eoe sub articles

EoE Sub Articles

1. Perform&#160;In Utero&#160;Electroporation
<ol>
	<li>Breed 6 to 8-week-old mice and prepare the tools for&#160;in utero&#160;electroporation. Cross male homozygous&#160;Rosa26-CAG-LSL-Cas9-P2A-EGFP&#160;mice with female CD-1 mice. Time the pregnancy of the CD-1 mice from the day the vaginal plug is detected (E0.5). Embryos are electroporated at day E13.5.
	<ol>
		<li>Pull borosilicate glass capillaries (inside diameter: 0.6&#8211;0.8 mm) with a micropipette puller. Use the following settings: P = 500, Heat = 560, Pull = 150, Vel = 75, Time = 250. Label the capillary tip with black ink for better visualization during the injection. Trim the capillary taper under a stereomicroscope using a ruler and sharp needle tweezers and trim the tip at a length of about 6 mm.</li>
		<li>Maintain the unity of the capillaries to keep the experiment reproducible. Create a one-sided beveled edge during the trimming. The tip should be as sharp as possible for easy penetration of the uterine wall and to avoid tissue damage of the embryo. 
		NOTE: Alternatively, use a micro-grinder to adjust a 35&#176; angle. The capillaries can be stored at room temperature in a 10 cm Petri dish under pathogen-free conditions.</li>
		<li>Autoclave the surgical instruments.</li>
		<li>Mix the sgRNA-plasmids in equal parts with pT2K-IRES-Luc to a final concentration of at least 1 &#181;g/&#181;L for each plasmid and color the plasmid-solution with fast green (final concentration of 0.05%). Prepare 1% fast green stock solution with endotoxin-free distilled water and filter through a 0.22 &#181;m filter to remove dye particles from the solution. 
		NOTE: Co-transfection of pT2K IRES-Luc is optional, but allows for identification of viable electroporated animals after birth using bioluminescence imaging. Prepare a sufficient amount of plasmid-mix for the total number of pregnant mice to be operated. Use about 15&#8211;20 &#181;L mix per mouse (~12 embryos). Proceed immediately with the surgery.</li>
	</ol>
	</li>
	<li>Prepare mice for surgery
	<ol>
		<li>Anesthetize pregnant CD-1 mice with isoflurane. Induce anesthesia in a box with 3&#8211;4 vol-% isoflurane (oxygen flow rate: 1.5 L/min) and maintain it with 2 vol-% during surgery via nose cone. 
		NOTE: The complete surgery should not take longer than 30 min. Reduce the number of injected and electroporated embryos, if necessary.&#160;Use sterile gloves for surgery.</li>
		<li>Place the mouse on its back on a heating pad and adjust anesthesia.</li>
		<li>Inject analgesic (Metamizol, 800 mg/kg body weight, subcutaneously (s.c.), 24 h depot). 
		NOTE: You may use other authorized analgesics than Metamizol.</li>
		<li>Apply eye ointment to prevent eye-dryness during surgery.</li>
		<li>Fix limbs with tape and sterilize the abdomen with a disinfectant. Cover the mouse with gauze, leaving only the surgical area exposed. Spread 70% ethanol over surgical area and gauze.</li>
		<li>Make a skin incision of about 2 cm in length and widen the gap gently with straight surgical scissors. Locate the linea alba and make a slightly smaller second incision through the peritoneum using tissue scissors with blunt tip.</li>
		<li>Moisten the opened abdominal cavity with pre-warmed sterile 1x PBS.</li>
		<li>Carefully extract the uterine horns from the abdominal cavity using ring forceps. Pull gently by grabbing the uterine wall solely at the gap between the yolk sacs of two neighbouring embryos. Avoid any pressure on the embryo while pulling it through the incision. Enlarge the incision if necessary and take extra care to position the uterine horns onto the abdomen while not compressing blood flow through the uterine artery. 
		NOTE: In some cases, it is advised to extract one uterine horn at a time and replace it before proceeding with the second uterine horn.</li>
	</ol>
	</li>
	<li>Injection and electroporation of plasmid DNAs
	<ol>
		<li>Aspirate approximately 15 &#181;L of colored plasmid-solution with the prepared glass capillary. Avoid any air-bubbles during this process. 
		NOTE: The plasmid-solution can clog the tip easily if its concentration is high. Test the capillary by releasing some DNA right before the injection.</li>
		<li>Gently hold the embryo with ring forceps and locate the neck area. 
		NOTE: If the embryo is in a position difficult to inject, skip it and go for the next embryo. Increased repositioning of the embryo may increase chances of damage to them.</li>
		<li>Slowly pierce with the tip of the previously prepared glass capillary into the fourth ventricle by penetrating through the dorsal hindbrain and subsequently inject about 1 &#181;L of the plasmid-mix. Confirm that the dyed DNA is not leaked from the brain and is visible as a diamond shaped structure. 
		NOTE: As an option, use 2.5-fold magnifying glasses for better visualization of the fourth ventricle and surrounding blood vessels. Deliver electric pulses immediately after injection to prevent diffusion of the plasmid-solution to the other ventricles.</li>
		<li>Apply electric square pulses (5 pulses, 32 mV, 50 ms-on, 950 ms-off) with forceps-like platinum tweezers (see&#160;Table of Materials). Place the electrodes laterally with the negative pole covering the ear and the positive pole positioned at the cerebellar primordium over the uterine wall. Use 5 mm-diameter electrode plates for effective electroporation of E13.5 embryos. 
		NOTE: Increase the survival rate of pups by manipulating less than 2/3rd&#160;of the total number of embryos per dam. Avoid embryos too close to the cervix. If manipulated, they might cause complications during labor and jeopardize the entire litter. If electrodes are too close to the embryo&#39;s heart, this may cause cardiac arrest.</li>
	</ol>
	</li>
</ol>

