Wang Yanzhuang, Wei Jen-Hsuan, Bisel Blaine, Tang Danming, Seemann Joachim
Department of Molecular, Cellular and Developmental Biology, University of Michigan, Ann Arbor, Michigan, USA.
PLoS One. 2008 Feb 20;3(2):e1647. doi: 10.1371/journal.pone.0001647.
The Golgi apparatus in mammalian cells is composed of flattened cisternae that are densely packed to form stacks. We have used the Golgi stacking protein GRASP65 as a tool to modify the stacking state of Golgi cisternae. We established an assay to measure protein transport to the cell surface in post-mitotic cells in which the Golgi was unstacked. Cells with an unstacked Golgi showed a higher transport rate compared to cells with stacked Golgi membranes. Vesicle budding from unstacked cisternae in vitro was significantly increased compared to stacked membranes. These results suggest that Golgi cisternal stacking can directly regulate vesicle formation and thus the rate of protein transport through the Golgi. The results further suggest that at the onset of mitosis, unstacking of cisternae allows extensive and rapid vesiculation of the Golgi in preparation for its subsequent partitioning.
哺乳动物细胞中的高尔基体由扁平的潴泡组成,这些潴泡紧密堆积形成堆叠结构。我们利用高尔基体堆叠蛋白GRASP65作为工具来改变高尔基体潴泡的堆叠状态。我们建立了一种检测方法,用于测量有丝分裂后细胞中蛋白质向细胞表面的转运,其中高尔基体处于非堆叠状态。与高尔基体膜堆叠的细胞相比,高尔基体非堆叠的细胞显示出更高的转运速率。与堆叠膜相比,体外从未堆叠潴泡出芽的囊泡显著增加。这些结果表明,高尔基体潴泡堆叠可直接调节囊泡形成,从而调节蛋白质通过高尔基体的转运速率。结果还进一步表明,在有丝分裂开始时,潴泡的非堆叠使高尔基体能够广泛而快速地形成囊泡,为其随后的分配做准备。
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