De Camilli P, Harris S M, Huttner W B, Greengard P
J Cell Biol. 1983 May;96(5):1355-73. doi: 10.1083/jcb.96.5.1355.
Synapsin I (protein I) is a major neuron-specific endogenous substrate for cAMP-dependent and Ca/calmodulin-dependent protein kinases that is widely distributed in synapses of the central and peripheral nervous system (De Camilli, P., R. Cameron, and P. Greengard, 1983, J. Cell Biol. 96:1337-1354). We have now carried out a detailed analysis of the ultrastructural localization of synapsin I in the synapse. For this purpose we have developed a novel immunocytochemical technique that involves the labeling of isolated synaptosomes immobilized in a thin agarose gel. Special fixation conditions were designed to maximize accessibility of synapsin I to marker molecules. Immunoferritin and immunoperoxidase studies of this preparation indicated that synapsin I is localized in the presynaptic compartment and that it is present in close to 100% of all nerve endings. Immunoferritin labeling also indicated that, inside the nerve ending, synapsin I is specifically associated with the cytoplasmic surface of synaptic vesicles. In agreement with these immunoferritin results, the labeling produced by immunoperoxidase was compatible with a specific association of synapsin I with synaptic vesicle membranes. However, at variance with the very specific distribution of immunoferritin, immunoperoxidase reaction product was also found on other membranes of the terminals, presumably as a result of its diffusion over a short distance from the synaptic vesicles. Anti-synapsin I immunoperoxidase staining of tissue sections for electron microscopy produced an uneven labeling of terminals of the neuropile, in agreement with results of a previous study (Bloom, F. E., T. Ueda, E. Battenberg, and P. Greengard, 1979, Proc. Natl. Acad. Sci. USA. 76:5982-5986). A comparison with results obtained in isolated synapses indicates that the limited labeling of nerve endings in tissue sections results from limited and uneven penetration by marker molecules. The specific association of synapsin 1 with synaptic vesicle membranes in the great majority of nerve terminals suggests a prominent role for this phosphoprotein in the regulation of synaptic vesicle function.
突触素I(蛋白质I)是一种主要的神经元特异性内源性底物,可被环磷酸腺苷(cAMP)依赖性蛋白激酶和钙/钙调蛋白依赖性蛋白激酶作用,广泛分布于中枢和外周神经系统的突触中(德·卡米利,P.,R. 卡梅伦,和P. 格林加德,1983年,《细胞生物学杂志》96:1337 - 1354)。我们现在对突触素I在突触中的超微结构定位进行了详细分析。为此,我们开发了一种新颖的免疫细胞化学技术,该技术涉及对固定在薄琼脂糖凝胶中的分离突触体进行标记。设计了特殊的固定条件,以使突触素I对标记分子的可及性最大化。对该制剂的免疫铁蛋白和免疫过氧化物酶研究表明,突触素I定位于突触前区室,并且存在于几乎所有神经末梢中。免疫铁蛋白标记还表明,在神经末梢内部,突触素I与突触小泡的细胞质表面特异性相关。与这些免疫铁蛋白结果一致,免疫过氧化物酶产生的标记与突触素I与突触小泡膜的特异性关联相符。然而,与免疫铁蛋白非常特异的分布不同,免疫过氧化物酶反应产物也在终末的其他膜上被发现,推测是由于其从突触小泡短距离扩散所致。用于电子显微镜检查的组织切片的抗突触素I免疫过氧化物酶染色对神经毡终末产生了不均匀的标记,这与先前一项研究的结果一致(布鲁姆,F. E.,T. 上田,E. 巴顿伯格,和P. 格林加德,1979年,《美国国家科学院院刊》76:5982 - 5986)。与在分离突触中获得的结果比较表明,组织切片中神经末梢标记有限是由于标记分子穿透有限且不均匀所致。突触素1在绝大多数神经末梢中与突触小泡膜的特异性关联表明该磷蛋白在调节突触小泡功能中起重要作用。
