植物向重力反应中PIN-FORMED介导的生长素极性运输调控

植物的向性,即植物对光或重力等环境刺激信号产生的定向生长反应。在向重力性反应中,植物器官将重力感知为定向环境信号,来控制其器官的生长方向以促进生存。植物激素生长素及其极性运输在植物向重力反应中起着决定性的调控作用。质膜定位的生长素输出蛋白PIN-FORMED(PIN)通过动态的亚细胞极性定位,改变生长素运输的方向以响应环境刺激,由此植物器官间建立的生长素浓度梯度是细胞差异化伸长和器官弯曲的基础,来调控植物的形态建成和生长发育过程。本文主要讨论发生在植物重力感受细胞内早期重力感知和信号转导机制的最新研究进展、PIN介导的生长素极性运输、PIN的极性定位以及质膜蛋白丰度的调控机制等。     

生长素输出载体PIN家族研究进展

生长素极性运输调控植物的生长发育。生长素极性运输主要依赖3类转运蛋白: AUX/LAX、PIN和ABCB蛋白家族。生长素在细胞间流动的方向与PIN蛋白在细胞上的极性定位密切相关。PIN蛋白由1个中心亲水环和2个由中心亲水环隔开的疏水区组成。中心亲水环上含多个磷酸化位点, 其为一些蛋白激酶的靶点。PIN蛋白受多方面调控, 包括转录调控、转录后修饰以及胞内循环与降解, 以响应内源和外源信号。目前, 利用全基因组测序方法在禾谷类作物水稻(Oryza sativa)、玉米(Zea mays)和高粱(Sorghum bicolor)中分别鉴定出12、15和11个PIN基因, 但仅有少数PIN基因的功能被报道。该文从蛋白结构、活性调控和功能验证等方面综述了PIN蛋白在拟南芥(Arabidopsis thaliana)和禾谷类作物中的研究进展, 以期为探究PIN蛋白家族介导的生长素极性运输过程提供新的思路与线索。     

ABI4调控侧根发育研究(综述)

生长素是调控植物侧根发育的关键植物激素,生长素运输载体PIN蛋白介导其极性分布。ABI4抑制生长素极性运输蛋白基因PIN1的表达,影响生长素的极性运输,抑制侧根形成。本文概述ABI4转录因子调控侧根发育的研究进展。     

植物ABCB亚家族生物学功能研究进展

ABC转运蛋白超家族结构和功能复杂多样, 包含ABCA-ABCH八个亚家族。ABCB是ABC转运蛋白的一个亚家族, 多数定位于质膜, 少数定位于线粒体膜或叶绿体膜。ABCB与其它生长素转运蛋白(AUX1/LAX、PIN)共同参与调控植物生长素的极性运输, 在植物生长发育的各个阶段发挥作用。此外, ABCB转运蛋白还调控植物的向性运动和重金属抗性等过程。近年来, 随着越来越多植物全基因组测序的完成, ABCB亚家族在禾谷类单子叶植物水稻(Oryza sativa)、玉米(Zea mays)和高粱(Sorghum bicolor)中的生物学功能开始有少量报道, 然而多数ABCB转运蛋白的功能尚未得到阐释。该文对拟南芥(Arabidopsis thaliana)和禾谷类作物ABCB转运蛋白的研究进展进行综述, 以期为全面揭示ABCB亚家族生物学功能提供线索。     

植物ABCB亚家族生物学功能研究进展

ABC转运蛋白超家族结构和功能复杂多样, 包含ABCA-ABCH八个亚家族。ABCB是ABC转运蛋白的一个亚家族, 多数定位于质膜, 少数定位于线粒体膜或叶绿体膜。ABCB与其它生长素转运蛋白(AUX1/LAX、PIN)共同参与调控植物生长素的极性运输, 在植物生长发育的各个阶段发挥作用。此外, ABCB转运蛋白还调控植物的向性运动和重金属抗性等过程。近年来, 随着越来越多植物全基因组测序的完成, ABCB亚家族在禾谷类单子叶植物水稻(Oryza sativa)、玉米(Zea mays)和高粱(Sorghum bicolor)中的生物学功能开始有少量报道, 然而多数ABCB转运蛋白的功能尚未得到阐释。该文对拟南芥(Arabidopsis thaliana)和禾谷类作物ABCB转运蛋白的研究进展进行综述, 以期为全面揭示ABCB亚家族生物学功能提供线索。     

