Chemiluminescence high performance liquid chromatography of corticosteroids using lucigenin as post-column reagent

A chemiluminescence high performance liquid chromatographic method for the determination of corticosteroids and tetrahydrocorticosteroids has been developed. Corticosteroids and their metabolites extracted from urine samples were separated using an ODS column and a mixture of methanol + water + 0.01 M sodium acetate solution (70:30:5) as eluent. The eluent from the column was mixed with the chemiluminescent solution containing lucigenin and Triton X-100 and a 0.28 M KOH solution by pumps and monitored by a chemiluminescence detector. No interference was encountered and the method is both precise and reproducible.     

Analysis of residual trifluoroacetic acid in a phosphate-buffered saline matrix by ion chromatography with suppressed conductivity detection

As part of the formulation of a cell-based pharmaceutical product, cells were harvested from mice and incubated in a cocktail containing cell culture media and high levels of trifluoroacetic acid (TFA). The cells were washed with a phosphate-buffered saline solution to remove residual cell culture media and other reagents before the cells were infused back into the mice from which they originated. Because of the potentially toxic nature of the TFA, the cells were washed multiple times and the final wash was monitored for residual TFA in order to demonstrate the efficient removal of the reagent before the cell product could be reintroduced into the test animal. This report describes the method that was developed incorporating anion-exchange chromatography with suppressed conductivity detection for the analysis of residual TFA (down to 50 ng/ml) in the presence of high concentrations of phosphate and chloride interferences. The ultimate sensitivity of the method was improved by selectively removing halide anions using a silver cartridge before sample analysis. The method proved to be rugged and reproducible enough to be validated and used to monitor residual TFA levels in cell washes in support of an acute toxicological study. Results demonstrating the method’s sensitivity, selectivity, precision and linearity were reported.     

Biovalidation of an SPE-HPLC-UV-fluorescence method for the determination of valsartan and its metabolite valeryl-4-hydroxy-valsartan in human plasma

A simple and fast method for the simultaneous determination of the antihypertensive drug Valsartan and its metabolite in human plasma has been validated. The proposed method deals with SPE, followed by an HPLC separation coupled with fluorimetric and photometric detection. The optimization of the SPE-HPLC method was achieved by an experimental design. The separation was performed on an RP C18 Atlantis 100 mmx3.9 mm column. The mobile phase consisted of a mixture of ACN 0.025% TFA and phosphate buffer (5 mM, pH = 2.5) 0.025% TFA and was delivered in gradient mode at a flow rate of 1.30 mL/min. The eluent was monitored with a fluorescence detector at 234 and 378 nm excitation and emission wavelengths, respectively, and at 254 nm using a photometric detector. The full analytical validation was performed according to the Food and Drug Administration (FDA) 'guidance for industry: bioanalytical method validation' and the recoveries obtained for Valsartan and its metabolite ranged from 94.6 to 108.8%. The validated method was successfully applied to 12 plasma samples obtained from patients under antihypertensive treatment with Valsartan.     

On-line pH modification of carbonate eluents using an electrolytic potassium hydroxide generator for ion chromatography

Classical gradient elution, based on the application of a gradient pump used for mixing two or more prepared eluent components in pre-determined concentrations, was replaced by a chromatography system equipped with an isocratic pump and an electrolytic KOH generator. The isocratic pump delivered a constant concentration eluent composed of pure hydrogencarbonate solution. Carbonate ions, the main component of carbonate/hydrogencarbonate-based eluents, were formed by titration of hydrogencarbonate with KOH formed on-line in the electrolytic KOH generator. By changing the concentration of electrolytically-generated KOH, the eluent composition could be changed from pure hydrogencarbonate to a carbonate/hydrogencarbonate buffer, and finally to a carbonate/hydroxide-based eluent. The described system was tested to achieve pH-based changes of retention behavior of phosphate under constant inflow eluent composition conditions.     

