Ca2+ signaling in plant responses to abiotic stresses

Adverse variations of abiotic environmental cues that deviate from an optimal range impose stresses to plants. Abiotic stresses severely impede plant physiology and development. Consequently, such stresses dramatically reduce crop yield and negatively impact on ecosystem stability and composition. Physical components of abiotic stresses can be, for example, suboptimal temperature and osmotic perturbations, while representative chemical facets of abiotic stresses can be toxic ions or suboptimal nutrient availability. The sheer complexity of abiotic stresses causes a multitude of diverse components and mechanisms for their sensing and signal transduction. Ca²⁺, as a versatile second messenger, plays multifaceted roles in almost all abiotic stress responses in that, for a certain abiotic stress, Ca²⁺ is not only reciprocally connected with its perception, but also multifunctionally ensures subsequent signal transduction. Here, we will focus on salt/osmotic stress and responses to altered nutrient availability as model cases to detail novel insights into the identity of components that link stress perception to Ca²⁺ signal formation as well as on new insights into mechanisms of Ca²⁺ signal implementation. Finally, we will deduce emerging conceptual consequences of these novel insights and outline arising avenues of future research on the role of Ca²⁺ signaling in abiotic stress responses in plants.     

MDP25 mediates the fine-tuning of microtubule organization in response to salt stress

Microtubules are dynamic cytoskeleton structures playing fundamental roles in plant responses to salt stress. The precise mechanisms by which microtubule organization is regulated under salt stress are largely unknown. Here, we report that Arabidopsis thaliana MICROTUBULE-DESTABILIZING PROTEIN 25 (MDP25; also known as PLASMA MEMBRANE-ASSOCIATED CATION-BINDING PROTEIN 1 (PCaP1)) helps regulate microtubule organization. Under salt treatment, elevated cytosolic Ca²⁺ concentration caused MDP25 to partially dissociate from the plasma membrane, promoting microtubule depolymerization. When Ca²⁺ signaling was blocked by BAPTA-AM or LaCl₃, microtubule depolymerization in wild-type and MDP25-overexpressing cells was slower, while there was no obvious change in mdp25 cells. Knockout of MDP25 improved microtubule reassembly and was conducive to microtubule integrity under long-term salt treatment and microtubule recovery after salt stress. Moreover, mdp25 seedlings exhibited a higher survival rate under salt stress. The presence microtubule-disrupting reagent oryzalin or microtubule-stabilizing reagent paclitaxel differentially affected the survival rates of different genotypes under salt stress. MDP25 promoted microtubule instability by affecting the catastrophe and rescue frequencies, shrinkage rate and time in pause phase at the microtubule plus-end and the depolymerization rate at the microtubule minus-end. These findings reveal a role for MDP25 in regulating microtubule organization under salt treatment by affecting microtubule dynamics.     

外源钙离子对盐胁迫玉米气孔特征、光合作用和生物量的影响

探讨盐胁迫下玉米气孔特征、光合作用和生物量对外源钙离子的响应,有助于深入理解添加外源钙离子(Ca²⁺)缓解玉米盐胁迫的作用机理.以‘京科665’品种为试材,研究了NaCl胁迫下(100 mmol·L^-1)添加不同浓度外源Ca²⁺(0、5、10、20、40、80 mmol·L^-1)对玉米幼苗气孔特征、光合作用和生物量的影响.结果表明: 不同Ca²⁺浓度对盐胁迫下玉米的气孔密度影响不大,但显著减小了气孔形状指数、气孔面积、气孔长度、气孔宽度和气孔周长.同时,随着外源Ca²⁺浓度的逐渐提高,玉米叶片的净光合速率(P_n)呈先升高后降低的趋势,且气孔导度(g_s)和胞间CO₂浓度(C_i)均显著降低,表明不同浓度Ca²⁺通过改变玉米气孔结构特征进一步限制光合作用过程,最终导致P_n降低.另外,外源Ca²⁺促进盐胁迫下玉米幼苗生物量增加,但根冠比显著降低,表明盐胁迫下添加外源Ca²⁺对地上部分的缓解作用大于地下部分.     

