eoe sub articles

EoE Sub Articles

All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.1. Golgi-Cox Staining<ol><li>Golgi-Cox Impregnation of Brains<ol style='list-style-type:decimal;'><li>Make the Golgi-Cox solution of 1% (w/v) potassium dichromate, 0.8% (w/v) potassium chromate, and 1% (w/v) mercuric chloride by dissolving the potassium dichromate and potassium chromate separately in high-quality water. Mix the solutions, add the mercuric chloride, and filter the final solution using grade 1 filter paper. Store the solution in the dark for up to one month.</li><li>Anesthetize the mouse using 5% isoflurane.</li><li>Euthanize the mouse by decapitation and quickly remove the brain.</li><li>Place the brain into a 20 mL glass scintillation vial containing 17 mL Golgi-Cox solution and incubate in the dark at RT for 25 d.</li><li>Cryoprotect the brain by placing it into a 50 mL conical tube containing 40 mL of sucrose cryoprotectant (30% (w/v) sucrose in 0.1 M phosphate buffer, pH 7.4) in the dark at 4 &#176;C for 24 h. NOTE:&#160;The following optional three steps may be employed as an alternative to the main protocol, in order to freeze the brain at this stage for long-term storage.</li><li>Freeze the whole brain by immersing it into 200 mL isopentane precooled on dry ice.</li><li>Place the frozen brain into a 50 mL conical tube and store it in the dark at -80 &#176;C.</li><li>When ready to proceed, thaw the brain by placing it into a 50 mL conical tube containing 40 mL of sucrose cryoprotectant and keeping it in the dark at 4 &#176;C for 24 h.</li></ol></li><li>Brain Sectioning<ol style='list-style-type:decimal;'><li>Remove the brain from the sucrose and block it for sectioning by cutting off the cerebellum using a razor blade and leaving a flat edge at the remaining caudal end of the brain.</li><li>Heat agar (3% (w/v) in water) until it is melted, then let it cool until it is slightly above its melting point.</li><li>Place the brain in a small disposable weigh dish with its caudal end face-down, and add a sufficient amount of melted agar to cover it.</li><li>Once the agar has solidified, trim excess agar, leaving approximately 2 - 4 mm surrounding the brain, and glue the brain to the stage of a vibratome with its caudal end face-down using a small amount of ethyl cyanoacrylate glue.</li><li>&#160;Fill the stage area of the vibratome with a sufficient amount of sucrose cryoprotectant to cover the brain, and section the brain at a slice thickness of 400 - 500 &#181;m (depending on the brain region to be examined) using a vibration frequency of 86 Hz and a blade advancement speed of 0.125 mm/s.</li><li>Using a small paint brush, place brain sections into a well of a 6-well tissue culture plate containing commercially available mesh-bottom inserts and pre-filled with 10 mL of 6% (w/v) sucrose in 0.1 M phosphate buffer, pH 7.4.</li><li>Incubate sections in the dark at 4 &#176;C O/N.</li></ol></li><li>Developing Brain Sections<ol style='list-style-type:decimal;'><li>Transfer brain sections into a new well containing 5 mL of 2% (w/v) paraformaldehyde (PBD) in 0.1 M phosphate buffer, pH 7.4, using the mesh-bottom inserts. Incubate on a rocker, moving slowly in the dark at RT for 15 min.</li><li>Sections should be washed twice by transferring them to new wells containing 5 mL of water. They should be washed on a rocker moving at a moderate speed in the dark at RT for 5 min.</li><li>Transfer sections into a new well containing 5 mL of 2.7% (v/v) ammonium hydroxide. Incubate on a rocker, moving slowly in the dark at RT for 15 min.