows clear visualization of the fly. This light intensity will vary across individual experiments. 
	NOTE: This protocol can be adapted by using an in&#160;situ brain&#160;explant method.</li>
	<li>Retrieve external recording saline. The saline contains in mM: 103 sodium chloride, NaCl, 3 potassium chloride, KCl, 5 N-tris(hydroxymethyl)methyl-2- aminoethane-sulfonic acid, 8 trehalose, 10 glucose, 26 sodium bicarbonate, NaHCO3, 1 sodium dihydrogen phosphate, NaH2PO4, 1.5 calcium chloride, CaCl2, and 4 magnesium chloride, MgCl2&#160;(adjusted to 270&#8211;275 m&#937;). The saline is bubbled with 95% O2/5% CO2&#160;(carbogen) and has a pH adjusted to 7.3.</li>
	<li>Place 4-6 drops of extracellular recording saline over the fly preparation. At this point, increase the light level at the dissection microscope for better visibility.</li>
	<li>Sharpen a tungsten wire using electrolysis. To make the wire, prepare a saturated solution of potassium nitrate, KNO3&#160;and apply approximately 20 V of alternating current (AC) while dipping the tip of the wire into the solution 20 times for 100 ms each until the tip is sharpened. Use the sharpened tungsten wire to remove the cuticle on the head of the fly and thus exposing the brain.</li>
	<li>Further expose the brain by removing trachea and fat bodies that surround it. If accessing the antennal lobes, use a bent tungsten wire or similar tool to gently tuck the antennae underneath the foil recording chamber to increase visibility. Use sharp forceps to gently tear away the glial sheathing covering the area of interest where recordings will be made.</li>
	<li>Transfer the recording chamber to the electrophysiology rig. Immediately start perfusion with external recording saline bubbled with carbogen to preserve the brain. The saline solution reservoir is placed above the microscope stage and is gravity-fed to the preparation. Use a vacuum line and a 2 L Erlenmeyer flask to collect the waste saline.</li>
</ol>
4. Obtain Whole-cell Recording
<ol>
	<li>Pull patch pipettes on a commercial pipette puller. Consult the manual for settings to achieve an appropriate pipette with a tip resistance near 7 m&#937;.</li>
	<li>Add 4 &#181;L of internal recording solution into a patch pipette. The internal saline consists of 140 potassium aspartate, 10 N-2-hydroxyethylpiperazine-N&#39;-2-ethanesulfonic acid&#160; (HEPES), 4 magnesium adenosine triphosphate (MgATP), 0.5 Guanosine 5&#39;-triphosphate trisodium salt hydrate (Na3GTP), 1 ethylene glycol tetraacetic acid (EGTA), and 1 potassium chloride (KCl) in mM.</li>
	<li>Set up patch clamp amplifier for whole-cell recording. Zero the amplifier&#39;s offset and set the amplifier to deliver test pulses. Here, an AM systems Patch clamp amplifier 2,400 is used.</li>
	<li>Apply positive pressure through the pipette and approach the cell. Use a micromanipulator to direct the pipette and contact the cell. Release positive pressure. Set the holding potential of the membrane to -60 mV. The pipette should form a gigaohm seal with the cell&#39;s membrane as evidenced by a low sub-picoamp holding current. 
	NOTE: If using green fluorescent protein (GFP) guided cell targeting, try to minimize use of epifluorescent light to prevent ChR2 activation and potential synaptic depression. Also wait for a few minutes before applying step 5.</li>
	<li>Set the amplifier to deliver test pulses from -50 mV to -60 mV. This setting is standard on patch-clamp amplifiers. Test pulses will reveal a large capacitative transient representing the current necessary to charge the patch pipette. Remove capacitative transients by adjusting the capacity compensation knobs on the AM 2400 or similar amplifier.</li>
	<li>Apply brief pulses of negative pressure to rupture the cell membrane and obtain whole-cell configuration.&#160;&#160; 
	NOTE: A whole cell configuration is observed when there is a large increase in the capacitative transients showing the capacitance of the neuron. A small increase in the holding current (baseline) will likely also be observed. Set the amplifier to the current clamp mode and adjust the cell&#39;s potential to -50 to -60 mV.</li>
