Electro membrane extraction of biological anions with ion chromatographic analysis

A simple and sensitive single step electro membrane extraction (EME) procedure was demonstrated for biological organic anions with determination by ion chromatography (IC). Nitrite, adipate, oxalate, iodide, fumarate, thiocyanate and perchlorate were extracted from aqueous donor solutions, across a supported liquid membrane (SLM) consisting of methanol impregnated in the walls of a porous polypropylene membrane bag and into an alkaline aqueous acceptor solution in the lumen of the propylene envelope by the application of potential of 12 V applied across the SLM. The acceptor solution was analyzed by IC. Parameters affecting the extraction performance such as type of SLM, extraction time, pH of the donor and acceptor solution, and extraction voltage were studied. The most favorable EME conditions were methanol as the SLM, extraction time of 5 min, pH of acceptor and sample solutions of 12 and 4, respectively, and a voltage of 12 V. Portable 12 V batteries were used in the study. Under these optimized conditions, all anions had enrichment factors ranging from 3.6 to 36.2 with relative standard deviations (n = 3) of between 6.6 and 17.5%. Good linearity ranging from 0.1 to 10 μg mL⁻¹ with coefficients of correlation (r) of between 0.9981 and 0.9996 were obtained. The limits of detection of the EME-IC method were from 0.01 to 0.14 μg mL⁻¹. The developed methodology was applied to amniotic fluid samples to evaluate the feasibility of the method for real applications.     

Simple hollow fiber renewal liquid membrane extraction method for pre-concentration of Cd(II) in environmental samples and detection by Flame Atomic Absorption Spectrometry

A hollow fiber renewal liquid membrane (HFRLM) extraction method to determine cadmium (II) in water samples using Flame Atomic Absorption Spectrometry (FAAS) was developed. Ammonium O,O-diethyl dithiophosphate (DDTP) was used to complex cadmium (II) in an acid medium to obtain a neutral hydrophobic complex (ML₂). The organic solvent introduced to the sample extracts this complex from the aqueous solution and carries it over the poly(dimethylsiloxane) (PDMS) membrane, that had their walls previously filled with the same organic solvent. The organic solvent is solubilized inside the PDMS membrane, leading to a homogeneous phase. The complex strips the lumen of the membrane where, at higher pH, the complex Cd-DDTP is broken down and cadmium (II) is released into the stripping phase. EDTA was used to complex the cadmium (II), helping to trap the analyte in the stripping phase. A multivariate procedure was used to optimize the studied variables. The optimized variables were: sample (donor phase) pH 3.25, DDTP concentration 0.05% (m/v), stripping (acceptor phase) pH 8.75, EDTA concentration 1.5 × 10⁻² mol L⁻¹, extraction temperature 40 °C, extraction time 40 min, a solvent mixture N-butyl acetate and hexane (60/40%, v/v) with a volume of 100 μL, and addition of ammonium sulfate to saturate the sample. The sample volume used was 20 mL and the stripping volume was 165 μL. The analyte enrichment factor was 120, limit of detection (LOD) 1.3 μg L⁻¹, relative standard deviation (RSD) 5.5% and the working linear range 2-30 μg L⁻¹.     

Carrier-mediated extraction of bipyridilium herbicides across the hydrophobic liquid membrane

Supported liquid membrane (SLM) method for preconcentration and enrichment of the two bipyridilium herbicides, namely diquat and paraquat, from environmental water samples has been developed. The permanently charged cationic herbicides were extracted from a flowing aqueous solution to a stagnant acidic acceptor solution across a liquid membrane containing 40% (v/v) di-(2-ethylhexyl) phosphoric acid dissolved in di-n-hexyl ether. The mass transfer of analytes is driven by the counter-coupled transport of hydrogen ions from the acceptor to the donor phase. The efficiency of the extraction process depends on the donor solution pH, the amount of the mobile carrier added to the liquid membrane and the concentration of the counter ion in the acceptor solution. The applicability of the method for extraction of these quaternary ammonium herbicides from environmental waters was also investigated by spiking analyte sample solutions in river water. With 24 h sample enrichment concentrations of diquat and paraquat down to ca. 10 ng/L could be detected in environmental waters.     