大体积进样-浓缩柱在线富集-离子色谱法测定水中痕量及超痕量溴酸盐

建立了一种测定水中痕量及超痕量溴酸盐的在线富集大体积进样离子色谱法。采用实验室常备的柱容量较高的Dionex IonPac AG23保护柱作为浓缩柱,连接在定量环处富集溴酸盐。淋洗液自动发生装置在线生成高纯度氢氧化钾淋洗液进行梯度洗脱,抑制电导检测。实验结果表明:溴酸盐质量浓度范围在0.05~51.2 μg/L之间时线性关系良好,相关系数r≥0.9995,方法检出限为0.01 μg/L。与常规进样相比,进样量可高达5 mL,浓缩因子约为240倍。本方法成功应用于市售纯净水中溴酸盐的测定,2个加标水平的回收率在90%~100%之间,RSD(n=6)为2.1%~6.4%。该方法无需前处理,操作简单,准确度和精密度良好。通过大体积进样实现高倍富集,适用于痕量及超痕量溴酸盐的分析。     

高效离子交换色谱-电化学检测法测定药物合成中间体中的6-磷酸甘露糖

在制备6-磷酸甘露糖过程中,将6-磷酸甘露糖与磷酸根杂质分开是纯化过程和建立质量标准的重要环节。本文建立了6-磷酸甘露糖和磷酸根的离子色谱分离-电化学检测方法。样品经溶解、过滤后进行色谱分析,以IonPac AG18离子交换柱(50 mm×4 mm)为保护柱,在Ionpac AS18离子交换色谱柱(250 mm×4 mm)上分离,以25 mmol/L氢氧化钾溶液为流动相,等度淋洗,流速1.0 mL/min,安培检测器和电导检测器串联检测,外标法定量。先使用安培检测器检测,在碱性条件下,6-磷酸甘露糖在安培检测器上被选择性检出;后使用电导检测器检测,经ASRS型抑制器抑制背景电导后,6-磷酸甘露糖和磷酸根同时被电导检测器检出,二者分离度良好。采用安培检测器检测时,进样量为25 μL, 6-磷酸甘露糖的线性范围为0.06～10.00 mg/L,相关系数为0.9998,回收率为92.1%～103.1%,相对标准偏差均小于3%,检出限(以信噪比为3计)为0.02 mg/L。该方法灵敏度高,无杂质干扰,前处理简便,可用于原料药合成中间体的检测,结果令人满意。     

稳定同位素稀释离子色谱-三重四极杆质谱法测定血浆和尿液中的氟乙酸

建立了离子色谱-三重四极杆质谱测定血浆和尿液样品中氟乙酸（MFA）的方法。血浆样品经高氯酸超声提取,尿液样品经高氯酸酸化,血浆和尿液提取液在pH 0.5~1.0条件下用叔丁基甲醚（MTBE）萃取,萃取液经氮吹浓缩后溶于0.1%（v/v）氨水溶液。以Ionpac AS 19型阴离子色谱柱为分析柱,在线自动产生的氢氧化钾作为淋洗液进行梯度分离,柱流出液经阴离子抑制器抑制后进入质谱系统。采用电喷雾电离源,在负离子、多离子监测（MRM）模式下检测,¹³C₂-氟乙酸稳定同位素内标法定量。血浆和尿液样品中氟乙酸的平均加标回收率为96.2%~120%,相对标准偏差为1.1%~13.1%（n=6）,方法的检出限（S/N=3）分别为0.03 μg/L和0.1 μg/L。该法简单、灵敏、准确,可用于生物样品中氟乙酸的检测。     

Sampling and identification of natural dyes in historical maps and drawings by liquid chromatography with diode-array detection

A simple and rapid liquid chromatographic with diode-array UV-vis spectrophotometric detection (HPLC-DAD) method for identification of natural dyes has been developed. Chromatographic retention of carminic acid, indigotin, crocetin, gambogic acid, alizarin and purpurin has been studied. The mobile phase consisted of 40 mM SDS-10 mM phosphate buffer solution (pH 2.3)-0.1% TFA (eluent A) and acetonitrile (eluent B) using a programmed gradient (5% B to 95% B). Analyses were carried out on a Phenomenex, Luna 5u NH2 100(a) column (250 mm x 4.60 mm i.d., 5 microm particle) and the operating conditions were: 0.6 ml min(-1) flow rate, 20 microl volume injection and 35 degrees C column temperature. Extracts of samples of natural dyes taken from historical maps belonging to The Royal Chancellery Archives in Granada were successfully analyzed using the proposed method including a new technique for sampling.     

