On-line HPLC combined with multivariate statistical process control for the monitoring of reactions

On-line high performance liquid chromatography is used to monitor a steady state reaction over 35.2 h, with 197 chromatograms recorded as the reaction progresses. For each chromatogram, peaks are detected, baseline corrected, aligned and integrated to provide a peak table consisting of the intensities of 19 peaks, two corresponding to the reactants, one to the product and one to the solvent, the remaining being impurities, by-products or intermediates. D-charts and Q-charts from multivariate statistical process control are applied to the data to determine which samples are out of control and also provide diagnostic insight into why these samples are problematic. The D-chart is best at looking at overall performance issues such as problems with mixing or difficulties with instrument operation, whereas the Q-charts are best at detecting impurities during the reaction.     

Validated HPLC method for the quantitative determination of CoQ(10) in dog plasma and its application to a pharmacokinetic study

Coenzyme Q₁₀ (CoQ₁₀) is a naturally occurring compound located in all membranes throughout the cell. A rapid and sensitive HPLC method was developed to determine the concentration of CoQ₁₀ in dog plasma using a surrogate matrix. Chromatographic separation was carried out on a Diamonsil C₁₈ column with the UV detector set at 275 nm. Methanol–2‐propanol (40:60, v/v) was used as a mobile phase delivered at a flow rate of 1.0 mL/min. Calibrators were prepared using blank plasma–K₂HPO₄ buffer (50 mm , pH 8.0)–saline (1:3:6, v/v/v) as surrogate matrix. It was shown that the surrogate matrix had similar properties to dog plasma for CoQ₁₀ in extraction, freeze–thaw and stability. The assay was linear over the concentration range of 0.10–100 µg/mL. The intra‐ and inter‐day precisions were within 13.3% in terms of relative standard deviation (RSD%) and the accuracy was within ±7.5% in terms of relative error. This simple and reproducible HPLC method with less plasma volume (0.4 mL) and adequate sensitivity was successfully applied to pharmacokinetic studies of CoQ₁₀ in dogs and an investigation of the effect of CoQ₁₀ formulation on CoQ₁₀ baseline levels. Copyright © 2010 John Wiley & Sons, Ltd.     

HPLC法快速测定食品添加剂的检测条件研究

建立一种HPLC法快速测定食品中苯甲酸、山梨酸和糖精钠的分析方法.采用C18反向高效液相色谱柱,以甲醇和乙酸铵溶液为流动相洗脱,用紫外检测器于230nm波长处检测.当流动相甲醇与乙酸铵的比例(V/V)为39∶61时,各组分均得到较好的分离,色谱峰分离度达到3.0以上,色谱峰型尖锐,保留时间较短.色谱峰面积和保留时间的RSD均小于1%,表明该方法具有很好的准确度和精密度.在该色谱条件下,分别对饮料、调料等实际样品进行检测,结果表明该色谱条件的HPLC法快速、准确,重现性好,可作为食品中防腐剂和甜味剂的定性定量的参考方法.     

HPLC Identification and Separation of Phenolic Compounds Diazotized With Sulphanilic Acid. Structural Effects on Retention Times

Abstract

A HPLC method for the separation of phenol derivatives has been developed either on a RP Phenyl-bonded or an alkyl C₁₈ -bonded columns. Derivatization with diazotized sulphanilic acid allows

a reversed-phase chromatography with spectrophotometric detection at 370 nm. The method sensitivity permits detection down to 0.08- 0.15 ng of phenols. In particular structure-retention time relationships are discussed.     

Determination of picroside II in dog plasma by HPLC and its application in a pharmacokinetics study

A sensitive and simple high-performance liquid chromatography method with UV detection was developed and validated for determining picroside II in dog plasma. Paeoniflorin was employed as internal standard and the sample pre-treatment procedure consists of deproteinization by addition of acetonitrile. Chromatographic separations were performed on a Shimadzu VP-ODS column (250 x 4.6 mm i.d., 5 microm). The mobile phase consisted of acetonitrile-0.1% acetic acid aqueous (v/v), 23:77, v/v, at a rate of 1 mL/min. Detection was carried out at a wavelength of 266 nm. Calibration standards ranged from 0.25 to 500 microg/mL in dog plasma and the mean correlation coefficient of 0.9981 was found for the linear calibration curves (n = 6). The limit of quantification (LOQ) was 0.25 microg/mL. Intra- and inter-assay RSD ranged from 0.70 to 7.5%. Accuracy (%bias) ranged from -6.3 to 6.0%. This method was applied to the pharmacokinetic study of picroside II in dogs. The study demonstrated the plasma picroside II concentration-time curves were fitted to the two-compartment open model and showed linear pharmacokinetics.     