</ol>
5. Test Synaptic Connectivity
<ol>
	<li>Configure the data acquisition (DAQ) system to trigger a light-emitting diode (LED) driver to generate light pulses. Here, a National Instruments DAQ system is used with Matlab to deliver an analog signal to a LED driver. The LED intensity is adjusted via the analog signal to the driver. The LED is a 620-630 nm wavelength LED.</li>
	<li>Position the high-powered red LED directly underneath the preparation. Adjust the light intensity so that 0.238 mW/mm2&#160;reaches the fly.</li>
	<li>Activate presynaptic neurons while recording from the postsynaptic cell of interest. Achieve cell activation optogenetically, pharmacogentically, or via nerve stimulation. Here, csChrimson and brief pulses of red light are applied. 
	NOTE: Synaptic connections can be monitored either in the current clamp as excitatory postsynaptic&#160;potentials (EPSPs) or voltage clamp as excitatory postsynaptic&#160;currents (EPSCs). A synaptic connection should be visible before applying TTX in response to a 40 ms light pulse. If no connection is observed, it is unlikely that the neurons are synaptically connected either mono- or polysynaptically. The holding potential may be adjusted to emphasize excitatory or inhibitory connections accordingly.</li>
	<li>If a connection is observed in normal saline, add TTX to the perfusion system to achieve a final concentration of 1 &#181;M. Use a recirculating pump to capture and reuse the saline to conserve TTX. The peristaltic pump will draw the saline solution from the bath and return it to the saline reservoir.</li>
	<li>Adjust the pump&#39;s speed to provide a strong constant vacuum that does not allow the saline level in the bath to rise and fall. 
	NOTE: The application of TTX should result in the cessation of spiking activity in the neuron that is being monitored in whole-cell. This confirms that enough TTX has been added to the saline.</li>
	<li>Apply brief pulses of red light (40 ms for each pulse) again. At this point, any synaptic connection that remains is likely monosynaptic.&#160;</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>UAS-csChrimson</td>
			<td>Bloomington Drosophila Stock Center</td>
			<td>55135</td>
			<td>Used as a neural activator</td>
		</tr>
		<tr>
			<td>UAS-NaChBac</td>
			<td>Bloomington Drosophila Stock Center</td>
			<td>9466</td>
			<td>Resotores excitibility in cells in TTX</td>
		</tr>
		<tr>
			<td>Tetrodotoxin</td>
			<td>Tochris</td>
			<td>1078</td>
			<td>Special permission may be needed to purchase TTX as it is a controlled substance</td>
		</tr>
		<tr>
			<td>all trans-Retinal</td>
			<td>Sigma-Aldrichall trans-Retinal</td>
			<td>R2500</td>
			<td>Require co-factor for channelrhodopsin</td>
		</tr>
		<tr>
			<td>Weldable 321 Stainless Steel&#160;Sheet,&#160;0.002&#34;&#160;Thick,&#160;10&#34;&#160;Wide</td>
			<td>McMaster Carr</td>
			<td>3254K7</td>
			<td>Used to make custom fly holder. Custom foil can be laser cut at pololu.com from the provided PDF file</td>
		</tr>
		<tr>
			<td>Dissection Microscope</td>
			<td>Zeiss</td>
			<td>Stemi 2000-C</td>
			<td>Used for dissection of preparation</td>
		</tr>
		<tr>
			<td>Waxer</td>
			<td>Almore</td>
			<td>Eectra Waxer 66000</td>
			<td>Used during dissection to secure fly in foil</td>
		</tr>
		<tr>
			<td>Paraffin Wax</td>
			<td>Joann</td>
			<td>4917217</td>
			<td>Used with waxer</td>
		</tr>
		<tr>
			<td>Number 5 forceps</td>
			<td>Fine Science Tools</td>
			<td>#5CO</td>
			<td>Used for dissection and desheathing</td>
		</tr>
		<tr>
			<td>Dissection Scissors</td>
			<td>Fine Science Tools</td>
			<td>15001-08</td>
			<td>Used to remove parts of the cuticle during dissection</td>
		</tr>
		<tr>
			<td>Tungsten wire</td>
			<td>A-M Systems</td>
			<td>797500</td>
			<td>Use with electrolysis to make sharpened needles for dissection</td>
		</tr>