2011年第9期《遗传》封面说明

生长素浓度梯度对生长素调控植物胚胎和器官发育、向地性和向光性生长等具有重要作用。生长素浓度梯度的形成依赖于生长素的极性运输。生长素极性运输主要由极性定位于细胞膜上的输出载体PIN(pin-formed family)家族蛋白     

植物生长素极性运输调控机理的研究进展

生长素极性运输特异地调控植物器官发生、发育和向性反应等生理过程。本文综述和分析了生长素极性运输的调控机制。分子遗传和生理学研究证明极性运输这一过程是由生长素输入载体和输出载体活性控制的。小G蛋白ARF附属蛋白GEF和GAP分别调控输出载体(PIN1)和输入载体(AUX1)的定位和活性, 并影响高尔基体等介导的细胞囊泡运输系统, 小G蛋白ROP也参与输出载体PIN2活性的调节。本 文基于作者的研究工作提出小G蛋白在调控生长素极性运输中的可能作用模式。     

Leukamenin E调节拟南芥幼苗根部生长素极性运输及根系生长发育

本文采用14种拟南芥转基因报告株系,研究了对映-贝壳杉烷二萜(leukamenin E)调节拟南芥根部生长素极性运输转运蛋白表达并影响根生长发育的机制。结果表明:leukamenin E浓度在20～40μmol·L~(-1)范围显著抑制拟南芥幼苗主根的生长,较低浓度leukamenin E(10μmol·L~(-1))促进侧根提前发生并增加侧根数量; 10～30μmol·L-1的leukamenin E在处理拟南芥幼苗48 h后可显著提高其根尖部生长素水平;进一步检测根部生长素极性运输转运蛋白表达,发现该浓度条件下leukamenin E促进PIN1在转录水平表达并增加其蛋白丰度,但在转录水平抑制PIN2表达并减少其蛋白丰度;同时,显著减少PIN3、PIN7和PIN4蛋白在小柱和静止中心及其周围细胞的丰度以及AUX1的定位丰度; Leukamenin E对PIN1丰度的上调以及对PIN2、PIN3、PIN4、PIN7和AUX1定位丰度的减少可导致生长素在根尖顶部的积累以及根部生长素浓度梯度的改变,引起根生长的抑制及侧根的提前发生。     

拟南芥根中生长素极性运输的研究进展

生长素极性运输影响植物的生长和发育,在植物器官形态建成、发育等过程中发挥重要的调控作用.生长素极性运输是一个依赖于生长素运输载体来完成的复杂过程.近年来生长素极性运输载体AUX/LAX蛋白、PIN蛋白家族和MDR/PGP蛋白家族在生长素极性运输中作用的研究日益深入,并且在植物激素联系和转运方面取得了重大发现——PILC蛋白.     

植物生长素的极性运输载体研究进展

生长素极性运输在植物生长发育中起重要的调控作用.植物细胞间的生长素极性运输主要通过生长素运输载体进行调控.该文对近年来有关生长素极性运输载体,包括输入载体AUX/LAX、输出载体PIN、尤其是新近发现的兼有输入和输出载体功能的MDR/PGP等蛋白家族,以及生长素极性运输中PIN与MDR/PGP蛋白间相互作用关系进行综述.     

The march of the PINs: developmental plasticity by dynamic polar targeting in plant cells

Development of plants and their adaptive capacity towards ever‐changing environmental conditions largely depend on the spatial distribution of the plant hormone auxin. At the cellular level, various internal and external signals are translated into specific changes in the polar, subcellular localization of auxin transporters from the PIN family thereby directing and redirecting the intercellular fluxes of auxin. The current model of polar targeting of PIN proteins towards different plasma membrane domains encompasses apolar secretion of newly synthesized PINs followed by endocytosis and recycling back to the plasma membrane in a polarized manner. In this review, we follow the subcellular march of the PINs and highlight the cellular and molecular mechanisms behind polar foraging and subcellular trafficking pathways. Also, the entry points for different signals and regulations including by auxin itself will be discussed within the context of morphological and developmental consequences of polar targeting and subcellular trafficking.     

