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Localization to the Golgi complex of Uukuniemi virus glycoproteins G1 and G2 expressed from cloned cDNAs.

机译:定位到Uukuniemi病毒糖蛋白G1和G2的高尔基复合体该蛋白由克隆的cDNA表达。

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摘要

The membrane glycoproteins G1 and G2 of Uukuniemi virus, a bunyavirus, accumulate in the Golgi complex (GC) during virus infection. These proteins have therefore been considered to be good models for studying the intracellular transport to and retention in the GC. In this study, I have used indirect immunofluorescence to localize in COS cells the Uukuniemi virus glycoproteins G1 and G2 expressed together or separately from cloned cDNAs with use of simian virus 40-based vectors. When expressed together from the full-length cDNA, G1 and G2 were correctly translocated, processed, and targeted to the GC, indicating that the information for GC targeting resides in the proteins. When the proteins were expressed separately, G1 was transported to the GC and retained there. In contrast, G2 could not be detected in the GC but was most probably retained and finally degraded in the endoplasmic reticulum. However, in cells cotransfected with G1 and G2 cDNAs, the proteins could both again be found in the GC. These results suggest that G1 is a responsible for targeting to and retention of the Uukuniemi virus glycoproteins in the GC. G2 would thus accumulate in the GC by virtue of its binding to G1.
机译:Uukuniemi病毒(一种布尼亚病毒)的膜糖蛋白G1和G2在病毒感染期间积聚在高尔基体(GC)中。因此,这些蛋白质被认为是研究细胞内向GC转运和保留的良好模型。在这项研究中,我使用间接免疫荧光技术,以猿猴病毒40为基础的载体,将Uukuniemi病毒糖蛋白G1和G2与克隆的cDNA一起或分开表达,定位在COS细胞中。当从全长cDNA一起表达时,G1和G2正确转运,加工并靶向GC,表明GC靶向信息存在于蛋白质中。当蛋白质分别表达时,G1被转运到GC并保留在那里。相反,G2在GC中无法检测到,但最有可能保留并最终在内质网中降解。但是,在用G1和G2 cDNA共转染的细胞中,可以再次在GC中找到这些蛋白。这些结果表明,G1负责靶向Uukuniemi病毒糖蛋白并将其保留在GC中。因此,由于G2与G1的结合,G2将在GC中积累。

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