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All procedures involving animal models have been reviewed by the local institutional animal care committee and the JoVE veterinary review board.
1. Isolation and Plating of Mixed Cortical Cells
Mixed cortical cell isolation for astrocyte cultures can be performed using P1 to P4 mouse pups. In order to achieve proper astrocyte density it is necessary to use 4 mouse pup cortices per T75 tissue culture flask. Therefore, volumes in the following protocol are calculated for a cell preparation using 4 mouse pups.
<ol>
	<li>Before starting the dissection procedure, prewarm 30 mL of astrocyte culture media (DMEM, high glucose + 10% heat-inactivated fetal bovine serum + 1% Penicillin/Streptomycin; see table) to 37 &#176;C. Coat one T75 flask with 20 mL of poly-D-lysine (PDL) at a concentration of 50 &#956;g/mL in cell culture grade water for 1 hr at 37 &#176;C in the CO2&#160;incubator.</li>
	<li>For the dissection procedure, prepare all necessary reagents and materials. You will need surgical scissors, smooth fine forceps, flat tip forceps, paper towels, a waste bag, 70% ethanol, and 2 dissecting dishes (3.5 cm diameter) on ice filled with 2 mL HBSS each.</li>
	<li>Gently hold and spray the head and neck of the mouse pup with 70% ethanol. The animal is sacrificed by decapitation using scissors.</li>
	<li>Perform a midline incision, posterior to anterior, along the scalp to reveal the skull.</li>
	<li>Cut the cranium carefully from the neck to the nose. Two additional cuts are performed to allow further access to the brain: The first cut is made anterior of the olfactory bulbs, the other one inferior of the cerebellum to disconnect the cranium from the skull base.</li>
	<li>Using the flat tip forceps, the cranial flaps are gently flipped to the side and the brain is taken out and placed into the first dissecting dish filled with HBSS. Place the dish back on ice and continue harvesting all 4 brains.</li>
	<li>The remainder of the dissection procedure is performed under a stereomicroscope. First, the olfactory bulbs and the cerebellum are removed using the fine dissecting forceps (Figure 1B).</li>
	<li>In order to retrieve the cortices, grab the posterior end of the brain with the fine forceps, perform a midline incision between the hemispheres, insert a second set of forceps to the created grove and peel away the plate-like structure of the cortex from the brain.</li>
	<li>Carefully dissect the meninges from the cortex hemispheres by pulling with the fine forceps (Figure 1D&#39;). This step avoids contamination of the final astrocyte culture by meningeal cells and fibroblasts. Transfer the prepared cortex hemispheres into the second dish filled with HBSS and return it onto ice. Continue accordingly with all 4 cortices.</li>
	<li>Finally, cut each cortex hemisphere into small pieces using sharp blades (approximately 4 to 8 times).</li>
	<li>Under sterile conditions, transfer cortex pieces into one 50 mL Falcon tube and add HBSS to a total volume of 22.5 mL.</li>
	<li>Add 2.5 mL of 2.5 % trypsin, mix and incubate the tissue in the water bath at 37 &#176;C for 30 min. Mix by occasional shaking every 10 min.</li>
	<li>Centrifuge for 5 min at 300 x g to pellet cortex tissue pieces.</li>
	<li>Carefully remove supernatant by decantation. In order to avoid losing the tissue pellet you may mechanically retain it using a pipette. Dissociate the tissue into a single cell suspension by adding 10 mL astrocyte plating medium and vigorous pipetting using a 10 mL plastic pipette until tissue pieces are dissociated into single cells (20 to 30 times). Adjust volume to 20 mL using astrocyte plating medium. You can proof the dissociation of the cortex tissue into single cells by counting using a hematocytometer. One preparation of 4 mouse pup cortices should yield 10&#8211;15 x106&#160;dissociated single cells.</li>
	<li>Aspirate PDL from the T75 culture flask, plate the dissociated single cell suspension and incubate at 37 &#176;C in the CO2&#160;incubator.</li>
</ol>
2. Obtaining an Enriched Astrocyte Culture
<ol>
	<li>Change the medium 2 days after plating of the mixed cortical cells and all 3 days thereafter.</li>
	<li>After 7 to 8 days, when astrocytes are confluent and overlaying microglia sit exposed on the astrocyte layer or are already detached from the astrocyte layer (Figure 2), shake the T75 flask at 180 rpm for 30 min on an orbital shaker to remove microglia. Discard the supernatant containing microglia or if you wish to culture and examine microglia, spin it down and plate for culture.</li>
	<li>Add 20 mL fresh astrocyte culture medium and continue by shaking the flask at 240 rpm for 6 hr to remove oligodendrocyte precursor cells (OPC). Since some OPCs will not completely detach from the astrocyte layer, continue to shake vigorously by hand for 1 min in order to prevent OPC contamination. Discard the supernatant or spin it down and plate, if you wish to culture OPCs.</li>
	<li>Rinse the remaining confluent astrocyte layer twice with PBS, aspirate the PBS, add 5 mL trypsin-EDTA and incubate in the CO2&#160;incubator at 37 &#176;C. Check detachment of astrocytes every 5 min and enforce detachment of astrocytes by hitting the flask against the palm of your hand (2&#8211;3 times).</li>
	<li>After astrocytes are detached from the culture flask, add 5 mL of astrocyte culture medium, spin cells at 180 x g for 5 min, aspirate supernatant and add 40 mL fresh astrocyte plating medium. One T75 tissue culture flask should yield around 1x106&#160;cells after the first cell split. Plate cells in two T75 culture flasks and incubate at 37 &#176;C in the CO2&#160;incubator. Change the medium every 2 to 3 days.</li>
	<li>12&#8211;14 days after the first split astrocytes are plated in the appropriate cell concentration 24&#8211;48 hr before performing the experiment. One T75 tissue culture flask should yield around 1.5&#8211;2 x106&#160;cells after the second cell split.</li>
</ol>

