Purkinje Cell Survival in Organotypic Cerebellar Slice Cultures

Jennifer Rakotomamonjy; Alicia Guemez-Gamboa

doi:10.3791/60353

Purkinje Cell выживания в органотипической церебеллярной части культур

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Neuroscience

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JoVE Journal Neuroscience

Purkinje Cell Survival in Organotypic Cerebellar Slice Cultures

Purkinje Cell выживания в органотипической церебеллярной части культур

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06:31 min

December 18, 2019

DOI: 10.3791/60353-v

Jennifer Rakotomamonjy¹, Alicia Guemez-Gamboa¹

¹Department of Physiology,Northwestern University, Feinberg School of Medicine

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Overview

This study describes a protocol for generating organotypic slice cultures of mouse cerebellum to model Purkinje cell death during neurodevelopment. The technique preserves tissue architecture and cell-cell connections, allowing for a closer simulation of in vivo conditions and facilitating the examination of neuroprotective agents.

Key Study Components

Area of Science

Neurodevelopment
Neuroprotection
Organotypic cultures

Background

Organotypic slice cultures serve as a model for studying neurodevelopmental and degenerative processes.
This approach preserves the architecture and connections of the tissue, unlike dissociated primary cell cultures.
The protocol focuses on the study of Purkinje cell death in the cerebellum.
It has potential for screening neuroprotective drug candidates.

Purpose of Study

To model neurodevelopmental death of Purkinje cells in organotypic slice cultures.
To identify effective neuroprotective agents through pharmacological treatments.
To facilitate research in neurodevelopment and neurodegeneration.

Methods Used

Organotypic slice cultures of mouse cerebellum were employed to study Purkinje cell death.
The tissue was dissected and sliced into sections, which were then cultured in a medium supplemented with pharmacological agents.
Immunofluorescence staining was performed for cellular analysis.
Key steps included careful harvesting, slicing of the brain, and setting up of culture conditions.

Main Results

At postnatal day six, low survival rates of Purkinje cells were observed, aligning with their vulnerability window.
Treatment with potassium chloride successfully induced depolarization and enhanced survival rates of the cells.
Consistent results were achieved by selecting viable cerebellar sections and efficient culture setups.

Conclusions

This study demonstrates an effective method to model Purkinje cell death and screen neuroprotective drugs.
Results highlight the importance of timing and tissue quality for consistent outcomes in neurodevelopmental studies.
The findings have significant implications for understanding neuroprotective strategies in degenerative diseases.

Frequently Asked Questions

What are the advantages of using organotypic slice cultures?

Organotypic slice cultures maintain the tissue architecture and cell-cell interactions, providing a more in vivo-like environment for the study of neurodevelopmental and neurodegenerative processes.

How is Purkinje cell death modeled in this protocol?

Purkinje cell death is modeled by generating organotypic slices of the cerebellum from mice and examining cell survival after treatment with various pharmacological agents.

What types of data or outcomes can be obtained from this method?

The method allows for the assessment of cell survival, immunofluorescence staining results, and any electrophysiological changes or responsiveness to pharmacological treatments.

Can this method be adapted for other regions of the central nervous system?

Yes, organotypic slice cultures can be adapted to model neurodegenerative diseases in various regions of the central nervous system.

What are key limitations or considerations for this protocol?

It is critical to select healthy cerebellar sections and perform the culture setup efficiently to ensure reproducibility and consistency in results.

How does this study contribute to neuroprotective drug discovery?

By modeling Purkinje cell death, researchers can screen for neuroprotective agents and validate their efficacy in a controlled environment that mimics in vivo conditions.

Органотипические срезные культуры являются мощным инструментом для изучения нейроразвития или дегенеративных / регенеративных процессов. Здесь мы описываем протокол, который моделирует нейроразвитие смерти клеток Purkinje в мыши мозжечковой культуры ломтик. Этот метод может принести пользу исследованиям в нейропротекторных открытий наркотиков.

Органотипическая культура ломтика является мощным инструментом для изучения нейроразвития и дегенеративных или регенеративных процессов. Этот метод может быть использован для быстрого экрана молекул кандидата для их нейропротекторного потенциала. Этот метод тесно имитирует условия in vivo, по сравнению с диссоциированными культурами первичных клеток, так как архитектура тканей и родных клеточных соединений сохраняются в плоскостях секций.

Здесь мы демонстрируем изучение смерти клеток Пуркинье в развивающемся мозжечках. Но органотипическая культура ломтика одинаково подходит для моделирования нейродегенеративных заболеваний почти в каждом регионе центральной нервной системы. Демонстрацией процедуры с Дженнифер Ракотомамонджи будет Шон МакДермотт, техник из моей лаборатории.

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