Headspace‐single drop microextraction with a commercial capillary electrophoresis instrument

Automated coupling of headspace‐single drop microextraction (HS‐SDME) and CE has been demonstrated using a commercial CE instrument. When a drop hanging at the inlet tip of a capillary for CE is used as the acceptor phase, HS‐SDME becomes a simple but powerful sample pretreatment technique for CE before injection to facilitate sample cleanup and enrichment. By combining HS‐SDME with an on‐line sample preconcentration technique, large volume sample stacking using an electroosmotic flow pump, the sensitivity can be improved further. The overall enrichment factors for phenolic compounds were from 1900 to 3400. HS‐SDME large volume sample stacking using an electroosmotic flow pump was successfully applied to a red wine sample to obtain an LOD of 4 nM (0.8 ppb) for 2,4,6‐trichlorophenol which is a precursor for 2,4,6‐trichloroanisole causing the foul odor in wine called cork taint.     

In-line coupling of two-phase single drop microextraction and large volume stacking using an electroosmotic flow pump in nonaqueous capillary electrophoresis

In order to improve the concentration sensitivity of capillary electrophoresis (CE), two sample preconcentration techniques, single drop microextraction (SDME) and large volume stacking using an electroosmotic flow pump (LVSEP), were coupled in-line in a commercial CE instrument. By simple programming of liquid handling sequences, a pentanol drop was prepared at the tip of a fused silica capillary over which a Teflon tube had been sleeved to serve as a hydrophobic support. After extraction of the analytes from an aqueous donor solution into the drop, the entire capillary column was filled with enriched pentanol extract. LVSEP, in which the sample matrix is automatically removed by the EOF, was then carried out using a methanolic run buffer. The overall enrichment factors for the analytes pentachlorophenol (PCP), 3-bromobenzoic acid (3-BBA), and 4-iodobenzoic acid (4-IBA), from a combination of 30 min SDME and LVSEP on a 27 cm capillary, were about 7000, even without agitation of the donor solution. The resulting limits of detection for PCP, 3-BBA, and 4-IBA were 0.7, 0.3 and 0.7 nM, respectively. Since no modification of the existing CE instrument is necessary and a bare capillary is used for LVSEP, this scheme can be adapted quite easily for many CE applications that require high concentration sensitivity.     

Double sample preconcentration by in‐line coupled large volume single drop microextraction and sweeping in capillary electrophoresis

Single drop microextraction (SDME) is a convenient and powerful preconcentration method for CE before injection. By simple combination of sample‐handling sequences without modification of the CE apparatus, a drop of an aqueous acceptor phase covered with a thin organic layer was formed at the tip of a capillary; 10 min SDME of fluorescein and 6‐carboxyfluorescein from a donor phase of pH 1 to an acceptor phase of pH 9 provided 110‐fold enrichments without stirring the donor phase. To improve the concentration effect further, SDME was coupled with an on‐line (after injection) sample preconcentration method, sweeping, in which analytes in a long sample zone are accumulated at the boundary of a pseudostationary phase penetrating into the sample zone. It is thus necessary to inject a sample of much larger volume than that of a drop in typical SDME. A Teflon sleeve over the capillary inlet allowed a large volume drop to be held stably during extraction. By in‐line coupling 10 min SDME and sweeping of a 30 nL sample using a cationic surfactant dodecyltrimethylammonium, enrichment factors of the double preconcentration were increased up to 32 000.     

Sensitive analysis of amino acids with carrier-mediated single drop microextraction in-line coupled with capillary electrophoresis

In order to analyze amino acids sensitively without derivatization, we have developed carrier-mediated single drop microextraction (SDME). Nonane-1-sulfonic acid was added to an acidic sample donor solution as a carrier to form neutral ion pair complexes with amino acids. The ion pair complexes were extracted to the organic phase, covering a drop of an aqueous basic acceptor phase hanging at the tip of a capillary, and then back-extracted to the basic acceptor phase, where both the amino acids and the carrier have negative charges and the ion pair complexes are broken. The resulting extract of enriched amino acids was injected into the capillary and analyzed by capillary electrophoresis. With 20-min SDME with agitation of the donor phase, enrichment factors of four aromatic amino acids were up to 120-fold, yielding the LOD of 70-500 nM. The linear dynamic ranges for corrected peak areas were 1-100 μM with linear correlation coefficients larger than 0.9959. With internal standardization, the intraday RSDs of migration times and corrected peak areas were 0.01-0.04% and 2.0-3.7%, respectively. The capabilities of sample cleanup including desalting and preconcentration of carrier-mediated SDME were demonstrated with the analysis of human urine after minimal pretreatment of acidification and centrifugation.     

