22 resultados para Ginseng.

em Chinese Academy of Sciences Institutional Repositories Grid Portal


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Ultrahigh pressure technique was employed to extract ginsenosides from roots of ginseng (Panax ginseng C.A. Meyer). The optimal conditions for ultrahigh pressure extraction (UPE) of total ginsenosides were quantified by UV-vis spectrophotometry with the ginsenoside Re as standard, the signal ginsenosides were quantified by HPLC and ELSD with ginsenosides Re, Rg(1), Rb-1, Rc and Rb-2 as standards. Orthogonal design was applied to evaluate the effects of four independent factors (extraction pressure, extraction temperature, extraction time and ethanol concentration) on the yield and 1,1-diphenyl-2-picrylhydrazyl (DPPH) radical scavenging activity of ginsenoside, which are based on microwave extraction (ME), ultrasound extraction (UE), soxhlet extraction (SE) and heat reflux extraction (HRE) method. The results showed that UPE method can produce ginsenoside with the highest yield and the best radical scavenging activity compared to other used ones. Scanning electron microscopic (SEM) images of the plant cells after ultrahigh pressure treatment was obtained to provide visual evidence of the disruption effect.

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To study the content variation of ginsenosides and alkaloids during combination of ginseng with veratrum nigrum, the ginsenosides and alkaloids in the decoction of ginseng with veratrum nigrum were analyzed and compared by high performance liquid chromatography-electrospray ionization-mass spectrometry (HPLC-ESI-MS) and electrospray ionization-mass spectrometry (ESI-MS). In the compatible decoction, eight ginsenosides and eight alkaloids. were detected, and the contents of six ginsenosides were found to be reduced, on the contrary, the contents of six alkaloids were increased. During combination of ginseng with veratrum nigrum, the contents of ginsenosides were reduced and those of the toxic alkaloids were increased. From the chemical point of view, the traditional theory is right that ginseng and veratrum nigrum are incompatible with each other.

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A high performance liquid chroatography-electrospray ionization-mass spectrometric method was developed for analysis and identification of ginsenosides from the decoction of ginseng, ginseng with trogopteroum feces and ginseng with semen raphani. Ten ginsenosides were separated and detected. The content variation of these ginsenosides was researched. The experimental results showed, that ginsenosides were less in compatible decoction than in separate one expect Ro. the stripping of ginsenosides were restrained by semen raphani and during combination of ginseng with trogopteroum feces, the precipitates were produced by ginsenosides.

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Membrane distillation is a new membrane separation process which has been developed in the last few years. When a piece of microporous hydrophobic membrane separates two kinds of aqueous solutions different in temperature, the solutions cannot transport through the pores of membrane in any directions because of the hydrophobicity of membrane. However, vapor can readily penetrate through the

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Ginseng is one of the most expensive Chinese herbal medicines and the effectiveness of ginseng depends strongly on its botanical sources and the use of different parts of the plants. In this study, a microchip electrophoresis method coupled with the polymerase chain reaction (PCR)-short tandem repeats (STR) technique was developed for rapid authentication of ginseng species. A low viscosity hydroxypropyl methylcellulose (HPMC) solution was used as the sieving matrix for separation of the amplified STR fragments. The allele sizing of the amplified PCR products could be detected within 240 s or less. Good reproducibility and accuracy of the fragment size were obtained with the relative standard deviation for the allele sizes less than 1.0% (n = 11). At two microsatellite loci (CT 12, CA 33), American ginseng had a different allele pattern on the electropherograms compared with that of the Oriental ginseng. Moreover, cultivated and wild American ginseng can be distinguished on the basis of allele sizing. This work establishes the feasibility of fast genetic authentication of ginseng species by use of microchip electrophoresis.