The application of qNMR for the determination of rosuvastatin in tablet form

In this study, quantative nuclear magnetic resonance (qNMR) method was used to determine the content of rosuvastatin in tablet. Linearity, range, limit of detection (LOD), limit of quantification (LOQ), accuracy, and precision were determined in validation study of rosuvastatin. Furthermore, validation study of rosuvastatin was performed with high performance liquid chromatography (HPLC). Uncertainties of qNMR and HPLC methods were determined using per EURACHEM/CITAC Guide CG 4 (3th edition), quantifying uncertainty in analytical measurement. qNMR and HPLC methods were linear in the ranges of 0.10 - 5.00 mg/mL and 0.001 - 0.0995 mg/mL, respectively and these lineraties indicate very good linearity performance with regression coefficients (R2 value) above > 0.99. Moreover, LOD and LOQ values using qNMR method were observed as 0.25 mg/mL and 0.80 mg/mL, respectively. These values using HPLC method were found as 0.00051 µg/mL and 0.001695 µg/mL, respectively. The strengths and weaknesses of qNMR method and HPLC method were determined with spectral emphasis on the role of identical reference standards in qualitive and quantitative analyses. It was found that qNMR method is simple, efficient, reliable, and accurate method. Moreover, qNMR method is an easy, practical, and useful method for the validation and optimization of rosuvastatin in the tablet.     

Simultaneous determination of serum propafenone and its metabolites using high‐performance liquid chromatography

Propafenone, a class Ic antiarrhythmic agent, is metabolized to 5‐hydroxypropafeone (5‐OHP) and N‐depropylpropafenone (NDPP). Simultaneous determination of serum propafenone and its metabolites was performed using HPLC equipped with a conventional octadecylsilyl silica column and ultraviolet detector. The wavelength was set at 250 nm. Propafenone and its metabolites in the serum were extracted using diethyl ether. The mobile phase solution, comprising 1‐pentanesulfonic acid sodium salt (0.1 m ), acetonitrile and acetic acid (280:185:2.5, v/v/v), was pumped at a flow rate of 1 mL/min. The recoveries of propafenone, 5‐OHP and NDPP were greater than 85, 82 and 60%, respectively, with the coefficients of variation (CVs) less than 5.4, 1.9 and 2.9%, respectively. The calibration curves were linear for a concentration range of 12.5–1500 ng/mL for propafenone and 2–500 ng/mL for 5‐OHP and NDPP (r > 0.999). CVs in the intraday assays were 1.0–3.8% for propafenone, 0.6–2.0% for 5‐OHP and 0.6–1.7% for NDPP. CVs in interday assays were 1.3–7.7% for propafenone, 1.1–6.5% for 5‐OHP and 5.4–8.0% for NDPP. The present HPLC method can be used to assess the disposition of propafenone and its metabolites for pharmacokinetic studies and therapeutic drug monitoring of propafenone.     

Batch process monitoring and its application to polymerization systems

Slight changes in raw material properties or operating conditions during critical periods of operation of batch and semi-batch polymerization reactors may have a strong influence on reaction mechanism and impact final product quality. Online process monitoring, fault detection, fault diagnosis, and product quality prediction in real-time ensure safe reactor operation and warn operators about excursions from normal operation that may lead to deterioration in product properties. Multivariate statistical process monitoring and quality prediction using multiway principal components analysis and multiway partial least squares have been successful in detecting abnormalities in process operation and product quality. When abnormal process operation is detected, fault diagnosis tools are used to determine the source cause of the deviation. Illustrative case studies are presented via simulated polyvinyl acetate polymerization.     

