Name: microscopic analysis of synapses in mouse hippocampal slices using immunofluorescence
Uploaded: 2025-04-28T12:01:41.000+00:00
Duration: 1 min 25 s
Description: Source: McLeod, F., et al. Evaluation of Synapse Density in Hippocampal Rodent Brain Slices. J. Vis. Exp. (2017).This video demonstrates a method for ...

microscopic analysis of synapses in mouse hippocampal slices using immunofluorescence

Microscopic Analysis of Synapses in Mouse Hippocampal Slices Using Immunofluorescence

To begin immunofluorescence staining, replace the PBS in the slice wells with blocking and permeabilizing buffer, and incubate at room temperature for 4 to 6 hours on the shaker. Towards the end of the blocking step, dilute the antibody to VGLUT1 1 to 2000 in blocking and permeabilizing buffer. Please note that this dilution may differ depending on the company and lot of the antibody used. Incubate the slices in the primary antibody solution overnight at 4 degrees Celsius. Use a shaking platform with vigorous movement.Even distribution of the primary and secondary antibodies is important for optimal staining. In our experience, vigorous shaking enables the best antibody penetration.After the incubation in primary antibody, wash the slices three times in PBS for 10 minutes each time as before. During the last wash, dilute the appropriate secondary antibodies 1 to 500 in blocking buffer. Then incubate the slices in this solution for 2 to 3 hours at room temperature. Ensure that the slices are protected from the light, as secondary antibodies are light-sensitive.After washing the slices as before, use a brush to carefully remove the slices from the 24-well plate and place them evenly onto pre-labeled glass slides. Add a drop of mounting medium on top of each slice. And then gently place a glass coverslip on top of the slices, being careful to avoid the formation of air bubbles.Protect from light and allow the slides to dry for a minimum of three to four days at room temperature. Store the slides at 4 degrees Celsius in the short term. But for long-term storage, keep them at minus 20 degrees Celsius. Start by using a 10x or 20x objective to identify the region of the hippocampus to be imaged-- in this case, the synapses between the CA1 pyramidal neurons and the Schaffer collateral axons.Change to a 40x or 63x oil immersion objective and make sure the slice anatomy is intact by identifying continuous neurites and an organized structure. Use a neuronal marker, such as MAP2, as a reference. Adjust the settings for each channel to obtain optimal signal and contrast with a 1024 by 1024 pixel resolution. Set the intensity of each laser to avoid the saturation of any pixels.Evaluate the depth where the staining is even, and then set the software to acquire image stacks of at least eight equidistant 250-nanometer planes. Then take three adjacent representative images stacks from the same area of interest per slice. Repeat the acquisition in at least three slices per condition and from six to eight animals per treatment group.