Simultaneous conduction of two- and three-phase hollow-fiber-based liquid-phase microextraction for the determination of aromatic amines in environmental water samples

This paper describes a simultaneously performed two-/three-phase hollow-fiber-based liquid-phase microextraction (HF-LPME) method for the determination of aromatic amines with a wide range of pK_a (−4.25 to 4.6) and log K_OW (0.9–2.8) values in environmental water samples. Analytes including aniline, 4-nitroaniline, 2,4-dinitroaniline and dicloran were extracted from basic aqueous samples (donor phase, DP) into the microliter volume of organic membrane phase impregnated into the pores of the polypropylene hollow fiber wall, then back extracted into the acidified aqueous solution (acceptor phase, AP) filling in the lumen of the hollow fiber. The mass transfer of the analytes from the donor phase through the organic membrane phase into acceptor phase was driven by both the counter-coupled transport of hydrogen ions and the pH gradient. Afterwards, the hollow fiber was eluted with 50 μL methanol to capture the analytes from both the organic membrane and the acceptor phase. Factors relevant to the enrichment factors (EFs) were investigated. Under the optimized condition (DP: 100 mL of 0.1 M NaOH with 2 M Na₂SO₄; organic phase: di-n-hexyl with 8% trioctylphosphine oxide (TOPO); AP: 10 μL of 8 M HCl; extraction time of 80 min), the obtained EFs were 405–2000, dynamic linear ranges were 5–200 μg/L (R > 0.9976), and limits of detection were 0.5–1.5 μg/L. The presence of humic acid (0–25 mg/L dissolved organic carbon) had no significant effect on the extraction efficiency. The proposed procedure worked very well for real environmental water samples with microgram per liter level of analytes, and good spike recoveries (80–103%) were obtained.     

Optimization of some experimental parameters in the electro membrane extraction of chlorophenols from seawater

An electro membrane extraction (EME) methodology was utilized to study the isolation of some environmentally important pollutants, such as chlorophenols, from aquatic media based upon the electrokinetic migration process. The analytes were transported by application of an electrical potential difference over a supported liquid membrane (SLM). A driving force of 10 V was applied to extract the analytes through 1-octanol, used as the SLM, into a strongly alkaline solution. The alkaline acceptor solution was subsequently analyzed by high performance liquid chromatography-ultraviolet (HPLC-UV) detection. The parameters influencing electromigration, including volumes and pH of the donor and acceptor phases, the organic solvent used as the SLM, and the applied voltage and its duration, were investigated to find the most suitable extraction conditions. Since the developed method showed a rather high degree of selectivity towards pentachlorophenol (PCP), validation of the method was performed using this compound. An enrichment factor of 23 along with acceptable sample clean-up was obtained for PCP. The calibration curve showed linearity in the range of 0.5–1000 ng/mL with a coefficient of estimation corresponding to 0.999. Limits of detection and quantification, based on signal-to-noise ratios of 3 and 10, were 0.1 and 0.4 ng/mL, respectively. The relative standard deviation of the analysis at a PCP concentration of 0.5 ng/mL was found to be 6.8% (n = 6). The method was also applied to the extraction of this contaminant from seawater and an acceptable relative recovery of 74% was achieved at a concentration level of 1.0 ng/mL.     

Multi-element preconcentration of heavy metal ions from aqueous solution by APDC impregnated activated carbon

Ammonium pyrrolidinedithiocarbamate impregnated activated carbon (APDC-AC) has been used for the preconcentration of Cd(II), Cu(II), Ni(II), and Zn(II) from aqueous solution by column solid phase extraction (SPE) technique. Trace metal ions in aqueous solution were quantitatively sorbed onto APDC-AC packed in a SPE column at pH 5.0 with a flow rate of 1.0 mL min⁻¹. The sorbed metals were eluted with 1 M nitric acid in acetone solution at a flow rate of 0.6 mL min⁻¹ and analyzed by flame atomic absorption spectrometry. The effects of sample volume, amount of APDC-AC, volume of eluent and ionic strength of working solution on metal ion recovery have been investigated. The present methodology gave recoveries from 90 to 106% and R.S.D. from 0.6 to 5.5%.     

