O3浓度升高和UV-B辐射增强对大豆叶片叶绿素含量和活性氧代谢的影响

以大豆栽培品种铁丰29为试验材料,利用开顶式气室研究O₃浓度升高和UV B辐射增强复合胁迫对大豆叶片叶绿素(Chl)含量、膜脂过氧化程度、活性氧产生速率、抗氧化酶活性和籽粒产量的影响.结果表明： 在大豆整个生育期内,与对照相比,O₃和UV-B单一胁迫及其复合胁迫下的大豆叶片Chl(a+b)、Chl a和Chl b含量均呈下降趋势;相对电导率、丙二醛含量增大,活性氧产生速率和H₂O₂含量增加,超氧化物歧化酶、过氧化物酶和过氧化氢酶活性下降,产量降低.O₃和UV-B复合胁迫加剧了大豆叶片膜脂过氧化程度,促进大豆体内活性氧自由基的产生,使大豆抗氧化能力减弱,叶绿素含量降低,对大豆表现为协同效应.O₃胁迫对大豆叶片的影响与复合胁迫更相近,其原因可能是在复合胁迫中臭氧起主要作用.     

外源表油菜素内酯对NaHCO3胁迫下黄瓜幼苗生长及氧化还原平衡的影响

以‘津研四号’黄瓜为试材,以30 mmol·L^-1NaHCO_3模拟盐碱环境,采用水培法研究了0.2μmol·L^-1外源2,4表油菜素内酯(2,4-epibrassinolide,EBR)对盐碱胁迫下黄瓜幼苗生长和活性氧代谢的影响.结果表明:NaHCO_3胁迫显著诱导了叶片及根系中O2-·的产生和H_2O_2的积累,导致丙二醛含量和电解质渗透率提高.NaHCO_3胁迫下,超氧化物歧化酶、过氧化物酶、过氧化氢酶、抗坏血酸过氧化物酶、脱氢抗坏血酸还原酶、单脱氢抗坏血酸还原酶、谷胱甘肽还原酶活性及还原型抗坏血酸、还原型谷胱甘肽含量随胁迫时间延长呈现先升后降的趋势.外源EBR显著提高了NaHCO_3胁迫下黄瓜叶片和根系中抗氧化酶活性、抗氧化物质的含量以及As A/DHA(双脱氢抗坏血酸)和GSH/GSSG(氧化型谷胱甘肽)比值,维持了植株内的氧化还原平衡,降低了活性氧积累水平,缓解了膜脂过氧化,从而提高了黄瓜幼苗的盐碱耐受性.     

外源表油菜素内酯对NaHCO3胁迫下黄瓜幼苗生长及氧化还原平衡的影响

以‘津研四号’黄瓜为试材,以30 mmol·L^-1 NaHCO₃模拟盐碱环境,采用水培法研究了0.2 μmol·L^-1外源2,4表油菜素内酯(2,4-epibrassinolide,EBR)对盐碱胁迫下黄瓜幼苗生长和活性氧代谢的影响.结果表明: NaHCO₃胁迫显著诱导了叶片及根系中O₂^-·的产生和H₂O₂的积累,导致丙二醛含量和电解质渗透率提高.NaHCO₃胁迫下,超氧化物歧化酶、过氧化物酶、过氧化氢酶、抗坏血酸过氧化物酶、脱氢抗坏血酸还原酶、单脱氢抗坏血酸还原酶、谷胱甘肽还原酶活性及还原型抗坏血酸、还原型谷胱甘肽含量随胁迫时间延长呈现先升后降的趋势.外源EBR显著提高了NaHCO₃胁迫下黄瓜叶片和根系中抗氧化酶活性、抗氧化物质的含量以及AsA/DHA(双脱氢抗坏血酸)和GSH/GSSG(氧化型谷胱甘肽)比值,维持了植株内的氧化还原平衡,降低了活性氧积累水平,缓解了膜脂过氧化,从而提高了黄瓜幼苗的盐碱耐受性.     

