quantifying newly generated neurons in rat brain tissue using the optical fractionator technique

Quantifying Newly Generated Neurons in Rat Brain Tissue Using the Optical Fractionator Technique

When ready to begin, immunostaining, allow the sections to come up to room temperature. Then use a paintbrush to transfer every fifth section from a series of hippocampal sections to 25-well staining nets placed in Petri dishes filled with PBS. There should be 8 to 12 sections per hippocampus for staining. Transfer the staining nets, containing the sections, to matching glass dishes, containing PBS, and wash the sections twice for 10 minutes in PBS.Then, incubate in 3% hydrogen peroxide for 20 minutes. After washing, move the sections through three hydrochloric acid solutions. Then, neutralize in 0.1 molar sodium tetraborate at room temperature for 20 minutes.After three 10-minute incubations in changes of washing buffer, transfer the sections to blocking solution for one hour at room temperature. Then, incubate the sections in mouse anti-BrdU, diluted 1 to 100 in blocking solution for 48 hours at 4 degrees Celsius.After the primary antibody incubation, wash three times for 10 minutes each in washing buffer, then incubate for 48 hours in horseradish peroxidase, diluted 1 to 10 in washing buffer. 48 hours later, transfer the sections to PBS for 10 minutes, and repeat for a total of five washes. After washing, transfer the sections to DAB solution for seven minutes. Then, transfer to DAB solution containing 0.02% hydrogen peroxide for 10 minutes.After a series of washes, mount the sections in numerical order on microscope slides. Allow to dry for approximately 30 minutes. Then, air dry the samples by placing them into a slide rack. Next, rehydrate the samples for 10 minutes in a slide staining dish containing distilled water.Then, transfer the slides to 0.02% crystal violet in distilled water for 15 minutes. After repeating the crystal violet stain, rehydrate the sections through an ethanol series. Then, clear the sections in xylene twice for 15 minutes each time. Finally, add rapid drying mounting medium, and coverslip the slides.After 24 hours, the slides can be used for microscopy. Begin by checking the thickness of the tissue by first placing the slides on the motorized stage of the microscope, and then opening the stereology software. Delineate the area of interest using a low magnification objective before changing to a 100x oil immersion objective.Then, pick a specific point in accounting frame, for example, an area adjacent to a corner, and locate the top of the section by moving along the focal plane until some feature of the section appears in focus. Register this z position as 0. Next, move the focal plane down through the tissue until the last z level of tissue is in focus, then mark this position. The local tissue thickness is defined from 0 to this endpoint, and can be read on the z-axis.Register the tissue thickness. The tissue thickness is measured in several places within the region of interest. The height of the dissector and the guard zones, the size of the counting, frame the step length, and the final magnification is determined in a pilot study. Now, you can begin to count the BrdU-positive neurons, usually at a final magnification of 2,000 to 3,000x, using a 60x oil, or 100x oil objective, and a high numerical aperture.Identify BrdU-positive neurons in each counting frame, but do not count those that touch the red exclusion line. Count those BrdU-positive neurons that touch the green inclusion line, and those that fall within the boundary of the counting frame. Only count BrdU-positive neurons when the feature of interest is clearly recognized within the dissector height. The semi-visible neurons shown here are not counted.