Rapid estimation of trace organophosphonate used as a scale inhibitor in aqueous systems by reactive pyrolysis-gas chromatography/mass spectrometry

The determination of trace organophosphonates which are used in cooling towers as a scale inhibitor usually involves extraction and/or concentration of the target components prior to analysis. The extracts are analyzed using chromatographic or spectroscopic methods. This methodology is not only cumbersome but also results in poor data quality. This work presents a novel approach for the rapid and sensitive determination of trace amounts of an organophosphonate: 1-hydroxyethylidene-1,1-diphosphonic acid (HEDP) in aqueous solution. This method is based upon reactive pyrolysis-GC/MS in the presence of tetramethyl ammonium hydroxide (TMAH). Approximately 10 μL of the aqueous sample containing a trace amount of HEDP and 1 μL of 25% a methanol TMAH solution was placed in the sample cup. The cup was then dropped into the furnace which was at 350 °C. The heat initiated the hydrolysis of the organophosphonate followed by the methylation of the hydrolysates. Trimethylphosphate (TMP) was detected by GC/MS. The level of TMP is related to the level of the phosphonate, HEDP in the aqueous sample. Using an external standard calibration curve, it was possible to make a rapid estimation of mg/L levels of organophosphate.     

Carbon nanotube reinforced hollow fiber solid/liquid phase microextraction: A novel extraction technique for the measurement of caffeic acid in Echinacea purpurea herbal extracts combined with high-performance liquid chromatography

A new design of hollow fiber solid–liquid phase microextraction (HF-SLPME) was developed for the determination of caffeic acid in medicinal plants samples as Echinacea purpure. The membrane extraction with sorbent interface used in this research is a three-phase supported liquid membrane consisting of an aqueous (donor phase), organic solvent/nano sorbent (membrane) and aqueous (acceptor phase) system operated in direct immersion sampling mode. The multi-walled carbon nanotube dispersed in the organic solvent is held in the pores of a porous membrane supported by capillary forces and sonification. It is in contact with two aqueous phases: the donor phase, which is the aqueous sample, and the acceptor phase, usually an aqueous buffer. All microextraction experiments were supported using an Accurel Q3/2 polypropylene hollow fiber membrane (600 μm I.D., 200 μm wall thicknesses, and 0.2 μm pore size). The experimental setup is very simple and highly affordable. The hollow fiber is disposable, so single use of the fiber reduces the risk of cross-contamination and carry-over problems. The proposed method allows the very effective and enriched recuperation of an acidic analyte into one single extract. In order to obtain high enrichment and extraction efficiency of the analyte using this novel technique, the main parameters were optimized. Under the optimized extraction conditions, the method showed good linearity (0.0001–50 μg/L), repeatability, low limits of detection (0.00005 μg/L) and excellent enrichment (EF = 2108).     

Selective extraction of triazine herbicides from food samples based on a combination of a liquid membrane and molecularly imprinted polymers

A selective extraction technique based on the combination of liquid membrane (microporous membrane liquid–liquid extraction) and molecularly imprinted polymers (MIP) was applied to triazines herbicides in food samples. Simazine, atrazine and propazine were extracted from aqueous food samples through the hydrophobic porous membrane that was impregnated with toluene, which also formed part of the acceptor phase. In the acceptor phase, the compounds were re-extracted onto MIP particles. The extraction technique was optimised for the amount of molecularly imprinted polymers particles in the organic acceptor phase, extraction time, and type of organic acceptor solvent and desorption solvent. An extraction time of 90 min and 50 mg of MIP were found to be optimum parameters. Toluene as the acceptor phase was found to give higher triazines binding onto MIP particles compared to hexane and combinations of diethyl ether and hexane. 90% methanol in water was found to be the best desorption solvent compared to acetonitrile, methanol and water. The selectivity of the technique was demonstrated by extracting spiked lettuce and apple extracts where clean chromatograms were obtained compared to liquid membrane extraction alone or to the microporous membrane liquid–liquid extraction – non-imprinted polymer combination. The MIP showed a certain degree of group specificity and the extraction efficiency in lettuce extract was 79% (0.72) for simazine, 98% (1.55) for atrazine and 86% (3.08) for propazine.     

