高效液相色谱法研究当归指纹图谱

目的:研究当归药材的指纹图谱.方法:高效液相色谱法,Hypersil ODS柱(4.6 mm×250 mm,5μm),Kromasil ODS保护柱(4.6 mm×10 mm,5μm).甲醇-1%醋酸梯度流动相,流速1.0 mL/min,柱温25℃.以当归对照药材为对照品,色谱峰光谱采集范围:190~400 nm;以阿魏酸为参照物并测定了阿魏酸的含量,检测波长:323nm,流动相:甲醇-1%醋酸(40∶60,V/V),流速0.7 mL/min.结果:找出了22个共有峰,其中5号峰为阿魏酸,11个样品与当归对照药材之间的相似度均在90%以上,平均相似度为96.77%.结论:样品处理方法简单,研究所得的当归指纹图谱稳定性、重复性好,可以作为当归极性部分的特征性指纹图谱.     

菊花中活性成分的高效液相色谱测定与指纹图谱研究

采用高效液相色谱(HPLC)法测定了12个菊花样品中绿原酸、黄芩苷、槲皮素、木犀草素和柯因五种活性成分的含量。色谱柱为Nov-pak C18,以0.1%磷酸-甲醇为流动相,流速0.6 mL/min,梯度洗脱,检测波长为254 nm。该方法在10-3~10-5g/mL范围内线性关系良好,保留时间和峰面积相对标准偏差(RSD)分别在0.20%~0.96%、0.23%~0.77%之间,回收率在96.5%~104.0%之间。同时建立了菊花样品的指纹图谱,采用夹角余弦和相关系数法计算了12个菊花样品的相似度,并且运用MATLAB程序对相关系数法计算值进行聚类分析,结果与实际样品种属区分一致,为菊花的质量控制和种属的区分提供依据。     

液相色谱指纹图谱在泽泻动态研究中的应用

应用指纹图谱技术,结合指标成分测定,采用高效液相色谱法,乙腈-水梯度洗脱,流速1．0mL／min,柱温20℃,色谱图光谱采集范围200～800nm,探讨了泽泻动态积累的规律。以泽泻标准对照药材为参照,用指标成分24-乙酰泽泻醇A和23-乙酰泽泻醇B进行了定位和测定,找出了21个共有峰,其中12号和20号峰分别为24-乙酰泽泻醇A和23-乙酰泽泻醇B。结果表明：泽泻样品指纹图谱及指标成分测定可为泽泻的最佳采收期提供科学依据。     

高效液相色谱指纹图谱在中药芦根上的应用

利用现代分离分析技术如高效液相色谱(HPLC)与气相色谱(GC),能够获得中草药的色谱指纹图谱。本实验报道了高效液相指纹图谱应用于快速检测中草药提取物以及应用于研究、开发与生产中的质量控制体系中,利用HPLC建立芦根的色谱指纹图谱。实验条件为反相C18柱,流速为1．0mL／min,紫外检测器(λ=230nm)。通过分析比较色谱指纹图谱中的相对保留值α以及相对面积St对不同产地的芦根进行对比研究。这种基于HPLC的分析策略为中草药的精确鉴定和质量控制提供了有效的信息,并为HPLC在复杂组分样品中的应用开拓了新的领域。     

穿心莲药材高效液相色谱指纹图谱研究及其应用

应用反相高效液相色谱(RP-HPLC)法建立穿心莲药材指纹图谱。首先以穿心莲对照药材为对象建立其乙醇提取物特征色谱图,再用5种不同来源穿心莲药材的乙醇提取物验证色谱图的指纹特性。在穿心莲药材乙醇提取物特征色谱图中有共有峰10个,各共有峰的相对保留时间与相对峰面积的相对标准偏差(RSD)均小于4%。对照药材中共有峰峰面积占总峰面积的98.5%以上。该指纹图谱用于清火栀麦胶囊中穿心莲的鉴别专属性良好。     

高效液相色谱指纹图谱在地黄研究中的应用(Ⅰ)

