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葡糖神经酰胺在各种高尔基体亚组分的胞质表面合成。

Glucosylceramide is synthesized at the cytosolic surface of various Golgi subfractions.

作者信息

Jeckel D, Karrenbauer A, Burger K N, van Meer G, Wieland F

机构信息

Institut für Biochemie, Universität Heidelberg, Germany.

出版信息

J Cell Biol. 1992 Apr;117(2):259-67. doi: 10.1083/jcb.117.2.259.

DOI:10.1083/jcb.117.2.259
PMID:1532799
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2289419/
Abstract

In our attempt to assess the topology of glucosylceramide biosynthesis, we have employed a truncated ceramide analogue that permeates cell membranes and is converted into water soluble sphingolipid analogues both in living and in fractionated cells. Truncated sphingomyelin is synthesized in the lumen of the Golgi, whereas glucosylceramide is synthesized at the cytosolic surface of the Golgi as shown by (a) the insensitivity of truncated sphingomyelin synthesis and the sensitivity of truncated glucosylceramide synthesis in intact Golgi membranes from rabbit liver to treatment with protease or the chemical reagent DIDS; and (b) sensitivity of truncated sphingomyelin export and insensitivity of truncated glucosylceramide export to decreased temperature and the presence of GTP-gamma-S in semiintact CHO cells. Moreover, subfractionation of rat liver Golgi demonstrated that the sphingomyelin synthase activity was restricted to fractions containing marker enzymes for the proximal Golgi, whereas the capacity to synthesize truncated glucosylceramide was also found in fractions containing distal Golgi markers. A similar distribution of glucosylceramide synthesizing activity was observed in the Golgi of the human liver derived HepG2 cells. The cytosolic orientation of the reaction in HepG2 cells was confirmed by complete extractability of newly formed NBD-glucosylceramide from isolated Golgi membranes or semiintact cells by serum albumin, whereas NBD-sphingomyelin remained protected against such extraction.

摘要

在我们评估葡萄糖神经酰胺生物合成拓扑结构的尝试中,我们使用了一种截短的神经酰胺类似物,它能穿透细胞膜,并在活细胞和分离的细胞中转化为水溶性鞘脂类似物。截短的鞘磷脂在高尔基体腔内合成,而葡萄糖神经酰胺则在高尔基体的胞质表面合成,如下所示:(a) 兔肝完整高尔基体膜中截短的鞘磷脂合成对蛋白酶或化学试剂DIDS处理不敏感,而截短的葡萄糖神经酰胺合成敏感;(b) 在半完整的CHO细胞中,截短的鞘磷脂输出对温度降低和GTP-γ-S的存在敏感,而截短的葡萄糖神经酰胺输出不敏感。此外,大鼠肝脏高尔基体的亚分级显示,鞘磷脂合酶活性局限于含有近端高尔基体标记酶的组分,而在含有远端高尔基体标记的组分中也发现了合成截短葡萄糖神经酰胺的能力。在人源肝癌HepG2细胞的高尔基体中也观察到了类似的葡萄糖神经酰胺合成活性分布。通过血清白蛋白可从分离的高尔基体膜或半完整细胞中完全提取新形成的NBD-葡萄糖神经酰胺,证实了HepG2细胞中该反应的胞质方向,而NBD-鞘磷脂仍受到保护,不被这种提取。

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