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鉴定多泡体为烟草BY-2细胞中的前液泡区室。

Identification of multivesicular bodies as prevacuolar compartments in Nicotiana tabacum BY-2 cells.

作者信息

Tse Yu Chung, Mo Beixin, Hillmer Stefan, Zhao Min, Lo Sze Wan, Robinson David G, Jiang Liwen

机构信息

Department of Biology, Chinese University of Hong Kong, Shatin, New Territories, Hong Kong, China.

出版信息

Plant Cell. 2004 Mar;16(3):672-93. doi: 10.1105/tpc.019703. Epub 2004 Feb 18.

Abstract

Little is known about the dynamics and molecular components of plant prevacuolar compartments (PVCs). We have demonstrated recently that vacuolar sorting receptor (VSR) proteins are concentrated on PVCs. In this study, we generated transgenic Nicotiana tabacum (tobacco) BY-2 cell lines expressing two yellow fluorescent protein (YFP)-fusion reporters that mark PVC and Golgi organelles. Both transgenic cell lines exhibited typical punctate YFP signals corresponding to distinct PVC and Golgi organelles because the PVC reporter colocalized with VSR proteins, whereas the Golgi marker colocalized with mannosidase I in confocal immunofluorescence. Brefeldin A induced the YFP-labeled Golgi stacks but not the YFP-marked PVCs to form typical enlarged structures. By contrast, wortmannin caused YFP-labeled PVCs but not YFP-labeled Golgi stacks to vacuolate. VSR antibodies labeled multivesicular bodies (MVBs) on thin sections prepared from high-pressure frozen/freeze substituted samples, and the enlarged PVCs also were indentified as MVBs. MVBs were further purified from BY-2 cells and found to contain VSR proteins via immunogold negative staining. Similar to YFP-labeled Golgi stacks, YFP-labeled PVCs are mobile organelles in BY-2 cells. Thus, we have unequivocally identified MVBs as PVCs in N. tabacum BY-2 cells. Uptake studies with the styryl dye FM4-64 strongly indicate that PVCs also lie on the endocytic pathway of BY-2 cells.

摘要

关于植物前液泡区室(PVCs)的动态变化和分子成分,我们所知甚少。我们最近已证明液泡分选受体(VSR)蛋白集中在PVCs上。在本研究中,我们构建了表达两种黄色荧光蛋白(YFP)融合报告基因的转基因烟草(Nicotiana tabacum)BY - 2细胞系,这两种报告基因分别标记PVC和高尔基体细胞器。两种转基因细胞系均呈现出对应于不同PVC和高尔基体细胞器的典型点状YFP信号,因为在共聚焦免疫荧光中,PVC报告基因与VSR蛋白共定位,而高尔基体标记物与甘露糖苷酶I共定位。布雷菲德菌素A诱导YFP标记的高尔基体堆叠形成典型的扩大结构,但未诱导YFP标记的PVCs形成。相反,渥曼青霉素使YFP标记的PVCs产生液泡化,但未使YFP标记的高尔基体堆叠产生液泡化。VSR抗体在由高压冷冻/冷冻置换样品制备的薄切片上标记了多泡体(MVBs),并且扩大的PVCs也被鉴定为MVBs。从BY - 2细胞中进一步纯化MVBs,并通过免疫金负染色发现其含有VSR蛋白。与YFP标记的高尔基体堆叠类似,YFP标记的PVCs在BY - 2细胞中是可移动的细胞器。因此,我们已明确在烟草BY - 2细胞中将MVBs鉴定为PVCs。用苯乙烯基染料FM4 - 64进行的摄取研究强烈表明,PVCs也位于BY - 2细胞的内吞途径上。

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