植物细胞质外体多肽与蛋白研究

细胞质膜以外的质外体是植物细胞的重要组成部分, 质外体是植物细胞的重要信号源和细胞器。当植物遭受生物或非生物环境刺激时,可能首先引起质外体信号系统的变化; 同时质外体作为植物细胞之间最方便的通道, 在细胞间信号传递和信息交流上起重要作用, 从而成为协调植物细胞分化、器官形成和整体生长发育的决定性因素之一。本文概括地介绍了我室在此领域的一些研究进展。     

植物细胞质外体pH感受机制的解析

质外体是植物感受和应答环境胁迫(包括生物和非生物胁迫)的前沿区域。质外体的pH值是被严格调控的重要生理参数。环境胁迫(如细菌病害)等会引起植物细胞质外体碱化现象。然而, 质外体pH如何协调根生长与免疫响应? 其分子调控机制尚不清楚。最近, 南方科技大学生命科学学院郭红卫团队与清华大学-德国马克斯普朗克研究所-科隆大学柴继杰团队以模式植物拟南芥(Arabidopsis thaliana)为研究材料, 通过遗传学、细胞生物学、生物化学和结构生物学等综合手段, 发现细胞表面小肽-受体复合物可作为质外体pH感受器, 感受和应答分子模式触发的免疫(PTI)引发的拟南芥根尖分生组织细胞质外体碱化。该研究揭示了植物根尖分生组织细胞质外体pH感受的蛋白质复合物及响应机制, 以及免疫与生长之间的协调机制, 加深了人们对植物如何平衡生长与免疫应答生物学反应过程的理解。     

细胞外钙调素——一种植物中的多肽信使?

钙调素历来被认为是细胞内钙信号的多功能受体蛋白,国内外10多年的研究已证实,它普遍存在于人、动物细胞外与植物质外体.我们的工作证明了钙调素不仅普遍存在于植物细胞外,而且在胞外位点具有促进悬浮培养细胞及其原生质体的增殖、调节花粉萌发与伸长和促进rbc小亚基基因的光不依赖性表达等多种重要生物学功能.在花粉体系中,还证明了胞外钙调素具有跨膜与胞外信号转导机制,其中包括异三聚体G蛋白、PLC/IP3/IP3R和胞内钙信号等组分的参与.因此,认为细胞外钙调素可能是植物中的一种多肽信使,这对传统上认为植物中不存在进行胞间通讯的多肽信使的观点,提出了新的质疑.     

植物质外体的研究方法

质外体是细胞之间的空间和细胞膜与细胞壁之间的微小空间通过细胞壁上的微孔连接而成的一个连续［１］。整株植物的质外体是连续的。它是养分运输的重要途径,并有贮存养分和活化养分的功能。因此,质外体在植物代谢中的作用倍受人们的重视。然而由于质外体在植物中所占的比例较小,它与膜内细胞质之间存在着水分与物质的平衡,从而给有关质外体的研究带来许多困难。近些年来,国际上在这方面的研究取得了一些进展。本文着重介绍目前在植物营养研究中几种常用的质外体研究方法。１植物地上部质外体的测定方法在质外体的研究中,根系质外体已…     

植物胞外钙调素与信号转导

植物体需要构建复杂的信号转导体系以调节自身的生长发育过程并适应外界环境的变化,这种功能的实现需要胞内和胞外诸多信号分子的参与,胞外钙调素的发现使人们开始相信植物细胞外多肽信使的存在。胞外钙调素的生物学功能极其广泛,几乎涉及到植物生长发育的各个阶段,其信号转导途径是目前研究得最多也是最为清楚的方面,异三聚体G蛋白、磷脂酶C(PLC)-肌醇三磷酸(IP3)-肌醇三磷酸受体(IP3R)信号通路、活性氧和Ca2 通道之间直接或间接的相互作用是胞外钙调素信号转导的核心。     

