monitoring recovery of laser-ablated interneuromast cells in zebrafish using confocal microscopy

Monitoring Recovery of Laser-Ablated Interneuromast Cells in Zebrafish Using Confocal Microscopy

For imaging of the cell bodies post-ablation, under the Channels menu, unclick the DAPI track to inactivate the ablation laser, and open the acquisition mode menu. Click Zoom and decrease the zoom to 0.7.To assess the success of the cell ablation, fast-scan the field of view. Using the same settings as those for the preablation imaging, capture and save a post-ablation image. Inspect the transmitted light photomultiplier tube channel image to further confirm the cellular damage. Damaged cells will demonstrate a granular appearance, and the nuclei will frequently swell or appear irregular in shape.To assess the post-ablation cell body recovery, activate both the stage position and time options for time lapse image capture, and set the time parameters to the appropriate experimental time point and 15 minute intervals. Then start the experiment to acquire images, and save the resulting file when complete.

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Source:&#160;Volpe, B. A.,&#160;et al.&#160;Confocal Microscope-Based Laser Ablation and Regeneration Assay in Zebrafish Interneuromast Cells.&#160;J. ...

Begin with a zebrafish larva containing fluorescently labeled interneuromast cells or INMCs, mounted on a coverslip and placed under a confocal microscope.&#160;INMCs are progenitor cells with regenerative ability that have been previously subjected to laser ablation.First, observe the damaged area in fluorescence mode. The absence of fluorescence confirms successful laser ablation.&#160;Next, use transmitted light imaging mode to examine the damaged area where the cell appears granular and swollen with irregular nuclei, confirming cell death.The recruitment of macrophages to the site indicates an active cellular response to injury.Now, switch back to fluorescence mode and capture time-lapse images at regular intervals to monitor recovery.&#160;During the recovery phase, INMCs extend projections into the gap, facilitating closure and promoting cellular repair.&#160;Save these time-series images for analysis. The reappearance of distinct fluorescence in the ablated area confirms successful cell recovery.

7 visualizações. Monitoring Recovery of Laser-Ablated Interneuromast Cells in Zebrafish Using Confocal Microscopy

Vídeo: Monitoring Recovery of Laser-Ablated Interneuromast Cells in Zebrafish Using Confocal Microscopy - Experimento

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.

Ablações de volume profunda e espacialmente controladas usando um microscópio de dois fótons no Gás de Peixe-Zebra

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

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Biologia do Desenvolvimento

Targeted Laser Ablation in the Embryo of Saccharina latissima

In Saccharina latissima, the embryo&#160;develops as a monolayered cell sheet called the lamina or the blade. Each embryo cell is easy to observe, readily distinguishable from its neighbors, and can be individually targeted. For decades, laser ablation has been used to study embryo development. Here, a protocol for cell-specific laser ablation was developed for early embryos of the brown alga S. latissima. The presented work includes: (1) the preparation of Saccharina embryos, with a description of the critical parameters, including culture conditions, (2) the laser ablation settings, and (3) the monitoring of the subsequent growth of the irradiated embryo using time-lapse microscopy. In addition, details are provided on the optimal conditions for transporting the embryos from the imaging platform back to the lab, which can profoundly affect subsequent embryo development. Algae belonging to the order Laminariales display embryogenesis patterns similar to Saccharina; this protocol can thus be easily transferred to other species in this taxon.

Targeted Laser Ablation in the Embryo of Saccharina latissima

The destruction of specific cells in the embryo is a powerful tool for studying cellular interactions involved in cell fate. The present protocol describes techniques for the laser ablation of targeted cells in the early embryo of the brown alga Saccharina latissima.

Ablação laser direcionada no embrião de Saccharina latissima

In Saccharina latissima, the embryo&#160;develops as a monolayered cell sheet called the lamina or the blade. Each embryo cell is easy to observe, readily ...

Laser Ablation and Intravital Microscopy to Study Intestinal Remodeling

Investigating intestinal recovery in vivo is an exquisite technical challenge. A lack of longitudinal imaging protocols has prevented deeper insights into the cell and tissue scale dynamics that orchestrate intestinal regeneration. Here, we describe an intravital microscopy method that locally induces tissue damage at the single crypt scale and follows the regenerative response of the intestinal epithelium in living mice. Single crypts or larger intestinal fields were ablated by a high-intensity multiphoton infrared laser in a time- and space-controlled manner. Subsequent long-term repetitive intravital imaging enabled the tracking of the damaged areas over time and allowed for the monitoring of crypt dynamics during tissue recovery over a period of multiple weeks. Crypt remodeling events such as crypt fission, fusion, and disappearance were observed in the neighboring tissue upon laser-induced damage. This protocol enables the study of crypt dynamics both in homeostatic and pathophysiological settings, such as aging and tumor initiation.

Here, we present a method to obtain images of the intestine upon laser-induced wounding. By exposing the mouse intestine to a multiphoton laser, the loss of a single or multiple crypt(s) is induced locally. By repeatedly imaging the damaged area over months, the real-time dynamics of intestinal recovery is captured.

Ablação a Laser e Microscopia Intravital no Estudo do Remodelamento Intestinal

Investigating intestinal recovery in vivo is an exquisite technical challenge. A lack of longitudinal imaging protocols has prevented deeper insights into ...

Monitoring Recovery of Laser-Ablated Interneuromast Cells in Zebrafish Using Confocal Microscopy

Transcrição

Monitoring Recovery of Laser-Ablated Interneuromast Cells in Zebrafish Using Confocal Microscopy