利用样本成分耗散物的非线性化学指纹图谱原理及相似度计算与评价

在恒温恒压条件下,以丙酮和样本中底物作为主要耗散物的不同成分的样本对非线性化学反应机理产生不同影响,从而引起反应体系电位-时间曲线形状不同变化为特征的B-Z化学振荡体系为例,就非线性化学指纹图谱原理进行了详细研究和讨论,并提出了计算非线性化学指纹图谱系统相似度的通用方法.利用系统相似度和欧氏距离、相关系数及夹角余弦对不同生产批次古汉养生精和18种其他样本的非线性化学指纹图谱的相似度进行了计算与分析.结果表明,相关系数和夹角余弦都不能用来作为评价非线性化指纹图谱相似度的指标.利用欧氏距离公式计算指纹图谱的非参数型相似度时,能正确反映指纹图谱的特征差异,但用其计算参数型相似度时,则有时不能正确反映样本非线性化学指纹图谱特征差异的相对程度.系统相似度能最真实反映样本指纹图谱之间差异程度,是4种相似度计算方法中最好的,可用于非线性化学指纹图谱相似度计算与评价.成功提出了一种经济、简便、易行和有效的鉴别样本真伪与评价其质量的科学方法.     

一种基于小波变换的近红外化学指纹图谱分析方法

提出了一种快速无损的化学指纹图谱分析新方法. 根据小波变换多分辨分析的特点, 对近红外(NIR)光谱进行小波分解, 从中提取被测样品的化学特征信息, 并作数字信息可视化处理, 构建形成可直观识别样品模式特征的NIR指纹图谱. 将该方法用于中药材丹参的质量检测, 检测结果与色谱指纹图谱检测结果相符, 能快速有效地识别丹参质量模式间的差异, 有望发展成为一种快速分析检测天然产物质量的方法.     

中药色谱指纹图谱的小波变换及分形表达方法

提出一种基于小波变换的色谱指纹图谱分形表达方法。该法运用小波变换将色谱谱线分解至不同分辨尺度，然后计算各尺度分量的分形维数，用色谱的小波基分形参量替代色谱指纹图谱的采样值。仿真实验结果表明，色谱小波基分形参量对谱峰保留时间漂移具有较好的抗干扰能力。以当归和川芎两种中药材的品种及道地性鉴别分类问题为实例，比较研究色谱采样值与小波基分形参量，k-近邻法的交叉验证计算结果表明，小波基分形参量的分类效果优于色谱采样值。     

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.     

中药指纹图谱的融合技术

中药指纹图谱作为中药材真伪鉴别及质量控制的有效手段,具有整体、宏观和模糊分析等特点。高效液相色谱是指纹图谱研究的主流方法,在中药质量控制中具有重要地位。针对栀子药材而言,包括3类主要物质：环烯醚萜苷类、有机酸类和色素类。仅采用一个特征波长下的色谱指纹图谱无法对栀子药材进行整体表达和全面评价。为此,     

桑叶HILIC特征指纹图谱研究

应用亲水色谱法(HILIC)建立了桑叶药材的指纹图谱,并对10批桑叶样品进行分析,为桑叶药材的真伪鉴别及质量控制提供了新方法。采用HILIC XBridgeTMAmide色谱柱,以乙腈-水(含0.2%甲酸、20mmol/L甲酸铵、20%甲醇)为流动相,梯度洗脱,流速为0.8 mL/min,柱温为25℃,检测波长为322 nm,进样量为20μL。该方法具有良好的精密度、重现性和稳定性,检测的10批桑叶指纹图谱有17个共有峰,4个特征峰,采用ESI-TOF/MS对4个特征峰进行了指认,结合相似度分析可以用于不同产区桑叶药材的鉴别。桑叶HILIC指纹图谱有望成为桑叶药材真伪鉴别及质量控制的有力工具。     

X衍射指纹图谱及相似度分析用于鉴别野生和栽培天麻

用X射线粉末衍射法建立了野生和栽培天麻及伪品羊角天麻的指纹图谱。通过数字信号处理技术提取天麻样品的特征信息,按2θ进行相似度计算和分析。天麻的XRD指纹图谱呈多峰重叠的弥散性峰,识别图谱的整体轮廓能区分真伪天麻。野生与栽培天麻的差异主要是2θ在5～10°和30～50°间,通过数字信号处理技术提取低频信号,能有效鉴别野生和栽培天麻。相似度的计算结果进一步表明方法的可行性。     

