Comparison of membrane assisted solvent extraction,stir bar sorptive extraction,and solid phase microextraction in analysis of tetramine in food

Three environmentally friendly extraction techniques, membrane assisted solvent extraction (MASE), stir bar sorptive extraction (SBSE), and headspace solid phase microextraction (HS‐SPME), were compared for the direct analysis of the highly toxic rodenticide tetramine in food. The optimized MASE method was applied to seven foods fortified with tetramine and compared to previously reported SBSE and HS‐SPME results. Parameters such as the standard addition linearity (MASE (0.964–0.999), SBSE (0.966–0.999), HS‐SPME (0.955–0.999)), recovery (MASE (12–86%), SBSE (36–130%), HS‐SPME (50–200%)), reproducibility (MASE (3.0–30%), SBSE (4.4–9.6%), HS‐SPME (1–12%)), and LOD (MASE (1.6–6.4 ng/g), SBSE (0.2–2.1 ng/g), HS‐SPME (0.9–4.3 ng/g)) were compared.     

碳纳米管顶空固相微萃取测定水中的多溴联苯醚

建立了顶空固相微萃取联结气相色谱-电子捕获检测器（HS-SPME-GC-ECD）测定水中多溴联苯醚的方法。制作了多壁碳纳米管涂层固相微萃取探头。优化了萃取时间,萃取温度,搅拌速度,顶空体积,溶液的pH,离子强度及有机溶剂等影响萃取效率的各种因素。比较了室温和100 ℃顶空萃取和直接萃取的效率。结果表明,室温下直接萃取比顶空萃取的效率高2-4倍,而在100 ℃时顶空萃取比直接萃取的效率高1-8倍。除BDE-154外,无论直接萃取还是顶空萃取,100 ℃时的萃取效率均高于室温。方法的线性范围50-1600 ng/L,相关系数为0.995-0.998,5种多溴联苯醚的最低检出限（S/N=3）为1.14-16.25 ng/L,相对标准偏差（RSD%,n=5）小于10%。本方法用于真实水样的测定,回收率为74.2%-98.7%。     

Analysis of Wine Bouquet Components Using Headspace Solid-Phase Microextraction-Capillary Gas Chromatography

Headspace solid-phase microextraction (HS/SPME) was studied and optimized for the capillary gas chromatographic (CGC) analysis of wine aroma compounds. The results were compared with those obtained using the direct sampling mode (DI/SPME) and using liquid/liquid extraction with Kaltron. The aromatic patterns obtained by HS/SPME-CGC were applied to the chemometric classification of wine varieties. The HS/SPME-CGC standard additional method is an appropriate technique for the quantitative analysis of volatile wine aroma compounds.     

顶空固相微萃取-气相法测定酒中的甲醇和杂醇油

 采用环氧树脂作为固相涂层制作固相微萃取 (SPME)装置 ,建立了顶空固相微萃取 气相法 (HS SPME GC)测定酒精饮料中甲醇和杂醇油的方法 ,并对萃取条件和条件进行了优化。方法的检出限为 0 0 2mg/L～0 0 4mg/L ,相对标准偏差为 1 4 %～ 4 1% ;与顶空气相法相比 ,灵敏度可提高 2 0倍～ 30 0倍。将该法用于啤酒、葡萄酒和保健酒中的甲醇和杂醇油的测定 ,加标回收率为 80 8%～ 110 3% ;与顶空气相法 (国家标准方法 )进行了比较 ,相对误差不大于 7 3%。该法简便、快速、灵敏、精密度好 ,拓宽了SPME的应用范围。     

Optimization of a novel headspace–solid‐phase microextraction–gas chromatographic method by means of a Doehlert uniform shell design for the analysis of trace level ethylene oxide residuals in sterilized medical devices

