鱼腥草中黄酮类成分的高效液相色谱指纹图谱分析

采用均匀实验设计和信息理论评价方法,建立了鱼腥草中黄酮类成分的高效液相色谱(HPLC)指纹图谱的分析方法。采用建立的方法和本研究室提出的指纹图谱评价软件,对同样种植条件下10个批次的鱼腥草指纹图谱进行了相似性评价,相似度均大于0.90;同时测定了芦丁、槲皮甙和槲皮素3个成分在10批鱼腥草药材中的含量分别为0.25%～0.34%、0.27%～0.37%、0.012%～0.016%。另外对不同采收季节和不同部位的鱼腥草药材中的黄酮类成分进行了指纹图谱的测定、主成分分析以及成分含量测定,结果表明,不同季节、不同部位的鱼腥草中黄酮类化合物的指纹图谱及成分含量存在较大的差异,且药用部位的差异大于采收季节的差异。该方法为规范鱼腥草中黄酮类成分在制药和用药的实际应用提供了一些可靠的基础信息。     

基于化学模式识别和熵权TOPSIS法分析鱼腥草不同部位的差异

基于高效液相色谱（HPLC）指纹图谱比较鱼腥草不同部位（茎、叶）化学成分的差异性,并综合评价鱼腥草不同部位的质量。建立鱼腥草不同部位的HPLC指纹图谱,通过相似度评价、化学模式识别及熵权TOPSIS法对其化学成分进行差异性研究,并对其质量标志物（槲皮苷）进行含量测定。建立的HPLC指纹图谱中鱼腥草药材及其茎叶均确定了8个共有峰,指认了其中6个成分;聚类分析（CA）和主成分分析（PCA）结果表明鱼腥草叶和茎的质量差异大,叶和药材的质量较接近;偏最小二乘法-判别分析（OPLS-DA）发现4种成分是造成不同批次样品差异性的主要标志物;熵权TOPSIS法分析显示同批次鱼腥草药材与其茎叶既有相关性也有差异性,且四川产地的鱼腥草药材质量较佳;含量测定结果显示,同批次鱼腥草中的槲皮苷含量由高到低均依次为叶、药材、茎。鱼腥草不同部位HPLC指纹图谱存在显著差异。该方法可反映鱼腥草不同部位质量差异性,为鱼腥草药材的质量控制及资源开发利用提供参考。     

气相色谱-质谱联用结合化学计量学方法分析光照对鱼腥草挥发性成分的影响

采用色谱-质谱联用技术结合化学计量学方法对不同光照生长条件的鱼腥草挥发性成分进行分析。水蒸气蒸馏法提取鱼腥草挥发油,气相色谱-质谱进行分析。色谱指纹图谱结合主成分分析与相似度评价以探究不同光照挥发油成分的异同。直观推导式演进特征投影法(Heuristic evolving latent projections,HELP)分辨重叠色谱峰,NIST标准质谱库结合相关文献进行定性,峰面积归一化法定量,t-检验比较不同光照组成分含量间是否有显著性差异。3种光照下的鱼腥草挥发油指纹图谱存在一定的共性和差异,共鉴定出33种化合物,共有化合物26种。随着光照强度的减少,单萜类化合物含量减少,非萜类含量增多,倍半萜类变化不大。癸酰乙醛和甲基正壬酮在全光照组的含量明显低于遮光组的含量。研究结果表明,适度的遮光有利于鱼腥草挥发性有效成分含量的提高,鱼腥草药材挥发性成分种类及含量与生长条件密切相关。     

气相色谱-质谱联用结合化学计量学方法分析光照对鱼腥草挥发性成分的影响

采用色谱-质谱联用技术结合化学计量学方法对不同光照生长条件的鱼腥草挥发性成分进行分析。水蒸气蒸馏法提取鱼腥草挥发油,气相色谱-质谱进行分析。色谱指纹图谱结合主成分分析与相似度评价以探究不同光照挥发油成分的异同。直观推导式演进特征投影法(Heuristic evolving latent projections,HELP)分辨重叠色谱峰,NIST标准质谱库结合相关文献进行定性,峰面积归一化法定量,t-检验比较不同光照组成分含量间是否有显著性差异。3种光照下的鱼腥草挥发油指纹图谱存在一定的共性和差异,共鉴定出33种化合物,共有化合物26种。随着光照强度的减少,单萜类化合物含量减少,非萜类含量增多,倍半萜类变化不大。癸酰乙醛和甲基正壬酮在全光照组的含量明显低于遮光组的含量。研究结果表明,适度的遮光有利于鱼腥草挥发性有效成分含量的提高,鱼腥草药材挥发性成分种类及含量与生长条件密切相关。     

