紫外导数分光光度法测定天麻中的天麻素和天麻甙元

样品用甲醇冷浸法提取。选用甲醇-乙醚(1 1)作为混合溶剂,采用二阶导数光谱可分离出天麻素和天麻甙元的吸收峰,在310～270nm间扫描,即可同时测定天麻中的天麻素和天麻甙元。方法简便,结果准确。样品中的其它组分不干扰测定。     

高效液相色谱法同时检测4种金线莲黄酮苷元及其在提取工艺评价中的应用

基于高效液相色谱(HPLC)和提取离子流色谱-质谱(EIC-MS),建立了金线莲提取成分定性定量分析及提取效率评价新方法。方法采用20RBAX Ecipse XDB-C18色谱柱,以乙腈-0.03%乙酸水溶液为流动相,采用梯度洗脱,同时分离测定金线莲提取液中芦丁、山奈酚、异鼠李素和槲皮素4种黄酮苷元的含量,经EIC-MS验证,结果可靠。以黄酮提取率为指标,评价酶解-醇提、回流-醇提、搅拌-醇提、超声-醇提、超声-微波-醇提和煎煮6种提取工艺,结果显示,最佳提取工艺为回流-醇提法,提取时间短,醇用量少,总提取率最高,可达14.96mg/g。     

密闭微波辅助萃取天麻中天麻素的研究

应用密闭微波萃取装置,对中药天麻中有效成分天麻素的萃取进行了研究。分别讨论了药材颗粒粒径、提取溶剂浓度、微波提取时间和提取剂的用量对微波萃取天麻素的影响。结果表明:当药材粒径<50μm,乙醇体积分数为50%,微波辐射时间为2min,提取剂质量为药材质量的30倍时,天麻素提取率最高。此外,将微波萃取与索氏萃取和超声波萃取进行了比较。     

三维荧光二阶校正法测定天麻中天麻素的含量

中药天麻背景复杂,对天麻素的激发-发射光谱(270nm/295nm)干扰特别大。本文利用三维荧光结合化学计量学二阶校正自加权交替三线性(SWATLD)算法对其进行解析,在不经分离的情况下测定了中药天麻中天麻素的含量。计算得到中药天麻中天麻素的平均含量是0.3766%,平均回收率为104.6%,分辨得到的天麻素解析光谱与真实光谱几乎完全重合。说明这种方法可用于中药天麻中天麻素含量的测定。     

天麻的化学研究——Ⅰ.天麻化学成分的分离和鉴定

从中药天麻的乙醇提取物中分离得到7个化学成分。根据红外光谱、核磁共振谱、质谱分析,衍生物制备,以及已知样品对照,证明为天麻苷(天麻素)(Gastrodin)、对羟基苯甲醇、对羟基苯甲醛、琥珀酸、β谷甾醇、蔗糖及一微量而未确证的1,4-二取代芳环化合物。其中天麻素的化学结构为对羟甲基苯β-D-吡喃葡葡糖苷。     

天麻化学成分的研究

天麻的石油醚和70%乙醇提取部分经硅胶柱层析,分得八个成分(Ⅰ～Ⅷ)。Ⅶ[C₁₃H₁₈O₇,熔点145～148℃[α]_D¹⁵-66.4°,(C.0.65,水)]为天麻主要成分,根据光谱分析、衍生物制备和苦杏仁酶水解产物的鉴定,确定其结构为对羟甲基苯β-D-吡喃葡葡糖苷,命名为天麻苷。其余七个化合物分别鉴定为天麻苷元——对羟基苯甲醇(Ⅲ)、β-谷甾醇(Ⅱ)及其D-葡葡糖苷即胡萝卜苷(Ⅵ)、柠檬酸(Ⅴ)及其单甲酯(Ⅳ)以及棕榈酸(Ⅰ)和蔗糖(Ⅷ)。     

不同产地金线莲根茎和叶中多糖含量对比

考察了不同产地金线莲根茎和叶中多糖含量。应用超声辅助法和微波-超声协同萃取法提取金线莲根茎和叶中多糖,用苯酚-硫酸法测定其含量。微波-超声协同萃取法提取优于超声辅助法提取,金线莲根茎部的多糖含量高于叶中多糖含量,福建华安产金线莲多糖含量最高。金线莲中多糖含量为0.8509%～6.400%,具有开发药用的价值。     