Medical devices sterilized by ethylene oxide (EtO) retain trace quantities of EtO residuals, which may irritate patients' tissue. Reliably quantifying trace level EtO residuals in small medical devices requires an extremely sensitive analytical method. In this research, a Doehlert uniform shell design was utilized in obtaining a response surface to optimize a novel headspace–solid‐phase microextraction–gas chromatographic (HS‐SPME‐GC) method developed for analyzing trace levels of EtO residuals in sterilized medical devices, by evaluating sterilized, polymer‐coated, drug‐eluting cardiovascular stents. The effects of four independent experimental variables (HS‐SPME desorption time, extraction temperature, GC inlet temperature and extraction time) on GC peak area response of EtO were investigated simultaneously and the most influential experimental variables determined were extraction temperature and GC inlet temperature, with the fitted model showing no evidence of lack‐of‐fit. The optimized HS‐SPME‐GC method demonstrated overall good linearity/linear range, accuracy, repeatability, reproducibility, absolute recovery and high sensitivity. This novel method was successfully applied to analysis of trace levels of EtO residuals in sterilized/aerated cardiovascular stents of various lengths and internal diameter, where, upon heating, trace EtO residuals fully volatilized into HS for extraction, thereby nullifying matrix effects. As an alternative, this novel HS‐SPME‐GC method can offer higher sensitivity compared with conventional headspace analyzer‐based sampling. Copyright © 2009 John Wiley & Sons, Ltd.     

Use of two different coating temperatures for a cold fiber headspace solid‐phase microextraction system to determine the volatile profile of Brazilian medicinal herbs

In this study, the experimental extraction conditions on applying headspace solid‐phase microextraction and cold fiber headspace solid‐phase microextraction (CF‐HS‐SPME) procedures to samples of six medicinal herbs commonly found in southern Brazil were optimized. The optimized conditions for headspace solid‐phase microextraction were found to be an extraction temperature of 60°C and extraction time of 40 min. For CF‐HS‐SPME, the corresponding values were 60°C and 15 min. In the case of the coating temperature for the CF‐HS‐SPME system, two approaches were investigated: (i) Temperature of 5°C applied during the whole extraction procedure; and (ii) the use of two fiber temperatures in the same extraction procedure with the aim of extracting the volatile and semivolatile compounds, the ideal condition being 60°C for the first 7.5 min and 5°C for the final 7.5 min. The three extraction procedures were compared. The CF‐HS‐SPME procedure had good performance only for the more volatile compounds whereas the strategy using two coating temperatures in the same procedure showed good performance for all compounds studied. It was also possible to determine the profile for the volatile fraction of each herb studied applying this technique followed by GC‐MS.     

Determination of Se4+ in drinkable water by solid-phase microextraction and gas chromatography/mass spectrometry

A method was developed for the selective determination of Se4+ in drinkable water by solid-phase microextraction (SPME) and gas chromatography/mass spectrometry (GC/MS). Se4+ was selectively derivatized to ethane, 1,1'-selenobis by reaction with sodium tetraethylborate, extracted by the SPME fiber, and determined by GC/MS. Both headspace (HS)-SPME and direct SPME were studied. The method requires only a few milliliters of sample and 20 min for completion. At 2.0 microg/L concentration, the relative standard deviation was 10.1% for HS-SPME and 9.1% for direct SPME. For HS-SPME, the theoretical detection limit was 81 ng/L and 166 ng/L for direct SPME. The recovery rate was 95%. The method was used to determine Se4+ in 10 tap water samples.     

Headspace-solid-phase microextraction preconcentration of phenols, indoles and on-fibre derivatised volatile fatty acids in liquid and gas samples from cow slurries

Odorous organic compounds from liquid and gas samples of animal wastes were studied by headspace (HS)-solid-phase microextraction (SPME)-GC-MS. 1-Pirenyldiazomethane (PDAM) was adsorbed/absorbed on the SPME fibre in order to obtain the corresponding ester derivatives during the preconcentration step. The SPME fibre was immersed into a PDAM solution. Then, the SPME fibre was withdrawn and exposed to the HS of the liquid cow slurry. This way derivatisation of VFAs took place in the SPME fibre together with the preconcentration of the rest of the analytes of interest. The analytes were desorbed in the hot injection port (300 degrees C) of a GC-MS for 3 min. Four different fibre types and different immersion periods of the fibre in the PDAM solution were studied in order to obtain the best sensitivity with the selected fibre. Accuracy, precision and the LODs were calculated using spiked liquid and gas samples. The possibility of storing liquid samples after sampling by preconcentration on the fibre was also considered. Storage time and temperature were studied. The optimised method was applied to the determination of the analytes in liquid and gas samples from cow slurries from an intensive production farm.     