HPLC指纹图谱结合灰色关联度分析综合评价云南丽江秦艽资源

对采自云南丽江17个不同产区秦艽样品建立其HPLC指纹图谱,测定了药材中9大质量指标并进行灰色关联度分析,建立一种新型秦艽质量综合评价方法。采用甲醇-0.1%磷酸为流动相体系,梯度洗脱,建立17批秦艽药材的高效液相色谱指纹图谱;采用HPLC法测定马钱苷酸,龙胆苦苷和獐牙菜苦苷含量;按药典方法测秦艽中醇溶性浸出物、总灰分、酸不溶性灰分含量;分光光度法测定多糖含量。建立的丽江秦艽药材的HPLC指纹图谱的相似度极高,通过对多项指标的灰色关联度分析遴选出X2和X12两个优级药材资源。指纹图谱结合多指标成分的灰色关联度分析,能全面评价秦艽药材质量,亦可从中筛选优质秦艽资源和为秦艽道地适宜产区的规划确定提供依据。     

鱼腥草注射液与其药材挥发油相关组分的分析

利用GC-MS提供的二维化学数据信息,通过多组分波谱相关色谱方法及化学计量学分辨技术,对中试生产的鱼腥草注射液及其对应的药材挥发性成分进行比较和归属分析。结果表明,在药材和注射液图谱的40个峰族中,只有5个非相关峰族,即在药材制成成品注射液过程中,尽管大量组分出现了浓度消长的现象,但是成品注射液的绝大部分成分来自药材,其中仅有少数组分出现了消失和生成现象。     

HPLC衍生化法分析决明子多糖水解产物中单糖组分及其多糖组成特征的研究

分别利用分光光度法和1-苯基-3-甲基-5-吡唑啉酮(PMP)衍生化/HPLC法分析了12批不同批次药材的决明子多糖及其水解产物中的单糖组分,以水解的单糖组分建立了决明子多糖的HPLC指纹图谱,并研究了决明子多糖的组成特征。结果表明,经过纯化的决明子多糖含量在93.41%~98.57%之间,以甘露糖为参照峰建立了12批药材的指纹图谱,相似度在0.963~0.999之间,多糖水解产物中单糖组分的含量在1.617~304.5 mg/g之间,7个共有峰组分含量大小分布均依次为:甘露糖木糖半乳糖葡萄糖阿拉伯糖葡萄糖醛酸氨基半乳糖,显示了决明子多糖的基本组成结构特征,12批药材的决明子多糖中各单糖的平均摩尔比为甘露糖∶木糖∶半乳糖∶葡萄糖∶阿拉伯糖∶葡萄糖醛酸∶氨基半乳糖=43.0∶24.2∶15.4∶5.6∶5.5∶3.4∶2.9。指纹图谱相似度分析和多糖的组成特征分析对市售药材的分析鉴定结果一致,可作为决明子多糖结构分析及其质量控制的依据。     

基于化学指纹图谱和抗血小板聚集效价的丹参质量评价

通过化学分析和生物活性评价考察丹参药材的品质差异,探讨丹参抗血小板聚集生物活性的主要贡献成分.采用高效液相色谱(HPLC)技术建立丹参药材HPLC指纹图谱,以抗血小板聚集相对效价作为指标,评价不同产地不同批次丹参药材的品质差异,构建基于化学表征及生物效价测定的评价模式.结果表明,不同批次丹参药材的HPLC指纹图谱相似度很高(相似度0.930~0.998),而其抗血小板聚集相对效价相差10倍,提示化学指纹图谱难以反映丹参的活性和质量差异.通过化学指纹图谱与抗血小板聚集生物效价进行谱效相关分析,筛选出与生物活性相关系数大于0.5的6个色谱峰:二氢丹参酮Ⅰ、隐丹参酮、丹参酮Ⅰ、丹参酮ⅡA及2个未知化合物.对上述4种已知化合物单体进行活性验证发现,隐丹参酮的抗血小板聚集活性最强,而其它3种丹参酮类化合物几乎没有体外抗血小板聚集活性.进一步比较丹参中高含量成分丹酚酸B与低含量成分隐丹参酮的活性贡献,结果表明,两者的活性贡献基本相当,说明隐丹参酮是丹参中低含量高活性成分,对评价丹参质量具有重要贡献度.     