<table><tbody><tr><td>Autoclave band&amp;nbsp;</td><td>Kisker Biotech</td><td>150262</td><td></td></tr><tr><td>Electro Square Porator</td><td>BTX</td><td>ECM830</td><td></td></tr><tr><td>Endofree Maxi Kit&amp;nbsp;&amp;nbsp;</td><td>Qiagen</td><td>12362</td><td></td></tr><tr><td>Ethanol&amp;nbsp;&amp;nbsp;</td><td>Merck</td><td>107017</td><td></td></tr><tr><td>Eye ointment (Bepanthen)&amp;nbsp;</td><td>Bayer&amp;nbsp;</td><td>81552983</td><td></td></tr><tr><td>Fast Green&amp;nbsp;</td><td>Merck</td><td>104022</td><td></td></tr><tr><td>Filter (0.22 &amp;micro;m)&amp;nbsp;</td><td>Merck</td><td>&amp;nbsp;F8148</td><td></td></tr><tr><td>Forceps straight&amp;nbsp;&amp;nbsp;</td><td>Fine Science Tools</td><td>91150-20</td><td></td></tr><tr><td>Gauze (X100 ES-pads 8f 10 x 10 cm)&amp;nbsp;&amp;nbsp;</td><td>Fisher Scientific</td><td>15387311</td><td></td></tr><tr><td>Glass Capillary with Filament&amp;nbsp;</td><td>Narishige&amp;nbsp;</td><td>GD1-2</td><td></td></tr><tr><td>Heating Pad&amp;nbsp;</td><td>ThermoLux&amp;nbsp;</td><td>463265 / -67</td><td></td></tr><tr><td>Isoflurane&amp;nbsp;</td><td>Zoetis&amp;nbsp;</td><td>TU061219</td><td></td></tr><tr><td>Ring Forceps&amp;nbsp;</td><td>Fine Science Tools</td><td>11103-09</td><td></td></tr><tr><td>Stereomicroscope&amp;nbsp;</td><td>Nikon</td><td>C-PS</td><td></td></tr><tr><td>Surgical scissors&amp;nbsp;&amp;nbsp;</td><td>Fine Science Tools</td><td>91460-11</td><td></td></tr><tr><td>Surgical scissors with blunt tip&amp;nbsp;&amp;nbsp;</td><td>Fine Science Tools</td><td>14072-10</td><td></td></tr><tr><td>Tweezers w/5mm- disk electrodes Platinum&amp;nbsp;</td><td>Xceltis&amp;nbsp; GmbH</td><td>CUY650P5</td><td></td></tr><tr><td>Metamizol&amp;nbsp;</td><td>WDT</td><td></td><td></td></tr><tr><td>Non-sterile Silk Suture Thread (0.12 mm)&amp;nbsp;&amp;nbsp;</td><td>Fine Science Tools</td><td>18020-50</td><td></td></tr><tr><td>PBS (1x)&amp;nbsp;</td><td>Life Technologies</td><td>14190169</td><td></td></tr><tr><td>Tissue scissors Blunt (11.5 cm)</td><td>Fine Science Tools</td><td>14072-10</td><td></td></tr><tr><td>pCAG-EGxxFP&amp;nbsp;</td><td>Addgene</td><td>50716</td><td></td></tr><tr><td>pX330 plasmid&amp;nbsp;</td><td>Addgene&amp;nbsp;</td><td>42230</td><td></td></tr></tbody></table>

in utero electroporation based gene delivery: a technique to inject plasmid dna into embryonic cerebellar cells of murine embryos

Source: Feng W. et al. <a href="https://www.jove.com/video/57311" target="_blank">CRISPR-mediated Loss of Function Analysis in Cerebellar Granule Cells Using In Utero Electroporation-based Gene Transfer.</a> J. Vis. Exp. (2018)
This video demonstrates the delivery of plasmid DNA into cerebellar neuronal cells of murine embryos using in utero electroporation. This method is useful to gain understanding of in vivo function of genes in normal brain development and the changes in gene expression of neuron cells during tumor progression.