<table border="1" fo:keep-together.within-page="1" fo:keep-with-next.within-page="always">
	<tbody>
		<tr>
			<td>Astrocyte culture media</td>
			<td></td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>DMEM high glucose</td>
			<td>&#160;Life Technologies</td>
			<td>&#160;31966-021</td>
			<td></td>
		</tr>
		<tr>
			<td>FBS heat-inactivated</td>
			<td>&#160;Life Technologies</td>
			<td>&#160;10082-147</td>
			<td>&#160;Final Concentration: 10%</td>
		</tr>
		<tr>
			<td>Penicillin-Streptomycin</td>
			<td>&#160;Life Technologies</td>
			<td>&#160;15140-122</td>
			<td>&#160;Final Concentration: 1%</td>
		</tr>
		<tr>
			<td>Solution for brain tissue digestion</td>
			<td></td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>HBSS</td>
			<td>&#160;Life Technologies</td>
			<td>&#160;14170-088</td>
			<td></td>
		</tr>
		<tr>
			<td>2.5% Trypsin</td>
			<td>&#160;Life Technologies</td>
			<td>&#160;15090-046</td>
			<td>&#160;Final Concentration: 0.25%</td>
		</tr>
		<tr>
			<td>Other</td>
			<td></td>
			<td></td>
			<td></td>
		</tr>
		<tr>
			<td>70% (vol/vol) ethanol</td>
			<td>&#160;Roth</td>
			<td>&#160;9065.2</td>
			<td></td>
		</tr>
		<tr>
			<td>Poly-D-Lysine</td>
			<td>&#160;Millipor A-003</td>
			<td>&#160;A-003-E</td>
			<td></td>
		</tr>
		<tr>
			<td>Water</td>
			<td>&#160;PAA</td>
			<td>&#160;S15-012</td>
			<td>&#160;Cell culture grade</td>
		</tr>
		<tr>
			<td>PBS</td>
			<td>&#160;PAA</td>
			<td>&#160;H15-002</td>
			<td>&#160;Cell culture grade</td>
		</tr>
		<tr>
			<td>0.05% Trypsin-EDTA</td>
			<td>&#160;Life Technologies</td>
			<td>&#160;25300-062</td>
			<td></td>
		</tr>
		<tr>
			<td>0.45 &#181;m Sterile filter</td>
			<td>&#160;Sartorius</td>
			<td>&#160;16555</td>
			<td></td>
		</tr>
		<tr>
			<td>3.5 cm petri dish</td>
			<td>&#160;BD Falcon</td>
			<td>&#160;353001</td>
			<td></td>
		</tr>
		<tr>
			<td>15 ml Falcon tube</td>
			<td>&#160;BD Falcon</td>
			<td>&#160;352096</td>
			<td></td>
		</tr>
		<tr>
			<td>50 ml Falcon tube</td>
			<td>&#160;BD Falcon</td>
			<td>&#160;352070</td>
			<td></td>
		</tr>
		<tr>
			<td>75 cm2 Tissue culture flask</td>
			<td>&#160;BD Falcon</td>
			<td>&#160;353136</td>
			<td></td>
		</tr>
		<tr>
			<td>Forceps fine</td>
			<td>&#160;Dumont</td>
			<td>&#160;2-1032; 2-1033</td>
			<td>&#160;#3c; #5</td>
		</tr>
		<tr>
			<td>Forceps flat tip</td>
			<td>&#160;KLS Martin</td>
			<td>&#160;12-120-11</td>
			<td></td>
		</tr>
		<tr>
			<td>13 cm surgical scissors</td>
			<td>&#160;Aesculap</td>
			<td>&#160;BC-140-R</td>
			<td></td>
		</tr>
		<tr>
			<td>Stereomicroscope</td>
			<td>&#160;Leica</td>
			<td></td>
			<td>&#160;MZ7.5</td>
		</tr>
		<tr>
			<td>Stereomicroscope + Camera</td>
			<td>&#160;Leica</td>
			<td></td>
			<td>&#160;MZ16F; DFC320</td>
		</tr>
		<tr>
			<td>Microscope + Camera</td>
			<td>&#160;Zeiss; Canon</td>
			<td></td>
			<td>&#160;Primo Vert; PowerShot A650 IS</td>
		</tr>
		<tr>
			<td>Centrifuge</td>
			<td>&#160;Eppendorf</td>
			<td>&#160;5805000.017</td>
			<td>&#160;Centrifuge5804R</td>
		</tr>
		<tr>
			<td>Orbital Shaker</td>
			<td>&#160;Thermo Scientific</td>
			<td>&#160;SHKE 4450-1CE</td>
			<td>&#160;MaxQ 4450</td>
		</tr>
		<tr>
			<td>Water bath</td>
			<td>&#160;Julabo</td>
			<td></td>
			<td>&#160;SW20; 37 &#176;C</td>
		</tr>
	</tbody>
</table>

