Comparison of solvent mixtures for pressurized solvent extraction of soil fatty acid biomarkers

The extraction and transesterification of soil lipids into fatty acid methyl esters (FAMEs) is a useful technique for studying soil microbial communities. The objective of this study was to find the best solvent mixture to extract soil lipids with a pressurized solvent extractor system. Four solvent mixtures were selected for testing: chloroform:methanol:phosphate buffer (1:2:0.8, v/v/v), chloroform:methanol (1:2, v/v), hexane:2-propanol (3:2, v/v) and acetone. Soils were from agricultural fields and had a wide range of clay, organic matter and microbial biomass contents. Total lipid fatty acid methyl esters (TL-FAMEs) were the extractable soil lipids identified and quantified with gas chromatography and flame ionization detection. Concentrations of TL-FAMEs ranged from 57.3 to 542.2 n mole g⁻¹ soil (dry weight basis). The highest concentrations of TL-FAMEs were extracted with chloroform:methanol:buffer or chloroform:methanol mixtures than with the hexane:2-propanol or acetone solvents. The concentrations of TL-FAMEs in chemical groups, including saturated, branched, mono- and poly-unsaturated and hydroxy fatty acids were assessed, and biological groups (soil bacteria, mycorrhizal fungi, saprophytic fungi and higher plants) was distinguished. The extraction efficiency for the chemical and biological groups followed the general trend of: chloroform:methanol:buffer ≥ chloroform:methanol > hexane:2-propanol = acetone. Discriminant analysis revealed differences in TL-FAME profiles based on the solvent mixture and the soil type. Although solvent mixtures containing chloroform and methanol were the most efficient for extracting lipids from the agricultural soils in this study, soil properties and the lipid groups to be studied should be considered when selecting a solvent mixture. According to our knowledge, this is the first report of soil lipid extraction with hexane:2-propanol or acetone in a pressurized solvent extraction system.     

Evaluation of Liquid–Liquid Extraction Methods for Determining the Levels of Lipids and Organochlorine Pollutants in Human Milk

Organic chlorine pesticides and polychlorinated biphenyls are organic pollutants that are stored in the adipose tissues of humans. The concentrations of those pollutants in human milk have previously been utilized as a biomarker for monitoring the body burden of lipophilic pollutants in humans. Liquid–liquid extraction methods have been applied to lipids, chlorinated pesticides, and polychlorinated biphenyls from breast milk. In this study, the effectiveness of four extraction methods, which have been widely used to isolate fats and organic pollutants from milk, were compared. The organic solvents included hexane, hexane/acetone (2:1, v/v), ethanol/ethyl ether/hexane (2:3:4, v/v), and methanol/chloroform (1:1, v/v). These results demonstrated that hexane yields the lowest extraction recoveries for lipids (approximately 21.3%) and analytes (approximately 50%). The other three organic solvents demonstrated better performance in extracting the target compounds, with the ethanol/ethyl ether/hexane system showing the optimum efficiency. The optimized system was employed to determine the analytes in human milk.     

Use of modifiers in on-line and off-line supercritical fluid extraction

For many applications using supercritical fluid extraction (SFE), modifiers may be required.This paper will present some findings regarding the use of various modifiers including methanol, hexane, acetone, chloroform, dichloromethane, toluene, and tributylphosphate, in on-line and off-line SFE with cryogenic adsorbent trapping. The specific applications involved the extractions of petroleum hydrocarbons and pesticides from naturally incurred soils.     

A comparison of carbon and nitrogen stable isotope ratios of fish tissues following lipid extractions with non-polar and traditional chloroform/methanol solvent systems

Stable isotope ratios act as chemical tracers of animal diet, and are used to study food web dynamics. Because carbon stable isotope values are influenced by tissue lipid content, a number of extraction methods have been used to remove lipid bias, but, in some species and tissues, extractions also alter nitrogen isotope values. We have analyzed delta(13)C and delta(15)N in Atlantic bluefin tuna liver and white muscle, and whole Atlantic herring, fish tissues covering a wide range of lipid content (bulk C:N 3.1-12.5). In order to compare delta(13)C and delta(15)N values from traditional chloroform/methanol extractions with non-polar solvent alternatives, we analyzed samples following (1) no treatment, (2) lipid removal using chloroform/methanol (2:1), and (3) Soxhlet extractions using chloroform, diethyl ether or hexane. Chloroform/methanol and chloroform extractions produced the lowest C:N values and highest delta(13)C values. In bluefin tuna, chloroform and hexane extractions significantly altered liver delta(15)N, and all methods significantly altered delta(15)N values in white muscle. Whole Atlantic herring delta(15)N was not altered by any extraction method, while the 2:1 chloroform/methanol extraction most completely removed fish tissue lipid components. Our results indicate that delta(15)N effects are not limited to common chloroform/methanol extractions and suggest that chloroform/methanol is the most effective extraction for delta(13)C correction. Given evidence for delta(15)N alteration among all tested methods, mathematical correction approaches should be further explored as an alternative to lipid correction.     

