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Knockout of the Golgi stacking proteins GRASP55 and GRASP65 impairs Golgi structure and function

机译:高尔基体堆积蛋白GRASP55和GRASP65的敲除削弱了高尔基体的结构和功能

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摘要

Golgi reassembly stacking protein of 65 kDa (GRASP65) and Golgi reassembly stacking protein of 55 kDa (GRASP55) were originally identified as Golgi stacking proteins; however, subsequent GRASP knockdown experiments yielded inconsistent results with respect to the Golgi structure, indicating a limitation of RNAi-based depletion. In this study, we have applied the recently developed clustered regularly interspaced short palindromic repeats (CRISPR)/Cas9 technology to knock out GRASP55 and GRASP65, individually or in combination, in HeLa and HEK293 cells. We show that double knockout of GRASP proteins disperses the Golgi stack into single cisternae and tubulovesicular structures, accelerates protein trafficking, and impairs accurate glycosylation of proteins and lipids. These results demonstrate a critical role for GRASPs in maintaining the stacked structure of the Golgi, which is required for accurate posttranslational modifications in the Golgi. Additionally, the GRASP knockout cell lines developed in this study will be useful tools for studying the role of GRASP proteins in other important cellular processes.
机译:高尔基体堆积蛋白65 kDa(GRASP65)和高尔基体堆积蛋白55 kDa(GRASP55)最初被鉴定为高尔基体堆积蛋白。然而,随后的GRASP敲低实验在高尔基体结构方面得出的结果不一致,表明基于RNAi的耗竭受到限制。在这项研究中,我们应用了最近开发的簇状规则间隔的短回文重复序列(CRISPR)/ Cas9技术,在HeLa和HEK293细胞中单独或联合敲除GRASP55和GRASP65。我们表明,GRASP蛋白质的双重敲除将高尔基体堆栈分散成单个的水箱和微管小体结构,加速蛋白质的运输,并损害蛋白质和脂质的准确糖基化。这些结果证明了GRASP在维持高尔基体的堆叠结构中的关键作用,这是高尔基体中准确的翻译后修饰所必需的。此外,在这项研究中开发的GRASP基因敲除细胞系将是研究GRASP蛋白在其他重要细胞过程中的作用的有用工具。

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