Trace enrichment of (fluoro)quinolone antibiotics in surface waters by solid-phase extraction and their determination by liquid chromatography-ultraviolet detection

A new and simple analytical methodology for the simultaneous analysis of acidic and zwitterionic (fluoro)quinolones in surface waters at trace concentration level is presented. The method is based on the preconcentration of these analytes by a solid-phase extraction procedure and their subsequent quantification by liquid chromatography using ultraviolet detection. The breakthrough volumes of the selected (fluoro)quinolones in four different sorbents--C18, styrenedivinylbenzene (SDB), C18-cation-exchange and SDB-cation-exchange--have been evaluated and varied between 25 and 150 ml depending on the antibiotic and the sorbent used. An exhaustive study of the influence of sample pH on the preconcentration step has been carried out in order to find a suitable procedure for extraction of acidic and zwitterionic FQs in one single step. Under optimum conditions, it was possible to percolate up to 250 ml of water solution onto both C18 and SDB-cation-exchange cartridges with quantitative recoveries for all the analytes tested. However, matrix components of the surface water samples analysed negatively affected the recoveries of the analytes in the SDB-cation-exchange cartridge and thus, C18 cartridges were finally selected for the analysis of the (fluoro)quinolones in lake and river water. The limits of detection achieved with this procedure varied between 8 and 20 ng l(-1) proving its suitability for the determination of the (fluoro)quinolones in water samples at a realistic environmental concentration level.     

Green methodology based on dispersive liquid–liquid microextraction and micellar electrokinetic chromatography for 5‐nitroimidazole analysis in water samples

Dispersive liquid–liquid microextraction has been proposed as an extraction technique combined with micellar electrokinetic chromatography (MEKC) for the analysis of eight 5‐nitroimidazole compounds, including some metabolites, in water samples. Determination has been carried out using a diode array detector, employing 20 mM sodium phosphate and 150 mM SDS as separation buffer. Separation has taken place under a voltage of 25 kV and a temperature of 20°C. Samples were prepared in a buffer without micelles and they were hydrodynamically injected at 50 mbar for 25 s, producing a sweeping effect on the analytes for increasing sensitivity. Different factors involved in the dispersive liquid–liquid microextraction procedure were optimized, such as sample pH, nature, and volume of extraction and dispersive solvents in the mixture, percentage of NaCl added to sample and shaking time after the injection of the extraction and dispersive solvents. The method was characterized for water samples, achieving detection limits lower than 2.4 μg/L. Trueness was checked in river, tap, and bottled water. Dispersive liquid–liquid microextraction combined with MEKC constitutes an easy, cheap, and green alternative for 5‐nitroimidazole analysis in environmental water samples.     

Analysis of microcystins using high‐performance liquid chromatography and magnetic solid‐phase extraction with silica‐coated magnetite with cetylpyridinium chloride

Microcystins (MCs), produced by freshwater cyanobacteria, can be serious water pollutants, so it is important to monitor their concentration in drinking water. We have developed a method for rapid and accurate determination of microcystin levels in environmental water, using magnetic solid‐phase extraction and high‐performance liquid chromatography with UV detection. The magnetic composite material, which was combined with cetylpyridinium chloride, was prepared by hydrothermal synthesis. The optimal extraction of microcystins in water sample was achieved by optimizing the amount of adsorbent, time of adsorption, ratio of eluting solvent, and volume of eluent. Under the optimal conditions, the limit of detection of MC‐LR was 0.001 μg/L, and the limit of quantification was 0.0028 μg/L. The limit of detection of MC‐RR was 0.001 μg/L, and the limit of quantification was 0.003 μg/L. These values are far lower than those established by the International Health Organization for the maximum concentration of microcystins in drinking water. The magnetic solid‐phase extraction adsorbent used in this method has the advantages of simple preparation, low price, and easy solid–liquid separation, and it can be used for the rapid and sensitive monitoring of trace microcystins in environmental water samples.     

