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神经元细胞骨架结构域的生化与免疫分析

Biochemical and immunological analyses of cytoskeletal domains of neurons.

作者信息

Peng I, Binder L I, Black M M

出版信息

J Cell Biol. 1986 Jan;102(1):252-62. doi: 10.1083/jcb.102.1.252.

Abstract

We have used cultured sympathetic neurons to identify microtubule proteins (tubulin and microtubule-associated proteins [MAPs]) and neurofilament (NF) proteins in pure preparations of axons and also to examine the distribution of these proteins between axons and cell bodies + dendrites. Pieces of sympathetic ganglia containing thousands of neurons were plated onto culture dishes and allowed to extend neurites. Dendrites remained confined to the ganglionic explant or cell body mass (CBM), while axons extended away from the CBM for several millimeters. Axons were separated from cell bodies and dendrites by dissecting the CBM away from cultures, and the resulting axonal and CBM preparations were analyzed using biochemical, immunoblotting, and immunoprecipitation methods. Cultures were used after 17 d in vitro, when 40-60% of total protein was in the axons. The 68,000-mol-wt NF subunit is present in both axons and CBM in roughly equal amounts. The 145,000- and 200,000-mol-wt NF subunits each consist of several variants which differ in phosphorylation state; poorly and nonphosphorylated species are present only in the CBM, whereas more heavily phosphorylated forms are present in axons and, to a lesser extent, the CBM. One 145,000-mol-wt NF variant was axon specific. Tubulin is roughly equally distributed between CBM and axon-like neurites of explant cultures. MAP-1a, MAP-1b, MAP-3, and the 60,000-mol-wt MAP are also present in the CBM and axon-like neurites and show distribution patterns similar to that of tubulin. In contrast, MAP-2 was detected only in the CBM, while tau and the 210,000-mol-wt MAP were greatly enriched in axons compared to the CBM. In immunostaining analyses, MAP-2 localized to cell bodies and dendrite-like neurites, but not to axon-like neurites, whereas antibodies to tubulin and MAP-1b localized to all regions of the neurons. The regional differences in composition of the neuronal cytoskeleton presumably generate corresponding differences in its structure, which may, in turn, contribute to the morphological differences between axons and dendrites.

摘要

我们利用培养的交感神经元,在轴突的纯制剂中鉴定微管蛋白(微管蛋白和微管相关蛋白[MAPs])和神经丝(NF)蛋白,并研究这些蛋白在轴突与细胞体+树突之间的分布。将含有数千个神经元的交感神经节片段接种到培养皿上,使其长出神经突。树突仍局限于神经节外植体或细胞体团(CBM),而轴突则从CBM延伸数毫米。通过从培养物中分离CBM,将轴突与细胞体和树突分离,然后使用生化、免疫印迹和免疫沉淀方法分析所得的轴突和CBM制剂。在体外培养17天后使用培养物,此时40 - 60%的总蛋白存在于轴突中。68,000道尔顿的NF亚基在轴突和CBM中的含量大致相等。145,000和200,000道尔顿的NF亚基各自由几种磷酸化状态不同的变体组成;磷酸化程度低和未磷酸化的种类仅存在于CBM中,而磷酸化程度更高的形式存在于轴突中,在较小程度上也存在于CBM中。一种145,000道尔顿的NF变体是轴突特异性的。微管蛋白在CBM和外植体培养物的轴突样神经突之间大致均匀分布。MAP - 1a、MAP - 1b、MAP - 3和60,000道尔顿的MAP也存在于CBM和轴突样神经突中,并且显示出与微管蛋白相似的分布模式。相比之下,MAP - 2仅在CBM中检测到,而与CBM相比,tau和210,000道尔顿的MAP在轴突中大量富集。在免疫染色分析中,MAP - 2定位于细胞体和树突样神经突,但不定位于轴突样神经突,而微管蛋白和MAP - 1b的抗体定位于神经元的所有区域。神经元细胞骨架组成的区域差异可能会导致其结构产生相应差异,这反过来可能有助于轴突和树突之间的形态差异。

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