Multivariate optimization of solvent extraction with 1,1,1-trifluoroacetylacetonates for the determination of total and labile Cu and Fe in river surface water by flame atomic absorption spectrometry

A procedure for simultaneous solvent extraction of Cu(II) and Fe(III) from river surface waters as diethyldithiocarbamates (DDC) 1,1,1-trifluoroacetylacetonates into isobutyl methyl ketone (IBMK) has been developed prior to their determination by flame atomic absorption spectrometry. Experimental design approaches were used in order to obtain the best compromise conditions for simultaneous solvent extraction. Variables such as pH, sodium DDC or 1,1,1-trifluoro-2,4-pentanodione (H(TFA)) concentrations, reaction time, IBMK volume and extraction time have been optimized. First, Plackett–Burman designs involving 13 experiments and 2 replicates were used as screening designs to determine which variables were significant. DDC or H(TFA) concentration, as well as pH and IBMK volume were found statistically significant and they were finally optimized by applying a central composite design (15 experiments and 2 replicates). Optimum values for these variables were selected for compromise extraction conditions of Cu(II) and Fe(III) species. An optimum pH of 5.3 was chosen for Cu–H(TFA) and Fe–H(TFA) formation with an optimum H(TFA) concentration of 0.20% (m/v). The optimum IBMK volume for extraction was 8 ml, allowing a pre-concentration factor of 10. A microwave-assisted peroxydisulfate oxidation was used to break down the metal–organic matter complexes in river surface waters in order to assess the total Cu and Fe contents. Applying the experimental design approach, optimum conditions was an irradiation for 5.0 min at a microwave power of 500 W using 0.5 g of ammonium peroxydisulfate. The method was applied to determine total Cu and Fe contents and also labile Cu(II) and Fe(III) contents in several river surface water samples.     

Optimization via experimental design of an SPE-HPLC-UV-fluorescence method for the determination of valsartan and its metabolite in human plasma samples

A chemometric approach was applied for the optimization of the extraction and separation of the antihypertensive drug valsartan and its metabolite valeryl-4-hydroxy-valsartan from human plasma samples. Due to the high number of experimental and response variables to be studied, fractional factorial design (FFD) and central composite design (CCD) were used to optimize the HPLC-UV-fluorescence method. First, the significant variables were chosen with the help of FFD; then, a CCD was run to obtain the optimal values for the significant variables. The measured responses were the corrected areas of the two analytes and the resolution between the chromatographic peaks. Separation of valsartan, its metabolite valeryl-4-hydroxy-valsartan and candesartan M1, used as internal standard, was made using an Atlantis dC18 100 mm x 3.9 mm id, 100 angstroms, 3 microm chromatographic column. The mobile phase was run in gradient elution mode and consisted of ACN with 0.025% TFA and a 5 mM phosphate buffer with 0.025% TFA at pH 2.5. The initial percentage of ACN was 32% with a stepness of 4.5%/min to reach the 50%. A flow rate of 1.30 mL/min was applied throughout the chromatographic run, and the column temperature was kept to 40+/-0.2 degrees C. In the SPE procedure, experimental design was also used in order at achieve a maximum recovery percentage and extracts free from plasma interferences. The extraction procedure for spiked human plasma samples was carried out using C8 cartridges, phosphate buffer (pH 2, 60 mM) as conditioning agent, a washing step with methanol-phosphate buffer (40:60 v/v), a drying step of 8 min, and diethyl ether as eluent. The SPE-HPLC-UV-fluorescence method developed allowed the separation and quantitation of valsartan and its metabolite from human plasma samples with an adequate resolution and a total analysis time of 1 h.     

Simultaneous determination of monofluoroacetate, difluoroacetate and trifluoroacetate in environmental samples by ion chromatography

A method is reported for the sensitive, simultaneous determination of mono- (MFA), di- (DFA), and trifluoroacetates (TFA) by ion chromatography (IC). These species were separated using a Dionex AS17 anion-exchange column employed with a potassium hydroxide gradient (via a Dionex EG40 eluent generator) and suppressed conductivity detection. The fluoroacetates were successfully separated from a range of inorganic and organic species likely to be present in environmental samples, in a total analysis time of 35 min (including re-equilibration of the column). Detection limits for mono-, di- and trifluoroacetate were 21, 38 and 36 microg/l, respectively, determined using a signal-to-noise ratio of 3, and were obtained using a sample injection volume of 50 microl. Precision was less than 0.83% relative standard deviation (RSD) for replicate injections performed over a period of 30 days. The method was applied to the determination of monofluoroacetate in river water samples and also in carrot baits.     

烟草中9种有机酸的梯度离子色谱法测定研究

采用淋洗液自动发生一梯度离子色谱分离,电导检测法分离测定了烟草中的甲酸、乙酸、乳酸、丙酸、丁酸、苹果酸、丙二酸、草酸和柠檬酸,并研究了9种有机酸在阴离子交换色谱中的保留行为.以淋洗液自动发生器生成的KOH为淋洗液,样品经提取、过滤稀释后,在IonPac AS1l-HC阴离子交换色谱柱上分离,抑制电导检测器进行检测,一次...     

