Hong Heng See

Determination of triazine herbicides using membrane-protected carbon nanotubes solid phase membrane tip extraction prior to micro-liquid chromatography.

A novel microextraction technique termed solid phase membrane tip extraction (SPMTE) was developed. Selected triazine herbicides were employed as model compounds to evaluate the extraction performance and multiwall carbon nanotubes (MWCNTs) were used as the adsorbent enclosed in SPMTE device. The SPMTE procedure was performed in semi-automated dynamic mode and several important extraction parameters were comprehensively optimized. Under the optimum extraction conditions, the method showed good linearity in the range of 1-100 microg/L, acceptable reproducibility (RSD 6-8%, n=5), low limits of detection (0.2-0.5 microg/L), and satisfactory relative recoveries (95-101%). The SPMTE device could be regenerated and reused up to 15 analyses with no analyte carry-over effects observed. Comparison was made with commercially available solid phase extraction-molecular imprinted polymer cartridge (SPE-MIP) for triazine herbicides as the reference method. The new developed method showed comparable or even better results against reference method and is a simple, feasible, and cost effective microextraction technique.

Electric Field-Driven Extraction of Lipophilic Anions across a Carrier-Mediated Polymer Inclusion Membrane

The use of a cationic carrier-mediated polymer inclusion membrane (PIM) for extraction and preconcentration of anionic model analytes driven by an electric field directly into an aqueous acceptor solution is demonstrated. The optimized membrane was 20 μm thick and consisted of 60% cellulose triacetate as base polymer, 20% o-nitrophenyl octyl ether as plasticizer, and 20% Aliquat 336 as cationic carrier in the perchlorate form. By applying voltages of up to 700 V across the membrane, the lipophilic model analytes propanesulfonate, octanesulfonate, and decanesulfonate could be transported from the aqueous donor solution to the aqueous acceptor solution with efficiences >90% within 5 to 20 min. A preconcentration factor of 26, defined by the volume ratio between donor and acceptor compartments of the current cell design, could be achieved. The utility of the method for analytical applications is demonstrated by extraction of the herbicide glyphosate and its breakdown product aminomethylphosphonic acid from spiked river water, followed by quantification with capillary electrophoresis using contactless conductivity detection. Limits of detection of 0.8 and 1.5 ng/mL were obtained for glyphosate and aminomethylphosphonic acid, respectively.

Rapid and direct determination of glyphosate, glufosinate, and aminophosphonic acid by online preconcentration CE with contactless conductivity detection

Rapid and direct online preconcentration followed by CE with capacitively coupled contactless conductivity detection (CE‐C4D) is evaluated as a new approach for the determination of glyphosate, glufosinate (GLUF), and aminophosphonic acid (AMPA) in drinking water. Two online preconcentration techniques, namely large volume sample stacking without polarity switching and field‐enhanced sample injection, coupled with CE‐C4D were successfully developed and optimized. Under optimized conditions, LODs in the range of 0.01–0.1 μM (1.7–11.1 μg/L) and sensitivity enhancements of 48‐ to 53‐fold were achieved with the large volume sample stacking‐CE‐C4D method. By performing the field‐enhanced sample injection‐CE‐C4D procedure, excellent LODs down to 0.0005–0.02 μM (0.1–2.2 μg/L) as well as sensitivity enhancements of up to 245‐ to 1002‐fold were obtained. Both techniques showed satisfactory reproducibility with RSDs of peak height of better than 10%. The newly established approaches were successfully applied to the analysis of glyphosate, glufosinate, and aminophosphonic acid in spiked tap drinking water.

Dynamic supported liquid membrane tip extraction of glyphosate and aminomethylphosphonic acid followed by capillary electrophoresis with contactless conductivity detection

