Use of large-volume sample stacking in on-line solid-phase extraction-capillary electrophoresis for improved sensitivity

We present a new system for the sensitive analysis of cephalosporins by CE using both on-line SPE and large-volume sample stacking (LVSS). Sample volumes of 250 muL were loaded onto the SPE microcolumn which was then desorbed with 426 nL of ACN. The SPE elution plug was injected into the CE system via an in-line valve interface filling approximately 60% of the volume of the separation capillary. Subsequently, LVSS was performed by applying a voltage of -5 kV, which resulted in the simultaneous removal of the elution solvent and the preconcentration of the analytes in a narrow zone. This way the amount of analyte loaded into the capillary could be considerably increased without serious loss of CE separation efficiency. LODs for cefoperazone and ceftiofur were in the ng/L range which represents an improvement of a factor of 8450 and 11 450 when compared with direct CE injection. The cephalosporin test compounds presented a good linear response (corrected peak area) between 0.5 and 10 mug/L with correlation coefficients higher than 0.995. The final method is compared with previously reported LVSS-CE and SPE-CE systems for the analysis of cephalosporins.     

Determination of sulfonamide residues in water samples by in-line solid-phase extraction-capillary electrophoresis

An in-line solid-phase extraction-capillary electrophoresis method with UV–vis detection was developed for the monitoring of residues of five sulfonamides (sulfadoxin, sulfadimethoxine, sulfamerazine, sulfachloropyridazine and sulfamethoxazole) in tap, bottled mineral and river waters. For this purpose an analyte concentrator was constructed, based on the introduction of a small portion of a solid-phase extraction sorbent into the electrophoretic capillary to carry out an in-line concentration step, improving sensitivity. A detailed study was carried out to optimize parameters affecting the in-line solid-phase extraction process, such as the design of the concentrator device, type of sorbent and conditions of elution and injection. The proposed method is simple for the environmental monitoring of these antibiotic residues in waters, allowing the direct injection of the samples without any off-line pretreatment and achieving limits of detection between 0.3 and 0.6 μg/L. Recoveries ranging 52.2–109.2% and relative standard deviations below 13.4% were obtained.     

Developments in coupled solid-phase extraction-capillary electrophoresis 2009-2011

This article presents an overview of the design and application of coupled solid-phase extraction-capillary electrophoresis (SPE-CE) systems that have been reported in the literature between January 2009 and July 2011. The present paper is an update of two previous review papers covering the years 2000-2009 (Electrophoresis 2008, 29, 108-128; Electrophoresis 2010, 31, 44-54). Both in-line and on-line SPE-CE approaches are treated and outlined. Attention is paid to emerging technological developments, such as the use of carbon nanotubes and magnetic particles for on-line extraction of sample components prior to CE analysis. Selected examples illustrate the applicability of SPE-CE in biomedical, pharmaceutical, environmental and food analysis. A full overview of recent SPE-CE studies is given in table format, providing information about sample type, SPE sorbent, coupling mode, detection mode and limit of detection. Finally, some general conclusions and future perspectives are given.     

Determination of nonsteroidal anti-inflammatory drugs in biological fluids by automatic on-line integration of solid-phase extraction and capillary electrophoresis

A new, automatic method for the clean-up, preconcentration, separation, and quantitation of nonsteroidal anti-inflammatory drugs (NSAIDs) in biological samples (human urine and serum) using solid-phase extraction coupled on-line to capillary electrophoresis is proposed. Automatic pretreatment is carried out by using a continuous flow system operating simultaneously with the capillary electrophoresis equipment, to which it is linked via a laboratory-made mechanical arm. This integrated system is controlled by an electronic interface governed via a program developed in GWBasic. Capillary electrophoresis is conducted by using a separation buffer consisting of 20 mM NaHPO4, 20 mM beta-cyclodextrin and 50 mM SDS at pH 9.0, an applied potential of 20 kV and a temperature of 20 degrees C. The analysis time is 10 min and the detection limits were between 0.88 and 1.71 microg mL(-1). Automatic clean-up and preconcentration is accomplished by using a C-18 minicolumn and 75% methanol as eluent. The limit of detection of NSAIDs can be up to 400-fold improved when using sample clean-up. The extraction efficiency for these compounds is between 71.1 and 109.7 microg mL(-1) (RSD 2.0-7.7%) for urine samples and from 77.2 to 107.1 microg mL(-1) (RSD 3.5-7.1%) for serum samples.     

