红背叶提取物的体外抗氧化活性

采用DPPH法、FRAP法、ABTS法和清除羟基自由基法四种抗氧化活性方法,测定了红背叶不同溶剂萃取60%EtOH提取物得到的部位清除自由基的能力.结果表明,乙酸乙酯提取物的抗氧化能力最强,强于阳性对照VC和Trolox;其次是60%乙醇提取物,其抗氧化能力基本与阳性对照BHA相当.     

红花桑寄生叶提取物的抗氧化活性及酚类物质分析

采用DPPH法、TEAC法、FRAP法对红花桑寄生叶不同溶剂提取物的抗氧化活性进行体外评价,并测定其总酚、总黄酮含量。结果表明,溶剂种类对红花桑寄生叶提取物的得率、总酚、总黄酮及抗氧化活性影响显著。在3种评价方法中,不同溶剂提取物的抗氧化活性均表现出不同程度的量效依赖关系。3种溶剂提取物的抗氧化活性强弱依次为丙酮提取物 >甲醇提取物 >水提取物,其中80%丙酮提取物(总酚含量最高,达276.83mg/g)抗氧化活性最强,清除DPPH自由基能力EC₅₀值为0.247,FRAP值(FeSO₄ mmol/100g)为115.81,浓度为1.0mg/ml时,TEAC值为2.04。     

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。     

薏苡根不同极性组分的抗氧化活性分析

目的:提取薏苡根有效成分并比较不同组分的抗氧化活性。方法:利用不同极性的溶剂对薏苡根进行提取,并进行显色反应,通过测定薏苡根的铁还原力,总抗氧化能力和对DPPH自由基清除率的测定,从中比较乙酸乙酯,正丁醇和水三个不同极性部位的体外抗氧化活性。结果:乙酸乙酯部位、水部位、正丁醇部位均含有不同程度的体外抗氧化活性物质,且总抗氧化力和铁还原力与浓度之间有相关性,有较好的量效关系。根据各样品的体外抗氧化活性实验可得出各部位所含抗氧化物质的含量或种类:正丁醇提取物水提取物乙酸乙酯提取物。结论:薏苡根各提取部位均具有一定的抗氧化活性,但抗氧化能力不同,其中正丁醇的抗氧化能力最强。     

诺丽发酵果汁中抗氧化物质的研究

本实验针对茜草科植物诺丽的发酵果汁中抗氧化物质进行了定性和定量研究。采用系统预实验法对其不同极性的洗脱部位可能含有的化学成分进行预实验,探索了各个部位的化学成分。采用DPPH·自由基清除、ABTS+·自由基清除和FRAP三种实验方法对各部位洗脱物的抗氧化活性进行了测定,结果显示50%~90%乙醇洗脱部位抗氧化能力最强,此部位主要含有多酚类、黄酮类、香豆素内酯类和蒽醌类成分,并且研究表明抗氧化能力与多酚成分的含量成极显著相关。本研究结果表明多酚类物质是诺丽发酵果汁发挥抗氧化作用的主要功能成分。     

枸杞子提取液抗氧化活性的研究

用Folin-Ciocalteu法、DPPH法和Fenton法分别对脱脂及未脱脂枸杞子的水和50%、80%、95%乙醇提取液的抗氧化活性进行测定。结果显示:3种方法所得结果具有一致的规律,相同提取条件下,未脱脂枸杞子的抗氧化活性大于脱脂枸杞子;随着乙醇浓度增大,枸杞子提取液的抗氧化活性逐渐减小,即水>50%乙醇>80%乙醇>95%乙醇枸杞子提取液。表明枸杞子中水溶性提取物的抗氧化活性高于脂溶性提取物;不同提取液抗氧化能力的差异说明枸杞子的抗氧化能力是枸杞子中水溶性和脂溶性多种成分协同作用的结果。     

菹草提取物总黄酮、总酚酸和抗氧化活性含量研究

研究菹草提取物的有效成分,测定其总黄酮含量及总酚酸含量,并确定它的乙酸乙酯和石油醚部位的抗氧化活性成分。采用紫外可见分光光度法,以芦丁和没食子酸作为控制材料,测定菹草的石油醚部位及乙酸乙酯部位中总黄酮和总酚酸含量;采用清除DPPH自由基能力测定法、测定总还原能力铁氰化钾法和水杨酸捕捉羟基自由基法来对菹草各组分提取物的抗氧化能力进行研究。菹草中有一定量的黄酮类化合物和酚酸类化合物存在,不同溶剂提取的部位所含有的总黄酮和总酚酸含量是有差异的,石油醚部位的总黄酮含量要高于乙酸乙酯部位的总黄酮含量,并且总酚酸的含量亦是如此;石油醚部位和乙酸乙酯部位的提取物具有清除DPPH、羟基自由基和还原Fe^3+的能力,各部位清除DPPH、羟基自由基的能力和还原Fe^3+的能力随着样品浓度的增大而增大,且乙酸乙酯部位的测定结果均低于石油醚部位。     

