selective single-neuron laser ablation in a zebrafish larva using a confocal microscope

Selective Single-Neuron Laser Ablation in a Zebrafish Larva Using a Confocal Microscope

Use an adjustable pipette to draw up a larva and let it sink to the bottom of the tip. Drop the larva in a minimal volume of liquid into preheated agarose, then draw up the fish with agarose and quickly dispense it into a previously prepared glass bottom 35-millimeter dish. Under a dissection microscope, use a standard paintbrush to position the animal, or multiple animals, within the agarose on their sides, so that the body and tail are flat.Allow the embedded fish to sit for 10 to 15 minutes until the agarose is firmly set. Then, use approximately two milliliters of egg water with trikane to carefully top up the 35-millimeter petri dish. Place the petri dish with an embedded larva on the confocal microscope stage, and using Brightfield illumination and 40X magnification, focus on the dorsal side of the animal spinal cord. Switch to an appropriate fluorescent setting, and visualize the structure of interest to confirm that all imaging parameters are as needed for subsequent ablation.To determine the thickness of the structure for UV laser ablation, use the Z drive to verify the top and bottom of the structure of interest by manually focusing up and down. Manually record the Z plane that will be ablated, for example, the center of the cell. To carry out laser ablation, start the FRAP wizard by clicking on the dropdown menu at the top of the software menu.From the new window, determine the image parameters for the ablation approach by selecting the format, scan speed, and averaging. If the Z plane for ablation hasn't already been selected, press the live button and focus through the specimen until the fluorescent structure, or the desired Z plane to be ablated is in focus. Once the general image parameters are set, access the bleach step to control the specific ablation components, then engage the 405-nanometer laser by activating it for the bleaching procedure.Next, use the zoom-in option to maximize the bleaching intensity at the selected ROI by reducing the scan field, therefore maximizing dwell time. Select one or multiple ROIs for the ablation by using any of the drawing tools in the image acquisition window. Target the axon hillock, for example, with the circular drawing tool of approximately 4 to 8 micrometers.After establishing the ROI, select the time course button and confirm the number of cycles the ROIs will be scanned and ablated. Choose the pre-bleach and post-bleach frames as desired to permit an overview of the whole image just before, and immediately after the bleaching process. &#160; These settings allow researchers multiple layers of refinement. Through the adjustment of laser power, scan speed, line averaging, size of region of interest, and repetitions, this technique offers a high degree of freedom to cause stress or death in individual cells.After establishing all the necessary ablation parameters, press Run experiment and monitor the efficiency of the ablation. Refer to the text protocol for additional details.

selective-single-neuron-laser-ablation-zebrafish-larva-using-confocal

Universidad de Cartagena UDEC

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JoVE Encyclopedia of Experiments

Neuroscience

Neuroimaging

Synaptic & Cellular Imaging

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Source:&#160;<a style='text-decoration:none;' href='https://appjove.unicartagenaproxy.elogim.com/v/54983/triggering-cell-stress-and-death-using-conventional-uv-laser-confocal-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;'>Morsch, M.,&#160;<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;'>&#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;'>,&#160;<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;'>Triggering Cell Stress and Death Using Conventional UV Laser Confocal 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;'> (2017)</a> &#160;In this video, we explore the technique of high-intensity UV laser ablation for precisely targeting and studying individual neurons in transgenic zebrafish. We demonstrate how to prepare, immobilize, and visualize neuronal responses, highlighting the cellular dynamics of injury and recovery.

Source:&#160;Morsch, M.,&#160;&#160;et. al.,&#160;Triggering Cell Stress and Death Using Conventional UV Laser Confocal Microscopy.&#160;J. Vis. Exp. ...

Take a preheated agarose solution containing an anesthetized transgenic zebrafish larva expressing a fluorescent protein in spinal motor neurons.&#160;Transfer the larva to a glass dish with an agarose ring.Using a microscope, turn the larva onto its side. Then, allow the agarose to solidify, immobilizing the larva.Add buffer containing anesthetic to maintain anesthesia.Place the dish on the confocal microscope stage and use bright-field imaging to locate the dorsal spinal cord region.Switch to fluorescence mode to visualize fluorescent motor neurons.&#160;Determine the central z-plane of the cell soma for precise ablation targeting.&#160;Configure imaging parameters for high-resolution acquisition while minimizing photodamage.&#160;Once the desired z plane is in focus, perform ablation on the target neuron region using a focused ultraviolet laser.&#160;Laser energy disrupts cellular structures, causing fluorescence loss and cell death. Irreversible fluorescence loss confirms precise ablation without affecting surrounding cells.