Highly sensitive chiral analysis of amino acids by in-line single drop microextraction and capillary electrophoresis with laser-induced fluorescence detection

A highly sensitive method for chiral analysis of amino acids by in-line single drop microextraction (SDME) and chiral capillary electrophoresis (CE) with laser-induced fluorescence (LIF) detection was developed. In SDME, a drop of a basic aqueous acceptor phase covered with a thin organic layer was formed at the tip of a capillary by simple combination of sample-handling sequences of a CE apparatus. Then fluorescein isothiocyanate (FITC)-derivatized amino acids in an acidic donor solution were enriched into the drop through the organic layer. The enriched enantiomers were then resolved using a dual chiral selector of β-cyclodextrin (β-CD) and sodium taurodeoxycholate (STC). Here, in addition to serving as a labeling reagent providing high fluorescence signal, hydrophobic FITC was primarily used as a modifier aiding the extraction of zwitterionic amino acids by blocking the amino groups and increasing the hydrophobicity, yielding 220 times increase in extraction efficiency. Several hundred-fold enrichments were achieved with 10 min SDME, yielding LODs of 30-60 pM and enabling direct analysis of d-AAs in a 99% enantiomeric excess mixture. In view of no additional modification of the existing commercial CE instrument, this method without stirring can be easily realized using known operations. When a microstirrer was customized to the CE instrument several thousand-fold enrichments could be obtained with LODs in the low picomolar range of 1-3 pM.     

Selective preconcentration of amino acids and peptides using single drop microextraction in-line coupled with capillary electrophoresis

Single drop microextraction (SDME) can be in-line coupled with capillary electrophoresis by attaching a drop to the tip of a capillary. With a 2-layer drop comprised of an aqueous basic acceptor phase covered with a thin organic layer, acidic analytes in an aqueous acidic donor phase can be extracted into the organic layer and then back-extracted into the acceptor phase. However, preconcentration of amino acids and peptides by SDME is difficult since their zwitterionic properties prevent them from being partitioned in the middle organic phase. When amino acids were derivatized with 4-fluoro-7-nitro-2,1,3-benzoxadiazole (NBD-F), amino acids without a charged side chain were converted to carboxylic acids. In the acidic donor phase, those NBD-amino acids were predominantly neutral and they were successfully concentrated into the basic acceptor phase. In the meantime, amino acids with a charged side chain after NBD-F derivatization were not concentrated via SDME. With this selective SDME, we were able to extract acidic and neutral amino acids obtaining several hundred-fold enrichments within 5 min at 25 °C, while leaving basic amino acids—Arg, Lys, and His—in the acidic donor phase. Furthermore, detection sensitivity was enhanced by employing laser-induced fluorescence detection. We then applied this technique to the selective concentration of peptides.     

Improving the sensitivity of the determination of ceftiofur by capillary electrophoresis in environmental water samples: in-line solid phase extraction and sample stacking techniques

This paper describes two different approaches for increasing the sensitivity for the analysis of ceftiofur by capillary electrophoresis (CE). Two different techniques based on the introduction of an enlarged volume of sample, namely large volume sample stacking (LVSS) and in-line solid phase extraction (SPE) were studied and compared. LVSS allowed the on-column electrophoretic preconcentration of ceftiofur without modification of the separation capillary. In-line SPE-CE was developed by using a home-made microcartridge that was filled with a reversed-phase sorbent (C₁₈). The microcartridge was coupled in-line near the inlet of the separation capillary. LVSS and in-line SPE-CE allowed automated operation and improved sensitivity for the analysis of ceftiofur with respect to conventional CE. When environmental water samples were analyzed, an additional pretreatment step based on off-line SPE was necessary in both cases to further decrease the detection limits. In terms of sensitivity for the determination of ceftiofur in river water samples, the combination of off-line SPE with in-line SPE-CE was found the most sensitive with a detection limit of 10 ng L⁻¹, whereas the method based on the use of off-line SPE with LVSS presented a detection limit of 100 ng L⁻¹.     

A glance at achievements in the coupling of headspace and direct immersion single‐drop microextraction with chromatographic techniques

The present article offers a glance at achievements in single‐drop microextraction(SDME), with a focus on the two most commonly used modes of this technique: headspace and direct immersion. Factors affecting SDME, such as the pH and ionic strength of the sample solution, the stirring rate, and the extraction time are briefly summarized. The requirements for the acceptor phase and the influence of the sampling temperature are presented. In addition, the potential of the application of microwave and ultrasonic energy in SDME is also discussed. Examples of the application of the headspace and direct immersion modes of SDME are given in a table as additional Supporting Information.     