Prevention of Intracellular Oxidative Stress to Lens by Pyruvate and Its Ester

Pyruvate is a well-known scavenger of hydrogen peroxide (H₂O₂). In addition, it scavenges superoxide radical (O₂). However, evidence on its intracellular antioxi-dant function is meager at present. Hence, we have examined the effectivekiess of this metabolite and its ethyl ester against intracellular oxidative damage to the lens under organ culture. Menadione, a redoxcycling quinone, was used to generate the reactive oxygen species (ROS). It was found to inhibit lens metabolism as evidenced by a decrease of ATP. Additionally, tissue oxidation was apparent by loss of glutathione (GSH), and increase in the level of oxidized glutathione (GSSG), coupled with increase of the urea soluble proteins (water insoluble). The overall physiological damage was apparent by the inhibition of the Na⁺-K⁺-ATPase dependent cation pump, as evidenced by a decreased rubidium transport. These deleterious effects were attenuated by pyruvate and ethyl-pyruvate. The later was found to be more effective.     

Free Radical Production by Azomethine H: Effects on Pancreatic and Hepatic Tissues

The antimalarial properties of azomethine H represent the basis for its use as a chemotherapeutic agent. This work was carried out in order to verify the biological side effects of azomethine H and to clarify the contribution of reactive oxygen species (ROS) in this process. It was shown that azomethine H increased serum activities of amylase, alanine transaminase (ALT) and the TBARS concentrations, in rats. No changes were observed in glutathione peroxidase and catalase activities. The drug-induced tissue damage might be due to superoxide radicals (O₂), since Cu-Zn superoxide dis-mutase activities were increased by azomethine H treatment. This study allows tentative conclusions to be drawn regarding which reactive oxygen metabolites play a role in azomethine H activity. We concluded that (O₂) maybe produced as a mediator of azomethine H action.     

Nitroxide-Stimulated H2O2 Decomposition by Peroxidases and Pseudoperoxidases

Nitroxide free radicals interact with Hb/metHb, Mb/metMb and with peroxidases/phenols to induce a catalase-like conversion of H₂O₂ to O₂ (catalatic activity), without being substantially consumed in the process. The mechanism of this reaction is postulated to involve a one-electron oxidation of the nitroxide to the immonium oxene, which then reacts further to release oxygen and the nitroxide. An involvement of the immonium oxene in the reaction mechanism is consistent with ferryl heme reduction by nitroxides and a detection of the reduced nitroxide when the reaction mixture is supplemented with the two-electron reductant sodium borohydride. The nitroxide-induced catalatic activity is completely inhibited when the reaction mixture is supplemented with glutathione. Nitroxides suppress free radical formation by hydroperoxide-activated heme proteins, as inferred from their inhibition of the spin-trapping of glutathionyl radicals. H₂O₂ decomposition and a suppression of reactive free radical formation by heme proteins appears to be an antioxidant activity of nitroxides, which is distinct from their previously reported superoxide dismutating activity and which may be a factor in their protective action in models of cardiac reperfusion injury.     

New method for the detection of reactive oxygen species in anti-tumoural activity of adriamycin: a comparison between hypoxic and normoxic cells

Tumour hypoxia plays a role in chemoresistance in several human tumours. However, how hyperbaric oxygen leads to chemotherapeutic gain is unclear. This study investigates the relation of reactive oxygen species (ROS) generation with anti-tumoural effect of adriamycin (ADR) on CCRF-CEM cells under hypoxic (2% O₂) and normoxic (21% O₂) conditions. A new method was used to measure intracellular ROS variations through the fluorescence lifetime of 1-pyrenebutyric acid. At 24 h, ADR, probably via semiquinone radical, enhances ROS levels in normoxic cells compared to hypoxic cells. Long-term studies show that ROS are also generated by a second mechanism related to cell functions perturbation. ADR arrests the cell cycle progression both under hypoxia and normoxia, indicating that oxygen and ROS does not influence the DNA damaging activity of ADR. The findings reveal that moderate improvement of ADR cytotoxicity results from higher ROS formation in normoxic cells, leading to elevated induction of cell death.     

