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拟南芥肌球蛋白相关蛋白 DRP2B 和 DRP1A 共同参与胞吞作用中网格蛋白包被小泡的形成。

Arabidopsis dynamin-related proteins DRP2B and DRP1A participate together in clathrin-coated vesicle formation during endocytosis.

机构信息

Laboratory of Plant Molecular Genetics, Graduate School of Agricultural and Life Sciences, University of Tokyo, 1-1-1 Yayoi, Bunkyo-ku, Tokyo 113-8657, Japan.

出版信息

Proc Natl Acad Sci U S A. 2010 Mar 30;107(13):6094-9. doi: 10.1073/pnas.0913562107. Epub 2010 Mar 15.

Abstract

Endocytosis performs a wide range of functions in animals and plants. Clathrin-coated vesicle (CCV) formation is an initial step of endocytosis, and in animal cells is largely achieved by dynamins. However, little is known of its molecular mechanisms in plant cells. To identify dynamin-related proteins (DRPs) involved in endocytic CCV formation in plant cells, we compared the behaviors of two structurally different Arabidopsis DRPs, DRP2B and DRP1A, with those of the clathrin light chain (CLC), a marker of CCVs, at the plasma membrane by variable incidence angle fluorescent microscopy (VIAFM). DRP2B shares domain organization with animal dynamins whereas DRP1A is plant-specific. We show that green fluorescent protein (GFP)-tagged DRP2B and DRP1A colocalized with CLC tagged with monomeric Kusabira Orange (mKO) in Arabidopsis cultured cells. Time-lapse VIAFM observations suggested that both GFP-DRP2B and GFP-DRP1A appeared and accumulated on the existing mKO-CLC foci and disappeared at the same time as or immediately after the disappearance of mKO-CLC. Moreover, DRP2B and DRP1A colocalized and assembled/disassembled together at the plasma membrane in Arabidopsis cells. A yeast two-hybrid assay showed that DRP2B and DRP1A interacted with each other. An inhibitor of clathrin-mediated endocytosis, tyrphostin A23, disturbed the localization of DRP1A, but had little effect on the localization of DRP2B, indicating that DRP1A and DRP2B have different molecular properties. These results suggest that DRP2B and DRP1A participate together in endocytic CCV formation in Arabidopsis cells despite the difference of their molecular properties.

摘要

内吞作用在动物和植物中发挥着广泛的功能。网格蛋白包被小泡(CCV)的形成是内吞作用的初始步骤,在动物细胞中主要由动力蛋白完成。然而,植物细胞中内吞 CCV 形成的分子机制知之甚少。为了鉴定参与植物细胞内吞 CCV 形成的与动力蛋白相关的蛋白(DRPs),我们通过可变入射角荧光显微镜(VIAFM)比较了两种结构不同的拟南芥 DRP,DRP2B 和 DRP1A,与质膜上的网格蛋白轻链(CLC)的行为,CLC 是 CCV 的标志物。DRP2B 与动物动力蛋白具有相同的结构域组织,而 DRP1A 是植物特异性的。我们表明,绿色荧光蛋白(GFP)标记的 DRP2B 和 DRP1A 与单体 Kusabira Orange(mKO)标记的 CLC 在拟南芥培养细胞中共定位。延时 VIAFM 观察表明,GFP-DRP2B 和 GFP-DRP1A 都出现在并积累在现有的 mKO-CLC 焦点上,并在 mKO-CLC 消失的同时或立即消失。此外,DRP2B 和 DRP1A 在拟南芥细胞的质膜上共定位并组装/解组装。酵母双杂交测定表明 DRP2B 和 DRP1A 相互作用。一种网格蛋白介导的内吞作用抑制剂 tyrphostin A23 扰乱了 DRP1A 的定位,但对 DRP2B 的定位几乎没有影响,这表明 DRP1A 和 DRP2B 具有不同的分子特性。这些结果表明,尽管分子特性不同,但 DRP2B 和 DRP1A 共同参与了拟南芥细胞内吞 CCV 的形成。

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