Headspace single-drop microextraction with in-drop derivatization and capillary electrophoretic determination for free cyanide analysis

A new method involving headspace single-drop microextraction (SDME) with in-drop derivatization and CE is developed for the preconcentration and determination of free cyanide. An aqueous microdrop (5 microL) containing Ni(II)-NH(3) (as derivatization agent), sodium carbonate and ammonium pyromellitate (as internal standard) was used as the acceptor phase. The extracted cyanide forms a stable Ni(CN)(4) (2-) complex which is then determined by CE. Common experimental parameters (sample and acceptor phase pH, extraction temperature, extraction time and sample ionic strength) affecting the extraction efficiency were investigated. Using headspace SDME, free cyanide can be effectively extracted from the neutral solutions, i.e. without the acidification of the sample which often is prone to errors due to incomplete liberation and artefactual cyanide production. Proposed SDME-CE method provided about 58-fold enrichment in 20 min. The calibration curve was linear for concentrations of CN(-) in the range from 0.25 to 20 micromol/L (R(2) = 0.997). The LOD (S/N = 3) was estimated to be 0.08 micromol/L of CN(-). Such a detection sensitivity is high enough for free cyanide determination in common environmental and physiological samples. Finally, headspace SDME was applied to determine free cyanide in human saliva and urine samples with spiked recoveries in the range of 91.7-105.6%. The main advantage of this method is that sample clean-up, preconcentration and derivatization procedures can be completed in a single step. In addition, the proposed technique does not require any sample pretreatment and thus is much less susceptible to interferences compared to existing methods.     

Simultaneous determination of serotonin and creatinine in urine by combining two ultrasound-assisted emulsification microextractions with on-column stacking in capillary electrophoresis

This article describes the development of a rapid, simple, and sensitive analytical approach for the simultaneous determination of serotonin (5‐hydroxytryptamine) and creatinine in urine samples by combining two ultrasound‐assisted emulsification microextractions (USAEMEs) in series with on‐column stacking in CE. This serial USAEME procedure comprises analytes extraction from the donor solution (urine with K₂CO₃ additive) to an organic solvent followed by a back‐extraction from the organic phase into a small volume of hydrochloric acid. After 15 min of sample pretreatment, the acidic acceptor solution was analyzed directly on CE in the mode of capillary zone electrophoresis. The adoption of HCl as the acceptor phase not only provided effective back‐extraction but also facilitated pH‐mediated on‐column stacking in CE analysis. About 360‐fold sensitivity enhancement was achieved for serotonin detection. The limits of detection were 7.9 nM for serotonin and 13.3 μM for creatinine, respectively. Satisfactory results were obtained with respect to precision and recovery. The proposed method has been demonstrated to be convenient and effective for the analysis of real urine samples. We believe that two USAEMEs in series will find wide applications in simplified sample pretreatment prior to CE analysis.     

Recent development in liquid phase microextraction for determination of trace level concentration of metals—A review

As the drive towards green extraction methods has gained momentum in recent years, it has not always been possible to eliminate organic solvents completely. However, the volumes employed have been reduced remarkably, so that a single microdrop is sufficient in some cases. This effort has led to the development of various liquid phase microextractions namely single drop microextraction (SDME), hollow fiber liquid phase microextraction (HF-LPME), dispersive liquid-liquid microextraction (DLLME) and solidified floating organic drop microextraction (SFODME). In this review, the historical development and overview of these miniaturized liquid phase extraction methodologies have briefly been discussed and a comprehensive collection of application of the these methods in combination with different analytical techniques for preconcentration and determination of ultra trace amounts of metals and organometal ions in various matrices have been summarized.     

On-line coupling of ionic liquid-based single-drop microextraction with capillary electrophoresis for sensitive detection of phenols

An ionic liquid-based single-drop microextraction (IL-SDME) procedure using IL as an extractant on-line coupled to capillary electrophoresis (CE) is proposed. The method is capable of quantifying trace amounts of phenols in environmental water samples. For the SDME of three phenols, a 2.40 nL IL microdrop was exposed for 10 min to the aqueous sample and then was directly injected into the capillary column for analysis. Extraction parameters such as the extraction time, the IL single-drop volume, pH of the sample solution, ionic strength, volume of the sample solution and the extraction temperature were systematically investigated. Detection limits to three phenols were less than 0.05 μg mL⁻¹, and their calibration curves were all linear (R² ≥ 0.9994) in the range from 0.05 to 50 μg mL⁻¹. And enrichment factors for three phenols were 156, 107 and 257 without agitation, respectively. This method was then utilized to analyze two real environmental samples from Yellow River and tap water, obtaining satisfactory results. Compared with the usual SDME for CE, IL-SDME–CE is a simple, low-cost, fast and environmentally friendly preconcentration technique.     

