植入到Madin-Darby犬肾细胞顶端质膜中的病毒膜糖蛋白的跨上皮运输。II. 免疫定量分析。
Transepithelial transport of a viral membrane glycoprotein implanted into the apical plasma membrane of Madin-Darby canine kidney cells. II. Immunological quantitation.
作者信息
Pesonen M, Simons K
出版信息
J Cell Biol. 1983 Sep;97(3):638-43. doi: 10.1083/jcb.97.3.638.
Abstract
The envelope of vesicular stomatitis virus was fused with the apical plasma membrane of Madin-Darby canine kidney cells by low pH treatment. The fate of the implanted G protein was then followed using a protein A-binding assay, which was designed to quantitate the amount of G protein in the apical and the basolateral membranes. The implanted G protein was rapidly internalized at 31 degrees C, whereas at 10 degrees C no uptake was observed. Already after 15 min at 31 degrees C, a fraction of the G protein could be detected at the basolateral membrane. After 60 min 25-48% of the G protein was basolateral as measured by the protein A-binding assay. At the same time, 25-33% of the implanted G protein was detected at the apical membrane. Internalization of G protein was not affected by 20 mM ammonium chloride or by 10 microM monensin. However, the endocytosed G protein accumulated in intracellular vacuoles and redistribution back to the plasma membrane was inhibited. We conclude that the implanted G protein was rapidly internalized from the apical surface of Madin-Darby canine kidney cells and a major fraction was routed to the basolateral domain.
摘要
通过低pH处理,水疱性口炎病毒的包膜与Madin-Darby犬肾细胞的顶端质膜融合。然后使用蛋白A结合测定法追踪植入的G蛋白的命运,该测定法旨在定量顶端膜和基底外侧膜中G蛋白的量。植入的G蛋白在31℃时迅速内化,而在10℃时未观察到摄取。在31℃下仅15分钟后,就可以在基底外侧膜中检测到一部分G蛋白。通过蛋白A结合测定法测量,60分钟后,25%-48%的G蛋白位于基底外侧。与此同时,在顶端膜中检测到25%-33%的植入G蛋白。G蛋白的内化不受20 mM氯化铵或10 microM莫能菌素的影响。然而,内吞的G蛋白积聚在细胞内液泡中,并且其重新分布回到质膜的过程受到抑制。我们得出结论,植入的G蛋白从Madin-Darby犬肾细胞的顶端表面迅速内化,并且大部分被转运到基底外侧结构域。
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