王不留行多糖的提取工艺及其抗氧化活性研究

通过单因素实验和正交实验,研究料液比、超声功率、超声提取温度和超声作用时间对王不留行多糖提取效果的影响。分别采用紫外分光光度法和邻苯三酚自氧化法测定其清除DPPH·和O-·2的作用进行试验,根据试验结果评价其体外抗氧化活性。得出优化工艺条件为:料液比(g∶m L)1∶50,提取温度60℃,超声功率100W,作用时间40 min。王不留行多糖的得率为9.60%,优选王不留行多糖的超声提取工艺,省时、高效、可靠、重现性好;体外抗氧化性试验显示王不留行多糖对DPPH·和O-·2具有较强的清除能力,且在一定范围内其抗氧化作用与浓度呈现良好的量效关系。     

使君子多糖的超声波提取及体外抗氧化

目的:利用超声波法提取使君子多糖,将得到的多糖进行抗氧化性实验,探究其抗氧化活性。方法:通过单因素实验和正交实验,研究料液比、超声作用时间、超声提取温度和超声功率对使君子多糖提取效果的影响。制备使君子多糖,通过对·OH及·O-2的清除实验结果来评价其抗氧化活性。结果:超声波法提取使君子多糖的最佳提取条件为料比液1∶30(g/m L)、提取时间40 min、提取温度70℃、超声波功率140 W,在此条件下使君子多糖的提取率为10.36%。抗氧化性试验数据显示使君子多糖对·OH及·O-2的清除作用显著。结论:使君子多糖具有较强的抗氧化活性,为使君子的资源利用与开发提供了科学依据。     

黑莓果渣中花色苷的提取工艺研究

通过提取方法优选,表明超声法对黑莓果渣中花色苷的提取效果最佳。以60%乙醇为超声法提取溶剂,通过单因素实验分别考察了料液比、超声时间、温度、功率、提取次数对提取黑莓果渣中花色苷的影响。综合单因素实验结果,通过响应面法筛选出最佳的工艺条件为:液料比14∶1(mL∶g),时间40 min,温度58℃,功率300 W,提取2次。通过提取物中花色苷含量与其清除DPPH.活性的相关性分析发现,黑莓果渣提取物清除DPPH.活性与其花色苷含量之间存在相关性,由此推断花色苷为黑莓果渣中主要的自由基清除物质。     

发酵芝麻饼粕中木脂素提取条件的优化及特征物质的鉴别

采用正交设计和响应面的试验方法,对酱油曲霉发酵芝麻饼粕中木脂素提取工艺进行了优化,并对发酵产生的特征物质进行了鉴别。结果表明,影响提取发酵芝麻饼粕中木脂素因素的主次顺序为:乙醇浓度液料比提取时间提取次数。通过响应面试验再优化,得到较优的提取条件为:时间120.4 min,液料比15.77mL/g,乙醇浓度61.38%,在此条件下,DPPH自由基清除率可达82.59%,对照为46.8%。HPLC检测发现发酵提取物中产生一种特征物质,利用硅胶柱色谱层析分离,薄层色谱检测和LC-MS鉴别,产生的新物质为芝麻素酚。     

正交设计优选五味子果实中总木脂素提取工艺

目的:比较不同方法对北五味子总木脂素提取的影响,优选最佳提取工艺方法。研究五味子木脂素抗微波辐射损伤作用。方法:以干燥北五味子果实为原料,分别采用传统加热回流法、超声提取法、微波提取法、微波—超声提取法提取北五味子总木脂素,对这四种提取方法分别进行正交试验分析,以确定最佳提取工艺。结果:通过结果比较分析,以微波提取工艺结果最佳,在微波提取功率为200W,乙醇体积分数为80%,提取时间为40min,料液比为1:12的提取条件下,北五味子总木脂素的产量达到了16.44mg/g,使得木脂素的提取产量较传统加热回流法、超声提取法、微波—超声提取法得到了显著的提高。     

超声波辅助大米草总黄酮提取及抗氧化活性研究

应用超声波技术,以大米草为原料提取黄酮类化合物,设计正交实验,研究乙醇浓度、料液比、超声处理温度和提取时间对总黄酮提取效果的影响,分析得出最佳提取工艺条件。并测定大米草黄酮体外抗氧化活性。结果表明:大米草总黄酮提取的最佳工艺条件为:乙醇浓度80%,提取时间20 min,料液比1∶30(g·mL-1),提取温度45℃。影响大米草黄酮提取率的主次因素是:料液比乙醇浓度提取温度提取时间。大米草黄酮总抗氧化活性和抗超氧阴离子活力随着浓度的增加逐渐增加,呈明显的量效关系,并且能有效清除氧化脂质(MDA)。     