An HPLC method for the determination of ethacridine lactate in human urine

An HPLC method was developed and validated for the determination of ethacridine lactate in human urine. Solid-phase extraction cartridges were used to extract urine samples. Separation was carried out on a C(18) column maintained at 30 degrees C with methanol-0.05% sodium dodecylsulfonate (70:30, v/v, pH 3) as mobile phase at a flow rate of 1.0 mL/min. Detection was at UV 272 nm. The calibration curve was linear in the concentration range of 4-4000 ng/mL, with linear correlation coefficient r equal to 0.9998. The limit of detection for the assay was 1.1 ng/mL. The within-day accuracy ranged from 94.8 to 101.6% and precision from 2.3 to 5.4%. The between-day accuracy ranged from 96.8 to 102.6% and precision from 4.0 to 5.3%. The absolute recovery was 95.4-101.2%. Urine samples were stable for at least 15 days if stored in the dark at -20 degrees C. This simple and accurate method allows the sensitive determination of ethacridine lactate in human urine. It was successfully applied to assess the urine level of ethacridine lactate in women received intra-amniotic injection.     

Synthesis of mesoporous silica for adsorption of chlordiazepoxide and its determination by HPLC: Experimental design

In this work, mesoporous silica (SBA‐15‐NH₂) was used as an efficient adsorbent for extraction of chlordiazepoxide from different samples based on dispersive nanomaterial‐ultrasound assisted microextraction followed by high‐performance liquid chromatography. The prepared sorbent was characterized by fourier transform infrared spectroscopy, scanning electron microscopy, low‐angle X‐ray diffraction, thermal analysis, and N₂ adsorption‐desorption surface area measurement. Several variables affecting the extraction efficiency of the chlordiazepoxide, including the amounts of adsorbent, time of adsorption, pH and volume of desorption solvent were optimized by central composite design combined with desirability function. The values of variables were set as 10 mg of SBA‐15‐NH₂, 15 min adsorption time, pH = 7.3 and 1 mL methanol. The linear response (0.998) was obtained in the range of 0.006–10 µgmL^?1 with detection limit 0.0014 µg/mL and extraction recovery was in the range of 91–96% with relative standard deviation < 6%.     

A Practical Interfacing of HPLC with Electron Capture Detection (HPLC-ECD)

Abstract

Conventional HPLC can be simply, conveniently, and inexpensively interfaced to the electron capture detector within any GC. Various parameters have been evaluated to determine the suitability of this approach for the selective trace analysis of aliphatic and aromatic nitro derivatives.     

HPLC测定一次性塑料用品中邻苯二甲酸酯类增塑剂

本文用高压、液体色谱柱Liehmspher C-18(250mm×4.6mmID,5μm),以乙腈-水为流动相,流速为1.0mL/min,线性梯度乙腈从70%到100%,采用质谱检测器对邻苯二甲酸酯进行定性鉴定.邻苯二甲酸二甲脂(DMP)、邻苯二甲酸二乙酯(DEP)、邻苯二甲酸二丁酯(DBP)和邻苯二甲酸二甲酸辛酯(DOP)浓度分别为1.1～89mg/L,0.9～74mg/L,0.9～71mg/L和0.9～68mg/L时线性关系良好,平均回收率分别为83%,89%,86%,87%(n=5).建立了准确度和灵敏度高,方便快捷有效的一次性塑料用品中邻苯二甲酸酯类增塑剂的高效液相色谱定量分析方法.     

Rapid monitoring of high-mannose glycans during cell culture process of therapeutic monoclonal antibodies using lectin affinity chromatography

We developed a simple high-performance liquid chromatography assay to monitor high-mannose glycans in monoclonal antibodies by monitoring terminal alpha-mannose as a surrogate marker. Analysis of glycan data of therapeutic monoclonal antibodies by 2-aminobenzamide assay showed a linear relationship between high mannose and terminal mannose of Fc glycans. Concanavalin A has a strong affinity to alpha-mannose in glycans of typical therapeutic monoclonal antibodies. To show that terminal mannose binds specifically to Concanavalin A column, exoglycosidase-treated monoclonal antibodies were serially blended with untreated monoclonal antibodies. Linear responses of terminal-mannose binding to the column and comparable data trending with high mannose levels by 2-aminobenzamide assay confirmed that terminal-mannose levels measured by the Concanavalin A column can be used as a surrogate for the prediction of high-mannose levels in monoclonal antibodies. The assay offers a simple, fast, and specific capability for the prediction of high-mannose content in samples compared with traditional glycan profiling by 2-aminobenzamide or mass spectrometry-based methods. When the Concanavalin A column was coupled with protein A column for purification of antibodies from cell culture samples in a fully automated two-dimensional analysis, high-mannose data could be relayed to the manufacturing team in less than 30 min, allowing near-real-time monitoring of high-mannose levels in the cell culture process.     

