Name: confocal imaging of mitochondrial movement within oligodendrocytes in organotypic brain slice cultures
Uploaded: 2025-04-28T12:03:10.000+00:00
Duration: 1 min 12 s
Description: Source: Kennedy, L. H., et. al. Visualization and Live Imaging of Oligodendrocyte Organelles in Organotypic Brain Slices Using Adeno-associated Virus and ...

confocal imaging of mitochondrial movement within oligodendrocytes in organotypic brain slice cultures

Confocal Imaging of Mitochondrial Movement within Oligodendrocytes in Organotypic Brain Slice Cultures

Use forceps to transfer the confetti with the slice from the Petri dish to the top of the bath. Then place the two tips of the forceps on each side of the confetti so that they touch the confetti without touching the slice. And push the confetti through the solution to the bottom of the bath. Center the confetti in the middle of the bath.Use forceps to place the hold-down anchor or harp on top of the confetti without touching the slice. Then turn the peristaltic pump back on. Lower the objective down to the sample. Then use the eyepieces and the fluorescent lamp to quickly find a healthy looking oligodendrocyte with fluorescent protein expression.Use the live function in the software to identify the cell on the screen. And choose the area of interest. Here, an area containing several primary processes and one myelin sheath will be imaged. Zoom in on the field of interest. This will typically produce an image with pixel size of 0.14 to 0.30 microns.Select the Regions tool and draw a rectangle around the area. Choose the option to scan only the selected region. Scanning time and thus laser exposure is reduced by only scanning the selected region.Adjust the laser power and gain to get a good view of the mitochondria. Use low laser power and high gain to avoid bleaching during live imaging. If necessary, adjust the digital offset.Minimize scanning time by selecting a fast scanning speed. Set the frequency and duration of timelapse recording for mitochondrial imaging and oligodendrocytes. Capture images every two seconds for a total of 20 minutes. Start the time lapse recording.The continuous flow of solution can cause movement of the slice. It's worth spending some time minimizing this movement by adjusting the in and outlets of the bath. You can also reduce the pump speed.Continually monitor the screen during time lapse imaging, as small changes in focus usually still occur. Adjust the focus as necessary. After time lapse imaging, capture a&#160;Z-stack of the whole cell, for future identification of the cell and imaged process.

confocal-imaging-mitochondrial-movement-within-oligodendrocytes

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<a href='https://app.jove.com/v/56237/visualization-live-imaging-oligodendrocyte-organelles-organotypic'>Source: Kennedy, L. H., et. al. Visualization and Live Imaging of Oligodendrocyte Organelles in Organotypic Brain Slices Using Adeno-associated Virus and Confocal Microscopy. J. Vis. Exp. (2017)</a>This video demonstrates the imaging of oligodendrocyte mitochondria in organotypic mouse brain slices. The slice is placed inside a bath chamber with continuous fluid circulation and controlled temperature. After setting up various parameters of the confocal microscope, time-lapse images of mitochondria with red fluorescence are captured, followed by Z-stack images of the oligodendrocyte with green fluorescence.

Source: Kennedy, L. H., et. al. Visualization and Live Imaging of Oligodendrocyte Organelles in Organotypic Brain Slices Using Adeno-associated Virus and ...

Begin with a confocal microscope bath chamber setup with a circulating imaging solution and controlled temperature.&#160;&#160;Take a hydrophilic polymeric membrane containing an organotypic mouse brain slice in which the oligodendrocytes have been transduced to express a mitochondria-specific red fluorescent protein and a cytosol-specific green fluorescent protein.Dual fluorescence allows clear visualization of mitochondrial dynamics within the cytosol of the oligodendrocyte.Submerge the slice in the center of the bath and secure it with a harp anchor.Lower the objective and select a healthy oligodendrocyte for scanning.Adjust laser power to minimize cell toxicity and photobleaching.Set microscope parameters and then record time-lapse images of fluorescently labeled mitochondria.Capture z-stack images at different depths to obtain a high-resolution, three-dimensional view of the entire cell.Process the images to visualize mitochondrial movement within the oligodendrocyte.

11 vistas. Confocal Imaging of Mitochondrial Movement within Oligodendrocytes in Organotypic Brain Slice Cultures

Video: Confocal Imaging of Mitochondrial Movement within Oligodendrocytes in Organotypic Brain Slice Cultures - Experimento

Time-lapse Confocal Imaging of Migrating Neurons in Organotypic Slice Culture of Embryonic Mouse Brain Using In Utero Electroporation

In utero electroporation is a rapid and powerful approach to study the process of radial migration in the cerebral cortex of developing mouse embryos. It has helped to describe the different steps of radial migration and characterize the molecular mechanisms controlling this process. To directly and dynamically analyze migrating neurons they have to be traced over time. This protocol describes a workflow that combines in utero electroporation with organotypic slice culture and time-lapse confocal imaging, which allows for a direct examination and dynamic analysis of radially migrating cortical neurons. Furthermore, detailed characterization of migrating neurons, such as migration speed, speed profiles, as well as radial orientation changes, is possible. The method can easily be adapted to perform functional analyses of genes of interest in radially migrating cortical neurons by loss and gain of function as well as rescue experiments. Time-lapse imaging of migrating neurons is a state-of-the-art technique that once established is a potent tool to study the development of the cerebral cortex in mouse models of neuronal migration disorders.