响应面优化大蒜总黄酮提取及抗氧化研究

本实验通过单因素试验探讨了乙醇浓度、料液比、超声时间、超声温度对大蒜总黄酮得率的影响,然后进一步通过响应面分析确定了超声波辅助乙醇提取大蒜总黄酮的最佳工艺条件为:乙醇浓度80%,料液比1∶16,超声时间18 min,超声温度53℃。在最佳工艺条件下,大蒜总黄酮得率达到3.99%。最后进行邻苯三酚自氧化试验,发现大蒜提取液对超氧阴离子自由基(O-·2)的抑制率为60.43%,表明大蒜总黄酮有较强的抗氧化活性。     

油菜花粉总黄酮的微波辅助提取及其抗氧化活性研究

采用微波辅助提取法提取油菜花粉总黄酮,通过单因素和正交试验,得到最佳提取条件：80％的乙醇、1：20的料液比、提取时间140s、微波功率242W、提取3次,总黄酮质量分数为（2．64±0．05）％。同时还研究提取物对羟自由基、DPPH自由基的清除作用,以及对小鼠肝组织脂质过氧化的抑制作用,自由基半清除质量浓度和脂质过氧化丰抑制盾奄浓度分剐为0．115、0．325和0．065mg／mL。     

超声波辅助大米草总黄酮提取及抗氧化活性研究北大核心CSCD

应用超声波技术,以大米草为原料提取黄酮类化合物,设计正交实验,研究乙醇浓度、料液比、超声处理温度和提取时间对总黄酮提取效果的影响,分析得出最佳提取工艺条件。并测定大米草黄酮体外抗氧化活性。结果表明:大米草总黄酮提取的最佳工艺条件为:乙醇浓度80%,提取时间20 min,料液比1∶30(g·mL-1),提取温度45℃。影响大米草黄酮提取率的主次因素是:料液比>乙醇浓度>提取温度>提取时间。大米草黄酮总抗氧化活性和抗超氧阴离子活力随着浓度的增加逐渐增加,呈明显的量效关系,并且能有效清除氧化脂质(MDA)。     

柿子渣中多酚的提取工艺及其抗氧化性研究

采用单因素试验设计,研究了料液比、提取温度、乙醇浓度、提取时间4个因素对柿子渣中总多酚提取效果的影响,运用正交试验设计对提取工艺进行了优化,并采用DPPH法检测了柿子渣多酚提取液清除自由基的能力.结果表明:(1)提取温度和提取时间对总多酚含量影响显著,乙醇浓度和料液比对总多酚含量影响不显著;柿子渣总多酚提取的最佳工艺为:料液比20:1(mL·g-1),提取温度90℃,乙醇浓度40%,提取时间4 h.(2)验证试验结果表明,优化条件下总多酚的提取量可达到21.402 mg·g-1,高于正交试验中任何一组.(3)抗氧化活性试验表明,当柿子渣多酚提取液质量浓度为0.24 mg·mL-1时,对DPPH自由基的清除率可达95.4%,与对照Vc抗氧化能力无显著差异,表明在该优化工艺下提取的柿子渣多酚具有较强的抗氧化活性.     

沙棘果渣总黄酮提取工艺优化及抗氧化活性研究

利用果胶酶协同超声波法,对沙棘果渣有效成分总黄酮的提取工艺及其抗氧化活性进行了研究。以提取率为指标,通过酶用量、液料比、乙醇浓度、提取时间、提取温度、超声功率等单因素分析,选定酶用量、液料比、超声提取时间3个因素进行响应面试验,确定提取优化工艺条件为:果胶酶用量5.1%,液料比41∶1,超声提取时间81 min,此条件下,沙棘果渣总黄酮提取率达到8.91 mg/g;以BHT为阳性对照,进行了抗氧化活性研究,得出沙棘果渣总黄酮提取液浓度为0.14 mg/mL时,对DPPH自由基的清除率达到了94.42%;提取液浓度为1.2 mg/mL时,对羟自由基和超氧阴离子的清除率分别为83.10%和43.41%。整体来看,沙棘果渣总黄酮具有较强的抗氧化能力。     

超声波提取加拿大蓬总黄酮的研究

目的:研究加拿大蓬中总黄酮提取方法及最佳工艺.方法:采用超声提取法,通过单因素试验和正交试验筛选最佳工艺条件.结果:最佳提取条件为60%乙醇、料液比1:20、60 kW下超声45 min.得率为31.076 mg/g.结论:该方法提取提取总黄酮快速、简便,可适用于生产中加拿大蓬总黄酮类物质的检测.该方法是提取加拿大蓬总...     

