On-line extraction coupled with liquid chromatography tandem mass spectrometry for quantitation of pravastatin and its metabolite in human serum

A high-throughput bioanalytical method for simultaneous quantitation of pravastatin and its metabolite (M1) in human serum was developed and validated using on-line extraction following liquid chromatography tandem mass spectrometry (LC-MS/MS). The on-line extraction was accomplished by the direct injection of a 50 microL serum sample, mixed 4:1 with an aqueous internal standard solution, into one of the extraction columns with aqueous 1 mm formic acid at flow rate of 3 mL/min. The separation and analysis were achieved by back-eluting the analytes from the extraction column and the analytical column to the mass spectrometer with an isocratic mobile phase consisting of 62% aqueous 1 mm formic acid and 38% acetonitrile at a flow rate of 0.8 mL/min. The second extraction column was being equilibrated while the first column was being used for analysis, and vice versa. The standard curve range was 0.500-100 ng/mL for pravastatin and M1. The lower limit of quantitation, 0.500 ng/mL for all the analytes, was achieved when 50 microL of human serum was used. The intra- and inter-day precisions were within 7.4%, and the accuracy was between 95 and 103%. The on-line extraction was finished in 0.5 min and total analysis time was 2.5 min per sample.     

Preconcentration of 2,4-dichlorophenoxyacetic acid on molecularly imprinted polymers and its subsequent determination by high performance liquid chromatography

The potency of molecularly imprinted polymers (MIP) for 2,4-dichlorophenoxyacetic acid (2,4-D) in the dynamic sorption preconcentration (solid phase extraction) of 2,4-D and three other structurally related species (2,4-dichlorophenol, 2-chlorophenol, and dikamba) from aqueous solutions is assessed. The optimal conditions for preconcentration are found: 0.01 M HCl, 25–100 mL of solution, flow rate of solution 0.7 mL/min, column (15 × 2.7 mL), and sorbent weight 0.04 g. The analytes are desorbed with 1 mL of methanol and detected in the eluate by reversed-phase HPLC with spectrophotometric detection at 225 nm. The detection limit for 2,4-D makes 0.4 μg/mL without preconcentration and 0.01 μg/mL with preconcentration from a volume of 100 mL. The procedure is applied to the analysis of model mixtures based on fresh river water.     

Separation and determination of 2,4-D, dicamba and 2,4,5-T in tobacco by nonaqueous capillary electrophoresis

A practical method for residue analysis of 2,4-D, dicamba and 2,4,5-T in baked tobacco leaves has been developed using nonaqueous CE (NACE). The herbicide residues of 2,4-D, dicamba and 2,4,5-T in tobaccos were extracted by ultrasonication with ethyl acetate, followed by a cleanup procedure with gel permeation chromatography. The separation of 2,4-D, dicamba and 2,4,5-T by NACE was optimized based on orthogonal experiment design with four factors at three levels. The optimal NACE condition was established with the running buffer of 40.0 mmol/L ammonium acetate in 90% CH3CN (apparent pH 10.2), and the applied voltage of -25 kV over a capillary of 50 microm id x 46 cm (37.5 cm to the detector window), which gave a baseline separation of 2,4-D, dicamba and 2,4,5-T within 15 min. The LOD were ca. 0.4-0.6 microg/mL for the three herbicides, whereas the overall recovery ranged from 80.8 to 84.1%. The proposed method has been successfully applied to measure 300 real tobacco samples, and the residue profiles of the three herbicides in tobacco samples were obtained and evaluated.     

Hybrid organic-inorganic octyl monolithic column for in-tube solid-phase microextraction coupled to capillary high-performance liquid chromatography

An octyl-functionalized hybrid silica monolithic column was developed for in-tube solid-phase microextraction (SPME) to perform on-line preconcentration coupled to capillary high-performance liquid chromatography (microHPLC) analysis. A hybrid silica monolithic column functionalized with octyl groups was conveniently synthesized by a two-step acid/base-catalyzed hydrolysis/co-condensation of tetraethoxysilane (TEOS) and n-octyltriethoxysilane (C8-TEOS). The size of through-pores as well as the carbon content can be adjusted by changing the ratio of TEOS to C8-TEOS in the polymerization mixture. The extraction characteristics of the monolithic column prepared under optimized fabrication conditions were studied by using polycyclic aromatic hydrocarbons (PAHs) as the analytes. The sample volume that could be injected into the system was increased up to 1mL with simultaneous increase of column efficiency, when hybrid silica monolithic column was used as a precolumn. Good linear calibration curves (R>0.999) were obtained, and the limits of detection (signal-to-noise ratio, S/N=3) for the analytes were found to be between 2.4 and 8.1ng/mL with a UV absorbance detector, which are 299-456 times lower than those obtained without preconcentration. The column-to-column RSD values were 1.3-8.0% for recoveries of PAHs investigated.     