基于牛舌草指纹图谱的多指标成分相对定量与鉴别方法

色谱指纹图谱法在中草药产地鉴别或中成药鉴别中发挥着重要作用,然而色谱峰强度和位置易受目标物提取和分离条件的影响,发展更加准确的指纹图谱具有重要意义。该文以色谱峰中某一个常见组分（芦丁）作为内标,分析其他组分的相对含量,以相对含量作为指纹图谱信息,结合化学模式识别可以精确给出产地的相似度。以牛舌草的液相色谱指纹图谱指纹峰为例,以其中芦丁的组分峰作为基准峰,其他指纹峰以芦丁为参照,计算每个指纹峰以芦丁计的含量,建立了牛舌草的指纹图谱。将获得的相对含量指纹图谱采用系统聚类分析和主成分分析进行化学模式识别研究,实现了不同产地牛舌草的区分。该方法建立了牛舌草多指标成分的相对定量与鉴别方法,既节省资源,又具有可操作性,对于其他中药或中成药的质量控制具有一定的借鉴意义。     

中药指纹图谱技术研究现状

中药指纹图谱特指中药样本经光谱或色谱等现代分析技术得到的中药各组分群体特征的图谱或图象。凭借实用的指纹图谱既可确认中药材或中药制剂的真伪,同时又能判断其质量的稳定与否。本文对中药指纹图谱技术研究领域内的国内外现状及主要技术进行了综述。     

绿茶的色谱指纹谱分类模式初探

以绿茶的数字化色谱指纹谱为基础,探讨用指纹谱来分类绿茶的新模式。各批次绿茶样品间的两两重叠率可作为筛选构建特征指纹谱样品的依据,14个绿茶样品按照特征指纹检出率和总差异率的不同初步划分为3个级别。本法从内在组成上为绿茶的分类提供了一个客观量化的界定标准,有别于过去凭借外形口感的经验评估,可为茶叶乃至自然界其它植物的化学分类提供新的视角。     

Development of Near Infrared Spectroscopy for Rapid Quality Assessment of Red Ginseng

Near infrared spectroscopy(NIRS) was developed as a rapid analysis method for the qualitative and quantitative assessment of the quality of red ginseng. Discriminant analysis(DA) based on principal component analysis and Mahalanobis distance was used to distinguish red ginseng from counterfeits non-destructively. The result shows that the proposed method could distinguish red ginseng from counterfeits correctly and no misclassified sample was found in both training and test sets. The partial least squares(P...     

基于遗传算法的色谱指纹峰配对识别方法

指纹峰配对识别是色谱指纹图谱分析中的关键环节之一，本文提出一种基于遗传算法的色谱指纹峰配对识别方法。该法根据对照色谱指纹图谱的峰分布特性初选出若干标定蜂，将其存入一个候选标定蜂库；同时根据这些候选标定峰从待测指纹图谱中选出相应的候选标定峰，也存入候选标定峰库；再用遗传算法从库中选取一组标定峰用于校正待测指纹图谱中各峰的峰位，并自动识别出与对照色谱指纹图谱相对应的各指纹峰。仿真实验及实际分析实验结果均表明，该法识别指纹峰准确可靠，可用于色谱指纹图谱相似度的快速自动计算。     

化学指纹图谱的相似性测度及其评价方法

提出化学指纹图谱相似性测度概念,并以峰数弹性、峰比例同态性和峰面积同 态性为评价指标,用于多角度评价化学指纹图谱相似性测试优劣,根据这些评价指 标,用计算机仿真方法研究比较了6种相似性测度,结果表明夹角余弦测试用于度 量指纹图谱间谱峰比例的波动较适宜,峰匹配测度可较灵敏地检测小峰个数波动, 而欧氏距离测试则具有较好的综合评价能力。最后,采用实测的参麦注射液色谱分 析谱图。研究考察了上述计算机仿真实验结果,证明仿真结果符合实际情况,这表 明本研究方法可用于评价化学指纹图谱相似性测度。     

Fingerprint Analysis of Euonymus alatus (Thuhb) siebold by LC–DAD and LC–ESI–MS

A liquid chromatography coupled with photodiode array detection and electrospray ionization tandem mass spectrometry method was first developed for a chemical fingerprint analysis of Euonymus alatus (Thuhb) siebold (EAS) and rapid identification of major compounds in the fingerprints. Fingerprint profiles were found to be consistent for the herbs acquired from different locations, but the relative abundance of peaks was varied. Twelve peaks were chosen as the common peaks. Quercetin and rutin were detected by comparing the retention times, MS and UV spectra with the standards. The relative retention time and relative peak area of the 12 peaks in the fingerprint were calculated by setting the quercetin as the reference peak. The experimental data were used for similarity calculation and hierarchical clustering analysis. By comparing the UV and MS spectra data with those of the authentic standards and literature, five main peaks in the fingerprints were identified. Finally, five medicinal portions of the herb (leaf, fruit, stem, pterygium and root) were also analyzed by this method. It was found that there were similar chemical components in different parts of this herb but the contents were very different. The developed fingerprint assay was specific and could be readily utilized for comprehensive evaluation of EAS, as well as to distinguish different medicinal portions.     