		<tr>
			<td>Reciculating Peristaltic Pump</td>
			<td>Simply Pumps (Amazon)</td>
			<td>PM200S</td>
			<td>for recirculating TTX</td>
		</tr>
		<tr>
			<td>Speed Controller for peristaltic pump</td>
			<td>Zitrades (Amazon)</td>
			<td>N/A</td>
			<td>PWM Dimming Controller For LED Lights or Ribbon, 12 Volt 8 Amp,Adjustable Brightness Light Switch Dimmer Controller DC12V 8A 96W for Led Strip Light B</td>
		</tr>
		<tr>
			<td>Versa-Mount&#160;Precision Compressed Air Regulator</td>
			<td>McMaster Carr</td>
			<td>1804T1</td>
			<td>For applying positive pressure during patching</td>
		</tr>
		<tr>
			<td>Glass capilaries</td>
			<td>World Precision Instruments</td>
			<td>TW150F-3</td>
			<td>For patch pipettes</td>
		</tr>
		<tr>
			<td>Multipurpose Gauge</td>
			<td>McMaster Carr</td>
			<td>3846K431</td>
			<td>Gauge for pressure regulator</td>
		</tr>
		<tr>
			<td>Electrophysiology Camera</td>
			<td>Dage MTI&#160;</td>
			<td>IR-1000</td>
			<td>Any camera that works in the IR range (850 nm) will work. You do not want to use red illumination as this can activate csChrimson</td>
		</tr>
		<tr>
			<td>IR LED</td>
			<td>Thorlabs&#160;</td>
			<td>M850F2</td>
			<td>For oblique illumination</td>
		</tr>
		<tr>
			<td>Fiber optic for IR LED</td>
			<td>Thorlabs</td>
			<td>M89L01</td>
			<td>Couples to IR LED</td>
		</tr>
		<tr>
			<td>Objective lens&#160;</td>
			<td>Olympus 40X</td>
			<td>LUMPlanFLN</td>
			<td>This can be used on most microscipes and works well for visualizing fly neurons.</td>
		</tr>
		<tr>
			<td>Amber LED</td>
			<td>Thorlabs</td>
			<td>M590L3d</td>
			<td>For visualizing RFP and mCherry</td>
		</tr>
		<tr>
			<td>Blue LED</td>
			<td>Thorlabs</td>
			<td>M470L3d</td>
			<td>For visualizing GFP</td>
		</tr>
		<tr>
			<td>GFP filter set</td>
			<td>Chroma</td>
			<td>49011</td>
			<td>For visualizing GFP or stimulating channel2rhodopsin</td>
		</tr>
		<tr>
			<td>Custom mCherry Filter Set</td>
			<td>Chroma</td>
			<td>&#160;et580/25x and t600lpxr (from the 49306 set) but with an et610lp barrier/emission optic</td>
			<td>Use only if you wish to patch identified neurons with channel2rhodopsin</td>
		</tr>
		<tr>
			<td>Dichroic to combine Amber and blue LED</td>
			<td>Thorlabs</td>
			<td>DMLP550R</td>
			<td>Use only patch under mCherry and excite channel2rhodopsin with blue light.</td>
		</tr>
		<tr>
			<td>Red LED</td>
			<td>LEDSupply</td>
			<td>Cree XPE 620 - 630 nm</td>
			<td>Used to drive csChrimson</td>
		</tr>
		<tr>
			<td>LED Driver</td>
			<td>LEDSupply</td>
			<td>3021-D-E-1000</td>
			<td>Used to drive LEDs for optogenetic stimulation</td>
		</tr>
		<tr>
			<td>Manipulator</td>
			<td>Sutter Instruments</td>
			<td>MP-225</td>
			<td>Used to position pipette during recordings</td>
		</tr>
		<tr>
			<td>Patchclamp Amplifier</td>
			<td>A-M Systems</td>
			<td>Model 2400</td>
			<td>An equivalent amplifier is suitable</td>
		</tr>
		<tr>
			<td>Bessel Filter</td>
			<td>Warner Instruments&#160;</td>
			<td>LPF 202A</td>
			<td>Auxillary filter used to filter current trace to oscilloscope during patching.</td>
		</tr>
		<tr>
			<td>Data Acquisition System&#160;</td>
			<td>National Instruments</td>
			<td>NI PCIe-6321&#160;&#160;&#160;&#160;&#160;&#160; 781044-01</td>
			<td>Used to record data from amplifier to computer</td>
		</tr>
		<tr>
			<td>Connector Block - BNC Terminal BNC-2090A</td>
			<td>National Instruments</td>
			<td>779556-01</td>
			<td>Used to connect amplifier to DAQ card.</td>
		</tr>
		<tr>
			<td>Steel Foil&#160;</td>
			<td>McMaster Carr</td>
			<td>3254K7</td>
			<td>Steel foil for custom recording chamber</td>
		</tr>
		<tr>
			<td>Magnets</td>
			<td>K&#38;J Magnetics</td>
			<td>D42</td>
			<td>To secure recording chamber to ring stand</td>
		</tr>
		<tr>
			<td>1/16&#34; Cell Cast Acrylic Clear</td>
			<td>Pololu</td>
			<td></td>
			<td>Used to make custom recording chamber. Acrylic can be laser cut at pololu.com from the provided PDF file</td>
		</tr>
	</tbody>
</table>