高效液相色谱法分析玉屏风散成分

建立玉屏风散高效液相色谱指纹图谱分析方法,探讨市售饮片对玉屏风散质量一致性的影响。用传统水煎法制备玉屏风散水煎液,采用高效液相色谱法对不同来源的单味药饮片制备的玉屏风散样品进行测定,用色谱指纹图谱相似度评价软件对指纹图谱进行分析,以对照药材制得的标准方剂为参照,评价不同批次饮片对玉屏风散成分的影响。试验结果表明,10批玉屏风散指纹图谱之间的相似度差异较大,与标准方剂的指纹图谱相比较,有6批相似度低于0.5,3批在0.5～0.8之间,1批高于0.9。10批样品指纹图谱中有22个共有峰,利用标准品对照法鉴定了其中6个成分。试验表明药材饮片的来源对玉屏风散的成分影响较大。     

灰色系统理论在中药色谱指纹图谱模式识别中的应用研究

建立了基于灰色系统理论的中药色谱指纹图谱模式识别模型。运用基于范数与信息熵赋权法的灰色关联分析,求出各待比较图谱特征变量数据序列与理想图谱特征变量数据序列之间的灰色关联度,并依据模糊匹配中的“最大匹配度”原则进行判断,从而达到品种识别和质量评价的目的。该模型在56批次不同品种化橘红药材样品的高效液相色谱分析中取得较满意的结果: 熵权与范数的灰色关联分析均能准确识别出毛橘红与光橘红两个品种,克服了传统相似度或灰色关联在化橘红色谱指纹图谱分析中的误判问题;对药材中化学成分的种类与含量十分接近的毛橘红不同栽培品种的识别率超过92.85%。此外,该模型计算量较少,整个模式识别过程通过计算机编程实现,操作简单。实验结果显示,灰色系统理论在中药色谱指纹图谱模式识别中有良好的适应性。     

Establishment of GC-MS fingerprint of fresh Houttuynia cordata

Fresh Houttuynia cordata THUNB. is a Chinese materia medica generally used in Chinese medicine therapy. It possesses the actions of clearing heat, eliminating toxins, reducing swelling, discharging pus and relieving stagnation. However, dry H. cordata has traditionally been used in clinical application instead of the fresh counterpart. In this paper, the chemical profiles of H. cordata were established using fingerprinting techniques. A modified GC-MS method was developed in the comparison of fingerprints among fresh and dry herbs of H. cordata. It was shown that the varieties, as well as relative levels of chemical components, in the fresh herb were more abundant than in the dry counterpart. Fingerprinting profiles were found to be consistent for fresh herbs acquired from various production areas, but the relative abundance of peaks were varied. Besides, the chemical components among different medicinal portions of fresh herbs were found to be inconsistent. The developed fingerprint can be successfully applied to distinguish between fresh and dry herbs, as well as determining differentiation among different medicinal portions.     

Establishment of HPLC-DAD-MS fingerprint of fresh Houttuynia cordata

A HPLC-DAD-MS fingerprint method of fresh Houttuynia cordata THUNB. was developed basing on the consistent chromatographic features among 11 batches of authentic samples. Major chemical components including phenolic compounds, flavones and alkaloids were simultaneously analyzed. Eleven common peaks in the fingerprint were chosen and identified by comparing their UV and ESI-MS data with the authentic compounds. The unique properties of this HPLC-DAD-MS fingerprint were successfully applied to analyze and differentiate samples from different geographical origins, processing methods and various medicinal parts of H. cordata. The results showed that these variations will give rise to differences in identities and/or abundance of chemical compounds, indicating that a comprehensive quality evaluation of those major ingredients in H. cordata is critical to assess and represent its overall quality.     

Tentative fingerprint-efficacy study of Houttuynia cordata injection in quality control of traditional Chinese medicine

To establish potent fingerprint for quality control of traditional Chinese medicine, Houttuynia cordata (Saururaceae) injection (HCI), the attempt on fingerprint-efficacy was developed in this study. HCI from ten different factories were determined by gas chromatography-mass spectrum (GC-MS) and classified by hierarchical clustering. The anti-inflammatory effect of HCI was characterized with the rat pleurisy model induced by carrageenin and the mice ear edema model by xylene. The results showed that anti-inflammatory effect of the injections from most of factories on the two models was significant. There was corresponding relationship between the fingerprint of HCI and efficacy to certain extent. The main common constitutes in injection from the factories that possess anti-inflammatory activity were analysed with GC-MS and identified using the NIST Mass Spectral Database. This common pattern of HCI based on the efficacy was helpful for the purpose of quality control.     

