Name: immunohistochemistry of mouse brain tissue sections for targeting dopamine neurons
Uploaded: 2025-04-29T13:00:44.000+00:00
Duration: 1 min 23 s
Description: Source: Kummari, E., et. al., Laser Capture Microdissection - A Demonstration of the Isolation of Individual Dopamine Neurons and the Entire Ventral ...

eoe sub articles

EoE Sub Articles

All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.&#160; &#160; &#160; &#160;1. Preparation of Slides and Tissue<ol><li>Use either Silane-prep slides or polyethylene napthalate (PEN) membrane glass slides.</li><li>For RNA isolation, dip slides in RNase decontamination solution, wash 3 times with RNase-free water then dehydrate with a graded series of RNase-free ethanol and vacuum dry for 30 min.</li><li>Cut tissue sections at 10 &#181;m thickness using a cryostat and mount on the prepared RNase free slides. Keep the sections frozen during sectioning to preserve RNA quality. NOTE: Be sure that the tissue is approximately 4 mm away from the edges of the slide as the LCM cannot remove tissue that is too close to the edges of the slide. In order to remove tissue from a PEN membrane slide, ensure that the tissue is 4 mm from the left, top and bottom and 7 mm from the right side of the slide which are the dimensions of the membrane that is not attached to the slide.</li><li>For isolation of individual cell populations using direct immunohistochemistry, section tissue onto either the Silane-prep slides or PEN membrane slides. For isolation of regions of tissue using indirect immunohistochemistry guided techniques, mount one set of sections on a Silane-prep slide for immunohistochemistry and alternate sections on either a PEN membrane slide and/or a Silane-prep slide to be used for LCM.</li></ol>2. Tissue Preparation for Laser Capture &#8211; Rapid Tyrosine Hydroxylase Immunohistochemistry for Direct Laser Capture of Immunoreactive Cells<ol><li>Outline tissue with a hydrophobic pen and allow to dry.</li><li>Fix tissue in acetone-methanol (1:1) solution at -20 &#176;C for 10 min. NOTE: Our experience has shown that the acetone-methanol fixation resulted in much more consistent immunohistochemistry than acetone or methanol alone.</li><li>Rinse slide in phosphate buffered saline (PBS) with 1% Triton (RNase free).</li><li>Cover sections with 100-200 &#181;l PBS with 1% Triton with tyrosine hydroxylase antibody diluted 1:100 with 400 U/ml RNasin. Incubate for 5-10 min.</li><li>Rinse briefly in PBS twice and PBS-1% Triton.</li><li>Cover tissue with 100-200 &#181;l of goat anti-Rabbit IgG labeled with Alexa Fluor 488 diluted 1:100 in PBS-1% Triton with 400 U/ml RNasin and 50 ng/ml DAPI. Incubate for 5 min.</li><li>Rinse 2 times in PBS then dehydrate 30 s in a graded series of RNase free ethanol (75%-75%-95%-95%-100%-100%).</li><li>Incubate in two washes of Xylene for 1 min then 5 min.</li><li>Remove slides from Xylene immediately prior to use for LCM and allow to air dry.</li></ol>

<figure class='table' style='width:691pt;'><table class='ck-table-resized'><colgroup><col style='width:39.07%;'><col style='width:34.01%;'><col style='width:26.92%;'></colgroup><tbody><tr><td style='height:14.5pt;'>Silane prep-slides</td><td>Sigma-Aldrich, St. Louis, MO</td><td>S4651</td></tr><tr><td style='height:14.5pt;'>95% Ethanol-RNase Free</td><td>Sigma-Aldrich, St. Louis, MO</td><td>E7148</td></tr><tr><td style='height:14.5pt;'>100% Ethanol-RNase Free</td><td>Sigma-Aldrich, St. Louis, MO</td><td>E7023</td></tr><tr><td style='height:14.5pt;width:270pt;'>Rnase Free Triton</td><td style='width:235pt;'>Sigma-Aldrich, St. Louis, MO</td><td style='width:186pt;'>T8787</td></tr><tr><td style='height:14.5pt;'>Anti-Tyrosine hydroxyase antibody</td><td>EDM Millipore, Billerica, MA</td><td>Ab152</td></tr><tr><td style='height:14.5pt;'>Alexa Fluor 488 goat anti-rabbit IgG</td><td>Life Technologies, Grand Island, NY</td><td>A-11008</td></tr><tr><td style='height:14.5pt;width:270pt;'>RNaseZap</td><td style='width:235pt;'>Life Technologies, Grand Island, NY</td><td style='width:186pt;'>AM9780</td></tr></tbody></table></figure>

