姜黄素键合硅胶固定相HPLC分离水溶性维生素和核苷

以ODS为参比,研究了5种水溶性维生素和5种核苷在姜黄素键合硅胶固定相(CCSP)上的色谱行为,考察了甲醇、流动相pH和离子强度对CCSP分离这类极性化合物的影响,探讨了该新固定相的色谱保留机理。结果表明,在V(甲醇)∶V(0.01 mol/L NaH2PO4)=40∶60(pH 3.5)流动相体系中,5种水溶性维生素在CCSP上实现较好分离;核苷的分离则是在以纯水为流动相的条件下实现的。与ODS柱相比,在相同条件下,CCSP对5种水溶性维生素具有较高的选择性,洗脱顺序与ODS具有显著差异,且保留明显比ODS强(B6除外);与此相反,相同色谱条件下,CCSP对核苷的保留比ODS弱,CCSP可实现核苷的简便有效分离,同时胸苷与黄苷的洗脱顺序也与ODS不同。以上说明不同保留机理的存在,CCSP具有典型的反相色谱特征,但疏水性比ODS弱;极性的配体使CCSP在对溶质的分离分析中除疏水作用外,还存在n-π和π-π作用、氢键作用、偶极-偶极等作用;协同作用的结果使CCSP在水溶性极性化合物的分离分析中显示出优势。     

生物碱在硅胶和键合高效液相色谱柱上的分离

在不同键合程度的ODS柱和硅胶柱上,以甲醇和磷酸盐缓冲液为移动相,研究了色谱分离吲哚生物碱的特性。具体考察了pH对容量因子,甲醇比例和离子强度对保留时间的影响。实验测得吲哚生物碱在三种选定的硅胶和ODS柱上有相似的保留行为,其容量因子都随pH的升高而增加,随甲醇比例和离子强度的增加而下降。在ODS柱上难以分离的一些生物碱在硅胶柱上用含磷酸缓冲液的甲醇为移动相时能得到满意的分离。     

在线免疫亲和净化-液相色谱-串联质谱快速测定中草药及中成药中10种真菌毒素

将复合毒素免疫亲和柱的柱填料填充至不锈钢柱(35 mm×4.6 mm),制成可重复使用的在线免疫亲和净化柱.在线净化过程的上样溶剂为磷酸盐缓冲液(PBS,pH 7.4),清洗溶剂为水,转移溶剂为乙腈-水(1∶1,V/V).采用PBS/甲醇溶液提取样品中真菌毒素,提取液直接进行在线免疫亲和净化-液相色谱-质谱/质谱分析,...     

基于巯基-烯点击反应制备有机-无机杂化硼酸亲和整体柱用于糖蛋白的选择性富集

发展了以巯基-烯点击反应制备有机-无机杂化硼酸亲和整体柱的新方法。首先以四甲氧基硅烷(TMOS)和巯丙基三甲氧基硅烷(MPTMS)作为反应单体,采用溶胶-凝胶反应制备表面含巯基的硅胶整体柱。然后利用巯基-烯(thiol-ene)的点击反应在整体柱上修饰硼酸配基3-丙烯酰胺基苯硼酸(AAPBA),制成AAPBA-硅胶杂化亲和整体柱。对影响硼酸亲和整体柱性能的条件如TMOS与MPTMS的比例、聚乙二醇和甲醇的用量等进行了优化。并采用扫描电镜、红外光谱等分析仪器对整体柱形貌和机械稳定性能进行了表征。研究了AAPBA-硅胶杂化亲和整体柱的分离性能,结果表明,其在中性条件下对含有顺式二醇的生物小分子核苷具有良好的特异亲和能力,并已成功地应用于卵清蛋白、辣根过氧化物酶等糖蛋白的分离。基于巯基-烯反应的制备方法新颖、可靠,可用于制备多种不同类型的硼酸亲和整体柱,具有较大的应用前景。     

免疫亲和色谱-高效液相色谱法测定河水和土壤中克百威、三唑磷和绿磺隆残留量

将河水或土壤样品的丙酮提取液通过串联的分别装有克百威、三唑磷和绿磺隆免疫亲和吸着剂的3支免疫亲和色谱柱(IAC)或同时装有上述3种吸着剂的多抗体IAC,对样品中克百威、三唑磷及绿磺隆3种农药进行分离。采用串联IAC分离时,在样品溶液过柱后,将串联的IAC柱分开,并用不同配比的甲醇-水溶液分别从3支IAC柱上洗脱农药,用ELISA和HPLC分别测得农药的含量。采用多抗体IAC分离时,用甲醇-水溶液洗脱后,用上述两种方法测得洗脱液中3种农药的含量。对2种分离方法作回收和精密度试验,两方法的回收率和重复性基本一致。     

