商陆和烟草对锰胁迫的抗氧化响应研究

研究植物的重金属累积能力对于植物修复和植物冶金意义重大.Mn超累积植物商陆(Phytolacca americana L.)的耐性/累积机制至今还不清楚,为了研究商陆在Mn胁迫下的抗氧化酶作用,将萌发6周的商陆和烟草幼苗分别放入1 mmol·L~(-1)或3 mmol·L~(-1)的1/2 Hoagland营养液处理4 d,实验表明商陆叶片光合速率降低幅度显著低于烟草,而烟草MDA含量和电解质渗漏量增加幅度大于商陆.如1 mmol·L~(-1) Mn处理4 d后,与对照相比,商陆和烟草的光合速率分别降低13.3%和75.5%;烟草MDA含量和电解质渗漏量分别增加347.3%和120.1%,而商陆的MDA含量和电解质渗漏量没有明显增加,表明Mn胁迫对超累积植物引起的氧化损伤明显低于非累积植物.随着Mn处理浓度的提高和时间的延长,2种植物叶片SOD和POD活性均迅速增加,其中商陆SOD活性的增加幅度大于烟草;另外,商陆CAT活性持续上升,而烟草CAT活性显著下降.如在1 mmol·L~(-1) Mn处理下,商陆SOD、POD和CAT活性分别提高161.1%、 111.3%和17.5%;烟草SOD和POD提高55.5%和206.0%,而CAT下降15.6%,表明商陆的抗氧化酶,特别是CAT,能够有效地清除Mn毒产生的自由基.这些结果说明抗氧化酶的抗氧化能力是重金属累积植物商陆的Mn耐性机制之一.     

镧对UV-B胁迫下大豆幼苗类黄酮含量与抗氧化能力影响

为进一步认识La(Ⅲ)提高类黄酮含量及减轻UV-B辐射伤害植物机制,以大豆幼苗为材料,采用水培实验的方法研究了La(Ⅲ)对UV-B辐射胁迫下大豆幼苗类黄酮抗氧化能力的动态影响.结果表明, UV-B辐射(T1:0.15W·m-2和T2:0.45W·m-2)胁迫下,大豆幼苗类黄酮含量在胁迫期和恢复期均先升后降,质膜透性、MDA含量先升(1～5d)后降(6～11d),类黄酮对O·-2和·OH的清除率与其含量变化趋势近同.各处理组类黄酮含量La(Ⅲ) UV-B>UV-B>La(Ⅲ)>CK, La(Ⅲ) T1>La(Ⅲ) T2;质膜透性、MDA含量UV-B>La(Ⅲ) UV-B>CK>La(Ⅲ), La(Ⅲ) T2>La(Ⅲ) T1;类黄酮对O-2和·OH清除率La(Ⅲ) UV-B>UV-B>La(Ⅲ)>CK, La(Ⅲ) T1, La(Ⅲ) T2,表明La(Ⅲ)对类黄酮的调控作用,提高了清除活性氧自由基的运行效率,降低了MDA浓度,维持了质膜正常透性,且对低剂量(T1)的防护效果优于高剂量(T2),进而在防御系统层面实现了La(Ⅲ)对UV-B辐射伤害大豆幼苗的防护效应.     

商陆耐重金属Cd关键酶抗氧化酶的研究

研究商陆(Phytolacca americana L.)对Cd胁迫的抗氧化酶响应,对于揭示其耐Cd机制具有重要意义.商陆幼苗在200μmol/L或400 μmol/L CdCl2营养液中处理4 d,叶片活性氧自由基和MDA含量升高,膜透性增加,光合速率降低,表明Cd胁迫诱导产生氧化胁迫.随着Cd处理含量的提高和时间的...     

