网地藻多糖清除DPPH·自由基活性的动力学研究

该研究通过超声辅助并采用醇沉、脱蛋白、脱色、干燥的方法,分别检测低(0.1 mg·mL~(-1))、中(0.25mg·mL~(-1))、高(0.5 mg·mL~(-1))三种浓度下的网地藻多糖对DPPH·自由基的清除能力,探讨质量浓度和反应时间对网地藻多糖清除DPPH·自由基活性的变化规律。按照一级反应动力学方程和二级反应动力学方程分别建立反应动力学模型。结果表明:不同的质量浓度和反应时间对网地藻多糖清除DPPH·自由基活性均有影响,网地藻多糖质量浓度提高,其清除DPPH·自由基的能力逐渐加强,当网地藻多糖浓度为0.5 mg·mL~(-1)时,反应20 min,网地藻多糖清除DPPH·自由基的清除率最高为86.06%,其清除DPPH·自由基活性半数清除率(IC_(50))为0.25 mg·mL~(-1)。准一级动力学模型拟合的线性相关性较差,相关系数R~2的范围分别为0.848~0.891;准二级动力学模型拟合的相关系数R~2的范围为0.902~0.967,因此采用二级动力学拟合方程能较好地描述网地藻多糖对DPPH·自由基的清除能力。网地藻多糖在低(0.1 mg·mL~(-1))、中(0.25 mg·mL~(-1))、高(0.5 mg·mL~(-1))三种浓度时对DPPH·的二级反应的清除速率常数(k_2)分别为0.011、0.054、0.421。这说明网地藻多糖随着反应浓度逐渐升高其清除DPPH·自由基的速度越来越快,清除自由基能力也越来越强,结合IC_(50)值来共同评价抗氧化能力,IC_(50)值越小,反应速率值越大,表明其抗氧化活性越好,这与实验得出的数据一致。     

荸荠皮提取物对DPPH自由基清除活性

采用70%丙酮溶液对荸荠皮中抗氧化物质进行提取,得到红棕色浸膏。通过定性及定量方法分析了荸荠皮提取物中可能存在的具有抗氧化活性的物质;采用DPPH自由基法测定了荸荠皮提取物对DPPH自由基的清除能力。结果显示,荸荠皮提取物中含有多酚类和黄酮类等化合物,其多酚含量为3.31%(w/w,以干物质计)。DPPH自由基法显示,荸荠皮提取物具有一定的清除DPPH自由基能力,其清除能力与提取物浓度之间显示出良好的剂量-效应关系。该提取物(IC50值为130.37 ppm)对DPPH自由基清除能力略低于BHT(IC50值为94.16 ppm)。     

短双歧杆菌A04菌株体外清除自由基的研究

采用化学比色法研究了短双歧杆菌A04菌株及其菌体破碎物对DPPH自由基、脂自由基的清除能力,采用化学发光法检测了其对DNA损伤的保护作用,应用电子自旋共振(ESR)法测定了其清除氧自由基的能力。结果显示:短双歧杆菌A04菌株及其菌体破碎物均具有明显的抗脂质过氧化能力,能有效地清除DPPH和活性氧自由基,同时还能很好地保护DNA免受自由基损伤。     

咪唑类氮氧自由基的合成及其DPPH清除能力的研究

目的:合成8种新型咪唑类氮氧自由基(4a~4h),并探讨其对1,1-二苯基-2-三硝基苯肼自由基(DPPH)的清除作用。方法:本文以2-硝基丙烷为原料,经烷基化、还原、缩合及氧化反应等步骤,合成8种新型咪唑类氮氧自由基(4a~4h)。将4a~4h分别与DPPH作用,使用紫外-可见分光光度法测定其中DPPH的浓度,考察4a~4h对DPPH自由基的清除作用,以四甲基哌啶氮氧自由基(Tempol)作为阳性对照。结果:合成中间体及终产物经~1H NMR、HRMS、EPR等光谱数据确证了结构。通过DPPH自由基清除实验,结果显示所合成的8种新型咪唑类氮氧自由基对DPPH均有清除作用。结论:合成了新型咪唑类氮氧自由基,并对其合成方法进行了重要改进。在对DPPH自由基清除能力方面,8种化合物在一定浓度范围(0.01μmol/mL-2.4μmol/mL)内,清除作用与浓度成依赖性增长关系。其中,4b与Tempol相当,4a优于阳性对照Tempol,具有进一步开发研究的潜在价值。     

