visualizing the synaptogenesis of cerebellar granule neurons at different developmental stages

Visualizing the Synaptogenesis of Cerebellar Granule Neurons at Different Developmental Stages

To study the morphology of single electroporated CGNs from sagittal brain sections of the experimental pup, take z stack images at 0.5 micrometers per stack on a confocal microscope. Image one cell per image window to allow for easy image analysis and 3D reconstruction. Analyze neurite length and dendritic claw formation in a blinded manner using simple neurite tracer.Upload single channel stack images of electroporated CGNs into Fiji, and click on Plugins, Segmentation and Simple Neurite Tracer. Select Create New 3D Viewer from the dropdown menu. Scroll to the base of a dendrite connecting to cell soma, and start a bath by clicking on the junction. Manually trace the path by clicking through the sections where the cell fill signal is brightest, and pressing Y to keep the trace.Trace until the end of the dendrite and confirm the path by pressing F. Alternatively, trace until the base of the claw. Next, trace the claw from the base of the structure until the end of the longest neurite. Trace secondary and tertiary branches by holding down Control on Windows, or Alt on a Mac OS and clicking the path. Confirm the path by pressing F. Observe that measurements for the traces are visible on a separate window. Add up all the sizes of the claw branches to obtain the total length for each claw.

visualizing-synaptogenesis-cerebellar-granule-neurons-at-different

Nanyang Technological University

Research

JoVE Encyclopedia of Experiments

Neuroscience

Neuroimaging

Advanced Microscopy & Imaging Technologies

EoE Sub Articles

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All procedures involving animal samples have been reviewed and approved by the appropriate animal ethical review committee.1. Morphological analyses of cerebellar granule neurons or CGNs - three-dimensional (3D) reconstruction and surface area and cellular volume<ol><li>Image single electroporated CGNs on a confocal microscope at 63x objective with a 2x zoom, taking z-stack images at 0.5 &#181;m per stack. Image one cell per image window to allow for easy image analysis and reconstruction.</li><li>Install the Simple Neurite Tracer plug-in for FIJI using the following link (https://imagej.net/Simple_Neurite_Tracer:_Basic_Instructions) to easily and efficiently trace the structure of electroporated CGNs in three-dimensional (3D) space.</li></ol>NOTE: There is an updated version of the plug-in (https://imagej.net/SNT).<ol start='3'><li>Analyze neurite length and dendritic claw formation in a blinded manner using a Simple Neurite Tracer. Upload single-channel z-stack images of electroporated CGNs onto FIJI, and click on Plugins | Segmentation | Simple Neurite Tracer (Figure 1D).</li><li>Access the drop-down menu, and select Create New 3D Viewer (Figure 1D).</li><li>Scroll to the base of a dendrite, where it connects to the cell soma, and start a path by clicking on the junction. Manually trace the path by clicking through the sections where the cell-fill signal is brightest, pressing [y] to keep the trace. Trace until the end of the dendrite if it does not contain a claw or until the base of the claw and confirm the path by pressing [f] (Figure 2D).</li><li>Next, trace the claw by starting a path at the base of the structure and tracing until the end of the longest neurite. Trace secondary and tertiary branches by holding down [ctrl] on Windows or [alt] on a Mac OS and clicking the path. Confirm the path by pressing [f].</li><li>Observe that measurements for the traces are visible on a separate window; add up all of the measurements of the claw branches (primary, secondary, tertiary) to obtain the total length for each claw.</li><li>For analyzing the surface area and cellular volume of electroporated CGNs, download Imaris cell analysis software (https://imaris.oxinst.com/).</li></ol>NOTE:&#160;FIJI can also be used to reconstruct cells in 3D from z-stack images using readily available and free plug-ins. Additionally, Simple Neurite Tracer has a volumetric rendering feature, but Imaris was used for the reasons outlined below.<ol start='9'><li>Upload a z-stack image of an electroporated CGN onto Imaris. Access the 3D-reconstruction toolkit by pressing Surpass.</li><li>To reconstruct the CGN, press Surfaces, and select a region of interest that encompasses the entirety of the cell within the image window. Once finished, press the blue forward arrow at the bottom right corner under Create.</li><li>If the image contains multiple channels for different signals, select the channel containing the electroporated CGN, and press the blue forward arrow.</li><li>Using the sidebar, set a desired threshold that most accurately fits the signal of the electroporated cell. Zoom in closer to the surface of the cell to accurately determine the threshold. Once finished, press the double green arrow to reconstruct the cell and obtain the surface area and volume size from the metadata.</li></ol>