In Utero Electroporation Based Gene Delivery: A Technique to Inject Plasmid DNA into Embryonic Cerebellar Cells of Murine Embryos

Source: Feng W. et al. CRISPR-mediated Loss of Function Analysis in Cerebellar Granule Cells Using In Utero Electroporation-based Gene Transfer. J. Vis. ...

Begin by taking a pregnant anesthetized female mouse model placed in a supine position. Prep the mouse by removing hair from the abdominal region. Incise the skin and underlying muscle layers to expose the uterine horns - the sites that host viable embryos.
Now, pull the uterine horns out of the abdominal cavity. Take a sharp tip glass capillary containing the desired plasmid DNA solution. Locate the brain of the embryo and inject the plasmid DNA solution through the uterus wall into the fourth ventricle. This position is anterior to the cerebellar primordium - the desired location for eventual DNA delivery.
After injection, retract the empty capillary. Next, for electroporation of the DNA injected embryo, position the two electrodes over the uterine wall such that the positive electrode covers the cerebellar primordium and the negative electrode covers the region around the ears.
Apply electric pulses for the desired duration. These pulses make the cerebellar neuronal cells permeable, allowing the plasmid DNA to enter the targeted cells. Finally, place the uterine horns back inside the abdominal cavity at their natural position. Suture the cuts, transfer the mouse to its cage, and allow it to recover.

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1.2K Aufrufe. Quelle: Feng W. et al. CRISPR-vermittelte Analyse des Funktionsverlusts in Kleinhirn-Körnerzellen mittels In-utero-Elektroporations-basiertem Gentransfer. J. Vis. Exp. (2018) Dieses Video zeigt die Abgabe von Plasmid-DNA in zerebelläre neuronale Zellen von Mausembryonen mittels in utero-Elektroporation. Diese Methode ist nützlich, um die in vivo Funktion von Genen bei der normalen Gehirnentwicklung und die Veränderungen in der Genexpression von Neuronenzellen während der Tumorprogression z...

Serie: In utero Elektroporation basierte Genabgabe: Eine Technik zur Injektion von Plasmid-DNA in embryonale Kleinhirnzellen von Mausembryonen - Konzept

In utero Electroporation followed by Primary Neuronal Culture for Studying Gene Function in Subset of Cortical Neurons

In vitro study of primary neuronal cultures allows for quantitative analyses of neurite outgrowth. In order to study how genetic alterations affect neuronal process outgrowth, shRNA or cDNA constructs can be introduced into primary neurons via chemical transfection or viral transduction. However, with primary cortical cells, a heterogeneous pool of cell types (glutamatergic neurons from different layers, inhibitory neurons, glial cells) are transfected using these methods. The use of in utero electroporation to introduce DNA constructs in the embryonic rodent cortex allows for certain subsets of cells to be targeted: while electroporation of early embryonic cortex targets deep layers of the cortex, electroporation at late embryonic timepoints targets more superficial layers. Further, differential placement of electrodes across the heads of individual embryos results in the targeting of dorsal-medial versus ventral-lateral regions of the cortex. Following electroporation, transfected cells can be dissected out, dissociated, and plated in vitro for quantitative analysis of neurite outgrowth. Here, we provide a step-by-step method to quantitatively measure neuronal process outgrowth in subsets of cortical cells.
The basic protocol for in utero electroporation has been described in detail in two other JoVE articles from the Kriegstein lab 1, 2. We will provide an overview of our protocol for in utero electroporation, focusing on the most important details, followed by a description of our protocol that applies in utero electroporation to the study of gene function in neuronal process outgrowth.

In utero Electroporation followed by Primary Neuronal Culture for Studying Gene Function in Subset of Cortical Neurons

In utero electroporation is a valuable method for transfecting neuronal progenitor cells in vivo. Depending upon the placement of the electrodes and the developmental timepoint of electroporation, certain subsets of cortical cells can be targeted. Targeted cells can then be analyzed in vivo or in vitro for effects of genetic alteration.

