大丽轮枝菌毒素与拟南芥互作反应中SA、NO与H2O2信号的相关性

本文研究了大丽轮枝菌毒素（VD-toxin)与拟南芥互作反应中外源SA、NO供体、NO合酶抑制剂等对拟南芥幼苗H2O2含量的影响,并对H2O2的积累部位进行了DAB组化染色检测。大丽轮枝菌毒素、外源SA、NO供体处理拟南芥幼苗均能诱导H2O2的积累,NO供体的诱导作用最强;NO合酶抑制剂处理则未表现出H2O2含量的增强;H2O2的积累部位主要在叶片的表皮毛和维管束组织。结果表明,在大丽轮枝菌毒素与拟南芥互作反应中,H2O2可能作为信号分子参与了SA和NO调控的拟南芥防卫反应,NO信号与H2O2信号间的关系可能更密切。     

大丽轮枝菌毒素与拟南芥互作反应中SA、NO与H2O2信号的相关性

本文研究了大丽轮枝菌毒素(VD-toxin)与拟南芥互作反应中外源SA、NO供体、NO合酶抑制剂等对拟南芥幼苗H2O2含量的影响,并对H2O2的积累部位进行了DAB组化染色检测.大丽轮枝菌毒素、外源SA、NO供体处理拟南芥幼苗均能诱导H2O2的积累,NO供体的诱导作用最强;NO合酶抑制剂处理则未表现出H2O2含量的增强;H2O2的积累部位主要在叶片的表皮毛和维管束组织.结果表明,在大丽轮枝菌毒素与拟南芥互作反应中,H2O2可能作为信号分子参与了SA和NO调控的拟南芥防卫反应,NO信号与H2O2信号间的关系可能更密切.     

燕麦幼苗对盐胁迫的响应及过氧化氢对响应的调节

为了探讨‘定莜6号’燕麦对盐胁迫的生理生化响应及H2O2的调节作用,采用水培方法,研究外源H2O2对盐胁迫下燕麦活性氧代谢、渗透溶质积累和Na+、K+平衡的影响。结果表明:小于100 mmol·L-1Na Cl未对‘定莜6号’幼苗的生长造成明显影响,150 mmol·L-1及以上浓度Na Cl使幼苗干重和叶片K+/Na+显著降低,O2-·产生速率、H2O2、丙二醛(MDA)、可溶性蛋白质和脯氨酸含量及过氧化氢酶(CAT)、质膜H+-ATP酶活性明显提高,但抗坏血酸(ASA)和谷胱甘肽(GSH)含量变化不大;外施5μmol·L-1H2O2可显著缓解150 mmol·L-1Na Cl胁迫对燕麦幼苗生长的抑制作用,使燕麦叶片超氧化物歧化酶(SOD)、抗坏血酸过氧化物酶(APX)和CAT活性及H2O2、GSH含量明显提高,O2-·产生速率和MDA含量显著降低;5μmol·L-1H2O2还提高了150 mmol·L-1Na Cl胁迫下燕麦叶片可溶性蛋白质、可溶性糖、有机酸和脯氨酸含量及质膜H+-ATP酶活性和K+/Na+,降低了游离氨基酸含量;表明外源H2O2可调控燕麦幼苗活性氧代谢和渗透溶质积累,维持K+、Na+平衡,从而增强耐盐性。     

CO2激光处理对大豆种子萌发及生理的影响

以大豆(Glycine max Merr.)为实验材料,研究了CO2激光不同功率密度和不同时间处理对大豆种子发芽率、淀粉酶活性、可溶性蛋白质、可溶性糖含量和氨基酸含量的影响。结果表明：(1)16mw／mm^2、18mw／mm^2、20mw／mm^2CO2激光处理均能提高种子发芽率、淀粉酶活力、可溶性蛋白质、可溶性糖含量和游离氨基酸含量,其中18mw／mm^2CO2激光处理效果最好;(2)相同功率(18mw／mm^2)不同时间处理均能提高种子发芽率、淀粉酶活力、可溶性蛋白质和游离氨基酸含量,处理时间以75s效果最好。     