楤木根皮多糖硫酸酯的制备、结构表征及抗氧化活性的研究

该研究以产自甘肃徽县太白乡的楤木根皮多糖(ACP)为材料,通过氯磺酸-吡啶法(CSA-Py)合成了楤木根皮多糖硫酸酯(SACP)。通过响应面(RSM)实验确定的最佳反应条件:CSA/Py为2.53,反应时间为5.23 h,反应温度为61.25℃,DS理论最大值为0.57。通过红外光谱分析(FT-IR)、X射线光电子能谱(XPS)对产物进行表征,SACP结构中已引入硫酸基团,S以S~(6+)形式存在。气相色谱-质谱联用法(GC-MS)检测显示,SACP由阿拉伯糖、葡萄糖、半乳糖和甘露糖组成。采用体积排阻色谱-激光光散射联用法(SECLLS)测得的平均分子量(Mw)显示,酸性反应导致Mw降低。体外抗氧化活性发现,SACP有极好的清除O_2~-·的能力,有较好的清除DPPH自由基、·OH自由基的能力,还原力很强,对Fe~(2+)有较好的螯合能力,具有浓度依赖性。从构效关系来看,清除DPPH自由基、·OH自由基、O_2~-·自由基以及还原力的能力均与DS呈正相关。上述研究表明了ACP及SACP的化学结构以及化学修饰对ACP抗氧化活性的影响。     

瘦柄红石蕊次生代谢产物Biruloquinone的抗氧化作用研究

讨论了从瘦柄红石蕊Cladonia macilenta发酵液中分离得到的一种自然界罕见的菲醌化合物biruloquinone的体外抗氧化能力;分别采用DPPH·自由基清除法和ABTS·+自由基清除法对其抗氧化活性进行测定。结果显示,biruloquinone具有较高的抗氧化活性,且在检测浓度范围内对自由基的清除效果呈现剂量依赖关系,在浓度分别为100μg/m L和1.2 mmol/L时对DPPH·和ABTS·+自由基清除能力最大值分别达到90.83%和75.39%,其自由基半数清除浓度(EC50)分别为24.91μg/m L和0.488 mmol/L,在ABTS·+法中,biruloquinone的总抗氧化能力为2.5 TEAC。     

紫薇花的抗氧化活性研究

采用DPPH法、ABTS法和FRAP三种测定法对银薇和红花紫薇体外抗氧化活性进行综合评价,并与阳性对照二丁基羟基甲苯(BHT)比较。研究结果发现紫薇花具有较好的抗氧化活性。银薇乙酸乙酯部位清除DPPH自由基的能力(IC50=7.4μg/m L)、清除ABTS自由基的能力(IC50=1.8μg/m L)和还原Fe3+的能力(TEAC=2664.7μmol/g)均强于阳性对照BHT(DPPH方法:IC50=23μg/m L;ABTS方法:IC50=2.3μg/m L;FRAP方法:TEAC=1532.7μmol/g),银薇乙酸乙酯部位抗氧化能力最强。     

荸荠皮多糖体外清除自由基活性的研究

采用DPPH自由基法、邻苯三酚自氧化法和水杨酸法分别表征了荸荠皮多糖清除DPPH自由基(DPPH.)、超氧阴离子自由基(O2-.)和羟基自由基(.OH)的能力。结果显示,脱蛋白和未脱蛋白荸荠皮多糖具有清除自由基的活性,但该活性明显低于茶多酚。脱蛋白多糖清除DPPH.的能力高于未脱蛋白多糖,其清除50%DPPH.的作用质量浓度(EC50)分别为50.26 mg.L-1和76.22 mg.L-1。两种多糖清除.OH和O2-.的能力相当,其EC50(g.L-1)分别为0.118和0.124以及10.87和9.53。     

洋虫成虫脱脂蛋白酶解液的抗氧化作用

对洋虫Martianus dermestoides Chevrolat成虫脱脂蛋白酶解液的抗氧化作用进行了研究。用木瓜蛋白酶水解洋虫成虫脱脂蛋白,用截留分子量分别为10 kDa和6 kDa的超滤膜将其分离成3个组分,用邻苯三酚 鲁米诺发光法、DPPH自由基清除法、Fenton法和Oyaizu法,分别测定不同分子量的洋虫成虫脱脂蛋白酶解液清除超氧阴离子自由基、DPPH自由基及羟基自由基的能力。结果表明：洋虫成虫蛋白酶解液3个组分都有很好的清除自由基能力,且还原性较强,以分子量＜6 kDa的组分清除效果最佳(P＜0.05)。结果揭示洋虫成虫脱脂蛋白酶解液具有很好的抗氧化作用。     