Development of the Fingerprints for the Quality Evaluation of Scutellariae Radix by HPLC-DAD and LC-MS-MS

A high-performance liquid chromatography coupled with photodiode array detection and electrospray ionization tandem mass spectrometry (HPLC-DAD-ESI-MS²) method was firstly developed for a chemical fingerprint analysis of Scutellariae Radix and rapid identification of major compounds in the fingerprints. The experimental data for chromatography were used for hierarchical clustering analysis and similarity calculation, and those for UV and MS spectra were applied for identifying characteristic peaks. Twenty samples including S. baicalensis Georgi., S. viscidula Bge. and S. amoena C. H. Wright were classified into three groups. By comparing the UV and MS spectra data with those of the authentic standards and literature, 20 main peaks in the fingerprints were identified for the first time. The developed fingerprint assay was specific and could be readily utilized for comprehensive evaluation of Scutellariae Radix.     

质谱差谱方法及其在中药复方研究中的应用

采用HPLC-ESI-MSn分析得到了复方合煎液中有效部分提取物的指纹图谱数据, 通过比对找出对复方指纹谱有贡献的有效成分峰. 再用质谱差谱方法处理多级质谱数据, 提取不同类型的中性丢失, 实现了对复方有效成分化合物的快速分类鉴定. 用该法研究了复方柴苓汤有效部分黄芩总黄酮和柴胡总皂苷.     

Chemical fingerprint of Ganmaoling granule by double‐wavelength ultra high performance liquid chromatography and ultra high performance liquid chromatography with quadrupole time‐of‐flight mass spectrometry

A method incorporating double‐wavelength ultra high performance liquid chromatography with quadrupole time‐of‐flight mass spectrometry was developed for the investigation of the chemical fingerprint of Ganmaoling granule. The chromatographic separations were performed on an ACQUITY UPLC HSS C₁₈ column (2.1 × 50 mm, 1.8 μm) at 30°C using gradient elution with water/formic acid (1%) and acetonitrile at a flow rate of 0.4 mL/min. A total of 11 chemical constituents of Ganmaoling granule were identified from their molecular weight, UV spectra, tandem mass spectrometry data, and retention behavior by comparing the results with those of the reference standards or literature. And 25 peaks were selected as the common peaks for fingerprint analysis to evaluate the similarities among 25 batches of Ganmaoling granule. The results of principal component analysis and orthogonal projection to latent structures discriminant analysis showed that the important chemical markers that could distinguish the different batches were revealed as 4,5‐di‐O‐caffeoylquinic acid, 3,5‐di‐O‐caffeoylquinic acid, and 4‐O‐caffeoylquinic acid. This is the first report of the ultra high performance liquid chromatography chemical fingerprint and component identification of Ganmaoling granule, which could lay a foundation for further studies of Ganmaoling granule.     

人参种类鉴别的傅里叶变换红外光谱法

用傅里叶变换红外光谱法对白参、高丽参、西洋参、红参、野山参等不同种类的人参进行了鉴别；结果表明，不同种类的人参都具有类同的人参皂苷吸收峰，根据红外指数I值、特定位置的吸收峰峰形以及峰位偏移情况可以很好地鉴别人参的种类；该法简便、实用、可靠。     

基于超高效液相色谱-高分辨质谱的多肽组学技术用于人参不同部位多肽的差异分析

采用基于超高效液相色谱-高分辨质谱的多肽组学技术对人参主根、支根、须根和芦头的多肽谱进行全面分析，旨在评价人参不同形态区域多肽表达的异同。本研究共表征62个数据库中已收录的人参多肽。结果表明，人参不同部位均富含多肽类成分。多肽组学研究发现，人参主根和支根、芦头与须根之间多肽含量具有显著差异，从鉴定到的多肽中共发现25个稳定表达的已知潜在多肽标志物。其中多肽种类及含量在主根与其他部位间差异最显著，为主根与非主根药效差异研究提供了新思路。本研究揭示了人参多肽结构多样性及人参不同部位人参多肽表达的异同，对人参化学特征评价具有重要意义，为人参质量控制和合理应用提供了化学依据。