整体柱在线固相微萃取-高效液相色谱同步富集检测水中的苯氧羧酸类除草剂

采用C18毛细管整体柱作为固相微萃取整体柱,构建在线固相微萃取-高效液相色谱联用系统,同步富集检测环境水样中的5种苯氧羧酸类除草剂。详细考察了联用系统运行条件对富集检测的影响。联用系统运行最佳参数为:固相微萃取整体柱长度20 cm,进样流速0.04 mL/min,进样13 min,洗脱流速0.02 mL/min,洗脱5 min。在最佳条件下,5种苯氧羧酸类除草剂的检出限为:9 μg/L (苯氧丙酸)、4 μg/L (2-(2-氯)-苯氧丙酸)、4 μg/L (2-(3-氯)-苯氧丙酸)、5 μg/L (2,4-二氯苯氧乙酸)、5 μg/L (2-(2,4-二氯苯氧基)丙酸)。与HPLC系统直接进样对比,联用系统对5种检测对象表现出优良的富集能力。5种苯氧羧酸类除草剂的回收率在79.0%~98.0%之间(RSD≤3.9%)。该方法成功应用于水样中5种苯氧羧酸类除草剂的检测,结果令人满意。     

Application of NaClO-treated multiwalled carbon nanotubes as solid phase extraction sorbents for preconcentration of trace 2,4-dichlorophenoxyacetic acid in aqueous samples

Multiwalled carbon nanotubes functionalized by oxidation of original multiwalled carbon nanotubes with NaClO were prepared and their application as solid phase extraction sorbent for 2,4-dichlorophenoxyacetic acid (2,4-D) was investigated systemically, and a new method was developed for the determination of trace 2,4-D in water samples based on extraction and preconcentration of 2,4-D with solid phase extraction columns packed with NaClO-treated multiwalled carbon nanotubes prior to its determination by HPLC. The optimum experimental parameters for preconcentration of 2,4-D, including the column activating conditions, the amount of the sorbent, pH of the sample, elution composition, and elution volume, were investigated. The results indicated 2,4-D could be quantitatively retained by 100 mg NaClO-treated multiwalled carbon nanotubes at pH 5, and then eluted completely with 10 mL 3:1 (v/v) methanol-ammonium acetate solution (0.3 mol/L). The detection limit of this method for 2,4-D was 0.15 μg/L, and the relative standard deviation was 2.3% for fortified tap water samples and 2.5% for fortified riverine water sample at the 10 μg/L level. The method was validated using fortified tap water and riverine water samples with known amount of 2,4-D at the 0.4, 10, and 30 μg/L levels, respectively.     

On-line solid-phase extraction with a monolithic weak cation-exchange column and simultaneous screening of alpha1-adrenergic receptor antagonists in human plasma

An on-line SPE-HPLC method, using a monolithic poly(glycidyl methacrylate-co-ethylene glycol dimethacrylate) (poly(GMA-EDMA)) based weak cation-exchange (WCX) column, was developed for simultaneous determination of alpha1-adrenergic receptor antagonists in human plasma. The monolithic WCX column was prepared by an in-situ polymerization protocol and modified stepwise with ethylenediamine and chloroacetic acid. On connecting this column to an injection valve, an on-line SPE protocol could be established for removal of matrices (mainly proteins and lipids) and preconcentration of four alpha1-adrenergic receptor antagonists in human plasma. This method was validated and then used for determination of terazosin, alfuzosin, prazosin, and doxazosin in clinical plasma samples. For all analytes, each calibration curve was found to be linear over a range of 0.005-5 microg/mL (R>0.997), and the limit of detection for each analyte was 0.5 ng/mL. Recovery (>80%) and precision (RSD<15%) for inter- and intra-day assay were tested at three concentration levels of each analyte and showed acceptable results for quantitative assay. Real samples from hypertensive patients were monitored and results were in agreement with those of the conventional liquid-liquid extraction-HPLC method. Furthermore, due to its good permeability and biocompatibility, the monolithic WCX sorbent could be reused more than 300 times. The proposed method was especially appropriate for multi-analyte monitoring in plasma samples.     