astrocyte isolation: a method to obtain pure preparation of mouse cortical astrocytes

Source: Schildge, S. et al. <a href="https://www.jove.com/v/50079/isolation-and-culture-of-mouse-cortical-astrocytes">Isolation and Culture of Mouse Cortical Astrocytes.</a> J. Vis. Exp. (2013)
In this video, we describe the method to obtain a pure preparation of astrocytes from newly born mice.

<img alt="Figure 1" src="/files/ftp_upload/20633/20633_Figure1.jpg" /> 
Figure 1. Dissection of postnatal (P3) mouse cortex.&#160;A) Whole brain. B) Brain after removal of olfactory bulbs and cerebellum. C) Isolation of cortices by peeling off the plate-like structure of the cortex from the brain. D, D&#39;) Cortex from ventral and dorsal site with meninges (black arrows indicate meningeal arteries). E) Cortex without meninges. Scale bar, 1.5 mm.
<p...

Astrocyte Isolation: A Method to Obtain Pure Preparation of Mouse Cortical Astrocytes

Source: Schildge, S. et al. Isolation and Culture of Mouse Cortical Astrocytes. J. Vis. Exp. (2013)
In this video, we describe the method to obtain a pure ...

The astrocyte in vitro culture helps investigate the biological role of astrocytes - the most abundant brain cells.
Begin with a neonatal mouse brain placed under a dissecting microscope.
Remove the olfactory bulbs and the cerebellum.
Perform a midline incision between the two hemispheres to separate the cortex.
Remove the meninges to avoid contamination in the astrocyte culture from fibroblasts and meningeal cells.
Transfer the cortex hemispheres into an ice-cold medium and mince into small pieces.
Collect the cortical pieces in a tube containing trypsin. Trypsin, a protease enzyme, digests the cell adhesion proteins, facilitating cell separation.
Centrifuge to pellet the digested tissue.
Remove the supernatant and add an astrocyte medium to the pellet. Pipette vigorously to release a mixed cell population of astrocytes, microglia, and oligodendrocyte precursor cells or OPCs.
Seed this cell suspension into a poly-lysine coated tissue culture flask and incubate.
The negatively charged cells attach to the positively charged poly-lysine and grow over the entire surface to form a confluent layer.
Shake the flask to detach the loosely bound microglia and OPCs. Remove the supernatant containing detached cells.
Add trypsin to the astrocyte layer. Collect the cells and centrifuge.
Resuspend the pellet and divide the astrocytes into multiple flasks.
Finally, assess the purity of the astrocyte culture by immunostaining cell-specific markers.