Time-lapse Confocal Imaging of Migrating Neurons in Organotypic Slice Culture of Embryonic Mouse Brain Using In Utero Electroporation

This protocol provides instructions for direct observation of radially migrating cortical neurons. In utero electroporation, organotypic slice culture, and time-lapse confocal imaging are combined to directly and dynamically study the effects of overexpression or downregulation of genes of interest in migrating neurons and to analyze their differentiation during development.

Time-lapse Imágenes confocales de las neuronas migratorias en la cultura organotípica en rebanadas de cerebro de ratón embrionario<em&gt; En Utero</em&gt; Electroporación

In utero electroporation is a rapid and powerful approach to study the process of radial migration in the cerebral cortex of developing mouse embryos. It ...

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Modified Roller Tube Method for Precisely Localized and Repetitive Intermittent Imaging During Long-term Culture of Brain Slices in an Enclosed System

Cultured rodent brain slices are useful for studying the cellular and molecular behavior of neurons and glia in an environment that maintains many of their normal in vivo interactions. Slices obtained from a variety of transgenic mouse lines or use of viral vectors for expression of fluorescently tagged proteins or reporters in wild type brain slices allow for high-resolution imaging by fluorescence microscopy. Although several methods have been developed for imaging brain slices, combining slice culture with the ability to perform repetitive high-resolution imaging of specific cells in live slices over long time periods has posed problems. This is especially true when viral vectors are used for expression of exogenous proteins since this is best done in a closed system to protect users and prevent cross contamination. Simple modifications made to the roller tube brain slice culture method that allow for repetitive high-resolution imaging of slices over many weeks in an enclosed system are reported. Culturing slices on photoetched coverslips permits the use of fiducial marks to rapidly and precisely reposition the stage to image the identical field over time before and after different treatments. Examples are shown for the use of this method combined with specific neuronal staining and expression to observe changes in hippocampal slice architecture, viral-mediated neuronal expression of fluorescent proteins, and the development of cofilin pathology, which was previously observed in the hippocampus of Alzheimer's disease (AD) in response to slice treatment with oligomers of amyloid-&#946; (A&#946;) peptide.

Presented here is a modified roller tube method for culturing and intermittent high-resolution imaging of rodent brain slices over many weeks with precise repositioning on photoetched coverslips. Neuronal viability and slice morphology are well maintained. Applications of this fully enclosed system using viruses for cell-type specific expression are provided.

Método de tubo de rodillo modificado precisamente localizada y repetitiva imagen intermitente durante el cultivo a largo plazo de las rebanadas de cerebro en un sistema cerrado

Cultured rodent brain slices are useful for studying the cellular and molecular behavior of neurons and glia in an environment that maintains many of ...

Visualizing and Analyzing Intracellular Transport of Organelles and Other Cargos in Astrocytes

Astrocytes are among the most abundant cell types in the adult brain, where they play key roles in a multiplicity of functions. As a central player in brain homeostasis, astrocytes supply neurons with vital metabolites and buffer extracellular water, ions, and glutamate. An integral component of the &#8220;tri-partite&#8221; synapse, astrocytes are also critical in the formation, pruning, maintenance, and modulation of synapses. To enable these highly interactive functions, astrocytes communicate among themselves and with other glial cells, neurons, the brain vasculature, and the extracellular environment through a multitude of specialized membrane proteins that include cell adhesion molecules, aquaporins, ion channels, neurotransmitter transporters, and gap junction molecules. To support this dynamic flux, astrocytes, like neurons, rely on tightly coordinated and efficient intracellular transport. Unlike neurons,&#160;where intracellular trafficking has been extensively delineated, microtubule-based transport in astrocytes has been less studied. Nonetheless, exo- and endocytic trafficking of cell membrane proteins and intracellular organelle transport orchestrates astrocytes&#8217; normal biology, and these processes are often affected in disease or in response to injury. Here we present a straightforward protocol to culture high quality murine astrocytes, to fluorescently label astrocytic proteins and organelles of interest, and to record their intracellular transport dynamics using time-lapse confocal microscopy. We also demonstrate how to extract and quantify relevant transport parameters from the acquired movies using available image analysis software (i.e., ImageJ/FIJI) plugins.

Here we describe an in vitro live-imaging method to visualize intracellular transport of organelles and trafficking of plasma membrane proteins in murine astrocytes. This protocol also presents an image analysis methodology to determine cargo transport itineraries and kinetics.

Visualización y análisis del transporte intracelular de organelos y otros Cargos en astrocitos

Astrocytes are among the most abundant cell types in the adult brain, where they play key roles in a multiplicity of functions. As a central player in ...

Confocal Imaging of Mitochondrial Movement within Oligodendrocytes in Organotypic Brain Slice Cultures

Transcripción

Confocal Imaging of Mitochondrial Movement within Oligodendrocytes in Organotypic Brain Slice Cultures