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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.&#160;&#160;&#160;1. Acute Hippocampal Slice Preparation<ol><li>Remove the mouse brain as quickly as possible, using a spatula and sharp scissors to cut the skull, and place it in ice-cold, oxygenated (95% O2, 5% CO2), high-sucrose artificial cerebrospinal fluid (ACSF, ~100 mL). </li><li>Place the mouse brain on a Petri dish and remove the cerebellum and a small section of the frontal cortex with a scalpel before hemisecting down the midline of the brain. </li><li>Place the two hemispheres on the side that was just cut and glue each hemisphere onto the stage of a vibratome. </li><li>Cut 200 - 300 &#181;m-thick sections of the complete region of interest. In the case of the hippocampus, approximately 3 - 4 slices per hemisphere should be obtained. </li><li>Using a plastic Pasteur pipette, transfer the slices to a chamber submerged in oxygenated (95% O2, 5% CO2) ACSF. Maintain at 34 &#176;C for 30 min. NOTE: At this stage, slices can be treated with active pharmacological agents, such as recombinant Dickkopf-1 (Dkk1) proteins, by adding the agents to the slice chamber. </li><li>Using a paintbrush, remove the slices from the chamber, place them into a 24-well plate, and fix them for 20 min to 1 h in 4% paraformaldehyde (PFA)/4% sucrose at room temperature (RT). Caution: PFA is toxic, wear appropriate protection. </li><li>Wash the slices three times in 1X phosphate-buffered saline (PBS, 10 min each). NOTE: The protocol can be paused here for 1 - 2 days, as long as the slices are kept at 4 &#176;C in 1X PBS.</li></ol>2. Immunofluorescence for Synaptic MarkersNOTE: The recipes of all buffers used can be found in&#160;Table 1.<ol><li>In the slice wells, replace the PBS with blocking/permeabilizing buffer (Table 1) and incubate at RT for 4 - 6 h. </li><li>Dilute the polyclonal guinea pig antibody against vesicular glutamate transporter 1 (vGlut1) at a 1:2,000 dilution in blocking/permeabilization buffer. NOTE: vGlut1 is a marker for pre-synaptic excitatory terminal visualization. For post-synaptic excitatory synapse identification, use a polyclonal antibody against postsynaptic density-95 (PSD-95) and dilute 1:500 in the same solution. Use a minimum volume of 300 &#181;L in each well. To identify the anatomical location of the hippocampus, use an antibody that can also identify the neuronal structure, such as microtubule associated protein 2 (MAP2) or Tubulin. Work out the correct concentrations of all primary antibodies for the synaptic markers of choice (pre- and post-synaptic) and dilute in fresh blocking/permeabilizing buffer. </li><li>Incubate the slices in the primary antibody solution overnight (or for 1 - 2 days) at 4 &#176;C. Use a shaking platform with vigorous movement. </li><li>Wash the slices three times in PBS (10 min each). </li><li>Dilute the appropriate secondary antibodies 1:500 in the blocking buffer. For example, when using the vGlut1 guinea pig antibody, apply a secondary antibody that recognizes the guinea pig component (e.g.,&#160;donkey anti-guinea pig) conjugated to a specific fluorophore. When using the PSD-95 rabbit antibody, apply a secondary antibody that recognizes the rabbit component (e.g.,&#160;donkey anti-rabbit) conjugated to a different specific fluorophore. </li><li>Incubate the slices in this solution for 2 - 3 h at RT. Ensure that the slices are protected from the light, as secondary antibodies are light-sensitive. </li><li>Wash the slices three times in PBS (10 min each). </li><li>Carefully remove the slices from the 24-well plate using a paintbrush and place them evenly onto pre-labeled glass slides. Add a drop of mounting medium on top of each slice and then gently place a glass coverslip on top of the slices. Avoid the formation of air bubbles. Take care to use enough mounting medium (300-400 &#181;L), as an insufficient amount may lead to dry slices. </li><li>Leave to dry for a minimum of 1 - 2 days at RT and keep the slides protected from light. </li><li>Store the slides at 4 &#176;C in the short-term, but for long-term storage, keep them at -20 &#176;C.