imaging hippocampal neuronal activation in mouse brain sections

Imaging Hippocampal Neuronal Activation In Mouse Brain Sections

Transfer three to five dorsal hippocampal sections for each mouse into the wells of a 24-multi-well plate containing 500 microliters of 0.1 molar PBS for each well. Wash the sections contained in each well with 500 microliters of 0.1 molar PBS. Perform all washes and incubations at room temperature with gentle agitation, unless otherwise mentioned. Under a fume hood, incubate the sections in 40% methanol, 1% hydrogen peroxide in 0.1 molar PBS for 20 minutes in order to quench the endogenous peroxidase activity.Following three more washes in 0.1 molar PBS, permeabilize the sections by incubating them in 500 microliters of 0.2% Triton X-100 for five minutes. While the sections are incubating, prepare enough blocking buffer for the entire experiment. Then, remove the permeabilization solution and add 100 microliters of the blocking buffer to each well. Incubate the sections for one hour.Next, remove the blocking buffer and cover the sections with phosphorylated extracellular regulated kinase primary antibody, diluted 1 to 500 in blocking buffer. Incubate the sections overnight at 4 degrees Celsius with gentle agitation. The next day, after washing the sections three times in 0.1 molar PBS for 5 minutes each, incubate the sections with a biotin conjugated secondary antibody diluted 1 to 250 blocking buffer for one hour at room temperature.During the incubation, prepare the ABC reagent at least 30 minutes before use in order to allow enough time for the avidin and biotin complex to form. After washing the sections three more times with 0.1 molar PBS, add the ABC reagent, and allow it to incubate with the sample for 45 minutes. During the next set of three washes in PBS, prepare the dab working solution in the fume hood according to the manufacturer's specifications. Aliquot the dab working solution in the plate.Then, transfer sections into the wells containing the DAB working solution, and slowly swirl the plate to allow maximum exposure of the sections to the solution. Monitor the DAB reaction on a microscope until adequate signal develops in about two to five minutes. Stop the reaction at the desired color intensity by washing the tissue in 0.1 molar PBS. After three more washes in PBS, mount the sections on gelatin coated slides, and dry them at room temperature for at least three to four hours.Once air dried, transfer slides in the fume hood, and dehydrate the sections by sequentially placing them into graded ethanol solutions for two minutes each. Then, clear the slides in 100% xylenes for five minutes. Coverslip the slides using mounting medium, and leave them in the fume hood overnight to dry.Transfer the slides to a bright field microscope equipped with a camera in 20x objective lens. Acquire multiple brightfield images from each section at 200x magnification, covering the dorsal hippocampus. Image three to five sections from each animal.