保留指数结合准确质量测定对鱼腥草挥发性成分的定性分析

采用顶空-气相色谱-四极质谱法和顶空-气相色谱-飞行时间质谱法对鱼腥草挥发性成分进行检测,运用保留指数结合准确质量测定,分别从鱼腥草茎和叶中鉴定出49、39种挥发性组分,并采用峰面积归一化法测定各组分的相对含量。鱼腥草茎和叶中的挥发性成分差别较大。鱼腥草茎以α-蒎烯(12.24%)、β-蒎烯(22.42%)、月桂烯(11.98%)、乙酸冰片酯(10.97%)、甲基正壬酮(10.83%)为主要成分,而鱼腥草叶则以月桂烯(39.48%)、(Z)-β-罗勒烯(26.52%)、癸醛(10.35%)、桧烯(4.43%)、甲基正壬酮(2.44%)为主。结合保留指数和准确质量测定能显著提高质谱定性的准确性,有利于解决质谱检索时定性不确定的问题。     

Flash Evaporation and Headspace Solid-phase Microextraction for the Analysis of the Essential Oils in Traditional Chinese Medicine, Houttuynia Cordata Thunb

We have investigated the use of flash evaporation, headspace solid-phase microextraction (HS-SPME) and steam distillation (SD) as sample concentration and preparation techniques for the analysis of volatile constituents present in Houttuynia cordata Thunb. The samples were analyzed by gas chromatography (GC) and identified by mass spectrometry (MS). Comparison studies were performed. It was found that the results obtained between Headspace solid-phase microextraction HS-SPME and SD techniques were in good agreement, Seventy-nine compounds in Houlluynia cordata Thunh were identified by MS. In flash evaporation, thirty-nine compounds were identified. Discrimination in the response for many constituents studied was not observed, which can be clearly observed in SD and HS-SPME techniques. As a conclusion, HS-SPME is a powerful tool for determining the volatile constitutes present in the Houttuynia cordata.     

Flash gas chromatography for analysis of volatile compounds from Houttuynia cordata Thunb

This paper describes a novel analytical method, flash gas chromatography (FGC), for the analysis of volatile compounds from Houttuynia cordata Thunb. This method does not demand time-consuming extraction process. The ground powder of the plant material can be directly applied for the analysis and only a few milligrams of sample are needed. The identification of the components was made by FGC-MS. The results between FGC and ordinary GC (using the extracted essential oil as sample) were compared and found that FGC offered a similar number and types of the components with GC. FGC is a novel and feasible method for the quality control of traditional Chinese medicines (TCMs).     

Comparing chemical fingerprints of herbal medicines using modified window target-testing factor analysis

A chromatographic fingerprint of a herbal medicine is essentially its chromatographic spectrum: a characteristic representation of its chemical components, some of which are pharmacologically active. Since a wide variety of factors, such as the geographical location, the harvest season, and the part used can influence the chemical constituents (and therefore the pharmacological activity) of any particular herbal medicine and its products, these fingerprints provide a way to compare and contrast the compositions of different variants of the same herbal medicine. In particular, it is possible to ascertain whether particular components present in one herbal fingerprint are also present in another fingerprint. In this work we use a novel method—modified window target-testing factor analysis (MWTTFA), based on the use of target factor analysis (TFA), fixed-size moving window evolving factor analysis (FSMWEFA) and a Gaussian shape correction to the chromatographic profiles—to achieve this end. To demostrate the strategy, the fingerprints of samples from garlics produced in different geographical locations were compared, as well as the fingerprints of samples taken from above-ground and below-ground parts of Houttuynia cordata Thunb. The results from these comparisons clearly show that four chemical components present in Hunan common edible garlic are absent in Xingping base garlic, while seven components are present in Xingping base garlic but absent in Hunan common edible garlic. Also, eleven components are present in the sample from the above-ground part of Houttuynia cordata Thunb but not in the sample from the below-ground part, while seven components are present in the sample from the below-ground part of Houttuynia cordata Thunb that are not present in the sample from the above-ground part. These interesting conclusions should be very useful for future pharmacological and clinical research into these herbal medicines, and the novel MWTTFA technique can also be used for quality control purposes.     

HPLC柱切换技术用于同时分析鱼腥草中3种黄酮类成分

利用柱切换技术解决了鱼腥草中难分离组分的分离和低含量组分的定量问题。以Synergi Fusion-RP柱(250 mm×4.6 mm i.d.,4μm)作为预柱,甲醇-0.05%磷酸溶液作流动相,以Acclaim120 C18柱(250mm×4.6 mm i.d.,5μm)作为分析柱,乙腈-0.05%磷酸溶液作流动相,对鱼腥草中的3种黄酮类成分进行分析。该方法在10.0～1 000.0 mg.L-1范围内线性关系良好,相关系数(r)不低于0.998,回收率为95%～99%,RSD值均小于3%。该方法操作简便、快速,可作为分析鱼腥草中黄酮类组分的有效手段。