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1. Perforation of Mouse Fertilized Eggs with XYClone Laser
<ol>
	<li>Setup and calibrate XYClone laser according to the manufacturer&#39;s recommendation. Other lasers, typically used for&#160;in vitro&#160;fertilization, can be substituted for XYClone laser to perforate fertilized eggs.
	<ol>
		<li>Attach the laser controller box wire to the laser apparatus on the microscope.</li>
		<li>Attach the laser controller box to the computer running the laser software via a USB port. 3.1.3. Plug in the laser controller and switch it on.</li>
		<li>Looking through the eyepiece, perforate a test sample (e.g. dry-erase markings on a glass slide).</li>
		<li>Use a small screw driver (included in the laser kit) to adjust the X and Y position of the laser to match the LED light visible through the microscope eyepiece and calibrate the laser.</li>
	</ol>
	</li>
	<li>Place a KSOM drop plate containing mouse fertilized eggs on the microscope stage. Do not keep the plate outside of the incubator for longer than 15 min.</li>
	<li>Look through the microscope eyepiece and ensure that the embryo&#39;s zona pellucida is in focus and the laser LED light is visible.</li>
	<li>Move the microscope stage to target the zona with the LED light/laser.</li>
	<li>Using the computer software set XYClone laser to 250 &#956;s.</li>
	<li>Adjust the LED light size to desired dimensions (setting 5 in this experiment).</li>
	<li>Perforate the zona of each fertilized egg thrice with the laser. The zona can be either pierced or thinned. Using the above settings, the laser will produce a hole with a diameter of 10 &#956;m (Figure 1).&#160;&#160; 
	NOTE: Aiming close to the polar body keeps laser away from the embryonic cell.</li>
	<li>Allow fertilized eggs to recover for 2 h in the tissue culture incubator before moving to the next step.</li>
</ol>
2. Transduction of Mouse Fertilized Eggs Following XYClone Laser Perforation
<ol>
	<li>Pipet 2 &#956;L of concentrated lentivirus (greater than 1e8 TU/mL titer) into the 50 &#956;L KSOM drop. Do not pipet up and down. Fertilized eggs readily attach to the pipet tip. Based on our experience, 1e5-5e5 transducing units of lentivirus in a volume less than 3 &#956;L is optimal for gene delivery.</li>
	<li>Allow fertilized eggs to develop into blastocyst for 4 days in the incubator. No need to change the media.</li>
</ol>
3. Non-surgical Transfer of Transduced Mouse Embryos to Pseudo-pregnant Mice
<ol>
	<li>Use pseudopregnant mice, 3.5 day after mating.</li>
	<li>Use Non-Surgical Embryo Transfer (NSET) device to implant mouse embryos into pseudopregnant mice.
	<ol>
		<li>Using a surgical or dissecting microscope, insert a vaginal speculum to visualize the cervix.</li>
		<li>Insert the Non-Surgical Embryo Transfer (NSET) device approximately 5 mm into the cervix and deposit embryos in a volume of approximately 2 &#956;L. 
		NOTE: A sterile NSET device is used for each transfer and discarded after the procedure. All reagents used in the manipulation of the embryos must be sterile.</li>
	</ol>
	</li>
	<li>Transfer 10&#8211;15 healthy blastocyst in 2 &#956;L volume of KSOM to each pseudopregnant mice.</li>
	<li>Continue to monitor and measure the weight gain in pseudopregnant mice in following days to determine whether the NSET was successful.</li>
	<li>Recover pups by allowing the pregnant mice to give birth naturally or performing a caesarean section 17 days after the embryo transfer. A C-section is often necessary if very few embryos are present and they grow too large for natural birth.</li>
	<li>Collect tissue from pups for genotyping to determine the rate of transgenesis.</li>
</ol>