</li><li>Sections should be washed twice by transferring them to new wells containing 5 mL of water. They should be washed on a rocker moving at a moderate speed in the dark at RT for 5 min.</li><li>Transfer sections into a new well containing 5 mL of Fixative A diluted in water 10x from its original purchased concentration. Incubate on a rocker, moving slowly in the dark at RT for 25 min.</li><li>Sections should be washed twice by transferring them to new wells containing 5 mL of water. They should be washed on a rocker moving at a moderate speed in the dark at RT for 5 min.</li></ol></li><li>Mounting Brain Sections<ol style='list-style-type:decimal;'><li>Using a small paintbrush, mount sections onto microscope slides. Using tweezers and a small tissue, remove excess water and agar. Ensure that all agar is removed before proceeding with dehydration.</li><li>Allow sections to air dry at RT for approximately 45 min (400 &#956;m sections) or 90 min (500 &#956;m sections). NOTE: The timing and proper level of dryness are critical and may need to be determined in each laboratory depending on ambient temperature and humidity. Too short a drying time leads to sections falling off of slides during subsequent dehydration steps, and too long a drying time leads to sections cracking. Sections will still appear to be shiny at the appropriate level of dryness.</li><li>Stain sections with cresyl violet by placing slides into Coplin staining jars as indicated. NOTE:&#160;This optional step may be employed for sections that have never been frozen to stain neuronal nuclei with cresyl violet. We have found that clearing and rehydrating sections before incubation in cresyl violet leads to even staining and low background across sections.<ol style='list-style-type:decimal;'><li>Place in clearing agent for 5 min. Repeat once.</li><li>Place in 100% ethanol for 5 min. Repeat once.</li><li>Place 95% ethanol in water, then 75% ethanol in water, and then 50% ethanol in water for 2 min each.</li><li>Place in water for 5 min.</li><li>Place in 0.5% (w/v) cresyl violet in water for 7 min.</li><li>Place in water for 2 min. Repeat once.</li></ol></li><li>Dehydrate sections by placing slides into Coplin staining jars as indicated.<ol style='list-style-type:decimal;'><li>Place in 50% ethanol in water, then 75% ethanol in water, and then 95% ethanol in water for 2 min each.</li><li>Place in 100% ethanol for 5 min. Repeat once.</li><li>Place in clearing agent for 5 min. Repeat once. NOTE: These dehydration and clearing times are sufficient to process mouse brains as described in this manuscript. However, we have observed that for other species, including rats and cowbirds, the final clearing step may need to be extended up to 15 minutes in total.</li></ol></li><li>Coverslip sections using an anhydrous mounting medium.</li><li>Allow slides to dry horizontally in the dark at RT for at least 5 d.</li></ol></li></ol>2. Imaging Stained Neurons within Thick Brain Sections<ol><li>Capturing Image Stacks<ol style='list-style-type:decimal;'><li>Turn on the microscope light bulb, camera, and stage controller.</li><li>Open the microscope software (e.g., Neurolucida).</li><li>Place a slide on the microscope stage.</li><li>Capture a 2D wide-view image of the brain section using a low magnification objective such as 1.25X 0.4 N.A. PlanAPO or 4X 0.16 N.A.<ol style='list-style-type:decimal;'><li>Focus on the image and adjust camera settings, including the exposure time and white balance.