Toxaphene (Polychlorinated Camphenes) Analysis in Human Blood

Abstract

A method for the determination of toxaphene in whole blood using gas chromatography (GC)-electron capture negative ion ECNI/MS and pure polychlorobornane congerners has been evaluated. Blood samples were extracted with hexane/acetone (9:1), extracts defatted with sulfuric acid, analytes fractionated on Carbopack-C/ Florisil (or silica gel) SPE columns then concentrated to final volumes for GC-ECNI/MS analysis. For confirmation, interference from PCBs and other organochlorine pesticides were removed by nitration.     

Validation of the Method of Selected Polychlorinated Biphenyls Determination in Human Milk Samples

A method for determination of trace concentrations of individual PCB congeners in human milk was validated. The analytical procedure included the following steps: acetone : hexane extraction, clean-up of extracts with concentrated sulfuric acid and solid phase extraction (SPE) on Florisil. The identification and quantification of analytes in purified extracts were carried out by high-resolution gas chromatography (HRGC) with electron capture detection (ECD) and/or with low-resolution mass spectrometry (LRMS). Recoveries of 14 PCB congeners from spiked cow milk samples, based on HRGC-ECD were between 87.3 and 93.6%. The precision of analyte determination was established as close to or less than 10%. The detection limits ranged between 0.14 and 0.26 ng/g fat and the quantification limits between 0.57 and 0.86 ng/g fat. The method was linear and characterized by good correlation coefficients (>0.99) for most of the compounds studied. The quality of the method under validation was verified by the analysis of Standard Reference Material (CRM-450) and interlaboratory exercise.     

Recovery efficiency of 2,3,7,8-tetrachlorodibenzo-p-dioxin from active carbon and other particulates

The use of Amoco active carbon (grade PX-21) as a cleanup step for the determination of 2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD) in environmental samples was investigated. Benzene/toluene (1:1) removed 95% TCDD from Amoco active carbon dispersed in silica gel. Other solvents, including benzene, carbon disulfide, dichloromethane, acetone, hexane, acetone/hexane (1:1), and diethyl ether, did not remove TCDD from Amoco active carbon. o-Dichlorobenzene is needed to remove TCDD from Pittsburgh active carbon completely. Hot benzene with Soxhlet extraction is adequate for TCDD removal from soil and fly ash particulates. The results derived from this study are consistent with past and present analytical practice for isolating TCDD from different matrices.     

Microwave-assisted extraction versus Soxhlet extraction in the analysis of 21 organochlorine pesticides in plants

A method to determine 21 organochlorine pesticides in vegetation samples using microwave-assisted extraction (MAE) is described and compared with Soxhlet extraction. Samples were extracted with hexane–acetone (1:1, v/v) and the extracts were cleaned using solid-phase extraction with Florisil and alumine as adsorbents. Pesticides were eluted with hexane–ethyl acetate (80:20, v/v) and determined by gas chromatography and electron-capture detection. Recoveries obtained (75.5–132.7% for Soxhlet extraction and 81.5–108.4% for MAE) show that both methods are suitable for the determination of chlorinated pesticides in vegetation samples. The method using microwave energy was applied to grass samples from parks of A Coruña (N.W. Spain) and to vegetation from the contaminated industrial area of Torneiros (Pontevedra, N.W. Spain).     

Pressurized liquid extraction of lipids for the determination of oxysterols in egg-containing food

Pressurized liquid extraction (PLE, ASE) was compared with the Folch procedure (a solid-liquid extraction with chloroform/methanol 2:1, v/v) for the lipid extraction of egg-containing food; the accuracy of PLE for the quantitative determination of oxysterols in whole egg powder was evaluated. Samples of spray-dried whole egg, an Italian vanilla cake (Pandoro) and egg noodles were used. Two different extraction solvents (chloroform/methanol 2:1, v/v, and hexane/isopropanol 3:2, v/v) were tested at different extraction temperatures and pressures (60 degrees C at 15 MPa, 100 degrees C at 15 MPa, 120 degrees C at 20 MPa). No significant differences in the lipid recovery of the egg powder sample using PLE were found. However, PLE of the vanilla cake and egg noodles with the chloroform/methanol mixture was not selective enough and led to the extraction of a non-lipid fraction, including nitrogen-containing compounds. In the same samples, the pressurized hexane/isopropanol mixture gave a better recovery result, comparable to that obtained using the Folch method. Cholesterol oxidation products of the Folch extract and the pressurized liquid extract of spray dried egg powder (obtained with hexane/isopropanol 3:2, v/v, at 60 degrees C and 15 MPa) were determined by gas chromatography. PLE performed under these conditions is suitable to replace the Folch extraction, because the differences between the two methods tested were not statistically significant. Moreover, PLE shows important advantages, since the analysis time was shortened by a factor of 10, the solvent costs were reduced by 80% and the use of chlorinated solvents was avoided.     