<table><tbody><tr><td>CD510B-1 plasmid</td><td>System Biosciences</td><td>CD510B-1</td><td>used to package the lentivirus expressing EF1a-copGFP</td></tr><tr><td>Dimethylpolysiloxane</td><td>Sigma</td><td>DMPS5X</td><td>culturing embryos</td></tr><tr><td>XYClone Laser</td><td>Hamilton Thorne Biosciences</td><td></td><td>perforating mouse fertilized eggs</td></tr><tr><td>Non-Surgical Embryo Transfer (NSET) Device</td><td>ParaTechs</td><td>60010</td><td>NSET of embryos</td></tr><tr><td>&lt;strong&gt;KSOM medium&lt;/strong&gt;</td><td>Millipore</td><td>MR-020P-5F</td><td>culturing embryos</td></tr><tr><td>&lt;strong&gt;Composition of KSOM:&lt;/strong&gt;</td><td></td><td></td><td>mg/100mL</td></tr><tr><td>NaCl</td><td></td><td></td><td>555</td></tr><tr><td>KCl</td><td></td><td></td><td>18.5</td></tr><tr><td>KH2PO4</td><td></td><td></td><td>4.75</td></tr><tr><td>MgSO4&amp;nbsp;7H2O</td><td></td><td></td><td>4.95</td></tr><tr><td>CaCl2&amp;nbsp;2H2O</td><td></td><td></td><td>25</td></tr><tr><td>NaHCO3</td><td></td><td></td><td>210</td></tr><tr><td>Glucose</td><td></td><td></td><td>3.6</td></tr><tr><td>Na-Pyruvate</td><td></td><td></td><td>2.2</td></tr><tr><td>DL-Lactic Acid, sodium salt</td><td></td><td></td><td>0.174mL</td></tr><tr><td>10 mM EDTA</td><td></td><td></td><td>100&amp;micro;L</td></tr><tr><td>Streptomycin</td><td></td><td></td><td>5</td></tr><tr><td>Penicillin</td><td></td><td></td><td>6.3</td></tr><tr><td>0.5% phenol red</td><td></td><td></td><td>0.1mL</td></tr><tr><td>L-Glutamine</td><td></td><td></td><td>14.6</td></tr><tr><td>MEM Essential Amino Acids</td><td></td><td></td><td>1mL</td></tr><tr><td>MEM Non-essential AA</td><td></td><td></td><td>0.5mL</td></tr><tr><td>BSA</td><td></td><td></td><td>100</td></tr></tbody></table>

laser-assisted lentiviral gene delivery: a technique to permeabilize mouse fertilized eggs to facilitate lentiviral gene delivery

Source: Martin, N. P., et al. <a href="https://www-jove-com.remotexs.ntu.edu.sg/v/58327">Laser-assisted Lentiviral Gene Delivery to Mouse Fertilized Eggs.</a> J. Vis. Exp. (2018).
In this video, we demonstrate the laser-assisted permeation of the protective layer of zona pellucida in mouse fertilized eggs for facilitating lentiviral gene delivery. Lentivirus enables the generation of transgenic animals with a gene of interest stably integrated into their genome.

<img alt="Figure 1" src="/files/ftp_upload/20995/20995_Figure1.jpg" /> 
Figure 1: Laser-Treatment of Mouse Fertilized Eggs. Examples of perforating the zona to produce a hole vs thinning of the zona.

Laser-Assisted Lentiviral Gene Delivery: A Technique to Permeabilize Mouse Fertilized Eggs to Facilitate Lentiviral Gene Delivery

Source: Martin, N. P., et al. Laser-assisted Lentiviral Gene Delivery to Mouse Fertilized Eggs. J. Vis. Exp. (2018).
In this video, we demonstrate the ...

Laser-assisted lentiviral gene delivery is a technique to transfer a transgene into a host system.
To produce transgenic mice, begin with isolated mouse fertilized eggs in a suitable culture medium. Place the fertilized egg-containing culture dish on a microscope stage pre-installed with a laser apparatus and attached to a controlling software. Observe at suitable magnification.
Fertilized eggs are surrounded by zona pellucida, a protective glycoprotein layer that barriers lentiviral particles. To permeate this barrier, turn on the laser apparatus and ensure the laser LED is visible over the zona pellucida. Using the controlling software, fire the laser. Adjust the firing duration according to the desired perforation diameter.
Place the eggs in an incubator for recovery. After brief incubation, remove the eggs and add lentivirus particles carrying the gene of interest and a fluorescent selectable marker.
With zona pellucida perforated, the lentivirus easily diffuses toward the egg cell membrane and enters via endocytosis. The lentivirus disassembles, releasing its RNA, which, when sequentially processed into a double-stranded DNA, enters the host nucleus, integrating the foreign genes into the host genome.
Incubate the eggs and allow them to develop into blastocysts. Implant the blastocysts into mated female mice. Once gestation is complete, recover the pups and analyze them for transgene presence.

laser-assisted-lentiviral-gene-delivery-technique-to-permeabilize

Nanyang Technological University

Research

JoVE Encyclopedia of Experiments

Biological Techniques

Gene Transfer Techniques

Transduction

957 ビュー. 出典:Martin, N. P., et al.マウス受精卵へのレーザー支援レンチウイルス遺伝子送達。J. Vis. Exp.(2018年)。 このビデオでは、レンチウイルス遺伝子の送達を促進するためのマウス受精卵の透明帯の保護層のレーザー支援透過を示しています。レンチウイルスは、目的の遺伝子がゲノムに安定して組み込まれたトランスジェニック動物の作製を可能にします。 

ビデオ: レーザー支援レンチウイルス遺伝子導入:レンチウイルス遺伝子導入を促進するためにマウス受精卵を透過化する技術 - 概念

Lentiviral Mediated Production of Transgenic Mice: A Simple and Highly Efficient Method for Direct Study of Founders