<figure class='table'><table class='ck-table-resized' style='border-collapse:collapse;font-family:Calibri;font-size:11pt;table-layout:fixed;' cellspacing='0' cellpadding='0' dir='ltr' border='1' data-sheets-root='1' data-sheets-baot='1'><colgroup><col style='width:25%;' width='130'><col style='width:25%;' width='130'><col style='width:25%;' width='130'><col style='width:25%;' width='130'></colgroup><tbody><tr style='height:20px;'><td style='background-color:#ffffff;color:#1a202c;font-family:Roboto;font-size:12pt;font-weight:normal;overflow:hidden;padding:0px 3px;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>Imaris</td><td style='background-color:#ffffff;color:#1a202c;font-family:Roboto;font-size:12pt;font-weight:normal;overflow:hidden;padding:0px 3px;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>Bitplane</td><td style='background-color:#ffffff;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td><td style='background-color:#ffffff;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr><tr style='height:21px;'><td style='background-color:#ffffff;color:#1a202c;font-family:Roboto;font-size:12pt;font-weight:normal;overflow:hidden;padding:0px 3px;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>Zeiss 780 Upright Confocal</td><td style='background-color:#ffffff;color:#1a202c;font-family:Roboto;font-size:12pt;font-weight:normal;overflow:hidden;padding:0px 3px;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>Zeiss</td><td style='background-color:#ffffff;color:#1a202c;font-family:Roboto;font-size:12pt;font-weight:normal;overflow:hidden;padding:0px 3px;vertical-align:bottom;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>780</td><td style='overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr></tbody></table></figure>

<figure class='image image_resized image-style-align-center' style='display:table;margin-left:auto;margin-right:auto;width:75%;'><img style='aspect-ratio:1758/2148;' src='https://cloudfront-jove-com.remotexs.ntu.edu.sg/files/ftp_upload/23446/23446_Figure_1_editor_23446.jpg' alt='23446_Figure_1.jpg' /></figure>Figure 1: Immunohistochemical analysis and three-dimensional reconstruction of electroporated granule neurons. P7 CD-1 mice were electroporated with a construct expressing green fluorescence protein or GFP. Brains were collected and subjected to immunohistochemistry, confocal microscopy, and 3D-reconstruction for morphological analysis. (A) Timeline from electroporation to image processing of a 10-DPI mouse. (B) Maximum projection image of a sagittal cross-section of electroporated cerebellum 10-DPI; white lines demarcate cerebellar layers, and scale bar is 25 &#181;m. (C) Maximum projection image of a single electroporated granule neuron 10-DPI and the corresponding 3D trace, scale bar is 10 &#181;m. (D) 3D-reconstructions were generated using the FIJI plugin Simple Neurite Tracer. All measurements were traced through the z-stack, following the cell-fill signal. Shaft and claw measurements were traced separately for every dendrite; dotted line denotes portion of dendrite within the current plane. Abbreviations: 3D = three-dimensional; GFP = green fluorescent protein; DPI = days post-injection; PSD-95 = postsynaptic density protein 95; GNPs = granule neuron progenitors; PFA = paraformaldehyde.&#160;<figure class='image image_resized image-style-align-center' style='display:table;margin-left:auto;margin-right:auto;width:75%;'><img style='aspect-ratio:3182/3675;' src='https://cloudfront-jove-com.remotexs.ntu.edu.sg/files/ftp_upload/23446/23446_Figure_2_editor_23446.jpg' alt='23446_Figure_2.jpg' /></figure>Figure 2: Analysis of granule neuron morphology during cerebellar development.&#160;(A) Maximum projection images of electroporated CGNs from 3-DPI to 14-DPI (postnatal age P10 to P21), nuclei (blue) and GFP (green); arrowheads indicate individual dendrite, and scale bar is 10 &#181;m. (B) Average number of dendrites. (C) Average dendrite length measured from the base of the soma to the tip of the dendrite. (D) Fraction of dendrites that contain a claw; a value of 1.00 is 100%, i.e., all dendrites have claw. (E) Total length of dendritic claw. N &gt; 30 cells per condition, collected from at least 4 animals per condition; all measurements were analyzed by one-way ANOVA and either a Dunnett's multiple comparison test (B, C, and D) or a Tukey's multiple comparison test (E), **** denotes significance with p &lt;0.0001 across time; errors bars are S.E.M. Abbreviations: GFP = green fluorescent protein; DPI = days post-injection; PSD-95 = postsynaptic density protein 95; CGNs = cerebellar granule neurons; ANOVA = analysis of variance; S.E.M. = standard error of the mean.&#160;

