visualizing motor neuron projections and axon branching using light sheet fluorescence microscopy

Visualizing Motor Neuron Projections and Axon Branching Using Light Sheet Fluorescence Microscopy

Set up 5X/0.1 illumination optics and 5X/0.16 detection optics. Assemble the sample holder and sample capillary. Prepare the sample chamber by filling it with clearing solution. To mount the embryo, prepare a P200 pipette tip by cutting away the upper part so that it fits the diameter of the capillary, and remove the pointed part for the sample attachment.Then, melt the blunted end of the pipette tip using a small flame. Extinguish the flame and quickly attach the embryo vertically onto the melted end. Fit the upper part of the pipette tip with the sample capillary, and put the prepared sample chamber into the microscope. Using the imaging software, select Locate Capillary under the Locate tab, and adjust the xy and z-axes.Next, select Locate Sample and zoom to 0.6X to focus on the embryo. Allow the chamber buffer to equilibrate with the embryo for some time to clear off any debris or bubbles. For image acquisition under the Acquisition tab, define the light path parameters, such as detection objectives, laser blocking filter, beam splitter, cameras, and lasers.Check the pivot scan checkbox for shadow reduction. Then, define the acquisition settings, bit depth to 16 bit. Zoom to the range between 0.36 and 0.7X single side illumination or dual-side illumination. Click Continuous, and set the laser intensity, exposure time, laser power, and light sheet position. Subsequently, press stop to end image acquisition.It is important to ensure that the transparent sample is positioned within the shortest light path to allow detailed acquisition of images of fine upright structures on individual motor nerves.For multidimensional acquisition, define the Z stack by moving the Z position for the first and last image. Click Optimal to set the slice number. Then, click Start Experiment to acquire the selected Z stack. When it is done, save the image in dot CZI format.To quantify axon arborization, open the image file in the imaging analysis software. Adjust the image color, brightness, and contrast using the display adjustment window to detect filaments based on local intensity contrast. Next, click on the Add New Filaments icon, and select the auto path algorithm in the dropdown menu. Select the region of interest.Then, define the starting and seed points by assigning the largest and thinnest diameter measurements, which can be measured using the slice mode. Assign a starting point at the edge of the region of interest. To achieve manual addition or removal of starting points, first, change the pointer mode, Navigate Select, and then shift and right-click at the points of interest.Next, select Manual Thresholds For Seed Points to ensure that all of the visible arborization is marked. Then, manually add or remove seed points. Check the box, Remove Disconnected Segments, and remove seed points around starting points. Subsequently, adjust the Threshold For Background Subtraction and finish the process.It is necessary to remove background artifacts and confirm the detector path reflect true axon arborization for accurate quantification.At the end, choose the desired style and color. Under the Statistics tab, select detailed, and use filament number dendrite terminal points to quantify the motor nerve terminals as an indicator of motor axon arborization. Then, export the image of the reconstructed axon as a .TIFF file.

visualizing-motor-neuron-projections-axon-branching-using-light-sheet

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#000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>Bitplane, Zurich, Switzerland</td><td style='border-bottom:1px solid #000000;border-right:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td><td style='border-bottom:1px solid #000000;border-right:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr><tr style='height:20px;'><td style='border-bottom:1px solid #000000;border-left:1px solid #000000;border-right:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>B6.Cg-Tg(Hlxb9-GFP)1Tmj/J (Hb9::GFP mice)</td><td style='border-bottom:1px solid #000000;border-right:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>The Jackson Laboratory</td><td style='border-bottom:1px solid #000000;border-right:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>005029</td><td style='border-bottom:1px solid #000000;border-right:1px solid #000000;overflow:hidden;padding:0px 3px;vertical-align:bottom;'>&#160;</td></tr></tbody></table></figure>

Source:&#160;<a style='text-decoration:none;' href='https://appjove.unicartagenaproxy.elogim.com/v/57546/visualization-of-motor-axon-navigation-and-quantification-of-axon-arborization-in-mouse-embryos-using-light-sheet-fluorescence-microscopy'><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;'>Liau, E. S.&#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;'> Visualization of Motor Axon Navigation and Quantification of Axon Arborization In Mouse Embryos Using Light Sheet Fluorescence Microscopy.&#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;'> (2018).</a> &#160;This video demonstrates the use of light sheet fluorescence microscopy to image motor neuron projections and axon branching in transgenic mouse embryos. It outlines the steps involved in sample preparation, imaging, and 3D reconstruction of axonal branching for assessing motor neuron growth and connectivity.

Source:&#160;Liau, E. S.&#160;et al. Visualization of Motor Axon Navigation and Quantification of Axon Arborization In Mouse Embryos Using Light Sheet ...

Take a chemically fixed and cleared tissue segment from a transgenic mouse embryo expressing green fluorescent protein (GFP) in spinal motor neurons.Mount the tissue vertically onto a modified pipette tip.Attach the tip to a capillary secured within the light sheet fluorescence microscope.Place a buffer-filled sample chamber beneath the tissue to immerse it and clear debris.Using imaging software, align the tissue in the light path.Begin image acquisition.&#160;The light source emits a thin sheet of laser light, exciting GFPs in a single plane of the tissue to emit fluorescence.A detector positioned perpendicular to the light path captures the emitted fluorescence.Acquire images of the spinal motor neurons to generate a 3D reconstruction of the axonal branching morphology.Use software to map axons, identifying branching patterns and endpoints to assess motor neuron growth and connectivity.