A dynamic supported liquid membrane tip extraction (SLMTE) procedure for the effective extraction and preconcentration of glyphosate (GLYP) and its metabolite aminomethylphosphonic acid (AMPA) in water has been investigated. The SLMTE procedure was performed in a semi-automated dynamic mode and demonstrated a greater performance against a static extraction. Several important extraction parameters such as donor phase pH, cationic carrier concentration, type of membrane solvent, type of acceptor stripping phase, agitation and extraction time were comprehensively optimized. A solution of Aliquat-336, a cationic carrier, in dihexyl ether was selected as the supported liquid incorporated into the membrane phase. Quantification of GLYP and AMPA was carried out using capillary electrophoresis with contactless conductivity detection. An electrolyte solution consisting of 12 mM histidine (His), 8 mM 2-(N-morpholino)ethanesulfonic acid (MES), 75 microM cetyltrimethylammonium bromide (CTAB), 3% methanol, pH 6.3, was used as running buffer. Under the optimum extraction conditions, the method showed good linearity in the range of 0.01-200 microg/L (GLYP) and 0.1-400 microg/L (AMPA), acceptable reproducibility (RSD 5-7%, n=5), low limits of detection of 0.005 microg/L for GLYP and 0.06 microg/L for AMPA, and satisfactory relative recoveries (90-94%). Due to the low cost, the SLMTE device was disposed after each run which additionally eliminated the possibility of carry-over between runs. The validated method was tested for the analysis of both analytes in spiked tap water and river water with good success.

Rapid separation of fatty acids using a poly(vinyl alcohol) coated capillary in nonaqueous capillary electrophoresis with contactless conductivity detection

The determination of fatty acids by nonaqueous CZE with capacitively coupled contactless conductivity detection was investigated. A new deoxycholate‐based BGE, which had previously been found to give significantly improved baseline stability in the determination of lipophilic organic ammonium ions, was found to be similarly beneficial for the determination of the anions. The use of a PVA‐coated capillary was required for suppression of the EOF and to obtain well reproducible results. The complete separation of 12 fatty acids could be achieved with 10 mM DOC in methanol within 6 min under optimized conditions. The PVA‐coated capillary demonstrated outstanding stability over 300 runs with no sign of depletion of the PVA layer. Method validation showed a good linearity range from 0.75 to 25 μM with correlation coefficients between 0.9949 and 0.9979. The LOD was determined as 0.5 μM for all fatty acids. The developed approach was successfully demonstrated for the separation of free fatty acids in commercial and home‐made edible oil.

Automated Electric-Field-Driven Membrane Extraction System Coupled to Liquid Chromatography−Mass Spectrometry

An automated analyte electroextraction and preconcentration system, which was used as the front end for a liquid chromatography-electrospray mass spectrometry instrument, is described. The extraction was based on driving the anionic analytes across a polymer inclusion membrane by application of a potential of 200 V to the cell. Five milliliters (5 mL) of sample were passed through a flow-through cell at a flow rate of 0.2 mL/min containing a membrane 20 μm thick. This consisted of 75% cellulose triacetate as base polymer, 12.5% of tris(2-ethylhexyl)phosphate as plasticizer, and 12.5% of Aliquat 336 as cationic carrier. The target analytes were enriched in 20 μL of a stagnant acceptor solution prior to online LC/MS analysis. The performance of the system was demonstrated for the determination of chlorinated phenoxyacetic acid herbicides in spiked river water. Enrichment factors of ~200 were achieved with recoveries of typically 99% and precision values of typically 5%. The limit of detection (LOD) values were found to be between 0.03 ng/mL to 0.08 ng/mL.

Development and evaluation of electromembrane extraction across a hollow polymer inclusion membrane

In this work, a new variation of the electromembrane extraction (EME) approach employing a hollow polymer inclusion membrane (HPIM) was developed. In this method, a HPIM was prepared by casting a solution of the desired proportions of cellulose acetate (CTA), tris(2-ethylhexyl)phosphate (TEHP) and di-(2-ethylhexyl)phosphoric acid (D2EHPA) in dichloromethane on glass capillary tubing. Three basic drugs namely amphetamine, methamphetamine, and 3,4-methylenedioxy-N-methylamphetamine (MDMA) were selected as model analytes to evaluate the extraction performance of this new approach. The drugs were extracted from human plasma samples, through a 20μm thickness HPIM, to an aqueous acceptor solution inside the lumen of the hollow membrane. Parameters affecting the extraction efficiency were investigated in detail. Under the optimized conditions, enrichment factors in the range of 97-103-fold were obtained from 3mL of sample solution with a 10min extraction time and an applied voltage of 300V across the HPIM. The detection limits of the method for the three drugs were in the range of 1.0-2.5ng/mL (at a signal/noise ratio of three), with relative standard deviations of between 6.4% and 7.9%. When the method was applied to spiked plasma samples, the relative recoveries ranged from 99.2% to 100.8%. Enrichment factors of 103, 99 and 97 were obtained for amphetamine, methamphetamine, and MDMA, respectively. A comparison was also made between the newly developed approach and EME using supported liquid membranes (SLM) as well as standard sample preparation methods (liquid-liquid extraction) used by the Toxicology Unit, Department of Chemistry, Malaysia.