Lowering the concentration limits of detection by on-line solid-phase extraction-capillary electrophoresis-electrospray mass spectrometry

The use of solid-phase extraction coupled on-line to capillary electrophoresis using electrospray mass spectrometry detection (SPE-CE-ESI-MS) is described for the analysis of peptides in dilute solutions. A SPE microcartridge or analyte concentrator containing C(18) derivatized silica particles as the extraction sorbent was easily constructed near the inlet of the separation capillary using commercially available materials. The reversed-phase sorbent selectively retained the target peptides, enabling large volumes of the sample to be introduced (>100muL). The captured analytes were eluted in a small volume of an appropriate solution (20-50nL). This resulted in sample clean-up and concentration enhancement, with minimum sample handling. As the SPE-CE conditions were compatible with on-line ESI-MS detection, the potential for identifying and characterizing the preconcentrated analytes by SPE-CE-ESI-MS using a sheath-flow CE-ESI-MS interface is also shown. Using separation electrolytes containing N-[carbamoylmethyl]-2-aminoethanesulfonic acid (ACES) at pH 7.4, an elution plug of 80:20 (v/v) (25mM of formic acid in MeCN):H(2)O and a sheath liquid of 20mM of acetic acid in 50:50 (v/v) methanol:H(2)O the concentration limits of detection for the analyzed peptides in the positive ion mode were lowered to nanogram per milliliter levels. The systematic optimization of the operational parameters involved in the development of the SPE-CE method is described in detail, in order to promote robust and quantitative SPE-CE-ESI-MS analysis and facilitate the widespread use of the technique.     

In-capillary solid-phase extraction-capillary electrophoresis for the determination of chlorophenols in water

A novel CE method combined with SPE in a single capillary was developed for analysis of chlorophenols in water. A frit of 0.5 mm was first made by a sol-gel method, followed by packing a SPE sorbent in the inlet end of the capillary. Two phenol derivatives, 2,4-dichlorophenol and 2,4,5-trichlorophenol, were used as the model compounds. By loading sample solutions into the capillary, the two chlorophenols were extracted into the sorbent. They were desorbed by injecting only about 4 nL of methanol. Finally, the analytes were separated by conventional CE. The technique provided a concentration enhancement factor of over 4000-fold for both chlorophenols. The detection limits (S/N = 3) of 2,4-dichlorophenol and 2,4,5-trichlorophenol were determined to be 0.1 ng/mL and 0.07 ng/mL, respectively. For replicate analyses of 5 ng/mL of 2,4-dichlorophenol, within-day and between-day RSDs of migration time, peak height and peak area were in the range of 1.8-2.0%, 4.0-4.4% and 4.1-4.6%, respectively. The method shows wide linear range, acceptable reproducibility and excellent sensitivity, and it was applied to the analyses of spiked river water samples. The capillary packed with the SPE sorbents can be used for more than 400 runs without performance deterioration.     

