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大鼠海马体的膜磷蛋白:对强直刺激和脑啡肽的敏感性

Membrane phosphoproteins of rat hippocampus: sensitivity to tetanic stimulation and enkephalin.

作者信息

Bär P R, Tielen A M, Lopes Da Silva F H, Zwiers H, Gispen W H

出版信息

Brain Res. 1982 Aug 5;245(1):69-79. doi: 10.1016/0006-8993(82)90340-7.

Abstract

Hippocampal slices are electrically stimulated in the perforant path with a pulse-train, which can lead to long-term potentiation (LTP). Of the thus stimulated slices, subcellular fractions are prepared and used in an endogenous protein phosphorylation assay. A phosphoprotein band which was reported earlier to be sensitive to electric stimulation as well as to methionine-enkephalin is now further analyzed: it consists of two phosphoproteins only slightly differing in molecular weight: 50,000 Mr (50 K) and 52,000 Mr (52 K), but having distinct biochemical properties and subcellular localization. Their IEP is dissimilar (3.5-4.3 and 5.3, respectively), they display different sensitivity towards calcium when tested in the phosphorylation assay, but are both cAMP-independently phosphorylated. Only one of them responds to tetanic stimulation with an increased phosphorylation post hoc. This protein, the 52 K component, is localized in synaptic membranes. Moreover, this protein also responds to incubation of slices with methionine-enkephalin. The phosphorylation of the 50 K component is not influenced by electric stimulation, nor by incubations with neuropeptides; its phosphorylation takes place in material sedimenting with the mitochondrial cell fractions and is strongly calcium- and calmodulin-dependent.

摘要

用脉冲串在穿通路径中对海马切片进行电刺激,这会导致长时程增强(LTP)。对如此刺激的切片制备亚细胞级分,并用于内源性蛋白质磷酸化测定。现在对先前报道的对电刺激以及甲硫氨酸脑啡肽敏感的磷蛋白条带进行进一步分析:它由两种分子量仅略有差异的磷蛋白组成:50,000 Mr(50 K)和52,000 Mr(52 K),但具有不同的生化特性和亚细胞定位。它们的等电点不同(分别为3.5 - 4.3和5.3),在磷酸化测定中测试时对钙显示出不同的敏感性,但两者都是非cAMP依赖性磷酸化。其中只有一种在强直刺激后磷酸化增加。这种蛋白质,即52 K组分,定位于突触膜中。此外,这种蛋白质也对用甲硫氨酸脑啡肽孵育切片有反应。50 K组分的磷酸化不受电刺激影响,也不受与神经肽孵育的影响;其磷酸化发生在线粒体细胞级分沉淀的物质中,并且强烈依赖于钙和钙调蛋白。

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