Electro-driven extraction across a polymer inclusion membrane in a flow-through cell

A flow-through arrangement for electrodriven extraction across a polymer inclusion membrane was developed. Sample introduction into the donor chamber was continuous, while the acceptor solution was stagnant. By adjustment of the total volume of the donor solution pumped through the cell the best compromise between enrichment factor and extraction time can be set. The enriched extract was analyzed by capillary electrophoresis with contactless conductivity detection. Membranes of 20μm thickness were employed which consisted of 60% cellulose triacetate as base polymer, 20% o-nitrophenyl octyl ether as plasticizer, and 20% Aliquat 336. By passing through 10mL of sample at a flow rate of 1mL/min the model analytes glyphosate (a common herbicide) and its major metabolite aminomethylphosphonic acid could be transported from the aqueous donor solution to the aqueous acceptor solution with efficiencies >87% in 10min at an applied voltage of 1500V. Enrichment factors of 87 and 95 and limits of detection down to 43 and 64pg/mL were obtained for glyphosate and aminomethylphosphonic acid, respectively. The intra- and interday reproducibilities for the extraction of the two compounds from spiked river water were about 6 and 7% respectively when new membranes were used for each experiment. For consecutive extractions of batches of river water with a single piece of membrane a deterioration of recovery by about 16% (after 20 runs) was noted, an effect not observed with purely aqueous standards.

Study on the effects of electrolytes and solvents in the determination of quaternary ammonium ions by nonaqueous capillary electrophoresis with contactless conductivity detection

A study on the separation of lipophilic quaternary ammonium cations in NACE coupled with contactless conductivity detection (NACE‐C4D) is presented. The suitability of different salts dissolved in various organic solvents as running electrolytes in NACE‐C4D was investigated. A solvent mixture of methanol/acetonitrile at a ratio of 90%:10% v/v showed the best results. Deoxycholic acid sodium salt as BGE was found to provide exceptional high stability with low baseline noise that leads to highest S/N ratios for the target analytes among all BGEs tested. Under the optimum conditions, capillaries with different internal diameters were examined and an id of 50 μm was found to give best detection sensitivity. The proposed method was validated and showed good linearity in the range from 2.5 to 200 μM, low limits of detection (0.1–0.7 μM) and acceptable reproducibility of peak area (intraday RSD 0.1–0.7%, n = 3; interday RSD 5.9–9.4%, n = 3).

Determination of free and total valproic acid in human plasma by capillary electrophoresis with contactless conductivity detection

A new approach for the determination of free and total valproic acid in small samples of 140 μL human plasma based on capillary electrophoresis with contactless conductivity detection is proposed. A dispersive liquid-liquid microextraction technique was employed in order to remove biological matrices prior to instrumental analysis. The free valproic acid was determined by isolating free valproic acid from protein-bound valproic acid by ultrafiltration under centrifugation of 100 μL sample. The filtrate was acidified to turn valproic acid into its protonated neutral form and then extracted. The determination of total valproic acid was carried out by acidifying 40 μL untreated plasma to release the protein-bound valproic acid prior to extraction. A solution consisting of 10 mM histidine, 10 mM 3-(N-morpholino)propanesulfonic acid and 10 μM hexadecyltrimethylammonium bromide of pH 6.5 was used as background electrolyte for the electrophoretic separation. The method showed good linearity in the range of 0.4-300 μg/mL with a correlation coefficient of 0.9996. The limit of detection was 0.08 μg/mL, and the reproducibility of the peak area was excellent (RSD=0.7-3.5%, n=3, for the concentration range from 1 to 150 μg/mL). The results for the free and total valproic acid concentration in human plasma were found to be comparable to those obtained with a standard immunoassay. The corresponding correlation coefficients were 0.9847 for free and 0.9521 for total valproic acid.