&lt;em&gt;In vitro&lt;/em&gt; Electroporation of the Lower Rhombic Lip of Midgestation Mouse Embryos

Holland, Patrick; George, Angela M.; Worrell, Leslie T.C.; Landsberg, Rebecca L.

doi:10.3791/3983

Cited by 2 publications

(2 citation statements)

References 18 publications

(20 reference statements)

Supporting

Mentioning

Contrasting

Order By: Relevance

“…In particular, the ex vivo culture model may be applied to hindbrains of genetically engineered mice defective in specific molecules implicated in neuronal migration, such as growth or guidance factor receptors, and combined with bead implants to test if responsiveness to ligands is lost. In addition to pharmacological manipulation, the ex vivo culture protocol could also be adapted to electroporate expression vectors that could manipulate expression of genes of interest; appropriate methods for electroporation have previously been described 22,23 . This protocol may also be adapted to visualize neuron migration by time-lapse microscopy in hindbrain explants from transgenic mice containing fluorescently labeled FBM neurons, e.g.…”

Section: Discussionmentioning

confidence: 99%

Mouse Hindbrain <em>Ex Vivo</em> Culture to Study Facial Branchiomotor Neuron Migration

Tillo

Schwarz

Ruhrberg

2014

JoVE

View full text Add to dashboard Cite

Citation: Tillo, M., Schwarz, Q., Ruhrberg, C. Mouse Hindbrain Ex Vivo Culture to Study Facial Branchiomotor Neuron Migration. J. Vis. Exp. (85), e51397, doi:10.3791/51397 (2014). AbstractEmbryonic neurons are born in the ventricular zone of the brain, but subsequently migrate to new destinations to reach appropriate targets. Deciphering the molecular signals that cooperatively guide neuronal migration in the embryonic brain is therefore important to understand how the complex neural networks form which later support postnatal life. Facial branchiomotor (FBM) neurons in the mouse embryo hindbrain migrate from rhombomere (r) 4 caudally to form the paired facial nuclei in the r6-derived region of the hindbrain. Here we provide a detailed protocol for wholemount ex vivo culture of mouse embryo hindbrains suitable to investigate the signaling pathways that regulate FBM migration. In this method, hindbrains of E11.5 mouse embryos are dissected and cultured in an open book preparation on cell culture inserts for 24 hr. During this time, FBM neurons migrate caudally towards r6 and can be exposed to function-blocking antibodies and small molecules in the culture media or heparin beads loaded with recombinant proteins to examine roles for signaling pathways implicated in guiding neuronal migration.

show abstract

Section: Discussionmentioning

confidence: 99%

Mouse Hindbrain <em>Ex Vivo</em> Culture to Study Facial Branchiomotor Neuron Migration

Tillo

Schwarz

Ruhrberg

2014

JoVE

View full text Add to dashboard Cite

show abstract

“…In this protocol, the area chose to study is the developing mouse cortex. In addition, in utero electroporation is also applied in the gene delivery in mouse auditory brainstem and hindbrain, such as rhombic lip ( David et al., 2014 ; Holland et al., 2012 ). Using a triple-electrode probe, the special high-performance and site-directed in utero electroporation are achievable ( dal Maschio et al., 2012 ).…”

Section: Limitationsmentioning

confidence: 99%

Protocol for analysis of senescent neuronal stem cells in genetic-modified embryonic mice using in utero electroporation technique

Chen¹,

Liu²,

Wu³

et al. 2022

STAR Protocols

View full text Add to dashboard Cite

<em>In vitro</em> Electroporation of the Lower Rhombic Lip of Midgestation Mouse Embryos

Cited by 2 publications

References 18 publications

Mouse Hindbrain <em>Ex Vivo</em> Culture to Study Facial Branchiomotor Neuron Migration

Mouse Hindbrain <em>Ex Vivo</em> Culture to Study Facial Branchiomotor Neuron Migration

Protocol for analysis of senescent neuronal stem cells in genetic-modified embryonic mice using in utero electroporation technique

Contact Info

Product

Resources

About