外源-氧化氮供体硝普钠对黑麦草幼苗耐碱性的影响

采用营养液砂培方法,研究外源一氧化氮(NO)供体硝普钠(SNP)对NaHCO3胁迫下黑麦草幼苗生长、活性氧代谢和渗透溶质积累的影响.结果表明:60 μmol·L-1 SNP能够缓解100 mmol·L-1NaHCO3胁迫对黑麦草幼苗生长的抑制作用,减缓NaHCO3胁迫导致的叶片O2产生速率、H2O2和丙二醛(MDA)含量的增加,提高NaHCO3胁迫下幼苗叶片超氧化物歧化酶(SOD)、过氧化物酶(POD)、抗坏血酸过氧化物酶(APX)、质膜H+-ATP酶的活性和谷胱甘肽(GSH)、可溶性糖、可溶性蛋白质和脯氨酸的含量及K+/Na+比,降低过氧化氢酶(CAT)活性和抗坏血酸(AsA)含量,对游离氨基酸含量影响不大.上述结果表明,NO可能通过激活抗氧化系统活性、促进渗透溶质积累和改善Na+、K+平衡等缓解碱胁迫对幼苗的伤害,从而提高黑麦草的耐碱性.     

盐碱胁迫下星星草种子萌发过程中氮代谢的初步研究

对不同浓度Ｎａ２ＣＯ３胁迫下星星草种子萌发过程中可溶性蛋白质,游离氨基酸及游离脯氨酸含量的变化进行了研究。结果表明：无盐胁迫下,伴随种子的萌发过程,可溶性蛋白质,游离氨基酸含量不断增加。     

不同生长温度对烟草叶片游离氨基酸含量及脯氨酸和苯丙氨酸代谢的影响

游离氨基酸是烟叶中的重要化合物,它很大程度上影响着烟叶的品质和风味。为了解不同生长温度对烟叶中游离氨基酸的含量及其代谢的影响,通过人工气候室设置均温18.5℃、23.5℃和28.5℃3个动态气温条件,在烟叶从早期生长至成熟的整个时期进行不同生长温度处理,用分光光度法、气相色谱-质谱法和荧光定量PCR分析,研究了不同生长温度下总游离氨基酸含量和单个游离氨基酸含量的变化规律及对脯氨酸和苯丙氨酸代谢的影响。结果表明,不同生长温度对烟叶生长发育过程中游离氨基酸总量和单一游离氨基酸含量有明显影响。其中,随着烟叶生长发育的进行,所含游离氨基酸含量逐渐下降。在不同生长温度处理下,随生长温度升高总游离氨基酸含量下降;各游离氨基酸含量基本上也随生长温度的升高而降低。对脯氨酸代谢相关酶(P5CS,OAT,ProDH)活性以及苯丙氨酸代谢相关酶(PAL,C4H)活性及其基因表达的定量研究表明,其酶活性和基因表达的变化与含量变化的趋势一致。上述研究结果表明,随着烟叶的生长发育和成熟,其游离氨基酸含量逐渐降低,而较低的生长温度有利于烟叶维持较高的游离氨基酸水平。     

低温条件下ABA和钨酸钠对茶树叶片中渗透调节物质含量及抗氧化酶活性的影响

为探讨外源脱落酸( ABA)及其抑制剂钨酸钠对茶树﹝Camellia sinensis ( Linn.) O. Ktze.﹞耐寒性的影响效应,以茶树品种‘龙井43’(‘Longjing 43’)的2年生幼苗为实验材料,在低温(4℃)条件下分别设置50 mg·L-1 ABA和20 mmol·L-1钨酸钠单一及复合处理共6个处理组( T1：仅喷施蒸馏水,对照;T2：仅喷施ABA;T3：仅喷施钨酸钠;T4：同时喷施ABA和钨酸钠; T5：0 h时喷施ABA,24 h时喷施钨酸钠; T6：0 h时喷施钨酸钠,24 h时喷施ABA),对处理0~72 h叶片中渗透调节物质含量和抗氧化酶活性的变化进行了比较分析。结果显示：低温条件下,各处理组幼苗叶片中可溶性糖、游离脯氨酸和可溶性蛋白质含量以及超氧化物歧化酶( SOD)、过氧化氢酶( CAT)和过氧化物酶( POD)活性均在处理初期逐渐升高,之后各指标的变化趋势存在差异。在处理的中后期,除T4处理组的游离脯氨酸含量低于对照组外,各处理组的可溶性糖、游离脯氨酸和可溶性蛋白质含量总体上显著高于对照组;T2处理组的SOD、CAT和POD活性均显著高于对照组,而T3处理组仅SOD活性明显高于对照组,其CAT和POD活性则低于或略高于对照组。对各单一与复合处理组的比较结果显示：T4处理组的SOD和POD活性总体上低于T2处理组,但高于T3处理组;而其CAT活性总体上低于T2和T3处理组。在处理24 h后,T5处理组的可溶性糖、游离脯氨酸和可溶性蛋白质含量以及SOD和POD活性的变化趋势与T2处理组一致;T6处理组的可溶性糖和游离脯氨酸含量及POD活性变化趋势与T3处理组一致,而其可溶性蛋白质含量以及SOD和CAT活性的变化趋势却与T3处理组有一定差异。上述研究结果表明：低温条件下喷施适量的ABA或钨酸钠均可以提升茶树叶片中渗透调节物质含量及抗氧化酶活性,但同时喷施ABA和钨酸钠对茶树叶片中渗透调节物质含量及抗氧化酶活性的影响却不显著。     