盐胁迫下外源褪黑素和Ca2+对甜瓜幼苗的缓解效应

以甜瓜品种‘羊角酥瓜’为试材,利用人工气候室控制环境条件(昼/夜25/18 ℃),研究盐胁迫条件下外源褪黑素(MT)和Ca²⁺对甜瓜幼苗根系和叶片中Cl^-、Na⁺、K⁺、Mg²⁺、Ca²⁺离子含量,Na⁺/K⁺、 Na⁺/Ca²⁺、Na⁺/Mg²⁺值,以及H⁺-ATP酶活性、渗透调节物质积累和细胞膜质过氧化的影响.结果表明: 与对照相比,盐胁迫处理显著抑制甜瓜幼苗生长,增加根系和叶片中Cl^-、Na⁺含量,降低K⁺、Mg²⁺、Ca²⁺含量.盐胁迫下,喷施外源MT或Ca²⁺处理均可以显著降低甜瓜根系和叶片中Cl^-、Na⁺含量,提高K⁺、Mg²⁺、Ca²⁺含量,植株体内Na⁺/K⁺、Na⁺/Ca²⁺和 Na⁺/Mg²⁺值下降;同时也提高了根系和叶片H⁺-ATP酶活性及叶片渗透调节物质的含量,降低盐胁迫对细胞膜的伤害,表现在甜瓜叶片相对电导率和丙二醛含量降低.总之,在盐胁迫条件下,外源MT、Ca²⁺单独和复配处理均可通过提高H⁺-ATP酶活性来降低盐害离子的含量,改善甜瓜幼苗中的离子平衡,同时增加渗透调节物质的含量,降低膜质过氧化水平,从而增强其对盐胁迫的适应性,其中MT和Ca²⁺复配处理时的效果更好.复配外施 MT 和Ca²⁺在诱导甜瓜幼苗提高耐盐方面具有协同增效作用.     

盐胁迫下外源褪黑素和Ca2+对甜瓜幼苗的缓解效应

以甜瓜品种‘羊角酥瓜’为试材,利用人工气候室控制环境条件(昼/夜25/18 ℃),研究盐胁迫条件下外源褪黑素(MT)和Ca²⁺对甜瓜幼苗根系和叶片中Cl^-、Na⁺、K⁺、Mg²⁺、Ca²⁺离子含量,Na⁺/K⁺、 Na⁺/Ca²⁺、Na⁺/Mg²⁺值,以及H⁺-ATP酶活性、渗透调节物质积累和细胞膜质过氧化的影响.结果表明: 与对照相比,盐胁迫处理显著抑制甜瓜幼苗生长,增加根系和叶片中Cl^-、Na⁺含量,降低K⁺、Mg²⁺、Ca²⁺含量.盐胁迫下,喷施外源MT或Ca²⁺处理均可以显著降低甜瓜根系和叶片中Cl^-、Na⁺含量,提高K⁺、Mg²⁺、Ca²⁺含量,植株体内Na⁺/K⁺、Na⁺/Ca²⁺和 Na⁺/Mg²⁺值下降;同时也提高了根系和叶片H⁺-ATP酶活性及叶片渗透调节物质的含量,降低盐胁迫对细胞膜的伤害,表现在甜瓜叶片相对电导率和丙二醛含量降低.总之,在盐胁迫条件下,外源MT、Ca²⁺单独和复配处理均可通过提高H⁺-ATP酶活性来降低盐害离子的含量,改善甜瓜幼苗中的离子平衡,同时增加渗透调节物质的含量,降低膜质过氧化水平,从而增强其对盐胁迫的适应性,其中MT和Ca²⁺复配处理时的效果更好.复配外施 MT 和Ca²⁺在诱导甜瓜幼苗提高耐盐方面具有协同增效作用.     

植物感受盐胁迫及相关钙信号的研究进展

盐胁迫对植物的生长和发育造成严重影响,其危害包括渗透胁迫、离子毒害等,严重损害了农业生产和粮食安全。在盐胁迫下,植物相关感受器接受刺激,使得Ca²⁺通过细胞膜以及细胞内钙库膜上打开的Ca²⁺通道进入细胞质基质,导致细胞质内Ca²⁺浓度升高,产生钙信号。钙离子作为重要的第二信使,在植物细胞内和细胞间传递信号,信号往下游传递,在不同生长和发育阶段引起植物一系列的生理响应来应对盐胁迫影响。钙信号主要通过钙调蛋白（CaM）、钙调素样蛋白（CML）、钙依赖性蛋白激酶（CDPK）、钙调磷酸酶B样蛋白（CBL）和CBL互作蛋白激酶（CIPK）感知并将特异的钙信号信息传递到下游;从而激活植物盐胁迫生理响应。本文主要综述植物如何感知盐胁迫刺激,以及钙信号产生与传导机制,并对该研究领域需解决的问题进行了展望。     