Formation of dioxygen complexes of transition metal chelates in oxygen saturated aprotic solvents. Cyclic voltammetric evidence at a micro glassy carbon disk electrode

Cyclic voltammetry at a micro electrode of Co(II) salen, Fe(II) salen, electrode generated Fe(II)(acac)₂, Fe(II) (salicylaldehyde)₂, Fe(II) (salicylaldoxime)₂, Fe(II) (bipy)₃, Fe(II) (bipy)₂, Co(II) (bipy)₃, Co(II) (benzacac)₂, and electrode generated Co(acac)₂ in oxygen saturated aprotic solvents show positive shift of the O₂ sigmoidal wave, as well as enhancement of the limiting current in the case of the first five compounds. In the case of Co(II) (bipy)₃ the slope of the sigmoidal wave due to O₂ becomes more positive, while for the other two Co(II) complexes there is no change except a small decrease in the wave height. The data are used to correlate and predict the O₂ binding properties of the chelates in solution. The data for the diketone complexes of Co(II) indicate absence of any direct association, which is in line with the interpretation offered in the literature on the mechanism of their catalytic role in the O₂ oxidation of substrates. The mechanism of the autoxidation of dimethylformamide in the presence of Fe(III) (bipy)₃ and Cu(II) (bipy)₂ is elucidated by the observation that these higher valent compounds are reduced to their next lower oxidation state by DMF.     

Iron (III) Stimulation of Lipid Hydroperoxide-Dependent Lipid Peroxidation

In an experimental system where both Fe²⁺ autoxidation and generation of reactive oxygen species is negligible, the effect of FeCl₂ and FeCl₃ on the peroxidation of phosphatidylcholine (PC) liposomes containing different amounts of lipid hydroperoxides (LOOH) was studied; Fe²⁺ oxidation, oxygen consumption and oxidation index of the liposomes were measured. No peroxidation was observed at variable FeCl₂/FeCl₃ ratio when PC liposomes deprived of LOOH by triphenyl-phosphine treatment were utilized. By contrast, LOOH containing liposomes were peroxidized by FeCl₂. The FeCl₂ concentration at which Fe²⁺ oxidation was maximal, defined as critical Fe²⁺ concentration [Fe²⁺]*, depended on the LOOH concentration and not on the amount of PC liposomes in the assay. The LOOH-dependent lipid peroxidation was stimulated by FeCl₃, addition; the oxidized form of the metal increased the average length of radical chains, shifted to higher values the [Fe²⁺]* and shortened the latent period. The iron chelator KSCN exerted effects opposite to those exerted by FeCl₃ addition. The experimental data obtained indicate that the kinetics of LOOH-dependent lipid peroxidation depends on the Fe²⁺/Fe³⁺ ratio at each moment during the time course of lipid peroxidation. The results confirm that exogenously added FeCl₃ does not affect the LOOH-independent but the LOOH-deendent lipid peroxidation; and suggest that the Feg, endogenously generated exerts a major role in the control of the LOOH-dependent lipid peroxidation.     

高浓度镉、锌及其复合作用对烟草抗氧化系统的影响

采用水培方法,研究高浓度镉(0.1 mmol·L^-1 Cd²⁺)、锌(0.15 mmol·L^-1 Zn²⁺)及其复合作用(0.1 mmol·L^-1 Cd²⁺+0.15 mmol·L^-1Zn²⁺)对烟草种子的萌发率、幼苗叶片活性氧(ROS)水平、抗氧化物浓度、抗氧化酶活性及膜脂过氧化程度的影响.结果表明: 单因子条件下,与对照相比,高浓度镉、锌处理烟草种子萌发率降低;叶片超氧自由基(O₂^-· )产生速率与过氧化氢(H₂O₂)含量升高;过氧化氢酶(CAT)、抗坏血酸过氧化物酶(APX)、脱氢抗化血酸还原酶(DHAR)、单脱氢抗坏血酸还原酶(MDAR)和谷胱甘肽还原酶(GR)活性升高;谷胱甘肽(GSH)含量及其与氧化型谷胱甘肽比值(GSH/GSSG)下降;丙二醛(MDA)含量升高.与镉、锌单因子处理相比,镉、锌复合处理的烟草种子萌发率显著升高;O₂^-· 产生速率、H₂O₂和MDA含量降低;CAT、APX、MDAR活性在处理末期升高.镉、锌胁迫对烟草可造成生理水平上的损伤,且毒性效应随着处理时间的延长而增强.镉、锌复合作用可缓解镉、锌单因子胁迫对烟草幼苗的毒害.     

