Name: ultrastructural analysis of a mouse brain section using transmission electron microscopy
Uploaded: 2025-04-28T11:36:59.000+00:00
Duration: 1 min 19 s
Description: Source: Lutz, D., et.al. Assessment of Ultrastructural Neuroplasticity Parameters After In Utero Transduction of the Developing Mouse Brain and Spinal ...

ultrastructural analysis of a mouse brain section using transmission electron microscopy

Ultrastructural Analysis of a Mouse Brain Section Using Transmission Electron Microscopy

To map an area of interest, select an image containing the area of interest from the previously prepared image atlas. Sketch the borders of the area of interest onto the sectioned image. Optically superimpose these borders onto the embedded specimen under the microscope, and use a one-inch 26 gauge needle to scratch these region borders onto the resin specimen. Then, heat the specimens to 95 degrees Celsius in order to soften the resin.Next, take out the warm resin specimens from the oven, and use a razor blade to excise the areas of interest. Glue the specimens onto acrylic glass holding bars of the appropriate caliber, and trim the mounted specimens for semi and ultra thin sectioning. Use an ultramicrotome to acquire semi thin 0.7 micrometer and ultra thin 70 nanometer sections, collecting the semi thin sections on glass carriers and the ultra thin sections on nickel grids.Stain the semi thin sections with 1% toluidine blue in PBS for four minutes, followed by several washes in deionized water before examining the sections by light microscopy. The ultra thin sections can then be directly assessed by transmission electron microscopy at 180 kilovolts, without further modification.

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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.1. Selection of Ultrastructural Neuroplasticity Parameters for Quantitative Analysis<ol><li>Mapping the area of interest<ol style='list-style-type:decimal;'><li>Choose an area of interest (e.g., hippocampus or cerebellum) and localize the area in the section atlas by choosing the image from the atlas that contains this area.</li><li>Sketch the borders of the area of interest onto the section image and find/superimpose these region borders onto the resin specimen.</li><li>Scratch-mark the borders of the area of interest (e.g., hippocampus or cerebellum) on the resin specimen, using a fine needle gauge (26 G, 1 in).</li><li>Heat the resin specimen to 85 &#176;C in an oven to soften the resin for trimming or, alternatively, use a trimming device, a thin blade, or sandpaper.</li><li>Excise the area of interest from the resin specimen with a razor blade. Mount the specimen on holding bars of acrylic glass of the required caliber (e.g., with a diameter of 8 mm and a length of 1 cm) with glue. Trim the mounted specimen for semi- and ultrathin sectioning.</li><li>Prepare semithin (0.75 &#181;m) and ultrathin (70 nm) sections of the trimmed area using an ultramicrotome: set it at 1.5 mm/s for 0.75 &#181;m thickness and at 0.7 mm/s for 70 nm thickness.</li><li>Collect the semithin sections on glass carriers and stain the sections with 1% toluidine blue in PBS (for 4 min).</li><li>Wash the sections several times in deionized water. Examine the stained sections under the light microscope using 4x (NA of 0.1 &#8734;/-), 10x (NA of 0.22 &#8734;/0.17), 40x (NA of 0.65 &#8734;/0.17), and 100x (NA of 1.25 &#8734;/0.17) objectives.</li><li>Collect ultrathin sections on nickel grids. Subject the grids to TEM at 180 kV and at 3,200x, 6,000x, and/or 8,000x magnification.</li></ol></li><li>TEM Analysis<ol style='list-style-type:decimal;'><li>Choose the ultrastructural parameters of interest for quantitative TEM analysis (e.g., boutons with vesicles and mitochondria or myelinated and nonmyelinated axons) and take TEM images of these parameters under 3,500x, 6,000x and/or 8,000x magnification.</li></ol></li></ol>