离子色谱-串联质谱法检测茶叶中的高氯酸盐

建立了离子色谱-串联质谱检测茶叶中高氯酸盐的分析方法。选用高容量、强亲水性的IonPac AS20阴离子交换柱（2 mm）进行分离,以淋洗液自动发生器在线产生的70 mmol/L氢氧化钾为淋洗液等浓度淋洗,TSQ Quantiva三重四极杆质谱仪作检测器,采用电喷雾电离源负离子（ESI^-）模式、多反应监测（MRM）模式进行分析,内标法定量。结果表明,高氯酸盐在0.02~10.0 μg/L范围内线性关系良好,相关系数（r）为0.9991,定量限为2 μg/kg。运用该方法测定5种茶叶中的高氯酸盐,加标回收率为87.3%~112.2%。该方法具有操作简单、专属性强、灵敏度高等优点,可满足茶叶中高氯酸盐的检测要求。     

Determination of n-acetylmuramoyl-l-alanyl-d-isoglutamine in liposomes by HPLC

A method using reversed-phase high-pressure liquid chromatography (with spectrometric detection at 218nm) is described for the determination in new pharmaceutical preparations (liposomes) of a new immunostimulating agent (N-acetylmuramoyl-l-alanyl-d-isoglutamine). Separation was achieved with a mu-bondapak column and phosphate buffer (pH 2.5)-methanol mixture (93:7 v/v) as eluent, at a flow-rate of 2 ml min . Sodium acetate was used as an internal standard. The detector response at 218 nm was linear in the range 10-170 mug ml . The method is simple and accurate.     

Separation and determination of carbohydrates in drinks by ion chromatography with a self-regenerating suppressor and an evaporative light-scattering detector

Analysis of glucose and other carbohydrates are often performed by use of normal phase HPLC methods with acetonitrile as major eluent coupled with evaporative light-scattering detector (ELSD) or by use of anion-exchange ion chromatography (IC) methods with NaOH as eluent coupled with pulsed amperimetric electrochemical detector. In this work, a novel method for the determination of carbohydrates by IC in conjunction with a self-regenerating suppressor and an ELSD detector was investigated. Three carbohydrates (glucose, fructose, and sucrose) were separated using a KOH eluent generator to avoid the effect of carbon dioxide absorption in the alkaline eluent. Due to the use of the suppressor, non-volatile components were removed and a low salt background (K+ approximately 0.070 microg/mL) can be obtained so the suppressed eluent could directly go into an ELSD detector without obvious interference of inorganic salts. After examining the changes in retention and resolution, an optimized method was established (for IC: using 32 mM KOH as the eluent at a flow rate of 1 mL/min; for ELSD: operated at 95 degrees C, 4.0 bar nitrogen with a gas flow rate of 2.0 L/min) and the linearity, reproducibility, and the limit of detection (LOD) for the three carbohydrates were further evaluated. Regression equations revealed acceptable linearity (correlation coefficients=0.994-0.998) across the working-standard range (100-1000 microg/mL for glucose and sucrose, 150-1000 microg/mL for fructose) and LODs of glucose, fructose, and sucrose were 93, 126, and 90 microg/mL, respectively. This method has successfully been applied to the determination of the three carbohydrates in carbonated cola drinks and fruit juices. The recoveries were between 95 and 113% (n=3) for different carbohydrates.     

MultiSimplex and experimental design as chemometric tools to optimize a SPE-HPLC-UV method for the determination of eprosartan in human plasma samples

A chemometric approach was applied for the optimization of the extraction and separation of the antihypertensive drug eprosartan from human plasma samples. MultiSimplex program was used to optimize the HPLC-UV method due to the number of experimental and response variables to be studied. The measured responses were the corrected area, the separation of eprosartan chromatographic peak from plasma interferences peaks and the retention time of the analyte.The use of an Atlantis dC18, 100 mm × 3.9 mm i.d. chromatographic column with a 0.026% trifluoroacetic acid (TFA) in the organic phase and 0.031% TFA in the aqueous phase, an initial composition of 80% aqueous phase in the mobile phase, a stepness of acetonitrile of 3% during the gradient elution mode with a flow rate of 1.25 mL/min and a column temperature of 35 ± 0.2 °C allowed the separation of eprosartan and irbesartan used as internal standard from plasma endogenous compounds. In the solid phase extraction procedure, experimental design was used in order to achieve a maximum recovery percentage. Firstly, the significant variables were chosen by way of fractional factorial design; then, a central composite design was run to obtain the more adequate values of the significant variables. Thus, the extraction procedure for spiked human plasma samples was carried out using C8 cartridges, phosphate buffer pH 2 as conditioning agent, a drying step of 10 min, a washing step with methanol-phosphate buffer (20:80, v/v) and methanol as eluent liquid. The SPE-HPLC-UV developed method allowed the separation and quantitation of eprosartan from human plasma samples with an adequate resolution and a total analysis time of 1 h.     