Simplified method for the determination of organochlorine pesticides in honey.

A method is described for the detection and quantitative determination of organochlorine pesticides in honey. After extraction with hexane, the pesticides were cleaned-up by adsorption chromatography on a Florisil Sep-Pak cartridge and eluted with 15% diethyl ether in hexane. The detection of organochlorine pesticides was performed by capillary gas chromatography with electron-capture detection. The quantification limit obtained for different pesticides ranged from 0.56 to 2.78 micrograms kg-1 and recoveries from fortified honey samples averaged 89.6%.     

顶空采样-毛细管气相色谱法分析格列美脲原料药中的溶剂残留

建立了顶空采样-毛细管气相色谱检测格列美脲原料药中溶剂残留的分析方法。对产自国内8个生产厂家的格列美脲样品中有机溶剂的残留状况进行了系统评价,结合药品生产工艺信息,确定了丙酮、乙酸乙酯、甲醇、异丙醇、乙醇、氯仿、甲苯、1,4-二氧六环、吡啶、氯苯、乙醚、二氯甲烷、正己烷和苯等14种有机溶剂为残留检测对象。根据被测组分在色谱柱上的保留性质将其分为两类,以实现基线分离。用Supelco-Wax极性色谱柱,以乙腈为内标物,分离检测了丙酮、乙酸乙酯、甲醇、异丙醇、乙醇、氯仿、甲苯、1,4-二氧六环、吡啶和氯苯的残留量;用Supelco OVI-G43弱极性色谱柱,以丁酮为内标,分离检测了乙醚、二氯甲烷、正己烷和苯的残留量。14种残留组分在各自的浓度范围内呈良好的线性关系(r=0.99167～0.99997,n=8),最低检出限范围为0.2～13.5 μg/g;14种残留组分检测的日间重复性(以相对标准偏差(RSD)计)为0.6%～9.2%(n=3),3种加标浓度的平均添加回收率为86.3%～104.1%(RSD为0.2%～5.3%,n=16)。实验结果表明,该方法简单、灵敏、可靠,适用于格列美脲中残留溶剂的分析确证。     

A clean‐up technology for the simultaneous determination of lysophosphatidic acid and sphingosine‐1‐phosphate by matrix‐assisted laser desorption/ionization time‐of‐flight mass spectrometry using a phosphate‐capture molecule,Phos‐tag

Lysophosphatidic acid (LPA) and sphingosine‐1‐phosphate (S1P) are growth factor‐like lipids having a phosphate group. The concentrations of these mediator lipids in blood are considered to be potential biomarkers for early detection of cancer or vascular diseases. Here, we report a method for simultaneous determination of LPA and S1P using Phos‐tag, a zinc complex that specifically binds to a phosphate‐monoester group. Although both LPA and S1P are hydrophilic compounds, we found that they acquire hydrophobic properties when they form complexes with Phos‐tag. Based on this finding, we developed a method for the enrichment of LPA and S1P from biological samples. The first partition in a two‐phase solvent system consisting of chloroform/methanol/water (1:1:0.9, v/v/v) is conducted for the removal of lipids. LPA and S1P are specifically extracted as Phos‐tag complexes at the second partition by adding Phos‐tag. The Phos‐tag complexes of LPA and S1P are detectable by matrix‐assisted laser desorption/ionization time‐of‐flight mass spectrometry (MALDI‐TOFMS) and quantifiable based on the relative intensities of ions using 17:0 LPA and C17 S1P as internal standards. The protocol was validated by analyses of these mediator lipids in calf serum, a rat brain and a lung. The clean‐up protocol is rapid, requires neither thin‐layer chromatography (TLC) nor liquid chromatography (LC), and is applicable to both blood and solid tissue samples. We believe that our protocol will be useful for a routine analysis of LPA and S1P in many clinical samples. Copyright © 2010 John Wiley & Sons, Ltd.     