Combination of a sub‐3 μm superficially porous particle packed column with charged aerosol detection for the simple and sensitive measurement of nine macrolides in human urine

Due to the lack of chromophores in many macrolides, analytical methods based on mass spectrometry and electrochemical detection coupled to liquid chromatography have been suggested to be suitable for the quantification of macrolides in complex matrices. In this study, a simple and sensitive analytical method was established for the simultaneous measurement of nine macrolides in human urine by combining a sub‐3 μm superficially porous particle packed column with charged aerosol detection. After thorough investigation of various sample preparation methods, including two liquid–liquid extraction methods and four solid‐phase extraction methods, HLB solid‐phase extraction was selected and further optimized. Absolute recovery of the optimized sample preparation method ranged from 99.5–110.2%, indicating its very high extraction/clean‐up efficiency. For chromatography, parameters influencing macrolide separation were systematically optimized, and the resulting conditions allowed baseline separation of nine macrolides within 24 min using a very simple mobile phase. The established method was validated for linearity, limit of detection, limit of quantification, absolute recovery, and precision. Based on its limit of detection (0.025–0.100 μg/mL), the method had similar or greater sensitivity than most methods based on electrochemical detection. It was found that the current method was appropriate for application to real human urine samples after drug administration.     

Determination of chlorophenols in water using dispersive liquid–liquid microextraction coupled with water‐in‐oil microemulsion electrokinetic chromatography in normal stacking mode

The current routes to couple dispersive liquid–liquid microextraction with capillary electrophoresis are the evaporation of water immiscible extractants and the back‐extraction of analytes. In this study, a new methodology for this combination using water‐in‐oil microemulsion electrokinetic chromatography coupled with normal stacking mode on‐line sample concentration was developed to analyze chlorophenols in water samples. The analytes were extracted with tributyl phosphate and the extractant dilution (3×) was directly injected into an electrophoresis buffer (7.7 cm) containing 5% sodium dodecyl sulfate, 78% 1‐butanol, 2% 1‐heptane, and 15% sodium acetate solution (pH 8.0). This proposed method is very simple and convenient compared to the conventional procedures. The key parameters affecting separation and concentration were systematically optimized. Under the optimized conditions, dispersive liquid–liquid microextraction contributed an enrichment factor of 45–50, and the overall sensitivity improvement was 312–418‐fold. Limits of detection between 1.4 and 3.0 ng/mL and limits of quantification between 4.5 and 10.2 ng/mL were achieved. Acceptable repeatability lower than 3.0% for migration time and 9.0% for peak areas were obtained. The developed method was successfully applied for analysis of the chlorophenols in real water samples.     

Salting‐out homogeneous liquid–liquid extraction in narrow‐bore tube: Extraction and preconcentration of phthalate esters from water

In this study a simple and rapid sample preparation technique, homogeneous liquid–liquid extraction based on phase separation in the presence of a salt performed in a narrow‐bore tube, followed by GC‐flame ionization detection has been developed. In this work, sodium chloride and ACN were used as the salting‐out agent and water‐soluble extraction solvent, respectively. The homogeneous solution of water and ACN was broken by addition of the salt. Small volume of ACN was collected on top of the tube and the extracted analytes in the collected phase were determined. It has been successfully used for the analysis of five phthalate esters as model compounds in aqueous sample. Experimental parameters affecting the extraction efficiency such as kind and volume of the water‐soluble organic solvent, length and diameter of the tube, and pH of the sample solution were investigated. Under the optimal conditions, the LODs were between 0.02 and 0.7 μg/L and enrichment factors were in the range of 172–309. In addition, good linearity (between 1 and 5000 μg/L) and high precision on the base of RSD (<8%, C = 600 μg/L, n = 6) were achieved.     

Determination of antibacterial agent tilmicosin in pig plasma by LC/MS/MS and its application to pharmacokinetics

A rapid and sensitive high‐performance liquid chromatography–tandem mass spectrometry (LC–MS/MS) method was developed and validated to quantify tilmicosin in pig plasma. Plasma samples were prepared by liquid–liquid extraction. Chromatographic separation was achieved on a C₁₈ column (2.1 × 30 mm, 3.5 μm) using acetonitrile–water (90:10, v /v; water included 0.1% formic acid) as the mobile phase. Mass detection was carried out using positive electrospray ionization in multiple reaction monitoring mode. The calibration curve was linear from 0.5 to 2000 ng/mL (r ² = 0.9998). The intra‐ and inter‐day accuracy and precision were within the acceptable limits of ±10% for all tilmicosin concentrations. The recoveries ranged from 95 to 99% for the three tested concentrations. The LC–MS/MS method described herein was simple, fast and less laborious than other methods, achieved high sensitivity using a small sample volume, and was successfully applied to pharmacokinetic studies of tilmicosin enteric granules after oral delivery to pigs. In comparison with tilmicosin premix, tilmicosin enteric granules slowed the elimination rate of tilmicosin, prolonged its period of action and significantly improved its bioavailability.     

