复方丹参提取物高效液相色谱-紫外-蒸发光散射检测指纹图谱的建立

采用紫外/蒸发光散射检测器(UV和ELSD)串联检测技术,建立了复方丹参提取物HPLC/UV/ELSD指纹图谱。运用指纹图谱相似度评价软件,对14批复方丹参提取物HPLC/UV/ELSD指纹图谱进行相似度计算,结果相似度良好。该指纹图谱能同时反映复方丹参提取物中丹参和三七的主要化学组分特征,可有效评价复方丹参提取物的质量稳定性。     

综合线性定量指纹法评价退热解毒注射液融合指纹图谱研究

该研究引入综合线性定性相似度Sl、综合线性定量相似度Pl%和指纹变异系数α3个参数建立了1种新颖的综合线性指纹图谱评价方法,从定性定量的角度全面评价了中药的整体质量。方法采用高效液相二极管阵列(HPLC/DAD)采集了退热解毒注射液样品在210、254、265、330、360 nm波长下的指纹图谱并进行数据融合,同时定量分析了绿原酸、连翘酯苷A、丹皮酚和柴胡皂苷D 4个指标成分。通过综合线性指纹法鉴定样品质量。结果显示,10批注射液样品被分成5个等级,10批中间体样品被分成4个等级。此外,4个指标成分的定量分析结果与融合指纹图谱的定量相似度Pl%具有高度相关性,表明综合线性定量指纹法具有代替标准物质用于样品定量分析的潜力。该方法为中药整体质量控制提供了一种新思路。     

双定性双定量相似度法评价银杏达莫注射液的高效液相色谱指纹图谱

建立了色谱指纹图谱的双定性双定量相似度评价法,并应用于银杏达莫注射液的高效液相色谱（HPLC）指纹图谱的评价。采用反相HPLC,以芦丁为参照物峰,确定了41个共有峰,建立了银杏达莫注射液的对照指纹图谱。以双定性相似度S和S′、双定量相似度C和P评价银杏达莫注射液的HPLC指纹图谱,分别考察在大峰缺失和小峰缺失两种情况下,4个相似度指标的变化特征。S能反映化学成分的分布比例,受大峰影响严重,无法反映小峰的丢失; S′对所有指纹峰等权,反映小峰缺失灵敏,二者构成双定性相似度。C能反映样品共有峰的总体含量,但受大峰影响严重,无法反映小峰的缺失; P对所有峰积分值等权,能较好地反映小峰的变动,二者构成双定量相似度。因此,由S与S′、C与P构成的双定性双定量相似度法能同时监测大峰和小峰的变动与缺失,能准确地解决色谱指纹图谱的宏观定性和定量评价问题。同时还提出了方向余弦作为对照指纹图谱的特征指纹的概念和分解相似度的概念,以此考察了各指纹峰对相似度贡献的大小及其在不同程度缺失时4种相似度的变化情况。所建立的HPLC对照指纹图谱可用于银杏达莫注射液的质量控制。     

气相色谱-质谱指纹图谱在甄别真假卷烟上的应用

运用固相微萃取／气相色谱-质谱法建立卷烟挥发性和半挥发性物质的指纹图谱。通过指纹图谱相似度评价软件，对12批正品卷烟和1个假冒品卷烟的指纹图谱进行了相似度计算，结果表明：12批样品间相似度很好，而假冒品卷烟与正品卷烟的相似度很低，该方法为探讨卷烟质量稳定和甄别真假卷烟提供了一种简便易行的方法模式。     

基于信息融合的中药多元色谱指纹图谱相似性计算方法

摘要用信息融合算法合并多张色谱指纹图谱, 解决中药多元指纹图谱相似性评价难题, 提出一种多元色谱指纹图谱相似度计算方法. 用该方法先对各单元指纹图谱进行串行或并行象素级信息融合, 再对融合了各指纹峰信息的多元色谱指纹图谱进行相似度评价. 计算机仿真和复方丹参滴丸多元HPLC指纹图谱应用结果表明, 该法能够评价中药多元色谱指纹图谱相似度, 定量表征中成药产品批次间质量波动情况.     