外生菌根真菌通过调节离子平衡提高蒙古栎耐盐性

为探究盐胁迫对蒙古栎生长的影响以及外生菌根真菌(ECMF)对蒙古栎离子平衡的调节作用,对蒙古栎幼苗接种4种ECMF(铆钉菇、褐环乳牛肝菌、厚环粘盖牛肝菌和美味牛肝菌)后,以1年生非菌根化与菌根化幼苗为试验材料,进行36 d的NaCl胁迫(0、100、200、300 mmol·L^-1)处理,分析幼苗的菌根特征、生长量、叶伤害症状、叶片电解质渗透率及含水量、根茎叶离子含量的变化特征。结果表明: 4种ECMF均能与蒙古栎建立共生体系,菌根化幼苗的根系较非菌根化幼苗粗壮。盐胁迫下,蒙古栎幼苗的生长受到抑制并出现焦叶症状,其叶片质膜损伤和失水程度随盐胁迫浓度升高而加重。低盐胁迫时(100 mmol·L^-1),蒙古栎优先将Na⁺积累在根和茎中,中高浓度盐胁迫下(200～300 mmol·L^-1),根成为积累Na⁺的首要器官。ECMF通过增加根部的Na⁺水平和减少茎、叶的Na⁺积累,加强对K⁺和Ca²⁺的吸收以提高K⁺/Na⁺和Ca²⁺/Na⁺,进而调节蒙古栎的离子平衡。4种ECMF对蒙古栎盐毒害的缓解作用存在差异,铆钉菇作用效果最好,褐环乳牛肝菌次之,厚环粘盖牛肝菌和美味牛肝菌的作用相对较小。     

外源褪黑素与钙离子互作对高温胁迫下黄瓜幼苗过氧化伤害的缓解效应

为了探明褪黑素(MT)和钙离子(Ca²⁺)在调控植物耐热性中是否存在互作关系,以黄瓜幼苗为试材,分析了内源MT和Ca²⁺对高温胁迫的响应;并通过叶面喷施100 μmol·L^-1 MT、10 mmol·L^-1 CaCl₂、3 mmol·L^-1乙二醇二乙醚二胺四乙酸(EGTA,Ca²⁺螯合剂)+100 μmol·L^-1 MT、0.05 mmol·L^-1氯丙嗪(钙调素拮抗剂,CPZ)+100 μmol·L^-1 MT、100 μmol·L^-1氯苯丙氨酸(p-CPA,MT合成抑制剂)+10 mmol·L^-1 CaCl₂和去离子水(H₂O),研究高温下(42/32 ℃)外源MT和Ca²⁺对黄瓜幼苗活性氧积累、抗氧化系统及热激转录因子(HSF)和热激蛋白(HSPs)等的影响。结果表明: 黄瓜幼苗内源MT和Ca²⁺均受高温胁迫诱导;外源MT可上调常温下钙调素蛋白(CaM)、钙依赖蛋白激酶(CDPK5)、钙调磷酸酶B类蛋白(CBL3)、CBL结合蛋白激酶(CIPK2)mRNA表达;CaCl₂处理的MT合成关键基因色氨酸脱羧酶(TDC)、5-羟色胺-N-乙酰转移酶(SNAT)和N-乙酰-5-羟色胺甲基转移酶(ASMT)水平也显著升高,MT含量快速增加。MT和CaCl₂可显著增强高温下黄瓜的抗氧化能力,减少活性氧(ROS)积累,同时上调HSF7、HSP70.1和HSP70.11 mRNA表达,从而减轻高温胁迫引起的过氧化伤害,植株热害症状明显减轻,热害指数和电解质渗漏率显著降低。加入EGTA和CPZ后,MT对黄瓜幼苗抗氧化能力和热激蛋白表达的促进效应明显减弱,Ca²⁺对高温下黄瓜幼苗过氧化伤害的缓解效应也被p-CPA逆转。可见,MT和Ca²⁺均可诱导黄瓜幼苗的耐热性,二者在热胁迫信号转导过程中存在互作关系。     