木犀草素-锡(Ⅱ)配合物的合成、表征及抗氧化活性研究

木犀草素与金属离子有较强的配位能力,形成配合物后,活性会发生变化,因此研究了木犀草素与锡(Ⅱ)配合物的合成及其抗氧化活性。采用紫外可见分光光度法、红外光谱法和核磁共振氢谱法对配合物的结构进行表征,并通过DPPH自由基法和邻二氮菲-Fe2+法分别测定了木犀草素-锡(Ⅱ)配合物对DPPH自由基和羟基自由基(.OH)的清除作用。结果表明,木犀草素与锡(Ⅱ)发生配位的位点在5-OH～4-C=O位和3’,4’-OH位,木犀草素-锡(Ⅱ)配合物具备一定的清除DPPH自由基和.OH自由基的性能,但是由于二价锡离子与木犀草素分子中的活性位点(酚羟基)发生了配位络合,所以清除上述自由基的性能较木犀草素均有所降低。     

7种广西产甜茶抗氧化活性的比较

通过清除二苯代苦味酰基(1,1-diphenyl-2-picrylhydrazyl,DPPH)法、铁离子还原测定(ferric reducing antioxidant power,FRAP)法、亚铁离子螯合(ferrous ion-chelating,FIC)法、β-胡萝卜素-亚油酸法等4种体外抗氧化活性测定方法,首次比较了3种茶科属茶叶和7种广西产甜茶水提物的抗氧化活性,同时用Folin-Ciocalteus法测定了其总多酚的含量。研究结果表明,多穗柯甜茶和藤茶的总多酚含量高于其他供试品。藤茶具有很好的清除DPPH·的能力,高于绿茶及阳性对照水溶性维生素E(Trolox)和人工合成抗氧化剂二丁基羟基甲苯(butylated hydroxytoluene,BHT)。甜叶菊茶和悬钩甜茶的金属离子螯合能力均高于绿茶。其中,黄杞和牛白藤两种植物的抗氧化活性为首次报道。由此可见,广西产甜茶均具有较高的开发利用价值,是治疗和防治慢性代谢性疾病的重要研究对象。对广西产甜茶的研究对于了解和抢救某些少数民族的历史文化具有重要意义,为别样茶的抗氧化研究奠定了基础,值得进一步探索和开发。     

Antioxidant properties ofErigeron annuus extract and its three phenolic constituents

The antioxidant activity of the extract ofErigeron annuus was assessed by means of two differentin vitro tests: bleaching of the stable 1,1-diphenyl-2-picrylhydrazyl radical (DPPH test) and the scavenging of authentic peroxynitrite in company with peroxynitrite generation from 3-morpholinosydnonimine (SIN-1). In both tests, the 85% aq. MeOH andn-BuOH soluble fractions of the crude extract showed a significant scavenging effect on peroxynitrite and DPPH radical in comparison to L-ascorbic acid. And bioassay-guided fractionation of then-BuOH soluble fraction led to the isolation of three compounds: Apigenin (1), quercetin-3-O-glucoside (2), and caffeic acid (3). The structures of the isolated compounds were elucidated on the basis of their spectroscopic data and their antioxidant activities were measured by determining their capacity to scavenge peroxynitrite and the DPPH radical.     

花脸香蘑菌丝体提取物的体外抗氧化活性

分别测定花脸香蘑Lepista sordida发酵菌丝体不同浓度乙醇溶剂提取液在4种抗氧化模型中的抗氧化作用。结果表明, 各种菌丝体提取液对二苯基苦味酰基苯肼自由基(·DPPH)和羟自由基(·OH)均有显著的清除作用, 其清除作用随着乙醇溶剂浓度的提高而降低: 在3 g/L菌丝生药浓度时, 去离子水提取物对DPPH自由基和羟自由基的清除率分别为90.55%和81.9%; 在6 g/L菌丝生药浓度时, 50%乙醇和70%乙醇提取物对DPPH自由基的清除率分别为53.7%和45.2%, 对羟自由基的清除率分别为79.4%和78.4%。各菌丝提取物也具有极强的抗脂质过氧化能力, 在5 g/L菌丝生药浓度64 h内, 水提物、50%乙醇和70%乙醇提取物对亚油酸过氧化物的抑制率分别为100%、96%和89.2%。在一定浓度下, 各提取液对邻苯三酚自氧化也均有抑制作用。     

Free radical scavenging activity of vanillin and o-vanillin using 1,1-diphenyl-2-picrylhydrazyl (DPPH) radical

