AtWRKY40参与拟南芥干旱胁迫响应过程

以拟南芥(Arabidopsis thaliana)野生型、AtWRKY40缺失突变体和过表达株系为材料,研究AtWRKY40在植物干旱胁迫响应过程中的作用及其生理和分子机制。结果显示,AtWRKY40受干旱胁迫诱导;AtWRKY40缺失导致干旱胁迫下种子萌发率降低,叶片失水加剧,而AtWRKY40过表达植株呈现出相反的表征;干旱胁迫下,At WRKY40缺失突变体植株叶片过氧化氢(H_2O_2)、超氧阴离子(O_2~-·)及丙二醛(MDA)含量显著高于野生型及其过表达株系,超氧化物歧化酶(SOD)和过氧化氢酶(CAT)活性、脯氨酸(Pro)和可溶性糖含量以及相关基因AtCu/ZnSOD、AtCAT1、AtP5C1S、AtG6PD5和AtBAM4表达量显著低于野生型,同时AtWRKY40过表达株系的渗透物质含量和保护酶活性及其基因表达量则高于野生型。由此说明,AtWRKY40通过调节植株抗氧化能力及渗透调节能力参与拟南芥干旱胁迫响应过程。     

拟南芥ABA敏感突变体asm1的分离与鉴定

以拟南芥(Arabidopsis thaliana)为研究材料,从T-DNA突变体库中筛选分离得到1株脱落酸(ABA)敏感突变体asm1(ABA sensitive mutant 1,asm1),在含有ABA的培养基中,与野生型相比,asm1突变体的根伸长明显受到抑制,且其种子萌发结果显示asm1对ABA同样表现出敏感特性。在生长发育方面,asm1突变体抽苔时间提前,植株矮化,并且荚果长度明显小于野生型。利用远红外成像系统分析发现,在干旱胁迫下asm1突变体叶面温度高于野生型;失水率分析显示突变体失水率降低以及水分散失减少。遗传学分析表明,asm1是单基因隐性突变且与一个T-DNA插入共分离;通过图位克隆成功获得候选基因ASM1。RT-PCR结果显示,在突变体中ASM1的表达受到抑制,并且能够调控多种ABA信号通路和胁迫应答基因的表达水平。研究结果表明,ASM1可能参与调控ABA信号转导并应答干旱胁迫。     

干旱胁迫下拟南芥中H_2S与ABA信号关系研究

以野生型拟南芥(WT)、硫化氢(H_2S)合成酶缺失型突变体lcd、脱落酸(ABA)合成缺失型突变体aba1实生苗为材料,以0.3 mol·L^-1甘露醇模拟干旱胁迫,研究干旱胁迫对ABA含量、H_2S含量的影响,及其在拟南芥抵抗干旱胁迫中的作用及信号关系。结果显示:干旱胁迫显著提高LCD和ABA1基因相对表达以及H_2S含量,ABA含量;干旱胁迫显著抑制突变体lcd、aba1的种子萌发;干旱胁迫下,外施NaHS促进干旱胁迫下WT、lcd和aba1中內源H_2S的产生及上调LCD、ABA1基因相对表达,而外施ABA提高干旱胁迫下WT、aba1中H_2S含量及LCD、ABA1基因相对表达,但是对lcd中H_2S含量及LCD基因相对表达没有显著影响。研究结果表明,信号分子H_2S和ABA在拟南芥的干旱胁迫响应中发挥一定的作用,且H_2S位于ABA的下游参与调控拟南芥的信号过程。     

水稻含有B-box锌指结构域的OsBBX25蛋白参与植物对非生物胁迫的响应

锌指蛋白在调控植物生长发育和应对逆境过程中发挥着重要作用.为进一步研究锌指类蛋白参与植物非生物胁迫响应的分子机制,对水稻(Oryza sativa)中一个编码含有B-box锌指结构域蛋白的OsBBX25基因进行了功能分析.OsBBX25受盐、干旱和ABA诱导表达.异源表达OsBBX25的转基因拟南芥(Arabidopsis thaliana)与野生型相比对盐和干旱的耐受性增强,且盐胁迫条件下转基因植物中KIN1、RD29A和COR15的表达上调,干旱胁迫下KIN1、RD29A和RD22的表达上调.外源施加ABA时,转基因植物的萌发率与野生型之间没有明显差异.OsBBX25可能作为转录调控的辅助因子调节胁迫应答相关基因的表达,进而参与植物对非生物胁迫的响应.     