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JoVE Encyclopedia of Experiments

Cancer Research

Cancers of the Nervous System

In vitro studies

1.5K Views. Source: Schildge, S. et al. Isolation and Culture of Mouse Cortical Astrocytes. J. Vis. Exp. (2013) In this video, we describe the method to obtain a pure preparation of astrocytes from newly born mice. 

Video: Astrocyte Isolation: A Method to Obtain Pure Preparation of Mouse Cortical Astrocytes - Concept

Primary Microglia Isolation from Mixed Glial Cell Cultures of Neonatal Rat Brain Tissue

Microglia account for approximately 12% of the total cellular population in the mammalian brain. While neurons and astrocytes are considered the major cell types of the nervous system, microglia play a significant role in normal brain physiology by monitoring tissue for debris and pathogens and maintaining homeostasis in the parenchyma via phagocytic activity 1,2. Microglia are activated during a number of injury and disease conditions, including neurodegenerative disease, traumatic brain injury, and nervous system infection 3. Under these activating conditions, microglia increase their phagocytic activity, undergo morpohological and proliferative change, and actively secrete reactive oxygen and nitrogen species, pro-inflammatory chemokines and cytokines, often activating a paracrine or autocrine loop 4-6. As these microglial responses contribute to disease pathogenesis in neurological conditions, research focused on microglia is warranted.
	Due to the cellular heterogeneity of the brain, it is technically difficult to obtain sufficient microglial sample material with high purity during in vivo experiments. Current research on the neuroprotective and neurotoxic functions of microglia require a routine technical method to consistently generate pure and healthy microglia with sufficient yield for study. We present, in text and video, a protocol to isolate pure primary microglia from mixed glia cultures for a variety of downstream applications. Briefly, this technique utilizes dissociated brain tissue from neonatal rat pups to produce mixed glial cell cultures. After the mixed glial cultures reach confluency, primary microglia are mechanically isolated from the culture by a brief duration of shaking. The microglia are then plated at high purity for experimental study.
	The principle and protocol of this methodology have been described in the literature 7,8. Additionally, alternate methodologies to isolate primary microglia are well described 9-12. Homogenized brain tissue may be separated by density gradient centrifugation to yield primary microglia 12. However, the centrifugation is of moderate length (45 min) and may cause cellular damage and activation, as well as, cause enriched microglia and other cellular populations. Another protocol has been utilized to isolate primary microglia in a variety of organisms by prolonged (16 hr) shaking while in culture 9-11. After shaking, the media supernatant is centrifuged to isolate microglia. This longer two-step isolation method may also perturb microglial function and activation. We chiefly utilize the following microglia isolation protocol in our laboratory for a number of reasons: (1) primary microglia simulate in vivo biology more faithfully than immortalized rodent microglia cell lines, (2) nominal mechanical disruption minimizes potential cellular dysfunction or activation, and (3) sufficient yield can be obtained without passage of the mixed glial cell cultures.
	It is important to note that this protocol uses brain tissue from neonatal rat pups to isolate microglia and that using older rats to isolate microglia can significantly impact the yield, activation status, and functional properties of isolated microglia. There is evidence that aging is linked with microglia dysfunction, increased neuroinflammation and neurodegenerative pathologies, so previous studies have used ex vivo adult microglia to better understand the role of microglia in neurodegenerative diseases where aging is important parameter. However, ex vivo microglia cannot be kept in culture for prolonged periods of time. Therefore, while this protocol extends the life of primary microglia in culture, it should be noted that the microglia behave differently from adult microglia and in vitro studies should be carefully considered when translated to an in vivo setting.