HPLC指纹图谱相似度研究

将HPLC指纹图谱看作多维空间内的向量,利用向量夹角余弦的基本公式计算两个指纹图谱间的相似度。用7个不同品种的金银花提取物的HPLC指纹图谱对计算方法进行了检验,结果表明相似度能较好地定量评价指纹图谱间的相似性,可应用于中药质量控制。     

系统指纹定量法鉴别龙胆泻肝丸质量

建立龙胆泻肝丸(Longdanxiegan pill,LDXGP)的高效液相色谱(HPLC)指纹图谱,以系统指纹定量法评价其质量.采用RP-HPLC法,以宏定性相似度为参量对12批LDXGP进行聚类分析,确定用其中10批生成对照指纹图谱(RFP),以此RFP为标准用系统指纹定量法评价12批LDXGP质量.以龙胆苦苷为参照物峰,确定60个共有指纹峰,建立了LDXGP的HPLC指纹图谱.用系统指纹定量法鉴别出8批质量合格,1批含量明显偏高,1批含量明显偏低,2批化学成分数量和分布比例不合格.系统指纹定量法将整体定性分析和整体定量分析密切结合,是评价中药质量的有效方法.     

五加生化胶囊的高效液相色谱指纹图谱研究

应用高效液相色谱(HPLC)法建立五加生化胶囊的指纹图谱。采用ANGLAVenusil XBP-C18色谱柱(250×4.6mm,5μm),以甲醇-0.1%磷酸溶液为流动相,梯度洗脱,检测波长为327nm,五加生化胶囊多数峰达到基线分离。采用2004A中药色谱指纹图谱相似度评价系统对11批样品的指纹图谱进行峰匹配,确定12个共有峰,11批五加生化胶囊指纹图谱的相似度均在0.90以上。结果表明:五加生化胶囊的HPLC指纹图谱特征性和专属性强,可较系统地用于五加生化胶囊的质量控制。     

基于三波长融合谱的系统指纹定量法鉴定龙胆泻肝丸的真实质量

建立了龙胆泻肝丸(Longdanxiegan pill,LDXGP)三波长融合高效液相色谱(HPLC)指纹图谱,以系统指纹定量法全面鉴定LDXGP的质量。采用反相高效液相色谱法(RP-HPLC),运用多波长融合指纹图谱技术对色谱图进行处理,以黄芩苷为参照物峰,确立了63个共有指纹峰,以宏定性相似度为参量对12个厂家的12批LDXGP进行聚类分析,确定用其中10批生成对照指纹图谱(RFP),以此RFP为标准用系统指纹定量法评价12批LDXGP的质量。结果鉴别出9批质量完全合格,1批含量明显偏高,2批化学成分数量和分布比例不合格。基于多波长融合技术的系统指纹定量法是评价中药真实质量的可靠方法。     

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。     

Quality evaluation of Yin Chen Hao Tang extract based on fingerprint chromatogram and simultaneous determination of five bioactive constituents

A completely validated method based on HPLC coupled with photodiode array detector (HPLC-UV) was described for evaluating and controlling quality of Yin Chen Hao Tang extract (YCHTE). First, HPLC-UV fingerprint chromatogram of YCHTE was established for preliminarily elucidating amount and chromatographic trajectory of chemical constituents in YCHTE. Second, for the first time, five mainly bioactive constituents in YCHTE were simultaneously determined based on fingerprint chromatogram for furthermore controlling the quality of YCHTE quantitatively. The developed method was applied to analyze 12 batches of YCHTE samples which consisted of herbal drugs from different places of production, showed acceptable linearity, intraday (RSD <5%), interday precision (RSD <4.80%), and accuracy (RSD <2.80%). As a result, fingerprint chromatogram determined 15 representative general fingerprint peaks, and the fingerprint chromatogram resemblances are all better than 0.9996. The contents of five analytes in different batches of YCHTE samples do not indicate significant difference. So, it is concluded that the developed HPLC-UV method is a more fully validated and complete method for evaluating and controlling the quality of YCHTE.     

