薄荷和罗勒提取物体外抗氧化及保肝活性研究

采用国际常用的ABTS和DPPH方法评价唇形科植物薄荷(Mentha haplocalyx) 和罗勒(Ocimum basilicum)水提物和乙醇提取物体外抗氧化活性,选用HepG2细胞,通过乙醇诱导损伤,构建体外酒精性肝损伤细胞模型,以细胞存活率评价薄荷和罗勒提取物的保肝效果。结果表明,DPPH自由基清除能力大小依次为薄荷醇提物、薄荷水提物、罗勒醇提物、罗勒水提物,半效应浓度(EC₅₀)分别为70.42 μg·mL^-1、75.77 μg·mL^-1、354.87 μg·mL^-1、451.53 μg·mL^-1。ABTS自由基清除能力大小依次为薄荷醇提物、罗勒醇提物、薄荷水提物、罗勒水提物,EC50值分别为9.04 μg·mL^-1、18.03 μg·mL^-1、22.18 μg·mL^-1、36.88 μg·mL^-1。薄荷提取物的抗氧化能力整体优于罗勒提取物,醇提物抗氧化能力优于水提物。酒精性肝损伤细胞活性检测表明,5、10、20、50 μg·mL^-1薄荷水提物、薄荷醇提物和罗勒水提物能剂量依赖性地提高乙醇诱导损伤的细胞存活率,具有一定的保肝活性。     

太行菊和野菊不同器官醇提液抗氧化活性比较研究

产地群众反映我国特有植物太行菊茶饮或药用效果远优于其近缘属的传统药食兼用野菊,为深入研究太行菊,本文比较研究太行菊和野菊不同器官醇提液的抗氧化活性,紫外-可见吸收光谱特性以及抗氧化活性与总黄酮和多酚含量的相关性。结果表明,太行菊和野菊醇提液均有一定抗氧化活性,在一定质量浓度范围,存在剂量效应关系,活性与提取温度相关;太行菊各器官提取液抗氧化活性,紫外-可见光谱吸收峰及总黄酮和多酚含量高于野菊对应器官;相关性分析结果显示,总黄酮和多酚对菊试样抗氧化活性有较大贡献,ABTS和DPPH两种抗氧化活性评价方法间存在较高相关性。太行菊较于野菊可能具有更好的保健或药用功效,有待合理开发利用。     

木豆叶醇提物对皮质酮诱导的PC12细胞损伤的保护作用

建立皮质酮诱导的PC12细胞损伤模型并观察木豆叶醇提物及不同组分对皮质酮损伤PC12细胞的保护作用.以100μ mol/L的皮质酮诱导PC12细胞损伤;损伤后的PC12细胞与木豆叶醇提物及不同组分孵育24h,通过形态学观察、MTT检测、LDH测定,研究各组分对皮质酮损伤PC12细胞的保护作用.结果表明,PC12细胞与皮质酮孵育48 h后细胞存活率明显降低,而LDH水平显著升高.而加入木豆叶醇提物及各组分时上述效果明显减轻,且存在明显的剂量依赖关系.从以上结果可知,木豆叶醇提物及不同组分对皮质酮损伤的PC12细胞均有保护作用,且醇提物的效果最好.     

有柄石韦醇提物抗氧化活性研究

通过DPPH自由基清除测定、还原能力、总抗氧化能力、羟自由基清除测定,评价有柄石韦Pyrrosia petiolosa醇提物的抗氧化活性。结果显示,有柄石韦醇提物清除DPPH·的IC50为75.82 μg·mL-1,清除·OH的IC50为46.30 μg·mL-1。有柄石韦醇提物清除DPPH· 的能力强于抗坏血酸,清除·OH的能力弱于抗坏血酸;同时,其还原能力和总抗氧化能力均强于抗坏血酸。该结果说明有柄石韦醇提物具有较强的抗氧化活性。     

五味子对H_2O_2诱导的HaCaT细胞氧化应激损伤的保护作用

检测五味子不同组分对H2O2诱导的HaCaT细胞氧化应激损伤的保护作用,筛选得到其活性组分。利用大孔吸附树脂法,对五味子果实提取物进行分离纯化,得到不同的组分段。以DPPH自由基清除能力和总抗氧化能力(ABTS法)为考察指标,对五味子各组分的抗氧化活性进行评价;采用MTT法筛选五味子各组分对H2O2诱导的HaCaT细胞氧化应激损伤的保护作用,获得活性组分。结果显示,50%乙醇洗脱物抗氧化活性最强,能提高H2O2处理后的HaCaT细胞存活率,减少MDA的生成,上调SOD酶和GSH酶活性。研究结果证实,50%乙醇洗脱物是五味子保护皮肤细胞免受H2O2诱导氧化应激的活性组分。     