For almost 40 years, pronuclear DNA injection represents the standard method to generate transgenic mice with random integration of transgenes. Such a routine procedure is widely utilized throughout the world and its main limitation resides in the poor efficacy of transgene integration, resulting in a low yield of founder animals. Only few percent of animals born after implantation of injected fertilized oocytes have integrated the transgene. In contrast, lentiviral vectors are powerful tools for integrative gene transfer and their use to transduce fertilized oocytes allows highly efficient production of founder transgenic mice with an average yield above 70%. Furthermore, any mouse strain can be used to produce transgenic animal and the penetrance of transgene expression is extremely high, above 80% with lentiviral mediated transgenesis compared to DNA microinjection. The size of the DNA fragment that can be cargo by the lentiviral vector is restricted to 10 kb and represents the major limitation of this method. Using a simple and easy to perform injection procedure beneath the zona pellucida of fertilized oocytes, more than 50 founder animals can be produced in a single session of microinjection. Such a method is highly adapted to perform, directly in founder animals, rapid gain and loss of function studies or to screen genomic DNA regions for their ability to control and regulate gene expression in vivo.

Here, we present a protocol to promote transgene integration and production of founder transgenic mice with high efficacy by a simple injection of a lentiviral vector in the perivitelline space of a fertilized oocyte.

レンチ ウイルス媒介トランスジェニック マウスの生産: シンプルで高効率な創設者の直接の研究法

For almost 40 years, pronuclear DNA injection represents the standard method to generate transgenic mice with random integration of transgenes. Such a ...

JoVE Journal

遺伝学

Lentiviral CRISPR/Cas9-Mediated Genome Editing for the Study of Hematopoietic Cells in Disease Models

Manipulating genes in hematopoietic stem cells using conventional transgenesis approaches can be time-consuming, expensive, and challenging. Benefiting from advances in genome editing technology and lentivirus-mediated transgene delivery systems, an efficient and economical method is described here that establishes mice in which genes are manipulated specifically in hematopoietic stem cells. Lentiviruses are used to transduce Cas9-expressing lineage-negative bone marrow cells with a guide RNA (gRNA) targeting specific genes and a red fluorescence reporter gene (RFP), then these cells are transplanted into lethally-irradiated C57BL/6 mice. Mice transplanted with lentivirus expressing non-targeting gRNA are used as controls. Engraftment of transduced hematopoietic stem cells are evaluated by flow cytometric analysis of RFP-positive leukocytes of peripheral blood. Using this method, ~90% transduction of myeloid cells and ~70% of lymphoid cells at 4 weeks after transplantation can be achieved. Genomic DNA is isolated from RFP-positive blood cells, and portions of the targeted site DNA are amplified by PCR to validate the genome editing. This protocol provides a high-throughput evaluation of hematopoiesis-regulatory genes and can be extended to a variety of mouse disease models with hematopoietic cell involvement.

Described are protocols for the highly efficient genome editing of murine hematopoietic stem and progenitor cells (HSPC) by the CRISPR/Cas9 system to rapidly develop mouse model systems with hematopoietic system-specific gene modifications.

疾患モデルにおける血化細胞の研究のためのレンチウイルスCRISPR/Cas9媒介ゲノム編集

Manipulating genes in hematopoietic stem cells using conventional transgenesis approaches can be time-consuming, expensive, and challenging. Benefiting ...

免疫・感染学

High Throughput Microinjections of Sea Urchin Zygotes

Microinjection into cells and embryos is a common technique that is used to study a wide range of biological processes. In this method a small amount of treatment solution is loaded into a microinjection needle that is used to physically inject individual immobilized cells or embryos. Despite the need for initial training to perform this procedure for high-throughput delivery, microinjection offers maximum efficiency and reproducible delivery of a wide variety of treatment solutions (including complex mixtures of samples) into cells, eggs or embryos. Applications to microinjections include delivery of DNA constructs, mRNAs, recombinant proteins, gain of function, and loss of function reagents. Fluorescent or colorimetric dye is added to the injected solution to enable instant visualization of efficient delivery as well as a tool for reliable normalization of the amount of the delivered solution. The described method enables microinjection of 100-400 sea urchin zygotes within 10-15 min.

Microinjection is a common technique used to deliver DNA constructs, mRNAs, morpholino antisense oligonucleotides or other treatments into eggs, embryos, and cells of various species.

ウニ​​接合体のハイスループットマイクロインジェクション

Microinjection into cells and embryos is a common technique that is used to study a wide range of biological processes. In this method a small amount of ...

Laser-Assisted Lentiviral Gene Delivery: A Technique to Permeabilize Mouse Fertilized Eggs to Facilitate Lentiviral Gene Delivery

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Laser-Assisted Lentiviral Gene Delivery: A Technique to Permeabilize Mouse Fertilized Eggs to Facilitate Lentiviral Gene Delivery