Name: Serie: Immunohistochemical Staining of Rat Coronal Tissue Cryosections for Microglia and Neurons - Konzept
Uploaded: 2025-04-28T12:00:53.000+00:00
Duration: 1 min 12 s
Description: 12 Aufrufe. Source: Evilsizor, M. N., et. al., Primer for Immunohistochemistry on Cryosectioned Rat Brain Tissue: Example Staining for Microglia and Neurons. J. Vis. Exp. (2015) This video demonstrates a step-by-step immunohistochemistry staining procedure on cryosectioned rat brain tissue to visualize the spatial arrangement of microglia and neurons.

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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.<ol><li>Tissue Staining<ol style='list-style-type:decimal;'><li>In a light-tight staining box, create a &#8220;humidity chamber&#8221; with lint-free tissues soaked with deionized water.</li><li>Dry the edges of the slide with a lint-free tissue, use a mini pap pen to make a liquid-repellent border at the very edge of the slide, away from tissue sections. This border should ensure ample space between the meniscus of the liquid and the edge of the tissue so that surface tension does not affect staining. NOTE: The pap pen-repellent border can be applied prior to 1.1.3 if the antibodies of interest do not require microwave antigen retrieval. If the pap pen has been applied prior to washing in PBS, the integrity of the liquid-repellent border must be checked at this step. Use a mini-pap pen to fill in any gaps in the border.</li><li>With slides laid horizontally, block nonspecific antigen binding by incubating in 4% v/v serum in PBS (block solution). Pipette 300 &#181;l of block solution per slide for 1hr at room temperature. Make sure the block solution extends to the pap pen at the edge of the slide and completely covers the tissue to avoid uneven staining caused by surface tension near the tissue.<ol style='list-style-type:decimal;'><li>Use serum from the same species in which the secondary antibody is made. Note: In this procedure, the secondary antibodies are made in donkey, and thus donkey serum is used. If secondary antibodies from two or more different species are used, include serum from each species.</li></ol></li><li>Pipette primary antibody onto slides. Note: Antibody concentrations for this staining have been optimized at 1:5,000 and 1:500 for Iba1 and Pan-neuronal, respectively. These concentrations have been found to show meaningful staining without background staining.<ol style='list-style-type:decimal;'><li>Dilute the block solution to 1% serum in PBS and add primary antibodies. Pipette 300 &#181;l of primary antibody solution in 1% serum per slide. Again, ensure the fluid is to the edge of the pap pen. Incubate overnight at 4 &#176;C.</li><li>Include three control slides: one that contains neither Iba1 nor Pan-neuronal antibodies, one with Iba1 without Pan-neuronal antibody, and one with Pan-neuronal antibody without Iba1. Stain these slides in the same run with the same solutions, however omit the primary antibodies to test the non-specific binding of the secondary antibodies.</li></ol></li><li>The following morning, wash slides three times in PBS for 5 min each, changing the solution between washes.</li><li>Fluorescent antibodies are light-sensitive, therefore, from this step forward, minimize light exposure by ensuring wash containers are wrapped in foil and hybridization boxes are either black or incubated in the dark. Pipette the appropriate secondary antibodies on all slides and incubate for 60 min at room temperature at a concentration of 1:250 in block solution (see step 1.2.3) in a light-tight &#8220;humidity chamber&#8221; (see step 1.2.1).<ol style='list-style-type:decimal;'><li>Use secondary antibodies of different wavelengths. Here, for the primary antibody rabbit anti-Iba1, use donkey anti-rabbit 594 as the appropriate secondary antibody. For the primary antibody mouse anti-Pan-neuronal, use donkey anti-mouse 488 as the appropriate secondary antibody. Alternatively, use anti-rabbit 488 and anti-mouse 594.</li></ol></li><li>Wash slides three times in PBS for 5 min each.</li><li>Optional: perform nuclear staining.<ol style='list-style-type:decimal;'><li>Place in Hoechst (or other nuclear stain) at a concentration of 0.03 &#181;g/ml in double distilled H2O for exactly 60 sec.</li><li>Wash slides three times in PBS for 5 min each.</li></ol></li><li>Wash in ddH2O.</li></ol></li><li>Coverslipping<ol style='list-style-type:decimal;'><li>Coverslip slides with an aqueous mounting medium, such as Fluoromount-G or ProlongGold. Take care to remove all bubbles using a cotton-tipped applicator. Note: Other mounting agents could be used, however high bleed-through between dyes has been noted by some within days of coverslipping.</li><li>Use clear nail polish to seal the edges, preventing the sections from drying out due to evaporation. Allow nail polish to dry in a light-tight container while slides remain flat and at room temperature, and then store in a light-tight container wrapped in foil at 4 &#176;C.</li></ol></li></ol>