HPLC法测定不同施肥模式栽培的金线莲中黄酮类成分

HPLC法测定不同施肥模式栽培的金线莲中3种黄酮类成分:槲皮素、山奈酚和异鼠李素.超声-微波协同提取法提取4种不同施肥模式下金线莲中的黄酮类成分.HPLC-电喷雾离子化法/质谱(HPLC-ESI-MS)对黄酮类化合物进行定性分析.HPLC分析得槲皮素在0.25~20.0μg/m L(r=0.999 2)、山奈酚在0.25~20.0μg/m L(r=0.999 5)、异鼠李素在1.0~80.0μg/m L(r=0.999 0)范围内峰面积与浓度呈良好的线性关系,不同栽培方法的金线莲药材中槲皮素、山奈酚、异鼠李素的质量分数分别在151.8~240.0、47.2~88.2、16.8~29.8μg/g之间.方法简单、精确,快速,可为科学评价不同培养模式金线莲质量提供依据.栽培过程施加氮、磷、钾(NPK)复合肥及添加腐植素和微量元素,能提高金线莲中3种黄酮类成分的含量.栽培过程施加硫、磷(SP)复合肥,槲皮素、山奈酚和异鼠李素的质量分数分别下降了2.3%、17.2%和18.8%.结果表明采用不同施肥模式直接影响到药材中的药效物质的含量.     

化学发光法测定天麻素

天麻为兰科天麻属植物天麻Gastrodia elata Blume的块茎,性味甘平,有祛风定惊之功效,以天麻素为有效成分应用于临床。对天麻素的测定多用薄层层析-紫外分光光度法,而用化学发光法却未见报道。本文使用鲁米诺-过氧化氢-高锰酸钾发光体系,对天麻素进行了定量分析,取得了良好的效果。     

大孔吸附树脂对天麻素的吸附与分离特性的研究

研究了AB 8、NKA 9和S 83种大孔吸附树脂对中药天麻提取液中有效成分天麻素的吸附与分离特性。结果表明,NKA 9和S 8树脂对天麻素具有较好的吸附和解吸特性。其中经NKA-9树脂纯化的天麻素纯度为16.4%,比粗提物的天麻素纯度提高了1倍多。     

Cocondensation of urea with methylolphenols in acidic conditions

The reactions of urea with methylolphenols under acidic conditions were investigated using 2- and 4-hydroxybenzyl alcohol and crude 2,4,6-trimethylophenol as model compounds. The reaction products were analyzed with ¹³C-NMR spectroscopy and GPC. From the reaction of urea with 4-hydroxybenzyl alcohol, the formations of 4-hydroxybenzylurea, N,N′-bis (4-hydroxybenzyl) urea, and tris(4-hydroxybenzyl) urea were confirmed and the formations of N,N-bis(4-hydroxybenzyl) urea and tetrakis (4-hydroxybenzyl) urea were suggested. From the reaction of urea and 2-hydroxybenzyl alcohol, 2-hydroxybenzylurea and N,N′-bis(2-hydroxybenzyl) urea were identified. Further, the alternative copolymer of urea and phenol could be synthesized by the reaction of urea with 2,4,6-trimethylophenol. It was also found that the cocondensation between p-methylol group and urea prevails against the self-condensation of the methylolphenol even at the low pH below 3.0, and that p-methylol group has the stronger reactivity to urea than o-methylol group. © 1992 John Wiley & Sons, Inc.     

Three‐phase hollow fiber liquid‐phase microextraction combined with HPLC for determination of three trace acidic plant growth regulators in Anoectochilus roxburghii (Wall.) Lindl

The analysis of plant growth regulators presents a challenge due to their trace quantities and complex matrices. A novel, simple, and effective analytical method for the determination of three trace acidic plant growth regulators in Anoectochilus roxburghii (Wall.) Lindl was developed to address this issue. Three‐phase hollow fiber liquid‐phase microextraction combined with high‐performance liquid chromatography was applied for the enrichment, purification, and determination of three acidic plant growth regulators, namely, indole‐3‐acetic‐acid, indole‐3‐butyric‐acid, and (+)‐abscisic acid. The factors affecting extraction performance, including extractant species, pH of donor and acceptor phases, salt addition dosage, extraction time, temperature, and stirring rate, were investigated and optimized. Under optimum conditions, the proposed method provided good linearity (R², 0.9994–0.9999), low limit of detection (0.038–0.12 ng/mL), and acceptable relative recoveries (56.7–117.6%). The enrichment factors were between 153 and 328. The developed method was successfully applied to the enrichment and determination of plant growth regulators in Anoectochilus roxburghii (Wall.) Lindl and exhibited increased purification capacity, higher sensitivity, and decreased organic solvent consumption compared with conventional sample preparation methods. This method may provide a testing platform for the monitoring of plant growth regulator residues, ensuring the safe and effective use of traditional Chinese medicine.     