Source: Chan, U.,&#160;et al., Utilizing In Vivo Postnatal Electroporation to Study Cerebellar Granule Neuron Morphology and Synapse Development.&#160;J. ...

Begin with pre-fixed brain tissue slices collected from early and late postnatal stages of mice.&#160;The slice contains cerebellar granule neurons, or CGNs, expressing a fluorescent protein.Using a confocal microscope, focus on a single fluorescent CGN.Capture z-stack images at varying depths to create a three-dimensional view of the neuron.Using imaging software, trace the neurons' neurites or long projections, including dendrites and axons.Measure dendrite length from the cell body to its tip.Analyze dendritic claw formation, specialized structures at dendrite tips where signals from other neurons are received.Also, assess the neuron's surface area and volume.In the early postnatal stage, neurons show an increased number of dendrites, with no claw formation.&#160;Meanwhile, in the late postnatal stage, there are fewer dendrites, but their lengths and the number of claws increase.Thus, with age, CGNs undergo synaptogenesis and form connections with other cells for signal transmission.

19 Views. Visualizing the Synaptogenesis of Cerebellar Granule Neurons at Different Developmental Stages

Video: Visualizing the Synaptogenesis of Cerebellar Granule Neurons at Different Developmental Stages - Experiment

Ex Vivo Imaging of Postnatal Cerebellar Granule Cell Migration Using Confocal Macroscopy

During postnatal development, immature granule cells (excitatory interneurons) exhibit tangential migration in the external granular layer, and then radial migration in the molecular layer and the Purkinje cell layer to reach the internal granular layer of the cerebellar cortex. Default in migratory processes induces either cell death or misplacement of the neurons, leading to deficits in diverse cerebellar functions. Centripetal granule cell migration involves several mechanisms, such as chemotaxis and extracellular matrix degradation, to guide the cells towards their final position, but the factors that regulate cell migration in each cortical layer are only partially known. In our method, acute cerebellar slices are prepared from P10 rats, granule cells are labeled with a fluorescent cytoplasmic marker and tissues are cultured on membrane inserts from 4 to 10 hr before starting real-time monitoring of cell migration by confocal macroscopy at 37 &#176;C in the presence of CO2. During their migration in the different cortical layers of the cerebellum, granule cells can be exposed to neuropeptide agonists or antagonists, protease inhibitors, blockers of intracellular effectors or even toxic substances such as alcohol or methylmercury to investigate their possible role in the regulation of neuronal migration.