陆地棉GhPYR1基因的克隆和功能分析

植物激素脱落酸(Abscisic acid,ABA)在植物应对干旱、盐碱等逆境胁迫以及植物种子萌发、根伸长、芽休眠等阶段发挥重要作用。PYR/PYL/RCAR蛋白家族是ABA受体,与ABA结合后能够启动ABA信号传导通路,诱导ABA应答基因的表达。利用电子克隆和RT-PCR技术从陆地棉中克隆了Gh PYR1基因,其编码的Gh PYR1蛋白与拟南芥中At PYR1蛋白相似度为73%。将Gh PYR1蛋白序列与拟南芥14个PYR/PYL/RCAR家族成员蛋白序列进行比对并构建进化树,发现它与拟南芥PYR/PYL/RCAR蛋白亚家族III亲缘关系最近。过表达Gh PYR1基因的T3代拟南芥在外源ABA处理下,其种子萌发和初期根生长均滞后于野生型,表现出对ABA更加敏感;高盐和干旱胁迫对转基因种子的萌发抑制更强烈,但苗期胁迫处理下转基因拟南芥的长势却明显优于野生型;同时在外源ABA诱导条件下ABA应答基因RD29A、RAB18的表达量较野生型有明显提高。以上结果说明Gh PYR1基因编码的蛋白是ABA的受体,过表达该基因能够提高植物对ABA的敏感性和增强应对逆境胁迫的能力。     

异源表达CkLEA1基因增强了拟南芥对非生物胁迫的耐受性

植物在生长过程中会受到各种非生物胁迫的伤害,导致生长发育和产量受到严重影响,胚胎晚期丰富蛋白（late embryogenesis abundant proteins,LEA蛋白）在植物抵抗非生物胁迫过程中起着重要的保护作用。在前期的研究基础上,将受多种胁迫诱导的柠条锦鸡儿CkLEA1（GenBank登录号KC309408）基因转入野生型拟南芥,通过实时荧光定量PCR从7株T₃代纯合体中筛选出3个转基因株系做进一步研究。种子萌发率实验发现,在200 mmol/L NaCl和400 mmol/L甘露醇处理下,转基因株系萌发率均高于野生型拟南芥。干旱处理2周大的幼苗后,转基因株系明显比野生型更抗旱,存活率高于野生型,并且失水率低于野生型。同时,转基因株系积累了较少的丙二醛（MDA）,超氧化物歧化酶（SOD）活性和谷胱甘肽（GSH）含量也高于野生型。这些结果表明,柠条锦鸡儿CkLEA1基因在种子萌发阶段提高了拟南芥对盐和渗透胁迫的耐受性,并且提高了转基因拟南芥幼苗生长阶段对干旱胁迫的抵抗能力。     