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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.1. Immunohistochemistry<ol><li>Transfer 3-5 dorsal hippocampal sections for each mouse into 24 multi-well plates containing 500 &#181;l of 0.1 M phosphate-buffered saline (PBS) for each well.</li><li>Wash the sections contained in each well with 500 &#181;l of 0.1 M PBS (5 min,&#160; 3 times with gentle shaking).</li><li>Quench endogenous peroxidase activity by incubating sections in 1% hydrogen peroxide (H2O2)&#160;in PBS for 20 min with gentle agitation.</li><li>Wash sections in 0.1 M PBS with gentle agitation (3 x 5 min).</li><li>Permeabilization of tissue: incubate sections for 5 min in 0.2% Triton X-100 in PBS.</li><li>During the above steps (1.4; 1.5), make enough blocking buffer (10% Goat Serum and 0.1% Triton-X100 in PBS) for the entire experiment (number of sections x 100 &#181;l x 3 steps).</li><li>NOTE: Use serum from the same species in which the secondary antibody (Ab) (conjugated to biotin) was made.</li><li>Prevent non-specific binding of the antibody by incubating sections in a blocking buffer (100 &#181;l/section) for 1 hr at room temperature (RT) with gentle agitation.</li><li>Incubate sections in primary Ab phosphorylated extracellular signal-regulated kinase (pERK) diluted in blocking buffer overnight at 4 &#176;C, with gentle agitation.</li><li>Wash sections in 0.1 M PBS with gentle agitation (3 x 5 min).</li><li>Incubate with the secondary Ab conjugated with biotin (1:250) diluted in blocking buffer (same as used in step 1.6) for 1 hr at RT with gentle agitation.</li><li>Prepare the avidin-biotin complex (ABC) reagent at the same time, as avidin and biotin require at least 30 minutes at room temperature to complex.</li><li>Prepare the required volume of ABC reagent according to the manufacturer&#8217;s protocol.</li><li>Wash sections in 0.1 M PBS with gentle agitation (3 x 5 min).</li><li>Incubate sections for 45 min at RT with ABC Reagent.</li><li>Wash sections in 0.1 M PBS with gentle agitation (3 x 5 min).</li><li>To prepare a diaminobenzidine (DAB) working solution, every step involving DAB must be done in the fume hood, as DAB is carcinogenic and teratogenic.</li><li>Transfer the DAB solution to a new plate with a plastic transfer pipette.</li><li>Place sections in the plate containing the DAB working solution and slowly swirl the plate by hand to allow maximum exposure to sections.</li><li>Monitor DAB reaction on microscope until adequate signal develops (2-5 min).</li><li>Stop the reaction at the desired color intensity by washing the tissue in 0.1 M PBS (3 x 5 min).</li><li>Use bleach to deactivate any remaining DAB substrate solution in the fume hood overnight and dispose of it according to laboratory guidelines.</li><li>Mount sections on gelatin-coated slides by floating them in PBS. Then, dry them at room temperature for at least 3-4 hours.</li><li>Dehydrate the sections sequentially in 50%, 70%, 95%, and 100% ethanol for 2 min each and clear in 100% xylene for 5 min.</li><li>Coverslip using mounting medium and leave in a fume hood to dry overnight.</li></ol>

<figure class='table' style='width:799pt;'><table class='ck-table-resized'><colgroup><col style='width:18.52%;'><col style='width:21.4%;'><col style='width:21.15%;'><col style='width:38.93%;'></colgroup><tbody><tr><td style='height:14.5pt;width:148pt;'>24 well plate</td><td style='width:171pt;'>Sigma</td><td style='width:169pt;'>CLS3524</td><td style='width:311pt;'>&#160;</td></tr><tr><td style='height:29.0pt;width:148pt;'>100% ethanol</td><td style='width:171pt;'>Fisher Scientific</td><td style='width:169pt;'>A406-20</td><td style='width:311pt;'>Used to make ethanol gradient for dehydration prior to slide mounting.</td></tr><tr><td style='height:29.0pt;width:148pt;'>Xylene</td><td style='width:171pt;'>VWR</td><td style='width:169pt;'>66004-950</td><td style='width:311pt;'>Toxic - to be used under hood. Change xylene every month depending on use.</td></tr><tr><td style='height:14.5pt;width:148pt;'>PBS</td><td style='width:171pt;'>Sigma</td><td style='width:169pt;'>P3813-10PAK</td><td style='width:311pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:148pt;'>Triton X-100</td><td style='width:171pt;'>Sigma</td><td style='width:169pt;'>T-8787</td><td style='width:311pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:148pt;'>Hydrogen peroxide</td><td style='width:171pt;'>Sigma</td><td style='width:169pt;'>H1009-100ML</td><td style='width:311pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:148pt;'>Normal goat serum</td><td style='width:171pt;'>Abcam</td><td style='width:169pt;'>G9023-10ML</td><td style='width:311pt;'>&#160;</td></tr><tr><td style='height:29.0pt;width:148pt;'>ABC kit Vectastain</td><td style='width:171pt;'>Vector Laboratories</td><td style='width:169pt;'>PK-6100</td><td style='width:311pt;'>Add in a volume of 5 ml of PBS 2 drops of reagent A, mix and then add 2 drops of reagent B and mix.</td></tr><tr><td style='height:43.5pt;width:148pt;'>DAB peroxidase substrate</td><td style='width:171pt;'>Vector Laboratories</td><td style='width:169pt;'>SK-4100</td><td style='width:311pt;'>Add in a volume of 5 ml double distilled water: 2 drops of buffer stock solution and mix; 4 drops of DAB and mix; 2 drops of hydrogen peroxide and mix.</td></tr><tr><td style='height:14.5pt;width:148pt;'>pERK antibody</td><td style='width:171pt;'>Cell Signaling Technologies</td><td style='width:169pt;'>4370</td><td style='width:311pt;'>Dilution 1:500</td></tr><tr><td style='height:29.0pt;width:148pt;'>Biotinylated goat anti-rabbit IgG antibody</td><td style='width:171pt;'>Vector Laboratories</td><td style='width:169pt;'>BA-1000</td><td style='width:311pt;'>Dilution 1:250</td></tr><tr><td style='height:14.5pt;width:148pt;'>SuperFrost Slides</td><td style='width:171pt;'>Carl Roth</td><td style='width:169pt;'>1879</td><td style='width:311pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:148pt;'>Coverslips</td><td style='width:171pt;'>Fisher</td><td style='width:169pt;'>12-548-B</td><td style='width:311pt;'>&#160;</td></tr><tr><td style='height:29.0pt;width:148pt;'>DPX</td><td style='width:171pt;'>Sigma</td><td style='width:169pt;'>317616</td><td style='width:311pt;'>Mounting medium for slides. Equivalent mounting medium can be used.</td></tr></tbody></table></figure>