姜黄素键合硅胶固定相高效液相色谱分离取代芳香酸类化合物

研究了13种取代芳香酸类化合物在姜黄素键合硅胶固定相(CCSP)上的色谱行为,考察了甲醇含量、流动相pH值对CCSP分离取代芳香酸类化合物的影响,探讨了该固定相对芳香酸类化合物的色谱保留机理,并应用于实际样品复方水杨酸搽剂的分离分析。结果表明,在不同含量的甲醇-0.02 mol.L-1NaH2PO4(pH=2.5)流动相体系中,三组芳香酸标准混合样和实际样品中四种主要成分在CCSP上实现基线分离。与ODS柱相比,在相同条件下,CCSP对这类酸性化合物具有较高的选择性,且对13种取代芳香酸类化合物的洗脱顺序与ODS具有显著差异,其中5种溶质在CCSP上的保留强于ODS,这说明不同保留机理的存在。研究表明,CCSP具有典型的反相色谱特征,但疏水性较ODS弱;除疏水作用外,n-π和π-π作用、氢键作用、电荷转移作用、偶极-偶极作用对分离也有贡献。CCSP对极性、电离性物质如水杨酸、对硝基苯甲酸、3,4,5-三羟基苯甲酸、邻苯二甲酸和邻溴苯甲酸等具有较强的保留;由于CCSP较弱的疏水性和多种分离机制,邻氯苯甲酸和苯甲酸在CCSP上的保留不会像在ODS上那么强,且分离度明显优于ODS。     

克百威的免疫亲和色谱分析研究

Sepharose CL-4B经碳酰二咪唑(CDI)活化后与纯化的克百威抗体共价偶联,合成了免疫亲和色谱(IAC)固定相,并用其制备了对克百威具有特异性亲和力的IAC柱。对IAC条件进行了优化,选择0.02 mol/L pH 7.2磷酸盐缓冲液(PB)作为吸附与平衡介质,60%（体积分数）甲醇水溶液作为洗脱剂。结果表明:在优化条件下,IAC柱对克百威的动态柱容量达1.58 mg/L。当标样溶液中克百威质量浓度低于 2　μg/L时,经IAC柱富集的效率高于167倍。在河水中按0.1 mg/L水平添加克百威标准品,经IAC柱分离富集,洗脱液采用包被抗体直接竞争酶联免疫吸附分析(ELISA)法检测,5次重复测定的平均回收率为89.8%,相对标准偏差为4.8%。同时采用高效液相色谱(HPLC)法测定洗脱液,与ELISA法测定结果基本一致。     

聚(4-乙烯基苯硼酸-季戊四醇三丙烯酸酯)亲和整体柱的制备与应用

以4-乙烯基苯硼酸为单体,季戊四醇三丙烯酸酯为交联剂,偶氮二异丁腈为引发剂,乙二醇和二甘醇为致孔剂,经原位聚合制备了聚(4-乙烯基苯硼酸-季戊四醇三丙烯酸酯)毛细管整体柱.以单体、交联剂、致孔剂和引发剂的用量为4种因素,最大吸附量、柱效和保留时间为3个考察标准,利用实验设计软件(DOE)优化了其合成条件,验证了正交实验最优结果,得到了整体柱合成的最佳配比为单体7.32 mg,交联剂6 mg,致孔L剂100 μL,引发剂1 mg.在最佳条件下合成整体柱,并进行表征,在微径液相色谱(μHPLC)和加压毛细管电色谱(pCEC)实验中考察了分离特性.结果表明,整体柱固定相表面的硼酸基团在碱性条件下能特异性吸附邻苯二酚、腺苷等含有邻二羟基结构的化合物,具有亲和色谱的特性;同时由于交联剂的性质使其具有反相分离机理,在含有20％有机相的条件下能够将极性不同的苯系物分开.     