丛枝菌根真菌调控根系构型与矿质元素平衡提高西瓜植株耐盐性的研究

丛枝菌根（arbuscular mycorrhiza,AM）真菌可通过多种途径或机制来增强植物的耐盐性,进而促进植株的生长发育。本研究在盆栽条件下设西瓜Citrullus lanatus品种‘京欣四号’幼苗接种变形球囊霉Glomus versiforme和不接种以及施加和不施加100mmol/L NaCl共4个处理,测定植株根系菌根侵染状况、根系构型及其根茎叶中钾（K）、钙（Ca）、磷（P）、钠（Na）含量、K⁺/Na⁺、Ca²⁺/Na和植株生长状况等。AM真菌显著增加了盐胁迫下西瓜植株总根长度、根表面积、根体积和根尖数量,改善了根系构型;促进了西瓜根系对K、Ca和P的吸收,提高了茎Ca和P含量、根系K和P含量、K⁺/Na⁺和Ca²⁺/Na⁺,而降低了根Na⁺含量;茎P和Na⁺、叶K和Ca的含量显著高于其他器官相应含量。典范对应分析表明,根系K含量、K⁺/Na⁺和Ca²⁺/Na⁺与总根长度、主根长度、根表面积、根体积、根尖数量、根平均直径呈正相关;叶K⁺/Na⁺与主根长度呈正相关;根系Na⁺含量与根系总根长、根平均直径和根尖数量呈负相关。接种AM真菌改善了矿质元素平衡及其分配状况。盐胁迫后西瓜植株对菌根的依赖性增强。结果表明,K、Ca、P是AM真菌介导植物耐盐性的关键养分;K⁺/Na⁺和Ca²⁺/Na⁺是重要的矿质元素平衡指标,接种AM真菌能调控植物根系构型和矿质元素平衡状况,从而缓解盐胁迫对西瓜生长的抑制作用,提高植株的耐盐性。     

镁转运体MGT7参与拟南芥对高钙环境的适应

高Ca²⁺环境对许多植物的生长不利, 因此研究植物对高Ca²⁺环境的适应机制非常重要。研究发现, 拟南芥(Ara- bidopsis thaliana)镁转运体MGT7功能缺失突变体mgt7-1和mgt7-2具有高Ca²⁺敏感表型: 在高Ca²⁺培养基上, 相对于野生型Col-0, 突变体叶鲜重显著下降, 但根长无显著差异。高Ca²⁺对MGT7启动子活性和包括MGT7在内的镁转运体基因表达无显著调节作用。Col-0与mgt7突变体之间, 在外加Ca²⁺诱导细胞质Ca²⁺瞬时升高和Ca²⁺含量方面无显著差异; 但是, 在正常和高Ca²⁺培养基上, mgt7突变体的Mg含量均显著低于Col-0。高Ca²⁺显著抑制Col-0和mgt7突变体内Mg的积累。因此我们假设, mgt7突变体的高Ca²⁺敏感表型是由于其体内Mg含量下降导致的。进一步的研究证实, 只有增加培养基中Mg²⁺的含量, 而不是N、P、K和S, 才可以使突变体的高Ca²⁺敏感表型得到恢复。     

疏叶骆驼刺适应盐渍生境的离子分布、吸收和运输特征

以塔里木盆地南缘关键物种疏叶骆驼刺为材料,研究了不同盐渍土壤生境(轻度盐渍土、中度盐渍土、重度盐渍土)下其器官间Na⁺、K⁺、Ca²⁺、Mg²⁺的分布、吸收及运输特征,以探讨疏叶骆驼刺对自然盐渍生境的适应特性.结果表明: 在轻度和中度盐渍土生境,Na⁺在各器官中的分布规律为茎≈刺>叶>根,而在重度盐渍土生境,Na⁺分布规律为叶>茎≈刺>根;Ca²⁺和Mg²⁺在疏叶骆驼刺体内的分布规律为叶>刺>茎>根.随着土壤含盐量的增加,疏叶骆驼刺体内各器官Na⁺含量都增大,而叶片中K⁺含量呈下降趋势;根和叶器官中K⁺/Na⁺值明显降低,各器官中Ca²⁺/Na⁺、Mg²⁺/Na⁺值都降低.盐渍生境下,疏叶骆驼刺体内Ca²⁺选择性运输系数和Mg²⁺选择性运输系数均为茎-叶>茎-刺>根-茎.疏叶骆驼刺为适应盐渍生境,在土壤含盐量较低时,将Na⁺聚集于茎和刺;而在土壤含盐量较高时,则将Na⁺聚集于叶片.此外,Ca²⁺和Mg²⁺可能是疏叶骆驼适应盐渍生境的无机渗透调节物质.     

