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Dendritic and postsynaptic localizations of glycine receptor alpha subunit mRNAs.甘氨酸受体α亚基mRNA的树突状和突触后定位
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Synapse-specific, long-term facilitation of aplysia sensory to motor synapses: a function for local protein synthesis in memory storage.海兔感觉运动突触特异性的长期易化:局部蛋白质合成在记忆存储中的作用。
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Dendritic and postsynaptic localizations of glycine receptor alpha subunit mRNAs.甘氨酸受体α亚基mRNA的树突状和突触后定位
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树突状和突触后蛋白合成机制。

Dendritic and postsynaptic protein synthetic machinery.

作者信息

Gardiol A, Racca C, Triller A

机构信息

Laboratoire de Biologie Cellulaire de la Synapse Normale et Pathologique, Institut National de la Santé et de la Recherche Médicale U497, Ecole Normale Supérieure, 75005 Paris, France.

出版信息

J Neurosci. 1999 Jan 1;19(1):168-79. doi: 10.1523/JNEUROSCI.19-01-00168.1999.

DOI:10.1523/JNEUROSCI.19-01-00168.1999
PMID:9870948
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6782360/
Abstract

There is a growing body of evidence that local protein synthesis beneath synapses may provide a novel mechanism underlying plastic phenomena. In vivo and in vitro biochemical data show that dendrites can perform translation and glycosylation. Using antibodies directed against the eukaryotic protein synthetic machinery, we sought to identify the structures implicated in nonperinuclear translation, namely dendritic and postsynaptic protein synthesis. We performed a morphological and immunocytochemical analysis of ventromedial horn rat spinal cord neurons using both light and electron microscopy. We show at the cellular level that, in vivo, protein synthesis macrocomplexes (ribosomes and eIF-2) as well as the endomembranous system implicated in cotranslational and posttranslational modifications (endoplasmic reticulum and Golgi cisternae) penetrated some dendrites. Membrane-limited organelles of different shape and size are present close to the postsynaptic differentiations of most synapses, independently of their localization on the neuronal surface. We demonstrate (1) that some cisternae are immunoreactive for antibodies against ribosomal proteins and eIF-2, and (2) that markers of endoplasmic reticulum (BiP), intermediate compartment, and Golgi complex (rab1, CTR433, TGN38) label subsets of these subsynaptic organelles. Therefore, these findings indicate that synapses are equipped with the essential elements required for the synthesis and insertion of a well folded and glycosylated transmembrane protein.

摘要

越来越多的证据表明,突触下的局部蛋白质合成可能为可塑性现象提供一种新的机制。体内和体外生化数据表明,树突可以进行翻译和糖基化。我们使用针对真核生物蛋白质合成机制的抗体,试图识别与非核周翻译相关的结构,即树突和突触后蛋白质合成。我们使用光学显微镜和电子显微镜对大鼠脊髓腹内侧角神经元进行了形态学和免疫细胞化学分析。我们在细胞水平上表明,在体内,蛋白质合成大复合物(核糖体和eIF-2)以及参与共翻译和翻译后修饰的内膜系统(内质网和高尔基池)穿透了一些树突。大多数突触的突触后分化附近存在不同形状和大小的膜性细胞器,与它们在神经元表面的定位无关。我们证明:(1)一些池对核糖体蛋白和eIF-2抗体具有免疫反应性;(2)内质网(BiP)、中间区室和高尔基复合体(rab1、CTR433、TGN38)的标记物标记了这些突触下细胞器的亚群。因此,这些发现表明,突触具备合成和插入折叠良好且糖基化的跨膜蛋白所需的基本元件。