连香树水提物和乙醇提取物的体外抗氧化研究

为了探究连香树水提物和乙醇提取物的主要成分和抗氧化作用,该研究采用水提和醇提两种方法提取连香树叶片中的代谢物并测定其主要成分,通过体外抗氧化实验,即清除羟自由基(·OH)、DPPH自由基(DPPH·)、超氧阴离子(O_2~-·)和还原铁离子(Fe~(3+))的能力等四个指标来评价其抗氧化作用。结果表明:连香树水提物和乙醇提取物中均含有山萘酚。此外,水提物中还含有苜蓿素和异槲皮苷等黄酮类物质;乙醇提取物中还含有柚皮素和槲皮素3-O-β-D-葡萄糖苷等黄酮类物质。水提物和乙醇提取物均有清除羟自由基、DPPH自由基、超氧阴离子及还原三价铁离子的能力。抗氧化的作用随提取物浓度的增大而增强,其中清除超氧阴离子(IC50值分别为0.092、0.002 mg·mL~(-1))的能力强于阳性对照Vc(IC_(50)值为0.241 mg·mL~(-1))且铁离子还原力的IC_(50)值(水提物为0.014 mg·mL~(-1),乙醇提取物为0.001 mg·mL~(-1))相对较小,说明其总抗氧化活性较强。由此可见,连香树水提物和乙醇提取物均具有良好的抗氧化作用,可作为一种潜在的天然抗氧化剂。     

铁皮石斛化学成分及其抗氧化活性研究

采用硫酸-苯酚法、AlCl^₃比色法、酸性染料比色法测定铁皮石斛(Dendrobium officinale)花、叶、茎中多糖、黄酮、生物碱含量，通过DPPH和ABTS清除实验评价铁皮石斛花、叶、茎的水提物和乙醇提取物的体外抗氧化活性。结果表明，铁皮石斛不同部位的多糖含量茎>花>叶，黄酮含量花>叶>茎，生物碱在各个部位分布均较少。其中茎的多糖含量可达23.92%，花中黄酮含量可达1.847%。抗氧化能力评价表明，铁皮石斛花水提物、茎醇提物、花醇提物的DPPH自由基清除能力相对较好，半效应浓度(EC₅₀)分别为410.4 μg·mL^-1、454.1 μg·mL^-1、573.2 μg·mL^-1；铁皮石斛茎醇提物、花醇提物、花水提物ABTS自由基清除能力相对较好，半效应浓度(EC₅₀)分别为61.1 μg·mL^-1、62.2 μg·mL^-1、103.0 μg·mL^-1。铁皮石斛花的提取物抗氧化活性整体优于叶和茎，醇提物抗氧化能力优于水提物。     

抑制前列腺癌的食药用菌醇提物的筛选及灵芝醇提物对癌细胞的抑制机理

比较了灰树花Grifola frondosa、巴氏蘑菇Agaricus blazei、 猴头菌Hericium erinaceus、刺芹侧耳Pleurotus eryngii、毛头鬼伞Coprinus comatus、蛹虫草Cordyceps militaris、灵芝Ganoderma lingzhi、香菇Lentinula edodes、桑黄Sanghuangporus sanghuang和桦褐孔菌Inonotus obliquus 10种食用菌醇提物对前列腺癌LNCaP细胞增殖的影响,其中灵芝醇提物对LNCaP细胞增殖及5ɑ-还原酶活性具有良好的抑制效果,对LNCaP细胞释放PSA的抑制效果也好于其他食用菌。进一步研究灵芝醇提物对LNCaP细胞的抑制机理,结果表明,灵芝醇提物通过诱导细胞凋亡、使Caspase-3、Bax、P53活性升高,PARP、Bcl-2活性下降来实现对LNCap细胞的抑制作用。利用自噬抑制剂氯喹和自噬激活剂雷帕霉素观察细胞自噬在灵芝醇提物抗肿瘤过程中的作用,结果表明,体外激活细胞自噬对LNCaP细胞起到保护,从而减弱了灵芝醇提物的抗肿瘤作用。     

大血藤醇提物抗炎镇痛和止血活性研究初探

为观察大血藤醇提物抗炎、镇痛、止血活性,该文采用75％乙醇提取制备大血藤醇提物(AESC),利用HPLC法测定其绿原酸含量;KM鼠(或新西兰兔)在测定抗炎、镇痛、止血活性时随机分为空白对照组、阳性对照组(云南白药酊组)、AESC组,依次测定其抑制二甲苯致小鼠耳肿胀度作用、痛阈值和兔肝脏局部创面损伤出血的记分分值,分别考...     