Effect of Ca channel blockers on glycerol levels in Dunaliella tertiolecta under hypoosmotic stress

The role of Ca²⁺ in glycerol dissimilation under hypoosmotic stress in the halotolerant alga Dunaliella tertiolecta was investigated using a pharmacological approach. A stretch-activated Ca²⁺ channel blocker, GdCl₃, inhibited glycerol dissimilation under hypoosmotic stress. However, addition of voltage-dependent Ca²⁺ channel blockers and inhibitors of mitochondrial and endoplasmic reticulum Ca²⁺ channels did not affect the glycerol dissimilation under hypoosmotic stress. The results of the present study suggest that the influx of Ca²⁺ from the extracellular space via the stretch-activated Ca²⁺ channels localized in the plasma membrane is required for the transduction of osmotic signal of D. tertiolecta.     

植物质膜蛋白质组的逆境应答研究进展

质膜作为原生质体与外界环境的屏障, 除了维持正常的细胞内稳态和营养状况, 还参与感知和应答各种环境胁迫。近年来, 植物质膜蛋白质组学研究为深入分析植物应答不同生物和非生物胁迫的分子机制提供了重要信息, 已经报道了模式植物拟南芥(Arabidopsis thaliana)和水稻(Oryza sativa)等10种植物质膜应对生物胁迫(白叶枯病菌(Xanthomonas oryzae pv. oryzae)感染)与非生物胁迫(冷、盐、水淹、渗透、高pH值、Fe缺乏及过量、氮素、脱落酸、壳聚糖和壳寡糖)过程的蛋白质丰度模式变化。通过整合分析植物质膜响应逆境的蛋白质组学研究结果, 揭示了质膜在植物应答逆境胁迫过程中的重要作用。植物通过调节转运蛋白、通道蛋白及膜泡运输相关蛋白的丰度变化促进细胞内外的信号传递、物质交换与运输; 同时利用膜相关的G蛋白、Ca²⁺信号、磷酸肌醇信号途径及BR信号途径等多种信号通路, 通过蛋白质可逆磷酸化作用感知和传递胁迫信号, 调节植物抵御胁迫。研究结果为从蛋白质水平认识质膜逆境应答分子调控机制提供了新线索。     

Exogenously applied ascorbic acid alleviates salt-induced oxidative stress in wheat

Although ascorbic acid (AsA) is one of the most important and abundantly occurring water soluble antioxidants in plants, relatively little is known about its role in counteracting the adverse effects of salt stress on plant growth. To address this issue that whether exogenous application of ascorbic acid (AsA) through rooting medium could alleviate the adverse effects of salt stress on wheat plants, a hydroponic experiment was conducted under glasshouse conditions using two wheat cultivars, S-24 (salt tolerant) and MH-97 (moderately salt sensitive). Plants of both cultivars were subjected to 0 or 150 mM NaCl solution supplemented with 0, 50, or 150 mg L⁻¹ AsA for 58 days. Imposition of salt stress reduced the growth of both wheat cultivars by causing reduction in photosynthesis, and endogenous AsA level, and enhancing accumulation of Na⁺ and Cl⁻ coupled with a decrease in K⁺ and Ca²⁺ in the leaves and roots of both cultivars thereby decreasing tissue K⁺/Na⁺ ratio. However, root applied AsA counteracted the adverse effects of salt stress on the growth of cv. S-24 only, particularly at 100 mg L⁻¹ AsA level. AsA-induced enhancement in growth of salt-stressed plants of S-24 was associated with enhanced endogenous AsA level and CAT activity, and higher photosynthetic capacity, and accumulation of K⁺ and Ca²⁺ in the leaves. Although root applied AsA did not improve the growth of salt-stressed plants of MH-97, it enhanced endogenous level of AsA, CAT activity, photosynthetic capacity, and leaf K⁺ and Ca²⁺. These findings led us to conclude that root applied AsA counteracts the adverse effects of salt stress on growth of wheat by improving photosynthetic capacity of wheat plants against salt-induced oxidative stress and maintaining ion homeostasis, however, these effects were cultivar specific.     