Source: Zhang, X. et al., <a href="https://app-jove-com.bdigitaluss.remotexs.co/v/57052">Examining Monosynaptic Connections in Drosophila Using Tetrodotoxin Resistant Sodium Channels.</a> J. Vis. Exp. (2018)
This video demonstrates testing monosynaptic connections using a transgenic fly. The fly has tetrodotoxin-resistant sodium channels and red light-activated channels in its presynaptic neurons, which are optogenetically excited to transmit signals to postsynaptic neurons.

1. Prepare Flies and Identify GAL4 promoter Lines

	Select a GAL4 promoter line and cross it with flies carrying both the UAS-NaChBac transgene and an ...

Begin with an electrophysiology setup containing an immobilized transgenic fly with an exposed brain.
Position a recording micropipette near a postsynaptic neuron connected to a presynaptic neuron co-expressing tetrodotoxin-resistant sodium channels and red light-sensitive channels, and an interneuron with tetrodotoxin-sensitive sodium channels. 
Apply mild suction to the micropipette to form a tight seal with the neuronal membrane. 
Then, apply a strong suction to disrupt the membrane. 
Maintain a constant cell potential. Introduce tetrodotoxin, which blocks sodium channels in the interneuron, preventing signal transmission from the interneuron to the postsynaptic neuron. 
However, the tetrodotoxin-resistant sodium channels remain unaffected, allowing sodium ions to enter the presynaptic neuron. 
Illuminate the fly with the red-light pulses.
This stimulates the light-sensitive channels, allowing cations to influx and activate the presynaptic neuron. 
This presynaptic neuron directly transmits a signal to the postsynaptic neuron without involving the interneuron, and the resulting electrical activity confirms the monosynaptic connection.

17 vistas. Prueba de conexiones monosinápticas utilizando tetrodotoxina y canales de sodio resistentes a la tetrodotoxina

Video: Prueba de conexiones monosinápticas utilizando tetrodotoxina y canales de sodio resistentes a la tetrodotoxina - Experimento

An Optogenetic Approach for Assessing Formation of Neuronal Connections in a Co-culture System

Here we describe a protocol to generate a co-culture consisting of 2 different neuronal populations. Induced pluripotent stem cells (iPSCs) are reprogrammed from human fibroblasts using episomal vectors. Colonies of iPSCs can be observed 30 days after initiation of fibroblast reprogramming. Pluripotent colonies are manually picked and grown in neural induction medium to permit differentiation into neural progenitor cells (NPCs). iPSCs rapidly convert into neuroepithelial cells within 1 week and retain the capability to self-renew when maintained at a high culture density. Primary mouse NPCs are differentiated into astrocytes by exposure to a serum-containing medium for 7 days and form a monolayer upon which embryonic day 18 (E18) rat cortical neurons (transfected with channelrhodopsin-2 (ChR2)) are added. Human NPCs tagged with the fluorescent protein, tandem dimer Tomato (tdTomato), are then seeded onto the astrocyte/cortical neuron culture the following day and allowed to differentiate for 28 to 35 days. We demonstrate that this system forms synaptic connections between iPSC-derived neurons and cortical neurons, evident from an increase in the frequency of synaptic currents upon photostimulation of the cortical neurons. This co-culture system provides a novel platform for evaluating the ability of iPSC-derived neurons to create synaptic connections with other neuronal populations.

