Dissection of Xenopus laevis Neural Crest for in vitro Explant Culture or in vivo Transplantation

Overview

This protocol describes the dissection of premigratory cranial neural crest (NC) from Xenopus laevis neurulas. The explants can be cultured in vitro or grafted back into host embryos to study NC migration and differentiation.

Key Study Components

Area of Science

• Neuroscience
• Developmental Biology
• Cell Migration

Background

• The neural crest is a group of cells that migrate during embryonic development.
• Xenopus laevis is a model organism for studying vertebrate development.
• Understanding NC migration is crucial for insights into various developmental processes.
• This method allows for both in vitro and in vivo studies of NC behavior.

Purpose of Study

• To track neural crest cell migration in Xenopus laevis.
• To investigate the mechanisms underlying NC epithelium-to-mesenchyme transition.
• To explore the differentiation of NC cells during development.

Methods Used

• Dissection of neural crests from embryos at the neural stage.
• Plating explants on fibronectin-coated dishes for in vitro studies.
• Grafting explants back into host embryos for in vivo tracking.
• Observation of cell migration patterns and behaviors.

Main Results

• Successful dissection and culture of NC explants.
• Demonstrated in vitro migration of NC cells on fibronectin.
• In vivo grafting allowed tracking of NC migration in host embryos.
• Insights gained into the role of NC migration in development.

Conclusions

• This protocol provides a reliable method for studying NC migration.
• Findings contribute to the understanding of embryonic development.
• Future studies can build on this method to explore related questions.

Frequently Asked Questions