The mouse cerebellar cortex in organotypic slice cultures: an in vitro model to analyze the consequences of mutations and pathologies on neuronal survival, development, and function.

Etienne Lonchamp, Jean-Luc Dupont, Huguette Beekenkamp, Bernard Poulain, Jean-Louis Bossu
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引用次数: 12

Abstract

Thin acute slices and dissociated cell cultures taken from different parts of the brain have been widely used to examine the function of the nervous system, neuron-specific interactions, and neuronal development (specifically, neurobiology, neuropharmacology, and neurotoxicology studies). Here, we focus on an alternative in vitro model: brain-slice cultures in roller tubes, initially introduced by Beat Gähwiler for studies with rats, that we have recently adapted for studies of mouse cerebellum. Cultured cerebellar slices afford many of the advantages of dissociated cultures of neurons and thin acute slices. Organotypic slice cultures were established from newborn or 10-15-day-old mice. After 3-4 weeks in culture, the slices flattened to form a cell monolayer. The main types of cerebellar neurons could be identified with immunostaining techniques, while their electrophysiological properties could be easily characterized with the patch-clamp recording technique. When slices were taken from newborn mice and cultured for 3 weeks, aspects of the cerebellar development were displayed. A functional neuronal network was established despite the absence of mossy and climbing fibers, which are the two excitatory afferent projections to the cerebellum. When slices were made from 10-15-day-old mice, which are at a developmental stage when cerebellum organization is almost established, the structure and neuronal pathways were intact after 3-4 weeks in culture. These unique characteristics make organotypic slice cultures of mouse cerebellar cortex a valuable model for analyzing the consequences of gene mutations that profoundly alter neuronal function and compromise postnatal survival.

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器官型切片培养的小鼠小脑皮层:一种体外模型,用于分析突变和病理对神经元存活、发育和功能的影响。
从大脑不同部位提取的急性薄切片和分离细胞培养物已被广泛用于检查神经系统功能、神经元特异性相互作用和神经元发育(特别是神经生物学、神经药理学和神经毒理学研究)。在这里,我们专注于另一种体外模型:滚轴管中的脑切片培养,最初由Beat Gähwiler引入用于大鼠研究,我们最近将其用于小鼠小脑的研究。培养的小脑切片具有分离培养神经元和薄急性切片的许多优点。从新生或10-15日龄小鼠中建立器官型切片培养。培养3-4周后,切片变平形成单层细胞。免疫染色技术可以识别小脑神经元的主要类型,膜片钳记录技术可以很容易地表征其电生理特性。从新生小鼠身上取切片,培养3周,显示小脑发育的各个方面。尽管没有苔藓纤维和攀爬纤维这两种兴奋性传入神经投射到小脑,但仍建立了功能性神经网络。10-15日龄小鼠处于小脑组织基本建立的发育阶段,经3-4周培养后结构和神经元通路完整。这些独特的特征使小鼠小脑皮层的器官型切片培养成为分析基因突变后果的有价值的模型,这些基因突变深刻地改变了神经元功能并损害了出生后的生存。
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