植物根中质外体屏障结构和生理功能研究进展

综述了近10年来植物根中质外体屏障结构和功能的研究进展。质外体屏障指根中内、外皮层初生壁的凯氏带,或次生壁栓质化和木质化,以及植物体表角质层组成的保护组织,能隔绝水、离子和氧气不能自由进出植物体的屏障结构,具有保护植物体的生理功能。根中凯氏带的分子发育机理研究表明根内皮层类似哺乳动物上皮组织的保护作用。植物根中质外体保证内部各种生理代谢在稳定的内部环境中进行,是植物适应各种逆境的重要屏障结构。根中质外体屏障在植物适应干旱、洪涝灾害、离子胁迫和病虫害的侵袭等方面具有重要作用,在探索适应并修复极端生态环境的植物资源中有广阔的应用前景。     

脂肪间充质干细胞来源外泌体的功能

外泌体是细胞外膜质纳米囊泡,将蛋白质、核酸(DNA和RNA)转运到靶细胞中,介导局部和系统的细胞间通信,从而改变受体细胞的行为.这些小泡在许多生物功能中发挥重要作用,如脂肪合成、免疫调节、神经再生和肿瘤调节等.脂肪间充质干细胞目前被认为是细胞治疗和再生医学领域中一种功能丰富的工具,可产生和分泌多种外泌体,继承细胞的多种...     

植物根系质外体屏障研究进展

根是植物吸收水分和矿质营养以维持生命活动的重要器官。根系的构型和超微结构具有物种特异性, 对水分和矿质营养的吸收有不同程度的影响。其中, 内、外皮层的木栓层和凯氏带是2种重要的质外体屏障, 可非定向地阻断水分和离子运输, 在植物生长发育及响应逆境胁迫中发挥重要作用。尽管如此, 植物根系质外体屏障的结构、化学组成、生理功能、生物合成及其调控仅在模式植物拟南芥(Arabidopsis thaliana)中被广泛研究。近年来, 关于作物大麦(Hordeum vulgare)、水稻(Oryza sativa)以及部分牧草的根系质外体屏障研究报道逐渐增多。该文系统比较了拟南芥、大麦、水稻以及部分牧草根系质外体屏障的异同, 提出今后的研究方向, 以期为深入探索禾本科作物和牧草根系质外体屏障在生长发育和逆境适应中的作用奠定理论基础, 并为作物和牧草育种工作提供新思路。     

钙调素及钙调素相关蛋白在植物细胞中的研究进展

植物对一系列生物和非生物刺激所产生的反应都与细胞内Ca2+信号转导有关,而钙调素、钙调素相关蛋白则是Ca2+信号转导的下游靶蛋白。该文介绍了钙调素的结构及其在植物细胞中的分布,钙调素及钙调素相关蛋白在植物细胞中的表达等方面的最近研究进展。     

微生物胞外多糖在修复重金属污染中的潜力及其生物化学机制

微生物常常通过分泌细胞外多糖类物质(胞外多糖)来保护细胞免受极端环境条件、不利因素(如干燥、高盐、辐射、高低温、强酸碱)以及有毒有害物质(如重金属等)的损伤。胞外多糖在微生物耐受和降低重金属污染中起重要作用,在环境科学研究中有重要意义。本文综述了微生物胞外多糖的生物化学性质,简述了重金属对微生物胞外多糖合成及其结构的影响,从生物吸附、生物转化两个方面总结了微生物胞外多糖降低环境重金属污染的生物化学机制,最后展望了未来的研究方向和有待解决的科学问题。     

Extracellular calmodulin: A polypeptide signal in plants?