14 Views. Selective Single-Neuron Laser Ablation in a Zebrafish Larva Using a Confocal Microscope

Video: Selective Single-Neuron Laser Ablation in a Zebrafish Larva Using a Confocal Microscope - Experiment

Measuring Protein Stability in Living Zebrafish Embryos Using Fluorescence Decay After Photoconversion (FDAP)

Protein stability influences many aspects of biology, and measuring the clearance kinetics of proteins can provide important insights into biological systems. In FDAP experiments, the clearance of proteins within living organisms can be measured. A protein of interest is tagged with a photoconvertible fluorescent protein, expressed in vivo and photoconverted, and the decrease in the photoconverted signal over time is monitored. The data is then fitted with an appropriate clearance model to determine the protein half-life. Importantly, the clearance kinetics of protein populations in different compartments of the organism can be examined separately by applying compartmental masks. This approach has been used to determine the intra- and extracellular half-lives of secreted signaling proteins during zebrafish development. Here, we describe a protocol for FDAP experiments in zebrafish embryos. It should be possible to use FDAP to determine the clearance kinetics of any taggable protein in any optically accessible organism.

Measuring Protein Stability in Living Zebrafish Embryos Using Fluorescence Decay After Photoconversion FDAP

Protein levels in cells and tissues are often tightly regulated by the balance of protein production and clearance. Using Fluorescence Decay After Photoconversion (FDAP), the clearance kinetics of proteins can be experimentally measured in vivo.

Protein stability influences many aspects of biology, and measuring the clearance kinetics of proteins can provide important insights into biological ...

JoVE Journal

Developmental Biology

Multi-Photon Time Lapse Imaging to Visualize Development in Real-time: Visualization of Migrating Neural Crest Cells in Zebrafish Embryos

Congenital eye and craniofacial anomalies reflect disruptions in the neural crest, a transient population of migratory stem cells that give rise to numerous cell types throughout the body. Understanding the biology of the neural crest has been limited, reflecting a lack of genetically tractable models that can be studied in vivo and in real-time. Zebrafish is a particularly important developmental model for studying migratory cell populations, such as the neural crest. To examine neural crest migration into the developing eye, a combination of the advanced optical techniques of laser scanning microscopy with long wavelength multi-photon fluorescence excitation was implemented to capture high-resolution, three-dimensional, real-time videos of the developing eye in transgenic zebrafish embryos, namely Tg(sox10:EGFP) and Tg(foxd3:GFP), as sox10 and foxd3 have been shown in numerous animal models to regulate early neural crest differentiation and likely represent markers for neural crest cells. Multi-photon time-lapse imaging was used to discern the behavior and migratory patterns of two neural crest cell populations contributing to early eye development. This protocol provides information for generating time-lapse videos during zebrafish neural crest migration, as an example, and can be further applied to visualize the early development of many structures in the zebrafish and other model organisms.

A combination of the advanced optical techniques of laser scanning microscopy with long wavelength multi-photon fluorescence excitation was implemented to capture high-resolution, three-dimensional, real-time imaging of neural crest migration in Tg(sox10:EGFP) and Tg(foxd3:GFP) zebrafish embryos.

Congenital eye and craniofacial anomalies reflect disruptions in the neural crest, a transient population of migratory stem cells that give rise to ...

Deep and Spatially Controlled Volume Ablations using a Two-Photon Microscope in the Zebrafish Gastrula

Morphogenesis involves many cell movements to organize cells into tissues and organs. For proper development, all these movements need to be tightly coordinated, and accumulating evidence suggests this is achieved, at least in part, through mechanical interactions. Testing this in the embryo requires direct physical perturbations. Laser ablations are an increasingly used option that allows relieving mechanical constraints or physically isolating two cell populations from each other. However, many ablations are performed with an ultraviolet (UV) laser, which offers limited axial resolution and tissue penetration. A method is described here to ablate deep, significant, and spatially well-defined volumes using a two-photon microscope. Ablations are demonstrated in a transgenic zebrafish line expressing the green fluorescent protein in the axial mesendoderm and used to sever the axial mesendoderm without affecting the overlying ectoderm or the underlying yolk cell. Cell behavior is monitored by live imaging before and after the ablation. The ablation protocol can be used at different developmental stages, on any cell type or tissue, at scales ranging from a few microns to more than a hundred microns.

Embryonic development requires large-scale coordination of cell motion. Two-photon excitation mediated laser ablation allows the spatially controlled 3-dimensional ablation of large groups of deep cells. In addition, this technique can probe the reaction of collectively migrating cells in vivo to perturbations in their mechanical environment.

Morphogenesis involves many cell movements to organize cells into tissues and organs. For proper development, all these movements need to be tightly ...

Selective Single-Neuron Laser Ablation in a Zebrafish Larva Using a Confocal Microscope

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Selective Single-Neuron Laser Ablation in a Zebrafish Larva Using a Confocal Microscope