长期以来,中药有效成分的提取分离和质量控制一直是中药产业中特有和尚未很好解决的问题.随着天然产物化学和现代仪器分析技术等相关学科的迅速发展,国内外在植物药及其制剂质量控制研究方面的重点均已转向利用各种仪器进行品质评价方面.中药来源于自然,其化学成分的多样性和复杂性是中药发挥其疗效的物质基础,同时也是质量评价与控制的重点与难点.中药的化学成分复杂,所体现的是综合效应和整体疗效.然而多年以来在中药的研究靠中,采取了与化学药品相同的研究思路,结果将药材及制剂内部各成分的综合作用和相互关系彼此孤立.在中药材及复方制剂质量标准的研究制定中,也往往是采用各种分析检测手段测定其中某种有效成分,并以其含量多少来判断比较某种药材的质量.这种质量控制模式很难做到全面衡量中药及其制剂的质量、疗效和稳定性.单一成分含量达标并不能说明该中药材质量合格.指纹图谱质量控制模式能综合反映某一特定药材各主要组分及其相对含量.因此它比测定任何一种或几种成分所提供的信息都丰富和有用的多.中药提取物在给定的实验条件下所得到色谱指纹图谱反映了该中药的化学组成及其含量分布状况,其特征峰可作为鉴别中药的依据.本文研究结果表明,利用色谱指纹图谱的相关参数来对中药原药材的质量进行控制,进而使中成药的质量得到保证,此方法的运用是切实可行的.另外,在有效成分不明确的前提下,利用色谱指纹图谱来评价中药的质量是有其意义的.色谱指纹图谱作为控制中药质量的新手段将在推进中药现代化进程上起到积极的作用.本文利用高效液相色谱建立了地黄的色谱指纹图谱.采用反相C18柱(5μm,150 mm×4.6 mm)、流动相甲醇:水(V/V=5:95)、检测波长为280 nm、流速1.0 mL/min进行试验.根据相对保留值和相对面积值对色谱指纹图谱进行分析对比研究,建立了控制地黄药材质量的新方法.该法为中药样品的鉴定提供了较全面的信息.     

高效液相色谱指纹图谱应用于板蓝根的鉴定

利用高效液相色谱建立了板蓝根的色谱指纹图谱。采用反相C18柱，流动相为水：甲醇（V/V=96：4），检测波长为260nm；流速1.0mL/min进行试验。根据相对保留值a和相对面积Sr对色谱指纹图谱进行分析对比研究，建立了一个快速、简易鉴别板蓝根样品的色谱指纹图谱分析方法。该法为中药样品的鉴定提供了较全面的信息，并为HPLC在复杂组分的样品分析和鉴别领域开拓了新的应用。     

丹参药材水溶性成分的高效液相色谱指纹图谱研究

采用高效液相色谱法(HPLC)对贵州铜仁丹参基地的丹参药材进行了指纹图谱研究。实验采用Zorbax SB-C18色谱柱 (5 μm, 4.6 mm i.d.×250 mm),以乙腈-0.4%(体积分数)冰醋酸水溶液为流动相,乙腈的体积分数在70 min内由0线性 增加到40%;流速1.0 mL/min;柱温25 ℃;检测波长254 nm。以19个主要共有峰为评价指标,采用国家药品监督管理局推荐 的“计算机辅助中药指纹图谱相似度计算软件”计算处理,建立了铜仁地区丹参药材的HPLC共有指纹图谱。该法操作简单 ,精密度、稳定性和重现性良好,有助于加强丹参药材的质量控制。     

不同产地白芷药材高效液相色谱指纹图谱研究

本文采用高效液相色谱-二极管阵列检测器(HPLC-DAD)法建立中药白芷的指纹图谱.应用化学计量学中两种不同的模式识别方法(主成分分析法和系统聚类分析法)对实验数据进行处理,以找出来自三个不同产地30个中药白芷样品间的相似性及差异性.两种模式识别方法均能成功地按样品的来源将不同产地的样品正确分类.建立了不同产地中药白芷的识别方法,该方法能有效地控制中药白芷的质量,并能为其它中药产品的化学模式识别提供参考.     

高效液相色谱指纹图谱应用于地黄的研究

利用高效液相色谱建立了地黄的色谱指纹图谱。采用反相C1 8柱 (5 μm ,1 5 0mm× 4.6mm) ,流动相甲醇∶水 (V V =5∶95 ) ,检测波长为 2 80nm ,流速 1 .0mL min进行实验。根据相对保留值和相对面积值对色谱指纹图谱进行分析对比研究 ,建立了控制地黄药材质量的新方法。该法为中药样品的鉴定提供了较全面的信息 ,并为HPLC在复杂组分的样品分析领域开拓了新的应用途径。     

Fingerprint chromatogram analysis of Pseudostellaria heterophylla (Miq.) Pax root by high performance liquid chromatography