Ionic liquid‐based headspace in‐tube liquid‐phase microextraction coupled with CE for sensitive detection of phenols

An ionic liquid‐based headspace in‐tube liquid‐phase microextraction (IL‐HS‐ITLPME) in‐line coupled with CE is proposed. The method is capable of quantifying trace amounts of phenols in environmental water samples. In the newly developed method, simply by placing a capillary injected with ionic liquids (IL) in the HS above the aqueous sample, volatile phenols were extracted into the IL acceptor phase in the capillary. After extraction, electrophoresis of the phenols in the capillary was carried out. Extraction parameters such as the extraction time, extraction temperature, ionic strength, volume of the sample solution, and IL types were systematically investigated. Under the optimized conditions, enrichment factors for four phenols were from 1510 to 1985. The proposed method provided a good linearity, low limits of detection (below 5.0 ng/mL), and good repeatability of the extractions (RSDs below 6.7%, n = 6). This method was then utilized to analyze two real environmental samples of Xiaoxi Lake and tap water, obtaining acceptable recoveries and precisions. Compared with the usual HS‐ITLPME for CE, IL‐HS‐ITLPME‐CE is a simple, low cost, fast, and environmentally friendly preconcentration technique.     

Selective extraction of alkaloids in human urine by on-line single drop microextraction coupled with sweeping micellar electrokinetic chromatography

A novel method of on-line single drop microextraction (SDME) coupled with sweeping micellar electrokinetic chromatography (MEKC) for the selective extraction and dual preconcentration of alkaloids was developed. In this technique, analytes of three alkaloids were firstly extracted from 4.0 mL basic aqueous sample solution (donor phase, 500 mM NaOH) into a layer of n-octanol at temperature 30 °C with the stirring rate of 1150 rpm, then back-extracted into the acidified aqueous acceptor (acceptor phase, 50 mM H₃PO₄) suspended at the tip of a capillary at 650 rpm. Then, the aqueous acceptor was introduced into capillary by hydrodynamic injection with a height difference of 15 cm between the inlet and outlet of capillary for 300 s, and analyzed directly by on-line sweeping MEKC. With the selective SDME, we were able to extract three alkaloids without any interfering components in human urine samples. Under the optimum conditions, the proposed method achieved limits of detections (LOD) of between 0.2 ng mL⁻¹ and 1.5 ng mL⁻¹ with 1583–3556-fold increases in detection sensitivity for three analytes, which indicated that it was a promising method for analysis of alkaloids in human urine.     

Novel approach to improve the detection of colchicine via online coupling of ionic liquid-based single-drop microextraction with capillary electrophoresis

A novel approach based on ionic liquid‐single‐drop microextraction (IL‐SDME) online coupling with capillary electrophoresis (CE) was used to determine a toxic alkaloid – colchicine. The IL‐SDME procedure was optimized by extraction solvent, drop volume controlling, sample volume and pH, extraction time, and ionic strength. Under optimum conditions, enrichment factor was as much as 41‐fold with a relative standard deviation of 2.8% (n=3). Linear range of response was observed from 1 to 100 μg/mL, with detection limit of 0.25 μg/mL and correlation coefficient (R²) of 0.9994. The extraction of colchicine from spiked Lanzhou lily sample was performed and obtaining good result with an average recovery rate of 102.4 and 98.8% at 5 and 50 μg/mL, respectively. Comparing with the previous methods, IL‐SDME‐CE is really a convenient, economical, and environmentally benign way for determining colchicine.     

