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突触素在非神经内分泌上皮细胞中被分选到特殊囊泡中。

Sorting of synaptophysin into special vesicles in nonneuroendocrine epithelial cells.

作者信息

Leube R E, Leimer U, Grund C, Franke W W, Harth N, Wiedenmann B

机构信息

Division of Cell Biology, German Cancer Research Center, Heidelberg, Federal Republic of Germany.

出版信息

J Cell Biol. 1994 Dec;127(6 Pt 1):1589-601. doi: 10.1083/jcb.127.6.1589.

DOI:10.1083/jcb.127.6.1589
PMID:7798314
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2120288/
Abstract

Synaptophysin is a major transmembrane glycoprotein of a type of small vesicle with an electron-translucent content (SET vesicles), including the approximately 50-nm presynaptic vesicles in neuronal cells, and of similar, somewhat larger (< or = approximately 90 nm) vesicles (SLMV) in neuroendocrine (NE) cells. When certain epithelial non-NE cells, such as human hepatocellular carcinoma PLC cells, were cDNA transfected to synthesize synaptophysin, the new molecules appeared in specific SET vesicles. As this was in contrast to other reports that only NE cells were able to sort synaptophysin away from other plasma membrane proteins into presynaptic- or SLMV-type vesicles, we have further characterized the vesicles containing synaptophysin in transfected PLC cells. Using fractionation and immunoisolation techniques, we have separated different kinds of vesicles, and we have identified a distinct type of synaptophysin-rich, small (30-90-nm) vesicle that contains little, if any, protein of the constitutive secretory pathway marker hepatitis B surface antigen, of the fluid phase endocytosis marker HRP, and of the plasma membrane recycling endosomal marker transferrin receptor. In addition, we have found variously sized vesicles that contained both synaptophysin and transferrin receptor. A corresponding result was also obtained by direct visualization, using double-label immunofluorescence microscopy for the endocytotic markers and synaptophysin in confocal laser scan microscopy and in double-immunogold label electron microscopy. We conclude that diverse non-NE cells of epithelial nature are able to enrich the "foreign" molecule synaptophysin in a category of SET vesicles that are morphologically indistinguishable from SLMV of NE cells, including one type of vesicle in which synaptophysin is sorted away from endosomal marker proteins. Possible mechanisms of this sorting are discussed.

摘要

突触素是一种主要的跨膜糖蛋白,存在于一类内容物电子密度低的小囊泡(SET囊泡)中,包括神经元细胞中约50纳米的突触前囊泡,以及神经内分泌(NE)细胞中类似的、稍大一些(≤约90纳米)的囊泡(SLMV)。当某些上皮性非NE细胞,如人肝癌PLC细胞,经cDNA转染以合成突触素时,新分子出现在特定的SET囊泡中。由于这与其他报道相反,其他报道称只有NE细胞能够将突触素与其他质膜蛋白分离开来,进入突触前或SLMV型囊泡,我们进一步对转染的PLC细胞中含有突触素的囊泡进行了表征。使用分级分离和免疫分离技术,我们分离出了不同种类的囊泡,并鉴定出一种独特类型的富含突触素的小(30 - 90纳米)囊泡,这种囊泡几乎不含有组成型分泌途径标记物乙型肝炎表面抗原、液相内吞标记物HRP以及质膜回收内体标记物转铁蛋白受体的蛋白质。此外,我们还发现了各种大小的同时含有突触素和转铁蛋白受体的囊泡。通过共聚焦激光扫描显微镜和双免疫金标记电子显微镜对内吞标记物和突触素进行双标记免疫荧光显微镜直接观察,也得到了相应的结果。我们得出结论,多种上皮性质的非NE细胞能够在一类SET囊泡中富集“外来”分子突触素,这些囊泡在形态上与NE细胞的SLMV无法区分,包括一种能将突触素与内体标记蛋白分离开来的囊泡类型。本文讨论了这种分选的可能机制。

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