A simple and reliable high performance liquid chromatographic (HPLC) method has been developed and validated for the fingerprinting of extracts from the root of Pseudostellaria heterophylla (Miq.) Pax. HPLC with gradient elution was performed on an authentic reference standard of powdered P. heterophylla (Miq.) Pax root and 11 plant samples of the root were collected from different geographic locations. The HPLC chromatograms have been standardized through the selection and identification of reference peaks and the normalization of retention times and peak intensities of all the common peaks. The standardized HPLC fingerprints show high stability and reproducibility, and thus can be used effectively for the screening analysis or quality assessment of the root or its derived products. Similarity index calculations based on cosine angle values or correlation methods have been performed on the HPLC fingerprints. As a group, the fingerprints of the P. heterophylla (Miq.) Pax samples studied are highly correlated with closely similar fingerprints. Within the group, the samples can be further divided into subgroups based on hierarchical clustering analysis (HCA). Sample grouping based on HCA coincides nicely with those based on the geographical origins of the samples. The HPLC fingerprinting techniques thus have high potential in authentication or source-tracing types of applications.     

Chemical fingerprint analysis of Fritillaria delavayi Franch. by high-performance liquid chromatography

Bulbus of Fritillaria delavayi Franch. is the most commonly used antitussive and apophlegmatic in China and commonly prepared by water decoction. In this study, a novel and reliable method of high-performance liquid chromatography (HPLC) was developed both for quantitative analysis of 10 bioactive compounds (uracil, cytidine, inosine, uridine, guanosine, thymidine, adenosine, hypoxanthine, adenine and 2-deoxyadenosine) and chemical fingerprint analysis of F. delavayi Franch. In quantitative analysis, 10 compounds showed good regressions (R(2) > 0.9982) within test ranges and the recovery of the method was in the range of 96.33-104.51%. In the fingerprint analysis, 11 characteristic peaks were selected to evaluate the similarities of F. delavayi Franch. samples, and the HPLC chromatograms of 16 samples from different regions of China showed similar patterns. The results from the experiment demonstrated that the combinations of the quantitative and chromatographic fingerprint analysis offer an efficient way to evaluate the quality consistency of F. delavayi Franch.     

Fingerprint quality control of Angelica sinensis (Oliv.) Diels by high-performance liquid chromatography coupled with discriminant analysis

High-performance liquid chromatography (HPLC) was employed in the fingerprint analysis of Angelica sinensis (Oliv.) Diels. A chromatographic profile of A. sinensis (Oliv.) Diels from the Dingxi District of Gansu province, China, was established as the characteristic fingerprint. The feasibility and advantages of employing chromatographic fingerprint combined with discriminant analysis were investigated and demonstrated for the evaluation of A. sinensis (Oliv.) Diels for the first time. Our results showed that the chromatographic fingerprint combining with discriminant analysis can efficiently distinguish A. sinensis (Oliv.) Diels from various areas.     

Fingerprint analysis of Dioscorea nipponica by high-performance liquid chromatography with evaporative light scattering detection

High-performance liquid chromatographic method (HPLC) with evaporative light scattering detection (ELSD) coupled with microwave-assisted extraction (MAE) as an efficient sample preparation technique has been developed for fingerprint analysis of Dioscorea nipponica. The samples were separated with an Agilent C8 column using water (A) and acetonitrile (B) under gradient conditions (0-10 min, linear gradient 20-40% B; 10-12 min, linear gradient 40-42% B; 12-25 min, isocratic 42% B) as the mobile phase at a flow rate of 1 mL min⁻¹ within 22 min. The ELSD conditions were optimized at nebulizer-gas flow rate 2.7 L min⁻¹ and drift tube temperature 90 °C. Precision experiments showed relative standard deviation (R.S.D.) of peak area and retention time were better than 2.5%; inter-day and intra-day variabilities showed that R.S.D. was ranged from 0.78% to 4.74%. Limit of detection was less than 50 μg mL⁻¹ and limit of quantification was less than 80 μg mL⁻¹. Accuracy validation showed that average recovery was between 97.39% and 104.07%. The method was validated to achieve the satisfactory precision and recovery. Relative retention time and relative peak area were used to identify the common peaks for fingerprint analysis. There are nine common peaks in the fingerprint. The quality of seven batches of D. nipponica samples was evaluated to be qualified or unqualified by the parameters “difference” and “total difference” of common peaks. Furthermore, the contents of important medicinal compounds (dioscin, prodioscin and gracillin) in different batches of D. nipponica samples were determined simultaneously using the developed HPLC-ELSD method. The results indicated variation of the herb quality which might be related to different producing area, growing condition, climate, harvest time, drug processing and so on. The developed analytical procedure was proved to be a reliable and rapid method for the quality control of D. nipponica.     