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A new HPLC-APCI/MS method for the identification of ginsenosides has been developed. The analyses were performed on a reversed-phase C-18 column using a binary eluent (acetonitrile and water) under gradient conditions. Although APCI is a high-temperature evaporative process, HPLC-APCI/MS could effectively identify thermo-labile ginsenosides. The [M-H](-) ions and the thermal degradation ions of ginsenosides could be clearly observed under negative and positive ion conditions, respectively, and these were used to identify the molecular masses, the aglycone structures and the sugar groups of ginsenosides. APCI/MS can provide more explicit information than ESI/MS for identifying and distinguishing ginsenosides. Using the HPLC-APCI/MS method, 35 ginsenosides were identified in Panax ginseng. Copyright (C) 2005 John Wiley & Sons, Ltd.

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以西洋参(Panax quinquefolium L.)为材料,从胚、胚乳、多年生主根等外植体诱导筛选得到多种胚性及非胚性愈伤组织,胚来源的胚性愈伤组织经用附加1.0ppm 2,4-D的MS培养基继代保持三年后仍具旺盛的体细胞胚胎发生能力,以胚性愈伤组织建立的液体培养系统可得到大量游离的胚状体,将胚状体包埋制成的人工种子能在附加0.1ppm NAA和1.0ppm GA_3的B_s培养基上萌发形成根、茎、叶健全的再生植株,并且移栽成活。松软型根愈伤组织以过长期继代培养后,也得到了胚状体发生。比较了多种培养因素对体细胞胚胎发生和愈伤组织的影响,其中外植体来源、基本培养基的无机盐组成以及生长素是决定愈伤组织形态结构类型和体细胞胚胎发生能力的主要因素。胚乳愈伤组织、质密型根愈伤组织以及来源于胚的松软型非胚性愈伤组织在多种诱导条件下均未能发生胚状体。 从松软型的胚或根愈伤组织均容易游离大量原生质体,用悬浮培养物游离原生质体的得率更高,从早期胚状体也可酶解得到可用于培养量的原生质体。原生质体体积均很小,培养中的行为也相似,有些形成细胞壁,细胞变形,个别进行细胞分裂,形成少数细胞团,但未形成愈伤组织;有些原生质体仍保持球形,体积剧裂膨大几十倍,小液泡汇聚成大液泡,有些液泡中积累紫红色素。 用石蜡切片、半薄切片、透射电镜和扫描电镜等方法对各种愈伤组织的内部结构及外部形态进行了详细观察,发现胚状体起源于愈伤组织的表皮或表皮下层细胞,有单个发生和成丛发生两种发生方式,不同愈伤组织细胞的显微及超微结构各具特色。胚乳愈伤组织、松软型根愈作组织以及胚状体的细胞虽然都具有某些胚性细胞结构特征,例如细胞体积小、细胞核大、细胞质浓厚、细胞器丰富等,但它们并不具有现实的体细胞胚胎发生能力。发生胚状体的细胞含大量多核糖体和内质网片段,小液泡数量少且形成多泡复合体,细胞壁也由于在组织中所外的位置不同而有厚薄两种类型之分,细胞常形成胚性细胞复合体,位于愈伤组织的外围,边缘可分化为许多小细胞团。胚性细胞复合体的表面质密平整,有许多丝状物和颗粒,细胞轮廓不清,但有显著突出的小细胞,细胞表面具沟脊;而其它各型愈伤组织的表面均为球形或半球形的大型细胞,表面仅具细小的纹理、凸起或颗粒。 胚来源的胚性愈伤组织的总蛋白组成与来源相同,但形态结构截然不同的非胚性愈作组织的总蛋白组成差异显著,后者与形态结构特征相似的根本源公软型愈伤组织具有相似的蛋白质电泳带型,但多一条33KD的蛋白带;培养基中去掉2,4-D后,松软型根愈伤组织的蛋白质组成发生轻微变化。等电聚焦和SDS聚丙烯酰胺凝胶双向电泳揭示出在单向电泳扫描上呈现最高峰的17KD蛋白质在胚性愈伤组织中随等电点的不同而分离,在其它三种构软型愈伤组织中则仅集中在等电点为5.9处,为一个大而染色深的点。 同样培养基上培养的形态结构不同的愈伤组织所含元素的量不同,说明细胞对无机盐的吸收是有选择性的,不同类型的愈伤组织可积累不同的元素。培养基中的元素组成情况在愈伤组织中也有一定反映,在含钠、钾元素较多的B_5培养基上生长的愈伤组织中这两种元素的含量也较高,培养基的离子胁迫作用和细胞对离子一定程度的被动吸收会影响细胞的代谢方式,从而导致细胞类型的分化,基本培养基对愈伤组织类型的转变及体细胞胚胎发生能力的影响可能正是通过影响细胞的离子吸收、代谢平衡而实现。

