visualizing astrocyte morphology using fluorescent dye iontophoresis in a fixed mouse brain slice

Visualizing Astrocyte Morphology Using Fluorescent Dye Iontophoresis in a Fixed Mouse Brain Slice

For the dye injection test, gently place a lightly fixed brain slice into a glass bottom dish filled with 0.1 molar PBS at room temperature. And hold the slice in place with a platinum harp with nylon strings.Connect the electrode to a voltage source and place the ground electrode into the bath containing the brain slice. Move the objective of a confocal microscope to the brain region of interest.And lower the electrode into the solution using the 10x water immersion lens, moving the electrode to the center of the field of view. Then, under bright field, slowly lower the electrode toward the slice, stopping just above the surface.To fill an astrocyte of interest with iontophoresis, use the infrared differential interference contrast to identify astrocytes with elongated, oval-shaped somata, about 10 micrometers in diameter, 40 to 50 micrometers below the slice surface.This is the stratum radiatum of the hippocampus directly below the pyramidal cell layer. As we move through the tissue, we can see blood vessels, neurons, astrocytes, and other cell types.Once an astrocyte has been selected, move the cell to the center of the field of view and slowly lower the electrode tip into the slice. Navigating through the tissue until the electrode is on the same plane as the cell body.Once the cell body of the astrocyte is clearly visible and outlined, slowly and gently advance the electrode forward, moving the electrode until the tip impales the soma of the cell.Move the focus of the objective slowly up and down to note if the electrode is inside the soma. Once the electrode tip is inside the cell, turn on the stimulator at 0.5 to 1 volt to continuously eject current into the cell.Using the confocal microscope, watch the cell fill, increasing the digital zoom to visualize the details of the cell, and to make sure that the tip of the electrode is visible inside the cell as necessary.Wait for about 15 minutes until the finer branches and processes appear defined, before turning off the voltage and gently withdrawing the electrode tip from the cell.To image the filled cell, wait 15 to 20 minutes for the cell to return to its original form, before adjusting the setting on the confocal microscope to make sure that the finer branches and processes appear defined under the 40x objective.Set up a z-stack with a step size of 0.3 micrometers, moving the objective while imaging until there is no signal from the cell. And set that step as the top.Then move the objective down, focusing through the cell until there is no signal. And set that step as the bottom.

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3px;vertical-align:top;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>P3911</td><td style='background-color:#ffffff;border-bottom:1px solid #000000;border-right:1px solid #000000;color:#1a202c;font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:top;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>An identical alternative can be used</td></tr><tr style='height:21px;'><td style='background-color:#ffffff;border-bottom:1px solid #000000;border-left:1px solid #000000;border-right:1px solid #000000;color:#1a202c;font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:top;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>Stimulator- Model Omnical 2010</td><td style='background-color:#ffffff;border-bottom:1px solid #000000;border-right:1px solid #000000;color:#1a202c;font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:top;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>World precision instruments</td><td style='background-color:#ffffff;border-bottom:1px solid #000000;border-right:1px solid #000000;color:#1a202c;font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:top;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>Omnical 2010</td><td style='background-color:#ffffff;border-bottom:1px solid #000000;border-right:1px solid #000000;color:#1a202c;font-size:12pt;overflow:hidden;padding:0px 3px;vertical-align:top;white-space:normal;word-wrap:break-word;wrap-strategy:4;'>A similar alternative can be used</td></tr></tbody></table></figure>

Source:&#160;<a style='text-decoration:none;' href='https://app.jove.com/v/60225/visualizing-astrocyte-morphology-using-lucifer-yellow-iontophoresis'><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;'>Moye, S. L.,&#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;'> Visualizing Astrocyte Morphology Using Lucifer Yellow Iontophoresis.&#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;'> (2019).</a> &#160;This video demonstrates the use of fluorescent dye iontophoresis to study astrocyte morphology in fixed brain slices. It details the piercing of the astrocyte soma with an electrode to deliver an anionic, hydrophilic dye into the cytoplasm under a low-voltage current, enabling the dye to diffuse and label the soma and branches. Confocal microscopy is then used to visualize the labeled astrocytes, providing morphological insights.

Source:&#160;Moye, S. L.,&#160;et.al. Visualizing Astrocyte Morphology Using Lucifer Yellow Iontophoresis.&#160;J. Vis. Exp. (2019).&#160;This video ...

Place a chemically fixed mouse brain slice in a glass bottom dish containing buffer and secure it with a mesh.Connect an electrode filled with an anionic, hydrophilic fluorescent dye to a voltage source. &#160;Insert a ground electrode into the buffer to complete the electrical circuit.Using brightfield illumination, advance the dye-filled electrode toward the slice.Switch to infrared differential interference contrast imaging to locate an astrocyte.Pierce the astrocyte soma with the electrode to access the cytoplasm.Apply an electric current to drive the dye into the cytoplasm via iontophoresis.Switch to confocal microscopy to monitor dye movement.The hydrophilic dye, unable to cross the hydrophobic membrane, diffuses within the cytoplasm to fill the soma and branches.Once the cell is filled, stop the current and withdraw the electrode.Allow the astrocyte membrane to reseal.Acquire images at various Z-planes and reconstruct them to visualize astrocyte morphology.