Facile preparation of magnetic graphene oxide/nanoscale zerovalent iron adsorbent for magnetic solid‐phase extraction of ultra‐trace quinolones in milk samples

A simple pH‐responsive magnetic solid‐phase extraction method was developed using graphene oxide–coated nanoscale zerovalent iron nanoparticles as an efficient adsorbent prior to high‐performance liquid chromatography‐tandem mass spectrometry for determination of ultra‐trace quinolones in milk samples. Various parameters affecting maghemite synthesis and separation such as pH of sample solution, amount of magnetic adsorbent, eluent type, and volume were optimized. The limits of detection are from 3.1 to 13.3 ng/L. The intra‐ and interprecision values are in the range of 2.9–6.9% and 7.6–15.1%, respectively. Recoveries are from 82.4 to 103.9%. Therefore, this simple and sensitive method is suitable for detecting ultra‐trace quinolone residues in milk.     

Determination of organophosphate esters in water samples by mixed‐mode liquid chromatography and tandem mass spectrometry

A simple and sensitive method for the determination of organophosphate esters in water samples by mixed‐mode liquid chromatography with electrospray ionization tandem mass spectrometry coupled with solid‐phase extraction is developed. Using seven alkyl phosphates, three chlorinated alkyl phosphates, and four aryl phosphates as the targets, the developed method was systematically evaluated on the basis of the influence of the solid‐phase extraction cartridge, eluting solvent, sample‐loading volume, mobile phase condition, and the separation of reversed‐phase chromatography and mixed‐mode liquid chromatography. Under the optimal conditions, these organophosphate esters can be extracted by ENVI‐18 cartridge, eluted by 6 mL of 25% dichloromethane in acetonitrile, and then qualified and quantified by mixed‐mode liquid chromatography with tandem mass spectrometry in the multiple reaction‐monitoring mode. The application of mixed‐mode liquid chromatography endows the separation with reasonable retention for both hydrophilic and hydrophobic organophosphate esters regardless of their polarity, which is hardly achieved by reversed‐phase chromatography. Good linearity (from 0.9877 to 0.9969), low quantification limits (1–35 ng/L after extraction of 100 mL of river water), and acceptable recovery rates (58.6–116.2%, with the relative standard deviation <18.0%) were obtained. Finally, the established method was used for analyzing surface water samples, and the good applicability of this method was demonstrated.     

Solvent‐assisted dispersive micro‐SPE by using aminopropyl‐functionalized magnetite nanoparticle followed by GC‐PID for quantification of parabens in aqueous matrices

In this research, solvent‐assisted dispersive micro‐SPE was introduced as a simple modified technique for the determination of parabens in water and cosmetic samples. Aminopropyl‐functionalized magnetite nanoparticles (MNPs) were successfully synthesized and applied. GC with photoionization detector was used for the separation and detection of parabens. In this method, hexylacetate (15 μL) as a solvent and aminopropyl‐functionalized MNPs (5 μg) as a sorbent were added to an aqueous sample (10 mL) and then the sample was sonicated. Dispersed magnetite was collected in the bottom of the conical tube by using a strong magnet and then ACN was added as a desorption solvent. Forty microliters of this solvent was transferred into a microvial and then acetic anhydride and pyridine were added, thus derivatization was performed by acetic anhydride. After evaporation, 1 μL of derivatized sample was injected into a gas chromatograph for analysis. Several important parameters, such as kind of organic solvent, desorption solvent and volume, amount of aminopropyl‐functionalized MNPs and effect of salt addition were investigated. Under optimum conditions, the limits of detection achieved were between 50 and 300 ng/L, with RSDs (n = 5) lower than 8%. Under the optimum conditions, the enrichment factors ranged from 217 to 1253 and the extraction recoveries ranged from 10 to 62%. The recoveries were obtained for the analytes in river water and mouthwash solution and hand cream in the range of 87–103%. The advantages of proposed method are simplicity of operation, rapidity, high extraction yields, and environmental friendly character.     

