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利用拟南芥幼苗的高通量瞬时转化对蛋白质亚细胞定位和相互作用进行系统分析。

Systematic analysis of protein subcellular localization and interaction using high-throughput transient transformation of Arabidopsis seedlings.

作者信息

Marion Jessica, Bach Lien, Bellec Yannick, Meyer Christian, Gissot Lionel, Faure Jean-Denis

机构信息

Laboratoire Biologie Cellulaire, Institute Jean-Pierre Bourgin, INRA, 78000 Versailles, France.

出版信息

Plant J. 2008 Oct;56(1):169-79. doi: 10.1111/j.1365-313X.2008.03596.x. Epub 2008 Jul 4.

DOI:10.1111/j.1365-313X.2008.03596.x
PMID:18643979
Abstract

The functional genomics approach requires systematic analysis of protein subcellular distribution and interaction networks, preferably by optimizing experimental simplicity and physiological significance. Here, we present an efficient in planta transient transformation system that allows single or multiple expression of constructs containing various fluorescent protein tags in Arabidopsis cotyledons. The optimized protocol is based on vacuum infiltration of agrobacteria directly into young Arabidopsis seedlings. We demonstrate that Arabidopsis epidermal cells show a subcellular distribution of reference markers similar to that in tobacco epidermal cells, and can be used for co-localization or bi-molecular fluorescent complementation studies. We then used this new system to investigate the subcellular distribution of enzymes involved in sphingolipid metabolism. In contrast to transformation systems using tobacco epidermal cells or cultured Arabidopsis cells, our system provides the opportunity to take advantage of the extensive collections of mutant and transgenic lines available in Arabidopsis. The fact that this assay uses conventional binary vectors and a conventional Agrobacterium strain, and is compatible with a large variety of fluorescent tags, makes it a versatile tool for construct screening and characterization before stable transformation. Transient expression in Arabidopsis seedlings is thus a fast and simple method that requires minimum handling and potentially allows medium- to high-throughput analyses of fusion proteins harboring fluorescent tags in a whole-plant cellular context.

摘要

功能基因组学方法需要对蛋白质亚细胞分布和相互作用网络进行系统分析,最好通过优化实验的简易性和生理意义来实现。在此,我们展示了一种高效的植物体内瞬时转化系统,该系统可在拟南芥子叶中实现含有各种荧光蛋白标签的构建体的单表达或多表达。优化后的方案基于将农杆菌直接真空渗入年轻的拟南芥幼苗。我们证明,拟南芥表皮细胞显示出与烟草表皮细胞中类似的参考标记的亚细胞分布,并且可用于共定位或双分子荧光互补研究。然后,我们使用这个新系统来研究参与鞘脂代谢的酶的亚细胞分布。与使用烟草表皮细胞或培养的拟南芥细胞的转化系统不同,我们的系统提供了利用拟南芥中现有的大量突变体和转基因品系的机会。该检测方法使用常规二元载体和常规农杆菌菌株,并且与多种荧光标签兼容,这一事实使其成为稳定转化前构建体筛选和表征的通用工具。因此,拟南芥幼苗中的瞬时表达是一种快速且简单的方法,需要最少的操作,并且有可能在全植物细胞环境中对携带荧光标签的融合蛋白进行中到高通量分析。

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