Oxidative stress mediated cytotoxicity of TiO2 nano anatase in liver and kidney of Wistar rat

This study examined the adverse effects of TiO₂ nanoparticle (nano-TiO₂) on the kidney and liver of Wistar rats. Changes of serum biochemical parameters and pathological lesions indicated that liver and kidney were significantly affected in animals treated with 50?mg?kg^?1 of nano-TiO₂. The inverse relationship between the level of reactive oxygen species and the activities of superoxide dismutase, catalase, and glutathione peroxidase indicates that nano-TiO₂ induces oxidative stress. A significant increase in the apoptosis of liver and kidney in a dose-dependent manner was also observed. The ultrastructural observations confirmed the internalization of nano-TiO₂ and their direct involvement in the mitochondria-mediated cytotoxicity. Data indicated that nano-TiO₂ induce oxidative stress which produces genotoxicity such as oxidative DNA damage, micronuclei (MN) induction, and cell apoptosis in liver and kidney.     

Effects of arsenic on reactive oxygen species and antioxidant defense system in tomato plants

In this study, the generation of reactive oxygen species, the induction of oxidative stress, and the response of the antioxidative system in hydroponically grown tomato plants as the cause of arsenic-induced phytotoxicity are investigated. Reduction in plant growth was measured in terms of dry weight and length of roots and shoots, the latter accumulating more arsenic than the roots. The treatment resulted in increased formation of superoxide anion (O₂^.?), H₂O₂, and thiobarbituric acid reactive substances, which indicate augmented lipid peroxidation. Superoxide dismutase, catalase (CAT), and ascorbate peroxidase activities were increased in arsenic-treated tomato plants while CAT activity was insignificantly increased.     

诺氟沙星对芽期玉米的毒性和氧化损伤研究

畜禽养殖废弃物的农田处置,使大量抗生素进入环境,从而对环境生物产生潜在危害.为了研究诺氟沙星(norfloxacin,Nor)对玉米发芽和幼苗生长的影响,采用水培发芽实验,测定了不同浓度下,诺氟沙星对玉米种子的发芽率和玉米幼苗对诺氟沙星的吸收与传输的影响;另外还研究了诺氟沙星对玉米幼苗生物量、自由基水平、丙二醛(MDA)含量、抗氧化酶活性的影响.结果显示,诺氟沙星能被玉米根吸收并传输到地上部分.0.5mg·L-1～50mg·L-1的诺氟沙星暴露均不影响玉米的发芽率.当诺氟沙星浓度大于1mg·L-1时,幼苗的生长受到抑制,其敏感指标依次为根重>根长>芽长>芽重.诺氟沙星暴露使玉米根、芽中MDA含量明显增加,玉米根中谷胱甘肽硫转移酶(GST),过氧化物酶(POD),超氧化物歧化酶(SOD)和过氧化氢酶(CAT)等抗氧化酶的活度有显著改变,这表明诺氟沙星暴露能够引起玉米体内的氧化损伤.用电子自旋共振结合二级自由基自旋捕获技术测定了玉米根中自由基水平,发现诺氟沙星能够引起玉米根中大量羟基自由基的产生,为诺氟沙星引起玉米幼苗的氧化损伤提供了直接的证据.     

Oxidative stress and DNA damages induced by cadmium accumulation

Experimental evidence shows that cadmium （Cd） could induce oxidative stress and then causes DNA damage in animal cells, however, whether such effect exists in plants is still unclear. In the present study, Vicia faba plants was exposed to 5 and 10 mg/L Cd for 4 d to investigate the distribution of Cd in plant, the metal effects on the cell lipids, antioxidative enzymes and DNA damages in leaves. Cd induced an increase in Cd concentrations in plants. An enhanced level of lipid peroxidation in leaves and an enhanced concentration of H2O2 in root tissues suggested that Cd caused oxidative stress in Vicia faba. Compared with control, Cd-induced enhancement in superoxide dismutase activity was significant at 5 mg/L than at 10 mg/kg in leaves, by contrast, catalase and peroxidaseactivities were significantly suppressed by Cd addition. DNA damage was detected by neutral/neutral, alkaline/neutral and alkaline/alkaline Comet assay. Increased levels of DNA damages induced by Cd occurred with reference to oxidative stress in leaves, therefore, oxidative stress induced by Cd accumulation in plants contributed to DNA damages and was possibly an important mechanism of Cd-phytotoxicity in Vicia faba plants.     