Liquid-phase microextraction in a microfluidic-chip – High enrichment and sample clean-up from small sample volumes based on three-phase extraction

In this work, a microfluidic-chip based system for liquid-phase microextraction (LPME-chip) was developed. Sample solutions were pumped into the LPME-chip with a micro-syringe pump at a flow rate of 3–4 μL min⁻¹. Inside the LPME chip, the sample was in direct contact with a supported liquid membrane (SLM) composed of 0.2 μL dodecyl acetate immobilized in the pores of a flat membrane of polypropylene (25 μm thickness). On the other side of the SLM, the acceptor phase was present. The acceptor phase was either pumped at 1 μL min⁻¹ during extraction or kept stagnant (stop-flow). Amitriptyline, methadone, haloperidol, loperamide, and pethidine were selected as model analytes, and they were extracted from alkaline sample solution, through the SLM, and into 10 mM HCl or 100 mM HCOOH functioning as acceptor phase. Subsequently, the acceptor phase was either analyzed off-line by capillary electrophoresis for exact quantification, or on-line by UV detection or electrospray ionization mass spectrometry for time profiling of concentrations. The LPME-chip was found to be highly effective, and extraction efficiencies were in the range of 52–91%. When the flow of acceptor phase was turned off during extraction (stop-flow), analyte enrichment increased linearly with the extraction time. After 10 min as an example, amitriptyline was enriched by a factor of 42 from only 30 μL sample solution, and after 120 min amitriptyline was enriched by a factor of 500 from 320 μL sample solution. This suggested that the LPME-chip has great potentials for very efficient analyte enrichments from limited sample volumes in the future.     

Electromembrane extraction (EME) and HPLC determination of non-steroidal anti-inflammatory drugs (NSAIDs) in wastewater samples

In this paper, an electromembrane extraction (EME) combined with a HPLC procedure using diode array (DAD) and fluorescence detection (FLD) has been developed for the determination of six widely used non-steroidal anti-inflammatory drugs (NSAIDs): salicylic acid (SAC), ketorolac (KTR), ketoprofen (KTP), naproxen (NAX), diclofenac (DIC) and ibuprofen (IBU). The drugs were extracted from basic aqueous sample solutions, through a supported liquid membrane (SLM) consisting of 1-octanol impregnated in the walls of a S6/2 Accurel^® polypropylene hollow fiber, and into a basic aqueous acceptor solution resent inside the lumen of the hollow fiber with a potential difference of 10 V applied over the SLM. Extractions that were carried out in 10 min using a potential of 10 V from pH 12 NaOH aqueous solutions shown concentration enrichments factors of 28-49 in a pH 12 NaOH aqueous acceptor solution. The proposed method was successfully applied to urban wastewaters. Excellent selectivity was demonstrated as no interfering peaks were detected. The procedure allows very low detection and quantitation limits of 0.0009-9.0 and 0.003-11.1 μg L⁻¹, respectively.     