Capillary scale monolithic trap column for desalting and preconcentration of peptides and proteins in one- and two-dimensional separations

Monolithic columns based on poly-(styrene-divinylbenzene) (PS-DVB) were utilized both for preconcentration (in 10 mm x 0.20 mm I.D. format) and analytical separation (in 60 mm x 0.20 and 0.10 mm I.D. format) of peptides and proteins in column switching micro-scale high-performance liquid chromatography. A special holder for short monolithic preconcentration columns was designed and pressure durability tests approved long-term stability up to 400 bar. An 11-20% decrease in the average peak widths of nine peptides was obtained upon combining a preconcentration column with an analytical column as compared with a setup using an analytical column only. Trapping efficiency, especially for small and hydrophilic peptides, was optimized by using 0.10% heptafluorobutyric acid instead of 0.050% trifluoroacetic acid as solvent additive during sample loading. Using a 10 mm x 0.20 mm I.D. preconcentration column, loadabilities between 0.5 and 1.6 microg were determined by frontal analysis of proteins and bioactive peptides, respectively. A 100-fold concentration followed by direct on-line intact mass determination is demonstrated for diluted (3 micromolL(-1)) protein solutions. The applicability of the monolithic preconcentration column for multidimensional chromatography was tested by off-line two-dimensional separation, combining strong cation-exchange chromatography and ion-pair reversed-phase chromatography. Peptide identification data from digested protein mixtures demonstrated reproducibilities of 46-75% in triplicate analyses, and confident peptide identifications of low abundant peptides even in the presence of a 650-fold molar excess of high abundant peptides.     

The evaluation of different sorbents for the preconcentration of phenoxyacetic acid herbicides and their metabolites from soils

A procedure using alkaline extraction, solid-phase extraction (SPE) and HPLC is developed to analyze the polar herbicides 2,4-dichlorophenoxyacetic acid (2,4-D) and 4-chloro-2-methylphenoxyacetic acid (MCPA) together with their main metabolites in soils. An ion-pairing HPLC method is used for the determination as it permits the baseline separation of these highly polar herbicides and their main metabolites. The use of a highly cross-linked polystyrene-divinylbenzene sorbent (PS-DVB) gives the best results for the analysis of these compounds. This sorbent allows the direct preconcentration of the analytes at the high pH values obtained after quantitative alkaline extraction of the herbicides from soil samples. Different parameters are evaluated for the SPE preconcentration step. The high polarity of the main analytes of interest (2,4-D and MCPA) makes it necessary to work at low flow rates (< or =0.5 mL min(-1)) in order for these compounds to be retained by the PS-DVB sorbent. A two stage desorption from the SPE sorbent is required to obtain the analytes in solvents that are appropriate for HPLC determination. A first desorption with a 50:50 methanol:water mixture elutes the most polar analytes (2,4-D, MCPA and 2CP). The second elution step with methanol permits the analysis of the other phenol derivatives. The humic and fulvic substances present in the soil are not efficiently retained by PS-DVB sorbents at alkaline pH's and so do not interfere in the analysis. This method has been successfully applied in the analysis of soil samples from a golf course treated with a commercial product containing esters of 2,4-D and MCPA as the active components.     

Solid phase extraction using a sulfoxide adsorbent for preconcentration and separation of Hg(II) in natural water followed by ICP-MS measurements

A separation and preconcentration method based on solid-phase extraction using sulfoxide adsorbent was developed for the determination of Hg(II) in natural water samples by inductively coupled plasma mass spectrometry (ICP-MS). The sulfoxide adsorbent was packed into a commercially available syringe-driven column (with a bed volume of 1.0 mL), which permitted off-line sample loading and on-line elution/measurement. The optimized operating conditions were as follows: sample condition for Hg(II) adsorption, 0.5% HCl; sample-loading flow rate, 10 mL min(-1); eluent for recovering Hg(II), 1% cysteine water solution. A test using multi-element mixed solution showed that most trace elements in natural water, except for Bi, could be completely separated from Hg(II). The recoveries of Hg(II) were 99.0 ± 3.2 and 100.7 ± 4.3%, respectively, when 0.64 and 0.16 ng mL(-1) of Hg(II) were added into the test sample. The detection limit of Hg(II) using a quadrupole ICP-MS after 10-fold preconcentration was 1.5 pg mL(-1). The blank value was 2.8 ± 0.5 pg mL(-1).     