</li></ol>3. Confocal Image Acquisition and Analysis<ol><li>Imaging using confocal laser scanning microscopy. <ol style='list-style-type:decimal;'><li>Identify the region of the hippocampus to be imaged (e.g., the cornu ammonis 1 and 3 (CA1, CA3) or the dentate gyrus (DG)) by means of a 10x or 20x objective. </li><li>Change to a 40x or 63x oil-immersion objective to make sure the slice anatomy is intact by identifying continuous neurites and organized structure. Use a neuronal marker, such as MAP2, as a reference (Figure 1A). </li><li>Subsequently, switch to a 60x oil-immersion objective (numerical aperture [NA] = ~1.3 - 1.4) and adjust the settings for each channel to obtain optimal signal and contrast. Use a high-/low-contrast option to set the intensity of each laser to avoid the saturation of any pixels. NOTE:&#160;These settings will depend on the microscope used, but refer to the&#160;Table of Materials for the laser power settings. For best results, use a 1024 x 1024-pixel resolution. The settings should remain constant throughout the different conditions of the same experiment. Additional zoom can be applied if required. </li><li>Evaluate the depth where the staining is even and acquire image stacks of at least 8 equidistant (250 nm) planes. Then take 3 adjacent representative image stacks from the same area of interest per slice. NOTE:&#160;The depth may vary from one slice to another but should always be approximately 2 - 5 &#181;m from the surface of the slice. </li><li>Repeat the acquisition in at least 3 slices per condition and from 6 - 8 animals per treatment group.</li></ol></li></ol>Table 1: Buffers used for immunofluorescent staining.&#160;<figure class='table' style='float:left;width:100%;'><table class='ck-table-resized'><colgroup><col style='width:33.33%;'><col style='width:33.33%;'><col style='width:33.34%;'></colgroup><tbody><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>Blocking/permeabilizing Buffer&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>Concentration&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>Notes</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>Donkey serum&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>10%</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>Triton-X&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>0.50%</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>PBS&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>1x</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>10x PBS&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>pH to 7.4&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>NaCl&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>1.37 M</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>KCl&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>27 mM</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>NaH2PO4&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>100 mM&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>KH2PO4&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>18 mM</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>4% PFA/4% Sucrose&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>pH to 7.4&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>PBS&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>1x</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;Dilute from 10x</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>PFA&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;1.33 M</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr><tr><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>Sucrose&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>117 mM&#160;</td><td style='border:1pt solid #000000;padding:5pt;vertical-align:top;'>&#160;</td></tr></tbody></table></figure>&#160;&#160;