In utero Elektroporation gefolgt von primären neuronalen Kultur für ein Studium Gene Function in Subset von kortikalen Neuronen

In vitro study of primary neuronal cultures allows for quantitative analyses of neurite outgrowth. In order to study how genetic alterations affect ...

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Cortex-, Hippocampus-, Thalamus-, Hypothalamus-, Lateral Septal Nucleus- and Striatum-specific In Utero Electroporation in the C57BL/6 Mouse

In utero electroporation is a widely used technique for fast and efficient spatiotemporal manipulation of various genes in the rodent central nervous system. Overexpression of desired genes is just as possible as shRNA mediated loss-of-function studies. Therefore it offers a wide range of applications. The feasibility to target particular cells in a distinct area further increases the range of potential applications of this very useful method. For efficiently targeting specific regions knowledge about the subtleties, such as the embryonic stage, the voltage to apply and most importantly the position of the electrodes, is indispensable.
Here, we provide a detailed protocol that allows for specific and efficient in utero electroporation of several regions of the C57BL/6 mouse central nervous system. In particular it is shown how to transfect regions the develop into the retrosplenial cortex, the motor cortex, the somatosensory cortex, the piriform cortex, the cornu ammonis 1-3, the dentate gyrus, the striatum, the lateral septal nucleus, the thalamus and the hypothalamus. For this information about the appropriate embryonic stage, the appropriate voltage for the corresponding embryonic stage is provided. Most importantly an angle-map, which indicates the appropriate position of the positive pole, is depicted. This standardized protocol helps to facilitate efficient in utero electroporation, which might also lead to a reduced number of animals.

Cortex-, Hippocampus-, Thalamus-, Hypothalamus-, Lateral Septal Nucleus- and Striatum-specific In Utero Electroporation in the C57BL/6 Mouse

This protocol describes in detail how to specifically transfect different regions in the C57BL/6 central nervous system via in utero electroporation. Included in this protocol are detailed instructions for transfections of regions that develop into the cortex, hippocampus, thalamus, hypothalamus, lateral septal nucleus and striatum.

Cortex, Hippocampus-, Thalamus-, Hypothalamus, Lateral Septal Nucleus- und Striatum spezifische<em&gt; In Utero</em&gt; Electroporation in der C57BL / 6-Maus,

In utero electroporation is a widely used technique for fast and efficient spatiotemporal manipulation of various genes in the rodent central nervous ...

In Vivo Targeting of Neural Progenitor Cells in Ferret Neocortex by In Utero Electroporation

Manipulation of gene expression in vivo during embryonic development is the method of choice when analyzing the role of individual genes during mammalian development. In utero electroporation is a key technique for the manipulation of gene expression in the embryonic mammalian brain in vivo. A protocol for in utero electroporation of the embryonic neocortex of ferrets, a small carnivore, is presented here. The ferret is increasingly being used as a model for neocortex development, because its neocortex exhibits a series of anatomical, histological, cellular, and molecular features that are also present in human and nonhuman primates, but absent in rodent models, such as mouse or rat. In utero electroporation was performed at embryonic day (E) 33, a midneurogenesis stage in ferret. In utero electroporation targets neural progenitor cells lining the lateral ventricles of the brain. During neurogenesis, these progenitor cells give rise to all other neural cell types. This work shows representative results and analyses at E37, postnatal day (P) 1, and P16, corresponding to 4, 9, and 24 days after in utero electroporation, respectively. At earlier stages, the progeny of targeted cells consists mainly of various neural progenitor subtypes, whereas at later stages most labeled cells are postmitotic neurons. Thus, in utero electroporation enables the study of the effect of genetic manipulation on the cellular and molecular features of various types of neural cells. Through its effect on various cell populations, in utero electroporation can also be used for the manipulation of histological and anatomical features of the ferret neocortex. Importantly, all these effects are acute and are performed with a spatiotemporal specificity determined by the user.

Presented here is a protocol to perform genetic manipulation in the embryonic ferret brain using in utero electroporation. This method allows for targeting of neural progenitor cells in the neocortex in vivo.

In Vivo Targeting von neuronalen Vorläuferzellen in Ferret Neocortex durch Utero Elektroporation

Manipulation of gene expression in vivo during embryonic development is the method of choice when analyzing the role of individual genes during mammalian ...

In Utero Electroporation Based Gene Delivery: A Technique to Inject Plasmid DNA into Embryonic Cerebellar Cells of Murine Embryos

Transkript

In Utero Electroporation Based Gene Delivery: A Technique to Inject Plasmid DNA into Embryonic Cerebellar Cells of Murine Embryos