Solid-phase microextraction for the evaluation of partition coefficients of a chlorinated dioxin and hexachlorobenzene into humic substances.

We developed a method for the evaluation of the partition coefficients (K(oc)) of hexachlorobenzene (HCB) and 1,2,3,4,6,7,8-heptachlorodibenzo-p-dioxin (HpCDD) into humic substances (HSs) by using solid-phase microextraction (SPME). In the aqueous solution containing HCB or HpCDD and HS, the unbound species of HCB or HpCDD were accumulated on the SPME fiber. Subsequently, HCB or HpCDD on the SPME fiber was directly analyzed by GC-ECD. When the concentration of organic carbon in HS ([OC]) was plotted against the ratio of [HCB] or [HpCDD] in the absence of HS to that in the presence of HS, linear relationships were observed. The slope of the line corresponded to the K(oc) value. The log K(oc) values for HCB and HpCDD evaluated were in the ranges of 3.9 - 4.9 and 5.9 - 7.2, respectively. These values were the same order as those in the literature, which were evaluated by other methods (e.g., solubility enhancement, solid-phase extraction and dialysis). The relative standard deviations of the log K(oc) values evaluated in this study were within 5%.     

Selective non-chromatographic determination of tributyltin in sediments using EDTA and diphenylcarbazone as masking agent

Two analytical procedures based on the generation of volatile tributyltin derivatives, their separation by headspace solid-phase microextraction (HS SPME) and subsequent determination using plasma optical emission spectrometry (OES) have been developed for the selective determination of trace tributyltin (TBT) in the presence of other butyltins and inorganic tin in sediments without the use of chromatography. A microwave-assisted leaching of tin compounds from the sediment using 25%_v/v acetic acid is applied for sample pretreatment. The first method takes advantage of TBT chloride releasing from the lecheate after adding 3 M hydrochloric acid, and subsequent separation of the analyte by HS SPME using Carboxen-poly(dimethylsiloxane) (CAR/PDMS). The second method involves the use of masking agents, namely ethylenediaminetetraacetic acid (EDTA) and diphenylcarbazone (DFC), which form stable chelates with monobutyltin (MBT) and dibutyltin (DBT), respectively, followed by the ethylation of tributyltin at pH 5 using sodium tetraethylborate (NaBEt4) solution. The final concentration of NaBEt4 is 0.05%_w/v. The parameters affecting the TBT derivatisation and separation by HS SPME have been optimised including the selection of SPME fibre coating (PDMS, CAR/PDMS), the amount of masking agents and NaBEt4 added, sorption time (2–40 min) and sorption temperature (25–60°C). Higher sensitivity and robustness are attained with the method involving ethylation derivatisation, leading to the limit of detection (LOD) of 3 ng L^?1. The selective release of TBT is observed from aqueous solutions, where the concentrations of MBT and DBT were in 2–50-fold excess to TBT. The SPME-TD-MIP-OES methods have been validated against several certified reference materials (CRMs), including SOPH-1 marine sediment, PACS-2 marine sediment and BCR 646 freshwater sediment.     

