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Isolation and characterization of postsynaptic densities from various brain regions: enrichment of different types of postsynaptic densities

机译:不同脑区突触后密度的分离和表征:不同类型突触后密度的富集

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摘要

Postsynaptic densities (PSDs) have been isolated from cerebral cortex, midbrain, cerebellum, and brain stem by the Triton X-100 method previously used in the isolation of cerebral PSDs (Cohen et al., 1977, J. Cell Biol. 74:181). These PSDs have been compared in protein composition, protein phosphorylation, and morphology. Thin-section electron microscopy revealed that cerebral cortex and midbrain PSDs were identical, being approximately 57 nm thick and composed of apparent aggregates 20-30 nm in diameter. Isolated cerebellar PSDs appeared thinner (33 nm) than cerebral cortex PSDs and lacked the apparent 20- to 30-nm aggregates, but had a latticelike structure. In unidirectional and rotary-shadowed replicas, the cerebrum and midbrain PSDs were circular in shape with a large central perforation or hole in the center of them. Cerebellum PSDs did not have a large perforation, but did have numerous smaller perforations in a lattice like structure. Filaments (6-9 nm) were observed connecting possible 20- to 30-nm aggregates in cerebrum PSDs and were also observed radiating from one side of the PSD. Both cerebral cortex and midbrain PSDs exhibited identical protein patterns on SDS gel electrophoresis. In comparison, cerebellar PSDs (a) lacked the major 51,000 Mr protein, (b) contained two times less calmodulin, and (c) contained a unique protein at 73,000 Mr. Calcium plus calmodulin stimulated the phosphorylation of the 51,000 and 62,000 Mr bands in both cerebral cortex and midbrain PSDs. In cerebellar PSDs, only the 58,000 and 62,000 Mr bands were phosphorylated. In the PSDs from all brain regions, cAMP stimulated the phosphorylation of Protein Ia (73,000 Mr), Protein Ib (68.000 Mr), and a 60,000 Mr protein, although cerebrum and midbrain PSDs contained very much higher levels of phosphorylated protein than did the cerebellum. On the basis of the morphological criteria, it is possible that PSDs isolated from cerebrum and midbrain were derived from the Gray type I, or asymmetric, synapses, whereas cerebellum PSDs were derived from the Gray type II, or symmetric, synapses. Since there is some evidence that the type I synapses are involved in excitatory mechanisms while the type II are involved in inhibitory mechanisms, the role of the PSD and of some of its proteins in these synaptic responses is discussed.
机译:已经通过以前用于分离脑PSD的Triton X-100方法从大脑皮层,中脑,小脑和脑干中分离出突触后密度(PSD)(Cohen等,1977,J.Cell Biol.74:181。 )。这些PSD在蛋白质组成,蛋白质磷酸化和形态方面已进行了比较。薄层电子显微镜显示,大脑皮层和中脑PSD是相同的,大约57 nm厚,由直径20-30 nm的表观聚集体组成。孤立的小脑PSD比大脑皮层PSD薄(33 nm),并且缺乏明显的20至30 nm聚集体,但具有格状结构。在单向和旋转阴影副本中,大脑和中脑PSD呈圆形,在它们的中央有一个大的中央穿孔或孔。小脑PSD没有较大的穿孔,但在格子状结构中确实有许多较小的穿孔。观察到细丝(6-9 nm)连接了大脑PSD中可能的20至30 nm的聚集体,并且还观察到从PSD的一侧辐射。在SDS凝胶电泳上,大脑皮层和中脑PSD均显示相同的蛋白质模式。相比之下,小脑PSD(a)缺少主要的51,000 Mr蛋白,(b)含有少两倍的钙调蛋白,(c)含有独特的蛋白,钙含量为73,000Mr。钙加钙调蛋白刺激了51,000和62,000 Mr带的磷酸化。大脑皮层和中脑PSD。在小脑PSD中,仅58,000和62,000 Mr带被磷酸化。在所有大脑区域的PSD中,cAMP刺激了蛋白Ia(73,000 Mr),蛋白Ib(68.000 Mr)和60,000 Mr蛋白的磷酸化,尽管大脑和中脑PSD的磷酸化蛋白水平比小脑高得多。 。根据形态学标准,从大脑和中脑中分离出的PSD可能源自I型灰色突触或不对称突触,而小脑PSD则源自II型灰色突触或对称性突触。由于有证据表明I型突触与兴奋机制有关,而II型与抑制机制有关,因此我们讨论了PSD及其某些蛋白质在这些突触反应中的作用。

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