在线固相萃取-离子色谱法测定4种芳环磺酸盐中的硫酸根离子

建立一种在线固相萃取-离子色谱测定4种芳环磺酸盐中硫酸根离子含量的新方法。将自装填的多孔石墨化碳固相萃取柱应用于离子色谱系统,对样品进行在线前处理。样品经过多孔石墨化碳固相萃取柱基体消除后进入收集环,通过阀切换方式使待测硫酸根离子转入阴离子分析柱和检测系统。固相萃取流路用1.5 mmol/L碳酸钠以0.8 mL/min的流速对基体在线富集,进样量为20μL,分析柱为SH-AC-3(250 mm×4.0 mm)+SH-AG-3(50 mm×4.0 mm)色谱柱,柱温为35℃,在6 mmol/L碳酸钠-4 mmol/L碳酸氢钠条件下等度洗脱,流速为0.8 mL/min。结果表明:硫酸根离子在0.50~20.00 mg/L范围内呈良好的线性关系,线性相关系数为0.998 3,保留时间、峰高和峰面积的相对标准偏差均在0.28%~2.86%之间,方法检出限为0.010 6 mg/L,回收率为91.01%~109.3%,具有良好的线性关系和重复性。整个在线分析过程在25 min之内完成。该方法进样量少、快速、高效。     

Poly (methacrylic acid-ethylene glycol dimethacrylate) monolithic capillary for in-tube solid phase microextraction coupled to high performance liquid chromatography and its application to determination of basic drugs in human serum

A poly (methacrylic acid-ethylene glycol dimethacrylate) monolithic capillary column was prepared for in-tube solid-phase microextraction. Comparing with the commonly used open tubular extraction capillary, which cannot provide sufficient extraction efficiency since the ratio of its coating volume to that of the capillary void volume is relatively small, the monolithic column with greater phase ratio combined with convective mass transfer provides the possibility to improve the extraction efficiency with shorter capillary. As to poly (methacrylic acid-ethylene glycol dimethacrylate), its hydrophobic main chains and acidic pendant groups make it a superior material for extraction of basic analytes from aqueous matrix.An on-line monolithic capillary column solid phase microextraction (SPME) method was developed for determination of theobromine, theophylline and caffeine in serum samples. The high extraction efficiency was obtained for all the three analytes, yielding the detection limits of 12, 8 and 6.5 ng/mL by UV detection, respectively. Excellent method reproducibility (R.S.D. < 2.9%) was found over a linear dynamic range of 0.05-2 μg/mL in serum sample. The monolithic capillary column was proved to be reusable in coping with serum samples, which would facilitate practical determination of basic drugs.     

Combining restricted access material (RAM) and turbulent flow for the rapid on-line extraction of the cyclooxygenase-2 inhibitor rofecoxib in plasma samples

Restricted access material (RAM) has been used in the packing of a solid-phase extraction (SPE) column for on-line extractions under turbulent flow conditions. The bio-compatible RAM material works by the principle of size exclusion in addition to conventional reversed-phase chromatography, thereby allowing the extraction and preconcentration of small analyte molecules from biological samples such as plasma. Using small column dimensions (0.76 mm x 50 mm) and a consequently high linear velocity, turbulent flow was achieved during online sample extractions. The improved mass-transfer rate characteristic of turbulent flow allows fast sample cleanup without decreased extraction efficiency. The novel use of the RAM column, connected upstream to a C18 monolithic column, allowed the direct injection, extraction, separation, and MS/MS detection of plasma samples spiked with rofecoxib in a span of 5 min. Calibration curves obtained using this RAM turbulent flow coupled column method showed good linearity (R2 > 0.99) and reproducibility (%RSD < or = 7%). The lower limit of quantitation of rofecoxib in plasma samples was found to be 40 ng/ml. The extraction method showed good recovery of rofecoxib from a plasma matrix with minimal signal loss and robustness after more than 200 plasma injections.     