一种可控离子比例的两性亲水色谱固定相的制备及性能研究

将不同比例的氨基和巯基的硅烷偶联剂键合到硅胶表面，再利用巯基与乙烯基膦酸之间的点击化学反应将膦酸基团引入到硅胶表面，制备了一种可调节正负离子比例的两性亲水色谱固定相。通过测定固定相中C、H、N、P元素的含量，证明了氨基与膦酸基团已成功键合到固定相的表面，同时通过N元素与P元素的质量分数确定固定相表面氨基与膦酸基团的比例。制备了3种不同电荷比例的氨基膦酸固定相，将其作为亲水模式下的固定相填料填装在150 mm×4.6 mm不锈钢色谱柱中。以一系列经典的极性小分子作为探针，研究了流动相中乙腈含量、缓冲盐pH值及缓冲盐浓度等因素对探针分子在3种色谱柱上的保留的影响，结果表明，分析物在固定相上是多重保留机理。最后通过比较核苷、水溶性维生素、碱性化合物、苯甲酸这几类标准物质在3种色谱柱上的保留行为来对比3种不同电荷比例的固定相的分离选择性与色谱性能。结果表明，对于不同的分析物，3种固定相表现出完全不同的分离选择性和色谱行为。可以根据分析物的特征选取不同电荷比例的固定相，表明此种固定相在极性化合物的分离上具有良好的应用前景。     

取代硼酸与羟乙基胺化合物间的相互作用研究

取代硼酸与顺式二羟基化合物间的可逆的共价相互作用为糖蛋白和糖等重要生物分子的识别和分离提供了独特的亲和作用.为了获得良好的选择性,以β-激动剂与β-阻断剂这两类典型的羟乙基胺化合物为研究对象,利用核磁共振和高效液相色谱研究了它们与苯硼酸间的相互作用.研究结果表明,在高pH值条件下,羟乙基胺化合物与苯硼酸间存在强亲和作用,而在低pH值条件下,该亲和作用变弱甚至消失.这种pH值调控的相互作用表观上与顺式二羟基和苯硼酸间的硼亲和作用很相似.但是,与硼亲和作用机理不同,质子化溶剂的存在能加强这种相互作用,而非质子化溶剂的存在会破坏相互作用.本研究为深入认识硼亲和作用和获得可靠的应用提供了新依据,同时也为利用取代硼酸和羟乙基胺化合物之间的相互作用奠定了基础.     

Synthesis of silica-based benzeneboronic acid affinity materials and application as pre-column in coupled-column high-performance liquid chromatography

Three silica-based benzeneboronic acid affinity materials were synthesized by using an m-aminobenzeneboronic acid as the ligand and using three different spacer arms. Under high-pressure, three affinity pre-columns were packed with these materials and the retention of every affinity pre-column with 11 urinary nucleosides was studied. With different spacer arms of boronic acid-substituted silica materials, the absorption to vicinal alcohols (cis-diols) and stability under acidic elution conditions are of great difference. Coupled-column liquid chromatographic methods for the direct analysis of urinary nucleosides were respectively established. As a result, two of three affinity pre-columns showed good chromatographic property in the on-line analysis of urinary nucleosides. The coupled-column system including pre-column I is the best with excellent linearity (R² > 0.995), good recoveries (85.6–96.9%) and reproducibility (R.S.D.: 1.01–4.02%). The pre-column I could at least endure 150 repetitive injections of a 100 μL urinary sample.     

肠癌患者尿中核苷排放的高效液相法研究

 用反相高效液相法测定尿中核苷。通过苯基硼酸亲和法提取尿中核苷,在柱(4 6mmi d ×250mm,5μm)上以25mmol/L磷酸二氢钾溶液(pH4 55)和60%的甲醇水溶液作为流动相进行二元梯度淋洗,于22℃下进行反相分离,260nm处紫外检测。用该法测定了41例肠癌患者和52例正常人尿中15种核苷的含量(用核苷与肌酐的摩尔比表示,下同),结果表明肠癌患者中有12种核苷的含量比正常人显著性增高(P<0 001)。以15种核苷的含量作为参量,结合主成分分析区分正常人和肠癌患者,对癌症病人的识别率达76%(31/41)。     