Faster analysis by reversed-phase high-performance liquid chromatography

Summary Many analysts are not taking full advantage of the high speed possibilities of modern LC. Some analytical procedures reported in the literature, and many in regular use in control laboratories, could be achieved in less time without loss in precision. Some factors which affect retention times are discussed and the advantages and disadvantages of employing shorter column lengths and finer packing materials in reversed-phase HPLC are examined. The effect on efficiency of increased flow rates with 10,5 and 3 m ODS materials is shown. The ability to couple shorter column lengths without loss of efficiency is also demonstrated. This allows a minimum length to be selected that gives adequate resolution. Examples of high speed separations are shown and limitations in state of the art HPLC equipment and chromatographic data systems are discussed briefly.Presented at the 14th International Symposium on Chromatography London, September, 1982     

Fingerprint analysis of Rhizoma chuanxiong by pressurized capillary electrochromatography and high-performance liquid chromatography

Pressurized capillary electrochromatography (pCEC) and high-performance liquid chromatography (HPLC) were used simultaneously to establish fingerprints of Rhizoma chuanxiong. Ten batches of Rhizoma chuanxiong collected from different regions in China were used to obtain the characteristic pCEC and HPLC fingerprints using a standardized procedure of sample preparation and analysis. A total of 22 common peaks were isolated within 60 min by pCEC and 16 common peaks by HPLC within 65 min. The fingerprints of Rhizoma chuanxiong were then used to identify the raw herbs from different sources in China. The two proposed methods demonstrated good stability and reproducibility with RSD less than 5% for retention time in pCEC and in HPLC, respectively. Finally, the data from the analyses of 10 batches of Rhizoma chuanxiong by pCEC and HPLC were all processed with similarity analysis with two mathematical methods, correlation coefficient and the included angle cosine. The fingerprints of Rhizoma chuanxiong established with pCEC and HPLC are suitable to identify samples from different sources and can be used to control the quality of raw herbs.     

Simultaneous determination of cyromazine,melamine and their biodegradation products by ion-pair high-performance liquid chromatography

An ion-pair high-performance liquid chromatography with ultraviolet detection method for the determination of cyromazine, melamine and its biodegradation products (ammeline, ammelide, cyanuric acid and biuret) was developed. C18 column was utilised to separate the six analytes with a mobile phase consisting of perchloric acid-ammonia solution and acetonitrile, under gradient elution and variable flow rate. The detection wavelengths were 205 nm for cyanuric acid and biuret and 222 nm for cyromazine, melamine, ammeline and ammelide. For analysis of sediment samples, the extraction solution containing acetonitrile, ammonia and water (80:10:10 by volume) was used to extract the analytes from sediment matrix. Using the extraction method for the spiked sediment sample, high linearity of matrix-matched standard curve could be obtained for the six analytes. The method detection limit was 0.1 μg g^?1 for melamine and cyromazine, 0.2 μg g^?1 for ammeline and ammelide, 1.2 μg g^?1 for cyanuric acid and 1.0 μg g^?1 for biuret in sediment matrix. The recoveries of these compounds were 70.1–98.3% and the relative standard deviations were 0.5–4.4%. Finally, the proposed method was successfully applied to the analysis of the sediment sample near the wastewater outlet of a melamine-producing factory.     

Chinese hamster ovary‐sphingomyelin synthase2 biospecific extraction and liquid chromatography with tandem mass spectrometry analysis for the prediction of bioactive components of Rhizoma Polygoni Cuspidati

A novel strategy for predicting bioactive components in traditional Chinese medicines using Chinese hamster ovary‐sphingomyelin synthase2 (CHO‐SMS₂) cell biospecific extraction and high‐performance liquid chromatography with diode array detection and tandem mass spectrometry analysis was proposed. The hypothesis is that when cells are incubated with the extract of traditional Chinese medicines, the potential bioactive components in the traditional Chinese medicines should selectively combine with the cells, while the cell‐combining components would be detectable in the extract of denatured cells. The identities of the cell‐combining components could be determined by liquid chromatography with tandem mass spectrometry. Using the proposed approach, the potential bioactive components of Rhizoma Polygoni Cuspidati, a commonly used traditional Chinese medicine for atherosclerosis, were detected and identified. Eight compounds in the extract of Rhizoma Polygoni Cuspidati were detected as the components selectively combined with CHO‐SMS₂ cells, which is a stable cell line that highly expresses sphingomyelin synthases, it was found that piceid, resveratrol, emodin‐8‐β‐d‐ glucoside, physcion‐8‐β‐d‐ glucoside, emodin, physcion, 3,5,4‘‐trihydroxystilbene‐3‐O‐(6“‐galloyl)‐glucoside, and emodin‐1‐O‐glucoside combined specifically with CHO‐SMS₂ cells. The results indicate that the proposed approach may be applied to predict the bioactive candidates in traditional Chinese medicines.     