<figure class='table' style='width:920pt;'><table class='ck-table-resized'><colgroup><col style='width:25%;'><col style='width:25%;'><col style='width:25%;'><col style='width:25%;'></colgroup><tbody><tr><td style='height:15.5pt;width:230pt;'>Name of Material/ Equipment</td><td style='width:230pt;'>&#160;</td><td style='width:230pt;'>&#160;</td><td style='width:230pt;'>&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Fisherbrand Superfrost Plus Glass Slides</td><td style='width:230pt;'>Fisher Scientific</td><td style='width:230pt;'>22-034-979</td><td style='width:230pt;'>Used for tissue mounting&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Oven</td><td style='width:230pt;'>Thermo Scientific</td><td style='width:230pt;'>51028112</td><td style='width:230pt;'>Used for tissue drying&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Mini Pap pen</td><td style='width:230pt;'>Life Technologies</td><td style='width:230pt;'>00-8877</td><td style='width:230pt;'>&#160;</td></tr><tr><td style='height:31.0pt;width:230pt;'>Andwin Scientific Tissue-tek Slide Staining Dish</td><td style='width:230pt;'>Fisher Scientific</td><td style='width:230pt;'>22-149-429</td><td style='width:230pt;'>Used for all washes during staining, as well as the Hoechst step&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Kimwipes</td><td style='width:230pt;'>Fisher Scientific</td><td style='width:230pt;'>06-666-A</td><td style='width:230pt;'>Used for drying slides&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Black Staining Box</td><td style='width:230pt;'>Ted Pella</td><td style='width:230pt;'>21050</td><td style='width:230pt;'>Used for blocking and staining steps&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Normal Donkey Serum</td><td style='width:230pt;'>Fisher Scientific</td><td style='width:230pt;'>50-413-253</td><td style='width:230pt;'>Used for block and antibody incubation</td></tr><tr><td style='height:15.5pt;width:230pt;'>Mouse &#945;-Pan-neuronal</td><td style='width:230pt;'>Millipore</td><td style='width:230pt;'>MAB2300</td><td style='width:230pt;'>Used for primary antibody&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Rabbit &#945;-Iba1</td><td style='width:230pt;'>Wako Chemical</td><td style='width:230pt;'>019-19741</td><td style='width:230pt;'>Used for primary antibody&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Donkey &#945;-Rabbit 594</td><td style='width:230pt;'>Jackson ImmunoResearch</td><td style='width:230pt;'>711-585-152</td><td style='width:230pt;'>Used for secondary antibody&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Donkey &#945;-mouse 488</td><td style='width:230pt;'>Jackson ImmunoResearch</td><td style='width:230pt;'>715-545-150</td><td style='width:230pt;'>Used for secondary antibody&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Fluoromount-G</td><td style='width:230pt;'>Southern Biotech</td><td style='width:230pt;'>0100-01</td><td style='width:230pt;'>Used for coverslipping&#160;</td></tr><tr><td style='height:15.5pt;width:230pt;'>Coverslips</td><td style='width:230pt;'>Fisher Scientific</td><td style='width:230pt;'>12544E</td><td style='width:230pt;'>Used for coverslipping</td></tr><tr><td style='height:31.0pt;width:230pt;'>Axio Observer.Z1 and LSM 710 (laser scanning, confocal)</td><td style='width:230pt;'>Carl Zeiss</td><td style='width:230pt;'>N/A</td><td style='width:230pt;'>Used for imaging</td></tr><tr><td style='height:15.5pt;width:230pt;'>Axioskop A2</td><td style='width:230pt;'>Carl Zeiss</td><td style='width:230pt;'>N/A</td><td style='width:230pt;'>Used for imaging&#160;</td></tr></tbody></table></figure>

immunohistochemical staining of rat coronal tissue cryosections for microglia and neurons

<a href='https://app-jove-com.remotexs.ntu.edu.sg/v/52293/primer-for-immunohistochemistry-on-cryosectioned-rat-brain-tissue'>Source: Evilsizor, M. N., et. al., Primer for Immunohistochemistry on Cryosectioned Rat Brain Tissue: Example Staining for Microglia and Neurons. J. Vis. Exp. (2015)</a>This video demonstrates a step-by-step immunohistochemistry staining procedure on cryosectioned rat brain tissue to visualize the spatial arrangement of microglia and neurons.

Immunohistochemical Staining of Rat Coronal Tissue Cryosections for Microglia and Neurons

Source: Evilsizor, M. N., et. al., Primer for Immunohistochemistry on Cryosectioned Rat Brain Tissue: Example Staining for Microglia and Neurons. J. Vis. ...