immunohistochemistry of mouse brain tissue sections for targeting dopamine neurons

<a href='https://app-jove-com.bdigitaluss.remotexs.co/v/52336/laser-capture-microdissection-demonstration-isolation-individual'>Source: Kummari, E., et. al., Laser Capture Microdissection - A Demonstration of the Isolation of Individual Dopamine Neurons and the Entire Ventral Tegmental Area., J. Vis. Exp. (2015)</a>In this video, we demonstrate the immunohistochemistry protocol for dopamine neurons in brain tissue sections for subsequent laser capture microdissection.

Immunohistochemistry of Mouse Brain Tissue Sections for Targeting Dopamine Neurons

Source: Kummari, E., et. al., Laser Capture Microdissection - A Demonstration of the Isolation of Individual Dopamine Neurons and the Entire Ventral ...

Take a polymer-coated slide with mouse brain tissue sections containing dopamine neurons expressing tyrosine hydroxylase, a key enzyme for dopamine synthesis. Outline the sections with a hydrophobic pen to ensure uniform staining.&#160; Fix the tissue in an acetone-methanol solution to preserve tissue morphology.&#160; Rinse with buffer containing detergent to permeabilize cell membranes. Incubate with primary antibodies targeting tyrosine hydroxylase in dopamine neurons, then wash to remove unbound antibodies. Add fluorescent dye-tagged secondary antibodies, nuclear dye, and RNase inhibitors. During incubation, secondary antibodies bind to primary antibodies, nuclear dyes label the nucleus, and RNase inhibitors inactivate RNases. Rinse with buffer. Then, dehydrate the tissue sections in increasing concentrations of ethanol. Incubate in xylene to clear the tissue. The processed tissue sections are now ready for laser capture microdissection, which allows precise visualization and dissection of target dopamine neurons.

immunohistochemistry-mouse-brain-tissue-sections-for-targeting

CrossRef

Research

JoVE Encyclopedia of Experiments

Neuroscience

Neuropathology

Neurodegenerative Diseases

42 Views. Source: Kummari, E., et. al., Laser Capture Microdissection - A Demonstration of the Isolation of Individual Dopamine Neurons and the Entire Ventral Tegmental Area., J. Vis. Exp. (2015) In this video, we demonstrate the immunohistochemistry protocol for dopamine neurons in brain tissue sections for subsequent laser capture microdissection. 

Video: Immunohistochemistry of Mouse Brain Tissue Sections for Targeting Dopamine Neurons - Concept

Laser-capture Microdissection of Human Prostatic Epithelium for RNA Analysis

The prostate gland contains a heterogeneous milieu of stromal, epithelial, neuroendocrine and immune cell types. Healthy prostate is comprised of fibromuscular stroma surrounding discrete epithelial-lined secretory lumens and a very small population of immune and neuroendocrine cells. In contrast, areas of prostate cancer have increased dysplastic luminal epithelium with greatly reduced or absent stromal population. Given the profound difference between stromal and epithelial cell types, it is imperative to separate the cell types for any type of downstream molecular analysis. Despite this knowledge, the bulk of gene expression studies compare benign prostate to cancer without micro-dissection, leading to stromal bias in the benign samples. Laser-capture micro-dissection (LCM) is an effective method to physically separate different cell types from a specimen section. The goal of this protocol is to show that RNA can be successfully isolated from LCM-collected human prostatic epithelium and used for downstream gene expression studies such as RT-qPCR and RNAseq.