Protective effects of ellagic and chlorogenic acids against oxidative stress in PC12 cells

Following exposure of differentiated neuronal PC12 cells to either t-BHP, hydrogen peroxide (H₂O₂) or FeSO₄ various kinds of reactive oxygen species (ROS) are generated leading to oxidative injury. The protective effects of two plant polyphenols, ellagic (EC) and chlorogenic acid (CGA), as well as of two metabolites, caffeic acid (CA) and ferulic acid (FA), were investigated in preincubation and coincubation experiments with respect to the following parameters: prevention of cell death, GSH depletion, lipid peroxidation and ROS formation.

The polyphenols more efficiently suppressed cytotoxicity and loss of GSH caused by peroxides than by iron, particularly in preincubation. Lipid peroxidation which increased much stronger in response to FeSO₄ was counteracted completely by the polyphenols. In case of iron, however, only coincubation was effective. EA and CGA and the metabolites CA and FA showed excellent elimination of ROS induced by all stressors. These findings suggest that two dietary antioxidants, EA and CGA, may have protective properties against oxidative stress induced in CNS.     

Effects of selenite on O2 consumption, glutathione oxidation and NADPH levels in isolated hepatocytes and the role of redox changes in selenite toxicity

Isolated hepatocytes incubated with selenite (30–100 μM) exhibited changes in the glutathione redox system as shown by an increase in O₂ consumption, oxidation of glutathione and loss of NADPH. Selenite (50 μM) raised O₂ consumption within the 1 h and induced an partial depletion of thiols with a concomitant increase in oxidized glutathione, as well as a decrease in NADPH levels within 2 h. With 100 μM selenite more pronounced effects were obtained such as a total depletion of thiols. This concentration of selenite also lysed cells within 3 h. Arsenite, HgCl₂ and KCN prevented the increase in O₂ uptake, counteracted loss of thiols and delayed selenite induced lysis. p-Tert-butylbenzoic acid, an inhibitor of gluconeogenesis, decreased selenite dependent O₂ consumption and potentiated the effect on NADPH levels as well as the toxic effect. Finally, methionine further enhanced O₂ consumption by selenite and also delayed loss of thiols and potentiated selenite toxicity. These results indicated that selenite catalyzed a reduction of O₂ in glutathione dependent redox cycles with NADPH as an electron donor. With subtoxic concentrations of selenite (50 μM) there were indications that O₂ reduction was terminated by selenite biotransformation to methylated metabolites. With toxic concentrations of selenite (100 μM) it appeared that O₂ reduction was eventually limited by the capacity of the cell to regenerate NADPH. It is suggested that a depletion of NADPH mediated the observed cytotoxicity of selenite.     

Peroxidative Changes in Brain Cortical Fatty Acids and Phospholipids, as Characterized During Fe2+- and Ascorbic Acid-Stimulated Lipid Peroxidation In Vitro

Abstract: The occurrence of peroxidative damage, as distinguished from anaerobic damage, to brain fatty acids and phospholipids was characterized in vitro. Fe²⁺ and ascorbic acid were used to stimulate peroxidation in cortical homogenates from rat brain incubated with or without oxygen. Lipid peroxidation was established in samples incubated with oxygen by increased diene conjugation, accumulation of thiobarbituric acid-reactive material (TBAR) and of lipid-soluble fluorescent products. No peroxidation occurred in samples incubated in the absence of oxygen (100% N₂). Lipid peroxidation was characterized by a selective loss of arachidonic acid and docosahexaenoic acid and by degradation of ethanolamine phosphoglyceride, while choline phosphoglyceride did not change. During the course of peroxidation there were parallel increases in products of lipid peroxidation concomitant with the decrease in polyenoic fatty acids. The maximal changes in diene conjugation and TBAR occurred earlier than the maximal changes in fluorescent material and fatty acids. It is concluded that measurements of changes in brain fatty acid and phospholipid composition may be a useful tool to establishment of whether peroxidative damage is important in vivo in situations with a critically reduced oxygen supply. Estimation of lipid-soluble fluorescence in vivo may also be useful, since it is considered to reflect the accumulation of stable end products of peroxidation.     