卷丝苣苔和勐醒芒毛苣苔抗氧化活性研究

利用3种方法DPPH、ABTS和FRAP分析两种苦苣苔科植物卷丝苣苔和勐醒芒毛苣苔提取物总抗氧化作用.在4种提取物中,卷丝苣苔甲醇提取物对DPPH自由基的清除能力(IC50=4.92μg/mL)比阳性对照BHT作用强(IC50=18.79 μg/mL);卷丝苣苔甲醇提取物对ABTS自由基的清除能力(IC50=11.10 μg/mL)比BHT(IC50=6.04 μg/mL)略低;卷丝苣苔甲醇提取物还原Fe3+的能力(FRAP=2403.77±38.05 μmol TE/g)比BHT(FRAP=1748.49±3.46 μmol TE/g)高.在4种提取物中,卷丝苣苔甲醇提取物抗氧化能力最高.     

丹参生品及炮制品的抗氧化活性研究

采用清除二苯代苦味酰基(DPPH)自由基、清除[2,2'-连氨-(3-乙基苯并噻唑啉-6-磺酸)二铵盐](ABTS)自由基及铁离子还原/抗氧化能力(FRAP)测定法,以二丁基羟基甲苯(BHT)为阳性对照,对丹参生品及炮制品进行抗氧化活性评价。实验结果表明,丹参生品及其炮制品均有一定的抗氧化活性。其中,丹参炭乙酸乙酯部位清除DPPH自由基的能力最强,IC50值为13.9μg/mL;炒丹参乙酸乙酯部位、酒丹参乙酸乙酯部位和丹参炭正丁醇部位清除ABTS自由基能力最强,IC50值均为2.1μg/mL;米丹参乙酸乙酯部位的FRAP值最高为1517.81μmol/g。不同炮制方法对丹参抗氧化活性的能力有所不同,其中,丹参炭的整体抗氧化活性相对较好。     

大血藤抗氧化及抗菌活性研究

本文评价了大血藤乙醇提取物和石油醚、二氯甲烷、乙酸乙酯和水部位的体外抗氧化和抑菌活性以及与总酚含量的相关性。采用清除DPPH自由基法、Fe3+还原力法评价了各部位的抗氧化活性,采用纸片扩散法评价各部位的抑菌活性。采用Folin-Ciocalteu法测定各部位总酚含量,并采用HPLC-UV解析活性部位物质基础。结果表明,水部位清除DPPH能力最强(IC505.53μg/m L),优于对照组Vc,其它部位顺序为乙酸乙酯部位乙醇提取物二氯甲烷部位石油醚部位,还原Fe3+的能力顺序与此相同。总酚含量与抗氧化活性正相关。石油醚部位、二氯甲烷部位、乙酸乙酯部位有中等强度的抑制革兰氏阴性菌作用。表明大血藤可能会成为有价值的天然抗氧化和抗菌资源。     

河南产景天三七抗氧化活性研究

用清除二苯代苦味酰基(DPPH)自由基、2,2′-连氨-(3-乙基苯并噻唑啉-6-磺酸)二氨盐(ABTS)自由基和铁离子还原/抗氧化能力(FRAP)测定法对洛阳和信阳产景天三七(Sedum aizoon)体外总抗氧化活性进行评价,并与阳性对照丁基羟基茴香醚(BHA)、没食子酸丙酯(PG)和二丁基羟基甲苯(BHT)比较。发现洛阳和信阳景天三七有较好的体外抗氧化活性。洛阳和信阳产乙酸乙酯部位活性最强,正丁醇部位活性次之。在6个提取部位中,信阳产景天三七乙酸乙酯部位活性最强,其清除DPPH、ABTS自由基能力强于阳性对照BHA和BHT,还原Fe3+的能力大于阳性对照BHT,洛阳产景天三七乙酸乙酯部位和正丁醇部位活性次之。     

Antimicrobial and antioxidant activities of Gentianella multicaulis collected on the Andean Slopes of San Juan Province, Argentina