Sensitive determination of three aconitum alkaloids and their metabolites in human plasma by matrix solid‐phase dispersion with vortex‐assisted dispersive liquid–liquid microextraction and HPLC with diode array detection

A simple and sensitive method for determination of three aconitum alkaloids and their metabolites in human plasma was developed using matrix solid‐phase dispersion combined with vortex‐assisted dispersive liquid–liquid microextraction and high‐performance liquid chromatography with diode array detection. The plasma sample was directly purified by matrix solid‐phase dispersion and the eluate obtained was concentrated and further clarified by vortex‐assisted dispersive liquid–liquid microextraction. Some important parameters affecting the extraction efficiency, such as type and amount of dispersing sorbent, type and volume of elution solvent, type and volume of extraction solvent, salt concentration as well as sample solution pH, were investigated in detail. Under optimal conditions, the proposed method has good repeatability and reproducibility with intraday and interday relative standard deviations lower than 5.44 and 5.75%, respectively. The recoveries of the aconitum alkaloids ranged from 73.81 to 101.82%, and the detection limits were achieved within the range of 1.6–2.1 ng/mL. The proposed method offered the advantages of good applicability, sensitivity, simplicity, and feasibility, which makes it suitable for the determination of trace amounts of aconitum alkaloids in human plasma samples.     

Application of packed porous nanofibers—Solid‐phase extraction for the detection of sulfonamide residues from environmental water samples by ultra high performance liquid chromatography with mass spectrometry

Porous electrospun nanofibers, as new materials for solid‐phase extraction, were synthesized by electrospinning and coupled with ultra high performance liquid chromatography and mass spectrometry to determine sulfonamide residues in environmental water. Aligned porous polystyrene electrospun nanofibers were fabricated under the mechanism of phase separation. The high‐specific surface of these nanofibers (70 m²/g) could improve recoveries of the target sulfonamides 4–10 times compared with that of polystyrene nonporous material (3.8 m²/g). Under the optimized conditions, 13 sulfonamide residues showed an excellent linear relationship in the range of 0.125–12.5 ng/mL with a linear correlation coefficient (r²) greater than 0.99, and the detection limits of sulfonamides were as low as 0.80–5.0 ng/L. Compared to the commercial C₁₈ and HLB columns, the homemade porous nanofibers columns had some merits including simple fabrication and extraction process, short process time and environmental friendliness. The optimized method was applied to eight water samples collected from different livestock farms (Xuzhou, China). The results showed that polystyrene porous nanofibers were promising to preconcentrate sulfonamides of different polarities in the waste water.     

Preconcentration and determination of ceftazidime in real samples using dispersive liquid–liquid microextraction and high‐performance liquid chromatography with the aid of experimental design

A rapid and simple method for the extraction and preconcentration of ceftazidime in aqueous samples has been developed using dispersive liquid–liquid microextraction followed by high‐performance liquid chromatography analysis. The extraction parameters, such as the volume of extraction solvent and disperser solvent, salt effect, sample volume, centrifuge rate, centrifuge time, extraction time, and temperature in the dispersive liquid–liquid microextraction process, were studied and optimized with the experimental design methods. Firstly, for the preliminary screening of the parameters the taguchi design was used and then, the fractional factorial design was used for significant factors optimization. At the optimum conditions, the calibration curves for ceftazidime indicated good linearity over the range of 0.001–10 μg/mL with correlation coefficients higher than the 0.98, and the limits of detection were 0.13 and 0.17 ng/mL, for water and urine samples, respectively. The proposed method successfully employed to determine ceftazidime in water and urine samples and good agreement between the experimental data and predictive values has been achieved.     