Exhaustive extraction of peptides by electromembrane extraction

This fundamental work illustrates for the first time the possibility of exhaustive extraction of peptides using electromembrane extraction (EME) under low system-current conditions (<50 μA). Bradykinin acetate, angiotensin II antipeptide, angiotensin II acetate, neurotensin, angiotensin I trifluoroacetate, and leu-enkephalin were extracted from 600 μL of 25 mM phosphate buffer (pH 3.5), through a supported liquid membrane (SLM) containing di-(2-ethylhexyl)-phosphate (DEHP) dissolved in an organic solvent, and into 600 μL of an acidified aqueous acceptor solution using a thin flat membrane-based EME device. Mass transfer of peptides across the SLM was enhanced by complex formation with the negatively charged DEHP. The composition of the SLM and the extraction voltage were important factors influencing recoveries and current with the EME system. 1-nonanol diluted with 2-decanone (1:1 v/v) containing 15% (v/v) DEHP was selected as a suitable SLM for exhaustive extraction of peptides under low system-current conditions. Interestingly, increasing the SLM volume from 5 to 10 μL was found to be beneficial for stable and efficient EME. The pH of the sample strongly affected the EME process, and pH 3.5 was found to be optimal. The EME efficiency was also dependent on the acceptor solution composition, and the extraction time was found to be an important element for exhaustive extraction. When EME was carried out for 25 min with an extraction voltage of 15 V, the system-current across the SLM was less than 50 μA, and extraction recoveries for the model peptides were in the range of 77–94%, with RSD values less than 10%.     

Nano-electromembrane extraction

The present work has for the first time described nano-electromembrane extraction (nano-EME). In nano-EME, five basic drugs substances were extracted as model analytes from 200 μL acidified sample solution, through a supported liquid membrane (SLM) of 2-nitrophenyl octyl ether (NPOE), and into approximately 8 nL phosphate buffer (pH 2.7) as acceptor phase. The driving force for the extraction was an electrical potential sustained over the SLM. The acceptor phase was located inside a fused silica capillary, and this capillary was also used for the final analysis of the acceptor phase by capillary electrophoresis (CE). In that way the sample preparation performed by nano-EME was coupled directly with a CE separation. Separation performance of 42,000–193,000 theoretical plates could easily be obtained by this direct sample preparation and injection technique that both provided enrichment as well as extraction selectivity. Compared with conventional EME, the acceptor phase volume in nano-EME was down-scaled by a factor of more than 1000. This resulted in a very high enrichment capacity. With loperamide as an example, an enrichment factor exceeding 500 was obtained in only 5 min of extraction. This corresponded to 100-times enrichment per minute of nano-EME. Nano-EME was found to be a very soft extraction technique, and about 99.2–99.9% of the analytes remained in the sample volume of 200 μL. The SLM could be reused for more than 200 nano-EME extractions, and memory effects in the membrane were avoided by effective electro-assisted cleaning, where the electrical potential was actively used to clean the membrane.     

Quantitation of atorvastatin in human plasma using directly suspended acceptor droplet in liquid-liquid-liquid microextraction and high-performance liquid chromatography-ultraviolet detection

A simple and sensitive methodology based on liquid-liquid-liquid microextraction (LLLME) followed by high-performance liquid chromatography-ultraviolet detection (HPLC-UV) has been successfully developed for the determination of atorvastatin (AT) in human plasma. AT was first extracted from 4.5 mL acidic aqueous sample (diluted plasma, donor phase, pH 1) at temperature 45 °C through 400 μL 1-octanol for 4.5 min, while being agitated by a stirring bar at 1250 rpm. Then, a 5.5 μL free suspended basic aqueous droplet (acceptor phase, pH 10) was delivered to the top-center position of the organic membrane. The mixture was stirred at 650 rpm for 7.5 min and the analyte was back-extracted into the droplet. Finally, the acceptor phase was taken into a microsyringe and injected directly into the HPLC. An enrichment factor of 187 along with substantial sample clean up was obtained under the optimized conditions. The calibration curve showed linearity in the range of 1-500 ng mL⁻¹ with regression coefficient corresponding to 0.996. Limits of detection (S/N = 3) and quantification (S/N = 10) were 0.4 and 1 ng mL⁻¹, respectively. A reasonable relative recovery (91%) and satisfactory intra-assay (4.4-7.0%, n = 6) and inter-assay (4.9-7.7%, n = 8) precision illustrated good performance of the analytical procedure. This technique was eventually applied for the determination of AT in human plasma after oral administration of 40 mg single dose of drug. The protocol proved to be highly cost-effective and reliable for the screening purpose.     