Simultaneous determination of six free fatty acids in alcohol extract of <Emphasis Type="Italic">P. japonicus</Emphasis> C. A. Mey. van <Emphasis Type="Italic">major</Emphasis> (Burk.) C. Y. Wu et K. M. Feng by gas chromatography-mass spectrometry

P. japonicus C. A. Mey. var. major (Burk.) C. Y. Wu et K. M. Feng is an important medicinal plant and has special beneficial effects on human health. Six types of free fatty acids (FFAs) were identified and quantified in the alcohol extract of P. japonicus C. A. Mey. var. major with a GC-MS method, including two fatty acids essential to the human body. All the six FFAs identified in alcohol extract were quantified using nonadecanoic acid as an internal standard. The results showed that the alcohol extract was abundant in four types of FFAs, unsaturated FFAs amounted to 47.04% of the total FFA content, and there were no trans FFAs. Palmitic acid (38.82%, 4.74 ± 0.09 mg/g) was the predominant fatty acid, followed by linoleic acid (27.92%, 2.31 ± 0.07 mg/g), stearic acid (14.14%, 1.54 ± 0.04 mg/g) and oleic acid (11.04%, 1.02 ± 0.03 mg/g).     

Determination of gastrodin,p-hydroxybenzyl alcohol, vanillyl alcohol,p-hydroxylbenzaldehyde and vanillin in tall gastrodia tuber by high-performance liquid chromatography

Summary A high-performance liquid chromatographic method for the separation and determination of gastrodin,p-hydroxybenzyl alcohol, vanillyl alcohol,p-hydroxylbenzaldehyde and vanillin in extract of Chinese herbal medicine tall gastrodia tuber (Chinese name: Tianma) was established. The chromatographic conditions were optimized by means of computer-assisted method development technique. Dry-Lab software was used to model the retention behavior of the compounds as a function of gradient conditions, based on the data from two scouting gradient runs. Under the optimized conditions: column, Kromasil-C18, 5 μm, 15×0.46-cm; solvent A, water; solvent B, methanol; gradient, 5/44/65/65% B at 0/9/12/15 min; flow rate, 1.00 mL min⁻¹; temperature, ambient, the quality of tall gastrodia tubers from different sources and tianma injection were examined.     

Application of Deep Eutectic Solvents as Additives in Ultrasonic Extraction of Two Phenolic Acids from Herba Artemisiae Scopariae

This paper reports the extraction of two phenolic acids from Herba Artemisiae Scopariae using deep eutectic solvents that were synthesized with various salt and hydrogen bond donors. The optimal conditions were found to be 50% of a synthesized deep eutectic solvent from tetramethyl ammonium chloride and urea (1:4) mixed with methanol/water (60:40, v/v). Phenolic acid extraction was optimized using an ultrasonic power of 89 W for 30 min with a solid/liquid ratio of 1:10. Under the optimized conditions, good calibration curves were observed at phenolic acid concentrations ranging from 10.0 to 500.0 µg/mL. The method recovery ranged from 97.3% to 100.4%, and the inter-day and intra-day relative standard deviations were less than 5%. Under the optimal extraction conditions, the amounts of chlorogenic acid and caffeic acid extracted from Herba Artemisiae Scopariae were 9.35 mg/g and 0.31 mg/g, respectively.     

Separation and purification of steroidal saponins from Paris polyphylla by microwave‐assisted extraction coupled with countercurrent chromatography using evaporative light scattering detection

A method of microwave‐assisted extraction coupled with countercurrent chromatography using evaporative light scattering detection was successfully developed for the separation and purification of steroidal saponins from Paris polyphylla. The main extraction conditions including microwave power, liquid/solid ratio, irradiation time, and extraction temperature were optimized using an orthogonal array design method. A suitable two‐phase solvent system consisting of n‐heptane/n‐butanol/acetonitrile/water (10:19:6:20, v/v/v/v) was employed in the separation and purification of the extracts of P. polyphylla. A total of 7.1 mg polyphyllin VII, 4.3 mg gracillin, 9.2 mg dioscin, and 10.2 mg polyphyllin I were obtained from 1.5 g P. polyphylla in less than 300 min, the purities of which determined by HPLC were 96.7, 97.3, 98.7, and 98.6%, respectively. The identification and characterization of these compounds were performed by LC–ESI‐MS and ¹H NMR spectroscopy. The results demonstrated that the proposed method is feasible, economical and efficient for the extraction, separation and purification of effective compounds from natural products.     

