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Golgi localization of ERManI defines spatial separation of the mammalian glycoprotein quality control system

机译:ERManI的高尔基体定位定义了哺乳动物糖蛋白质量控制系统的空间分离

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The Golgi complex has been implicated as a possible component of endoplasmic reticulum (ER) glycoprotein quality control, although the elucidation of its exact role is lacking. ERManI, a putative ER resident mannosidase, plays a rate-limiting role in generating a signal that targets misfolded N-linked glycoproteins for ER-associated degradation (ERAD). Herein we demonstrate that the endogenous human homologue predominantly resides in the Golgi complex, where it is subjected to O-glycosylation. To distinguish the intracellular site where the glycoprotein ERAD signal is generated, a COPI-binding motif was appended to the N terminus of the recombinant protein to facilitate its retrograde translocation back to the ER. Partial redistribution of the modified ERManI was observed along with an accelerated rate at which N-linked glycans of misfolded α1-antitrypsin variant NHK were trimmed. Despite these observations, the rate of NHK degradation was not accelerated, implicating the Golgi complex as the site for glycoprotein ERAD substrate tagging. Taken together, these data provide a potential mechanistic explanation for the spatial separation by which glycoprotein quality control components operate in mammalian cells.
机译:高尔基复合体被认为是内质网(ER)糖蛋白质量控制的可能组成部分,尽管尚不清楚其确切作用。 ERManI,一种假定的ER驻留甘露糖苷酶,在产生信号中发挥限速作用,该信号靶向与ER相关的降解(ERAD)的错误折叠的N-连接糖蛋白。在本文中,我们证明内源性人类同源物主要存在于高尔基体中,在该处进行O-糖基化。为了区分产生糖蛋白ERAD信号的细胞内位点,将COPI结合基序附加到重组蛋白的N末端,以促进其逆行易位回到ER。观察到修饰的ERManI的部分重新分布,以及修剪掉折叠错误的α1-抗胰蛋白酶变体NHK的N-连接聚糖的加速速率。尽管有这些观察结果,但NHK降解的速度并未加快,这暗示高尔基复合体是糖蛋白ERAD底物标签的位点。总之,这些数据为糖蛋白质量控制成分在哺乳动物细胞中发挥作用的空间分离提供了潜在的机理解释。

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