<figure class='table' style='width:750pt;'><table class='ck-table-resized'><colgroup><col style='width:23.73%;'><col style='width:19.73%;'><col style='width:16.53%;'><col style='width:40.01%;'></colgroup><tbody><tr><td style='height:15.5pt;'>Vibratome</td><td>Leica</td><td>VT1000S</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>Primary antibody</td><td>Millipore</td><td>AB5905</td><td style='width:300pt;'>vGlut1 (1:2000)</td></tr><tr><td style='height:15.5pt;'>Primary antibody</td><td>Thermo Scientific</td><td>MA1-046</td><td style='width:300pt;'>PSD-95 (1:500)</td></tr><tr><td style='height:15.5pt;'>Primary antibody</td><td>Synaptic Systems</td><td>131 004</td><td style='width:300pt;'>vGAT (1:500)</td></tr><tr><td style='height:15.5pt;'>Primary antibody</td><td>Synaptic Systems</td><td>147011</td><td style='width:300pt;'>Gephyrin (1:500)</td></tr><tr><td style='height:15.5pt;'>Primary antibody</td><td>Abcam</td><td>ab5392</td><td style='width:300pt;'>MAP2 (1:10000)</td></tr><tr><td style='height:15.5pt;'>Secondary antibody</td><td>Jackson Laboratories</td><td>706-545-148</td><td style='width:300pt;'>Donkey Anti-Guinea Pig Alexa Fluor 488 (1:600)</td></tr><tr><td style='height:15.5pt;'>Secondary antibody</td><td>Abcam</td><td>ab175470</td><td style='width:300pt;'>Donkey Anti-Rabbit Alexa Fluor 568 (1:600)</td></tr><tr><td style='height:15.5pt;'>Mounting medium</td><td>SouthernBiotech</td><td>00-4958-02</td><td style='width:300pt;'>Fluoromount-G</td></tr><tr><td style='height:62.0pt;'>Confocal Microscope</td><td>Olympus</td><td>NA</td><td style='width:300pt;'>FV1000 confocal microscope using a 60x 1.35 numerical aperture (NA) oil objective. For vGlut1, use a 488 laser with a percentage power of 14%. For PSD-95 use a 559 laser with a percentage power of 20%.</td></tr><tr><td style='height:15.5pt;'>Analysis software</td><td>PerkinElmer</td><td>NA</td><td style='width:300pt;'>Volocity</td></tr><tr><td style='height:15.5pt;'>Scalpel</td><td>Swann-Morton</td><td>203</td><td style='width:300pt;'>No 11</td></tr><tr><td style='height:15.5pt;'>Super Glue</td><td>Loctite</td><td>1446875</td><td style='width:300pt;'>&#160;</td></tr><tr><td style='height:15.5pt;'>95% O2, 5% CO2</td><td>BOC</td><td>NA</td><td style='width:300pt;'>Cylinder</td></tr><tr><td style='height:15.5pt;'>24-well plate</td><td>Corning</td><td>3524</td><td style='width:300pt;'>&#160;</td></tr><tr><td style='height:15.5pt;'>Glass slides</td><td>Thermo</td><td>7107</td><td style='width:300pt;'>08-1.0mm thick</td></tr><tr><td style='height:15.5pt;'>Petri Dish</td><td>Corning</td><td>430167</td><td style='width:300pt;'>&#160;</td></tr><tr><td style='height:93.0pt;'>iDkk1 mice</td><td>N/A</td><td>N/A</td><td style='width:300pt;'>Mice were obtained by crossing tetO Dkk1 transgenic mice with CaMKII&#945; rtTA2 transgenic mice. TetO Dkk1 transgenic mice and CaMKII&#945; rtTA2 were crossed in a heterozygous state. Both mouse lines were bred in a C57BL/6J background. Single transgenic and WT littermate were used as controls.</td></tr><tr><td style='height:15.5pt;'>Reagents for solutions:</td><td>&#160;</td><td>&#160;</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>NaCl</td><td>Sigma</td><td>V800372</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>KCl</td><td>Sigma</td><td>P9333</td><td>&#160;</td></tr><tr><td style='height:17.5pt;'>Na2HPO4</td><td>Sigma</td><td>255793</td><td>&#160;</td></tr><tr><td style='height:17.5pt;'>KH2PO4</td><td>Sigma</td><td>P9791</td><td>&#160;</td></tr><tr><td style='height:17.5pt;'>CaCl2</td><td>Sigma</td><td>223506</td><td>&#160;</td></tr><tr><td style='height:17.5pt;'>MgCl2</td><td>Sigma</td><td>M9272</td><td>&#160;</td></tr><tr><td style='height:17.5pt;'>NaH2PO4</td><td>Sigma</td><td>71505</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>Kynurenic acid</td><td>Sigma</td><td>K3375</td><td>&#160;</td></tr><tr><td style='height:17.5pt;'>NaHCO3</td><td>Sigma</td><td>S5761</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>Pyruvic acid</td><td>Sigma</td><td>107360</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>EDTA</td><td>Sigma</td><td>E6758</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>D-Glucose</td><td>Sigma</td><td>G5767</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>Sucrose</td><td>Sigma</td><td>S8501</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>Triton-X</td><td>Sigma</td><td>T8787</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>Donkey Serum</td><td>Millipore</td><td>S30-100ml</td><td>&#160;</td></tr><tr><td style='height:15.5pt;'>PFA</td><td>Sigma</td><td>P6148</td><td>&#160;</td></tr></tbody></table></figure>

