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韦弗小鼠小脑颗粒神经元在体外无法在野生型星形胶质细胞突起上迁移。

Weaver mouse cerebellar granule neurons fail to migrate on wild-type astroglial processes in vitro.

作者信息

Hatten M E, Liem R K, Mason C A

出版信息

J Neurosci. 1986 Sep;6(9):2676-83. doi: 10.1523/JNEUROSCI.06-09-02676.1986.

DOI:10.1523/JNEUROSCI.06-09-02676.1986
PMID:3528411
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6568692/
Abstract

To study the regulation of glial-guided neuronal migration, we have analyzed the behavior of cerebellar granule neurons purified from the homozygous weaver (wv/wv) B6CBA-w mouse, an autosomal recessive genetic mutation that suffers a failure of granule cell migration along Bergmann glial processes (Rakic and Sidman, 1973a, b; Rezai and Yoon, 1972), on the processes of astroglia purified from homozygous normal B6CBA-Aw-J-wv (+/+) mouse cerebella. When co-cultured with normal astroglia, weaver granule neurons failed to form neuron-glia contacts characteristic of migrating neurons and impaired normal astroglial morphological differentiation. Normal astroglial cells co-cultured with weaver granule cells had enlarged cell somata with stunted processes and enlarged endfeet compared to normal astroglia co-cultured with normal granule cells. In contrast, normal neurons associated with weaver astroglia, forming tight appositions seen for migrating neurons in vivo, and enhanced weaver astroglial morphological differentiation. Weaver astroglia co-cultured with normal granule cells contained a more normal complement of glial filaments and had a smaller perikaryon with longer, more tapered processes than their counterparts co-cultured with weaver neurons. These results suggest, in agreement with the study of Goldowitz and Mullen (1982) on heterozygous mutant chimeras, that the granule neuron is a primary site of action of the weaver gene, and further support our previous findings that neuron-glia interactions regulate astroglial morphological differentiation (Hatten, 1985).

摘要

为了研究胶质细胞引导的神经元迁移的调控机制,我们分析了从纯合织工(wv/wv)B6CBA-w小鼠中纯化得到的小脑颗粒神经元的行为。该小鼠存在常染色体隐性基因突变,其颗粒细胞沿伯格曼胶质细胞突起的迁移过程出现障碍(拉基奇和西德曼,1973a,b;雷扎伊和尹,1972)。我们将这些神经元与从纯合正常B6CBA-Aw-J-wv(+/+)小鼠小脑中纯化得到的星形胶质细胞的突起共同培养。当与正常星形胶质细胞共培养时,织工颗粒神经元无法形成迁移神经元特有的神经元-胶质细胞接触,并且损害了正常星形胶质细胞的形态分化。与正常颗粒细胞共培养的正常星形胶质细胞相比,与织工颗粒细胞共培养的正常星形胶质细胞的细胞体增大,突起发育不良,终足增大。相反,正常神经元与织工星形胶质细胞相互作用,形成了在体内迁移神经元中可见的紧密附着,并增强了织工星形胶质细胞的形态分化。与正常颗粒细胞共培养的织工星形胶质细胞含有更正常的胶质丝成分,其核周体较小,突起更长且更呈锥形,而与织工神经元共培养的对应细胞则不然。这些结果表明,与戈德洛维茨和马伦(1982)对杂合突变嵌合体的研究一致,颗粒神经元是织工基因的主要作用位点,并进一步支持了我们之前的发现,即神经元-胶质细胞相互作用调节星形胶质细胞的形态分化(哈滕,1985)。

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