Simultaneous determination of major bioactive components in Qingkailing injection by high-performance liquid chromatography with evaporative light scattering detection

High-performance liquid chromatography with evaporative light scattering detection (HPLC/ELSD) was established for simultaneous determination of seven major bioactive components of Qingkailing injection including adenosine, geniposide, chlorogenic acid, baicalin, ursodeoxycholic acid, cholic acid, and hyodeoxycholic acid. The proposed method was applied to analyze ten various Qingkailing injections and produced data with acceptable linearity, repeatability, precision and accuracy having a limit of detection (LOD) of 10-50 ng. In comparison with UV detection, HPLC/ELSD permits the determination of non-chromophoric compounds without prior derivatization, and shows good compatibility to the multi-components of complex analytes. The proposed method is a useful alternative for routine analysis in the quality control of traditional Chinese medicine.     

葛根药材指纹图谱分析方法研究

以安徽产葛根药材为分析对象,选择Agilent ZORBAX SB-C18柱(4.6 mm×250 mm,5μm),甲醇-水梯度洗脱,流量为0.9 mL.min-1,检测波长为250 nm,柱温25℃,建立了葛根药材HPLC指纹图谱。结果表明,10批供试品的保留时间在60 min之内,共有18个典型的共有色谱峰。采用HPLC法获得的葛根药材指纹图谱稳定、可靠、重复性好,能较全面地反映葛根药材的内在质量,可用于葛根药材的质量控制。     

Development of a Special Two-Dimensional Fingerprint for the Quality Evaluation of Euonymus Alatu by HPLC with Diode Array Detector Coupled with Chemiluminescence Detection

A special two-dimensional fingerprint developed by a hyphenated method, HPLC–DAD coupled with flow injection analysis and chemiluminescence detection (HPLC–DAD–FIA–CL), was applied to evaluate the quality of Euonymus alatu. Chromatographic fingerprint and active characteristics of Euonymus alatu from different habitats were investigated by HPLC–DAD–FIA–CL method. The similarity of two-dimensional fingerprint obtained by a vectorial angle method was used to evaluate the quality of Euonymus alatu. The results suggested that the two-dimensional fingerprint could reveal more objective conclusions for the quality of Euonymus alatu, and might be helpful to improve the quality control ability of herbal medicines.     

Simple Method for Simultaneous Quantitation and Fingerprint Analysis of Ginkgo biloba Tablets by High Performance Liquid Chromatography-UV-Evaporative Light Scattering Detector

By optimizing the separation and analytical conditions, a reliable, simple and accurate high-performance liquid chromatography(HPLC) method coupled with ultraviolet(UV) and evaporative light scattering detector(ELSD) was developed for the simultaneous determination of lactones and flavonoid, that is, bilobalide, ginkgolide A, ginkgolide B, and rutin, in more than 10 batches of Ginkgo biloba tablets from different pharmaceutical companies. The method could also be applied to fingerprint research, for a more general evaluation of the quality of this preparation. The separation of the components was achieved on a Hanbon C18 column with gradient elution using water and methanol containing 0.1% trifluoroacetic acid(TFA). The column temperature was 30 ℃ and the flow-rate of the mobile phase was 0.6 mL/min. The drift tube temperature of the ELSD was set at 100 ℃, and the nitrogen flow-rate was 2 L/min. Good linear relationships were shown with correlation coefficients for analytes exceeding 0.9913. The limits of detection(LODs, S/N=3) and the limits of quantitation(LOQs, S/N=10) were 0.00887--0.0508 μg/μL and 0.0171-0.0636 μg/μL, respectively, on the column. The relative standard deviations(RSD) of the analytes were less than 3.61% for intraday and 3.70% for interday, respectively. The average recovery rates obtained were in the range of (97.3±4.3)% to (101.9±3.1)% for all the compounds. The results of quantitative and fingerprint analysis proved that the contents of the components were totally similar in the preparation of Ginkgo biloba tablets from the same pharmaceutical company; whereas, they varied significantly in the preparations of Ginkgo biloba tablets from different companies.     

