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敲除 RSN1、TVP18 或 CSC1-2 会导致毕赤酵母高尔基体潴泡结构紊乱。

Knockout of RSN1, TVP18 or CSC1-2 causes perturbation of Golgi cisternae in Pichia pastoris.

机构信息

Department of Chemical Engineering, Imperial College London, London, UK.

Imperial College Centre for Synthetic Biology, Imperial College London, London, United Kingdom.

出版信息

Traffic. 2021 Mar;22(3):48-63. doi: 10.1111/tra.12773. Epub 2020 Dec 12.

Abstract

The structural organization of the Golgi stacks in mammalian cells is intrinsically linked to function, including glycosylation, but the role of morphology is less clear in lower eukaryotes. Here we investigated the link between the structural organization of the Golgi and secretory pathway function using Pichia pastoris as a model system. To unstack the Golgi cisternae, we disrupted 18 genes encoding proteins in the secretory pathway without loss of viability. Using biosensors, confocal microscopy and transmission electron microscopy we identified three strains with irreversible perturbations in the stacking of the Golgi cisternae, all of which had disruption in genes that encode proteins with annotated function as or homology to calcium/calcium permeable ion channels. Despite this, no variation in the secretory pathway for ER size, whole cell glycomics or recombinant protein glycans was observed. Our investigations showed the robust nature of the secretory pathway in P. pastoris and suggest that Ca concentration, homeostasis or signalling may play a significant role for Golgi stacking in this organism and should be investigated in other organisms.

摘要

哺乳动物细胞中高尔基体堆叠的结构组织与功能(包括糖基化)密切相关,但在较低等真核生物中,形态的作用还不太清楚。在这里,我们使用巴斯德毕赤酵母(Pichia pastoris)作为模型系统,研究了高尔基体结构组织与分泌途径功能之间的联系。为了去堆叠高尔基体潴泡,我们敲除了 18 个编码分泌途径中蛋白质的基因,而细胞没有失去活力。使用生物传感器、共聚焦显微镜和透射电子显微镜,我们鉴定了三株高尔基体潴泡堆叠不可逆扰动的菌株,它们都敲除了编码具有钙/钙渗透性离子通道注释功能或同源性的蛋白质的基因。尽管如此,内质网大小、全细胞糖组学或重组蛋白聚糖的分泌途径没有观察到变化。我们的研究表明,巴斯德毕赤酵母的分泌途径具有很强的稳健性,并表明 Ca 浓度、动态平衡或信号转导可能在该生物体的高尔基体堆叠中发挥重要作用,应该在其他生物体中进行研究。

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