</li><li>Create a reference point by left-clicking anywhere on the section</li><li>Capture the image by selecting "acquire single image" within the image acquisition window.</li></ol></li><li>Capture mid-resolution image stacks of the area containing the neurons(s) of interest using a 10X 0.3 N.A. UPlan FL N objective.<ol style='list-style-type:decimal;'><li>Focus on the image and adjust camera settings, including the exposure and white balance.</li><li>Set the upper and lower boundaries for the image stack by focusing to the top of the section and selecting "set" next to "top of stack" within the image acquisition window, and then focusing to the bottom of the section and selecting "set" next to "bottom of stack" within the image acquisition window.</li><li>Set the step distance to 5 &#956;m by entering "5 &#956;m" next to "distance between images" within the image acquisition window.</li><li>Capture the image stack by selecting "acquire image stack" within the image acquisition window.</li><li>Repeat the above steps to capture the entire area of interest, ensuring that all image stacks overlap by at least 10% in the X and Y axes.</li></ol></li><li>Capture high-resolution image stacks of the area containing the neuron of interest using a 30X 1.05 N.A. silicone oil-immersion objective.<ol style='list-style-type:decimal;'><li>Apply 3 - 4 drops of silicone immersion oil to the slide and place the objective over the slide, ensuring contact between the objective and the oil.</li><li>Focus on the image and adjust camera settings, including the exposure and white balance.</li><li>Set the upper and lower boundaries for the image stack by focusing to the top of the section and selecting "set" next to "top of stack" within the image acquisition window, and then focusing to the bottom of the section and selecting "set" next to "bottom of stack" within the image acquisition window.</li><li>Set the step distance to 1 &#956;m by entering "1 &#956;m" next to "distance between images" within the image acquisition window.</li><li>Capture the image stack by selecting "acquire image stack" within the image acquisition window.</li><li>Repeat the above steps to capture the entire area of interest, ensuring that all image stacks overlap by at least 10% in the X and Y axes.</li></ol></li><li>Save the data file and all image files in TIFF format for external processing.</li></ol></li><li>Creating Z-projection Images and Image Montages<ol style='list-style-type:decimal;'><li>Create Z-projection images in ImageJ<ol style='list-style-type:decimal;'><li>Open ImageJ software that has the Bio-Formats plugin installed.</li><li>Select "Plugins" -&gt; "Bio-Formats" -&gt; "Bio-Formats Importer."</li><li>Select the image stack file to be opened.</li><li>Once the file is opened, change the format to RGB by selecting "Image" -&gt; "Type" -&gt; "RGB Color".</li><li>Create the Z-projection by selecting "Image" -&gt; "Stacks" -&gt; "Z Project&#8230;".</li><li>Save the two-dimensional Z-projection image as a TIFF file.</li></ol></li><li>Create a two-dimensional image montage of the entire area of interest.<ol style='list-style-type:decimal;'><li>Open the software (e.g., Adobe Photoshop).</li><li>Select "File" -&gt; "Automate" -&gt; "Photomerge".</li><li>Select "Browse" and then add all image files to be merged.</li><li>Ensure that "Blend Images" is selected and then select "OK".</li><li>Save the resulting montage image of the entire area of interest as a TIFF file.</li></ol></li></ol></li></ol>