高效液相色谱法测定强化奶及食品中维生素D含量

介绍用反相高效液相色谱法（ＨＰＬＣ）测定食品中ＶＤ含量,样品经皂化、正己烷提取、正相ＨＰＬＣ净化,用反相ＨＰＬＣ定量分析。回收率为９４．８８％～９９．７０％,批内和批间ＣＶ分别为１．６２％和２．１２％。分析了奶粉、要素膳、肉松、儿保饮料等８种食品中ＶＤ含量,亦可用于各种食品中ＶＤ分析。     

Ion chromatography tandem mass spectrometry for simultaneous confirmation and determination of indandione rodenticides in serum

This paper describes a simple method for the simultaneous determination and confirmation of the indandione rodenticides in serum. After samples were extracted with 10% (v/v) methanol in acetonitrile and cleaned by solid‐phase extraction, chromatographic separation was performed on an IonPac® AS11 analytical column (250 × 4.0 mm) using gradient KOH eluent with 10% (v/v) methanol as organic modifier. Confirmation was depended on the extensive fragmentation of the indandione molecule under MS/MS conditions which provides sufficient structural information. Quantification was performed by negative electrospray ionization in multiple reaction monitoring mode. All the method parameters were validated. It was confirmed that this method could be used in clinical diagnosis and forensic toxicology. Copyright © 2009 John Wiley & Sons, Ltd.     

离子色谱-串联质谱法检测酒类产品中10种有机酸

建立了一种离子色谱-串联质谱(IC-MS/MS)测定白酒、黄酒、干红葡萄酒3种酒类样品中10种有机酸含量的方法。白酒样品氮吹后,经去离子水稀释,用IC-MS/MS分析检测;干红葡萄酒样品和黄酒样品,对比不同固相萃取小柱净化能力,最终选择石墨化炭黑固相萃取小柱进行净化,经去离子水稀释,用IC-MS/MS分析检测。选用高容量、强亲水性的Dionex IonPac^TM AS11-HC型阴离子分析柱进行分离,以淋洗液自动发生器在线产生的KOH水溶液为淋洗液,进行梯度淋洗。淋洗液经抑制器抑制后直接进入电喷雾电离串联质谱(ESI-MS/MS),采用负离子模式电离,多反应监测(MRM)模式检测,外标法定量。在该实验条件下:草酸、富马酸、马来酸、苹果酸、酒石酸、柠檬酸、奎尼酸和乌头酸在0.05~2 mg/L范围内线性关系良好;琥珀酸在0.05~5 mg/L范围内线性关系良好;乳酸在0.05~10 mg/L范围内线性关系良好(相关系数r²>0.99)。10种有机酸的检出限(S/N=3)在1.0~8.0 μg/L范围内,定量限(S/N=10)在3.5~26.5 μg/L范围内,在3个不同浓度的添加水平下,平均回收率在83.0%~112.1%之间,相对标准偏差≤9.1%,满足检测要求。该方法前处理简单,不使用有机溶剂,不需进行衍生化处理,测定快速、准确,灵敏度高,适用于3种酒类样品中10种有机酸的定量分析,为酒类食品的风味及品质测定提供方法支持。     

高温热水解-离子色谱法测定铬矿中氟含量

建立了一种快速、准确的离子色谱法测定铬矿中氟含量的方法,将铬矿与石英砂混合,控制氧气和水蒸气的流量,于1 100℃高温下热水解30min,水解液经吸收后,选用Dionex AS11-HC阴离子分析柱,以KOH(20mmol/L)作淋洗液,自动再生抑制型电导检测器检测,离子色谱法测定铬矿中氟的含量。方法的检出限为0.022μg/mL,定量限为0.073μg/mL,方法的检测范围为0.0015%~0.20%,加标回收率在92%~101%。应用于实际样品的测定结果表明,铬矿中氟含量的测定值与标准方法的测定值一致。方法简单快速、检出限低、精密度高、准确度好。能满足铬矿中氟含量的快速准确检测要求。