钙传感蛋白互作激酶CIPK14参与拟南芥盐和ABA胁迫应答调节

钙和蛋白激酶在植物胁迫应答过程中起重要作用．本研究以拟南芥蛋白激酶CIPKl4的T—DNA插入突变体为材料,系统研究了CIPK14基因在不同组织与生长发育期的表达情况,和CIPKl4基因的钙调节属性及其在胁迫应答过程中的作用．研究发现CIPKl4基因在拟南芥根、茎、叶、花各组织器官中都有所表达,其中花器官和根部表达量较为显著;不同阶段比较发现CIPKl4在幼苗期具有较高的转录水平．研究同时发现,ABA和盐胁迫能激活CIPKl4基因的转录;CIPKl4T-DNA插入突变体中一系列胁迫应答基因的转录水平全都不同程度地降低或表达滞后,说明CIPKl4基因在胁迫应答中起作用．另外,CIPKl4突变体的种子萌发和根伸长对各种渗透胁迫敏感,并且ABA合成抑制剂哒草伏（Norflurazon）能部分恢复突变体对ABA,盐等的敏感表型．进一步证明CIPKl4是胁迫应答相关基因．研究还发现,CIPKl4的转录受到极端浓度下外源钙离子的激活,另外在一定胁迫条件下,突变体中RD29A基因的表达对外源钙离子浓度变化不敏感,说明CIPKl4基因功能缺失降低了受钙调节的胁迫相关基因对外源钙的敏感性．相应的表型分析发现,突变体种子萌发和根伸长与野生型相比对外源钙敏感性下降,进一步证明CIPKl4基因接受钙信号调节,并作用于拟南芥ABA和盐胁迫应答信号途径,激活胁迫相关转录因子．     

敲除AMP1基因可以提高干旱响应基因的表达量从而增强拟南芥的抗旱能力

干旱严重影响植物的生长发育及农作物产量,因此研究植物的干旱反应机制显得至关重要.我们发现在拟南芥中一个推测的谷氨酸羧肽酶, AMP1, 其缺失突变体amp1的抗旱能力大大增强.基因芯片分析表明,amp1突变体抗旱能力的提高与许多干旱响应基因的高表达息息相关,例如,在amp1突变体中2个干旱诱导表达的转录因子基因,DREB2A和DREB1A的表达量升高;AT1G61340 (LEA 蛋白)的表达量也升高了很多,它在干旱条件下具有解毒和缓解细胞伤害的作用.而且,在amp1突变体中DREB2A 转录因子的2个下游基因RD29A 和COR47受干旱诱导的表达量和时间都比野生型中高和早. 在突变体中一些参与蛋白代谢、糖代谢和脂代谢的基因上调,一些保护和解毒相关基因表达量也升高,这些都可以给突变体在抗旱反应过程提供一定的保护作用.因此,我们认为AMP1基因在干旱胁迫反应中对干旱响应基因的表达起到一个负调控作用.实验中我们还发现, amp1突变体具有较低的水势与非常发达的根系,这也可能在抗旱反应中起到了一定作用.     

敲除AMP1基因可提高干旱响应基因的表达量从而增强拟南芥的抗旱能力

干旱严重影响植物的生长发育及农作物产量,因此研究植物的干旱反应机制显得至关重要.我们发现在拟南芥中一个推测的谷氨酸羧肽酶,AMP1,其缺失突变体amp1的抗旱能力大大增强.基因芯片分析表明,amp1突变体抗旱能力的提高与许多干旱响应基因的高表达息息相关,例如,在amp1突变体中2个干旱诱导表达的转录因子基因,DREB2A和DREB1A的表达量升高;AT1G61340(LEA蛋白)的表达量也升高了很多,它在干旱条件下具有解毒和缓解细胞伤害的作用.而且,在amp1突变体中DREB2A转录因子的2个下游基因RD29A和COR47受干旱诱导的表达量和时间都比野生型中高和早.在突变体中一些参与蛋白代谢、糖代谢和脂代谢的基因上调,一些保护和解毒相关基因表达量也升高,这些都可以给突变体在抗旱反应过程提供一定的保护作用.因此,我们认为AMP1基因在干旱胁迫反应中对干旱响应基因的表达起到一个负调控作用.实验中我们还发现,amp1突变体具有较低的水势与非常发达的根系,这也可能在抗旱反应中起到了一定作用.     