Flow-through solid-phase energy transfer-room temperature phosphorescence for orthophosphate determinations at trace levels

The development of a flow-through solid-phase room temperature phosphorescence (RTP) method for the sensitive determination of orthophosphate in aqueous samples, based on the energy transfer from a phosphor molecule (acting as a donor) to an orthophosphate dye-indicator (acting as an acceptor) is described.The proposed method, to our knowledge the first RTP optosensor for orthophosphate developed so far, is based on the injection in a flow system of 1 ml sample treated to form phosphomolybdenum blue from the orthophosphate. After injection, the phosphomolybdenum blue is on-line co-immobilised onto a polymeric resin containing adsorbed erythrosine B. This selected donor molecule exhibits strong RTP in a de-oxygenated aqueous media when retained on the surface of polymeric resin beads. Absorption spectra of the phosphomolybdenum blue possess a desirable spectral overlap with the emission spectra of the RTP donor and a non-radiative energy transfer occurs from the phosphor molecule to the acceptor dye. An increase in the concentration of orthophosphate of the solution causes an absorption increase of the acceptor (phosphomolybdenum blue) and, therefore, an increase in the energy transfer, which brings about a decrease of the RTP emission. After measurement, the active sensing phase can be regenerated by passing 2 ml of 2 M sodium hydroxide plus 2 ml of methanol. After the injection of 1 ml of 2×10⁻⁶ M erythrosine B the system is prepared again for a new sample injection.Potential interferences by ions present in natural waters, which could affect the optosensor response, and analytical performance characteristics of the RTP method are discussed in detail. An orthophosphate detection limit of 0.5 ng ml⁻¹ (for 1 ml sample injection volume) was achieved. Finally, the selected RTP flow-through optical sensor has been successfully tested for the determination of orthophosphate in different water samples at a very few ng ml⁻¹ levels.     

Focused microwave-assisted solvent extraction and HPLC determination of effective constituents in Eucommia ulmodies Oliv. (E. ulmodies)

A new focused microwave-assisted solvent extraction method using water as solvent has been developed for leaching geniposidic and chlorogenic acids from Eucommia ulmodies Oliv. The extraction procedures were optimized using a two indexes orthogonal experimental design and graphical analysis, by varying irradiation time, solvent volume, solvent composition and microwave power. The optimum extraction conditions were obtained: for geniposidic acid, 50% micorwave power, 40 s irradiation, and 80% (v/v) aqueous methanol as extraction solvent (20 ml g⁻¹ sample); and for chlorogenic acid, 50% micorwave power, 30 s irradiation, and 20% aqueous methanol (20 ml g⁻¹ sample). The composition of the extraction solvent was optimized and can be directly used as the mobile phase in the HPLC separation. Quantification of organic acids was done by HPLC at room temperature using Spherigel C₁₈ chromatographic column (, i.d. 5 μm), the methanol:water:acetic acid (20:80:1.0, v/v) mobile phase and UV detection at 240 nm. The R.S.D. of the extraction process for geniposidic and chlorogenic acid were 3.8 and 4.1%, respectively.     

Micro-porous membrane liquid-liquid extraction as an enrichment step prior to nonaqueous capillary electrophoresis determination of sulfonylurea herbicides

A method based on micro-porous membrane liquid-liquid extraction (MMLLE) enrichment and nonaqueous capillary electrophoresis (CE) separation, was established for the analysis of sulfonylurea herbicides in water samples. After MMLLE, the analyte trapped in the chloroform was treated mildly with nitrogen flow to dryness and then dissolved in 200 μl of 4 mM Tris methanol solution for CE analysis. Five sulfonylurea herbicides were separated by nonaqueous CE with Tris/acetate of methanol solution as the run buffer. MMLLE related parameters such as organic solvent used as acceptor, sample flow rate, sample pH, enrichment time, and salt effect were investigated with tribenuron methyl (TBM) as a model compound. Results showed that with a sample flow rate of 3.0 ml min⁻¹ and an enrichment time of 20 min, the proposed method has good linear relationship over the scope of 1-15 ng ml⁻¹ with related coefficient of R²=0.9911, and a detection limit of 0.4 ng ml⁻¹. This method was applied to determine TBM in realworld water samples with recoveries over the range of 89-97%.     

