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鞘糖脂和胆固醇对小窝内吞作用的选择性刺激。

Selective stimulation of caveolar endocytosis by glycosphingolipids and cholesterol.

作者信息

Sharma Deepak K, Brown Jennifer C, Choudhury Amit, Peterson Timothy E, Holicky Eileen, Marks David L, Simari Robert, Parton Robert G, Pagano Richard E

机构信息

Department of Biochemistry and Molecular Biology, Mayo Clinic and Foundation, Rochester, Minnesota 55905, USA.

出版信息

Mol Biol Cell. 2004 Jul;15(7):3114-22. doi: 10.1091/mbc.e04-03-0189. Epub 2004 Apr 23.

Abstract

Internalization of some plasma membrane constituents, bacterial toxins, and viruses occurs via caveolae; however, the factors that regulate caveolar internalization are still unclear. Here, we demonstrate that a brief treatment of cultured cells with natural or synthetic glycosphingolipids (GSLs) or elevation of cholesterol (either by acute treatment with mbeta-cyclodextrin/cholesterol or by alteration of growth conditions) dramatically stimulates caveolar endocytosis with little or no effect on other endocytic mechanisms. These treatments also stimulated the movement of GFP-labeled vesicles in cells transfected with caveolin-1-GFP and reduced the number of surface-connected caveolae seen by electron microscopy. In contrast, overexpression of caveolin-1 decreased caveolar uptake, but treatment with GSLs reversed this effect and stimulated caveolar endocytosis. Stimulation of caveolar endocytosis did not occur using ceramide or phosphatidylcholine and was not due to GSL degradation because similar results were obtained using a nonhydrolyzable GSL analog. Stimulated caveolar endocytosis required src kinase and PKC-alpha activity as shown by i) use of pharmacological inhibitors, ii) expression of kinase inactive src or dominant negative PKCalpha, and iii) stimulation of src kinase activity upon addition of GSLs or cholesterol. These results suggest that caveolar endocytosis is regulated by a balance of caveolin-1, cholesterol, and GSLs at the plasma membrane.

摘要

一些质膜成分、细菌毒素和病毒通过小窝进行内化;然而,调节小窝内化的因素仍不清楚。在这里,我们证明用天然或合成糖鞘脂(GSL)对培养细胞进行短暂处理,或提高胆固醇水平(通过用甲基-β-环糊精/胆固醇急性处理或改变生长条件),可显著刺激小窝内吞作用,而对其他内吞机制几乎没有影响。这些处理还刺激了用小窝蛋白-1-GFP转染的细胞中GFP标记囊泡的移动,并减少了电子显微镜下可见的表面连接小窝的数量。相反,小窝蛋白-1的过表达降低了小窝摄取,但用GSL处理可逆转这种效应并刺激小窝内吞作用。使用神经酰胺或磷脂酰胆碱不会刺激小窝内吞作用,且这并非由于GSL降解,因为使用不可水解的GSL类似物可获得类似结果。如以下几点所示,刺激小窝内吞作用需要src激酶和PKC-α活性:i)使用药理抑制剂;ii)表达激酶失活的src或显性负性PKCα;iii)添加GSL或胆固醇后刺激src激酶活性。这些结果表明,小窝内吞作用受质膜上小窝蛋白-1、胆固醇和GSL平衡的调节。

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