Evaluation of Active Oxygen Effect on Photosynthesis of Chlorella vulgaris

The relationship between O₂ and an active oxygen scavenging system in Chlorella vulgaris var.vulgaris (IAM C-534) was investigated. When Chlorella vulgaris was exposed to 2% O₂, only traces of active oxygen scavenging enzymes were found. When the Chlorella vulgaris was treated with 20% or 50% O₂, it was shown that the level of enzyme activity increased as the O₂ concentration increased. An increase in enzyme activity was not found in any specific enzyme but in all of the enzymes, but the level of glutathione and ascorbate remained the same in all the cases. In addition, the photosynthetic efficiency also decreased as the concentration of O₂ was increased. These results suggest that an O₂ enriched environment can lead to an increase in the production of active oxygen species such as O_bullet2 and H₂O₂ and to a decrease in the photosynthetic efficiency in Chlorella vulgaris. The hydroxyl radical (^bulletOH) was detected directly in the Chlorella vulgaris suspension with a spin trapping reagent. It was also clear that the increase in the ^bulletOH intensity as the visible light intensity increased was unrelated to the O₂ concentration. It was suggested that the conditions for producing ^bulletOH and the other active oxygen species were different, and that two types of oxygen stress should exist in the Chlorella vulgaris.     

Mitochondrial complex III is required for hypoxia-induced ROS production and cellular oxygen sensing

Multicellular organisms initiate adaptive responses when oxygen (O₂) availability decreases, but the underlying mechanism of O₂ sensing remains elusive. We find that functionality of complex III of the mitochondrial electron transport chain (ETC) is required for the hypoxic stabilization of HIF-1 and HIF-2 and that an increase in reactive oxygen species (ROS) links this complex to HIF- stabilization. Using RNAi to suppress expression of the Rieske iron-sulfur protein of complex III, hypoxia-induced HIF-1 stabilization is attenuated, and ROS production, measured using a novel ROS-sensitive FRET probe, is decreased. These results demonstrate that mitochondria function as O₂ sensors and signal hypoxic HIF-1 and HIF-2 stabilization by releasing ROS to the cytosol.     

Acutely administered melatonin reduces oxidative damage in lung and brain induced by hyperbaric oxygen

Pablos, Marta I., Russel J. Reiter, Jin-Ing Chuang, GenaroG. Ortiz, Juan M. Guerrero, Ewa Sewerynek, Maria T. Agapito, DanielaMelchiorri, Richard Lawrence, and Susan M. Deneke. Acutely administered melatonin reduces oxidative damage in lung and brain induced by hyperbaric oxygen. J. Appl.Physiol. 83(2): 354-358, 1997.Hyperbaric oxygenexposure rapidly induces lipid peroxidation and cellular damage in avariety of organs. In this study, we demonstrate that the exposure ofrats to 4 atmospheres of 100% oxygen for 90 min is associated withincreased levels of lipid peroxidation products [malonaldehyde(MDA) and 4-hydroxyalkenals (4-HDA)] and withchanges in the activities of two antioxidative enzymes[glutathione peroxidase (GPX) and glutathione reductase (GR)], as well as in the glutathione status in the lungs and in the brain. Products of lipid peroxidation increased after hyperbaric hyperoxia, both GPX and GR activities were decreased, and levels oftotal glutathione (reduced+oxidized) and glutathione disulfide (oxidized glutathione) increased in both lung and brain areas (cerebralcortex, hippocampus, hypothalamus, striatum, and cerebellum) but not inliver. When animals were injected with melatonin (10 mg/kg) immediatelybefore the 90-min hyperbaric oxygen exposure, all measurements ofoxidative damage were prevented and were similar to those in untreatedcontrol animals. Melatonin's actions may be related to a variety ofmechanisms, some of which remain to be identified, including itsability to directly scavenge free radicals and its induction ofantioxidative enzymes via specific melatonin receptors.