<a href='https://app.jove.com/v/56153/evaluation-of-synapse-density-in-hippocampal-rodent-brain-slices'>Source: McLeod, F., et al. Evaluation of Synapse Density in Hippocampal Rodent Brain Slices. J. Vis. Exp. (2017).</a>This video demonstrates a method for visualizing synaptic markers in hippocampal brain slices using confocal immunofluorescence analysis. The slices are immunostained with primary antibodies targeting presynaptic and postsynaptic markers, followed by fluorophore-conjugated secondary antibodies. The labeled markers are then visualized using confocal microscopy to evaluate the synaptic architecture through their colocalization.

Table 1: Buffers used for immunofluorescent staining.&#160;<figure class='table' style='width:73.67%;'><table class='ck-table-resized'><colgroup><col style='width:33.33%;'><col style='width:33.33%;'><col style='width:33.34%;'></colgroup><tbody><tr><td style='border:1.0pt solid black;padding:5.0pt;vertical-align:top;width:156.0pt;'>Blocking/permeabilizing Buffer&#160;</td><td style='border-bottom-style:solid;border-color:black;border-left-style:none;border-right-style:solid;bor...

Source: McLeod, F., et al. Evaluation of Synapse Density in Hippocampal Rodent Brain Slices. J. Vis. Exp. (2017).This video demonstrates a method for ...

Place a hippocampal slice from a mouse brain into a well containing a buffer. The slice contains a network of neurons that communicate through synapses.Presynaptic neuron terminals contain neurotransmitter-filled vesicles with characteristic transmembrane transporters, while postsynaptic terminals feature characteristic scaffold proteins that regulate neurotransmitter receptors. Both serve as key markers for synaptic structures.Replace the buffer with a permeabilization-blocking solution and incubate with agitation to permeabilize cellular membranes and block non-specific binding sites.Add primary antibodies targeting the presynaptic and postsynaptic markers and incubate with agitation to allow binding.&#160;Wash the slice, add fluorophore-conjugated secondary antibodies specific to the primary antibodies, and incubate with agitation in the dark.Wash the slice, then mount it onto a slide.Using a confocal microscope, identify the region of interest and magnify to visualize synapses.Capture images to identify the fluorescently labeled presynaptic and postsynaptic markers and evaluate their colocalization at the synapses.

8 vues. Microscopic Analysis of Synapses in Mouse Hippocampal Slices Using Immunofluorescence

Vidéo: Microscopic Analysis of Synapses in Mouse Hippocampal Slices Using Immunofluorescence - Expérience

Quantifying the Heterogeneous Distribution of a Synaptic Protein in the Mouse Brain Using Immunofluorescence

The presence, absence, or levels of specific synaptic proteins can severely influence synaptic transmission. In addition to elucidating the function of a protein, it is vital to also determine its distribution. Here, we describe a protocol employing immunofluorescence, confocal microscopy, and computer-based analysis to determine the distribution of the synaptic protein Mover (also called TPRGL or SVAP30). We compare the distribution of Mover to that of the synaptic vesicle protein synaptophysin, thereby determining the distribution of Mover in a quantitative manner relative to the abundance of synaptic vesicles. Notably, this method could potentially be implemented to allow for comparison of the distribution of proteins using different antibodies or microscopes or across different studies. Our method circumvents the inherent variability of immunofluorescent stainings by yielding a ratio rather than absolute fluorescence levels. Additionally, the method we describe enables the researcher to analyze the distribution of a protein on different levels: from whole brain slices to brain regions to different subregions in one brain area, such as the different layers of the hippocampus or sensory cortices. Mover is a vertebrate-specific protein that is associated with synaptic vesicles. With this method, we show that Mover is heterogeneously distributed across brain areas, with high levels in the ventral pallidum, the septal nuclei, and the amygdala, and also within single brain areas, such as the different layers of the hippocampus.

Here, we describe a quantitative approach to determining the distribution of a synaptic protein relative to a marker protein using immunofluorescence staining, confocal microscopy, and computer-based analysis.

Quantifier la répartition hétérogène d’une protéine synaptique dans le cerveau de souris à l’aide d’Immunofluorescence

The presence, absence, or levels of specific synaptic proteins can severely influence synaptic transmission. In addition to elucidating the function of a ...