23 Views. Visualizing Motor Neuron Projections and Axon Branching Using Light Sheet Fluorescence Microscopy

Video: Visualizing Motor Neuron Projections and Axon Branching Using Light Sheet Fluorescence Microscopy - Experiment

Light Sheet-based Fluorescence Microscopy of Living or Fixed and Stained Tribolium castaneum Embryos

The red flour beetle Tribolium castaneum has become an important insect model organism in developmental genetics and evolutionary developmental biology. The observation of Tribolium embryos with light sheet-based fluorescence microscopy has multiple advantages over conventional widefield and confocal fluorescence microscopy. Due to the unique properties of a light sheet-based microscope, three dimensional images of living specimens can be recorded with high signal-to-noise ratios and significantly reduced photo-bleaching as well as photo-toxicity along multiple directions over periods that last several days. With more than four years of methodological development and a continuous increase of data, the time seems appropriate to establish standard operating procedures for the usage of light sheet technology in the Tribolium community as well as in the insect community at large. This protocol describes three mounting techniques suitable for different purposes, presents two novel custom-made transgenic Tribolium lines appropriate for long-term live imaging, suggests five fluorescent dyes to label intracellular structures of fixed embryos and provides information on data post-processing for the timely evaluation of the recorded data. Representative results concentrate on long-term live imaging, optical sectioning and the observation of the same embryo along multiple directions. The respective datasets are provided as a downloadable resource. Finally, the protocol discusses quality controls for live imaging assays, current limitations and the applicability of the outlined procedures to other insect species.
This protocol is primarily intended for developmental biologists who seek imaging solutions that outperform standard laboratory equipment. It promotes the continuous attempt to close the gap between the technically orientated laboratories/communities, which develop and refine microscopy methodologically, and the life science laboratories/communities, which require 'plug-and-play' solutions to technical challenges. Furthermore, it supports an axiomatic approach that moves the biological questions into the center of attention.

Light Sheet-based Fluorescence Microscopy of Living or Fixed and Stained Tribolium castaneum Embryos

Imaging the morphogenesis of insect embryos with light sheet-based fluorescence microscopy has become state of the art. This protocol outlines and compares three mounting techniques appropriate for Tribolium castaneum embryos, introduces two novel custom-made transgenic lines well suited for live imaging, discusses essential quality controls and indicates current experimental limitations.

The red flour beetle Tribolium castaneum has become an important insect model organism in developmental genetics and evolutionary developmental biology. ...

JoVE Journal

Developmental Biology

Visualizing Surface T-Cell Receptor Dynamics Four-Dimensionally Using Lattice Light-Sheet Microscopy

The signaling and function of a cell are dictated by the dynamic structures and interactions of its surface receptors. To truly understand the structure-function relationship of these receptors in situ, we need to visualize and track them on the live cell surface with enough spatiotemporal resolution. Here we show how to use recently developed Lattice Light-Sheet Microscopy (LLSM) to image T-cell receptors (TCRs) four-dimensionally (4D, space and time) at the live cell membrane. T cells are one of the main effector cells of the adaptive immune system, and here we used T cells as an example to show that the signaling and function of these cells are driven by the dynamics and interactions of the TCRs. LLSM allows for 4D imaging with unprecedented spatiotemporal resolution. This microscopy technique therefore can be generally applied to a wide array of surface or intracellular molecules of different cells in biology.

The goal of this protocol is to show how to use Lattice Light-Sheet Microscopy to four-dimensionally visualize surface receptor dynamics in live cells. Here T cell receptors on CD4+ primary T cells are shown.

The signaling and function of a cell are dictated by the dynamic structures and interactions of its surface receptors. To truly understand the ...

Biochemistry

Visualization of Thalamocortical Axon Branching and Synapse Formation in Organotypic Cocultures

Axon branching and synapse formation are crucial processes for establishing precise neuronal circuits. During development, sensory thalamocortical (TC) axons form branches and synapses in specific layers of the cerebral cortex. Despite the obvious spatial correlation between axon branching and synapse formation, the causal relationship between them is poorly understood. To address this issue, we recently developed a method for simultaneous imaging of branching and synapse formation of individual TC axons in organotypic cocultures.
This protocol describes a method which consists of a combination of an organotypic coculture and electroporation. Organotypic cocultures of the thalamus and cerebral cortex facilitate gene manipulation and observation of axonal processes, preserving characteristic structures such as laminar configuration. Two distinct plasmids encoding DsRed and EGFP-tagged synaptophysin (SYP-EGFP) were co-transfected into a small number of thalamic neurons by an electroporation technique. This method allowed us to visualize individual axonal morphologies of TC neurons and their presynaptic sites simultaneously. The method also enabled long-term observation which revealed the causal relationship between axon branching and synapse formation.

This protocol describes a method for simultaneous imaging of thalamocortical axon branching and synapse formation in organotypic cocultures of the thalamus and cerebral cortex. Individual thalamocortical axons and their presynaptic terminals are visualized by a single cell electroporation technique with DsRed and GFP-tagged synaptophysin.

Axon branching and synapse formation are crucial processes for establishing precise neuronal circuits. During development, sensory thalamocortical (TC) ...

Visualizing Motor Neuron Projections and Axon Branching Using Light Sheet Fluorescence Microscopy

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Visualizing Motor Neuron Projections and Axon Branching Using Light Sheet Fluorescence Microscopy