干旱胁迫下磷脂酶Dδ和9-脂氧合酶对拟南芥茉莉酸合成及种子萌发的影响

以拟南芥哥伦比亚野生型(WT)、磷脂酶Dδ(PLDδ)缺失型突变体pldδ和9-脂氧合酶(9-LOX)缺失型突变体lox1、lox5实生苗为材料,以0.3 mol·L-1甘露醇模拟干旱胁迫,分析PLDδ和9-LOX参与干旱胁迫下拟南芥茉莉酸(JA)生物合成和在种子萌发中作用。结果表明:干旱胁迫显著提高PLDδ和LOX1基因表达以及PLD和LOX酶活性;干旱胁迫下,pldδ突变体幼苗的LOX活性和JA含量显著低于WT,外源添加磷脂酸(PA)后LOX活性和JA含量显著上升,并高于WT;干旱胁迫显著抑制pldδ、lox1和lox5突变体的种子萌发,以对lox1的抑制效果最为明显;干旱胁迫下PLD活性上升与PLDδ基因表达上调有关,LOX活性上升与LOX1和LOX5基因表达上调有关,其中LOX1基因起主要作用;PLDδ/PA位于9-LOX上游参与9-LOX诱导的JA合成过程;PLDδ、LOX1和LOX5基因均参与干旱胁迫下拟南芥的种子萌发,LOX1在此过程中作用最为明显;PLDδ和9-LOX均参与PA和JA介导的种子萌发过程。     

Azospirillum brasilense ameliorates the response of Arabidopsis thaliana to drought mainly via enhancement of ABA levels

Production of phytohormones is one of the main mechanisms to explain the beneficial effects of plant growth‐promoting rhizobacteria (PGPR) such as Azospirillum sp. The PGPRs induce plant growth and development, and reduce stress susceptibility. However, little is known regarding the stress‐related phytohormone abscisic acid (ABA) produced by bacteria. We investigated the effects of Azospirillum brasilense Sp 245 strain on Arabidopsis thaliana Col‐0 and aba2‐1 mutant plants, evaluating the morphophysiological and biochemical responses when watered and in drought. We used an in vitro‐grown system to study changes in the root volume and architecture after inoculation with Azospirillum in Arabidopsis wild‐type Col‐0 and on the mutant aba2‐1, during early growth. To examine Arabidopsis development and reproductive success as affected by the bacteria, ABA and drought, a pot experiment using Arabidopsis Col‐0 plants was also carried out. Azospirillum brasilense augmented plant biomass, altered root architecture by increasing lateral roots number, stimulated photosynthetic and photoprotective pigments and retarded water loss in correlation with incremented ABA levels. As well, inoculation improved plants seed yield, plants survival, proline levels and relative leaf water content; it also decreased stomatal conductance, malondialdehyde and relative soil water content in plants submitted to drought. Arabidopsis inoculation with A. brasilense improved plants performance, especially in drought.     

The genes ABI1 and ABI2 are involved in abscisic acid- and drought-inducible expression of the Daucus carota L. Dc3 promoter in guard cells of transgenic Arabidopsis thaliana (L.) Heynh.

 The ABA INSENSITIVE1 (ABI1) and ABI2 genes encode homologous type-2C protein phosphatases with redundant yet distinct functions in abscisic acid (ABA) responses. Results from Northern blot analysis showed that ABA- and mannitol-inducible expression of the COR47 and COR78/LTI78/RD29A (COR78) genes was more impaired in the abi2 mutant of Arabidopsis thaliana (L.) Heynh than in the abi1 mutant. Furthermore, ABA-plus-mannitol treatments were additive towards COR47 gene expression; however, the ABA-deficient aba1 mutant showed reduced COR expression relative to the wild type in response to mannitol and ABA-plus-mannitol treatments. These results support the notion that drought- and ABA-signalling pathways are separate yet overlapping. To facilitate quantitative analysis of the genetic control of tissue-specific ABA- and desiccation-response pathways, we analyzed ABA- and mannitol-inducible expression of a carrot (Daucus carota L.) Dc3 promoter:uidA (β-glucuronidase; GUS) chimaeric reporter (Dc3-GUS) in transgenic wild-type, ABA-deficient aba1, and ABA-insensitive abi1 and abi2 mutants. The Dc3 promoter directed ABA- and mannitol-inducible GUS expression in Arabidopsis guard cells and the two treatments were additive. The aba1, abi1, and abi2 mutant genotypes had reduced GUS expression in guard cells of cotyledons in response to mannitol, whereas abi1 and abi2 mutants were reduced in ABA-inducible GUS expression, consistent with overlapping ABA- and drought-response pathways. Quantitative fluorometric GUS assays of leaf extracts showed that abi2 mutants responded less to exogenous ABA than did abi1 mutants, and abi2 mutants responded more to mannitol than did abi1 mutants. We conclude that Dc3-GUSArabidopsis is a tractable system in which to study tissue-specific ABA and drought signalling and suggest that ABI2 functions predominantly over ABI1 in COR78 and COR47 gene expression and guard-cell Dc3-GUS expression. Received: 23 May 1999 / Accepted: 3 December 1999     