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buffer</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Capital Region Pharmacy, DK</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>866533</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>0.1 mol/l, pH 7.4</td></tr><tr style='height:20px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Rapid drying mounting medium</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Histolab Products AB</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>801</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Pertex</td></tr><tr style='height:21px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Sodium Tetraborate</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Merck A/S</td><td 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style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>VWR</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>48311-703</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>SuperFrost+</td></tr><tr style='height:21px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Motorized stage</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Prior</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>H101A</td><td style='overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr><tr style='height:21px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Multidish Containers</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Sigma-Aldrich</td><td style='font-size:12pt;overflow:hidden;padding:0px 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style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Objective 4x</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Nikon</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>CFI Plan Fluor 4X</td><td style='overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr><tr style='height:21px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Objective 10x</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Nikon</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>CFI Plan Fluor 10X</td><td style='overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr><tr style='height:21px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Objective 100x oil immersion</td><td style='font-size:12pt;overflow:hidden;padding:0px 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style='overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr><tr style='height:21px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Slide staining dishes</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Sakura</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>4457</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Tissue-Tek</td></tr><tr style='height:21px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Specimen disc</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Leica</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>14037008637</td><td style='overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr><tr style='height:21px;'><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Staining nets</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Brain Research Laboratories</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>2512</td><td style='font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>25-wells</td></tr></tbody></table></figure>

Source:<a style='text-decoration:none;' href='https://app.jove.com/v/55737/the-optical-fractionator-technique-to-estimate-cell-numbers-in-a-rat-model-of-electroconvulsive-therapy'><span style='-webkit-text-decoration-skip:none;font-family:Arial,sans-serif;font-size:12pt;font-style:normal;font-variant:normal;font-weight:400;text-decoration-skip-ink:none;vertical-align:baseline;white-space:pre-wrap;'> Olesen, M. V.,&#160;et al<span style='-webkit-text-decoration-skip:none;font-family:Arial,sans-serif;font-size:12pt;font-style:normal;font-variant:normal;font-weight:400;text-decoration-skip-ink:none;vertical-align:baseline;white-space:pre-wrap;'>. The Optical Fractionator Technique to Estimate Cell Numbers in a Rat Model of Electroconvulsive Therapy.&#160;J. Vis. Exp.<span style='-webkit-text-decoration-skip:none;font-family:Arial,sans-serif;font-size:12pt;font-style:normal;font-variant:normal;font-weight:400;text-decoration-skip-ink:none;vertical-align:baseline;white-space:pre-wrap;'> (2017).</a> &#160;The video demonstrates the technique for quantifying newly generated neurons in brain tissue. Hippocampal tissue slices containing Bromodeoxyuridine (BrdU)-labeled neurons were stained using immunohistochemistry and subsequently quantified across the tissue thickness using the optical fractionator technique.

<figure class='image image-style-align-center image_resized' style='display:table;margin-left:auto;margin-right:auto;width:75%;'><img style='aspect-ratio:1954/1106;' src='https://cloudfront.jove.com/files/ftp_upload/23449/23449_Figure_1_editor_23449.jpg' alt='23449_Figure_1.jpg' /></figure>Figure 1: Schematic illustration showing tissue processing according to the fractionator principles used in the present study. The hemispheres are separated following experimentation, and the right or left hemisphere chosen is systematically and randomly (A). The complete brain extending over the entire hippocampus is cut into 80-&#181;m-thick coronal sections (B), and each 5th section is sub-sampled, starting randomly between sections 1 to 5, for final immunostaining and stereological quantification (C).<figure class='image image-style-align-center image_resized' style='display:table;margin-left:auto;margin-right:auto;width:75%;'><img style='aspect-ratio:1964/1548;' src='https://cloudfront.jove.com/files/ftp_upload/23449/23449_Figure_2_editor_23449.jpg' alt='23449_Figure_2.jpg' /></figure><meta charset='utf-8'>Figure 2:&#160;Illustration showing the stereological sampling procedure using optical dissectors. (A) Following histological processing, the hippocampal GCL/SGZ was delineated, and optical dissectors were applied uniformly and randomly over the region. (B) In the optical dissectors (left), the BrdU-positive neurons were counted only if their features of interest were recognized within the dissector height and located inside the counting frame or touching the inclusion line (right). Neurons touching the exclusion line were not counted. Scale bars = 10 &#181;m.

Source: Olesen, M. V.,&#160;et al. The Optical Fractionator Technique to Estimate Cell Numbers in a Rat Model of Electroconvulsive Therapy.&#160;J. Vis. ...