Combining solid-phase microextraction and on-line preconcentration-capillary electrophoresis for sensitive analysis of pesticides in foods

The combined use of solid-phase microextraction (SPME) and different on-line preconcentration strategies for ultrasensitive capillary electrophoresis-ultraviolet (CE-UV) analysis of five pesticides in a single run is investigated. Normal stacking mode (NSM), field-enhanced sample injection (FESI), and stacking with matrix removal (SWMR) are explored to increase the sensitivity of the CE-UV analysis of a selected group of pesticides (cyprodinil, cyromazine, pyrifenox, pirimicarb, and pyrimethanil). It could be observed that reverse polarity-stacking with matrix removal (RP-SWMR) provided the best results in terms of sensitivity (enhancement was up to 272-fold compared with normal injection). The separation buffer consisted of 0.4 mM cetyltrimethylammonium chloride (CTAC), 0.4 M acetic acid at pH 4 containing 5% v / v 2-propanol. This approach was then combined with SPME to determine the pesticides in water, apple, and orange juice. The combination of both preconcentration procedures allowed the determination of these pesticides at concentrations down to 2.5 microg / L in water and 3.1 microg / L in juices (i.e., levels well below the maximum residue limits allowed for these compounds). To our knowledge, this is the first report showing the great possibilities of the combined use of SPME, on-line sample preconcentration, and CE for pesticide analysis.     

Determination of urea-derived pesticides in fruits and vegetables by solid-phase preconcentration and capillary electrophoresis

A multiresidue analytical method based on solid-phase extraction (SPE) enrichment combined with capillary electrophoresis (CE), using micellar electrokinetic capillary chromatography (MEKC), was developed to determine ten substituted urea pesticides in orange and tomato samples. Several factors such as pH, composition and concentration of the buffer, concentration of surfactant, addition of organic solvent, and working voltage were optimized to obtain the best compound separation in the shortest time. Separation can be achieved in 7 min using a micellar aqueous pH 9 buffer composed of 4 mM borate and 35 mM sodium dodecyl sulfate. After an SPE procedure, which provided a 10-fold enrichment, the limit of detection was about 0.05 mg kg(-1), which is in the order of the maximum residue limits (MRLs) established by the European Union (EU) for most of these compounds. Increasing the enrichment factor by using a larger amount of sample is difficult in oranges due to the matrix interferences, but is possible in tomatoes, which gave cleaner extracts and easily reached a 25-fold enrichment factor. The procedure involving SPE and CE provided acceptable recoveries (ranged 42-118%) and relative standard deviations (RSDs; < 19%) at levels between 0.3 and 5 mg kg(-1).     

Preconcentration and frontal electroelution of amino acids for in-line solid-phase extraction-capillary electrophoresis

A new frontal electroelution approach that can be used for the preconcentration of amino acids in in-line solid-phase extraction-capillary electrophoresis (SPE-CE) has been developed. A single capillary was employed featuring a short monolithic SPE column created inside the capillary via photo-initiated, free-radical polymerisation of 3-sulfopropyl methacrylate and butyl methacrylate monomers. A weak electrolyte of dilute H₂SO₄, pH 2.9, was found to promote adsorption of the amino acids onto the SPE column. Elution of the amino acids was achieved using a dual solvation/ion-exchange transient boundary mobilised via EOF by using a strong electrolyte containing 62.5 mM ethylenediamine, pH 2.9 with H₂SO₄ and 40% (v/v) acetonitrile. Using these two electrolytes, tryptophan was adsorbed onto the SPE column in weak electrolyte and eluted via a frontal electroelution mechanism in the strong electrolyte. Injections up to 20 min, corresponding to over 14 column volumes (or 1400% of the capillary volume) of sample provided quantitative extraction of tryptophan from the weak electrolyte and were eluted without any loss in efficiency. This represents a practical increase of approximately 300-fold when compared to a typical hydrodynamic injection occupying 5% of the capillary volume.     

Determination of triazine herbicides in natural waters by solid-phase extraction and non-aqueous capillary zone electrophoresis

Capillary zone electrophoresis (CZE) in an organic medium was used to analyse triazines at sub-ppb concentration levels in natural waters after a preconcentration step using conventional C18 cartridges and new Oasis HLB devices. With both sorbents, satisfactory results were obtained on analysing deionized water. However, on analysing natural waters, both sorbents showed very different types of behaviour. The different variables affecting the elution of both sorbents were studied, resulting in the choice of Oasis HLB as the most suitable for later separation by CZE in non-aqueous medium. Combination of a preconcentration step with electrokinetic injection revealed that capillary electrophoresis with simple UV detection can also be used satisfactorily for the quantification of micropollutants in natural waters. The detection limits obtained varied between 0.01 and 0.05 microg l(-1), depending on the type of matrix analysed. The day-to-day precision varied between 0.9% and 2.3%, expressed as the relative standard deviation.     