     

臭氧浓度升高对坪用高羊茅生长、亚细胞结构及活性氧代谢的影响

通过开顶箱(OTCs)模拟,以环境臭氧(O₃)浓度约40 nmol·mol^-1为对照,研究大气O₃浓度升高(80和160 nmol·mol^-1O₃)对冷季型草坪草高羊茅生长、亚细胞结构及其活性氧代谢的影响.结果表明: 14 d的80 nmol·mol^-1O₃熏蒸使高羊茅株高和叶宽降低,总生物量降低43.7%,老叶变黄,而160 nmol·mol^-1O₃处理高羊茅叶出现大量枯死褐斑,叶尖坏死,新叶卷曲,总生物量降低46.2%,叶肉细胞膜卷曲,叶绿体和线粒体受损严重.与对照相比,80和160 nmol·mol^-1O₃熏蒸下高羊茅叶片超氧阴离子(O₂^-·)产生速率、过氧化氢(H₂O₂)和丙二醛(MDA)含量显著增加,抗氧化酶活性显著升高,但叶片总酚含量和抗氧化能力随O₃浓度升高而先升高后降低.在明显O₃伤害症状出现之前,O₃已对高羊茅的生长和抗氧化代谢产生不利影响;高羊茅抗氧化系统虽对O₃浓度的升高存在一定的适应性反应,但其不能抵御过高浓度的长期胁迫和伤害.     

Dopamine oxidation products inhibit Na+, K+-ATPase activity in crude synaptosomal-mitochondrial fraction from rat brain

The diverse damaging effects of dopamine (DA) oxidation products on brain subcellular components including mitochondrial electron transport chain have been implicated in dopaminergic neuronal death in Parkinson's disease. It has been shown in this study that DA (50-200 μM) causes dose-dependent inhibition of Na₊, K₊-ATPase activity of rat brain crude synaptosomal-mitochondrial fraction during in vitro incubation up to 2 h. The enzyme inactivation is prevented by catalase and the metal-chelator (diethylenetriamine penta-acetic acid) but not by superoxide dismutase or hydroxyl-radical scavengers like mannitol and dimethylsulphoxide (DMSO). Further, reduced glutathione and cysteine, markedly prevent DA-mediated inactivation of Na₊, K₊-ATPase. Under similar conditions of incubation, DA (200 μM) leads to the formation of quinoprotein adducts (protein-cysteinyl catechol) with synaptosomal-mitochondrial proteins and the phenomenon is also prevented by glutathione (5 mM) or cysteine (5 mM).

The available data imply that the inactivation of Na₊, K₊-ATPase in this system involves both H₂O₂ and metal ions. The reactive quinones by forming adducts with protein thiols also probably contribute to the process, since reduced glutathione and cysteine which scavenge quinones from the system protect Na₊, K₊-ATPase from DA-mediated damage. The inactivation of neuronal Na₊, K₊-ATPase by DA may give rise to various toxic sequelae with potential implications for dopaminergic cell death in Parkinson's disease.     

大气臭氧浓度升高对银杏叶片活性氧代谢及相关基因表达的影响

采用开顶式气室熏蒸法,设置自然条件下臭氧(O₃)浓度(对照,约40 nmol·mol^-1)、80、160及200 nmol·mol^-14个臭氧浓度,观测了不同浓度臭氧条件下银杏叶片可见伤害、活性氧生成量、抗氧化酶活性及相关基因表达变化情况,分析大气臭氧浓度升高对植物活性氧代谢的影响.结果表明: 160和200 nmol·mol^-1 O₃熏蒸明显伤害银杏叶片,80 nmol·mol^-1与对照无差异,无可见伤害.O₃处理20 d后,160和200 nmol·mol^-1条件下银杏叶片的超氧自由基(O₂^-·)产生速率显著高于80 nmol·mol^-1和对照,而80 nmol·mol^-1与对照无差异;O₃处理40 d后,160和200 nmol·mol^-1熏蒸下叶片过氧化氢(H₂O₂)含量显著高于80 nmol·mol^-1和对照,而过氧化氢酶(CAT)活性显著高于80 nmol·mol^-1和对照,各臭氧处理抗坏血酸过氧化物酶(APX)活性均低于对照.熏蒸40 d后,CAT、APX基因的转录表达持续加强;防御素(GbD)的表达强度则随着臭氧浓度的增加及熏蒸时间的延长而呈显著加强.高浓度臭氧胁迫可使银杏叶片活性氧生成量增加、抗氧化酶活性下降、相关基因表达水平上调,有明显可见叶片伤害.