A protocol to generate a co-culture system consisting of neurons derived from induced pluripotent stem cells (iPSCs), primary cortical neurons and astrocytes is described. This co-culture system allows detection of the formation of synaptic contacts and circuits between new, iPSC-derived neurons and pre-existing cortical neurons expressing channelrhodopsin-2.

Un enfoque optogenética para Evaluar formación de conexiones neuronales en un sistema de co-cultura

Here we describe a protocol to generate a co-culture consisting of 2 different neuronal populations. Induced pluripotent stem cells (iPSCs) are ...

Investigación

JoVE Journal

Biología del Desarrollo

Electrophysiological and Morphological Characterization of Neuronal Microcircuits in Acute Brain Slices Using Paired Patch-Clamp Recordings

The combination of patch clamp recordings from two (or more) synaptically coupled neurons (paired recordings) in acute brain slice preparations with simultaneous intracellular biocytin filling allows a correlated analysis of their structural and functional properties. With this method it is possible to identify and characterize both pre- and postsynaptic neurons by their morphology and electrophysiological response pattern. Paired recordings allow studying the connectivity patterns between these neurons as well as the properties of both chemical and electrical synaptic transmission. Here, we give a step-by-step description of the procedures required to obtain reliable paired recordings together with an optimal recovery of the neuron morphology. We will describe how pairs of neurons connected via chemical synapses or gap junctions are identified in brain slice preparations. We will outline how neurons are reconstructed to obtain their 3D morphology of the dendritic and axonal domain and how synaptic contacts are identified and localized. We will also discuss the caveats and limitations of the paired recording technique, in particular those associated with dendritic and axonal truncations during the preparation of brain slices because these strongly affect connectivity estimates. However, because of the versatility of the paired recording approach it will remain a valuable tool in characterizing different aspects of synaptic transmission at identified neuronal microcircuits in the brain.

Patch-clamp recordings and simultaneous intracellular biocytin filling of synaptically coupled neurons in acute brain slices allow a correlated analysis of their structural and functional properties. The aim of this protocol is to describe the essential technical steps of electrophysiological recording from neuronal microcircuits and their subsequent morphological analysis.

Electrofisiológico y Caracterización Morfológica de microcircuitos neuronales en el infarto agudo rodajas de cerebro Usando Emparejados patch-clamp grabaciones

The combination of patch clamp recordings from two (or more) synaptically coupled neurons (paired recordings) in acute brain slice preparations with ...

Neurociencias

Quantitative Analysis of Neuronal Dendritic Arborization Complexity in Drosophila

Dendrites are the branched projections of a neuron, and dendritic morphology reflects synaptic organization during the development of the nervous system. Drosophila larval neuronal dendritic arborization (da) is an ideal model for studying morphogenesis of neural dendrites and gene function in the development of nervous system. There are four classes of da neurons. Class IV is the most complex with a branching pattern that covers almost the entire area of the larval body wall. We have previously characterized the effect of silencing the Drosophila ortholog of SOX5 on class IV neuronal dendritic arborization complexity (NDAC) using four parameters: the length of dendrites, the surface area of dendrite coverage, the total number of branches, and the branching structure. This protocol presents the workflow of NDAC quantitative analysis, consisting of larval dissection, confocal microscopy, and image analysis procedures using ImageJ software. Further insight into da neuronal development and its underlying mechanisms will improve the understanding of neuronal function and provide clues about the fundamental causes of neurological and neurodevelopmental disorders.

Quantitative Analysis of Neuronal Dendritic Arborization Complexity in Drosophila

This protocol focuses on quantitative analysis of neuronal dendritic arborization complexity (NDAC) in Drosophila, which can be used for studies of dendritic morphogenesis.

Análisis cuantitativo de la complejidad de la arborización dendrítica Neuronal en Drosophila

Dendrites are the branched projections of a neuron, and dendritic morphology reflects synaptic organization during the development of the nervous system. ...

Testing Monosynaptic Connections Using Tetrodotoxin and Tetrodotoxin-Resistant Sodium Channels

Transcripción

Testing Monosynaptic Connections Using Tetrodotoxin and Tetrodotoxin-Resistant Sodium Channels