Name: CreER-LoxP System-Based Target Gene Inactivation: A Tamoxifen-Inducible Cre Recombinase System for Target Gene Knockout in a Mouse Model
Uploaded: 2023-04-30T14:56:20
Description: Source: Hubner, E. K., et al. Constitutive and Inducible Systems for Genetic&#160;In Vivo&#160;Modification of Mouse Hepatocytes Using Hydrodynamic Tail ...

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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. Induction of Transfected CreER with Tamoxifen
CAUTION: Tamoxifen is harmful, may be cancerous or damage fertility. Please refer to the safety data sheet.
<ol>
	<li>Plan intraperitoneal tamoxifen injections on three consecutive days.</li>
	<li>On day 1, dissolve 10 mg of tamoxifen in 40 &#181;L ethanol. Incubate at 55 &#176;C for 10 min. Vortex several times until the tamoxifen has dissolved.</li>
	<li>Add 960 &#181;L corn oil. Incubate for 5 mins at 55 &#176;C. Vortex several times to get a clear solution.</li>
	<li>Prepare the solution in a 1-mL insulin syringe with a 27 G needle.</li>
	<li>Scruff the mouse by grabbing the neck of the mouse carefully with the thumb and the second finger, fixing the tail between the base of the hand and the fourth and fifth finger.</li>
	<li>Inject 0.1 mL (= 1 mg of tamoxifen) of the solution intraperitoneally into the left lower quadrant of the abdomen.</li>
	<li>Repeat the injections on days two and three.</li>
</ol>

creer-loxp system-based target gene inactivation: a tamoxifen-inducible cre recombinase system for target gene knockout in a mouse model

Source: Hubner, E. K., et al. <a href="https://www.jove.com/v/56613">Constitutive and Inducible Systems for Genetic&#160;In Vivo&#160;Modification of Mouse Hepatocytes Using Hydrodynamic Tail Vein Injection.</a>&#160;J. Vis. Exp. (2018)
This video describes a procedure for target gene knockout using a tamoxifen-inducible Cre-recombinase system following intraperitoneal injection of tamoxifen in a mouse model.

CreER-LoxP System-Based Target Gene Inactivation: A Tamoxifen-Inducible Cre Recombinase System for Target Gene Knockout in a Mouse Model

Source: Hubner, E. K., et al. Constitutive and Inducible Systems for Genetic&#160;In Vivo&#160;Modification of Mouse Hepatocytes Using Hydrodynamic Tail ...

Begin with a genetically engineered mouse model comprising a modified genome that harbors LoxP sites - specific sequences recognized by Cre-recombinase enzymes - flanking the gene of interest. The mouse is further transfected with a plasmid vector encoding organ-specific CreER recombinase, leading to the integration of CreER recombinase-expressing element into the genome of liver cells.
The expressed CreER recombinase, an inactive fusion protein involving Cre recombinase and the mutant ligand-binding domain of the estrogen receptor, ER, interacts and binds to heat-shock protein in the cytoplasm. This binding confines CreER recombinase in the cytoplasm.
Prepare a solution of tamoxifen, a hydrophobic drug, using ethanol and suitable oil. Now, inject the tamoxifen solution intraperitoneally into the left lower quadrant of the mouse&#39;s abdomen to prevent damage to the abdominal organs.
The injected tamoxifen is metabolized in the liver to 4-hydroxytamoxifen, 4-OHT. Further, 4-OHT, a selective estrogen receptor modulator, binds to the ER-ligand binding domain of CreER recombinase, causing its conformational change. This leads to the release of the CreER recombinase from the heat-shock protein.
The activated CreER recombinases translocate into the nucleus and recognize the LoxP sites in the host genome. The CreER recombinases catalyze site-specific recombination between the LoxP sites, resulting in the excision of the gene of interest, thereby achieving tissue-specific gene knockout.

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1.9K Views. Source: Hubner, E. K., et al. Constitutive and Inducible Systems for Genetic In Vivo Modification of Mouse Hepatocytes Using Hydrodynamic Tail Vein Injection. J. Vis. Exp. (2018) This video describes a procedure for target gene knockout using a tamoxifen-inducible Cre-recombinase system following intraperitoneal injection of tamoxifen in a mouse model. 