<figure class='table' style='width:657pt;'><table class='ck-table-resized'><colgroup><col style='width:31.66%;'><col style='width:21.77%;'><col style='width:18.42%;'><col style='width:28.15%;'></colgroup><tbody><tr><td style='height:14.5pt;width:208pt;'>Potassium dichromate</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>P188-100</td><td style='width:185pt;'>Hazardous</td></tr><tr><td style='height:14.5pt;width:208pt;'>Potassium chromate</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>P220-100</td><td style='width:185pt;'>Hazardous</td></tr><tr><td style='height:14.5pt;width:208pt;'>Mercuric chloride</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>S25423</td><td style='width:185pt;'>Hazardous</td></tr><tr><td style='height:14.5pt;width:208pt;'>Whatman grade 1 filter paper</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>1001-185</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Isoflurane</td><td style='width:143pt;'>Pharmaceutical Partners of Canada</td><td style='width:121pt;'>CP0406V2</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>20 mL scintillation vial</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>03-337-4</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Sucrose</td><td style='width:143pt;'>Bioshop Canada</td><td style='width:121pt;'>SUC700.1</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Sodium phosphate monobasic</td><td style='width:143pt;'>Sigma Aldrich</td><td style='width:121pt;'>S5011-500G</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Sodium phosphate dibasic</td><td style='width:143pt;'>Sigma Aldrich</td><td style='width:121pt;'>S9390-500G</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>50 mL conical tube</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>12-565-271</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Isopentane</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>AC126470010</td><td style='width:185pt;'>also known as 2-methylbutane. Hazardous</td></tr><tr><td style='height:14.5pt;width:208pt;'>Agar</td><td style='width:143pt;'>Sigma Aldrich</td><td style='width:121pt;'>A1296-100G</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Small weigh dish</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>02-202-100</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Vibratome</td><td style='width:143pt;'>Leica</td><td style='width:121pt;'>VT1000 S</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>6 well tissue culture plates</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>08-772-1b</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Mesh bottom tissue culture inserts</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>07-200-214</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:14.5pt;width:208pt;'>Paraformadelhyde, 16%</td><td style='width:143pt;'>Electron Microscope Sciences</td><td style='width:121pt;'>15710-S</td><td style='width:185pt;'>Hazardous</td></tr><tr><td style='height:14.5pt;width:208pt;'>Ammonium hydroxide</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>A669S-500</td><td style='width:185pt;'>Hazardous</td></tr><tr><td style='height:14.5pt;width:208pt;'>Kodak Fixative A</td><td style='width:143pt;'>Sigma Aldrich</td><td style='width:121pt;'>P7542</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>Superfrost plus slides</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>12-550-15</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>CitroSolv clearing agent</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>22-143-975</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>Anhydrous ethyl alcohol</td><td style='width:143pt;'>Commercial Alcohols</td><td style='width:121pt;'>N/A</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>Cresyl violet</td><td style='width:143pt;'>Sigma Aldrich</td><td style='width:121pt;'>C1791</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>Permount</td><td style='width:143pt;'>Fisher Scientific</td><td style='width:121pt;'>SP15-100</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>Upright microscope</td><td style='width:143pt;'>Olympus</td><td style='width:121pt;'>BX53 model</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>Colour camera, 12 bit</td><td style='width:143pt;'>MBF Biosciences</td><td style='width:121pt;'>DV-47d</td><td style='width:185pt;'>QImaging part 01-MBF-2000R-F-CLR-12</td></tr><tr><td style='height:15.75pt;width:208pt;'>Three-dimensional motorized microscope stage, controller and enoders</td><td style='width:143pt;'>MBF Biosciences</td><td style='width:121pt;'>N/A</td><td style='width:185pt;'>Supplied and integrated with microscope by MBF Biosciences</td></tr><tr><td style='height:15.75pt;width:208pt;'>4x microscope objective</td><td style='width:143pt;'>Olympus</td><td style='width:121pt;'>4x 0.16 N.A. UplanSApo</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>10x microscope objective</td><td style='width:143pt;'>Olympus</td><td style='width:121pt;'>10x 0.3 N.A. UPlan FL N</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>30x microscope objective</td><td style='width:143pt;'>Olympus</td><td style='width:121pt;'>30x 1.05 N.A. UPlanSApo</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>60x microscope objective</td><td style='width:143pt;'>Olympus</td><td style='width:121pt;'>60x 1.42 N.A. PlanAPO N</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>Silicone immersion oil</td><td style='width:143pt;'>Olympus</td><td style='width:121pt;'>Z-81114</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>Neurolucida software</td><td style='width:143pt;'>MBF Biosciences</td><td style='width:121pt;'>Version 10</td><td style='width:185pt;'>&#160;</td></tr><tr><td style='height:15.75pt;width:208pt;'>ImageJ software</td><td style='width:143pt;'>U. S. National Institutes of Health</td><td style='width:121pt;'>Current version</td><td style='width:185pt;'>With the OME Bio-Formats plugin installed</td></tr><tr><td style='height:15.75pt;width:208pt;'>Photoshop software</td><td style='width:143pt;'>Adobe</td><td style='width:121pt;'>version CS6</td><td>&#160;</td></tr></tbody></table></figure>