Expression of an Arabidopsis molybdenum cofactor sulphurase gene in soybean enhances drought tolerance and increases yield under field conditions

LOS5/ABA3 gene encoding molybdenum cofactor sulphurase is involved in aldehyde oxidase (AO) activity in Arabidopsis, which indirectly regulates ABA biosynthesis and increased stress tolerance. Here, we used a constitutive super promoter to drive LOS5/ABA3 overexpression in soybean (Glycine max L.) to enhance drought tolerance in growth chamber and field conditions. Expression of LOS5/ABA3 was up‐regulated by drought stress, which led to increasing AO activity and then a notable increase in ABA accumulation. Transgenic soybean under drought stress had reduced water loss by decreased stomatal aperture size and transpiration rate, which alleviated leaf wilting and maintained higher relative water content. Exposed to drought stress, transgenic soybean exhibited reduced cell membrane damage by reducing electrolyte leakage and production of malondialdehyde and promoting proline accumulation and antioxidant enzyme activities. Also, overexpression of LOS5/ABA3 enhanced expression of stress‐up‐regulated genes. Furthermore, the seed yield of transgenic plants is at least 21% higher than that of wide‐type plants under drought stress conditions in the field. These data suggest that overexpression of LOS5/ABA3 could improve drought tolerance in transgenic soybean via enhanced ABA accumulation, which could activate expression of stress‐up‐regulated genes and cause a series of physiological and biochemical resistant responses.     

OsASR5 enhances drought tolerance through a stomatal closure pathway associated with ABA and H2O2 signalling in rice

Drought is one of the major abiotic stresses that directly implicate plant growth and crop productivity. Although many genes in response to drought stress have been identified, genetic improvement to drought resistance especially in food crops is showing relatively slow progress worldwide. Here, we reported the isolation of abscisic acid, stress and ripening (ASR) genes from upland rice variety, IRAT109 (Oryza sativa L. ssp. japonica), and demonstrated that overexpression of OsASR5 enhanced osmotic tolerance in Escherichia coli and drought tolerance in Arabidopsis and rice by regulating leaf water status under drought stress conditions. Moreover, overexpression of OsASR5 in rice increased endogenous ABA level and showed hypersensitive to exogenous ABA treatment at both germination and postgermination stages. The production of H₂O₂, a second messenger for the induction of stomatal closure in response to ABA, was activated in overexpression plants under drought stress conditions, consequently, increased stomatal closure and decreased stomatal conductance. In contrast, the loss‐of‐function mutant, osasr5, showed sensitivity to drought stress with lower relative water content under drought stress conditions. Further studies demonstrated that OsASR5 functioned as chaperone‐like protein and interacted with stress‐related HSP40 and 2OG‐Fe (II) oxygenase domain containing proteins in yeast and plants. Taken together, we suggest that OsASR5 plays multiple roles in response to drought stress by regulating ABA biosynthesis, promoting stomatal closure, as well as acting as chaperone‐like protein that possibly prevents drought stress‐related proteins from inactivation.