Traditionally, calmodulin (CaM) was thought to be a multi-functional receptor for intracellular Ca²⁺ signals. But in the last ten years, it was found that CaM also exists and acts extracellularly in animal and plant cells to regulate many important physiological functions. Laboratory studies by the authors showed that extracellular CaM in plant cells can stimulate the proliferation of suspension cultured cell and protoplast; regulate pollen germination and pollen tube elongation, and stimulate the light-independent gene expression of Rubisco small subunit (rbcS). Furthermore, we defined the trans-membrane and intracellular signal transduction pathways for extracellular CaM by using a pollen system. The components in this pathway include heterotrimeric G-protein, phospholipase C, IP₃, calcium signal and protein phosphorylation etc. Based on our findings, we suggest that extracellular CaM is a polypeptide signal in plants. This idea strongly argues against the traditional concept that there is no intercellular polypeptide signal in plants.     

Endogenous ascorbate restrains apoplastic peroxidase activity during sunflower leaf development

Several apoplastic enzymes have been implicated in the control of elongation growth of plant cells. Among them, peroxidases contribute to both loosening and stiffening of the cell wall. They appear to be regulated by various mechanisms, including the action of extracellular inhibitors. To obtain evidence of the role of the enzyme–inhibitor interaction during leaf development, the intercellular washing fluids from Helianthus annuus leaves of different ages were isolated using standard methods of vacuum infiltration and centrifugation. Peroxidase activities, assessed using tetramethylbenzidine as substrate, increased during leaf development, reaching a maximum value after the leaves were fully expanded. An inhibitor, chemically characterised as ascorbate, co‐localised with the enzyme in the apoplast. Moreover, there was a strong negative correlation between the action of peroxidase and the micromolar concentration of ascorbate in the apoplastic fluid. The results show that in growing leaves, the in planta ascorbate concentration is able to restrain peroxidase enzyme activity. Then, at the time of growth cessation, the loss of extracellular ascorbate relieves the inhibition on this enzyme that contributes to wall fixation.     

An apoplastic mechanism for short-term effects of rare earth elements at lower concentrations

The short-term effects of rare earth elements on pollen germination and tube growth were tested. Concentrations of 2.5 approximately 20 micro m lanthanum(La3+) or cerium (Ce3+)increased pollen germination and pollen tube growth, whereas concentrations higher than 40 micro m La3+ and Ce3+ inhibited this process. The most effective concentration of La3+ needed for promotion shifted from 10 to 40 micro m, depending on the Ca2+ concentration in the medium. Calmodulin (CaM) antagonist W7-agarose and anti-CaM antibody depressed La3+-promoted pollen germination and tube growth in a dose-dependent manner. La3+-CaM complexes (La3+-CaM) increased pollen germination and tube growth more than CaM or La3+ alone. Pertussis toxin (PTX) inhibited La3+-promoted pollen germination and tube growth. Cholera toxin (CTX) partially recovered the inhibition of the above La3+-promoted process by the anti-CaM antibody. Concentrations of 10-7 approximately 10-9 m La3+-CaM increased GTPase activity inside plasma membrane vesicles of the pollen tube, but apo-CaM or La3+ alone had no positive effects. The results suggest that apoplastic CaM may be involved in the promotion effects of lower concentrations of La3+ on pollen germination and tube growth, and the heterotrimeric G-protein on the plasma membrane may transduce La3+-activated CaM signalling. The present studies provide an apoplastic mechanism for short-term effects of rare earth elements at lower concentrations in the pollen system.     

Extracellular calmodulin: A polypeptide signal in plants?