固相萃取-离子色谱法测定饮用水中的痕量卤代乙酸

建立了固相萃取-离子色谱(SPE-IC)测定饮用水中痕量卤代乙酸(HAAs)(包括一氯乙酸、二氯乙酸、三氯乙酸、一溴乙酸和二溴乙酸)的方法。固相萃取采用LiChrolut EN SPE柱来进行痕量待测物的预浓缩（25倍）和基体杂质的消除,用NaOH(10 mmol/L)洗脱;色谱分离采用亲水性、高容量、氢氧化物选择型阴离子交换柱Dionex IonPac AS16(250 mm×4 mm i.d.),以NaOH为流动相进行浓度梯度淋洗,淋洗速度为0.8 mL/min,电导检测,进样量为500 μL。结果表明,用SPE-IC法测定HAAs,一溴乙酸的检测限为12.5 μg/L,其余4种HAAs的检测限为0.38~1.69　μg/L。该法可实现对饮用水中痕量卤代乙酸的测定。     

直接衍生离子液体富集高效液相色谱分析水基胶中脂肪族醛酮

建立了以2,4-二硝基苯肼(DNPH)直接衍生,1-丁基-3-甲基咪唑六氟磷酸盐(［BMIM］PF6)萃取富集,高效液相色谱(HPLC)分析水基胶中痕量脂肪族醛酮的方法。分散的水基胶乳液用80 mg/L DNPH衍生化试剂(含0.44 mol/L磷酸)于40 ℃衍生18 min。取离心后的上层衍生液,加入0.5 mL ［BMIM］PF6于30 ℃萃取富集,离子液体相过滤后进行HPLC分析。采用Dionex Acclaim Explosives E2色谱柱(250 mm×4.6 mm, 5 μm),以水-乙腈为流动相在流速1.2 mL/min进行梯度洗脱,色谱柱温度为35 ℃,检测波长为365 nm。结果表明,8种脂肪族醛酮的检出限为0.022～0.221 mg/kg,定量限为0.073～0.738 mg/kg,相对标准偏差为3.5%～7.3%,回收率为84.0%～102.5%。与溶剂萃取法相比,该法具有检出限和定量限低、稳定性高、测定更准确的优势。     

On-line preconcentration of pharmaceutical residues from large volume water samples using short reversed-phase monolithic cartridges coupled to LC-UV-ESI-MS

A simplified preconcentration method for a range of ultra-trace level pharmaceuticals in natural waters has been developed. Solid phase extraction was performed on-line using a micro-reversed-phase monolithic silica column, allowing for very rapid trace enrichment from large volume (500 ml) samples with minimal sample handling. Acceptable recoveries of >70% were obtained for the majority of compounds investigated and the monolithic columns could be washed and conditioned on-line with no sample carryover and used reproducibly for up to eight extractions each. The on-line SPE-LC-UV method was coupled to electrospray ionisation ion trap mass spectrometry (ESI-MS) to increase both selectivity and specificity. Detection limits were determined in spiked river and tap water samples and found to lie in the low ng/l region using sample volumes of 500 ml, loaded at a flow rate of 10 ml/min, and therefore, were suitable for ultra trace analysis.     

基于分子络合的分散液液微萃取与高效液相色谱联用检测环境水样中2种苯氧羧酸类除草剂

建立了基于分子络合的分散液液微萃取（DLLME）方法,以磷酸三丁酯为萃取剂,以甲醇为分散剂,与高效液相色谱联用检测了环境水样中麦草畏和2,4-二氯苯氧乙酸（2,4-D酸）2种苯氧羧酸类除草剂,对影响前处理效果的因素（包括水样的pH值、萃取剂的种类和体积、分散剂的种类和体积、反萃液的pH值、反萃液的体积和盐浓度等）进行了详细考察,在最佳萃取条件下（水样体积10 mL,水样的pH值为0~1.0、100 μL磷酸三丁酯萃取剂、1000 μL甲醇分散剂、0.01 mol/L的氢氧化钾反萃液的体积为80 μL）,2种苯氧羧酸类除草剂在0.50~1000 μg/L范围内具有良好的线性,相关系数不小于0.9985,麦草畏和2,4-D酸的检出限分别为0.44 μg/L和0.49 μg/L,富集倍数分别为85和90,在实际样品中的加标回收率为75.7%~104.0%。该方法基于分子络合反应机理,将新型萃取剂磷酸三丁酯应用于分散液液微萃取,与HPLC联用实现了麦草畏和2,4-D酸的富集与检测,为环境水样中苯氧羧酸类除草剂的检测提供了新的前处理方法。     