<figure class='table' style='width:1045pt;'><table class='ck-table-resized'><colgroup><col style='width:18.09%;'><col style='width:17.13%;'><col style='width:23.92%;'><col style='width:40.86%;'></colgroup><tbody><tr><td style='height:15.75pt;width:189pt;'>Light microscope Basic DM E</td><td style='width:179pt;'>Leica</td><td style='width:250pt;'>-</td><td style='width:427pt;'>4x (N.A. 0.1 &#8734;/-), 10x (N.A. 0.22 &#8734;/0.17), 40x (N.A. 0.65 &#8734;/0.17), 100x (N.A. 1.25 &#8734;/0.17) objectives</td></tr><tr><td style='height:15.75pt;width:189pt;'>Mosquito hemostatic forceps (12.5cm, curved)</td><td style='width:179pt;'>FST</td><td style='width:250pt;'>13010-12</td><td style='width:427pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:189pt;'>Nickel grids, 200 mesh</td><td style='width:179pt;'>Ted Pella</td><td style='width:250pt;'>1GC200</td><td style='width:427pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:189pt;'>Razor blades</td><td style='width:179pt;'>Schick</td><td style='width:250pt;'>87-10489</td><td style='width:427pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:189pt;'>Technovit 4004 two components glue</td><td style='width:179pt;'>Kulzer</td><td style='width:250pt;'>&#160;</td><td style='width:427pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:189pt;'>Thin vibrating razor blade device</td><td style='width:179pt;'>Krup</td><td style='width:250pt;'>-</td><td style='width:427pt;'>with Szabo thin blades</td></tr><tr><td style='height:15.75pt;width:189pt;'>Toluidine blue</td><td style='width:179pt;'>Sigma-Aldrich</td><td style='width:250pt;'>89640</td><td style='width:427pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:189pt;'>Transmission electron microscope C20</td><td style='width:179pt;'>Phillips</td><td style='width:250pt;'>-</td><td style='width:427pt;'>up to 200 kV</td></tr><tr><td style='height:15.75pt;width:189pt;'>Ultracut E</td><td style='width:179pt;'>Reichert-Jung</td><td style='width:250pt;'>-</td><td style='width:427pt;'>ultramicrotome</td></tr><tr><td style='height:15.75pt;width:189pt;'>Araldite</td><td style='width:179pt;'>CIBA-GEIGY</td><td style='width:250pt;'>23857.9</td><td style='width:427pt;'>resin for embedding of tissue</td></tr><tr><td style='height:15.75pt;'>Osmium (VIII)-oxid&#160;</td><td>Degussa&#160;</td><td>73219</td><td>&#160;</td></tr></tbody></table></figure>

<a href='https://app.jove.com/v/59084/assessment-ultrastructural-neuroplasticity-parameters-after-utero'>Source: Lutz, D., et.al. Assessment of Ultrastructural Neuroplasticity Parameters After In Utero Transduction of the Developing Mouse Brain and Spinal Cord. J. Vis. Exp. (2019).</a>This video demonstrates the preparation and transmission electron microscopy (TEM) analysis of a brain section from a mouse pup. The protocol starts with osmium tetroxide-fixed tissue embedded in resin, followed by precise trimming to isolate the region of interest and ultramicrotomy to produce semithin and ultrathin sections, which are visualized using light microscopy and TEM, respectively.

Source: Lutz, D., et.al. Assessment of Ultrastructural Neuroplasticity Parameters After In Utero Transduction of the Developing Mouse Brain and Spinal ...

Take an osmium tetroxide-fixed mouse brain section embedded in a resin block.Obtain a section image and align it with a pre-prepared atlas image to identify the region of interest.Mark the borders of this region on the block.Heat the resin to soften it and excise the marked region.Glue the specimen to a glass holding bar and trim it.Using an ultramicrotome, prepare semithin and ultrathin sections.Transfer the semithin and ultrathin sections onto glass carriers and nickel grids, respectively.Stain the semithin sections with a dye that binds to nucleic acids, ribosome-rich cytoplasm, and the extracellular matrix.Wash the sections and examine them under a light microscope to confirm the presence of the target area.Observe the ultrathin sections under a transmission electron microscope.Osmium tetroxide enhances the electron density of cellular and organelle membranes, providing high contrast against the less electron-dense cytoplasm, enabling visualization of cellular ultrastructure.

11 조회수. Ultrastructural Analysis of a Mouse Brain Section Using Transmission Electron Microscopy

비디오: Ultrastructural Analysis of a Mouse Brain Section Using Transmission Electron Microscopy - 실험

Large-scale Scanning Transmission Electron Microscopy (Nanotomy) of Healthy and Injured Zebrafish Brain

Large-scale 2D electron microscopy (EM), or nanotomy, is the tissue-wide application of nanoscale resolution electron microscopy. Others and we previously applied large scale EM to human skin pancreatic islets, tissue culture and whole zebrafish larvae1-7. Here we describe a universally applicable method for tissue-scale scanning EM for unbiased detection of sub-cellular and molecular features. Nanotomy was applied to investigate the healthy and a neurodegenerative zebrafish brain. Our method is based on standardized EM sample preparation protocols: Fixation with glutaraldehyde and osmium, followed by epoxy-resin embedding, ultrathin sectioning and mounting of ultrathin-sections on one-hole grids, followed by post staining with uranyl and lead. Large-scale 2D EM mosaic images are acquired using a scanning EM connected to an external large area scan generator using scanning transmission EM (STEM). Large scale EM images are typically ~ 5 - 50 G pixels in size, and best viewed using zoomable HTML files, which can be opened in any web browser, similar to online geographical HTML maps. This method can be applied to (human) tissue, cross sections of whole animals as well as tissue culture1-5. Here, zebrafish brains were analyzed in a non-invasive neuronal ablation model. We visualize within a single dataset tissue, cellular and subcellular changes which can be quantified in various cell types including neurons and microglia, the brain&#39;s macrophages. In addition, nanotomy facilitates the correlation of EM with light microscopy (CLEM)8 on the same tissue, as large surface areas previously imaged using fluorescent microscopy, can subsequently be subjected to large area EM, resulting in the nano-anatomy (nanotomy) of tissues. In all, nanotomy allows unbiased detection of features at EM level in a tissue-wide quantifiable manner.