Quantitative determination of bioactive alkaloids lysergol and chanoclavine in Ipomoea muricata by reversed-phase high-performance liquid chromatography

A rapid, simple, sensitive, gradient and reproducible, reverse‐phase high‐performance liquid chromatographic method was developed for the quantitative estimation of bioactive alkaloids, lysergol and chanoclavine in the seeds of Ipomoea muricata. The clavine alkaloid, lysergol, is a bioenhancer for the drugs and nutrients. The samples were analyzed by reverse‐phase chromatography on a Waters spherisorb ODS2 column (250 × 4.6 mm, i.d., 10 µm) using binary gradient elution with acetonitrile and 0.01 m phosphate buffer (NaH₂PO₄) containing 0.1% glacial acetic acid at a flow rate of 0.8 mL/min, a column temperature of 25 °C and UV detection at λ 254 nm. The limits of detection (LOD) and quantitation (LOQ) were 0.035 and 0.106 µg/mL for lysergol and 0.039 and 0.118 µg/mL for chanoclavine, respectively. Standard curves were linear in the range of 2–10 µg/mL (r > 99) for both analytes. Good results were achieved with respect to repeatability (RSD < 2%) and recovery (99.20–102.0). The method was validated for linearity, accuracy repeatability, LOQ and LOD. The method is simple, accurate and precise, and may be recommended for routine quality control analysis of I. muricata seed extracts containing these two clavine alkaloids (1, 2) as bioactive principles of the herb. Copyright © 2011 John Wiley & Sons, Ltd.     

Comparison of microemulsion electrokinetic chromatography with high-performance liquid chromatography for fingerprint analysis of resina draconis

Microemulsion electrokinetic chromatography (MEEKC) has been developed for fingerprint analysis of resina draconis, a substitute for sanguis draconis in the Chinese market. The microemulsion as the running buffer was made up of 3.3% (w/v) sodium dodecyl sulfate (SDS), 6.6% (w/v) n-butanol, 0.8% (w/v) n-octane, and 10 mmol/L sodium tetraborate buffer (pH 9.2), which was also used as the solvent for ultrasonic extraction of both water- and fat-soluble compounds in the traditional Chinese medicine samples. Four batches of resina draconis obtained from different pharmaceutical factories located in different geographic regions were used to establish the electrophoretic fingerprint. MEEKC was performed using a Beckman PACE/MDQ system equipped with a diode-array detector and with monitoring at 280 nm. The fingerprint of resina draconis comprised 27 common peaks within 100 min. The relative standard deviations of the relative migration time of these common peaks were less than 2.1%. Through repetitive injection of the sample solution six times in 24 h, all relative standard deviations of the migration time and peak area of loureirin A and loureirin B were less than 2.5 and 3.8%, which demonstrated that the method had good stability and reproducibility. The relative peak areas of these common peaks in the electropherograms of four batches of resina draconis were processed with two mathematical methods, the correlation coefficient and the interangle cosine, to valuate the similarity. The values of the similarity degree of all samples were more than 0.91, which showed resina draconis samples from different origins were consistent. On the other hand, high-performance liquid chromatography (HPLC) coupled with photodiode-array detection was also applied to establish the fingerprint of resina draconis. The samples were separated with a LiChrospher C₁₈ column using acetonitrile (solvent A) and water containing 0.1% H₃PO₄ (solvent B) as the mobile phase in linear gradient elution mode at a flow rate of 0.6 mL/min and detection was at 280 nm. There were only 20 common peaks in the HPLC fingerprint, and the values of the similarity degree of all samples were also more than 0.91. Though the similarity results of fingerprint analysis seemed to be the same, MEEKC resulted in more common peaks and higher separation efficiency for a variety of polarities of the components than HPLC. So, MEEKC was more suitable for development of the fingerprint of resina draconis.