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Horizontal Hippocampal Slices of the Mouse Brain

The hippocampus is a highly organized structure in the brain that is a part of the limbic system and is involved in memory formation and consolidation as well as the manifestation of severe brain disorders, including Alzheimer&#8217;s disease and epilepsy. The hippocampus receives a high degree of intra- and inter-connectivity, securing a proper communication with internal and external brain structures. This connectivity is accomplished via different informational flows in the form of fiber pathways. Brain slices are a frequently used methodology when exploring neurophysiological functions of the hippocampus. Hippocampal brain slices can be used for several different applications, including electrophysiological recordings, light microscopic measurements as well as several molecular biological and histochemical techniques. Therefore, brain slices represent an ideal model system to assess protein functions, to investigate pathophysiological processes involved in neurological disorders as well as for drug discovery purposes.
There exist several different ways of slice preparations. Brain slice preparations with a vibratome allow a better preservation of the tissue structure and guarantee a sufficient oxygen supply during slicing, which present advantages over the traditional use of a tissue chopper. Moreover, different cutting planes can be applied for vibratome brain slice preparations. Here, a detailed protocol for a successful preparation of vibratome-cut horizontal hippocampal slices of mouse brains is provided. In contrast to other slice preparations, horizontal slicing allows to keep the fibers of the hippocampal input path (perforant path) in a fully intact state within a slice, which facilitates the investigation of entorhinal-hippocampal interactions. Here, we provide a thorough protocol for the dissection, extraction, and acute horizontal slicing of the murine brain, and discuss challenges and potential pitfalls of this technique. Finally, we will show some examples for the use of brain slices in further applications.

This article aims to describe a systematic protocol to obtain horizontal hippocampal brain slices in mice. The objective of this methodology is to preserve the integrity of hippocampal fiber pathways, such as the perforant path and the mossy fiber tract to assess dentate gyrus related neurological processes.

Tranches hippocampiques horizontales du cerveau de souris

The hippocampus is a highly organized structure in the brain that is a part of the limbic system and is involved in memory formation and consolidation as ...

Ex Vivo Optogenetic Interrogation of Long-Range Synaptic Transmission and Plasticity from Medial Prefrontal Cortex to Lateral Entorhinal Cortex

Studying the physiological properties of specific synapses in the brain, and how they undergo plastic changes, is a key challenge in modern neuroscience. Traditional in vitro electrophysiological techniques use electrical stimulation to evoke synaptic transmission. A major drawback of this method is its nonspecific nature; all axons in the region of the stimulating electrode will be activated, making it difficult to attribute an effect to a particular afferent connection. This issue can be overcome by replacing electrical stimulation with optogenetic-based stimulation. We describe a method for combining optogenetics with in vitro patch-clamp recordings. This is a powerful tool for the study of both basal synaptic transmission and synaptic plasticity of precise anatomically defined synaptic connections and is applicable to almost any pathway in the brain. Here, we describe the preparation and handling of a viral vector encoding channelrhodopsin protein for surgical injection into a pre-synaptic region of interest (medial prefrontal cortex) in the rodent brain and making of acute slices of downstream target regions (lateral entorhinal cortex). A detailed procedure for combining patch-clamp recordings with synaptic activation by light stimulation to study short- and long-term synaptic plasticity is also presented. We discuss examples of experiments that achieve pathway- and cell-specificity by combining optogenetics and Cre-dependent cell labeling. Finally, histological confirmation of the pre-synaptic region of interest is described along with biocytin labeling of the post-synaptic cell, to allow further identification of the precise location and cell type.

Ex Vivo Optogenetic Interrogation of Long-Range Synaptic Transmission and Plasticity from Medial Prefrontal Cortex to Lateral Entorhinal Cortex

Here we present a protocol describing viral transduction of discrete brain regions with optogenetic constructs to permit synapse-specific electrophysiological characterization in acute rodent brain slices.

Ex Vivo Interrogation optogénétique de la transmission synaptique à longue distance et de la plasticité du cortex préfrontal médian au cortex entorhinal latéral

Studying the physiological properties of specific synapses in the brain, and how they undergo plastic changes, is a key challenge in modern neuroscience. ...

Microscopic Analysis of Synapses in Mouse Hippocampal Slices Using Immunofluorescence

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Microscopic Analysis of Synapses in Mouse Hippocampal Slices Using Immunofluorescence