The infusion of the aerial parts of Gentianella multicaulis (Gillies ex Griseb.) Fabris (Gentianaceae), locally known as 'nencia', is used in San Juan Province, Argentina, as stomachic and as a bitter tonic against digestive and liver problems. The bioassay-guided isolation of G. multicaulis extracts and structural elucidation of the main compounds responsible for the antifungal and free radical scavenging activities were performed. The extracts had strong free radical scavenging effects in the 1,1-diphenyl-2-picrylhydrazyl (DPPH) assay (45-93% at 10 microg/mL) and ferric-reducing antioxidant power (FRAP) assay at 200 microg/mL. Demethylbellidifolin (4) had high antioxidant activity in the DPPH and FRAP assay. The dermatophytes Microsporum gypseum, Trichophyton mentagrophytes, and T. rubrum were moderately inhibited by the different extracts (MIC values of 125-250 microg/mL). Demethylbellidifolin (4), bellidifolin (5), and isobellidifolin (6) showed an antifungal effect (MIC values of 50 microg/mL), while swerchirin (3) was less active with a MIC value of 100 microg/mL. In addition, oleanolic acid (1) and ursolic acid (2) were also isolated. These findings demonstrate that Gentianella multicaulis collected in the mountains of the Province of San Juan, Argentina, is an important source of compounds with antifungal and antioxidant activities.     

<Emphasis Type="Italic">In vivo</Emphasis> and <Emphasis Type="Italic">in vitro</Emphasis> antioxidant effects of three Veronica species

The aim of the present study was to examine the antioxidant activity of three Veronica species (Plantaginaceae). The antioxidant potential of various extracts obtained from aerial flowering parts was evaluated by DPPH-free (1,1-diphenyl-2-picrylhydrazyl-free) radical scavenging activity and ferric-reducing antioxidant power assays. Considerable antioxidant activity was observed in the plant samples (FRAP values ranged from 0.97 to 4.85 mmol Fe²⁺/g, and DPPH IC₅₀ values from 12.58 to 66.34 μg/ml); however, these levels were lower than the activity of the control compound butylated hydroxytoluene (BHT) (FRAP: 10.58 mmol Fe²⁺/g; DPPH IC₅₀: 9.57 μg/ml). Also, the in vivo antioxidant effects were evaluated in several hepatic antioxidant systems in rats (activities of glutathione peroxidase, glutathione reductase, peroxidase, catalase, xanthine oxidase, glutathione content and level of thiobarbituric acid reactive substances) after treatment with different Veronica extracts, or in combination with carbon tetrachloride (CCl₄). Pretreatment with 100 mg/kg b.w. of Veronica extracts inhibited CCl₄-induced liver injury by decreasing TBA-RS level, increasing GSH content, and bringing the activities of CAT and Px to control levels. The present study suggests that the extracts analyzed could protect the liver cells from CCl₄-induced liver damage by their antioxidative effect on hepatocytes.     

Antioxidant activities of different parts of Gnetum gnemon L.

Analyses on biological activities of Gnetum gnemon were done to determine the total phenolic and antioxidants of the plant. Four parts of G. gnemon were used in this study, which were leaf, bark, twig, and seeds of the plant. All parts were extracted in methanol, ethanol, hexane, chloroform and hot water using reflux. The total phenolic content of the plant extracts were determined by using Folin-Ciocalteu method. The results demonstrated that the bark from hot water extract showed the highest total phenolic at 10.71?±?0.01 mg GAE/ FDW, while the lowest was chloroform extract of seed at 2.15?±?0.01 mg GAE/ FDW. The antioxidant activity of the plant extracts were determined by using DPPH and FRAP assays, respectively. The DPPH results showed that all plant extracts demonstrated weak free radical scavenging activity tested at the final concentration of 300 μg/ml. In contrast, the methanolic twig extract showed strong reducing power activity (FRAP) at 83.55?±?1.05%, while the hot water seed extract showed the least activity at 41.86?±?4.22% tested at the final concentration of 300 μg/ml. However, there were no correlation between total phenolics and both antioxidant assays tested.     

不同种竹笋及笋壳提取物抗氧化活性的研究

采用醇提法,分别对毛竹、麻竹、雷竹的竹笋及笋壳进行醇提,并对醇提物进行抗氧化活性测定.对DPPH·、OH·、O2-·自由基的清除作用分别通过分光光度法、邻二氮菲法、邻苯三酚自氧化法进行测定,相对还原能力、总抗氧化能力的测定则采用普兰士蓝反应法和FRAP法.结果表明:不同种的竹笋及笋壳的醇提物含量与自由基清除能力、相对还...     