Application of solid-phase microextraction and gas chromatography-mass spectrometry for the determination of chlorophenols in leather

This paper proposes a new analytical procedure based on the headspace solid‐phase microextraction (HS‐SPME) technique and gas chromatography‐selected ion monitoring‐mass spectrometry (GC‐SIM‐MS) for the determination of 16 phenols extracted from leather samples. The optimized conditions for the HS‐SPME were obtained through two experimental designs – a two‐level fractional factorial design followed by a central composite design – using the commercial SPME fiber polyacrylate 85 μm (PA). The best extraction conditions were as follows: 200 μL of derivatizing agent (acetic anhydride), 20 mL of saturated aqueous NaCl solution and extraction time and temperature of 50 min and 75°C, respectively. All optimized conditions were obtained with fixed leather sample mass (250 mg), vial volume (40 mL) and phosphate buffer pH (12) and concentration (50 mmol/L). Detection limits ranging from 0.03 to 0.20 ng/g, and relative standard deviation (RSD) lower than 10.23% (n=6) for a concentration of 800 ng/g (chlorophenols) and 1325 ng/g (2‐phenylphenol) in the splitless mode were obtained. The recovery was studied at three concentration levels by adding different amounts of phenols to the leather sample and excellent recoveries ranging from 90.0 to 107.2% were obtained. The validated method was shown to be suitable for the quantification of phenols in leather samples, as it is simple, relatively fast and sensitive.     

Speciation of inorganic and tetramethyltin by headspace solid‐phase microextraction and gas chromatography–mass spectrometry

A headspace solid‐phase microextraction (HS‐SPME) method coupled to GC‐MS was developed in order to determine trace levels of tetramethyltin (TeMT) and inorganic tin (iSn) after ethylation to tetraethyltin (TeET) in various matrices. The derivatization of iSn and the extraction of both TeMT and iSn as TeET were performed in one step. Sodium tetraethylborate (NaBEt₄) was used as derivatization agent and the volatile derivatives were absorbed on a PDMS‐coated fused silica fiber. The conditions for the HS‐SPME procedure were optimized in order to gain in repeatability and sensitivity. Several critical parameters of GC‐MS were also studied. The detection of TeMT and iSn as TeET peaks was performed by the SIM mode. The precision of the proposed method is satisfactory providing RSD values below 10% for both tin species and good linearity up to 10 μg/L. The developed method was successfully applied to the determination of tin species in several samples like canned fish, fish tissues, aquatic plants, canned mineral water and sea water. The proposed HS‐SPME‐GC‐MS method was proved suitable to monitor the concentration levels of toxic tin compounds in environmental and biological samples.     

Active sampling followed by solid-phase microextraction for the determination of pyrethroids in indoor air

A method based on solid-phase enrichment followed by headspace (HS)-solid-phase microextraction (SPME) is optimized to determine pyrethroids in air. By active sampling, pyrethroids present in air are retained in 25 mg of activated florisil and then transferred from the solid sorbent to an SPME fiber in the HS mode. A small volume of solvent is added to the adsorbent to favor this process. The selection of the adsorbent, as well as the optimization of certain parameters affecting the SPME, is performed using an experimental design strategy. Linearity is studied by external calibration in a wide range of concentrations using gas chromatography coupled to three different detection systems: electron capture detection, micro-electron capture detection, and mass spectrometry. An analysis of variance with a lack-of-fit test is run to validate the calibration data. Breakthrough of the adsorbent was studied sampling from 0.5 to 10 m(3) air, demonstrating that 1 m(3) air could be sampled without losses of pyrethroids. Quantitative recoveries are obtained at three concentration levels, with adequate repeatability. Limits of detection of the method are estimated at the sub-ng/m(3) level in most cases, well below the regulatory limits. Finally, several real indoor samples are collected and analyzed by the proposed method. Identification and quantitation of all target analytes present in the room air are possible.     

Determination of heavy metal complexes with humic substances by HPLC/ICP-MS coupling using on-line isotope dilution technique

An isotope dilution mass spectrometric (IDMS) method has been developed for the simultaneous determination of the complexes of 11 heavy metals (Ag, Cd, Cu, Mo, Ni, Pb, Tl, U, W, Zn and Zr) with humic substances (HS) by coupling HPLC with ICP-MS and applying the on-line isotope dilution technique. The HPLC separation was carried out with size exclusion chromatography. This HPLC/ICP-IDMS method was applied to samples from a brown water, ground water, sewage and seepage water as well as for a sample containing isolated fulvic acids. The total contents of heavy metals and of their complexes were analyzed in these samples with detection limits in the range of 5–110 ng/L. The analysis of heavy metal/HS complexes from the different waters resulted in characteristic fingerprints of the distribution pattern of heavy metals in the separated HS fractions. A comparison between the total heavy metal concentrations and their portions bound to humic substances showed distinct differences for the various metals. Simultaneous ¹²C detection was used for the characterization of HS complexes not identified by UV detection and for the determination of relative DOC concentrations of chromatographic peaks. Received: 21 February 1997 / Revised: 27 May 1997 / Accepted: 28 May 1997     