手性试剂柱前衍生化高效液相色谱法测定α-苯乙胺的光学纯度

建立了一种简便的手性试剂柱前衍生化反相高效液相色谱测定α-苯乙胺光学纯度的方法。采用2,3,4,6-四-O-β-D-吡喃葡萄糖异氰酸酯(GITC)对α-苯乙胺进行衍生化,优化了衍生化反应参数;使用Agilent Zorbax C18色谱柱分离衍生化产物,流动相为甲醇-磷酸盐缓冲溶液(pH 3.0)(体积比为58:42),流速1.0 mL/min,检测波长241 nm,柱温为30 ℃。实验结果表明,α-苯乙胺两个对映体的衍生化产物分离良好,在0.15～15.0 mg/L范围内呈现良好的线性关系。方法的检出限为0.05 mg/L,定量限为0.15 mg/L,日内和日间精密度考察中测定值的相对标准偏差(RSD)均小于0.5%。建立的方法适用于α-苯乙胺的质量控制。     

高效液相色谱法测定化妆品中的维生素C及其衍生物

建立了化妆品中维生素C及其3种衍生物(抗坏血酸葡糖苷(AA-2G)、抗坏血酸磷酸酯镁(AA-2P)、抗坏血酸乙基醚(Only VCE))的高效液相色谱分析方法。化妆水、水乳液等含油脂较少的样品先采用30 mL 0.02 mol/L磷酸二氢钾溶液(pH 3.0)直接提取,然后定容至50 mL;面膏等含油脂较高及凝胶类、啫喱类的样品先加入1.0 mL二氯甲烷分散均匀后再加25 mL 0.02 mol/L磷酸二氢钾溶液(pH 3.0)提取。提取液在12000 r/min下离心后用0.22 μm滤膜过滤。样品分析采用YMC-Triart C18色谱柱,以0.02 mol/L磷酸二氢钾溶液(pH 3.0)和甲醇溶液为流动相,梯度洗脱,流速为1.0 mL/min,柱温为25 ℃,使用二极管阵列检测器(DAD)检测,检测波长为250 nm,外标法定量。结果显示:4种化合物在其线性范围内线性关系良好,相关系数(r²)均大于0.9999;方法的定量限(以信噪比为10计)为0.04~0.08 g/kg;添加水平为0.25~5.0 g/kg时的回收率为95.6%~101.0%,相对标准偏差为0.62%~3.0%。该方法前处理简单、回收率高、精密度好,适用于化妆品中维生素C及其衍生物的测定。     

高效液相色谱法同时测定化妆品中的10种美白活性成分及2种禁用成分

建立了同时测定化妆品中10种美白活性成分及2种禁用成分的高效液相色谱分析方法。水基、乳液等含油脂较少的样品采用0.02 mol/L磷酸二氢钾溶液(pH 6.0)直接提取;油脂含量高的样品及蜡基、粉基类的样品先加入2.5 m L二氯甲烷溶解后再用0.02 mol/L磷酸二氢钾溶液(pH 6.0)提取。提取液在9 500r/min下离心后用0.22μm滤膜过滤。样品采用Eclipse XDB-C_(18)色谱柱为固定相,以0.02 mol/L磷酸二氢钾溶液(pH 6.0)和甲醇溶液为流动相,梯度洗脱,流速为1.0 m L/min,柱温为25℃,使用二极管阵列检测器(DAD)进行检测,检测波长为230 nm和250 nm,外标法定量。结果显示:12种化合物在2.5~100 mg/L范围内线性关系良好,相关系数(r)均大于0.999 0。方法的定量下限(以信噪比为10计)为0.006 5%~0.025%,添加水平为0.025%~0.5%时回收率为87%~102%,相对标准偏差均小于4%。该方法前处理简单、回收率高、精密度好,适用于化妆品中10种美白活性成分及2种禁用成分的快速测定。     

Analysis of normal and modified nucleosides in urine by capillary electrophoresisa)

Summary Modified nucleosides excreted in urine have been studied as potential diagnostic markers for cancer and AIDS, and as indicators for the whole-body turnover of RNA. Until now, reversed-phase (RP) HPLC and, to some extent, immunoassays are the preferred analytical methods for urinary nucleosides. A new capillary electrophoretic method for the analysis of normal and modified nucleosides in urine has been developed and optimized in our laboratory. The separation of nucleosides extracted from normal human urine on phenyl boronic acid affinity chromatography columns was performed in uncoated 565 mm (500 mm to detection window) × 50 μm i.d. capillary tubing using a 300 mM SDS—25 mM borate—50 mM phosphate buffer (pH 6.7), a 45-s load, a voltage of 7.5 kV (41 μA) and UV detection at 260 and 210 nm. The average recovery of the nucleosides was 91 %. The calibration curves were linear over all physiological and pathophysiological concentration ranges and the limits of detection were at micromolar levels. Reproducibility of migration times were better than 1 % (coefficient of variation,CV), and the reproducibilities of the determined concentrations were better than 5 % for standards and 6–15 % for extracted urine. The developed method was used to quantify 15 normal and modified nucleosides in 25 normal urines to establish reference ranges. The analysis time was less than 45 min. Dedicated to Professor E. Bayer on the occasion of his 70th birthday. Presented at the 21^st ISC held in Stuttgart, Germany, 15^th–20^th September, 1996.     