Traditionally, calmodulin (CaM) was thought to be a multi-functional receptor for intra-cellular Ca2+ signals. But in the last ten years, it was found that CaM also exists and acts extracel-lularly in animal and plant cells to regulate many important physiological functions. Laboratory studies by the authors showed that extracellular CaM in plant cells can stimulate the proliferation of suspension cultured cell and protoplast; regulate pollen germination and pollen tube elongation, and stimulate the light-independent gene expression of Rubisco small subunit (rbcS). Furthermore, we defined the trans-membrane and intracellular signal transduction pathways for extracellular CaM by using a pollen system. The components in this pathway include heterotrimeric G-protein, phospholipase C, IP3, calcium signal and protein phosphorylation etc. Based on our findings, we suggest that extracellular CaM is a polypeptide signal in plants. This idea strongly argues against the traditional concept that there is no interce     

Target sites of aluminum phytotoxicity

The primary phytotoxic effect of aluminum (Al) is confined to the root apex. It is a matter of debate whether the primary injury of Al toxicity is apoplastic or symplastic. This review paper summarizes our current understanding of the spatial and metabolic sites of Al phytotoxicity. At tissue level, the meristematic, distal transition, and apical elongation zones of the root apex are most sensitive to Al. At cellular and molecular level, many cell components are implicated in Al toxicity including DNA in nucleus, numerous cytoplastic compounds, the plasma membrane, and the cell wall. Although it is difficult to distinguish the primary targets from the secondary effects so far, understanding of the target sites of Al toxicity is helpful for elucidating the mechanisms by which Al exerts its deleterious effects on root growth.This work was partly supported by fund from the Huoyingdong Foundation, Education Ministry of China and Natural Science Foundation of China (Contact No. 30170548).     

Role of apoplastic ascorbate and hydrogen peroxide in the control of cell growth in pine hypocotyls

The growth cessation of plant axis has been related with the formation of diphenyl bridges among the pectic components of the cell wall caused by the action of apoplastic peroxidases using hydrogen peroxide as electron acceptor. The formation of diphenyl bridges is prevented by the presence of ascorbate in the apoplastic fluid which acts as a hydrogen peroxide scavenger. The current work focuses on the role of the apoplastic ascorbate and hydrogen peroxide in the cell growth. The addition of hydrogen peroxide caused an inhibition of the auxin-induced growth as well as a significant decrease in the cell wall creep induced by acid-pH solutions. The hydrogen peroxide content in apoplastic fluid increased with the hypocotyl age and along the hypocotyl axis of 10-day-old pine seedlings, as the growth capacity decreased. On the other hand, the ascorbate content in the apoplastic fluid decreased with the hypocotyl age and along the hypocotyl axis of 10-day-old seedlings. A very significant correlation between the hydrogen peroxide apoplastic level and the growth rate as well as between the ascorbate/hydrogen peroxide molar ratio and the growth rate of hypocotyls have been found suggesting that the redox state is the main factor controlling the cell wall stiffening mechanism and thus growth in pine hypocotyls.     

Signal Integration by ABA in the Blue Light-Induced Acidification of Leaf Pavement Cells in Pea (Pisum sativum L. var. Argenteum)

Leaf pavement cell expansion in light depends on apoplastic acidification by a plasma membrane proton-pumping ATPase, modifying cell wall extensibility and providing the driving force for uptake of osmotically active solutes generating turgor. This paper shows that the plant hormone ABA inhibits light-induced leaf disk growth as well as the blue light-induced pavement cell growth in pea (Pisum sativum L.). In the phytochrome chromophore-deficient mutant pcd2, the effect of ABA on the blue light-induced apoplastic acidification response, which exhibits a high fluence phase via phytochrome and a low fluence phase via an unknown blue light receptor, is still present, indicating an interaction of ABA with the blue light receptor pathway. Furthermore, it is shown that ABA inhibits the blue light-induced apoplastic acidification reversibly. These results indicate that the effect of ABA on apoplastic acidification can provide a mechanism for short term, reversible adjustment of leaf growth rate to environmental change.Key Words: ABA, apoplastic acidification, blue light, epidermal pavement cell growth, leaf growth, pea (Pisum sativum L.), signal integration     

Review article. Apoplastic barriers in roots: chemical composition of endodermal and hypodermal cell walls

