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单个分子分析 PIP2;1 动力学和分配揭示了拟南芥质膜水通道调节的多种模式。

Single-molecule analysis of PIP2;1 dynamics and partitioning reveals multiple modes of Arabidopsis plasma membrane aquaporin regulation.

机构信息

Key Laboratory of Plant Molecular Physiology, Institute of Botany, Chinese Academy of Sciences, Beijing 100093, China.

出版信息

Plant Cell. 2011 Oct;23(10):3780-97. doi: 10.1105/tpc.111.091454. Epub 2011 Oct 18.

Abstract

PIP2;1 is an integral membrane protein that facilitates water transport across plasma membranes. To address the dynamics of Arabidopsis thaliana PIP2;1 at the single-molecule level as well as their role in PIP2;1 regulation, we tracked green fluorescent protein-PIP2;1 molecules by variable-angle evanescent wave microscopy and fluorescence correlation spectroscopy (FCS). Single-particle tracking analysis revealed that PIP2;1 presented four diffusion modes with large dispersion of diffusion coefficients, suggesting that partitioning and dynamics of PIP2;1 are heterogeneous and, more importantly, that PIP2;1 can move into or out of membrane microdomains. In response to salt stress, the diffusion coefficients and percentage of restricted diffusion increased, implying that PIP2;1 internalization was enhanced. This was further supported by the decrease in PIP2;1 density on plasma membranes by FCS. We additionally demonstrated that PIP2;1 internalization involves a combination of two pathways: a tyrphostin A23-sensitive clathrin-dependent pathway and a methyl-β-cyclodextrin-sensitive, membrane raft-associated pathway. The latter was efficiently stimulated under NaCl conditions. Taken together, our findings demonstrate that PIP2;1 molecules are heterogeneously distributed on the plasma membrane and that clathrin and membrane raft pathways cooperate to mediate the subcellular trafficking of PIP2;1, suggesting that the dynamic partitioning and recycling pathways might be involved in the multiple modes of regulating water permeability.

摘要

PIP2;1 是一种整合膜蛋白,可促进质膜的水转运。为了在单分子水平上解决拟南芥 PIP2;1 的动力学及其在 PIP2;1 调节中的作用,我们通过可变角消逝波显微镜和荧光相关光谱(FCS)跟踪绿色荧光蛋白-PIP2;1 分子。单粒子跟踪分析表明,PIP2;1 呈现出四种扩散模式,扩散系数的分散性较大,这表明 PIP2;1 的分配和动力学是不均匀的,更重要的是,PIP2;1 可以进入或离开膜微区。响应盐胁迫时,扩散系数和受限扩散的百分比增加,表明 PIP2;1 内化增强。这通过 FCS 进一步证实了质膜上 PIP2;1 密度的降低。我们还证明了 PIP2;1 内化涉及两种途径的结合:氯高铁血红素 A23 敏感的网格蛋白依赖性途径和甲基-β-环糊精敏感的膜筏相关途径。在后一种途径中,在 NaCl 条件下能有效地被刺激。总之,我们的研究结果表明,PIP2;1 分子在质膜上呈不均匀分布,网格蛋白和膜筏途径共同介导 PIP2;1 的亚细胞运输,这表明动态分配和回收途径可能参与了水通透性的多种调节模式。

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