Determination of vanilmandelic acid in urine by coupled-column liquid chromatography combining affinity to boronate and separation by anion exchange

An automated liquid chromatographic method for assaying vanilmandelic acid in urine is described. Vanilmandelic acid and potential interfering substances, such as catechol compounds and their metabolites, have been tested for affinity to boronic acid-substituted silica at various pH values. Vanilmandelic acid and the internal standard, isovanilmandelic acid, were bound to the boronate matrix at an acidic pH, whereas for instance catecholamines were unretained and passed through the column. The alpha-hydroxycarboxylic acids were then desorbed by another mobile phase (pH 6.0) and transferred to an anion exchanger for chromatography and electrochemical detection. A relative standard deviation of 2.8% was obtained for the analysis of human urine samples containing 6.6 microM vanilmandelic acid.     

Optimization and Validation of an LC Method for the Determination of Cefdinir in Dosage Form and Human Urine

A simple and reliable liquid chromatographic method has been developed and validated for the determination of cefdinir in human urine and capsule samples. A chromatographic separation was achieved on a C₁₈ column using a mobile phase consisting of potassium dihydrogen phosphate (10 mM, pH 4.5)–acetonitrile (90:10, v/v). Quantitation was achieved with UV detection at 285 nm, based on peak area with linear calibration curve at a concentration range of 0.7–39 µg mL^?1. This method was successfully applied for the establishment of an urinary excretion pattern after oral dose.     

Two green chromatographic methods for the quantification of tamsulosin and solifenacin along with four of their impurities

Modern analytical procedures often include impurity profiling to verify the potency, safety, and effectiveness of new formulations. We had to develop techniques based on green analysis since the detrimental influence of solvents and chemicals on the environment has now become a serious concern. Two selective, sensitive, and green liquid chromatography methods were established and fully validated for quantitation of tamsulosin hydrochloride and solifenacin succinate along with four of their official and/or related impurities namely; tamsulosin sulfonic acid, tamsulosin impurity H, solifenacin impurity A and solifenacin impurity C. The first used high-performance thin-layer chromatography with silica gel 60 F254 plates as the stationary phase and an elution system of ethyl acetate:butanol:glacial acetic acid (10.0:0.4:0.1, by volume) and a scanning wavelength of 225.0 nm. The second method depended on HPLC with diode array detection. Chromatographic separation was accomplished on a Zorbax SB C₁₈ (250 × 4.6 mm², 5 μm) column utilizing a mixture of 10.0 mM sodium dihydrogen phosphate (pH 3.0, adjusted by o-phosphoric acid) and methanol, at a flow rate of 0.8 mL/min in a gradient elution mode and then the separated peaks were scanned at a wavelength of 225.0 nm. To assess the greenness profile, three distinct methodologies were applied.     

Simple determination of azasetron in rat plasma by column-switching high-performance liquid chromatography

For the quantification of azasetron in rat plasma samples, a column-switching HPLC method was developed and validated. Following dilution of plasma samples with mobile phase A (17?mM potassium phosphate buffer (pH 3.0)) and simple protein precipitation by addition of perchloric acid (60%), the mixture was directly injected onto the pre-column. After endogenous plasma substances were eluted to waste, the analyte was transferred to the trap column by switching the system. Then, the analyte was back-flushed to the analytical column for separation with mobile phase B (a 22:78 v/v mixture of acetonitrile and 17?mM potassium phosphate buffer (pH 3.0)) and detected at 250?nm using a photodiode array detector. A linear standard curve was obtained in the concentration range of 10-800?ng/mL with the correlation coefficient (r) of 0.9998. The intra- and inter-day precision and accuracy values for azasetron were in the ranges of 0.3-12.9% and 89.7-101.4%, respectively. The method was valid in terms of specificity, precision, and accuracy. In addition, this efficient analytical method was successfully applied to determine plasma concentrations of azasetron following oral administration of azasetron at a dose of 4.0?mg/kg to rats.