<a href='https://app.jove.com/v/52919/immunohistochemical-visualization-hippocampal-neuron-activity-after'>Source: Provenzano, G., et al.&#160;Immunohistochemical Visualization of Hippocampal Neuron Activity After Spatial Learning in a Mouse Model of Neurodevelopmental Disorders. J. Vis. Exp.&#160;(2015)</a>This video demonstrates immunohistochemical imaging to visualize hippocampal neuronal activation. Stained brain sections reveal darker regions under a bright-field microscope, indicating activated neurons.

Source: Provenzano, G., et al.&#160;Immunohistochemical Visualization of Hippocampal Neuron Activity After Spatial Learning in a Mouse Model of ...

Start with mouse brain sections exposing the dorsal hippocampus, rich in neurons.Add hydrogen peroxide to quench neuronal peroxidase activity, followed by washing.&#160;Treat with a permeabilization buffer, then apply a blocking buffer to block non-specific binding.Add the primary antibodies and incubate with agitation. These antibodies bind to neuronal activation marker proteins.Wash and apply biotin-conjugated secondary antibodies to bind the primary antibodies.&#160;Rinse and introduce an avidin-biotin-peroxidase complex that binds to biotin on the conjugates.&#160;Wash again, then add a chromogenic substrate, which is oxidized by peroxidase to generate a brown precipitate. Stop the reaction with PBS.&#160;&#160;Transfer the sections to a gelatin-coated slide and dehydrate them using increasing concentrations of ethanol. Then, clear the sections in xylene and mount them.Place the slide under a bright-field microscope.Under light illumination, unstained regions transmit light and appear bright, while stained neurons absorb and reflect light and appear darker.&#160;The distinct darker area indicates neuronal activation within the hippocampus.

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Immunohistochemical Analysis in the Rat Central Nervous System and Peripheral Lymph Node Tissue Sections

Immunohistochemistry (IHC) provides highly specific, reliable and attractive protein visualization. Correct performance and interpretation of an IHC-based multicolor labeling is challenging, especially when utilized for assessing interrelations between target proteins in the tissue with a high fat content such as the central nervous system (CNS).
Our protocol represents a refinement of the standard immunolabeling technique particularly adjusted for detection of both structural and soluble proteins in the rat CNS and peripheral lymph nodes (LN) affected by neuroinflammation. Nonetheless, with or without further modifications, our protocol could likely be used for detection of other related protein targets, even in other organs and species than here presented.