不同施氮水平对烟草叶片游离氨基酸含量及脯氨酸和苯丙氨酸代谢的影响

人工施氮量是影响烟叶中游离氨基酸含量的重要因素,而后者很大程度上影响着烟叶的品质和风味。为了解不同施氮量对烟叶中游离氨基酸含量的影响,在大田条件下通过设置施氮量为60 kg/hm~2、90 kg/hm~2和120 kg/hm~2 3个施氮水平进行处理,用分光光度法和气相色谱-质谱联用法分析,研究了不同施氮水平对游离氨基酸含量以及脯氨酸和苯丙氨酸代谢关键酶及其基因表达的影响。结果表明,随施氮水平的不同,烟叶中总游离氨基酸、脯氨酸和苯丙氨酸含量随施氮水平增加而增高;而亮氨酸、异亮氨酸、丙氨酸和4-氨基丁酸含量在施氮水平为60 kg/hm~2时最高。脯氨酸代谢相关酶和苯丙氨酸代谢相关酶活性均随施氮水平升高而增强,其基因相对表达量也随之上调。上述研究结果表明施氮水平可显著影响烟叶中游离氨基酸含量、种类及其代谢过程。     

水杨酸调节决明根系铝诱导的氧化胁迫

水杨酸(Salicylicacid,SA)在调节生物和非生物胁迫,诱导植物氧化胁迫中起着重要的作用,但对铝诱导的氧化胁迫的调节作用尚不清楚。本文研究了SA对决明(CassiatoraL.)根系铝诱导的H2O2和O2-含量变化,包括抗氧化酶活性以及细胞质膜过氧化胁迫变化的影响。介质中20mmol/L铝处理增加质膜透性,导致MDA含量上升及根尖细胞Evansblue染色加重(测定细胞死亡),而外源供给5mmol/LSA能缓解铝诱导的氧化胁迫。SA处理能明显降低根尖H2O2和O2-的含量,但两者含量与CAT、APX和GR的活性变化没有相关性,而与POD活性增加有关。水杨酸诱导H2O2含量的下降与抑制O2-积累和SOD活性有关。结果表明,SA可能激活一条由H2O2介导的、依赖于POD的抗氧化机制来缓解脂质的过氧化作用。     

Involvement of protein kinases and calcium in the * NO-signalling cascade for defence-gene induction in ozonated tobacco plants

This study analyses the signalling pathways triggered by nitric oxide (NO) in response to ozone (O(3)) fumigation of tobacco plants, with particular attention to protein kinase cascades and free cytosolic Ca(2+) in defence-gene activation. NO was visualized with the NO probe DAF-FM. Using a pharmacological approach, the effects of different inhibitors on the expression profiles of NO-dependent defence genes were monitored using RT-PCR. The assay of the kinase activity of the immunoprecipitates complexes shows that O(3) stimulates a 48 kDa salicylic acid (SA)-induced protein kinase (SIPK) in an NO-dependent manner. The O(3)-induced alternative oxidase 1a (AOX1a) and phenylalanine ammonia lyase a (PALa) genes are modulated by phosphorylation by protein kinases, and SIPK might have a role in this up-regulation. By contrast, protein dephosphorylation mediates pathogenesis-related protein 1a (PR1a) expression in O(3)-treated tobacco plants. Ca(2+) is essential, but not sufficient, to promote NO accumulation in ozonated tobacco plants. Intracellular Ca(2+) transients are also essential for PALa up-regulation and cGMP-induced PR1a expression. Partial dependence on intracellular Ca(2+) suggests two different pathways of SA accumulation and PR1a induction. A model summarizing the signalling networks involving NO, SA, and the cellular messengers in this O(3)-induced defence gene activation is proposed.     