Single‐drop microextraction combined in‐line with capillary electrophoresis for the determination of nonsteroidal anti‐inflammatory drugs in urine samples

This study describes a method to determine nonsteroidal anti‐inflammatory drugs (NSAIDs) in urine samples based on the use of single‐drop microextraction (SDME) in a three‐phase design as a preconcentration technique coupled in‐line to capillary electrophoresis. Different parameters affecting the extraction efficiency of the SDME process were evaluated (e.g. type of extractant, volume of the microdroplet, and extraction time). The developed method was successfully applied to the analysis of human urine samples with LODs ranging between 1.0 and 2.5 μg/mL for all of the NSAIDs under study. This method shows RSD values ranging from 8.5 to 15.3% in interday analysis. The enrichment factors were calculated, resulting 27‐fold for ketoprofen, 14‐fold for diclofenac, 12‐fold for ibuprofen, and 44‐fold naproxen. Samples were analyzed applying the SDME–CE method and the obtained results presented satisfactory recovery values (82–115%). The overall method can be considered a promising approach for the analysis of NSAIDs in urine samples after minimal sample pretreatment.     

Large volume sample stacking of cationic tetracycline antibiotics toward 10 ppb level analysis by capillary electrophoresis with UV detection

This paper aimed to build up a sensitive CE method for the analysis of tetracyclines (TCs) antibiotics (including tetracycline, chlorotetracycline, oxytetracycline, and doxycycline) with conventional UV detection. Here, the large volume sample stacking was applied to achieve in capillary preconcentration of the targets. To achieve large volume sample stacking, the essential step was a large volume of sample (around 83.3% of total capillary length from inlet to detection window) hydrodynamically loaded. Then, the reserved voltage was added in order to push the sample matrix out of the capillary. Due to different pH between sample solution (pH 4.6) and BGE (pH 11.0), the cationic TCs would turn into negatively charged while the sample matrix was removing from the capillary. Finally, the anionic TCs were stacked at the inlet for the subsequent separation. Although the loss of sample existed during their charge transformation, the LODs could be improved around 40 times than that obtained by normal hydrodynamic injection CE method. Here, the LODs were in the range of 8.1–14.5 μg/L, around 10 ppb that close to the level by electrochemiluminescence or laser‐induced fluorescence detection of TCs by CE. The precision was characterized by RSDs of migration times and peak areas, which were in the range of 0.19–0.24% and 0.97–2.54%, respectively. The recoveries of the developed method were in the range of 95–112% by spiking TCs in the tap water. The proposed inline preconcentration CE method could be a simple, speed, and sensitive method for the quantitative analysis of TCs.     

三相中空纤维式液相微萃取用于快速富集血浆中的尼古丁

建立了一种以三相中空纤维式液相微萃取(TP-HF-LPME)进行样品前处理,采用高效液相色谱快速、准确测定血浆中尼古丁含量的方法。研究表明该方法集萃取、富集、净化为一步,极大地简化了传统血浆成分测定的前处理过程,是一种快速、有效、绿色的前处理方法。方法的线性范围为0.1～50 mg/L,相关系数(r2)为0.9996,检测限为0.05 mg/L (信噪比为3),相对标准偏差小于5%。     

Application of single-drop microextraction coupled with gas chromatography for the determination of multiclass pesticides in vegetables with nitrogen phosphorus and electron capture detection

In the present work the single-drop microextraction (SDME) technique coupled with GC-NPD and GC-ECD was evaluated for the determination of multi-class pesticides in vegetables. The donor sample solution preparation was optimized by testing different mixtures of solvents and dilutions with water. The SDME procedure was optimized by controlling drop organic solvent, drop volume, agitation, and exposure time. The optimum sample preparation was achieved with the use of a mixture of acetone/H(2)O (10/90, v/v) in donor sample solution preparation and the consequent SDME using a toluene drop under mild stirring for 25min. The efficiency of the extraction process was studied in fortified tomato and courgette samples and matrix effects were further estimated. The proposed method showed good linearity, limits of detection at the sub-microgkg(-1) level and high precision (RSD <15%) and was applied with success in real vegetable samples showing that SDME can be a promising way for sample preparation in pesticide residue analysis.     

环境水样中百菌清残留的单滴微萃取-反相液相色谱测定

应用单滴微萃取(SDME)-反相液相色谱(RPLC)检测了环境水样中的百菌清残留.优化了单滴微萃取条件:环己烷萃取剂6 μL、单滴体积2 μL、搅拌速率350 r/min、萃取时间40 min、水溶液温度35 ℃、无盐度.水样经单滴微萃取后,使用Hypersil C18柱反相液相色谱分离测定百菌清.反相液相色谱条件:100%甲醇流动相、流速1.0 mL/min、柱温25 ℃、224 nm检测.方法的线性范围、检出限、相对标准偏差和富集倍数分别为1.0 ～50 μg/L、0.02 μg/L、6.1%和427倍.采用该法对环境水样中的百菌清残留进行了测定,环境水样的加标回收率为98% ～106%.