Take hippocampal brain slices from a rat injected with Bromodeoxyuridine, or BrdU, a nucleoside analog of thymidine.BrdU integrates into DNA during cell division, labeling newly generated neurons within the dentate gyrus, a region for neurogenesis.&#160;Incubate with an oxidizing agent to inactivate endogenous peroxidase enzymes.Treat with acid to denature DNA and expose BrdU, then neutralize the acid.Incubate with a detergent to permeabilize cellular membranes and a blocking solution to mask non-specific binding sites.Incubate with primary antibodies targeting BrdU, followed by peroxidase-tagged secondary antibodies specific to the primary antibodies.Introduce a chromogenic substrate and an oxidizing agent, allowing peroxidase to convert the substrate into a colored residue.Mount the tissue and counterstain with a nucleic acid-binding dye.Dehydrate the tissue, then treat it to increase transparency.Under a microscope, identify the dentate gyrus.Using the optical fractionator technique, analyze multiple planes across the tissue thickness to quantify BrdU-labeled neurons.

10 Görüntüleme. Quantifying Newly Generated Neurons in Rat Brain Tissue Using the Optical Fractionator Technique

Video: Quantifying Newly Generated Neurons in Rat Brain Tissue Using the Optical Fractionator Technique - Deney

Stereological Estimation of Dopaminergic Neuron Number in the Mouse Substantia Nigra Using the Optical Fractionator and Standard Microscopy Equipment

In pre-clinical Parkinson&#39;s disease research, analysis of the nigrostriatal tract, including quantification of dopaminergic neuron loss within the substantia nigra, is essential. To estimate the total dopaminergic neuron number, unbiased stereology using the optical fractionator method is currently considered the gold standard. Because the theory behind the optical fractionator method is complex and because stereology is difficult to achieve without specialized equipment, several commercially available complete stereology systems that include the necessary software do exist, purely for cell counting reasons. Since purchasing a specialized stereology setup is not always feasible, for many reasons, this report describes a method for the stereological estimation of dopaminergic neuronal cell counts using standard microscopy equipment, including a light microscope, a motorized object table (x, y, z plane) with imaging software, and a computer for analysis. A step-by-step explanation is given on how to perform stereological quantification using the optical fractionator method, and pre-programmed files for the calculation of estimated cell counts are provided. To assess the accuracy of this method, a comparison to data obtained from a commercially available stereology apparatus was performed. Comparable cell numbers were found using this protocol and the stereology device, thus demonstrating the precision of this protocol for unbiased stereology.

This work presents a step-by-step protocol for the unbiased stereological estimation of dopaminergic neuronal cell numbers in the mouse substantia nigra using standard microscopy equipment (i.e., a light microscope, a motorized object table (x, y, z plane), and public domain software for digital image analysis.

Optik Fractionator ve standart mikroskobu ekipmanlar kullanarak fare gözlemliyorum Nigra dopaminerjik nöron sayısının stereological tahmin

In pre-clinical Parkinson&#39;s disease research, analysis of the nigrostriatal tract, including quantification of dopaminergic neuron loss within the ...

JoVE Journal

Nörobilim

Combining Multiplex Fluorescence In Situ Hybridization with Fluorescent Immunohistochemistry on Fresh Frozen or Fixed Mouse Brain Sections