13 次观看. Visualizing Astrocyte Morphology Using Fluorescent Dye Iontophoresis in a Fixed Mouse Brain Slice

视频: Visualizing Astrocyte Morphology Using Fluorescent Dye Iontophoresis in a Fixed Mouse Brain Slice - 实验

Extracellular Recording of Neuronal Activity Combined with Microiontophoretic Application of Neuroactive Substances in Awake Mice

Differences in the activity of neurotransmitters and neuromodulators, and consequently different neural responses, can be found between anesthetized and awake animals. Therefore, methods allowing the manipulation of synaptic systems in awake animals are required in order to determine the contribution of synaptic inputs to neuronal processing unaffected by anesthetics. Here, we present methodology for the construction of electrodes to simultaneously record extracellular neural activity and release multiple neuroactive substances at the vicinity of the recording sites in awake mice. By combining these procedures, we performed microiontophoretic injections of gabazine to selectively block GABAA receptors in neurons of the inferior colliculus of head-restrained mice. Gabazine successfully modified neural response properties such as the frequency response area and stimulus-specific adaptation. Thus, we demonstrate that our methods are suitable for recording single-unit activity and for dissecting the role of specific neurotransmitter receptors in auditory processing.
The main limitation of the described procedure is the relatively short recording time (~3 hr), which is determined by the level of habituation of the animal to the recording sessions. On the other hand, multiple recording sessions can be performed in the same animal. The advantage of this technique over other experimental procedures used to manipulate the level of neurotransmission or neuromodulation (such as systemic injections or the use of optogenetic models), is that the drug effect is confined to the local synaptic inputs to the target neuron. In addition, the custom-manufacture of electrodes allows adjustment of specific parameters according to the neural structure and type of neuron of interest (such as the tip resistance for improving the signal-to-noise ratio of the recordings).

We present methods for the construction of electrodes to simultaneously record extracellular neural activity and release multiple neuroactive substances at the vicinity of the recording sites in awake mice. This technique allows the detailed analysis of putative local synaptic inputs to the neuron of interest.

神经元电活动外记录与神经活性物质在清醒小鼠微电泳应用相结合

Differences in the activity of neurotransmitters and neuromodulators, and consequently different neural responses, can be found between anesthetized and ...

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Real-time Iontophoresis with Tetramethylammonium to Quantify Volume Fraction and Tortuosity of Brain Extracellular Space

This review describes the basic concepts and protocol to perform the real-time iontophoresis (RTI) method, the gold-standard to explore and quantify the extracellular space (ECS) of the living brain. The ECS surrounds all brain cells and contains both interstitial fluid and extracellular matrix. The transport of many substances required for brain activity, including neurotransmitters, hormones, and nutrients, occurs by diffusion through the ECS. Changes in the volume and geometry of this space occur during normal brain processes, like sleep, and pathological conditions, like ischemia. However, the structure and regulation of brain ECS, particularly in diseased states, remains largely unexplored. The RTI method measures two physical parameters of living brain: volume fraction and tortuosity. Volume fraction is the proportion of tissue volume occupied by ECS. Tortuosity is a measure of the relative hindrance a substance encounters when diffusing through a brain region as compared to a medium with no obstructions. In RTI, an inert molecule is pulsed from a source microelectrode into the brain ECS. As molecules diffuse away from this source, the changing concentration of the ion is measured over time using an ion-selective microelectrode positioned roughly 100 &#181;m away. From the resulting diffusion curve, both volume fraction and tortuosity can be calculated. This technique has been used in brain slices from multiple species (including humans) and in vivo to study acute and chronic changes to ECS. Unlike other methods, RTI can be used to examine both reversible and irreversible changes to the brain ECS in real time.

This protocol describes real-time iontophoresis, a method that measures physical parameters of the extracellular space (ECS) of living brains. The diffusion of an inert molecule released into the ECS is used to calculate the ECS volume fraction and tortuosity. It is ideal for studying acute reversible changes to brain ECS.

用四甲基铵进行实时离子电渗疗法，以量化体细胞分数和脑细胞外空间的变性

This review describes the basic concepts and protocol to perform the real-time iontophoresis (RTI) method, the gold-standard to explore and quantify the ...

Analysis of Astrocyte Territory Volume and Tiling in Thick Free-Floating Tissue Sections

Astrocytes possess an astounding degree of morphological complexity that enables them to interact with nearly every type of cell and structure within the brain. Through these interactions, astrocytes actively regulate many critical brain functions, including synapse formation, neurotransmission, and ion homeostasis. In the rodent brain, astrocytes grow in size and complexity during the first three postnatal weeks and establish distinct, non-overlapping territories to tile the brain. This protocol provides an established method for analyzing astrocyte territory volume and astrocyte tiling using free-floating tissue sections from the mouse brain. First, this protocol describes the steps for tissue collection, cryosectioning, and immunostaining of free-floating tissue sections. Second, this protocol describes image acquisition and analysis of astrocyte territory volume and territory overlap volume, using commercially available image analysis software. Lastly, this manuscript discusses the advantages, important considerations, common pitfalls, and limitations of these methods. This protocol requires brain tissue with sparse or mosaic fluorescent labeling of astrocytes, and is designed to be used with common lab equipment, confocal microscopy, and commercially available image analysis software.

This protocol describes methods for sectioning, staining, and imaging free-floating tissue sections of the mouse brain, followed by a detailed description of the analysis of astrocyte territory volume and astrocyte territory overlap or tiling.

厚自由漂浮组织切片中星形胶质细胞区域体积和瓷砖的分析

Astrocytes possess an astounding degree of morphological complexity that enables them to interact with nearly every type of cell and structure within the ...

Visualizing Astrocyte Morphology Using Fluorescent Dye Iontophoresis in a Fixed Mouse Brain Slice

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Visualizing Astrocyte Morphology Using Fluorescent Dye Iontophoresis in a Fixed Mouse Brain Slice