Vanillin, a plant derived natural product, used as food flavoring agent and its positional isomer o-vanillin, have been tested for their ability to scavenge 1,1-diphenyl-2-picrylhydrazyl (DPPH) radical using high performance liquid chromatography (HPLC). Trolox, a water-soluble analogue of vitamin E and a well-known antioxidant was used as a reference compound. The DPPH radical was monitored at 517 nm and its retention time was 8.6 min. From the decrease in optical density of DPPH radical in the presence of the test compounds, it was observed that o-vanillin was a more effective scavenger than vanillin. At equimolar concentrations (1 mM), vanillin and o-vanillin exhibited 22.9% and 66.4% DPPH radical scavenging activity, respectively. The kinetics of the reaction of vanillin and o-vanillin with DPPH radical was studied using stopped flow spectrophotometry and their rate constants were estimated to be 1.7 +/- 0.1 M(-1)s(-1) and 10.1 +/- 0.8 M(-1)s(-1), respectively. In comparison, the rate constant for the reaction of trolox with DPPH was estimated to be 360.2 +/- 10.1 M(-1)s(-1). These scavenging reactions involve electron/H-atom transfer from antioxidant to DPPH. To confirm this, one electron reduction potentials of these compounds were estimated using cyclic voltammetry which showed that o-vanillin was more easily oxidized than vanillin. The reduction potential for o-vanillin was about 1.5 times that of trolox. These results demonstrate that o-vanillin is a more potent antioxidant than vanillin.     

Quantitative structure-activity relationship analyses of antioxidant and free radical scavenging activities for hydroxybenzalacetones

Antioxidant activities for a series of hydroxybenzalacetones, OH-BZ, were evaluated by measuring inhibitory potencies of OH-BZ against lipid peroxidation induced by t-BuOOH or gamma-irradiation. Their quantitative structure-activity relationship (QSAR) studies indicated that the activities are mainly governed by electronic and steric factors. To rationalize these results, we also performed QSAR analyses for DPPH radical scavenging activities of OH-BZ, which indicated that antioxidant and radical scavenging activities could be expressed by the same physicochemical parameters but the hydrogen bonding behavior of phenolic OH varies with the reaction medium.     

Screening of free radical scavengers from Erigeron breviscapus using on-line HPLC-ABTS/DPPH based assay and mass spectrometer detection

Erigeron breviscapus is a well-known traditional Chinese herbal medicine. In this study, on-line HPLC-ABTS/DPPH assay coupled with MS detection were applied to screen and identify the free radical scavengers in 70% methanol extracts of E. breviscapus. Using on-line HPLC-ABTS-MS and HPLC-DPPH-MS assay, 13 radical scavengers (including 4-O-caffeoylquinic acid (4-CQA) (1), 9-caffeoyl-2,7-anhydro-2-octulosonic acid (9-COA) (2), 3-caffeoyl-2,7-anhydro-3-deoxy-2-octulopyranosonic acid (3-CDOA) (3), erigeside I (4), quercetin-3-O-glucuronide (5), eriodictyol-7-O-glucuronide (6), scutellarin (7), 1,4-di-O-caffeoylquinic acid (1,4-di-CQA) (8), 3,5-di-CQA (9), 1-malonyl-3,5-di-CQA (10), erigoster B (11), 4,5-di-CQA (12) and 4,9-di-CDOA (13)) and 9 radical scavengers (including 1, 4, 7, 8, 9, 10, 11, 12 and 13) were discovered, respectively. Furthermore, the anti-oxidative activities of 4 compounds, including 7, 9, 11 and 12 were evaluated. Reverse anti-oxidative activity order of scutellarin and 3,5-di-CQA was observed in on-line HPLC-ABTS assay and on-line HPLC-DPPH assay. To validate their anti-oxidative activities, the off-line ABTS and DPPH assays were performed. Given sufficient reaction time, 3,5-di-CQA showed higher activity than scutellarin, which was consistent with the order obtained in on-line HPLC-ABTS assay. These results revealed that on-line HPLC-ABTS assay is a more sensitive method for screening and determining free radical scavengers, especially more suitable for those compounds with slower reaction kinetics.     

