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Transepithelial transport of a viral membrane glycoprotein implanted into the apical plasma membrane of Madin-Darby canine kidney cells. I. Morphological evidence

机译:病毒膜糖蛋白的跨上皮运输,被植入Madin-Darby犬肾细胞的顶质膜。一,形态学证据

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摘要

The G protein of vesicular stomatitis virus was implanted in the apical plasma membrane of Madin-Darby canine kidney cells by low pH-dependent fusion of the viral envelope with the cellular membrane. The amount of fusion as determined by removal of unfused virions, either by tryptic digestion or by EDTA treatment at 0 degree C, was 22-24% of the cell- bound virus radioactivity. Upon incubation of cells after implantation, the amount of G protein as detected by immunofluorescence diminished on the apical membrane and appeared within 30 min on the basolateral membrane. At the same time some G protein fluorescence was also seen in intracellular vacuoles. The observations by immunofluorescence were confirmed and extended by electron microscopy. Using immunoperoxidase localization, G protein was seen to move into irregularly shaped vacuoles (endosomes) and multivesicular bodies and to appear on the basolateral plasma membrane. These results suggest that the apical and basolateral domains of Madin-Darby canine kidney cells are connected by an intracellular route.
机译:通过病毒包膜与细胞膜的低pH依赖性融合,将水泡性口腔炎病毒的G蛋白植入Madin-Darby犬肾细胞的顶质膜。通过胰蛋白酶消化或在0℃下通过EDTA处理去除未融合的病毒体而确定的融合量为细胞结合病毒放射性的22-24%。植入后孵育细胞后,通过免疫荧光检测到的G蛋白量在顶膜上减少,并在30分钟内出现在基底外侧膜上。同时,在细胞内液泡中也观察到一些G蛋白荧光。通过免疫荧光的观察得到证实并通过电子显微镜进行了扩展。使用免疫过氧化物酶定位,可以看到G蛋白移动到不规则形状的液泡(内体)和多囊泡体中,并出现在基底外侧质膜上。这些结果表明,Madin-Darby犬肾细胞的顶端和基底外侧结构域通过细胞内途径连接。

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  • 年度 1983
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