Hydrogen Peroxide Stimulates Salicylic Acid Biosynthesis in Tobacco

Hydrogen peroxide induced the accumulation of free benzoic acid (BA) and salicylic acid (SA) in tobacco (Nicotiana tabacum L. cv Xanthi-nc) leaves. Six hours after infiltration with 300 mM H2O2, the levels of BA and SA in leaves increased 5-fold over the levels detected in control leaves. The accumulation of BA and SA was preceded by the rapid activation of benzoic acid 2-hydroxylase (BA2H) in the H2O2-infiltrated tissues. This enzyme catalyzes the formation of SA from BA. Enzyme activation could be reproduced in vitro by addition of H2O2 or cumene hydroperoxide to the assay mixture. H2O2 was most effective in vitro when applied at 6 mM. In vitro activation of BA2H by peroxides was inhibited by the catalase inhibitor 3-amino-1,2,4-triazole. We suggest that H2O2 activates SA biosynthesis via two mechanisms. First, H2O2 stimulates BA2H activity directly or via the formation of its substrate, molecular oxygen, in a catalase-mediated reaction. Second, higher BA levels induce the accumulation of BA2H protein in the cells and provide more substrate for this enzyme.     

Induction of Benzoic Acid 2-Hydroxylase in Virus-Inoculated Tobacco

Salicylic acid (SA) plays an important role in the induction of plant resistance to pathogens. An accompanying article (N. Yalpani, J. Leon, M.A. Lawton, I. Raskin [1993] Plant Physiol 103: 315-321) shows that SA is synthesized via the decarboxylation of cinnamic acid to benzoic acid (BA), which is, in turn, hydroxylated to SA. Leaf extracts of tobacco (Nicotiana tabacum L. cv Xanthi-nc) catalyze the 2-hydroxylation of BA to SA. The monooxygenase catalyzing this reaction, benzoic acid 2-hydroxylase (BA2H), required NAD(P)H or reduced methyl viologen as an electron donor. BA2H activity was detected in healthy tobacco leaf extracts (1-2 nmol h-1 g-1 fresh weight) and was significantly increased upon inoculation with tobacco mosaic virus (TMV). This increase paralleled the levels of free SA in the leaves. Induction of BA2H activity was restricted to tissue expressing a hypersensitive response at 24[deg]C. TMV induction of BA2H activity and SA accumulation were inhibited when inoculated tobacco plants were incubated at 32[deg]C. However, when inoculated plants were incubated for 4 d at 32[deg]C and then transferred to 24[deg]C, they showed a 15-fold increase in BA2H activity and a 65-fold increase in free SA content compared with healthy plants incubated at 24[deg]C. Treatment of leaf tissue with the protein synthesis inhibitor cycloheximide blocked the induction of BA2H activity by TMV. The effect of TMV inoculation on BA2H could be duplicated by infiltrating leaf discs of healthy plants with BA. This response was observed even when applied levels of BA were much lower than the levels observed in vivo after virus inoculation. Feeding tobacco leaves with phenylalanine, cinnamic acid, or o-coumaric acid (putative precursors of SA) failed to trigger the induction of BA2H activity. BA2H appears to be a pathogen-inducible protein with an important regulatory role in SA accumulation during the development of induced resistance to TMV in tobacco.     

小麦叶片顺乌头酸酶对NO和H2 O2 的敏感性

外源一氧化氮（nitric oxide,NO)供体硝普钠（sodium nitroprusside,SNP)和过氧化氢（hydrogen peroxide,H2O2)处理抑制小麦（Triticu aestivum L.)叶片顺乌头酸酶活性,抑制呈明显的浓度及时间效应;同时外源NO衍生代谢物过氧亚硝酸阴离子（peroxynitrite,ONOO^-)的供体3－morpholinosydnonimine hydrochlloride(SIN-1)和水杨酸（salicylic acid,SA)对酶活性也具有抑制作用,而且小麦叶片线粒体顺乌头酸酶对H2O2和SIN－1更敏感。分别以SNP与过氧化氢酶（catalase,CAT)专一性抑制剂氨基三唑（3－amino-1,2,4-triazole,3-AT)处理离体小麦叶片,发现在其内源H2O2含量上升的同时,顺乌头酸酶活性均呈浓度与时间依赖性下降趋势。表明NO除直接抑制顺乌头酸酶活性外,还可能经H2O2介导间接对顺乌头酸酶产生抑制作用。     

Mechanism of peroxidase actions for salicylic acid-induced generation of active oxygen species and an increase in cytosolic calcium in tobacco cell suspension culture

