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新合成的膜蛋白从高尔基体复合体的反式潴泡转运至质膜。

Exit of newly synthesized membrane proteins from the trans cisterna of the Golgi complex to the plasma membrane.

作者信息

Griffiths G, Pfeiffer S, Simons K, Matlin K

出版信息

J Cell Biol. 1985 Sep;101(3):949-64. doi: 10.1083/jcb.101.3.949.

Abstract

The intracellular location at which the G protein of vesicular stomatitis virus accumulated when transport was blocked at 20 degrees C has been studied by biochemical, cytochemical, and immunocytochemical methods. Our results indicated that the viral G protein was blocked in that cisterna of the Golgi stack which stained for acid phosphatase. At 20 degrees C this trans cisterna became structurally altered by the accumulation of G protein. This alteration was characterized by extensive areas of membrane buds which were covered by a cytoplasmic coat. These coated structures were of two kinds--those that labeled with anti-clathrin antibodies and those that did not. The clathrin-coated pits consistently did not label with anti-G antibodies. Upon warming infected cells to 32 degrees C, G protein appeared on the surface within minutes. Concomitantly, the trans cisterna lost its characteristic structural organization. Double-labeling experiments were performed in which G protein localization was combined with staining for horseradish peroxidase, which had been taken up from the extracellular medium by endocytosis. The results suggest that the trans cisterna was distinct from the endosome compartment and that the latter was not an obligatory station in the route taken by G protein to the cell surface.

摘要

利用生化、细胞化学和免疫细胞化学方法,研究了在20℃阻断转运时水泡性口炎病毒G蛋白在细胞内的积聚位置。我们的结果表明,病毒G蛋白在高尔基体堆叠中对酸性磷酸酶染色的那个潴泡中被阻断。在20℃时,这个反式潴泡因G蛋白的积聚而发生结构改变。这种改变的特征是有大量被细胞质衣被覆盖的膜芽区域。这些有被结构有两种——那些用抗网格蛋白抗体标记的和那些未被标记的。网格蛋白包被小窝始终未用抗G抗体标记。将感染细胞升温至32℃后,G蛋白在几分钟内出现在细胞表面。与此同时,反式潴泡失去了其特征性的结构组织。进行了双重标记实验,将G蛋白定位与辣根过氧化物酶染色相结合,辣根过氧化物酶是通过内吞作用从细胞外培养基中摄取的。结果表明,反式潴泡与内体区室不同,并且后者不是G蛋白到达细胞表面所经过途径中的必经站点。

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