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2
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[Molecules of regulated secretion are differentiation markers of neuroendocrine tumors].[受调节分泌的分子是神经内分泌肿瘤的分化标志物]
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Protein measurement with the Folin phenol reagent.使用福林酚试剂进行蛋白质测定。
J Biol Chem. 1951 Nov;193(1):265-75.
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Identification of a synaptic vesicle-specific membrane protein with a wide distribution in neuronal and neurosecretory tissue.在神经元和神经分泌组织中广泛分布的一种突触小泡特异性膜蛋白的鉴定。
J Cell Biol. 1981 Oct;91(1):257-69. doi: 10.1083/jcb.91.1.257.
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One-step purification of mouse monoclonal antibodies from ascitic fluid by DEAE Affi-Gel blue chromatography.通过DEAE亲和蓝胶色谱法从腹水原液中一步纯化小鼠单克隆抗体。
J Immunol Methods. 1982 Sep 30;53(3):313-9. doi: 10.1016/0022-1759(82)90178-8.
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Effects of stimulation of the chorda tympani in bursts on submaxillary responses in the cat.鼓索神经阵发性刺激对猫下颌下腺反应的影响。
J Physiol. 1982 Jan;322:469-83. doi: 10.1113/jphysiol.1982.sp014050.
5
Transfer of synaptic vesicle antigens to the presynaptic plasma membrane during exocytosis.胞吐过程中突触小泡抗原向突触前质膜的转移。
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Bioactive cardiac substances: potent vasorelaxant activity in mammalian atria.生物活性心脏物质:在哺乳动物心房中具有强大的血管舒张活性。
Science. 1983 Jul 1;221(4605):71-3. doi: 10.1126/science.6857267.
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Distribution of protein I in mammalian brain as determined by a detergent-based radioimmunoassay.采用基于去污剂的放射免疫分析法测定蛋白质I在哺乳动物脑中的分布。
Proc Natl Acad Sci U S A. 1981 Apr;78(4):2130-4. doi: 10.1073/pnas.78.4.2130.
8
Immunoelectron microscopy using thin, frozen sections: application to studies of the intracellular transport of Semliki Forest virus spike glycoproteins.使用薄冰冻切片的免疫电子显微镜技术:应用于研究塞姆利基森林病毒刺突糖蛋白的细胞内运输
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Synapsin I in nerve terminals: selective association with small synaptic vesicles.神经末梢中的突触素I:与小突触小泡的选择性结合。
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Neuron-specific phosphoproteins as models for neuronal gene expression.神经元特异性磷酸化蛋白作为神经元基因表达的模型。
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蛋白质p38:一种神经元和神经内分泌细胞小囊泡特有的整合膜蛋白。

Protein p38: an integral membrane protein specific for small vesicles of neurons and neuroendocrine cells.

作者信息

Navone F, Jahn R, Di Gioia G, Stukenbrok H, Greengard P, De Camilli P

出版信息

J Cell Biol. 1986 Dec;103(6 Pt 1):2511-27. doi: 10.1083/jcb.103.6.2511.

DOI:10.1083/jcb.103.6.2511
PMID:3097029
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2114586/
Abstract

An intrinsic membrane protein of brain synaptic vesicles with Mr 38,000 (p38, synaptophysin) has recently been partially characterized (Jahn, R., W. Schiebler, C. Ouimet, and P. Greengard, 1985, Proc. Natl. Acad. Sci. USA, 83:4137-4141; Wiedenmann, B., and W. W. Franke, 1985, Cell, 41:1017-1028). We have now studied the presence of p38 in a variety of tissues by light and electron microscopy immunocytochemistry and by immunochemistry. Our results indicate that, within the nervous system, p38, like the neuron-specific phosphoprotein synapsin I, is present in virtually all nerve terminals and is selectively associated with small synaptic vesicles (SSVs). No p38 was detectable on large dense-core vesicles (LDCVs). p38 and synapsin I were found to be present in similar concentrations throughout the brain. Outside the nervous system, p38 was found in a variety of neuroendocrine cells, but not in any other cell type. In neuroendocrine cells p38 was localized on a pleiomorphic population of small, smooth-surfaced vesicles, which were interspersed among secretory granules and concentrated in the Golgi area, but not on the secretory granules themselves. Immunoblot analysis of endocrine tissues and cell lines revealed a band with a mobility slightly different from that of neuronal p38. This difference was attributable to a difference in glycosylation. The finding that p38, like synapsin I, is a component of SSVs of virtually all neurons, but not of LDCVs, supports the idea that SSVs and LDCVs are organelles of two distinct pathways for regulated neuronal secretion. In addition, our results indicate the presence in a variety of neuroendocrine cells of an endomembrane system, which is related to SSVs of neurons but is distinct from secretory granules.

摘要

一种分子量为38,000的脑突触小泡内在膜蛋白(p38,突触素)最近已得到部分特性描述(扬恩,R.,W. 席布勒,C. 奥伊梅特,和P. 格林加德,1985年,《美国国家科学院院刊》,83:4137 - 4141;维登曼,B.,和W. W. 弗兰克,1985年,《细胞》,41:1017 - 1028)。我们现在通过光镜和电镜免疫细胞化学以及免疫化学方法研究了多种组织中p38的存在情况。我们的结果表明,在神经系统内,p38与神经元特异性磷蛋白突触结合蛋白I一样,几乎存在于所有神经末梢中,并选择性地与小突触小泡(SSV)相关联。在大致密核心小泡(LDCV)上未检测到p38。发现p38和突触结合蛋白I在整个大脑中的浓度相似。在神经系统之外,p38存在于多种神经内分泌细胞中,但不存在于任何其他细胞类型中。在神经内分泌细胞中,p38定位于一群多形性的小的、表面光滑的小泡上,这些小泡散布在分泌颗粒之间并集中在高尔基体区域,但不在分泌颗粒本身上。对内分泌组织和细胞系的免疫印迹分析显示出一条迁移率与神经元p38略有不同的条带。这种差异归因于糖基化的差异。p38与突触结合蛋白I一样,是几乎所有神经元的SSV的组成成分,但不是LDCV的组成成分,这一发现支持了SSV和LDCV是调节神经元分泌的两条不同途径的细胞器的观点。此外,我们的结果表明在多种神经内分泌细胞中存在一种内膜系统,它与神经元的SSV相关,但与分泌颗粒不同。