色谱指纹图谱在香精香料质量控制中的应用

烟用香精香料化学成分复杂,现无合适的化学质量控制方法,通过实例,对10个批次正常生产的香料标样进行同时蒸馏萃取,取其萃取液进行气相色谱氢焰检测.进行同组分色谱峰的匹配,根据相对峰面积求出标准指纹图谱,然后10批标样各自与标准指纹图谱进行相似度计算,据此设立待测样品的合格性允差范围.待测样品与标准指纹图谱进行谱峰匹配,计算与标准指纹图谱的相似度,依据合格性允差范围,判定其质量状况.     

Chemical fingerprinting of Shexiang Baoxin Pill and simultaneous determination of its major constituents by HPLC with evaporative light scattering detection and electrospray mass spectrometric detection

High-performance Liquid Chromatography (HPLC) with evaporative light scattered detection (ELSD) and electrospray ionization mass spectrometric detection (ESI-MS) was employed to establish chemical fingerprint of Shexiang Baoxin Pill (SBP) and to simultaneously determinate its seven major constituents, including cholic acid, deoxycholic acid, ursodeoxycholic acid, chenodeoxycholic acid, cinobufagin, recibufogenin, and ginsenoside Rb1. The analysis was performed on a C18 column with water-acetonitrile gradient elution, and the investigated constituents were authenticated by comparing their retention times and mass spectra with those of reference compounds. The proposed method was applied to analyze nine SBP samples and produced data with acceptable linearity, precision, stability and accuracy. Both the chemical fingerprints and quantification data were used to evaluate the quality of various SBP products. The proposed method allows obtaining chemical fingerprint and quantification of multi-components in one run, and therefore can be readily utilized as a comprehensive quality control approach for traditional Chinese medicine.     

指纹图谱法在参麦注射液质控中的应用

 中医药理论和实践要求综合评价中药的质量 ,指纹图谱法是对中药制剂进行综合宏观分析的可行手段之一 ,因此采用反相高效液相建立了参麦注射液的特征指纹图谱。条件 :Hypersil C18(4 6mmi d × 2 5 0mm ,5 μm)反相柱 ,流动相由水 (A)和乙腈 (B)组成 ,B的体积分数在 5 0min内由 5 %线性增长到 95 % ,流速为1 0mL/min ;紫外检测 ,波长为 2 0 2nm。 2 3个特征指纹峰与内标 (联苯 )的峰面积比作为指标 ,结合主成分分析 投影判别法比较了同一厂家不同批次产品和不同厂家同类产品的化学指纹差异。     

High-throughput purification of combinatorial libraries I: a high-throughput purification system using an accelerated retention window approach

We have developed a high-throughput purification system to purify combinatorial libraries at a 50-100-mg scale with a throughput of 250 samples/instrument/day. We applied an accelerated retention window method to shorten the purification time and targeted one fraction per injection to simplify data tracking, lower QC workload, and simplify the postpurification processing. First, we determined the accurate retention time and peak height for all compounds using an eight-channel parallel LC/UV/MS system, and calculated the specific preparative HPLC conditions for individual compounds. The preparative HPLC conditions include the compound-specific gradient segment for individual compounds with a fixed gradient slope and the compound-specific UV or ELSD threshold for triggering a fraction collection device. A unique solvent composition or solvent strength was programmed for each compound in the preparative HPLC in order to elute all compounds at the same target time. Considering the possible deviation of the predicted retention time, a 1-min window around the target time was set to collect peaks above a threshold based on UV or ELSD detection. Dual column preparative instruments were used to maximize throughput. We have purified more than 500 000 druglike compounds using this system in the past 3 years. We report various components of this high-throughput purification system and some of our purification results.