蛹虫草MF27高抗氧化活性提取物筛选及保肝作用研究

本研究对一株优质蛹虫草菌株MF27不同提取物进行体外抗氧化活性比较,筛选得到高抗氧化活性提取物,并进一步探究该提取物对CCl₄诱导的小鼠肝损伤的修复作用。以DPPH自由基和羟自由基的清除率为抗氧化评价指标,从菌丝体发酵液、菌丝体水提物/醇提物、以及子实体水提物/醇提物中筛选菌株MF27的高抗氧化活性提取物;以CCl₄致小鼠急性肝损伤为模型,通过检测血清生化指标、肝功指标的变化,来评价该高活性提取物的体内抗氧化保肝效果。体外抗氧化实验结果表明,MF27的不同提取物均具有较好的体外抗氧化活性,但对清除DPPH和OH自由基能力最好的提取物是子实体水提物,其对DPPH自由基的半数有效浓度（EC₅₀）为0.096mg/mL,对羟自由基的半数有效浓度（EC₅₀）为0.196mg/mL,当在1mg/mL 时对DPPH自由基的清除率为94.94%,对羟自由基的清除率为70.17%;体内抗氧化保肝结果显示,给药组（子实体水提物）相比模型组而言,小鼠血清中ALT、AST以及肝脏中MDA水平极显著降低（P<0.01）、SOD水平极显著升高（P<0.01）,表明子实体水提物能有效改善氧化性肝损伤,同时与阳性对照（联苯双酯）对比,给药组在肝脏指数上表现出相当的作用（P>0.05）。本研究表明菌株MF27的最有效抗氧化活性提取物是子实体水提物,它对体内氧化性肝损伤有一定的修复能力,揭示MF27子实体水提物具有成为抗氧化性肝损伤功能产品的潜力。     

Hepatoprotective effect of aqueous extract of Aframomum melegueta on ethanol-induced toxicity in rats

In recent years there have been remarkable developments in the prevention of diseases, especially with regards to the role of free radicals and antioxidants. Ethanol-induced oxidative stress appears to be one mechanism by which ethanol causes liver injury. The protective effect of aqueous plant extract of Aframomum melegueta on ethanol-induced toxicity was investigated in male Wistar rats. The rats were treated with 45 % ethanol (4.8 g/kg b.w.t.) for 16 days to induce alcoholic diseases in the liver. The activities of alanine aminotransferase, aspartate aminotransferase and triglyceride were monitored and the histological changes in liver examined in order to evaluate the protective effects of the plant extract. Hepatic malondialdehyde and reduced glutathione, as well as superoxide dismutase and glutathione-S-transferase activities were determined for the antioxidant status. Chronic ethanol administration resulted in a statistically significant elevation of serum alanine aminotransferases and triglyceride levels, as well as a decrease in reduced glutathione and superoxide dismutase which was dramatically attenuated by the co-administration of the plant extract. Histological changes were related to these indices. Co-administration of the plant extract suppressed the elevation of lipid peroxidation, restored the reduced glutathion, and enhanced the superoxide dismutase activity. These results highlight the ability of Aframomum melegueta to ameliorate oxidative damage in the liver and the observed effects are associated with its antioxidant activities.     