Assessment of antioxidant activity by using different in vitro methods

In this study, six common tests for measuring antioxidant activity were evaluated by comparing four antioxidants and applying them to beverages (tea and juices): Trolox equivalent antioxidant capacity assay (TEAC I-III assay), Total radical-trapping antioxidant parameter assay (TRAP assay), 2,2-diphenyl- l -picrylhydrazyl assay (DPPH assay), N , N -dimethyl- p -phenylendiamine assay (DMPD assay), Photochemiluminescence assay (PCL assay) and Ferric reducing ability of plasma assay (FRAP assay). The antioxidants included gallic acid representing the group of polyphenols, uric acid as the main antioxidant in human plasma, ascorbic acid as a vitamin widely spread in fruits and Trolox ® as water soluble vitamin E analogue. The six methods presented can be divided into two groups depending on the oxidising reagent. Five methods use organic radical producers (TEAC I-III, TRAP, DPPH, DMPD, PCL) and one method works with metal ions for oxidation (FRAP). Another difference between these tests is the reaction procedure. Three assays use the delay in oxidation and determine the lag phase as parameter for the antioxidant activity (TEAC I, TRAP, PCL). They determine the delay of radical generation as well as the ability to scavenge the radical. In contrast, the assays TEAC II and III, DPPH, DMPD and FRAP analyse the ability to reduce the radical cation (TEAC II and III, DPPH, DMPD) or the ferric ion (FRAP). The three tests acting by radical reduction use preformed radicals and determine the decrease in absorbance while the FRAP assay measures the formed ferrous ions by increased absorbance. Gallic acid was the strongest antioxidant in all tests with exception of the DMPD assay. In contrast, uric acid and ascorbic acid showed low activity in some assays. Most of the assays determine the antioxidant activity in the micromolar range needing minutes to hours. Only one assay (PCL) is able to analyse the antioxidant activity in the nanomolar range. Black currant juice showed highest antioxidant activity in all tests compared to tea, apple juice and tomato juice. Despite these differences, results of these in vitro assays give an idea of the protective efficacy of secondary plant products. It is strongly recommended to use at least two methods due to the differences between the test systems investigated.     

Laurus nobilis L. Extracts against Paenibacillus larvae: Antimicrobial activity,antioxidant capacity,hygienic behavior and colony strength

The aim of this work was to compare the antimicrobial activity against Paenibacillus larvae and the antioxidant capacity of two Laurus nobilis L. extracts obtained by different extraction methods. The hydroalcoholic extract was moreover added as supplementary diet to bees in field conditions to test behavioural effects and colony strength. Both laurel extracts were subjected to different phytochemical analysis to identify their bioactive compounds. Antimicrobial activity was analyzed by the minimal inhibitory concentration (MIC) determination by means the agar dilution method. The hydroalcoholic extract (HE) was able to inhibit the bacterial growth of all P. larvae strains, with 580 µg/mL mean value. This better antibacterial activity in relation to the essential oil (EO) could be explained by the presence of some phenolic compounds, such as flavonoids, evidenced by characteristic bands resulting from the Fourier Transform Infrared Spectroscopy (FTIR) analysis. Antioxidant activities of the extracts were evaluated by 2,2-diphenyl-1-picrylhydrazyl (DPPH) free radical-scavenging ability and ferric reducing antioxidant power (FRAP) assays. The HE showed the highest antioxidant activity as measured by DPPH, with IC50 values of 257 ± 12 μg/mL. The FRAP assay method showed that the HE was 3-fold more effective reducing agent than the EO. When the bee colonies were supplied with laurel HE in sugar paste an improvement in their general condition was noticed, although neither the hygienic behavior nor the proportions of the breeding cells varied statistically due to the treatment. In conclusion, the inhibition power against P. larvae attributable to the phenolic compounds, the antioxidant capacity of the HE, and the non-lethal effects on adult honey bees on field trials suggest the HE of laurel as a promising substance for control American foulbrood disease.     

Quantification of Phenolic Component by LC-HESI-MS/MS and Evaluation of Antioxidant Activities of Crocus Ancyrensis (Ankara Çiğdemi) Extracts Obtained with Different Solvents

In this study, Crocus ancyrensis was extracted from different parts of the plants with various solvents and their antioxidant activities and phenolic contents were investigated in detail for the first time. The highest amount of total phenolic substance in all parts of the plant was determined in the stigmaless flower. In the DPPH and FRAP methods, the highest antioxidant activity was obtained from the water extraction from the plant. Rutin is the highest detected by LC MS/MS. Stigmaless flower extract in all solvents is attributed to the component that contributes the most to antioxidant capacity. p-hydroxy benzoic acid was detected as the highest phenolic component after rutin. When the antioxidant activity results were examined, it was determined that the highest activity was in the water extract. As a result, it is evaluated that rutin and p-hydroxybenzoic acid in the plant contribute to the antioxidant capacity.