Multiclass method for the quantification of 92 veterinary antimicrobial drugs in livestock excreta,wastewater, and surface water by liquid chromatography with tandem mass spectrometry

A simple multiresidue method was developed for detecting and quantifying 92 veterinary antimicrobial drugs from eight classes (β‐lactams, quinolones, sulfonamides, tetracyclines, lincomycins, macrolides, chloramphenicols, and pleuromutilin) in livestock excreta and water by liquid chromatography with tandem mass spectrometry. The feces samples were extracted by ultrasound‐assisted extraction with a mixture of acetonitrile/water (80:20, v/v) and edetate disodium, followed by a cleanup using solid‐phase extraction with an amino cartridge. Water samples were purified with hydrophilic–lipophilic balance solid‐phase extraction column. Urine samples were extracted with acetonitrile and edetate disodium. Detection of veterinary antimicrobial drugs was achieved by liquid chromatography with tandem mass spectrometry using both positive and negative electrospray ionization mode. The recovery values of veterinary antimicrobial drugs in feces, urine, and water samples were 75–99, 85–110, and 85–101% and associated relative standard deviations were less than 15, 10, and 8%, respectively. The limits of quantification in feces, urine, and water samples were 0.5–1, 0.5–1, and 0.01–0.05 μg/L, respectively. This method was applied to determine real samples obtained from local farms and provides reliable quantification and identification results of 92 veterinary antimicrobial drugs in livestock excreta and water.     

High‐density extraction solvent‐based solvent de‐emulsification dispersive liquid–liquid microextraction combined with MEKC for detection of chlorophenols in water samples

For the first time, the high‐density solvent‐based solvent de‐emulsification dispersive liquid–liquid microextraction (HSD‐DLLME) was developed for the fast, simple, and efficient determination of chlorophenols in water samples followed by field‐enhanced sample injection with reverse migrating micelles in CE. The extraction of chlorophenols in the aqueous sample solution was performed in the presence of extraction solvent (chloroform) and dispersive solvent (acetone). A de‐emulsification solvent (ACN) was then injected into the aqueous solution to break up the emulsion, the obtained emulsion cleared into two phases quickly. The lower layer (chloroform) was collected and analyzed by field‐enhanced sample injection with reverse migrating micelles in CE. Several important parameters influencing the extraction efficiency of HSD‐DLLME such as the type and volume of extraction solvent, disperser solvent and de‐emulsification solvent, sample pH, extraction time as well as salting‐out effects were optimized. Under the optimized conditions, the proposed method provided a good linearity in the range of 0.02–4 μg/mL, low LODs (4 ng/mL), and good repeatability of the extractions (RSDs below 9.3%, n = 5). And enrichment factors for three phenols were 684, 797, and 233, respectively. This method was then utilized to analyze two real environmental samples from wastewater and tap water and obtained satisfactory results. The obtained results indicated that the developed method is an excellent alternative for the routine analysis in the environmental field.     

Determination of seven drugs of abuse and their metabolites in surface and wastewater using solid‐phase extraction coupled to liquid chromatography with high‐resolution mass spectrometry

A method based on liquid chromatography with electrospray ionization high‐resolution mass spectrometry (Exactive Orbitrap) combined with solid‐phase extraction using a strong cationic exchange mixed‐mode sorbent has been developed for the determination of seven drugs of abuse, including two synthetic cathinones, as well as some of their metabolites in environmental water samples. The method provides low detection limits and a high confirmation power thanks to the diagnostic and two fragment ions monitored for each compound in high‐resolution mass spectrometry, providing six identification points for each analyte. The clean‐up step based on methanol in the extraction step adequately decreased the matrix effect, mainly for river and effluent water, and provided suitable process efficiency. Method detection and quantitation limits for environmental waters were at low nanogram per liter. The method was applied to analyze the samples of influent and effluent wastewater, as well as surface water. Codeine, methadone, and its metabolite were determined in all samples of wastewater and the metabolite of cocaine, benzoylecgonine, was found at the highest concentration.     

Highly sensitive method for the determination of a novel triple kinase inhibitor with anti‐cancer activity,JI‐101, in rat plasma by liquid chromatography–electrospray ionization tandem mass spectrometry: application to a pharmacokinetic study