Drop-to-drop microextraction across a supported liquid membrane by an electrical field under stagnant conditions

Electromembrane extraction (EME) of basic drugs from 10 μL sample volumes was performed through an organic solvent (2-nitrophenyl octyl ether) immobilized as a supported liquid membrane (SLM) in the pores of a flat polypropylene membrane (25 μm thickness), and into 10 μL 10 mM HCl as the acceptor solution. The driving force for the extractions was 3–20 V d.c. potential sustained over the SLM. The influence of the membrane thickness, extraction time, and voltage was investigated, and a theory for the extraction kinetics is proposed. Pethidine, nortriptyline, methadone, haloperidol, and loperamide were extracted from pure water samples with recoveries ranging between 33% and 47% after only 5 min of operation under totally stagnant conditions. The extraction system was compatible with human urine and plasma samples and provided very efficient sample pretreatment, as acidic, neutral, and polar substances with no distribution into the organic SLM were not extracted across the membrane. Evaluation was performed for human urine, providing linearity in the range 1–20 μg/mL, and repeatability (RSD) in average within 12%.     

Determination of linear alkylbenzene sulfonates by ion-pair solid-phase extraction and high-performance liquid chromatography

In this paper, the potential use of multiwalled carbon nanotubes (MWCNTs) as solid phase extraction (SPE) adsorbent was evaluated for preconcentration of linear alkylbenzene sulfonates (LAS) using ion-pair (IP)-SPE with tetrabutylammonium hydroxide (TBAH). The LAS homologues present in the aqueous sample were ion-paired with TBAH and the solution was passed through the MWCNT cartridges. The analytes retained in the cartridge were eluted with methanol and the concentrated methanol extract was analysed by HPLC-UV. In order to obtain the satisfactory recovery of LAS homologues, various parameters including the type and amount of the ion-pair reagents, the desorption and enrichment conditions such as the effect of eluent and its volume, pH, the flow rate, the ultrasonic time of sample, and the volume of sample solution were systematically optimized. Under the optimal conditions, LAS homologues could be easily extracted by the proposed SPE cartridge. The favorable limits of detection (LOD) for LAS homologues were in the range from 0.02 to 0.03 μg L⁻¹, and the relative standard deviations (RSDs) were 1.55-2.54% for 10 μg L⁻¹ LAS (n = 6). The proposed method has been successfully applied for the analysis of LAS homologues in aqueous environmental samples. A comparison study with ion-pair solid extraction on MWCNTs, C8 and C18 as adsorbents for LAS demonstrated that ion pair-based solid extraction on MWCNTs adsorbent was advantageous over C8 and C18, the widely used traditional adsorbents.     

A simple novel configuration for in-vial microporous membrane liquid–liquid extraction

A novel arrangement for microporous membrane liquid–liquid extraction from the aqueous donor phase to the organic acceptor phase within a micro-vial, which is compatible with the chromatograph autosampler is presented. The device consisted of a stoppered glass micro-vial containing the organic solvent where the septum of the screw stopper was replaced by a sized piece of membrane which is hermetically assembled to the volumetric flask containing the aqueous donor solution. The placement of the membrane in alternative contact with the solutions was achieved by orbital agitation. As a preliminary study, 2-ethylhexyl 4-(dimethylamino)benzoate has been determined (limit of quantification 0.11 μg L⁻¹, precision 7.4%). The small quantity of organic solvent used, the achieved sample cleanup, and the minimal handling and risk of cross-contamination are significant operational advantages.