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Immunoelectron microscopic studies of the intracellular transport of the membrane glycoprotein (G) of vesicular stomatitis virus in infected Chinese hamster ovary cells

机译:感染性中国仓鼠卵巢细胞中水泡性口炎病毒膜糖蛋白(G)在细胞内转运的免疫电子显微镜研究

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摘要

An immunoelectron microscopic study was undertaken to survey the intracellular pathway taken by the integral membrane protein (G- protein) of vesicular stomatitis virus from its site of synthesis in the rough endoplasmic reticulum to the plasma membrane of virus- infected Chinese hamster ovary cells. Intracellular transport of the G- protein was synchronized by using a temperature-sensitive mutant of the virus (0-45). At the nonpermissive temperature (39.8 degrees C), the G- protein is synthesized in the cell infected with 0-45, but does not leave the rough endoplasmic reticulum. Upon shifting the temperature to 32 degrees C, the G-protein moves by stages to the plasma membrane. Ultrathin frozen sections of 0-45-infected cells were prepared and indirectly immunolabeled for the G-protein at different times after the temperature shift. By 3 min, the G-protein was seen at high density in saccules at one face of the Golgi apparatus. No large accumulation of G- protein-containing vesicles were observed near this entry face, but a few 50-70-mm electron-dense vesicular structures labeled for G-protein were observed that might be transfer vesicles between the rough endoplasmic reticulum and the Golgi complex. At blebbed sites on the nuclear envelope at these early times there was a suggestion that the G- protein was concentrated, these sites perhaps serving as some of the transitional elements for subsequent transfer of the G-protein from the rough endoplasmic reticulum to the Golgi complex. By 3 min after its initial asymmetric entry into the Golgi complex, the G-protein was uniformly distributed throughout all the saccules of the complex. At later times, after the G-protein left the Golgi complex and was on its way to the plasma membrane, a new class of G-protein-containing vesicles of approximately 200-nm diameter was observed that are probably involved in this stage of the transport process. These data are discussed, and the further prospects of this experimental approach are assessed.
机译:进行了免疫电子显微镜研究,以调查水泡性口腔炎病毒的整体膜蛋白(G蛋白)从其在粗糙内质网中的合成位点到感染了病毒的中国仓鼠卵巢细胞的质膜所采取的细胞内途径。通过使用病毒的温度敏感突变体(0-45)同步G蛋白的细胞内运输。在不允许的温度(39.8摄氏度)下,G蛋白在被0-45感染的细胞中合成,但不会离开粗糙的内质网。将温度转移到32摄氏度后,G蛋白逐步移至质膜。制备了0-45感染细胞的超薄冷冻切片,并在温度变化后的不同时间间接免疫标记了G蛋白。到3分钟时,在高尔基体的一侧面上的囊中高密度地看到了G蛋白。在该进入面附近未观察到大量含G蛋白的囊泡积聚,但观察到一些标记有G蛋白的50-70 mm电子致密囊泡结构,可能是粗糙内质网与高尔基体之间的转移囊泡复杂。在这些早期的核膜上起泡的部位,有人暗示G蛋白集中,这些部位可能是随后G蛋白从粗糙的内质网转移到高尔基体的一些过渡元素。 。最初不对称进入高尔基复合体后3分钟,G蛋白均匀分布在复合体的所有囊泡中。后来,在G蛋白离开高尔基体并进入质膜的途中,观察到一类新的大约200 nm直径的含G蛋白的囊泡,可能参与了这一阶段。运输过程。讨论了这些数据,并对这种实验方法的进一步前景进行了评估。

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