Extracellularly secreted peroxidases in cell suspension culture of tobacco (Nicotiana tabacum L. cv. Bright Yellow-2, cell line BY-2) catalyse the salicylic acid (SA)-dependent formation of active oxygen species (AOS) which, in turn, triggers an increase in cytosolic Ca2+ concentration. Addition of horseradish peroxidase (HRP) to tobacco cell suspension culture enhanced the SA-induced increase in cytosolic Ca2+ concentration, suggesting that HRP enhanced the production of AOS. The mechanism of peroxidase-catalysed generation of AOS in SA signalling was investigated with chemiluminescence sensitive to AOS and electron spin resonance (ESR) spectroscopy, using the cell suspension culture of tobacco, and HRP as a model system of peroxidase reaction. The results showed that SA induced the peroxidase inhibitor-sensitive production of superoxide and H2O2 in tobacco suspension culture, but no production of hydroxy radicals was detected. Similar results were obtained using HRP. It was also observed that SA suppressed the H2O2-dependent formation of hydroxy radicals in vitro. The results suggest that SA protect the cells from highly reactive hydroxy radicals, while producing the less reactive superoxide and H2O2 through peroxidase-catalysed reaction, as the intermediate signals. The formation of superoxide was followed by that of H2O2, suggesting that superoxide was converted to H2O2. In addition, it was observed that superoxide dismutase-insensitive ESR signal of monodehydroascorbate radical was induced by SA both in the tobacco suspension culture and HRP reaction mixture, suggesting that SA free radicals, highly reactive against ascorbate, were formed by peroxidase-catalysed reactions. The formation of SA free radicals may lead to subsequent monovalent reduction of O2 to superoxide.     

Studies on the Salicylic Acid Inducted Lipid Peroxidation and Defense Gene Expression in Tobacco Cell Culture

Salicylic acid (SA) could inhibit catalase activity, induce rapid lipid peroxidation and PR-1 gene expression of the tobacco ( Nicotiana tabacum L. ) cell culture which was incubated with exogenous SA. Ρ-ihydroxybenzene and H2O2 could also induce lipid peroxidation and PR-1 gene expression at different level, but they were not able to inhibit the catalase activity of tobacco cells. Inhi0itors of mRNA and protein-synthesis (a-amanitine and cycloheximide, respectively) could not induce both lipid peroxidation and PR-1 gene expression of tobacco cell culture. However, coordinated action with SA respectively, a-amanitine or cycloheximide was able to induce lipid peroxidation effectively, but strongly blocked the activation of PR-1 gene expression by SA in tobacco cell culture. These results suggested that the generation of reactive metabolites or free radicals, which were induced by SA or other inducers through reaction with catalase or other compounds, initiated lipid peroxidation, subsequently activated pathogen-resistance genes expression. Obviously the lipid peroxidation molecule played an important role in SA signal transduction in tobacco.     

外源CO和NO对水稻种子萌发过程中干旱胁迫损伤的缓解效应

选用水稻品种‘Ⅱ优128’种子为材料,以1.0μmol.L-1高铁血红素(Hematin,H)和200μmol.L-1硝普钠(sodium nitroprusside,SNP)分别作为CO和NO供体,采用PEG-6000模拟干旱胁迫,研究外源CO和NO对干旱胁迫下水稻种子萌发和萌发过程中抗氧化能力的影响。结果表明:高铁血红素和硝普钠处理可以显著提高干旱胁迫下水稻种子的发芽率、芽长和根长;同时显著提高种子淀粉酶活性,显著增加其可溶性糖、可溶性蛋白和脯氨酸含量;还不同程度地诱导增强超氧化物歧化酶(SOD)、过氧化氢酶(CAT)和过氧化物酶(POD)的活性,同时降低质膜相对透性和丙二醛(MDA)含量。研究证实,外源CO和NO可通过调节渗透调节物质含量和保护酶活性来有效缓解干旱胁迫对萌发水稻种子造成的氧化伤害,促进种子萌发生长。     

外源一氧化氮供体硝普钠浸种对盐胁迫下小麦幼苗碳氮代谢及抗氧化系统的影响

预先用0.1mmol/L的SNP(硝普钠,NO供体)浸种,研究NO预处理对120mmol/L NaCl胁迫下两小麦品种(扬麦12和淮麦17)幼苗叶片抗氧化系统、碳氮代谢及蛋白酶活性的影响。结果表明,NO预处理能有效地抑制NaCl胁迫下小麦幼苗叶片超氧阴离子释放(O.2-)和过氧化氢(H2O2)积累,提高超氧化物歧化酶(SOD)和过氧化氢酶(CAT)活性,降低丙二醛(MDA)含量,提高叶绿素、类胡萝卜素和可溶性总糖含量。另外,NO预处理显著提高叶片可溶性蛋白质含量,以及内肽酶和羧肽酶活性。分析表明,NO有利于维持盐胁迫下小麦碳氮代谢正常运转,从而促进植株生长,提高小麦幼苗株高、鲜重和干重。试验条件下,NO对淮麦17的促进作用大于扬麦12。