Large-scale Scanning Transmission Electron Microscopy Nanotomy of Healthy and Injured Zebrafish Brain

Large-scale 2D electron microscopy (EM), or nanotomy, is the tissue-wide application of nanoscale resolution EM. Here we describe a universal method for nanotomy applied to investigate the zebrafish larval brain in health and upon non-invasive brain injury.

건강 및 부상 Zebrafish의 두뇌의 대규모 스캐닝 투과 전자 현미경 (Nanotomy)

Large-scale 2D electron microscopy (EM), or nanotomy, is the tissue-wide application of nanoscale resolution electron microscopy. Others and we previously ...

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Preparation of Newborn Rat Brain Tissue for Ultrastructural Morphometric Analysis of Synaptic Vesicle Distribution at Nerve Terminals

Our laboratory and many others have exploited the high resolving power of transmission electron microscopy to study the morphology and spatial organization of synaptic vesicles. In order to obtain high-quality electron micrographs that can yield the degree of morphological detail necessary for quantitative analysis of pre-synaptic vesicle distribution, optimal specimen preparation is critical. Chemical fixation is the first step in the process of specimen preparation, and of utmost importance to preserve fine ultrastructure. Vascular fixation with a glutaraldehyde-formaldehyde solution, followed by treatment of vibratome-sectioned specimens with osmium tetroxide, stabilizes the maximum number of molecules, especially proteins and lipids, and results in superior conservation of ultrastructure. Tissue is then processed with counterstaining, sequential dehydration and resin-embedding. En bloc staining with uranyl acetate (i.e., staining of vibratome-sectioned tissue before resin embedding) enhances endogenous contrast and stabilizes cell components against extraction during specimen processing. Contrast can be further increased by applying uranyl acetate as a post-stain on ultrathin sections. Double-staining of ultrathin sections with lead citrate after uranyl acetate treatment also improves image resolution, by intensifying electron-opacity of nucleic acid-containing structures through selective binding of lead to uranyl acetate. Transmission electron microscopy is a powerful tool for characterization of the morphological details of synaptic vesicles and quantification of their size and spatial organization in the terminal bouton. However, because it uses fixed tissue, transmission electron microscopy can only provide indirect information regarding living or evolving processes. Therefore, other techniques should be considered when the main objective is to study dynamic or functional aspects of synaptic vesicle trafficking and exocytosis.

We describe procedures for processing newborn rat brain tissue to obtain high-resolution electron micrographs for morphometric analysis of synaptic vesicle distribution at nerve terminals. The micrographs obtained with these methods can also be used to study the morphology of a number of other cellular components and their dimensional structural relationships.

신경 말단에서 시 냅 스 소포 분포의 미세 구조 형태학 적 분석을 위한 신생아 쥐 뇌 조직의 제조

Our laboratory and many others have exploited the high resolving power of transmission electron microscopy to study the morphology and spatial ...

신경과학

Preparation and Observation of Thick Biological Samples by Scanning Transmission Electron Tomography

This report describes a protocol for preparing thick biological specimens for further observation using a scanning transmission electron microscope. It also describes an imaging method for studying the 3D structure of thick biological specimens by scanning transmission electron tomography. The sample preparation protocol is based on conventional methods in which the sample is fixed using chemical agents, treated with a heavy atom salt contrasting agent, dehydrated in a series of ethanol baths, and embedded in resin. The specific imaging conditions for observing thick samples by scanning transmission electron microscopy are then described. Sections of the sample are observed using a through-focus method involving the collection of several images at various focal planes. This enables the recovery of in-focus information at various heights throughout the sample. This particular collection pattern is performed at each tilt angle during tomography data collection. A single image is then generated, merging the in-focus information from all the different focal planes. A classic tilt-series dataset is then generated. The advantage of the method is that the tilt-series alignment and reconstruction can be performed using standard tools. The collection of through-focal images allows the reconstruction of a 3D volume that contains all of the structural details of the sample in focus.

This report describes a sample preparation protocol and specific imaging conditions for performing scanning transmission electron tomography of thick biological specimens.

주사 투과 전자 단층 촬영에 의해 준비 및 두꺼운 생물 샘플의 관측

This report describes a protocol for preparing thick biological specimens for further observation using a scanning transmission electron microscope. It ...

Ultrastructural Analysis of a Mouse Brain Section Using Transmission Electron Microscopy

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Ultrastructural Analysis of a Mouse Brain Section Using Transmission Electron Microscopy