A protective role for the polyamine spermine against drought stress in Arabidopsis

Cellular polyamine content often changes in response to abiotic stresses. However, its physiological relevance is unknown. We found that an Arabidopsis mutant plant (acl5/spms), which cannot produce spermine, is hypersensitive to high salt. Examination of drought sensitivity of the mutant and comparison with wild type plants indicated hypersensitivity to drought. This phenotype was cured by spermine pretreatment but not by the other polyamines putrescine and spermidine, suggesting that drought-hypersensitivity exhibited by the mutant is due to spermine deficiency. The water loss rate of wild type and mutant plants were similar until 20 min after onset of dehydration stress, but after a longer exposure the rate in mutant plants was higher than in wild type plants. Consistent with this result, the stomata of the mutant leaves remained open while in wild type leaves they closed. Based on the collected data, we discuss a role for spermine in response to drought stress.     

The Arabidopsis phosphatase PP2C49 negatively regulates salt tolerance through inhibition of AtHKT1;1

Type 2C protein phosphatases (PP2Cs) are the largest protein phosphatase family. PP2Cs dephosphorylate substrates for signaling in Arabidopsis, but the functions of most PP2Cs remain unknown. Here, we characterized PP2C49 (AT3G62260, a Group G PP2C), which regulates Na⁺ distribution under salt stress and is localized to the cytoplasm and nucleus. PP2C49 was highly expressed in root vascular tissues and its disruption enhanced plant tolerance to salt stress. Compared with wild type, the pp2c49 mutant contained more Na⁺ in roots but less Na⁺ in shoots and xylem sap, suggesting that PP2C49 regulates shoot Na⁺ extrusion. Reciprocal grafting revealed a root‐based mechanism underlying the salt tolerance of pp2c49. Systemic Na⁺ distribution largely depends on AtHKT1;1 and loss of function of AtHKT1;1 in the pp2c49 background overrode the salt tolerance of pp2c49, resulting in salt sensitivity. Furthermore, compared with plants overexpressing PP2C49 in the wild‐type background, plants overexpressing PP2C49 in the athtk1;1 mutant background were sensitive to salt, like the athtk1;1 mutants. Moreover, protein–protein interaction and two‐voltage clamping assays demonstrated that PP2C49 physically interacts with AtHKT1;1 and inhibits the Na⁺ permeability of AtHKT1;1. This study reveals that PP2C49 negatively regulates AtHKT1;1 activity and thus determines systemic Na⁺ allocation during salt stress.     

Recovery of development and functionality of nodules and plant growth in salt-stressed Pisum sativum--Rhizobium leguminosarum symbiosis by boron and calcium

Nodules developed in Pisum sativum L. cv. Argona inoculated with Rhizobium leguminosarum bv. viciae 3841 and growing under saline conditions (75 mmol/L NaCl) are non functional and had abnormal structure. The infected cells contained a low amount of endophytic bacteria, compared to treatments without salt. Addition of B (up to 55.8 μmol/L) and Ca²⁺ (up to 2.72 mmol/L) increased bacterial population of host plant cells in salt-stressed nodules. Furthermore, symbiosomes developed inside the nodules from salt treated plants presented a degraded peribacteroid membrane. This effect was also prevented by combined addition of B and Ca²⁺. Given the importance of both nutrients in cell wall structure, the pectin fraction was studied by electron microscopy and immunological methods. Salt stress produced cells with walls dramatically altered or even degraded in several zones. Pectin polysaccharides, detected by JIM 5 monoclonal antibody, increased in cells under salinity. These effects resembled typical effects of B-deficiency reactions in cell walls, and the increase of both Ca²⁺ and especially B also prevented these alterations.     

