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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;&#160;1. Pre-embedding Immunohistochemistry (Figure 1C)<ol><li>Prepare a 4 L stock solution of Tris-buffered Saline (TBS, 50 mM, pH 7.6) as follows.<ol style='list-style-type:decimal;'><li>Measure 2L of distilled water in a 4 L beaker, add 24.23 g of trihydroxymethyl aminomethane (THAM; C4H11NO3), and stir to dissolve.</li><li>Adjust the pH to 7.6 with approximately 148 mL of 1 N HCl. The acid should be added with caution to avoid reaching a pH below 7.6. The total volume should be 4 L. CAUTION: HCl is highly corrosive. Wear the appropriate PPE.</li></ol></li><li>Select sections containing the region of interest to be processed for EM immunohistochemistry.</li><li>Wash the free-floating sections 3x&#160;in PBS (0.1 M, pH 7.4) for 5 min at RT&#160;to rinse the antifreeze solution.</li><li>Prepare a 0.5% solution of NaBH4&#160;diluted in PBS.<ol style='list-style-type:decimal;'><li>Weigh 0.05 g of NaBH4&#160;and dilute it in 10 mL of PBS. Do not cover. Prepare this solution just before use.</li></ol></li><li>Incubate the sections in the freshly prepared NaBH4&#160;solution for 30 min at RT. Rock gently. Do not cover.</li><li>Wash 3x&#160;in PBS for 10 min at RT, rocking vigorously until none of the reaction gas remains.</li><li>Prepare a blocking solution for EM with 2% appropriate normal serum and 0.5% cold fish gelatin diluted in PBS. NOTE: The quantity should be calculated in order to have enough for the following three steps. Use a serum made from the same animal species hosting the secondary antibody.&#160;Avoid the use of antigen retrieval methods or the addition of small amounts of triton (to increase the penetration of antibodies), as these methods significantly compromise the quality of the tissue.</li><li>Incubate the sections in the blocking solution for 1 h at RT. Rock gently.</li><li>Prepare primary antibody solution diluted in the blocking solution. NOTE: The concentration of the primary antibody is usually the same as that of LM immunohistochemistry, but consider conducting tests with different antibody concentrations beforehand, as some primary antibodies may not work with acrolein. If so, it is possible to use a mix of glutaraldehyde (0.1 - 2%) and 4% PFA for transcardiac perfusion and obtain similar results. Optimize the incubation time and temperature as well.</li><li>Incubate the sections in primary antibody solution overnight at RT with gentle rocking. Use a previously tested incubation time and temperature.</li><li>Wash the sections 3x in PBS for 5 min at RT with gentle rocking.</li><li>Prepare a 1:1,000 solution of biotinylated secondary antibody diluted in the blocking solution. NOTE: The secondary antibody must be raised against the host species used to generate the primary antibody.</li><li>Incubate the sections in a secondary antibody solution for 1.5 h at RT. Rock gently.</li><li>Prepare an avidin-biotin-peroxidase (ABC) solution at least 60 min prior to the end of the secondary antibody incubation.<ol style='list-style-type:decimal;'><li>Use a calibrated pipette to measure 8.80 &#181;L/mL of solutions A and B and dilute them in PBS.</li><li>Rock mildly for at least 60 min at RT to allow the complete binding between the avidin and biotin molecules.</li></ol></li><li>After the incubation in the secondary antibody solution, wash 3x in PBS for 10 min at RT.</li><li>Incubate the sections in the ABC solution for 1 h at RT. Rock gently.</li><li>Wash once in PBS and twice in TBS for 10 min at RT with gentle rocking.</li><li>Prepare a fresh solution of 0.05% 3,3'-diaminobenzidine (DAB) with 0.005% H2O2&#160;diluted in TBS.<ol style='list-style-type:decimal;'><li>Weigh 12.5 mg of DAB and dilute it in 25 mL of cold TBS. Protect from light. CAUTION: The DAB powder is highly volatile and harmful if inhaled. It is carcinogenic and teratogenic. Thus, pregnant or nursing women should not manipulate this product, even when diluted. Use an N95 mask when manipulating and wear PPE.</li><li>Filter the solution and add 4.5 &#181;L of 30% H2O2&#160;just before use.</li></ol></li><li>Incubate sections in the DAB solution for 3 to 7 min at RT. Rock gently. NOTE: The brown precipitate should not be too dark in order to avoid a high level of background staining. The incubation time should be optimized accordingly.</li><li>Stop the reaction by quickly washing twice in cold TBS, then twice for 10 min in cold TBS at RT, followed by twice for 10 min in PB, with mild rocking. NOTE: The use of PB (and not PBS) is critical in order to eliminate any traces of NaCl, as it would react with osmium and form crystals.</li></ol>

performing immunohistochemistry on a non-human primate brain tissue

<a href='https://app-jove-com.remotexs.ntu.edu.sg/v/55397/preparation-non-human-primate-brain-tissue-for-pre-embedding'>Source: Eid, L. &amp; Parent, M. Preparation of Non-human Primate Brain Tissue for Pre-embedding Immunohistochemistry and Electron Microscopy.&#160;J. Vis. Exp. (2017).</a>This video demonstrates the preparation of aldehyde-fixed non-human primate brain tissue using pre-embedding immunohistochemistry for electron microscopy. It outlines the steps for immunolabeling a specific neuronal protein, followed by a peroxidase reaction that produces a colored precipitate, enabling visualization of the target protein in electron microscopy.