瓦宁木层孔菌中多酚和黄酮类成分分离及清除自由基活性的研究

采用硅胶和反相C18柱层析方法,首次从瓦宁木层孔菌中分离得到了5个化合物,运用NMR波谱法分析和鉴定为樱花亭、7-甲氧基二氢莰非素、二氢莰非素、4-(3,4-二羟苯基)-3-丁烯-2-酮、hispolon。并通过建立体外二苯基苦味酰基苯肼自由基（·DPPH）、超氧阴离子自由基（·O2?）以及羟自由基（·OH）发生体系,研究了5个化合物对·DPPH、·OH和·O2?的清除作用。结果表明当浓度达到100μg/mL时,化合物4-(3,4-二羟苯基)-3-丁烯-2-酮和hispolon对·DPPH清除率分别为92%和93%,对·OH的清除率分别为90%和95%,而对·O2?的清除率分别为70%和77%,略低于清除·DPPH和·OH的能力;二氢莰非素对·O2?自由基的清除率为39%,强于清除·OH和·DPPH的能力;而樱花亭和7-甲氧基二氢莰非素对3种自由基的清除率均低于30%。2个多酚类化合物清除自由基的能力均强于3个黄酮类化合物。5个化合物清除自由基能力均表现出一定的浓度依赖性。     

Antioxidative effect of melatonin on DNA and erythrocytes against free-radical-induced oxidation

The aim of this work is to investigate the antioxidative effect of melatonin (N-acetyl-5-methoxytryptamine) on the oxidation of DNA and human erythrocytes induced by 2,2'-azobis(2-amidinopropane hydrochloride) (AAPH). First, the 50% inhibition concentration (IC50) of melatonin is measured by reacting with two radical species, i.e., 2,2'-azinobis(3-ethylbenzothiazoline-6-sulfonate) radical cation (ABTS*+) and 2,2'-diphenyl-1-picrylhydrazyl (DPPH). The IC50 of melatonin are 75microM and 300microM when melatonin reacts with ABTS*+ and DPPH, respectively. Especially, the reactions of melatonin with ABTS*+ and DPPH are the direct evidence for melatonin to trap radicals. Then, melatonin is applied to protect DNA and human erythrocytes against oxidative damage and hemolysis induced by 2,2'-azobis(2-amidinopropane hydrochloride) (AAPH). The presence of melatonin prolongs the occurrence of the oxidative damage of DNA and hemolysis of erythrocytes, generating an inhibition period (t(inh)). The proportional relationship between t(inh) and the concentration of melatonin ([MLT]) is treated by the chemical kinetic equation, t(inh)=(n/R(i))[MLT], in which n means the number of peroxyl radical trapped by an antioxidant, and R(i) stands for the initiation rate of the radical reaction. It is found that every molecule of melatonin can trap almost two radicals in protecting DNA and erythrocytes. Furthermore, quantum calculation proves that the indole-type radical derived from melatonin is much stable than amide-type radical. Finally, melatonin is able to accelerate hemolysis of erythrocytes induced by hemin, indicating that melatonin leads to the collapse of the erythrocyte membrane in the presence of hemin. This may provide detailed information for the usage of melatonin and helpful reference for the design of indole-related drugs.     

蛹虫草无性型菌丝体提取液体外抗氧化活性研究

分别测定了蛹虫草无性型菌丝体不同溶剂提取液在不同抗氧化模型中的抗氧化作用。结果表明,各种提取液对二苯基苦味酰基苯肼自由基(·DPPH)和羟自由基(·OH)均有显著的清除作用:在50mg/mL时,去离子水、70%乙醇和70%丙酮提取物对DPPH自由基的清除率分别为89.2%、83.6%和75.9%;70%乙醇提取物在30mg/mL时对·OH自由基的清除率达到100%;在50mg/mL时70%丙酮和去离子水提取物的·OH自由基清除率分别为95.6%和89.6%。在一定浓度下,各提取液对邻苯三酚自氧化也均有抑制作用;不同溶剂提取物的还原能力强弱为:70%乙醇>去离子水>70%丙酮。各种提取物的抗氧化组分不同,提取物浓度与抗氧化性成正相关。     

Sulfated modification and antioxidant activity of exopolysaccahrides produced by Enterobacter cloacae Z0206

Nine modification conditions were designed to sulfate exopolysaccharides (EPS) produced by Enterobacter cloacae Z0206 by chlorosulfonic acid-pyridine (CSA-Pyr) method according to the orthogonal test and focusing on three affecting factors such as the ratio of CSA to Pyr, reaction temperature and reaction time. And nine sulfated derivatives with various degrees of substitution (DS) were obtained. Their antioxidant activities were evaluated in vitro, by scavenging abilities on superoxide radical and hydroxyl radical. The results indicated that sulfated derivatives of EPS showed noticeable effects on scavenging superoxide radical and hydroxyl radical compared with native one, and sulfated derivative with moderate DS of 0.60 showed highest antioxidant activities. The optimum sulfated conditions of EPS were the ratio of CSA to Pyr of 1:2, the reaction time of 2h and reaction temperature of 70 °C.