Dissection and Culture of Mouse Embryonic Kidney

Overview

This protocol describes a method for isolating and culturing metanephric rudiments from mouse embryos. It aims to observe the effects of specific treatments on ureteric bud branching morphology.

Key Study Components

Area of Science

• Neuroscience
• Developmental Biology
• Kidney Organogenesis

Background

• Understanding tubular branching morphogenesis is crucial for kidney development.
• Epithelial mesenchyme interactions play a significant role in organogenesis.
• Congenital malformations can arise from disruptions in these processes.
• This method provides direct access to the organ for study.

Purpose of Study

• To isolate metanephric rudiments from mouse embryos.
• To culture these rudiments for experimental treatments.
• To investigate branching morphology of ureteric buds.

Methods Used

• Use sterile forceps to place polycarbonate membrane filters in culture wells.
• Prepare culture medium in a four-well plate.
• Modify micropipette tips for easier transfer of samples.
• Incubate samples in a controlled environment.

Main Results

• The technique allows for effective isolation of kidney rudiments.
• Facilitates observation of ureteric bud branching.
• Simple and cost-effective method for organ culture.
• Can be modified for various experimental conditions.

Conclusions

• This method enhances understanding of kidney development.
• It provides insights into the mechanisms of congenital malformations.
• Future studies can build on this protocol to explore further questions in organogenesis.

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