Clathrin-mediated constitutive endocytosis of PIN auxin efflux carriers in Arabidopsis

Endocytosis is an essential process by which eukaryotic cells internalize exogenous material or regulate signaling at the cell surface [1]. Different endocytic pathways are well established in yeast and animals; prominent among them is clathrin-dependent endocytosis [2, 3]. In plants, endocytosis is poorly defined, and no molecular mechanism for cargo internalization has been demonstrated so far [4, 5], although the internalization of receptor-ligand complexes at the plant plasma membrane has recently been shown [6]. Here we demonstrate by means of a green-to-red photoconvertible fluorescent reporter, EosFP [7], the constitutive endocytosis of PIN auxin efflux carriers [8] and their recycling to the plasma membrane. Using a plant clathrin-specific antibody, we show the presence of clathrin at different stages of coated-vesicle formation at the plasma membrane in Arabidopsis. Genetic interference with clathrin function inhibits PIN internalization and endocytosis in general. Furthermore, pharmacological interference with cargo recruitment into the clathrin pathway blocks internalization of PINs and other plasma-membrane proteins. Our data demonstrate that clathrin-dependent endocytosis is operational in plants and constitutes the predominant pathway for the internalization of numerous plasma-membrane-resident proteins including PIN auxin efflux carriers.     

Functional Analysis of the Hydrophilic Loop in Intracellular Trafficking of Arabidopsis PIN-FORMED Proteins

Different PIN-FORMED proteins (PINs) contribute to intercellular and intracellular auxin transport, depending on their distinctive subcellular localizations. Arabidopsis thaliana PINs with a long hydrophilic loop (HL) (PIN1 to PIN4 and PIN7; long PINs) localize predominantly to the plasma membrane (PM), whereas short PINs (PIN5 and PIN8) localize predominantly to internal compartments. However, the subcellular localization of the short PINs has been observed mostly for PINs ectopically expressed in different cell types, and the role of the HL in PIN trafficking remains unclear. Here, we tested whether a long PIN-HL can provide its original molecular cues to a short PIN by transplanting the HL. The transplanted long PIN2-HL was sufficient for phosphorylation and PM trafficking of the chimeric PIN5:PIN2-HL but failed to provide the characteristic polarity of PIN2. Unlike previous observations, PIN5 showed clear PM localization in diverse cell types where PIN5 is natively or ectopically expressed and even polar PM localization in one cell type. Furthermore, in the root epidermis, the subcellular localization of PIN5 switched from PM to internal compartments according to the developmental stage. Our results suggest that the long PIN-HL is partially modular for the trafficking behavior of PINs and that the intracellular trafficking of PIN is plastic depending on cell type and developmental stage.     

Cell polarity in plants: a PARspective on PINs

Plants have acquired the ability for organized multicellular development independent from animals. Because of this, they represent an independent example in nature for the development of coordinated, complex cell polarity from the simple polarity found in unicellular eukaryotes. Plants display a striking array of polarized cell types, with different axes of polarity being defined in one cell. The most investigated and best understood aspect of plant polarity is the apical-basal polarity of the PIN family of auxin efflux facilitators, which are of crucial importance for the organization of the entire plant body. Striking differences exist between the PAR-polarity modules known in animals and the ways PINs polarize plant cells. Nonetheless, a common regulatory logic probably applies to all polarizing eukaryotic cells, which includes self-reinforcing, positive feedback loops, intricate interactions between membrane-attached proteins, lipid signatures, and the targeting of transmembrane proteins to the correct domains of the plasma membrane.     

Recycling,clustering, and endocytosis jointly maintain PIN auxin carrier polarity at the plasma membrane

Cell polarity reflected by asymmetric distribution of proteins at the plasma membrane is a fundamental feature of unicellular and multicellular organisms. It remains conceptually unclear how cell polarity is kept in cell wall‐encapsulated plant cells. We have used super‐resolution and semi‐quantitative live‐cell imaging in combination with pharmacological, genetic, and computational approaches to reveal insights into the mechanism of cell polarity maintenance in Arabidopsis thaliana. We show that polar‐competent PIN transporters for the phytohormone auxin are delivered to the center of polar domains by super‐polar recycling. Within the plasma membrane, PINs are recruited into non‐mobile membrane clusters and their lateral diffusion is dramatically reduced, which ensures longer polar retention. At the circumventing edges of the polar domain, spatially defined internalization of escaped cargos occurs by clathrin‐dependent endocytosis. Computer simulations confirm that the combination of these processes provides a robust mechanism for polarity maintenance in plant cells. Moreover, our study suggests that the regulation of lateral diffusion and spatially defined endocytosis, but not super‐polar exocytosis have primary importance for PIN polarity maintenance.     