Take a slide containing fixed and permeabilized rat coronal tissue cryosections.Outline the sections with a hydrophobic pen to create a controlled staining environment.Transfer the sections into a humidity chamber to prevent drying of reagents and tissue during subsequent steps.Treat the sections with serum proteins to block non-specific binding sites.Rinse with buffer to remove excess serum proteins.Incubate with primary antibodies targeting specific proteins on microglia and neurons.Wash with buffer to remove unbound primary antibodies.Incubate with fluorophore-conjugated secondary antibodies that bind to the primary antibodies.Wash with buffer to remove unbound secondary antibodies. Then, rinse with double-distilled water.Apply aqueous mounting media to protect the fluorescent signal, place a coverslip, and seal it.Image the sections under a fluorescence microscope to visualize immunolabeled microglia and neurons.

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Nanyang Technological University

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Neuroscience

Neuropathology

Neurodegenerative Diseases

12 Aufrufe. Source: Evilsizor, M. N., et. al., Primer for Immunohistochemistry on Cryosectioned Rat Brain Tissue: Example Staining for Microglia and Neurons. J. Vis. Exp. (2015) This video demonstrates a step-by-step immunohistochemistry staining procedure on cryosectioned rat brain tissue to visualize the spatial arrangement of microglia and neurons. 

Serie: Immunohistochemical Staining of Rat Coronal Tissue Cryosections for Microglia and Neurons - Konzept

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.

Immunhistochemische Analyse im Rat des Zentralnervensystems und peripheren Lymphknoten Gewebeschnitte

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

Forschung

JoVE Journal

Neurowissenschaften

Simultaneous Cryosectioning of Multiple Rodent Brains

Histology and immunohistochemistry are routine methods of analysis to visualize microscopic anatomy and localize proteins within biological tissue. In neuroscience, as well as a plethora of other scientific fields, these techniques are used. Immunohistochemistry can be done on slide mounted tissue or free-floating sections. Preparing slide-mounted samples is a time intensive process. The following protocol for a technique, called the Megabrain, reduced the time taken to cryosection and mount brain tissue by up to 90% by combining multiple brains into a single frozen block. Furthermore, this technique reduced variability seen between staining rounds, in a large histochemical study. The current technique has been optimized for using rodent brain tissue in downstream immunohistochemical analyses; however, it can be applied to different scientific fields that use cryosectioning.

Here, we present a protocol to freeze and section brain tissue from multiple animals as a timesaving alternative to processing single brains. This reduces staining variability during immunohistochemistry and reduces time cryosectioning and imaging.

Gleichzeitige Kryoschneiden mehrere Nagetier Gehirne

Histology and immunohistochemistry are routine methods of analysis to visualize microscopic anatomy and localize proteins within biological tissue. In ...

Using Near-infrared Fluorescence and High-resolution Scanning to Measure Protein Expression in the Rodent Brain

Neuroscience is the study of how cells in the brain mediate various functions. Measuring protein expression in neurons and glia is critical for the study of neuroscience as cellular function is determined by the composition and activity of cellular proteins. In this article, we describe how immunocytochemistry can be combined with near-infrared high-resolution scanning to provide a semi-quantitative measure of protein expression in distinct brain regions. This technique can be used for single or double protein expression in the same brain region. Measuring proteins in this fashion can be used to obtain a relative change in protein expression with an experimental manipulation, molecular signature of learning and memory, activity in molecular pathways, and neural activity in multiple brain regions. Using the correct proteins and statistical analysis, functional connectivity among brain regions can be determined as well. Given the ease of implementing immunocytochemistry in a laboratory, using immunocytochemistry with near-infrared high-resolution scanning can expand the ability of the neuroscientist to examine neurobiological processes at a systems level.

Here, we present a protocol that uses near-infrared dyes in conjunction with immunohistochemistry and high-resolution scanning to assay proteins in brain regions.

Einsatz von Infrarot-Fluoreszenz und hochauflösendem Scannen zur Messung des Protein-Expression im Rodentrains

Neuroscience is the study of how cells in the brain mediate various functions. Measuring protein expression in neurons and glia is critical for the study ...

Immunohistochemical Staining of Rat Coronal Tissue Cryosections for Microglia and Neurons

Transkript

Immunohistochemical Staining of Rat Coronal Tissue Cryosections for Microglia and Neurons

Immunhistochemische Analyse im Rat des Zentralnervensystems und peripheren Lymphknoten Gewebeschnitte

Gleichzeitige Kryoschneiden mehrere Nagetier Gehirne

Einsatz von Infrarot-Fluoreszenz und hochauflösendem Scannen zur Messung des Protein-Expression im Rodentrains