Video: CreER-LoxP System-Based Target Gene Inactivation: A Tamoxifen-Inducible Cre Recombinase System for Target Gene Knockout in a Mouse Model - Concept

Protocols for Analyzing the Role of Paneth Cells in Regenerating the Murine Intestine using Conditional Cre-lox Mouse Models

The epithelial surface of the mammalian intestine is a dynamic tissue that renews every 3 - 7 days. Understanding this renewal process identified a population of rapidly cycling intestinal stem cells (ISCs) characterized by their expression of the Lgr5 gene. These are supported by a quiescent stem cell population, marked by Bmi-1 expression, capable of replacing them in the event of injury. Investigating the interactions between these populations is crucial to understanding their roles in disease and cancer. The ISCs exist within crypts on the intestinal surface, these niches support the ISC in replenishing the epithelia. The interaction between active and quiescent ISCs likely involves other differentiated cells within the niche, as it has previously been demonstrated that the &#8216;&#8216;stemness&#8217;&#8217; of the Lgr5 ISC is closely tied to the presence of their neighboring Paneth cells. Using conditional cre-lox mouse models we tested the effect of deleting the majority of active ISCs in the presence or absence of the Paneth cells. Here we describe the techniques and analysis undertaken to characterize the intestine and demonstrate that the Paneth cells play a crucial role within the ISC niche in aiding recovery following substantial insult.

Protocols for Analyzing the Role of Paneth Cells in Regenerating the Murine Intestine using Conditional Cre-lox Mouse Models

Intestinal epithelial stem cells (ISCs) are intermingled with Paneth cells. These cells are differentiated progeny of the ISC, which support the ISCs and provide antibacterial protection. Here we demonstrate how we used transgenic conditional mouse models to establish that Paneth cells play a crucial role in maintaining the intestinal epithelia.

The epithelial surface of the mammalian intestine is a dynamic tissue that renews every 3 - 7 days. Understanding this renewal process identified a ...

JoVE Journal

Developmental Biology

A High-throughput Cre-Lox Activated Viral Membrane Fusion Assay to Identify Inhibitors of HIV-1 Viral Membrane Fusion

This assay is designed to specifically report on HIV-1 fusion via the expression of green fluorescent protein (GFP) detectable by flow cytometry or fluorescence microscopy. An HIV-1 reporter virus (HIV-1 Gag-iCre) is generated by inserting Cre recombinase into the HIV-1 genome between the matrix and the capsid proteins of the Gag polyprotein. This results in a packaging of Cre recombinase into virus particles, which is then released into a target cell line stably expressing a Cre recombinase-activated red fluorescent protein (RFP) to GFP switch cassette. In the basal state, this cassette expresses RFP only. Following the delivery of Cre recombinase into the target cell, the RFP, flanked by loxP sites, excises, resulting in GFP expression. This assay can be used to test any inhibitors of viral entry (specifically at the fusion step) in cell-free and cell-to-cell infection systems and has been used to identify a class of purinergic receptor antagonists as novel inhibitors of HIV-1 viral membrane fusion.

We describe a cell-based assay to report on HIV-1 fusion via the expression of green fluorescent protein detectable by flow cytometry or fluorescence microscopy. It can be used to test inhibitors of viral entry (specifically at the fusion step) in cell-free and cell-to-cell infection systems.

This assay is designed to specifically report on HIV-1 fusion via the expression of green fluorescent protein (GFP) detectable by flow cytometry or ...

Immunology and Infection

Inducing Cre-lox Recombination in Mouse Cerebral Cortex Through In Utero Electroporation

Cell-autonomous neuronal functions of genes can be revealed by causing loss or gain of function of a gene in a small and sparse population of neurons. To do so requires generating a mosaic in which neurons with loss or gain of function of a gene are surrounded by genetically unperturbed tissue. Here, we combine the Cre-lox recombination system with in utero electroporation in order to generate mosaic brain tissue that can be used to study the cell-autonomous function of genes in neurons. DNA constructs (available through repositories), coding for a fluorescent label and Cre recombinase, are introduced into developing cortical neurons containing genes flanked with loxP sites in the brains of mouse embryos using in utero electroporation. Additionally, we describe various adaptations to the in utero electroporation method that increase survivability and reproducibility. This method also involves establishing a titer for Cre-mediated recombination in a sparse or dense population of neurons. Histological preparations of labeled brain tissue do not require (but can be adapted to) immunohistochemistry. The constructs used guarantee that fluorescently labeled neurons carry the gene for Cre recombinase. Histological preparations allow morphological analysis of neurons through confocal imaging of dendritic and axonal arbors and dendritic spines. Because loss or gain of function is achieved in sparse mosaic tissue, this method permits the study of cell-autonomous necessity and sufficiency of gene products in vivo.

Inducing Cre-lox Recombination in Mouse Cerebral Cortex Through In Utero Electroporation

Cell-autonomous functions of genes in the brain can be studied by inducing loss or gain of function in sparse populations of cells. Here, we describe in utero electroporation to deliver Cre recombinase into sparse populations of developing cortical neurons with floxed genes to cause loss of function in vivo.

Cell-autonomous neuronal functions of genes can be revealed by causing loss or gain of function of a gene in a small and sparse population of neurons. To ...

CreER-LoxP System-Based Target Gene Inactivation: A Tamoxifen-Inducible Cre Recombinase System for Target Gene Knockout in a Mouse Model

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