microscopic imaging of neurons in a mouse brain section using golgi-cox metallic staining

<a href='https://appjove.unicartagenaproxy.elogim.com/v/55358/imaging-neurons-within-thick-brain-sections-using-the-golgi-cox-method'>Source: Louth, E. L.,&#160; et al. Imaging neurons within thick brain sections using the Golgi-Cox method. J. Vis. Exp. (2017)</a>This video demonstrates imaging neurons in a Golgi-Cox stained thick brain section by setting upper and lower focus boundaries and capturing overlapping images. Multiple locations are imaged to ensure detailed neuronal projections, which are combined to create a 3D representation.

Microscopic Imaging of Neurons in a Mouse Brain Section Using Golgi-Cox Metallic Staining

Source: Louth, E. L.,&#160; et al. Imaging neurons within thick brain sections using the Golgi-Cox method. J. Vis. Exp. (2017)This video demonstrates ...

Start with a thick brain section that was stained with Golgi-Cox solution to selectively darken neurons and counterstained with cresyl violet to highlight the brain region.&#160;Place them on a slide that has been pretreated with a clearing agent to enhance tissue transparency.&#160;Place the slide on the microscope stage, apply silicone oil, and lower the objective lens until it contacts the oil.&#160;&#160;Silicone oil matches the refractive index of the objective lens and slide, enabling detailed imaging.Focus on the sample, then adjust the camera's exposure and white balance for optimal image quality.&#160;&#160;Focus on the top layer to set the upper boundary, then on the bottom layer to set the lower boundary.&#160;&#160;Adjust the spacing between images with sufficient overlap to capture details of neuronal projections.&#160;Repeat imaging at different locations to capture areas of interest, then overlay these images to create a three-dimensional representation of the neurons.

microscopic-imaging-neurons-mouse-brain-section-using-golgi-cox

Universidad de Cartagena UDEC

Research

JoVE Encyclopedia of Experiments

Neuroscience

Neuroimaging

Advanced Microscopy & Imaging Technologies

55 조회수. Source: Louth, E. L.,  et al. Imaging neurons within thick brain sections using the Golgi-Cox method. J. Vis. Exp. (2017) This video demonstrates imaging neurons in a Golgi-Cox stained thick brain section by setting upper and lower focus boundaries and capturing overlapping images. Multiple locations are imaged to ensure detailed neuronal projections, which are combined to create a 3D representation. 

비디오: Microscopic Imaging of Neurons in a Mouse Brain Section Using Golgi-Cox Metallic Staining - 개념

Assessment of Hippocampal Dendritic Complexity in Aged Mice Using the Golgi-Cox Method

Dendritic spines are the protuberances from the neuronal dendritic shafts that contain&#160; excitatory synapses. The morphological and branching variations of the neuronal dendrites within the hippocampus are implicated in cognition and memory formation. There are several approaches to Golgi staining, all of which have been useful for determining the morphological characteristics of dendritic arbors and produce a clear background. The present Golgi-Cox method, (a slight variation of the protocol that is provided with a commercial Golgi staining kit), was designed to assess how a relatively low dose of the chemotherapeutic drug 5-flurouracil (5-Fu) would affect dendritic morphology, the number of spines, and the complexity of arborization within the hippocampus. The 5-Fu significantly modulated the dendritic complexity and decreased the spine density throughout the hippocampus in a region-specific manner. The data presented show that the Golgi staining method effectively stained the mature neurons in the CA1, the CA3, and the dentate gyrus (DG) of the hippocampus. This protocol reports the details for each step so that other researchers can reliably stain tissue throughout the brain with high quality results and minimal troubleshooting.

Here we present a Golgi-Cox protocol in extensive detail. This reliable tissue stain method allows for a high-quality assessment of the cytoarchitecture in the hippocampus, and throughout the entire brain, with minimal troubleshooting.

골지 - 콕스 방법을 이용한 고령의 해마 상피 세포의 수지상 돌기 복잡성 평가

Dendritic spines are the protuberances from the neuronal dendritic shafts that contain&#160; excitatory synapses. The morphological and branching ...