Alcohol steatosis and cytotoxicity: The role of cytochrome P4502E1 and autophagy

The goal of the current study was to evaluate whether CYP2E1 plays a role in binge-ethanol induced steatosis and if autophagy impacts CYP2E1-mediated hepatotoxicity, oxidative stress and fatty liver formation produced by ethanol. Wild type (WT), CYP2E1 knockin (KI) and CYP2E1 knockout (KO) mice were gavaged with 3g/kg body wt ethanol twice a day for four days. This treatment caused fatty liver, elevation of CYP2E1 and oxidative stress in WT and KI mice but not KO mice. Autophagy was impaired in ethanol-treated KI mice compared to KO mice as reflected by a decline in the LC3-II/LC3-I ratio and lower total LC-3 and Beclin-1 levels coupled to increases in P62, pAKT/AKT and mTOR. Inhibition of macroautophagy by administration of 3-methyladenine enhanced the binge ethanol hepatotoxicity, steatosis and oxidant stress in CYP2E1 KI, but not CYP2E1 KO mice. Stimulation of autophagy by rapamycin blunted the elevated steatosis produced by binge ethanol. Treatment of HepG2 E47 cells which express CYP2E1 with 100mM ethanol for 8 days increased fat accumulation and oxidant stress but decreased autophagy. Ethanol had no effect on these reactions in HepG2 C34 cells which do not express CYP2E1. Inhibition of autophagy elevated ethanol toxicity, lipid accumulation and oxidant stress in the E47, but not C34 cells. The antioxidant N-acetylcysteine, and CYP2E1 inhibitor chlormethiazole blunted these effects of ethanol. These results indicate that CYP2E1 plays an important role in binge ethanol-induced fatty liver. We propose that CYP2E1-derived reactive oxygen species inhibit autophagy, which subsequently causes accumulation of lipid droplets. Inhibition of autophagy promotes binge ethanol induced hepatotoxicity, steatosis and oxidant stress via CYP2E1.     

In-vitro antioxidative,antiinflammatory properties of Aurea helianthus leaf extract a Korean traditional medicinal plant

The leaf of Aurea helianthus (A. helianthus Jinhuakui) is popularly used in China traditional medicine, however, scientific evidence on its antioxidant properties rarely studied. In this study, biological activities of A. helianthus leave’s 80% ethanol extract (AHL) were investigated. The measured total polyphenol and flavonoid content of AHL was 184.24 ± 5.01 mg GAE/g and 102.53 ± 0.98 mg NAR/g. AHL showed the highest α, α-diphenyl-β-picrylhydrazyl (DPPH) and 2,2′-azino-bis-3-ethylbenzo-thiazoline-6-sulfonic acid (ABTS) radical scavenging activities of 98.30 ± 0.18% at 1000 µg/mL. DPPH and ABTS radical scavenging activities significantly increased in a AHL concentration-dependent manner. AHL treatment significantly suppressed the generation of pro-inflammatory mediators, including nitric oxide (NO), in lipopolysaccharide (LPS)-stimulated RAW 264.7 macrophages. AHL demonstrated strong anti-inflammatory activity that reduced NO production in LPS-stimulated RAW 264.7 cells. To test the potential protective effect of AHL, the antioxidant capacity, on the cell growth, viability of a human hepatoma cell (HepG2) and Raw 264.7 cell were investigated. AHL also enhanced cytotoxicity on the proliferation of HepG2 cells and was capable of inhibiting 56% against LPS at 400 µg/mL. The results of this study the potential of AHL as an excellent antioxidant substance for inhibiting inflammatory mediators. Therefore, AHL may be used as a therapeutic approach to various inflammatory diseases.     

6-Gingerdione Reduces Apoptotic Conditions in HepG2 Cells and Inhibits Inflammatory Cytokine Gene Expression in Alcoholic Liver Injured Zebrafish Larvae

Antioxidant natural products and their analogs especially phenolic compounds, exhibit diverse biological properties, including anti-inflammatory, antioxidant, and anticancer activities. Ginger which is widely used worldwide for various beneficial effects also contains several phenolic antioxidants, and 6-gingerol is one of the natural products studied extensively. However, the molecular mechanism of synthetically synthesized 6-gingerdione (compound 1 ) from 6-gingerol was not known. In this study, compound 1 and methylated 6-gingerdione (compound 2 ) were obtained semi synthetically from 6-gingerol. Compound 1 and 2 are subjected to SwissADME prediction. Then the protective effect of compound 1 was analyzed in 2 % EtOH induced HepG2 cells and zebrafish larvae. Hydroxyl and nitric oxide scavenging assays reveal that compound 1 showed more antioxidant activity than compound 2 at 50 μM. Moreover, compound 1 exhibited good anti-inflammatory activity via lipoxygenase inhibition and proteinase inhibition. Apoptosis and oxidative stress in HepG2 cells were induced by 2 % EtOH and treated with compound 1 . Compound 1 significantly inhibited the EtOH induced nitric oxide production, apoptosis, and ROS generation in HepG2 cells. Encouraged by the in-vitro antioxidant and anti-inflammatory activities, compound 1 was then investigated for its protective effect in 2 % EtOH induced ALD zebrafish larva. Compound 1 protected the zebrafish larvae from liver injury by suppressing inflammatory (COX-2, TNF-α, and IL-1β) and lipogenic genes (C/EBP-α, SREBP1, and IL-1β) while upregulating the antioxidant gene. Our findings indicate that compound 1 synthesized from 6-gingerol ameliorated liver injury that likely, contributes to its potential antioxidant and anti-inflammatory properties.     