Regulation of the polarity of protein trafficking by phosphorylation

The asymmetry of environmental stimuli and the execution of developmental programs at the organism level require a corresponding polarity at the cellular level, in both unicellular and multicellular organisms. In plants, cell polarity is important in major developmental processes such as cell division, cell enlargement, cell morphogenesis, embryogenesis, axis formation, organ development, and defense. One of the most important factors controlling cell polarity is the asymmetric distribution of polarity determinants. In particular, phosphorylation is implicated in the polar distribution of the determinant protein factors, a mechanism conserved in both prokaryotes and eukaryotes. In plants, formation of local gradients of auxin, the morphogenic hormone, is critical for plant developmental processes exhibiting polarity. The auxin efflux carriers PIN-FORMEDs (PINs) localize asymmetrically in the plasma membrane and cause the formation of local auxin gradients throughout the plant. The asymmetry of PIN distribution in the plasma membrane is determined by phosphorylationmediated polar trafficking of PIN proteins. This review discusses recent studies on the role of phosphorylation in polar PIN trafficking.     

Drug response prediction using graph representation learning and Laplacian feature selection

Background

Essential proteins are indispensable to the development and survival of cells. The identification of essential proteins not only is helpful for the understanding of the minimal requirements for cell survival, but also has practical significance in disease diagnosis, drug design and medical treatment. With the rapidly amassing of protein–protein interaction (PPI) data, computationally identifying essential proteins from protein–protein interaction networks (PINs) becomes more and more popular. Up to now, a number of various approaches for essential protein identification based on PINs have been developed.

Results

In this paper, we propose a new and effective approach called iMEPP to identify essential proteins from PINs by fusing multiple types of biological data and applying the influence maximization mechanism to the PINs. Concretely, we first integrate PPI data, gene expression data and Gene Ontology to construct weighted PINs, to alleviate the impact of high false-positives in the raw PPI data. Then, we define the influence scores of nodes in PINs with both orthological data and PIN topological information. Finally, we develop an influence discount algorithm to identify essential proteins based on the influence maximization mechanism.

Conclusions

We applied our method to identifying essential proteins from saccharomyces cerevisiae PIN. Experiments show that our iMEPP method outperforms the existing methods, which validates its effectiveness and advantage.

     

Molecular architecture of postsynaptic Interactomes

The postsynaptic density (PSD) plays an essential role in the organization of the synaptic signaling machinery. It contains a set of core scaffolding proteins that provide the backbone to PSD protein-protein interaction networks (PINs). These core scaffolding proteins can be seen as three principal layers classified by protein family, with DLG proteins being at the top, SHANKs along the bottom, and DLGAPs connecting the two layers. Early studies utilizing yeast two hybrid enabled the identification of direct protein-protein interactions (PPIs) within the multiple layers of scaffolding proteins. More recently, mass-spectrometry has allowed the characterization of whole interactomes within the PSD. This expansion of knowledge has further solidified the centrality of core scaffolding family members within synaptic PINs and provided context for their role in neuronal development and synaptic function. Here, we discuss the scaffolding machinery of the PSD, their essential functions in the organization of synaptic PINs, along with their relationship to neuronal processes found to be impaired in complex brain disorders.     

Phospholipase A2 Is Required for PIN-FORMED Protein Trafficking to the Plasma Membrane in the Arabidopsis Root

Phospholipase A₂ (PLA₂), which hydrolyzes a fatty acyl chain of membrane phospholipids, has been implicated in several biological processes in plants. However, its role in intracellular trafficking in plants has yet to be studied. Here, using pharmacological and genetic approaches, the root hair bioassay system, and PIN-FORMED (PIN) auxin efflux transporters as molecular markers, we demonstrate that plant PLA₂s are required for PIN protein trafficking to the plasma membrane (PM) in the Arabidopsis thaliana root. PLA₂α, a PLA₂ isoform, colocalized with the Golgi marker. Impairments of PLA₂ function by PLA₂α mutation, PLA₂-RNA interference (RNAi), or PLA₂ inhibitor treatments significantly disrupted the PM localization of PINs, causing internal PIN compartments to form. Conversely, supplementation with lysophosphatidylethanolamine (the PLA₂ hydrolytic product) restored the PM localization of PINs in the pla₂α mutant and the ONO-RS-082–treated seedling. Suppression of PLA₂ activity by the inhibitor promoted accumulation of trans-Golgi network vesicles. Root hair–specific PIN overexpression (PINox) lines grew very short root hairs, most likely due to reduced auxin levels in root hair cells, but PLA₂ inhibitor treatments, PLA₂α mutation, or PLA₂-RNAi restored the root hair growth of PINox lines by disrupting the PM localization of PINs, thus reducing auxin efflux. These results suggest that PLA₂, likely acting in Golgi-related compartments, modulates the trafficking of PIN proteins.