We here present an optimized, detailed protocol for double immunostaining in formalin-fixed, paraffin-embedded rat central nervous system (CNS) and peripheral lymph node (LN) tissue sections.

Analyse immunohistochimique dans le système nerveux central et périphérique Rat ganglionnaire sections de tissu

Immunohistochemistry (IHC) provides highly specific, reliable and attractive protein visualization. Correct performance and interpretation of an IHC-based ...

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Primer for Immunohistochemistry on Cryosectioned Rat Brain Tissue: Example Staining for Microglia and Neurons

Immunohistochemistry is a widely used technique for detecting the presence, location, and relative abundance of antigens in situ. This introductory level protocol describes the reagents, equipment, and techniques required to complete immunohistochemical staining of rodent brain tissue, using markers for microglia and neuronal elements as an example. Specifically, this paper is a step-by-step protocol for fluorescent visualization of microglia and neurons via immunohistochemistry for Iba1 and Pan-neuronal, respectively. Fluorescence double-labeling is particularly useful for the localization of multiple proteins within the same sample, providing the opportunity to accurately observe interactions between cell types, receptors, ligands, and/or the extracellular matrix in relation to one another as well as protein co-localization within a single cell. Unlike other visualization techniques, fluorescence immunohistochemistry staining intensity may decrease in the weeks to months following staining, unless appropriate precautions are taken. Despite this limitation, in many applications fluorescence double-labeling is preferred over alternatives such as 3,3&#39;-diaminobenzidine tetrahydrochloride (DAB) or alkaline phosphatase (AP), as fluorescence is more time efficient and allows for more precise differentiation between two or more markers. The discussion includes troubleshooting tips and advice to promote success.

This introductory level protocol describes the reagents, equipment, and techniques required to complete immunohistochemical staining of rodent brains, using markers for microglia and neuronal elements as an example.

Primaire pour Immunohistochimie sur tissus Cryosectioned cerveau de rat: Exemple coloration pour microglies et les neurones

Immunohistochemistry is a widely used technique for detecting the presence, location, and relative abundance of antigens in situ. This introductory level ...

Histological-Based Stainings Using Free-Floating Tissue Sections

Immunohistochemistry is a widely used technique to visualize specific tissue structures as well as protein expression and localization. Two alternative approaches are widely used to handle the tissue sections during the staining procedure, one approach consists of mounting the sections directly on glass slides, while a second approach, the free-floating, allows for fixed sections to be maintained and stained while suspended in solution. Although slide-mounted and free-floating approaches may yield similar results, the free-floating technique allows for better antibody penetration and thus should be the method of choice when thicker sections are to be used for 3D reconstruction of the tissues, for example when the focus of the experiment is to gain information on dendritic and axonal projections in brain regions. In addition, since the sections are kept in solution, a single aliquot can easily accommodate 30 to 40 sections, handling of which is less laborious, particularly in large-scale biomedical studies. Here, we illustrate how to apply the free-floating method to fluorescent immunohistochemistry staining, with a major focus on brain sections. We will also discuss how the free-floating technique can easily be modified to fit the individual needs of researchers and adapted to other tissues as well as other histochemical-based stainings, such as hematoxylin and eosin and cresyl violet, as long as tissue samples are properly fixed, typically with paraformaldehyde or formalin.

The free-floating technique allows researchers to perform histological-based stainings including immunohistochemistry on fixed tissue sections to visualize biological structures, cell type, and protein expression and localization. This is an efficient and reliable histochemical technique that can be useful for investigating a multitude of tissues, such as brain, heart, and liver.

Colorations histologiques utilisant des sections de tissus flottant librement

Immunohistochemistry is a widely used technique to visualize specific tissue structures as well as protein expression and localization. Two alternative ...

Imaging Hippocampal Neuronal Activation In Mouse Brain Sections

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Imaging Hippocampal Neuronal Activation In Mouse Brain Sections