Based on the characterization of the chemical composition of endodermal and hypodermal cell walls isolated from seven monocotyledonous and three dicotyledonous plant species, a model of the composition of apoplastic barriers in roots is proposed. Depending on the species, endodermal and hypodermal cell walls of roots contained varying amounts of the biopolymers suberin, lignin, cell wall proteins, and carbohydrates. Although analysis of the chemical composition of these apoplastic barriers of roots is now possible, it is pointed out that conclusions from these data concerning the functional properties of these cell walls can not easily be drawn. However, in analogy to suberized periderms it is argued that the suberin should play a role in establishing an apoplastic transport barrier in roots, albeit not a perfect barrier. Furthermore, due to the combined occurrence of suberin, lignin and cell wall proteins it is argued that endodermal and hypodermal cell walls also have an important function as barriers towards pathogens. Finally, it is pointed out that additional experimental approaches combining the investigation of transport properties and of the chemical composition of apoplastic transport barriers in roots are necessary before the function of endodermal and hypodermal cell walls in roots can be fully understood.     

Apoplastic pH and Ammonium Concentration in Leaves of Brassica napus L

A vacuum infiltration technique was developed that enabled the extraction of apoplastic solution with very little cytoplasmic contamination as evident from a malate dehydrogenase activity of less than 1% in the apoplastic solution relative to that in bulk leaf extracts. The volume of apoplastic water, a prerequisite for determination of the concentration of apoplastic solutes, was determined by vacuum infiltration of indigo carmine with subsequent analysis of the dilution of the dye in apoplastic extracts. Indigo carmine was neither transported across the cell membrane nor significantly adsorbed to the cell walls, ensuring reproducible (SE < 2%) and precise determination of apoplastic water. Analysis of leaves from four different positions on senescing Brassica napus plants showed a similar apoplastic pH of 5.8, while apoplastic NH4+ increased from 1.1 mM in lower leaves to 1.3 mM in upper leaves. Inhibition of glutamine synthetase in young B. napus plants resulted in increasing apoplastic pH from 6.0 to 6.8 and increasing apoplastic NH4+ concentration from 1.0 to 25.6 mM, followed by a marked increase in NH3 emission. Calculating NH3 compensation points for B. napus plants on the basis of measured apoplastic H+ and NH4+ concentrations gave values ranging from 4.3 to 5.9 nmol NH3 mol-1 air, consistent with an estimate of 5.3 [plus or minus] 3.6 nmol NH3 mol-1 air obtained by NH3 exchange experiments in growth chambers. A strong linear relationship was found between calculated NH3 compensation points and measured NH3 emission rates in glutamine synthetase-inhibited plants.     

Depolymerization of actin cytoskeleton is involved in stomatal closure-induced by extracellular calmodulin in<Emphasis Type="Italic">Arabidopsis</Emphasis>

Extracellular calmodulin(CaM)plays significant roles in many physiological processes,but little is known about its mechanism of regulating stomatal movements.In this paper,whether CaM exists in the guard cell walls of Arabidopsis and whether depolymerization of actin cytoskeleton is involved in extracellular CaM-induced stomatal closing are investigated.It is found that CaM exists in guard cell walls of Arabidopsis,and its molecular weight is about 17 kD.Bioassay using CaM antagonists W7-agarose and anti-CaM serum shows that the endogenous extracellular CaM promotes stomatal closure and delays stomatal opening.The long radial actin filaments in guard cells undergo disruption in a time-dependent manner during exogenous CaM-induced stomatal closing.Pharmacological experiments show that depolymerization of actin cytoskeleton enhances the effect of exogenous CaM-induced stomatal closing and polymerization reduces the effect.We also find that exogenous CaM triggers an increase in [Ca2+]cyt of guard cells.If [Ca2+]cyt increase is blocked with EGTA,exogenous CaM-induced stomatal closure is inhibited.These results indicate that extracellular CaM causes elevation of [Ca2+]cyt in guard cells,subsequently resulting in disruption of actin filaments and finally leading to guard cells closure.