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活植物细胞中磷脂酰肌醇-3-磷酸(PtdIns3P)动力学的可视化。

Visualization of PtdIns3P dynamics in living plant cells.

作者信息

Vermeer Joop E M, van Leeuwen Wessel, Tobeña-Santamaria Rafa, Laxalt Ana M, Jones David R, Divecha Nullin, Gadella Theodorus W J, Munnik Teun

机构信息

Section of Molecular Cytology, Swammerdam Institute for Life Sciences, University of Amsterdam, Kruislaan 316, Amsterdam, The Netherlands.

出版信息

Plant J. 2006 Sep;47(5):687-700. doi: 10.1111/j.1365-313X.2006.02830.x. Epub 2006 Jul 19.

DOI:10.1111/j.1365-313X.2006.02830.x
PMID:16856980
Abstract

To investigate PtdIns3P localization and function in plants, a fluorescent PtdIns3P-specific biosensor (YFP-2xFYVE) was created. On lipid dot blots it bound specifically and with high affinity to PtdIns3P. Transient expression in cowpea protoplasts labelled vacuolar membranes and highly motile structures undergoing fusion and fission. Stable expression in tobacco BY-2 cells labelled similar motile structures, but labelled vacuolar membranes hardly at all. YFP-2xFYVE fluorescence strongly co-localized with the pre-vacuolar marker AtRABF2b, partially co-localized with the endosomal tracer FM4-64, but showed no overlap with the Golgi marker STtmd-CFP. Treatment of cells with wortmannin, a PI3 kinase inhibitor, caused the YFP-2xFYVE fluorescence to redistribute into the cytosol and nucleus within 15 min. BY-2 cells expressing YFP-2xFYVE contained twice as much PtdIns3P as YFP-transformed cells, but this had no effect on cell-growth or stress-induced phospholipid signalling responses. Upon treatment with wortmannin, PtdIns3P levels were reduced by approximately 40% within 15 min in both cell lines. Stable expression of YFP-2xFYVE in Arabidopsis plants labelled different subcellular structures in root compared with shoot tissues. In addition labelling the motile structures common to all cells, YFP-2xFYVE strongly labelled the vacuolar membrane in leaf epidermal and guard cells, suggesting that cell differentiation alters the distribution of PtdIns3P. In dividing BY-2 cells, YFP-2xFYVE-labelled vesicles surrounded the newly formed cell plate, suggesting a role for PtdIns3P in cytokinesis. Together, these data show that YFP-2xFYVE may be used as a biosensor to specifically visualize PtdIns3P in living plant cells.

摘要

为了研究磷脂酰肌醇-3-磷酸(PtdIns3P)在植物中的定位和功能,构建了一种荧光PtdIns3P特异性生物传感器(YFP-2xFYVE)。在脂质斑点印迹上,它与PtdIns3P特异性且高亲和力地结合。在豇豆原生质体中的瞬时表达标记了液泡膜以及经历融合和裂变的高度动态结构。在烟草BY-2细胞中的稳定表达标记了类似的动态结构,但几乎没有标记液泡膜。YFP-2xFYVE荧光与液泡前体标记物AtRABF2b强烈共定位,与内体示踪剂FM4-64部分共定位,但与高尔基体标记物STtmd-CFP没有重叠。用PI3激酶抑制剂渥曼青霉素处理细胞,导致YFP-2xFYVE荧光在15分钟内重新分布到细胞质和细胞核中。表达YFP-2xFYVE的BY-2细胞中PtdIns3P的含量是表达YFP的细胞的两倍,但这对细胞生长或应激诱导的磷脂信号反应没有影响。用渥曼青霉素处理后,两种细胞系中的PtdIns3P水平在15分钟内均降低了约40%。与地上组织相比,YFP-2xFYVE在拟南芥植物中的稳定表达标记了根部不同的亚细胞结构。除了标记所有细胞共有的动态结构外,YFP-2xFYVE还强烈标记了叶表皮和保卫细胞中的液泡膜,表明细胞分化改变了PtdIns3P的分布。在分裂的BY-2细胞中,YFP-2xFYVE标记的囊泡围绕着新形成的细胞板,表明PtdIns3P在胞质分裂中起作用。总之,这些数据表明YFP-2xFYVE可作为一种生物传感器,用于在活植物细胞中特异性地可视化PtdIns3P。

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