Determination of pharmaceutical residues in waters by solid-phase extraction and large-volume on-line derivatization with gas chromatography-mass spectrometry

This work presents a modified method to analyze selected pharmaceutical residues (clofibric acid, ibuprofen, carbamazepine, naproxen, ketoprofen and diclofenac) in water samples. Various solid-phase extraction cartridges were investigated. The newly developed Oasis HLB (polystyrene-divinylbenzene-N-vinyl pyrrolidone terpolymer) solid-phase extraction (SPE) cartridge provides the optimal sample extraction results. The analytes were then identified and quantitatively determined by gas chromatography-mass spectrometry (GC-MS) via on-line derivatization in the injection-port using a large-volume (10 microl) sample injection with tetrabutylammonium (TBA) salts. This injection-port derivatization technique provides sensitivity, fast and reproducible results for pharmaceutical residues analysis. Mass spectra of butylated derivatives and tentative fragmentation profiles are proposed. Molecular ions and some characteristic ions were used as the quantitation ions to obtain maximum detection sensitivity and specificity. The quantitation limits of these compounds ranged from 1.0 to 8.0 ng/l in 500 ml tap water samples. Recovery of these residues in spiked various water samples ranged from 50 to 108% while RSD ranged from 1 to 10%. The selected analytes were detected in concentrations of 30 to 420 ng/l in wastewater treatment plant effluent and river water samples.     

快速溶剂萃取-毛细管电泳法测定土壤和底泥中磺胺类药物残留

建立了一种快速溶剂萃取(ASE)-毛细管电泳检测土壤和底泥中磺胺类药物残留的新方法。通过优化ASE的萃取条件,选取甲醇为萃取剂,在70℃、10.3 MPa的条件下提取土壤和底泥样品中的磺胺类药物。毛细管电泳检测磺胺嘧啶,磺胺甲基嘧啶和磺胺间二甲氧基嘧啶的标准曲线具有良好的线性(r>0.999)。方法的定量限(LOQ,S/N=10)为0.056～0.070 mg/kg。日内相对标准偏差在0.4%～2.5%之间,日间相对标准偏差在1.2%～4.6%之间。3个加标水平0.100、0.625、2.50 mg/kg的平均回收率在82%～103%之间,RSD≦4.3%。方法已用于土壤和底泥样品前处理和磺胺类药物残留检测。     

Determination of alkyl- and alkanolamines in drinking and natural waters by capillary electrophoresis with isotachophoretic on-line preconcentration

A procedure is developed for the determination of several amines in drinking and natural waters by capillary electrophoresis with isotachophoretic on-line preconcentration without sample preparation. A background electrolyte based on acridine as an absorbing ion is proposed for analysis with isotachophoretic on-line preconcentration and indirect photometric detection. The sample was injected in the hydrodynamic mode. The procedure was tested on drinking and natural water samples. The accuracy of data obtained was confirmed by the added–found method. The analytical range was from 0.25 to 5 mg/L. The time of one analysis was 5–6 min.     

Determination of organophosphorus pesticides in soil by headspace solid-phase microextraction