Isolating primary microglia from the cellular heterogeneity of the brain is essential to investigate their role in both physiological and pathological conditions. This protocol describes a mechanical isolation and mixed cell culture technique that provides high yield and high purity, viable primary microglial cells for in vitro study and downstream applications.

Microglia account for approximately 12% of the  total cellular population in the mammalian brain. While neurons and astrocytes are considered  the major ...

JoVE Journal

Immunology and Infection

Culturing In Vivo-like Murine Astrocytes Using the Fast, Simple, and Inexpensive AWESAM Protocol

The AWESAM (a low-cost easy stellate astrocyte method) protocol entails a fast, simple, and inexpensive way to generate large quantities of in vivo-like mouse and rat astrocyte monocultures: Brain cells can be isolated from different brain regions, and after a week of cell culture, non-astrocytic cells are shaken off by placing the culture dishes on a shaker for 6 h in the incubator. The remaining astrocytes are then passaged into new plates with an astrocyte-specific medium (termed NB+H). NB+H contains low concentrations of heparin-binding EGF-like growth factor (HBEGF), which is used in place of serum in medium. After growing in NB+H, AWESAM astrocytes have a stellate morphology and feature fine processes. Moreover, these astrocytes have more in vivo-like gene expression than astrocytes generated by previously published methods. Ca2+ imaging, vesicle dynamics, and other events close to the membrane can thus be studied in the fine astrocytic processes in vitro, e.g., using live cell confocal or TIRF microscopy. Notably, AWESAM astrocytes also exhibit spontaneous Ca2+ signaling similar to astrocytes in vivo.

Culturing In Vivo-like Murine Astrocytes Using the Fast, Simple, and Inexpensive AWESAM Protocol

The AWESAM protocol described here is optimal for culturing murine astrocytes in isolation from other brain cells in a fast, simple, and inexpensive manner. AWESAM astrocytes exhibit spontaneous Ca2+ signaling, morphology, and gene expression profiles similar to astrocytes in vivo.

The AWESAM (a low-cost easy stellate astrocyte method) protocol entails a fast, simple, and inexpensive way to generate large quantities of in vivo-like ...

Neuroscience

In vitro Modeling for Neurological Diseases using Direct Conversion from Fibroblasts to Neuronal Progenitor Cells and Differentiation into Astrocytes

Research on neurological disorders focuses primarily on the impact of neurons on disease mechanisms. Limited availability of animal models severely impacts the study of cell type specific contributions to disease. Moreover, animal models usually do not reflect variability in mutations and disease courses seen in human patients. Reprogramming methods for generation of induced pluripotent stem cells (iPSCs) have revolutionized patient specific research and created valuable tools for studying disease mechanisms. However, iPSC technology has disadvantages such as time, labor commitment, clonal selectivity and loss of epigenetic markers. Recent modifications of these methods allow more direct generation of cell lineages or specific cell types, bypassing clonal isolation or a pluripotent stem cell state. We have developed a rapid direct conversion method to generate induced Neuronal Progenitor Cells (iNPCs) from skin fibroblasts utilizing retroviral vectors in combination with neuralizing media. The iNPCs can be differentiated into neurons (iNs) oligodendrocytes (iOs) and astrocytes (iAs). iAs production facilitates rapid drug and disease mechanism testing as differentiation from iNPCs only takes 5 days. Moreover, iAs are easy to work with and are generated in pure populations at large numbers. We developed a highly reproducible co-culture assay using mouse GFP+ neurons and patient derived iAs to evaluate potential therapeutic strategies for numerous neurological and neurodegenerative disorders. Importantly, the iA assays are scalable to 384-well format facilitating the evaluation of multiple small molecules in one plate. This approach allows simultaneous therapeutic evaluation of multiple patient cell lines with diverse genetic background. Easy production and storage of iAs and capacity to screen multiple compounds in one assay renders this methodology adaptable for personalized medicine.

We describe a protocol to reprogram human skin-derived fibroblasts into induced Neuronal Progenitor Cells (iNPCs), and their subsequent differentiation into induced Astrocytes (iAs). This method leads to fast and reproducible generation of iNPCs and iAs in large quantities.

Research on neurological disorders focuses primarily on the impact of neurons on disease mechanisms. Limited availability of animal models severely ...

Astrocyte Isolation: A Method to Obtain Pure Preparation of Mouse Cortical Astrocytes

Transcript