연구

JoVE Journal

신경과학

Facial Transplants in Xenopus laevis Embryos

Craniofacial birth defects occur in 1 out of every 700 live births, but etiology is rarely known due to limited understanding of craniofacial development. To identify where signaling pathways and tissues act during patterning of the developing face, a 'face transplant' technique has been developed in embryos of the frog Xenopus laevis. A region of presumptive facial tissue (the "Extreme Anterior Domain" (EAD)) is removed from a donor embryo at tailbud stage, and transplanted to a host embryo of the same stage, from which the equivalent region has been removed. This can be used to generate a chimeric face where the host or donor tissue has a loss or gain of function in a gene, and/or includes a lineage label. After healing, the outcome of development is monitored, and indicates roles of the signaling pathway within the donor or surrounding host tissues. Xenopus is a valuable model for face development, as the facial region is large and readily accessible for micromanipulation. Many embryos can be assayed, over a short time period since development occurs rapidly. Findings in the frog are relevant to human development, since craniofacial processes appear conserved between Xenopus and mammals.

Facial Transplants in Xenopus laevis Embryos

A technique for transplanting "Extreme Anterior Domain" facial tissue between Xenopus laevis embryos has been developed. Tissue can be moved from one gene expression background into another, allowing the study of local requirements for craniofacial development and for signaling interactions between facial regions.

의 얼굴 이식<em&gt;는 Xenopus laevis의</em&gt; 태아

Craniofacial birth defects occur in 1 out of every 700 live births, but etiology is rarely known due to limited understanding of craniofacial development. ...

생물학

Quantitative Localization of a Golgi Protein by Imaging Its Center of Fluorescence Mass

The Golgi complex consists of serially stacked membrane cisternae which can be further categorized into sub-Golgi regions, including the cis-Golgi, medial-Golgi, trans-Golgi and trans-Golgi network. Cellular functions of the Golgi are determined by the characteristic distribution of its resident proteins. The spatial resolution of conventional light microscopy is too low to resolve sub-Golgi structure or cisternae. Thus, the immuno-gold electron microscopy is a method of choice to localize a protein at the sub-Golgi level. However, the technique and instrument are beyond the capability of most cell biology labs. We describe here our recently developed super-resolution method called Golgi protein localization by imaging centers of mass (GLIM) to systematically and quantitatively localize a Golgi protein. GLIM is based on standard fluorescence labeling protocols and conventional wide-field or confocal microscopes. It involves the calibration of chromatic-shift aberration of the microscopic system, the image acquisition and the post-acquisition analysis. The sub-Golgi localization of a test protein is quantitatively expressed as the localization quotient. There are four main advantages of GLIM; it is rapid, based on conventional methods and tools, the localization result is quantitative, and it affords ~ 30 nm practical resolution along the Golgi axis. Here we describe the detailed protocol of GLIM to localize a test Golgi protein.

The precise localization of Golgi residents is essential for understanding the cellular functions of the Golgi. However, conventional optical microscopy is unable to resolve the sub-Golgi structure. Here we describe the protocol for a conventional microscopy based super-resolution method to quantitatively determine the sub-Golgi localization of a protein.

이미징 센터의 형광 질량으로 Golgi 단백질의 양적 지역화

The Golgi complex consists of serially stacked membrane cisternae which can be further categorized into sub-Golgi regions, including the cis-Golgi, ...

Microscopic Imaging of Neurons in a Mouse Brain Section Using Golgi-Cox Metallic Staining

내레이션 대본

Microscopic Imaging of Neurons in a Mouse Brain Section Using Golgi-Cox Metallic Staining

골지 - 콕스 방법을 이용한 고령의 해마 상피 세포의 수지상 돌기 복잡성 평가

의 얼굴 이식

이미징 센터의 형광 질량으로 Golgi 단백질의 양적 지역화