用于寡糖链分析的HPLC柱前衍生化方法研究进展

糖复合物中的糖链具有广泛的生理和病理作用. 在研究糖复合物中糖链的功能时, 需要解析其化学结构, 以便进一步研究结构与功能的关系. 糖链的释放常采用化学法或酶法, 如何纯化释放的糖链对结构解析至关重要, 目前常用的方法是高效液相色谱法(HPLC), 为提高检测的灵敏度, 往往需要对糖链衍生化. 对糖链的HPLC柱前衍生化方法进行综述和评价.     

Capillary electrophoresis as an alternative to HPLC for determination of honey flavonoids

Summary The general objective is to provide an alternative methodology based on capillary electrophoresis (CE) to characterize flavonoids from honey and hence determine its botanical origin. The specific objective is to compare the separation of flavonoids by CE with those achieved by HPLC to assess CE as an alternative technique for the determination of honey flavonoids. Fourteen different flavonoids isolated from honey were analysed by MECC and compared to the HPLC separations. It was difficult to find specific experimental conditions to separate all the flavonoids from honey in a single MEKC run. Three chromatographic conditions are optimized and, depending on the flavonoid markers sought in honey, the appropriate detection method should be chosen. Compared to the HPLC results, it is clear that CE could be an alternative technique in honey flavonoids analysis and particularly in the study of its geographical and floral origin.     

Direct injection HPLC method for the determination of selected phenothiazines in plasma using a Hisep column

A direct plasma injection HPLC method has been developed for the determination of selected phenothiazines (promethazine, promazine, chlorpromazine) using a Hisep column. The method is easy to perform and requires 20 microL of a filtered plasma sample. The chromatographic run time is less than 11 min using a mobile phase of 15:85 v/v acetonitrile-0.18 m ammonium acetate pH 5.0 and UV detection at 254 nm. The method is linear in the concentration range 0.1-25 microg mL(-1) (r > 0.99, n = 6) for each analyte with RSD less than 6%. Interday and intraday variability were found to be < or =14%. The limits of detection and quantitation were 0.1 (S/N > 3) and 0.25 microg mL(-1) (S/N > 10), respectively, for each of the three phenothiazines. We can also apply this method to separate three other phenothiazines (ethopromazine, trifluoroperazine, prochlorperazine), although it lacks the selectivity to determine the concentration of all six drugs concurrently. The separation is feasible using these drugs in certain combinations.     

Optimization of extraction of total trans‐resveratrol from peanut seeds and its determination by HPLC

Resveratrol, a stilbene phytoalexin in plants, is believed to benefit human health. In this study, an optimized enzyme‐assisted method was developed to extract the total content of trans‐resveratrol (free or combined with glucose) in peanut seeds, followed by detection using high‐performance liquid chromatography. The extraction process was optimized by Box–Behnken design and response surface methodology. The optimized enzyme concentration, digestion time, pH, and temperature were 3.02 g/L, 57.06 min, 5.88, and 51.05°C, respectively. Validation tests indicated that the experimental yield of trans‐resveratrol was 0.183 ± 0.007 µg/g with a relative standard deviation of 3.87% (n = 5) under the optimal condition, which was closely agreed with the predicted value (0.182 µg/g). The recoveries obtained from the spiked samples were varied from 89.4 to 103.9%. Therefore, this study will provide a useful method for quantification of total trans‐resveratrol in peanut seeds.     

紫草油有效成分的高效液相色谱测定法及其在超临界流体萃取制备紫草油中的应用

紫草提取制备成的紫草油能够预防及治疗婴儿尿布疹、皮肤溃烂、湿疹等多种皮肤疾患,临床应用非常广泛,超临界流体萃取是紫草有效成分提取的优选方法.该文建立了紫草油有效成分的高效液相色谱(HPLC)测定方法,并以紫草油所含的有效成分含量为评价指标,采用三因素三水平正交试验法对紫草超临界流体萃取制备过程中的几个重要因素(萃取压力...