HS-SPME determination of volatile carbonyl and carboxylic compounds in different matrices

Specific chromatographic methodologies are developed for the analysis of carboxylic acids (C(2)-C(6), benzoic) and aldehydes (C(2)-C(10)) of low molecular weight in diverse matrices, such as air, automotive exhaust gases, human breath, and aqueous matrices. For carboxylic acids, the method is based on their reaction with pentafluorobenzyl bromide in aqueous solution, followed by the separation and identification of the resultant pentafluorobenzyl esters by means of headspace (HS)-solid-phase microextraction (SPME) combined with gas chromatography (GC) and electron capture detection (ECD). Detection limits in the microg/m(3) range are reached, with relative standard deviation (RSD) less than 10% and linear response (R(2) > 0.99) over two orders of magnitude. The analytical methodology for aldehydes is based on SPME with simultaneous derivatization of the analytes on the fiber, by reaction with pentafluorophenylhydrazine. The derivatization reagent is previously deposited on the SPME fiber, which is then exposed to the gaseous matrix or the HS of the sample solution. The pentafluorophenyl hydrazones formed on the fiber are analyzed selectively by means of GC-ECD, with detection limits in the ng/m(3) range, RSD less than 10%, and linear response (R(2) > 0.99) over two orders of magnitude.     

固相微萃取中高分子涂层的研究

聚甲基乙烯基硅氧烷首次被用作固相微萃取（ＳＰＭＥ）装置的固相涂层,通过顶空固相微萃取气相色谱分析（ＨＳ－ＳＰＭＥ－ＧＣ）对使用聚甲基乙烯基硅氧烷固相涂层的ＳＰＭＥ装置进行了评价。对其使用厚度、温度及选择性进行了较深入的研究,找到了它的最佳使用条件和适用范围,并与商品化的ＳＰＭＥ涂层作了比较。对ＨＳ－ＳＰＭＥ－ＧＣ和ＨＳ－ＧＣ两种方法也作了比较,指出两者的适用范围不同。     

Water solubility and octanol/water-partitioning of hydrophobic chlorinated organic substances determined by using SPME/GC

The critical step in the determination of water solubilitiy (S _w) and octanol-water partition coefficient (K _ow) of hydrophobic organic chemicals by using the generator-column technique and the slow-stirring procedure, respectively, is the exact quantification of the low water-phase concentrations of the substances under investigation. We have tested the applicability of solid-phase microextraction (SPME) and gas chromatography with seven chlorinated organic compounds. The substances cover a S _w range from 500 mg/L to 7 ng/L and a log K _ow range from 3 to 8. The results show that SPME can be a valuable alternative to common preconcentration techniques in the quantification of hydrophobic organics in pure and octanol-saturated water. The apparent SPME distribution constants K _SPME (obtained with the 100 μm-PDMS fiber for analyte’s partitioning between fiber coating and aqueous sample) do not correlate directly with octanol/water partition coefficients and thus cannot be recommended as a surrogate parameter for K _ow. Received: 15 January 1997 / Revised: 2 May 1997 / Accepted: 8 May 1997     

Determination of polar pesticides in soil by solid phase microextraction coupled to high-performance liquid chromatography-electrospray/mass spectrometry

The determination of carbamate and triazine pesticides from soil leachates and slurries was investigated using solid phase microextraction (SPME) coupled to high-performance liquid chromatography-electrospray/ mass spectrometry (HPLC-ESI/MS). SPME was carried out using fibres with a newly developed 50 μm Carbowax/ template coating which are suitable for relatively polar analytes. These fibers exhibit precisions better than 10% RSD, and are resistant against high contents of organic solvents during desorption. The technique shows a high sampling frequency resulting in an increasing sample throughput. Received: 17 December 1997 / Revised: 30 October 1998 / Accepted: 10 November 1998     