整体柱高效液相色谱法测定草甘膦原药中甲醛含量

建立了衍生化-高效液相色谱法对草甘膦原药中痕量甲醛含量进行测定的方法。样品中残留甲醛经超声波水浴提取，与2，4-二硝基苯肼衍生反应，生成的2，4-二硝基苯腙用反相整体柱色谱进行快速分离，在360nm紫外波长下检测，外标法定量。该分析方法在2．0～200mg/L浓度范围呈良好线性，添加回收率在88％～105％之间，相对标准偏差小于5％。样品中甲醛的最小检测浓度为0．5mg/kg。比较了整体色谱柱和常规C18反相柱分离效果，表明整体色谱柱可在1．5min内实现衍生化产物的快速分离并进行定性定量，同时发现相对于常规柱，采用整体柱提高了检测灵敏度约10倍。     

Advantages of monolithic over particulate columns for multiresidue analysis of organic pollutants by in-tube solid-phase microextraction coupled to capillary liquid chromatography

The performance of a monolithic C(18) column (150 mm×0.2 mm i.d.) for multiresidue organic pollutants analysis by in-tube solid-phase microextraction (IT-SPME)-capillary liquid chromatography has been studied, and the results have been compared with those obtained using a particulate C(18) column (150 mm×0.5 mm i.d., 5 μm). Chromatographic separation has been carried out under isocratic elution conditions, and for detection and identification of the analytes a UV-diode array detector has been employed. Several compounds of different chemical structure and hydrophobicity have been used as model compounds: simazine, atrazine and terbutylazine (triazines), chlorfenvinphos and chlorpyrifos (organophosphorous), diuron and isoproturon (phenylureas), trifluralin (dinitroaniline) and di(2-ethylhexyl)phthalate. The results obtained revealed that the monolithic column was clearly advantageous in the context of multiresidue organic pollutants analysis for a number of reasons: (i) the selectivity was considerably improved, which is of particular interest for the most polar compounds triazines and phenyl ureas that could not be resolved in the particulate column, (ii) the sensitivity was enhanced, and (iii) the time required for the chromatographic separation was substantially shortened. In this study it is also proved that the mobile-phase flow rates used for separation in the capillary monolithic column are compatible with the in-valve IT-SPME methodology using extractive capillaries of dimensions similar to those used in conventional scale liquid chromatography (LC). On the basis of these results a new method is presented for the assessment of pollutants in waters, which permits the characterization of whole samples (4 mL) in less than 30 min, with limits of detection in the range of 5-50 ng/L.     

分散固相萃取-高效液相色谱法快速测定果蔬中的6种保鲜剂残留量

建立了采用分散固相萃取-高效液相色谱同时测定果蔬中2,4-滴、噻苯咪唑、乙萘酚、邻苯基苯酚、二苯醚和联苯6种保鲜剂残留量的方法。样品经乙腈提取(同时加入氯化钠和无水硫酸镁),提取液经酸性氧化铝分散固相萃取净化,采用Agilent TC C18色谱柱(250 mm×4.6 mm, 5 μm),以甲醇-0.02 mol/L的磷酸二氢钾溶液(pH 6)作为流动相,流速1.0 mL/min,梯度洗脱,用紫外检测器检测,检测波长为235 nm,外标法峰面积定量。6种保鲜剂在0.5～20 mg/L范围内线性关系良好,相关系数均大于0.99; 6种保鲜剂在样品中添加1、2和10 mg/kg 3个浓度水平的回收率为84.2%～99.1% (n=6),相对标准偏差为1.67%～10.3%;方法的定量限为1 mg/kg。该法简便、准确,适用于果蔬中6种保鲜剂残留量的检测。