A highly sensitive, rapid assay method has been developed and validated for the estimation of JI‐101 in rat plasma with liquid chromatography coupled to tandem mass spectrometry with electrospray ionization in the positive‐ion mode. The assay procedure involves extraction of JI‐101 and phenacetin (internal standard, IS) from rat plasma with a solid‐phase extraction process. Chromatographic separation was achieved using a binary gradient using mobile phase A (acetonitrile) and B (0.2% formic acid in water) at a flow rate of 0.30 mL/min on a Prodigy ODS column with a total run time of 4.0 min. The MS/MS ion transitions monitored were 466.1 → 265 for JI‐101 and 180.1 → 110.1 for IS. Method validation and sample analysis were performed as per FDA guidelines and the results met the acceptance criteria. The lower limit of quantitation achieved was 5.03 ng/mL and the linearity range extended from 5.03 to 2014 ng/mL. The intra‐day and inter‐day precisions were in the ranges of 1.17–19.6 and 3.09–10.4%, respectively. This method has been applied to a pharmacokinetic study of JI‐101 in rats. Copyright © 2010 John Wiley & Sons, Ltd.     

Microwave‐assisted liquid–liquid microextraction based on solidification of ionic liquid for the determination of sulfonamides in environmental water samples

An easy, quick, and green method, microwave‐assisted liquid–liquid microextraction based on solidification of ionic liquid, was first developed and applied to the extraction of sulfonamides in environmental water samples. 1‐Ethy‐3‐methylimidazolium hexafluorophosphate, which is a solid‐state ionic liquid at room temperature, was used as extraction solvent in the present method. After microwave irradiation for 90 s, the solid‐state ionic liquid was melted into liquid phase and used to finish the extraction of the analytes. The ionic liquid and sample matrix can be separated by freezing and centrifuging. Several experimental parameters, including amount of extraction solvent, microwave power and irradiation time, pH of sample solution, and ionic strength, were investigated and optimized. Under the optimum experimental conditions, good linearity was observed in the range of 2.00–400.00 μg/L with the correlation coefficients ranging from 0.9995 to 0.9999. The limits of detection for sulfathiazole, sulfachlorpyridazine, sulfamethoxazole, and sulfaphenazole were 0.39, 0.33, 0.62, and 0.85 μg/L, respectively. When the present method was applied to the analysis of environmental water samples, the recoveries of the analytes ranged from 75.09 to 115.78% and relative standard deviations were lower than 11.89%.     

On-line micro-volume introduction system developed for lower density than water extraction solvent and dispersive liquid–liquid microextraction coupled with flame atomic absorption spectrometry

A simple and fast preconcentration/separation dispersive liquid–liquid micro extraction (DLLME) method for metal determination based on the use of extraction solvent with lower density than water has been developed. For this purpose a novel micro-volume introduction system was developed enabling the on-line injection of the organic solvent into flame atomic absorption spectrometry (FAAS). The effectiveness and efficiency of the proposed system were demonstrated for lead and copper preconcentration in environmental water samples using di-isobutyl ketone (DBIK) as extraction solvent. Under the optimum conditions the enhancement factor for lead and copper was 187 and 310 respectively. For a sample volume of 10 mL, the detection limit (3 s) and the relative standard deviation were 1.2 μg L⁻¹ and 3.3% for lead and 0.12 μg L⁻¹ and 2.9% for copper respectively. The developed method was evaluated by analyzing certified reference material and it was applied successfully to the analysis of environmental water samples.     

Determination of carbamates at trace levels in water and cucumber by capillary liquid chromatography

A sensitive and reliable method using capillary HPLC with UV-diode array detection (DAD) has been developed and validated for trace determination of carbamate pesticides in cucumber and environmental water samples. The analytes, including carbofuran, carbaryl, methiocarb, promecarb, benthiocarb and fenoxycarb, present legal residue levels regulated by the EU Council Directive 98/83/EC on drinking water and by the Regulation (EC) No. 396/2005 on vegetables. A previous off-line solid-phase extraction (SPE) procedure was required for preconcentration and sample clean-up. The separation was achieved using a C₁₈ column (150?mm?×?0.5?mm I.D, 5?µm particle size) and a mobile phase consisting of ACN?:?water using gradient mode, with a flow rate of 10?µl min^?1. Taking advantages of the characteristics of capillary HPLC, low volume of sample and solvents were required, achieving limits of detection for the studied compounds ranged from 10.0–29.6?ng l^?1 for water samples and 1.8–5.6?µg kg^?1 for cucumber, using UV-detection. Recoveries studies for fortified samples, at three different concentration levels, were carried out obtaining recoveries ranging from 70.0 to 111.1% and relative standard deviations (RSDs) lower than 10.6%.