<figure class='image image-style-align-center image_resized' style='display:table;margin-left:auto;margin-right:auto;'><img style='aspect-ratio:5415/4359;' src='https://cloudfront-jove-com.remotexs.ntu.edu.sg/files/ftp_upload/23359/23359_Figure1_editor_23359.jpg' alt='23359_Figure1.jpg' /></figure>Figure 1: Schematics of Essential Steps of the Protocol.&#160;The monkey brain (A) is cut into serial sections with a cooling vibratome (B). It is then processed for pre-embedding immunohistochemistry and electron microscopy, after which the region of interest is placed on the tip of a resin block (C) and cut into 80 nm thick sections with an ultramicrotome (D). Ultrathin sections are then collected on bare 150 mesh copper grids or formvar-coated nickel grids (E), stained with lead citrate and ready to be observed under transmission electron microscope (F). Scale bars: 1 mm.

Performing Immunohistochemistry on a Non-Human Primate Brain Tissue

Source: Eid, L. &amp; Parent, M. Preparation of Non-human Primate Brain Tissue for Pre-embedding Immunohistochemistry and Electron Microscopy.&#160;J. ...

Begin with a chemically fixed non-human primate brain section.The aldehyde-based fixative cross-links proteins, preserving tissue structure, but leaves some reactive aldehyde residues.Wash to remove the cryoprotectant layer surrounding the tissue section.Add a reducing agent to neutralize the reactive aldehyde groups, producing reaction by-products.Wash to remove these by-products and excess reducing agents.Apply a blocking solution to prevent non-specific antibody binding.Add primary antibodies targeting a protein expressed on specific sites on the neuronal membrane.&#160;Wash to remove unbound antibodies.Add biotinylated secondary antibodies targeting the primary antibodies.&#160;Wash to remove unbound antibodies.Overlay with avidin-biotin-peroxidase complexes that bind to the secondary antibodies.&#160;&#160;&#160;Wash again to remove unbound complexes.Introduce a chromogenic substrate along with hydrogen peroxide. In the presence of hydrogen peroxide, the peroxidase enzyme oxidizes the substrate, forming brown precipitates.

performing-immunohistochemistry-on-a-non-human-primate-brain-tissue

Nanyang Technological University

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JoVE Encyclopedia of Experiments

Neuroscience

Neuropathology

Neurodegenerative Diseases

55 Görüntüleme. Source: Eid, L. & Parent, M. Preparation of Non-human Primate Brain Tissue for Pre-embedding Immunohistochemistry and Electron Microscopy. J. Vis. Exp. (2017). This video demonstrates the preparation of aldehyde-fixed non-human primate brain tissue using pre-embedding immunohistochemistry for electron microscopy. It outlines the steps for immunolabeling a specific neuronal protein, followed by a peroxidase reaction that produces a colored precipitate, enabling visualization of the targe...

Video: Performing Immunohistochemistry on a Non-Human Primate Brain Tissue - Kavram

Evaluation of Biomarkers in Glioma by Immunohistochemistry on Paraffin-Embedded 3D Glioma Neurosphere Cultures

Analysis of protein expression in glioma is relevant for several aspects in the study of its pathology. Numerous proteins have been described as biomarkers with applications in diagnosis, prognosis, classification, state of tumor progression, and cell differentiation state. These analyses of biomarkers are also useful to characterize tumor neurospheres (NS) generated from glioma patients and glioma models. Tumor NS provide a valuable in vitro model to assess different features of the tumor from which they are derived and can more accurately mirror glioma biology. Here we describe a detailed method to analyze biomarkers in tumor NS using immunohistochemistry (IHC) on paraffin-embedded tumor NS.

Neurospheres grown as 3D cultures constitute a powerful tool to study glioma biology. Here we present a protocol to perform immunohistochemistry while maintaining the 3D structure of glioma neurospheres through paraffin embedding. This method enables the characterization of glioma neurosphere properties such as stemness and neural differentiation.

Biyolojik gliyom immünhistokimya parafin gömülü 3D tümörü Neurosphere kültürü üzerinde tarafından değerlendirilmesi

Analysis of protein expression in glioma is relevant for several aspects in the study of its pathology. Numerous proteins have been described as ...

JoVE Journal

Kanser Araştırmaları

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.

Sıçan Santral Sinir Sistemi immunohistokimyasal Analizi ve Çevresel lenf nodu Doku Bölümler

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

Nörobilim

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.

Mikroglia ve nöronlar için örnek Boyama: Cryosectioned Rat Beyin Dokusu Üzerine İmmünohistokimya için Astar

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

Performing Immunohistochemistry on a Non-Human Primate Brain Tissue

TRANSKRIPT

Performing Immunohistochemistry on a Non-Human Primate Brain Tissue

Biyolojik gliyom immünhistokimya parafin gömülü 3D tümörü Neurosphere kültürü üzerinde tarafından değerlendirilmesi

Sıçan Santral Sinir Sistemi immunohistokimyasal Analizi ve Çevresel lenf nodu Doku Bölümler

Mikroglia ve nöronlar için örnek Boyama: Cryosectioned Rat Beyin Dokusu Üzerine İmmünohistokimya için Astar