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糖基磷脂酰肌醇(GPI)锚定蛋白在其于Caco-2细胞内的转运过程中会相互结合形成微结构域。

GPI-anchored proteins associate to form microdomains during their intracellular transport in Caco-2 cells.

作者信息

Garcia M, Mirre C, Quaroni A, Reggio H, Le Bivic A

机构信息

Biologie de la Différenciation Cellulaire, U.R.A. 179, Faculté des Sciences de Luminy, Marseille, France.

出版信息

J Cell Sci. 1993 Apr;104 ( Pt 4):1281-90. doi: 10.1242/jcs.104.4.1281.

Abstract

In this study, we have investigated the possibility that glycosyl-phosphatidylinositol (GPI)-anchored proteins form insoluble membrane complexes in Caco-2 cells and that transmembrane proteins are associated with these complexes. GPI-anchored proteins were mainly resistant to Triton X-100 (TX-100) extraction at 4 degrees C but fully soluble in n-octyl-glucoside. Resistance to Triton X-100 extraction was not observed in the endoplasmic reticulum but appeared during transport through the Golgi complex. It was not dependent upon N-glycosylation processing, or pH variation from 6.5 to 8.5, and was not affected by sterol-binding agents. Other apical or basolateral transmembrane proteins were well solubilized in TX-100, with the exception of sucrase-isomaltase, which was partly insoluble. We isolated a membrane fraction from Caco-2 cells that contained GPI-anchored proteins and sucrase-isomaltase but no antigen 525, a basolateral marker, or dipeptidylpeptidase IV, an apical one. These data suggest that GPI-anchored proteins cluster to form membrane microdomains together with an apical transmembrane protein, providing a possible apical sorting mechanism for intestinal cells in vitro that might be related to apical sorting in MDCK cells, and that other mechanisms might exist to sort proteins to the apical membrane.

摘要

在本研究中,我们探讨了糖基磷脂酰肌醇(GPI)锚定蛋白在Caco-2细胞中形成不溶性膜复合物以及跨膜蛋白与这些复合物相关联的可能性。GPI锚定蛋白在4℃下主要抵抗Triton X-100(TX-100)提取,但在正辛基葡萄糖苷中完全可溶。在内质网中未观察到对Triton X-100提取的抗性,但在通过高尔基体复合体的转运过程中出现。它不依赖于N-糖基化加工,也不受pH从6.5到8.5变化的影响,并且不受固醇结合剂的影响。除了部分不溶的蔗糖酶异麦芽糖酶外,其他顶端或基底外侧跨膜蛋白在TX-100中很容易溶解。我们从Caco-2细胞中分离出一个膜组分,其含有GPI锚定蛋白和蔗糖酶异麦芽糖酶,但不含有基底外侧标记物抗原525或顶端标记物二肽基肽酶IV。这些数据表明,GPI锚定蛋白与顶端跨膜蛋白聚集形成膜微区,为体外肠道细胞提供了一种可能的顶端分选机制,这可能与MDCK细胞中的顶端分选有关,并且可能存在其他将蛋白分选到顶端膜的机制。

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