Induction of glutathione reductase enzyme activity by β‐aminobutyric acid in plant leaves

Abstract

Treatment of pea and tobacco leaf discs with the resistance inducer DL‐β‐amino‐n‐butyric acid (BABA) led to a substantial induction of glutathione reductase (GR, E.C. 1.6.4.2.) enzyme activity. After exposure to 1 mM BABA for 96 hrs, the GR activities were 3.2‐fold and 2.9‐fold higher in pea and tobacco leaf discs, respectively, than GR activities in untreated controls. Elevated GR levels may contribute to the antioxidative protection of plants during pathogen attack.     

Phytotoxicity and antioxidative enzymes of green microalga (Desmodesmus subspicatus) and duckweed (Lemna minor) exposed to herbicides MCPA,chloridazon and their mixtures

In this study, we evaluate the toxicity of MCPA (auxin-like growth inhibitor), chloridazon (CHD) (PSII-inhibitor) and their mixtures to floating plants and planktonic algae. Toxicity of MCPA (4-chloro-2-methylphenoxyacetic acid) and CHD (5-amino-4-chloro-2-phenyl-3(2H)-pyridazinone) was first assessed in two growth inhibition tests with Lemna minor (ISO/DIS 20079) and Desmodesmus subspicatus (ISO 8692). Next, herbicide mixtures at concentrations corresponding to the EC values were used to assess their interactive effects, and the biomarkers were: for duckweed fresh weight, frond area, chlorophyll content and number of fronds, and for algae cell count and cell volume. The 3d EC₁₀ and EC₅₀ values using cell counts of D. subspicatus were 142.7 and 529.1 mg/L for MCPA and 1.7 and 5.1 mg/L for CHD. The 7d EC₁₀ and EC₅₀ values using frond number of L. minor amounted to 0.8 and 5.4 mg/L for MCPA and 0.7 and 10.4 mg/L for CHD. Higher sensitivity of reproductive (number of cells/fronds) than growth processes (cell volume/frond area) to herbicides applied individually and in mixtures was especially pronounced in the responses of Desmodesmus. Herbicide interactions were assessed by the two-way ANOVA and Abbott's formula. Generally, an antagonistic interaction with Lemna was revealed by MCPA and chloridazon, whereas additive effect of both herbicides was observed for Desmodesmus. A significant stimulation of SOD and APX activity by binary mixtures was noted in algal cells mainly after 24 and 48 hours of exposure. The extremely high stimulation of the activity of both enzymes was induced by the combination EC₁₀CHD + EC₅₀MCPA (48 h). Presumably due to oxidative stress, the treatment with CHD at concentration EC₅₀ after 72h was lethal for algae grown in aerated cultures, in contrast to standardized test conditions. Taking into account the consequences of risk assessment for herbicide mixtures we can state that a relatively low toxicity, as well as the lack of significant synergy between MCPA and CHD to non-target plants appears to be the most important result.     

Oxidative stress in duckweed (Lemna minor L.) caused by short-term cadmium exposure

The mechanisms of plant defence against cadmium toxicity have been studied by short-term exposure of Lemna minor L. (common duckweed) to concentrations of CdCl2 ranging from 0 to 500microM. High accumulation of cadmium was observed (12,320+/-2155microgg(-1) at 500microM CdCl2), which caused a gradual decrease of plant growth, increased lipid peroxidation, and weakened the entire antioxidative defence. Total glutathione concentration decreased significantly; however, the concentration of oxidized glutathione remained stable. The responses of four antioxidant enzymes showed that catalase was the most inhibited after CdCl2 exposure, ascorbate peroxidase and guaiacol peroxidase moderately, and glutathione reductase least. The total antioxidative potential revealed an induced antioxidative network at 0.1microM CdCl2 (137+/-13.2% of the control) and its reduction to only 47.4+/-4.0% of the control at higher cadmium concentrations. The possible application of the examined biomarkers in ecotoxicological research is discussed.