Fluorescent in situ hybridization (FISH) is a molecular technique that identifies the presence and spatial distribution of specific RNA transcripts within cells. Neurochemical phenotyping of functionally identified neurons usually requires concurrent labelling with multiple antibodies (targeting protein) using immunohistochemistry (IHC) and optimization of in situ hybridization (targeting RNA), in tandem. A &#34;neurochemical signature&#34; to characterize particular neurons may be achieved however complicating factors include the need to verify FISH and IHC targets before combining the methods, and the limited number of RNAs and proteins that may be targeted simultaneously within the same tissue section.
Here we describe a protocol, using both fresh frozen and fixed mouse brain preparations, which detects multiple mRNAs and proteins in the same brain section using RNAscope FISH followed by fluorescence immunostaining, respectively. We use the combined method to describe the expression pattern of low abundance mRNAs (e.g., galanin receptor 1) and high abundance mRNAs (e.g., glycine transporter 2), in immunohistochemically identified brainstem nuclei.
Key considerations for protein labelling downstream of the FISH assay extend beyond tissue preparation and optimization of FISH probe labelling. For example, we found that antibody binding and labelling specificity can be detrimentally affected by the protease step within the FISH probe assay. Proteases catalyze hydrolytic cleavage of peptide bonds, facilitating FISH probe entry into cells, however they may also digest the protein targeted by the subsequent IHC assay, producing off target binding. The subcellular location of the targeted protein is another factor contributing to IHC success following FISH probe assay. We observed IHC specificity to be retained when the targeted protein is membrane bound, whereas IHC targeting cytoplasmic protein required extensive troubleshooting. Finally, we found handling of slide-mounted fixed frozen tissue more challenging than fresh frozen tissue, however IHC quality was overall better with fixed frozen tissue, when combined with RNAscope.

Combining Multiplex Fluorescence In Situ Hybridization with Fluorescent Immunohistochemistry on Fresh Frozen or Fixed Mouse Brain Sections

This protocol describes a method for combining fluorescence in situ hybridization (FISH) and fluorescence immunohistochemistry (IHC) in both fresh frozen and fixed mouse brain sections, with the goal of achieving multilabel FISH and fluorescence IHC signal. IHC targeted cytoplasmic and membrane attached proteins.

Multipleks Floresan In Situ Hibridizasyonun Floresan İmmünohistokimya ile Taze Dondurulmuş veya Sabit Fare Beyin Kesitlerinde Birleştirilmesi

Fluorescent in situ hybridization (FISH) is a molecular technique that identifies the presence and spatial distribution of specific RNA transcripts within ...

Immunohistochemistry Techniques to Analyze Cellular Proliferation and Neurogenesis in Rats Using the Thymidine Analog BrdU

One of the most important things in the field of adult hippocampal neurogenesis (AHN) is the identification of the newly generated cells. The immunodetection of thymidine analogs (such as 5-Bromo-2&#39;-deoxyuridine (BrdU)) is a standard technique used for visualizing these newly generated cells. Therefore, BrdU is usually injected in small animals intraperitoneally, so the thymidine analog gets incorporated into dividing cells during DNA synthesis. Detection is performed by immunohistochemical analysis of brain slices. Every research group that has been using this technique can appreciate that it requires special attention to minute details to achieve a successful stain. For instance, an important step is DNA denaturation with HCl, which allows it to reach the cell nucleus to stain it. However, the existing scientific reports describe very few of such steps in detail. Therefore, standardizing the technique is challenging for new laboratories as it can take several months to yield positive and successful outcomes. The purpose of this work is to describe and elaborate the steps to obtain positive and successful outcomes of the immunostaining technique in detail when working with the thymidine analog BrdU. The protocol includes the reagent preparation and setup, administration of thymidine analog in a rodent, transcardial perfusion, tissue preparation, peroxidase immunohistochemical reaction, use of avidin-biotin complex, immunofluorescence, counterstaining, microscopy imaging, and cell analysis.

This paper presents four of the most common techniques for visualizing BrdU positive cells to measure adult neurogenesis in rats. This work includes instructions for reagent preparation, thymidine analog administration, transcardial perfusion, tissue preparation, peroxidase immunohistochemical reaction, immunofluorescence, signal amplification, counterstaining, microscopy imaging, and cell analysis.

Quantifying Newly Generated Neurons in Rat Brain Tissue Using the Optical Fractionator Technique

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Quantifying Newly Generated Neurons in Rat Brain Tissue Using the Optical Fractionator Technique