The goal of this protocol is to use laser-capture micro-dissection as an effective method to isolate pure populations of cell types from heterogeneous prostate tissues for downstream RNA analysis.

The prostate gland contains a heterogeneous milieu of stromal, epithelial, neuroendocrine and immune cell types.  Healthy prostate is comprised of ...

JoVE Journal

Medicine

RNA Isolation from Cell Specific Subpopulations Using Laser-capture Microdissection Combined with Rapid Immunolabeling

Laser capture microdissection (LCM) allows the isolation of specific cells from thin tissue sections with high spatial resolution. Effective LCM requires precise identification of cells subpopulations from a heterogeneous tissue. Identification of cells of interest for LCM is usually based on morphological criteria or on fluorescent protein reporters. The combination of LCM and rapid immunolabeling offers an alternative and efficient means to visualize specific cell types and to isolate them from surrounding tissue. High-quality RNA can then be extracted from a pure cell population and further processed for downstream applications, including RNA-sequencing, microarray or qRT-PCR. This approach has been previously performed and briefly described in few publications. The goal of this article is to illustrate how to perform rapid immunolabeling of a cell population while keeping RNA integrity, and how to isolate these specific cells using LCM. Herein, we illustrated this multi-step procedure by immunolabeling and capturing dopaminergic cells in brain tissue from one-day-old mice. We highlight key critical steps that deserve special consideration. This protocol can be adapted to a variety of tissues and cells of interest. Researchers from different fields will likely benefit from the demonstration of this approach.

Gene expression analysis of a subset of cells in a specific tissue represents a major challenge. This article describes how to isolate high-quality total RNA from a specific cell population by combining a rapid immunolabeling method with laser capture microdissection.

Laser capture microdissection (LCM) allows the isolation of specific cells from thin tissue sections with high spatial resolution. Effective LCM requires ...

Biology

Laser-assisted Microdissection (LAM) as a Tool for Transcriptional Profiling of Individual Cell Types

The understanding of developmental processes at the molecular level requires insights into transcriptional regulation, and thus the transcriptome, at the level of individual cell types. While the methods described here are generally applicable to a wide range of species and cell types, our research focuses on plant reproduction. Plant cultivation and seed production is of crucial importance for human and animal nutrition. A detailed understanding of the regulatory networks that govern the formation of the reproductive lineage (germline) and ultimately of seeds is a precondition for the targeted manipulation of plant reproduction. In particular, the engineering of apomixis (asexual reproduction through seeds) into crop plants promises great improvements, as it leads to the formation of clonal seeds that are genetically identical to the mother plant. Consequently, the cell types of the female germline are of major importance for the understanding and engineering of apomixis. However, as the corresponding cells are deeply embedded within the floral tissues, they are very difficult to access for experimental analyses, including cell-type specific transcriptomics. To overcome this limitation, sections of individual cells can be isolated by laser-assisted microdissection (LAM). While LAM in combination with transcriptional profiling allows the identification of genes and pathways active in any cell type with high specificity, establishing a suitable protocol can be challenging. Specifically, the quality of RNA obtained after LAM can be compromised, especially when small, single cells are targeted. To circumvent this problem, we have established a workflow for LAM that reproducibly results in high RNA quality that is well suitable for transcriptomics, as exemplified here by the isolation of cells of the female germline in apomictic Boechera. In this protocol, procedures are described for tissue preparation and LAM, also with regard to RNA extraction and quality control.

Laser-assisted Microdissection LAM as a Tool for Transcriptional Profiling of Individual Cell Types

Here we present a protocol for laser-assisted microdissection of specific plant cell types for transcriptional profiling. While the protocol is suitable for different species and cell types, the focus is on highly inaccessible cells of the female germline important for sexual and apomictic reproduction in the crucifer genus Boechera.

The understanding of developmental processes at the molecular level requires insights into transcriptional regulation, and thus the transcriptome, at the ...