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采用电喷雾多极串联质谱技术,对正、负离子条件下人参中的皂苷类化合物的碎裂机理、苷元类型和糖基的种类、连接顺序及连接位点的信息进行了系统的研究。并用高效液相色谱-电喷雾质谱联用技术, 对人参中的皂苷类化合物进行了在线分析,建立了中药粗提物中皂苷类化合物快速检测的方法。 采用电喷雾质谱和高效液相色谱-电喷雾质谱联用技术对人参与不同比例酸、甘味中药:五味子、麦冬、金银花、黄芪、何首乌配伍前后溶液中人参皂苷的种类与含量的变化进行了研究。建立了一种快速、简便地鉴别药对中人参皂苷化合物的方法。试验结果表明,各单体皂苷含量的变化十分复杂。有机酸对人参皂苷的溶出和水解有较为显著的影响。 采用电喷雾质谱和高效液相色谱-电喷雾质谱联用技术对人参与不同比例苦、辛味中药:附子、黄连、赤芍、大黄、干姜配伍前后溶液中人参皂苷的种类与含量的变化进行了研究。试验结果也表明,有机酸对人参皂苷的溶出和水解有一定的影响;附子和黄连中所含的生物碱类化合物在水溶液中对人参皂苷的影响不大,而将提取液换成50%的乙醇溶液则可以促进人参皂苷的溶出。 采用高效液相色谱-电喷雾质谱联用技术对与人参相反、相恶、相畏的中药藜芦、五灵脂、莱菔子与人参的配伍进行研究,观察人参皂苷在配伍前后的变化。试验结果表明:人参与这三种中药配伍后,溶液中人参皂苷总量下降,且人参对藜芦中毒性较大的藜芦生物碱的溶出具有促进作用。 采用高效液相色谱-电喷雾质谱联用技术对不同pH值水溶液中的人参皂苷的溶出,水解变化进行研究,试验结果表明:在碱性溶液中人参皂苷的溶出量增加且不易水解;在酸性溶液中,酸性越强人参皂苷溶出量越低且更易水解,水解产物较复杂,多为失去C20位糖基的小分子量人参皂苷和其C20的手性异构体,还可发现分子量为802Da的水合分子。 采用半制备液相色谱对二醇型皂苷Rb1和三醇型皂苷Re的水解产物进行分离和鉴定。共分离出四种分子量为802Da的水解产物。通过高分辨质谱仪对这几个化合物的特征质谱行为进行了系统研究,总结了该类化合物特征的质谱裂解规律,并鉴定了它们的结构。

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The intestinal bacterial metabolites of ginsenosides are responsible for the main pharmacological activities of ginseng. The purpose of this study was to find whether these metabolites influence hepatic metabolic enzymes and to predict the potential for ginseng-prescription drug interactions. Utilizing the probe reaction of CYP3A activity, testosterone 6beta-hydroxylation, the effects of derivatives of 20(S)-protopanaxadiol and 20(S)-protopanaxatriol families on CYP3A activity in rat liver microsomes were assayed. Our results showed that ginsenosides from the 20(S)-protopanaxadiol and 20(S)-protopanaxatriol family including Rb-1, Rb-2, Rc, Compound-K, Re, and Rg(1), had no inhibitory effect, whereas Rg(2), 20(S)-panaxatriol and 20(S)-protopanaxatriol exhibited competitive inhibitory activity against CVP3A activity in these microsomes with the inhibition constants (K) of 86.4+/-0.8mum, 1.7+/-0.1mum, and 3.2+/-0.2 mum, respectively. This finding demonstrates that differences in their chemical structure might influence the effects of ginsenosides on CYP3A activity and that ginseng-derived products might have potential for significant ginseng-drug interactions.