微波辅助提取荔枝核黄酮类化合物及其抗氧化性研究

研究微波辅助法提取荔枝核黄酮类化合物的工艺,考察了提取溶剂、微波功率、溶剂用量、辐射时间、提取次数等因素对提取的影响。通过正交实验确定最佳的提取参数为:60%乙醇作为提取溶剂,微波功率700 W,料液比1∶25,辐射时间150 s,提取一次。在此优化条件下用微波辅助,黄酮类化合物的得率为6.86%,提取物中黄酮含量达到36.7%。抗氧化性研究表明荔枝核黄酮类化合物有良好的抗氧化活性,能有效清除羟基自由基(OH.)和超氧阴离子自由基(O2-.)。     

甘草提取物对鼠肝线粒体氧化损伤的保护作用

用60%乙醇回流甘草,得粗提物(RG0),经AB-8大孔树脂纯化RG0得到甘草精提物(RG1),并对RG0和RG1主要活性成分的含量进行测定。为研究RG0和RG1对鼠肝线粒体氧化损伤的保护作用,用Vc-Fe2+诱导线粒体损伤,测定RG0和RG1对ATP酶的活性、线粒体肿胀度和蛋白质羰基含量的影响;用H2O2-Fe2+体系诱导线粒体脂质过氧化,测定RG0和RG1对丙三醛(MDA)含量的影响;用NBT法测定RG0和RG1抑制线粒体产生超氧阴离子的作用。结果显示:RG0和RG1可以显著地抑制线粒体的氧化损伤,并能防止线粒体肿胀和ATP酶活力下降,降低蛋白质羰基化水平,以及具有有效清除线粒体产生的超氧阴离子自由基的作用。因此,RG0和RG1对鼠肝线粒体的氧化损伤具有良好的保护作用,RG1的作用比RG0好。     

超声波法提取野生石蒜中加兰他敏

石蒜是我国丰富的野生资源之一,其鳞茎富含重要药用成分加兰他敏。为了获得石蒜中加兰他敏的超声波提取方法,以野生石蒜为原料,用乙醇作提取剂,探讨了超声波提取加兰他敏的工艺条件,并与常规溶剂法进行了比较。分析了料液比、超声波功率、提取温度、提取时间、提取次数等因素对加兰他敏提取效果的影响,运用正交实验L9(34)确定了最佳提取工艺条件。结果显示,超声波提取加兰他敏的最佳工艺条件为:料液比1:6,超声波功率250 W,提取温度60℃,提取时间1.5 h,提取2次;加兰他敏的提取率为94.6%,产率为0.0543%;提取物中加兰他敏含量为15.53%。与常规溶剂法相比,超声波法具有用时少、提取率高、提取次数少等优点,整体效果优于常规溶剂法。     

青橄榄浸膏的提取及其抗氧化活性研究

为优化青橄榄浸膏提取工艺,并探讨其抗氧化性。以茂名盛产的青橄榄为原料,采用超声波辅助乙醇提取法,以总黄酮和总多酚得率为评价指标,考察各因素对青橄榄浸膏提取效果的影响。采用邻苯三酚自氧化法、结晶紫法和DPPH清除能力评价青橄榄浸膏的抗氧化活性。结果显示,浸膏的最佳提取工艺为:乙醇体积分数70%,料液比1∶18 (g∶mL),超声提取温度50℃,时间6 min(超声提取阶段);单纯有机溶剂提取温度60℃,时间45 min(有机溶剂浸提阶段);此条件下总黄酮得率为1. 76%,总多酚得率为15. 53%。终产物浸膏在0. 3 mg/mL浓度下对超氧阴离子自由基抑制率为22. 74%,相当于同等质量浓度的抗坏血酸抑制效果的23. 47%;在0. 02 mg/mL浓度下对羟基自由基的清除率为67. 32%,相当于同等质量浓度的抗坏血酸清除效果的112. 58%;在0. 2 mmol/mL的DPPH溶液体系中,0. 15 mg/mL的浸膏对DPPH的清除率为95. 40%,相当于同等质量浓度的抗坏血酸清除效果的140. 83%;总体来讲,浸膏具有良好的抗氧化能力,虽然对超氧阴离子自由基抑制率弱于抗坏血酸,但羟基自由基的清除率及DPPH清除率均优于抗坏血酸。     

Effect of oilseed cakes on alpha-amylase production by Bacillus licheniformis CUMC305

The effects of oilseed cakes on extracellular thermostable alpha-amylase production by Bacillus licheniformis CUMC305 was investigated. Each oilseed cake was made of groundnut, mustard, sesame, linseed, coconut copra, madhuca, or cotton. alpha-Amylase production was considerably improved in all instances and varied with the oilseed cake concentration in basal medium containing peptone and beef extract. Maximum increases were effected by a low concentration (0.5 to 1.0%) of groundnut or coconut, a high concentration (3%) of linseed or mustard, and an Rintermediate concentration (2%) of cotton, madhuca, or sesame. The oilseed cakes made of groundnut or mustard could completely replace the conventional peptone-beef extract medium as the fermentation base for the production of alpha-amylase by B. licheniformis. The addition of corn steep liquor to cotton, linseed, sesame, or madhuca cake in the medium improved alpha-amylase production.     