Headspace solid-phase microextraction (SPME) has been developed for the analysis of common organophosphorus pesticides in soil. Factors such as adsorption-time, sampling temperature and matrix modification by addition of water were carefully considered to optimize the extraction efficiency. This technique could achieve limits of detection of 143 ng/g for Malathion and Parathion, and 28.6 ng/g for Phorate, Diazinon and Disulfoton in humic soil when the extracted sample was analyzed by gas chromatography-flame ionization detector (GC-FID). Lower limits of detection of 28.6 ng/g for Malathion and Parathion, and 14.3 ng/g for Phorate, Diazinon and Disulfoton can be achieved by analyzing the extracted sample with gas chromatography/mass spectrometric detector (GC/MS). As the extraction efficiency was generally better when analyzing sandy soil, the limits of detection are envisaged to be even better for such a matrix. The technique was found to be reliable with good precision of about 6.5% RSD for the sandy soil and about 15% for the humic material. The poorer precision of extraction from the humic material is probably related to the poorer homogeneity of this material. The linearity of extraction was good with linear calibration in the range of 0.143 to 28.6 μg/g. Finally, headspace SPME was compared to aqueous extraction of soil followed by SPME (LE-SPME). The recoveries obtained by headspace SPME were comparable to those from liquid-liquid extraction of soil followed by SPME. However, the analysis of headspace SPME has less background interference. Perhaps, the greatest advantage of this technique is its non-destructive nature so that it is possible to perform further laboratory analysis of the samples after headspace SPME has been carried out. Received: 13 July 1998 / Revised: 10 November 1998 / Accepted: 17 November 1998     

Determination of organophosphorus pesticides in soil by headspace solid-phase microextraction

Headspace solid-phase microextraction (SPME) has been developed for the analysis of common organophosphorus pesticides in soil. Factors such as adsorption-time, sampling temperature and matrix modification by addition of water were carefully considered to optimize the extraction efficiency. This technique could achieve limits of detection of 143 ng/g for Malathion and Parathion, and 28.6 ng/g for Phorate, Diazinon and Disulfoton in humic soil when the extracted sample was analyzed by gas chromatography-flame ionization detector (GC-FID). Lower limits of detection of 28.6 ng/g for Malathion and Parathion, and 14.3 ng/g for Phorate, Diazinon and Disulfoton can be achieved by analyzing the extracted sample with gas chromatography/mass spectrometric detector (GC/MS). As the extraction efficiency was generally better when analyzing sandy soil, the limits of detection are envisaged to be even better for such a matrix. The technique was found to be reliable with good precision of about 6.5% RSD for the sandy soil and about 15% for the humic material. The poorer precision of extraction from the humic material is probably related to the poorer homogeneity of this material. The linearity of extraction was good with linear calibration in the range of 0.143 to 28.6 μg/g. Finally, headspace SPME was compared to aqueous extraction of soil followed by SPME (LE-SPME). The recoveries obtained by headspace SPME were comparable to those from liquid-liquid extraction of soil followed by SPME. However, the analysis of headspace SPME has less background interference. Perhaps, the greatest advantage of this technique is its non-destructive nature so that it is possible to perform further laboratory analysis of the samples after headspace SPME has been carried out.     

Determination of organochlorine pesticides by gas chromatography with solid-phase microextraction

Summary A study of different extraction techniques for the determination of a selected group of organochlorine compounds in surface waters is presented. Comparison of liquid-liquid extraction (LLE) with solid-phase extraction (SPE) and solid-phase microextraction (SPME) with fibers of different polarity shows that SPME with a recently commercialised fiber of polydimethylsiloxane divinylbenzene allows these compounds to be determined in surface waters with good extraction efficiencies. Extraction time, effect of temperature, ionic strength and pH were optimised, allowing quantification in agricultural effluents in the range 1.0–60 ng·L⁻¹.     

Improved solid-phase microextraction device for use in on-line immunoaffinity capillary electrophoresis