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Four different methods were used to process fresh ginseng into red ginseng in this paper. The contents of AFG in these red ginseng were determined by ESI-MS. The results show that the indirect steaming method plays an important role in increasing the AFG content, while soakage in vinegar alone has no effect on it.

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Four saponins were isolated from the leaves of Aralia elata, and established using NMR and other spectroscopic methods, as well as data reported in the literature. Three Aralia saponins from the leaves of Aralia elata sharing the same structures as those isolated from the root bark suggested that the leaves would be a good substitute for the root bark of Aralia elata. These four Aralia saponins were then extensively investigated using complementarily positive and negative electrospray ionization multistage tandem mass spectrometry (ESI-MSn). Two isomers of saponins with different sugar linkages were then successfully differentiated by positive ESI-MSn and verified with different retention times and the collision-induced dissociation (CID) spectra by LC-MS. A simple and effective LC-MS method was thus developed for the rapid identification and screening of these saponins in plant extracts from leaves of Aralia elata.

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Oligonucleotide from SARS virus was selected as a target molecule in the paper. The noncovalent complexes of ginsenosides with the target molecule were investigated by electrospray ionization mass spectrometry. The effects of experimental conditions were examined firstly on the formation of noncovalent complexes. Based on the optimized experimental conditions, the interaction of different ginsenosides with the target molecule was researched, finding that the interaction orders are relative with the structure of aglycons, the length and terminal sugar types of saccharide chains in the ginsenosides. There are certain rules for the interaction between the ginsenosides and DNA target molecule. For different type ginsenosides, the interaction intensity takes the orders 20-S-protopanaxatriol > 20-S-protopanaxadiol, and panaxatriol ginsenosides > panaxadiol ginsenosides. For the ginsenosides with the same type aglycone, tri-saccharide chain > di-saccharide chain > tetra-saccharide chain and single-saccharide chain > panaxatriol. For the ginsenosides with the same tetra-saccharide chain, the ginsenosides with smaller molecule masses > the ginsenosides with larger molecule masses.

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Five different processed methods for ginseng were used transferred ginsenosides with large molecule mass into low polar ginsenosides.The contents of low polar ginsenosides in these ginseng products were determined by ESI-MS.The results show that the high pressure steaming method make for increasing the concent of low polar ginsenosides,while soakage in vinegar is not good comparing with it.

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The hydrolysis of ginsenoside standards and the crude extracts of ginseng has been investigated at different pH values (2.4 - 11.2) using high performance liquid chromatography-electrospray ionization mass spectrometry (HPLC-ESI-MS). The experimental results indicated that the pH value of aqueous solutions is an important factor in changing the composition of ginsenosides. For (20S)-protopanaxadiol ginsenosides, ginsenosides with a large mass hydrolyzed to form hydrolysates (20S)-Rg(3) and (20R)-Rg(3) at pH 4.3. There were more hydrolyzed products observed at pH 3.3: (20S)-F-2, C-25,26 hydrated ginsenoside "C-Y-1" and "C-Y-2" (MW = 802 Da) accompanied with (20S)-Rg(3), (20R)-Rg(3). At pH 2.4, only (20R)-Rg(3), (20S)-F-2, a small quantity of (20S)-Rg(3) and three C-25,26 hydrated ginsenosides were obtained. For (20S)protopanaxatriol Re, no hydrolysates were observed at pH 4.3; it was hydrolyzed at pH 3.3 to form hydrolysates (20S)-Rg, (20R)Rg(2) and hydrated C-25,26 (MW = 802 Da) and at pH 2.4 only C-25,26 hydrated ginsenosides "C-Y-1" and "C-Y-2" (MW = 802 Da) were left in the solution. Similar hydrolysis reactions could be also observed for the crude extracts of ginseng. It showed that HPLC/ESI-MS is a fast and convenient method to study the hydrolysis of ginseng.