Hepatoprotective and antioxidant effects of Morus bombycis Koidzumi on CCl4-induced liver damage

The antioxidant activity and liver protective effect of Morus bombycis Koidzumi were investigated. Aqueous extracts of M. bombycis Koidzumi had higher superoxide radical scavenging activity than other types of extracts. The aqueous extract at a dose of 100 mg/kg showed significant hepatoprotective activity when compared with that of a standard agent. The biochemical results were confirmed by histological observations indicating that M. bombycis Koidzumi extract together with CCl(4) treatment decreased ballooning degeneration. The water extract recovered the CCl(4)-induced liver injury and showed antioxidant effects in assays of FeCl(2)-ascorbic acid-induced lipid peroxidation in rats. Based on these results, we suggest that the hepatoprotective effect of the M. bombycis Koidzumi extract is related to its antioxidative activity.     

Effects of anabolic steroids and antioxidant vitamins on ethanol-induced tissue injury

Various mechanisms are involved in the process of ethanol-induced tissue impairment. Oxidative stress and its effects are among the most important. We compared the effects of antioxidant vitamins (vitamin C and E in combination) and steroids (testosterone and nandrolone separately) on the toxicity of ethanol in rats. Animals (male Wistar rats, n = 48) were randomised into following groups-Control, Ethanol, Testosterone, Ethanol + Testosterone, Ethanol + Nandrolone, Ethanol + Vitamins. Alcohol was given daily by gavage in a dose of 5 g/kg of body weight. On the 27th day of the study the animals were sacrificed by decapitation and tissue samples were taken. Metabolic status, parameters of the hepatic metabolism, hormone levels (testosterone, ACTH, corticosterone), lipoperoxidation markers (malondialdehyde and conjugated diens in forebrain cortex and in cerebellum) and advanced glycation end-products were analysed. Tissue samples underwent histological examination. Histological outcomes showed a protective effect of antioxidants on hepatic and cerebellar injury caused by chronic ethanol intake. Anabolic steroids protected especially the central nervous tissue against the toxicity of alcohol. Both, antioxidant vitamins and anabolic steroids protect against the ethanol-induced toxicity, however, this effect is tissue specific.     

Preventive effects of indole-3-carbinol against alcohol-induced liver injury in mice via antioxidant,anti-inflammatory,and anti-apoptotic mechanisms: Role of gut-liver-adipose tissue axis

Indole-3-carbinol (I3C), found in Brassica family vegetables, exhibits antioxidant, anti-inflammatory, and anti-cancerous properties. Here, we aimed to evaluate the preventive effects of I3C against ethanol (EtOH)-induced liver injury and study the protective mechanism(s) by using the well-established chronic-plus-binge alcohol exposure model. The preventive effects of I3C were evaluated by conducting various histological, biochemical, and real-time PCR analyses in mouse liver, adipose tissue, and colon, since functional alterations of adipose tissue and intestine can also participate in promoting EtOH-induced liver damage. Daily treatment with I3C alleviated EtOH-induced liver injury and hepatocyte apoptosis, but not steatosis, by attenuating elevated oxidative stress, as evidenced by the decreased levels of hepatic lipid peroxidation, hydrogen peroxide, CYP2E1, NADPH-oxidase, and protein acetylation with maintenance of mitochondrial complex I, II, and III protein levels and activities. I3C also restored the hepatic antioxidant capacity by preventing EtOH-induced suppression of glutathione contents and mitochondrial aldehyde dehydrogenase-2 activity. I3C preventive effects were also achieved by attenuating the increased levels of hepatic proinflammatory cytokines, including IL1β, and neutrophil infiltration. I3C also attenuated EtOH-induced gut leakiness with decreased serum endotoxin levels through preventing EtOH-induced oxidative stress, apoptosis of enterocytes, and alteration of tight junction protein claudin-1. Furthermore, I3C alleviated adipose tissue inflammation and decreased free fatty acid release. Collectively, I3C prevented EtOH-induced liver injury via attenuating the damaging effect of ethanol on the gut-liver-adipose tissue axis. Therefore, I3C may also have a high potential for translational research in treating or preventing other types of hepatic injury associated with oxidative stress and inflammation.