胞质Ca2+参与外源H2S促进盐碱胁迫下裸燕麦种子萌发

硫化氢（Hydrogen sulfide,H₂S）是植物新型气体信号分子,钙离子（Calcium,Ca²⁺）为重要的第二信使,两者在植物逆境响应中分别发挥着重要作用。为明确胞质Ca²⁺在外源H₂S促进盐碱胁迫下作物种子萌发中的作用,以裸燕麦（Avena nude）为材料,采用培养皿培养,以混合盐碱（NaCl、Na₂SO₄、Na₂CO₃、NaHCO₃的摩尔比为12：8：1：9）模拟甘肃裸燕麦种植地盐碱环境,蒸馏水为对照,测定了胞外Ca²⁺螯合剂乙二醇-双-（2-氨基乙醚）四乙酸（EGTA）、质膜Ca²⁺通道阻断剂氯化镧（LaCl₃）、液泡Ca²⁺释放抑制剂钌红（RR）和内质网钙泵阻断剂毒胡萝卜素（Thaps）分别与H₂S供体硫氢化钠（NaHS）共处理下种子的发芽势、发芽率、发芽指数、活力指数、平均发芽速率、胚根长和胚芽长7个发芽指标,利用隶属函数分析方法综合评价胞质Ca²⁺对H₂S缓解盐碱胁迫抑制种子萌发的影响。结果表明,随着盐碱胁迫浓度增大,裸燕麦种子的发芽势、发芽率、发芽指数、活力指数、平均发芽速率、胚根长和胚芽长显著下降。与对照相比,15~75 mmol·L^-1盐碱胁迫导致裸燕麦种子萌发的隶属函数综合评价值（D）显著降低,30 mmol·L^-1盐碱胁迫下D值下降了73.1%;100~1 000 μmol·L^-1 NaHS不同程度提高了裸燕麦种子萌发的D值,且100 μmol·L^-1 NaHS缓解30 mmol·L^-1盐碱胁迫下D值下降的作用最大;EGTA、LaCl₃和RR均显著逆转了100 μmol·L^-1 NaHS对30 mmol·L^-1盐碱胁迫下D值下降的缓解作用,而Thaps对NaHS的作用无显著影响。表明胞质Ca²⁺参与外源H₂S促进盐碱胁迫下裸燕麦种子萌发的信号传导过程,且胞质Ca²⁺主要来源于胞外Ca²⁺的内流和液泡中Ca²⁺的释放。     

Exogenous polyamines alleviating salt stress on peanuts (Arachis hypogaea) grown in pots

Aims Soil salinity is a major limiting factor for plant establishment, development and productivity. In recent years, the contradiction between oil crops and food crops for land is increasingly prominent. In order not to take up the land for food, peanut planting on saline-alkali land could be a promising option. However, peanuts have been rarely grown in saline-alkali land, which may be due to the reduction of peanut yield caused by salt stress. Therefore, research of peanut salt resistance has important practical significance.Methods In order to investigate the effects of exogenous polyamines on peanut (Arachis hypogaea) grown in pots under salt stress, ‘Huayu 22’, one of the peanut cultivars, was used as materials by being foliar-sprayed with 1 mmol·L^-1 putrescine (Put), 1 mmol·L^-1 spermidine (Spd) and 1 mmol·L^-1 spermine (Spm) to elucidate the role of exogenous polyamines on peanuts under 150 mmol·L^-1NaCl. Important findingsResults showed that growth, yield, chlorophyll contents and antioxidant enzyme activities of peanut seedling decreased, however, malondialdehyde (MDA) content and relative electrolytic leakage increased under salt stress. Meanwhile, exogenous polyamines significantly improved the activities of superoxide dismutase (SOD), peroxidase (POD) and catalase (CAT), and reduced the relative electrolytic leakage and MDA content in peanut leaves under salt stress and thus alleviating the oxidative damage of salt stress on plasma membrane. It is obvious that exogenous polyamines could improve chlorophyll contents, plant height, number of branch and the amount of dry matter accumulation, even pod yield under salt stress. Among these three polyamines, the effects of exogenous Spm on alleviating salt stress were most effective These results showed that exogenous polyamines, especially Spm, were favorable for the seedlings to increase reactive oxygen metabolism and photosynthesis, which improved peanut growth and reduced the inhibitory effects of salt stress on peanuts.