A simple solid-phase microextraction device was fabricated for use in on-line immunoaffinity capillary electrophoresis (CE). The device, designed in the form of a four-part cross-shaped or cruciform configuration, includes a large-bore tube to transport samples and washing buffers and a small-bore fused-silica capillary for separation of analytes. At the intersection of the transport and separation tubes, a small cavity was fabricated, termed the analyte concentrator-microreactor, which contains four porous walls or semipermeable membranes (one for each inlet and outlet of the tubes) permitting the confinement of beads or suitable microstructures. The surface of the beads in the analyte concentrator carried a molecular recognition adsorbing chemical or affinity ligand material. The improved cruciform configuration of the analyte concentrator-microreactor device, designed for use in on-line immunoaffinity CE, enables it to specifically trap, enrich, and elute an analyte from any biological fluid or tissue sample extract without any sample pretreatment except filtration, centrifugation, and/or dilution allowing the separation and characterization of target analyte(s) with improved speed, sensitivity, and lower cost than existing techniques. As a model system, Fab' fragments derived from a purified immunoglobulin G (IgG) antibody were covalently bound to controlled-porosity glass and used as constituents of the analyte-microreactor device. The high-specificity polyclonal antibodies employed in these experiments were individually raised against the acidic nonsteroidal anti-inflammatory drugs ibuprofen and naproxen, and the neuropeptides angiotensin II, and neurotensin. These compounds, which were present in simple and complex matrices were captured by and eluted from the analyte concentrator-microreactor using a 50 mM sodium tetraborate buffer solution, pH 9.0, followed by a 100 nL plug of 300 mM glycine buffer, pH 3.4. Two analyte concentrators were tested independently: one containing Fab' fragments derived from antibodies raised against ibuprofen and naproxen; the other containing Fab' fragments derived from antibodies raised against angiotensin II and neurotensin. Each resulting electropherogram demonstrated the presence of two eluted materials in less than 20 min. Immunoaffinity CE performed in a cruciform structure was simpler and faster than previously reported in the literature using on-line microextraction devices designed in a linear format. The new concentration-separation system operated consistently for many runs, maintaining reproducible migration times and peak areas for every analyte studied.     

Determination of organophosphorus pesticides in honeybees after solid-phase microextraction

The solvation parameter model has been applied to the characterization of micellar electrokinetic chromatographic (MEKC) systems with mixtures of lithium dodecyl sulfate and lithium perfluorooctanesulfonate as surfactant. The variation in MEKC surfactant composition results in changes in the coefficients of the correlation equation, which in turns leads to information on solute-solvent and solute-micelle interactions. Lithium perfluorooctanesulfonate is more dipolar and hydrogen bond acidic but less polarizable and hydrogen bond basic than lithium dodecyl sulfate. Therefore mixtures of lithium dodecyl sulfate and lithium perfluorooctanesulfonate cover a very wide range of polarity and hydrogen bond properties, which in turn results in important selectivity changes for analytes with different solute properties.     

Determination of thiabendazole in foods and waters by solid-phase transmitted room-temperature phosphorescence

A new method for the determination of thiabendazole (TBZ) is proposed, based on enhanced native phosphorescence at room temperature when the pesticide is fixed on paper and using Pb (CH₃-COO)₂ as the enhancer. The sample and enhancer solutions were deposited on a slip of paper (Whatman No. 4), previously humidified with pH 4.0 acetic/acetate buffer solution, after which the paper was dried and placed between two quartz plates. The diffuse transmitted phosphorescence intensity was measured directly at _ex = 303 nm and _em = 472 nm. The applicable concentration range was 160.0–1200.0 ng/ml, with a relative standard deviation of 1.2%. The detection and quantification limits were 47.7 and 158.9 ng/ml, respectively. This simple method was used to measure the levels of this pesticide in potatoes, green beans, lettuce and different types of waters, showing good selectivity in all instances.     

Determination of herbicides and their metabolites in natural waters by capillary zone electrophoresis combined with dispersive liquid-liquid microextraction and on-line preconcentration

A method has been proposed for the determination of 17 herbicides and their metabolites in natural waters by capillary zone electrophoresis with UV detection at 190 nm. Dispersive liquid-liquid microextraction with trichloromethane has been used for pesticide recovery from water. The high sensitivity of determination has been provided by additional intracappilary preconcentration: the limits of pesticide detection in water involving off- and on-line preconcentration are 0.5–3.0 μg/L. The analysis takes 1–1.5 h; the relative standard deviation of the analysis results does not exceed 5%.