Extraction and preconcentration of residual solvents in pharmaceuticals using dynamic headspace–liquid phase microextraction and their determination by gas chromatography–flame ionization detection

The present study describes a microextraction and determination method for analyzing residual solvents in pharmaceutical products using dynamic headspace–liquid phase microextraction technique followed by gas chromatography–flame ionization detection. In this method dimethyl sulfoxide (μL level) placed into a GC liner‐shaped extraction vessel is used as a collection/extraction solvent. Then the liner is exposed to the headspace of a vial containing the sample solution. The effect of different parameters influencing the microextraction procedure including collection/extraction solvent type and its volume, ionic strength, extraction time, extraction temperature and concentration of NaOH solution used in dissolving the studied pharmaceuticals are investigated and optimized. Under the optimum extraction conditions, the method showed wide linear ranges between 0.5 and 5000 mg L⁻¹. The other analytical parameters were obtained in the following ranges: enrichment factors 240–327, extraction recoveries 72–98% and limits of detection 0.1–0.8 mg L⁻¹ in solution and 0.6–3.2 μg g⁻¹ in solid. Relative standard deviations for the extraction of 100 mg L⁻¹ of each analyte were obtained in the ranges of 4–7 and 5–8% for intra ‐ day (n = 6) and inter ‐ day (n = 4) respectively. Finally the target analytes were determined in different samples such as erythromycin, azithromycin, cefalexin, amoxicillin and co‐amoxiclav by the proposed method.     

Extraction and isolation of lithospermic acid B from Salvia miltiorrhiza Bunge using aqueous two‐phase extraction followed by high‐performance liquid chromatography

A rapid and effective method integrating separation and purification of lithospermic acid B from Salvia miltiorrhiza Bunge was developed by combining an aqueous two‐phase system extraction with preparative chromatography. An aqueous two‐phase system of n‐butyl alcohol/KH₂PO₄ was chosen from seven systems. The influence of parameters including concentration of KH₂PO₄, n‐butyl alcohol concentration, pH, and the ratio of an aqueous two‐phase system to crude extract were investigated using a single factor design. Response surface methodology was subsequently used to find the optimal compositions of an aqueous two‐phase system. Keeping a solvent‐to‐solid ratio of 10, the final optimized composition of an aqueous two‐phase system was 39.1% w/w n‐butyl alcohol and 22.6% w/w KH₂PO₄. Under these conditions a recovery yield of 99.8% and a high partition coefficient of 310.4 were obtained. In a pilot‐scale experiment using optimized conditions, 18.79 g of lithospermic acid B with a purity of 70.5% and in a yield of 99.8% was separated from 0.5 kg of crude extract. Subsequently, 9.94 g lithospermic acid B with a purity of 99.3% and recovery yield of 70.3% was obtained with a preparative chromatographic process, and the two‐step total recovery was 70.1%.     

Optimized Analytical Conditions for Eicosapentaenoic and Docosahexaenoic Acids in Antarctic krill Using Gas Chromatography

A simple method for the esterification of EPA and DHA in Antarctic krill was developed. When EPA and DHA standard solution (1.0 mg/mL in acetonitrile) reacted with equal volumes of 0.5% sulfuric acid-methanol at 60°C for 30 min, approximately 100% esterification conversion of EPA and DHA was achieved. Based on the esterification of EPA and DHA in Antarctic krill extraction solutions under these optimization conditions, the concentrations of EPA and DHA in fresh Antarctic krill were, respectively, 4.87 and 4.26 mg/g in the head, and 2.79 and 2.62 mg/g in the pleon. In the freeze-dried Antarctic krill, the amount of EPA and DHA were, respectively, 27.80 and 24.68 mg/g in the head, and 19.89 and 18.46 mg/g in the pleon.     

Microwave‐assisted extraction coupled with countercurrent chromatography for the rapid preparation of flavonoids from Scutellaria barbata D. Don

As a famous Chinese herb having good inhibitory effects on numerous human cancers both in vitro and in vivo, Scutellaria barbata D. Don attracts extensive attention worldwide. In this work, four flavonoids named scutellarin, baicalin, luteolin, and apigenin were simply and rapidly prepared from S. barbata by microwave‐assisted extraction coupled to countercurrent chromatography. Extraction conditions including irradiation time, extraction temperature, liquid/solid ratio, and microwave power were optimized using an orthogonal array design method. The extract of S. barbata was separated and purified with a two‐phase solvent system composed of hexane/ethyl acetate/methanol/acetic acid/water (1:5:1.5:1:4, v/v/v/v/v) and 4.5 mg of scutellarin, 4.6 mg of baicalin, 1.1 mg of luteolin, 2.1 mg of apigenin were obtained from 2.0 g original sample in a single run. The purities of scutellarin, baicalin, luteolin, and apigenin determined by HPLC were 93.6, 97.3, 97.6, and 98.4%, respectively. The targeted compounds were identified by LC with MS and ¹H NMR spectroscopy. The total time including extraction, separation, and purification was <300 min. Compared to traditional methods, microwave‐assisted extraction coupled to countercurrent chromatography method is more simple and rapid for the extraction, separation, and purification of flavonoid compounds from natural products.