Solid-phase microextraction method for carbon isotopic analysis of volatile carboxylic acids in human plasma by gas chromatography/combustion/isotope ratio mass spectrometry

A new analytical method is described for the determination of the physiological concentration and low-level enrichment of (13)C-short-chain volatile organic acids (SCVAs) (e.g. (13)C-acetate and (13)C-butyrate) in human plasma. This two-step method involves solid-phase microextraction (SPME) coupled to gas chromatography/combustion/isotope ratio mass spectrometry (GC/C/IRMS) without any organic solvents or derivatizing agents. Two SCVA extraction methods were compared using a carboxen/polydimethylsiloxane fiber: headspace sampling (HS) and liquid sampling (LS) SPME. The influences of extraction temperature and time were tested to optimize the adsorption of SCVAs onto the fiber. The comparison of the peak area responses of the acids in the two adsorption methods showed better sensitivity in the human physiological concentration range in the LS mode than in the HS mode.The accuracy of isotopic enrichment measurement was determined using plasma spiked with (13)C-acetate and (13)C-butyrate solution from 0 to 1 mol percent excess (MPE). The linearity and repeatability (RSD < 5%) were measured in LS mode. Plasma SCVA concentrations were also determined relative to 3-methylvalerate (internal standard). Linearity and repeatability were observed from 0 to 400 microM for acetate, from 0 to 20 microM for propionate, and from 0 to 10 microM for butyrate. This method was also used to determine plasma acetate production obtained from lactulose (an undigestible disaccharide) fermentation in one healthy volunteer over 3 h. The acetate concentration increased twofold, 2 h after oral lactulose intake. These results are in agreement with the data obtained by GC/MS in healthy volunteers and obese adults following a lactulose intake by using higher amounts of labelled tracers.SPME coupled with GC/C/IRMS can be used to analyze (13)C-SCVAs at low enrichment (<0.5 MPE) within the physiological concentration measured in human plasma.     

Evaluation of headspace solid-phase microextraction for analysis of phosphine residues in wheat

In headspace (HS) analysis, a fumigant is released from a commodity into a gas-tight container by grinding, heating, or microwaves. A new technique uses HS-solid-phase microextraction (SPME) for additional preconcentration of fumigant. HS-SPME was tested for detection of phosphine (PH3), chosen for examination because of its wide use on stored commodities. PH3 was applied to 50 g wheat in separate 250 mL sealed flasks, which were equipped either with a septum for conventional HS analysis or with one of four HS-SPME fibers [100 microm polydimethylsiloxane (PDMS), 85 microm carboxen (CAR)/PDMS, 75 microm CAR/PDMS, and 65 pm PDMS/divinylbenzene (DVB)]. The wheat was heated at 45 degrees C for 20 min. In conventional HS analysis, a gaseous aliquot (80 pL) was taken from the HS and injected into the GC instrument. In the HS-SPME procedure, the fiber was removed from the HS and exposed in the heated injection port of the GC instrument. In all cases, PH3 was determined under the same chromatographic conditions with a GC pulsed flame photometric detector. In a comparison of the efficacy of the fibers, the bipolar fibers (CAR/PDMS and PDMS/DVB) contained more PH3 than the aliquot in the conventional HS analysis; larger size bipolar fibers extracted PH3 more efficiently than smaller fibers (e.g., 85 > 75 > 65 microm). The nonpolar fiber (PDMS) contained no PH3. Four fortification levels of PH3 on wheat were tested: 0.01, 0.05, 0.1, and 0.3 microg/g. The response of each bipolar fiber increased with the fortification levels, but the conventional HS analysis detected no fumigant at the lowest fortification level of 0.01 mg/g. Under the conditions of the validation study, the LOD was in the range of 0.005-0.01 ng PH3/g wheat.