Ex Vivo Imaging of Postnatal Cerebellar Granule Cell Migration Using Confocal Macroscopy

During postnatal cerebellum development, immature granule cells originating from the germinal zone exhibit distinct modalities of migration to reach their final destination and to establish neuronal networks. This protocol describes the preparation of cerebellar slices and the confocal macroscopic approach used to investigate the factors that regulate neuronal migration.

During postnatal development, immature granule cells (excitatory interneurons) exhibit tangential migration in the external granular layer, and then ...

JoVE Journal

Modeling Neuronal Death and Degeneration in Mouse Primary Cerebellar Granule Neurons

Cerebellar granule neurons (CGNs) are a commonly used neuronal model, forming an abundant homogeneous population in the cerebellum. In light of their post-natal development, abundance, and accessibility, CGNs are an ideal model to study neuronal processes, including neuronal development, neuronal migration, and physiological neuronal activity stimulation. In addition, CGN cultures provide an excellent model for studying different modes of cell death including excitotoxicity and apoptosis. Within a week in culture, CGNs express N-methyl-D-aspartate (NMDA) receptors, a specific ionotropic glutamate receptor with many critical functions in neuronal health and disease. The addition of low concentrations of NMDA in conjunction with membrane depolarization to rodent primary CGN cultures has been used to model physiological neuronal activity stimulation while the addition of high concentrations of NMDA can be employed to model excitotoxic neuronal injury. Here, a method of isolation and culturing of CGNs from 6 day old pups as well as genetic manipulation of CGNs by adenoviruses and lentiviruses are described. We also present optimized protocols on how to stimulate NMDA-induced excitotoxicity, low-potassium-induced apoptosis, oxidative stress and DNA damage following transduction of these neurons.

This protocol describes a simple method for isolating and culturing primary mouse cerebral granule neurons (CGNs) from 6-7 day old pups, efficient transduction of CGNs for loss and gain of function studies, and modelling NMDA-induced neuronal excitotoxicity, low-potassium-induced cell death, DNA-damage, and oxidative stress using the same culture model.

Cerebellar granule neurons (CGNs) are a commonly used neuronal model, forming an abundant homogeneous population in the cerebellum. In light of their ...

Isolation and Cultivation of Neural Progenitors Followed by Chromatin-Immunoprecipitation of Histone 3 Lysine 79 Dimethylation Mark

Brain development is a complex process, which is controlled in a temporo-spatial manner by gradients of morphogens and different transcriptional programs. Additionally, epigenetic chromatin modifications, like histone methylation, have an important role for establishing and maintaining specific cell fates within this process. The vast majority of histone methylation occurs on the flexible histone tail, which is accessible to histone modifiers, erasers, and histone reader proteins. In contrast, H3K79 methylation is located in the globular domain of histone 3 and is implicated in different developmental functions. H3K79 methylation is evolutionarily conserved and can be found in a wide range of species from Homo sapiens to Saccharomyces cerevisiae. The modification occurs in different cell populations within organisms, including neural progenitors. The location of H3K79 methylation in the globular domain of histone 3 makes it difficult to assess. Here, we present methods to isolate and culture cortical progenitor cells (CPCs) from embryonic cortical brain tissue (E11.5-E14.5) or cerebellar granular neuron progenitors (CGNPs) from postnatal tissue (P5-P7), and to efficiently immunoprecipitate H3K79me2 for quantitative PCR (qPCR) and genome-wide sequencing.

We present an effective and reproducible method to isolate and culture neural progenitor cells from embryonic and postnatal brain tissue for chromatin immunoprecipitation (ChIP) of histone 3 lysine 79 dimethylation (H3K79me2) - a histone mark located within the globular domain of histone 3.

Brain development is a complex process, which is controlled in a temporo-spatial manner by gradients of morphogens and different transcriptional programs. ...

Visualizing the Synaptogenesis of Cerebellar Granule Neurons at Different Developmental Stages

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Visualizing the Synaptogenesis of Cerebellar Granule Neurons at Different Developmental Stages