Effect of oilseed cakes on alpha-amylase production by Bacillus licheniformis CUMC305.

The effects of oilseed cakes on extracellular thermostable alpha-amylase production by Bacillus licheniformis CUMC305 was investigated. Each oilseed cake was made of groundnut, mustard, sesame, linseed, coconut copra, madhuca, or cotton. alpha-Amylase production was considerably improved in all instances and varied with the oilseed cake concentration in basal medium containing peptone and beef extract. Maximum increases were effected by a low concentration (0.5 to 1.0%) of groundnut or coconut, a high concentration (3%) of linseed or mustard, and an Rintermediate concentration (2%) of cotton, madhuca, or sesame. The oilseed cakes made of groundnut or mustard could completely replace the conventional peptone-beef extract medium as the fermentation base for the production of alpha-amylase by B. licheniformis. The addition of corn steep liquor to cotton, linseed, sesame, or madhuca cake in the medium improved alpha-amylase production.     

Ionic liquid based ultrasonic assisted extraction of isoflavones from Iris tectorum Maxim and subsequently separation and purification by high-speed counter-current chromatography

We developed an ionic liquid based ultrasonic assisted extraction (ILUAE) method for the extraction of the three isoflavones, namely tectoridin, iristectorin B and iristectorin A from Iris tectorum Maxim of the Iridaceae family. Three kinds of 1-alkyl-3-methylimidazolium ionic liquids with different alkyl chain and anion were investigated. The results indicated that ionic liquids (ILs) showed remarkable effects on the extraction yield of isoflavones. In addition, the ILUAE, including several ultrasonic parameters, such as the concentration, extraction time and solvent to solid ratio have been optimized. Under these optimal conditions (e.g., with 30 min extraction time and the solvent to solid ratio of 30 ml/g), this approach gained the highest extraction yields of tectoridin (37.45 mg/g), iristectorin B (2.88 mg/g) and iristectorin A (5.28 mg/g). Meanwhile, tectoridin, iristectorin B and iristectorin A in the ILUAE extract were separated and purified successfully through the high-speed counter-current chromatography (HSCCC) with a two-phase solvent system consisting of n-butanol-water (1:1, v/v). The additional advantage of this approach is that 60.21 mg tectoridin, 4.33 mg iristectorin B and 8.24 mg iristectorin A with more than 95.0% purities have been obtained from 400 mg ILUAE extract of I. tectorum within 5 h and one-step elution under the most optimized conditions (e.g., a flow rate of 2.0 ml/min, 900 rpm and the wavelengh of 280 nm). The obtained fractions were successfully analyzed by HPLC and identified by (1)H-NMR and (13)C-NMR.     

Ca2+ and Mg2+-enhanced reduction of arsenazo III to its anion free radical metabolite and generation of superoxide anion by an outer mitochondrial membrane azoreductase

At the concentrations usually employed as a Ca2+ indicator, arsenazo III underwent a one-electron reduction by rat liver mitochondria to produce an azo anion radical as demonstrated by electron-spin resonance spectroscopy. Either NADH or NADPH could serve as a source of reducing equivalents for the production of this free radical by intact rat liver mitochondria. Under aerobic conditions, addition of arsenazo III to rat liver mitochondria produced an increase in electron flow from NAD(P)H to molecular oxygen, generating superoxide anion. NAD(P)H generated from endogenous mitochondrial NAD(P)+ by intramitochondrial reactions could not be used for the NAD(P)H azoreductase reaction unless the mitochondria were solubilized by detergent or anaerobiosis. In addition, NAD(P)H azoreductase activity was higher in the crude outer mitochondrial membrane fraction than in mitoplasts and intact mitochondria. The steady-state concentration of the azo anion radical and the arsenazo III-stimulated cyanide-insensitive oxygen consumption were enhanced by calcium and magnesium, suggesting that, in addition to an enhanced azo anion radical-stabilization by complexation with the metal ions, enhanced reduction of arsenazo III also occurred. Accordingly, addition of cations to crude outer mitochondrial membrane preparations increased arsenazo III-stimulated cyanide-insensitive O2 consumption, H2O2 formation, and NAD(P)H oxidation. Antipyrylazo III was much less effective than arsenazo III in increasing superoxide anion formation by rat liver mitochondria and gave a much weaker electron spin resonance spectrum of an azo anion radical. These results provide direct evidence of an azoreductase activity associated with the outer mitochondrial membrane and of a stimulation of arsenazo III reduction by cations.