A Method for the Determination of Octa- and Nonachloro-2-phenoxyphenols in Chicken Tissue

Abstract

A gas-liquid chromatographic method was developed capable of determining octa-and nonachloro-2-phenoxyphenols in chicken liver or muscle at 0.25 ppb and fat at 2.5 ppb. The method involves extraction with acidified acetone:hexane, cleanup with concentrated H₂SO₄ and Florisil column chromatography, methylation with diazomethane, and quantitation by capillary column gas-liquid chromatography with electron capture detection. Fortification of liver and muscle at 0.25 or 0.5 ppb and fat at 2.5 or 5.0 ppb and subsequent analysis yielded recoveries averaging 91% for octa-and 97% for nonachlorophenoxyphenol.     

Pyrethroid soil extraction,properties of mixed solvents and time profiles using GC/MS-NICI analysis

Ultrasonic extraction was used to develop a suitable binary solvent system for the analysis of synthetic pyrethroid pesticides and mirex on soil. The analysis was carried out by gas chromatography with negative ion chemical ionization mass spectrometry (GC/MS-NICI). In the initial experiments, accurately weighed soil samples were spiked with a mixture of standard solution pyrethroids and mirex and shaken for 24?h to ensure homogeneity, then extracted with solvent. The extracts were evaporated to dryness before the volumetric internal standard was added.

The binary solvents used in this study were various mixtures of hexane?:?acetone, hexane?:?dichloromethane (DCM), isooctane?:?acetone and isooctane?:?dichloromethane, representing different classes of polarity. The recoveries of all pyrethroids and mirex were satisfactory over three solvent systems: hexane?:?acetone, hexane?:?DCM and isooctane?:?acetone, but results of isooctane?:?DCM produced low recoveries. The average recovery increased with the extraction time, but the increase was not statistically significant. A 30-min optimum extraction was deemed sufficient for recovering pyrethroids from soil. After 30?min, extraction decreased owing to the re-distribution of the analyte on the soil matrix.     

23种挥发性有机化合物在3种吸附剂上漏出容量的测定评价

采用吸附热解吸－气相色谱－质谱法对23种挥发性有机化合物Chromosorb 106、Tenax TA、Tenax TG等3种吸附剂上漏出容量进行了测定。根据实验结果确定了不同的化合物应选择不同的吸附剂及相应的采样体积。结果表明,Chromosorb 106可较好地吸附低沸点的挥发性有机化合物,Tenax TA、Tenax TG均可用于沸点较高的挥发笥有机化合物吸附,这对测定大气中的有机化合物含量采样有一定的参考价值。     

Synthetic oligomer analysis using atmospheric pressure photoionization mass spectrometry at different photon energies

Atmospheric pressure photoionization (APPI) followed by mass spectrometric detection was used to ionize a variety of polymers: polyethylene glycol, polymethyl methacrylate, polystyrene, and polysiloxane. In most cases, whatever the polymer or the solvent used (dichloromethane, tetrahydrofuran, hexane, acetone or toluene), only negative ion mode produced intact ions such as chlorinated adducts, with no or few fragmentations, in contrast to the positive ion mode that frequently led to important in-source fragmentations. In addition, it was shown that optimal detection of polymer distributions require a fine tuning of other source parameters such as temperature and ion transfer voltage. Series of mass spectra were recorded in the negative mode, in various solvents (dichloromethane, tetrahydrofuran, hexane, toluene, and acetone), by varying the photon energy from 8 eV up to 10.6 eV using synchrotron radiation. To these solvents, addition of a classical APPI dopant (toluene or acetone) was not necessary. Courtesy of the synchrotron radiation, it was demonstrated that the photon energy required for an efficient ionization of the polymer was correlated to the ionization energy of the solvent. As commercial APPI sources typically use krypton lamps with energy fixed at 10 eV and 10.6 eV, the study of the ionization of polymers over a wavelength range allowed to confirm and refine the previously proposed ionization mechanisms. Moreover, the APPI source can efficiently be used as an interface between size exclusion chromatography or reverse phase liquid chromatography and MS for the study of synthetic oligomers. However, the photoionization at fixed wavelength of polymer standards with different molecular weights showed that it was difficult to obtain intact ionized oligomers with molecular weights above a few thousands.     

Liquid chromatographic determination of flumetsulam in soybeans

A liquid chromatography (LC) method with UV detection is reported for the determination of the sulfonamide herbicide flumetsulam in soybeans. The ground soybean sample was partitioned between methanol and hexane. The hexane removed the lipids, and the methanol layer containing the analyte was further partitioned between dichloromethane and aqueous phosphate buffer at pH 7.0. The aqueous layer, containing the analyte, was acidified to pH 2.2 and partitioned with fresh dichloromethane. The dichloromethane layer containing the analyte was evaporated, and the residue was dissolved in the LC mobile phase for analysis. A polar embedded C18 column was used with a mobile phase of pH 2.2 aqueous phosphate buffer-acetonitrile (68 + 32), run isocratically with detection at 225 nm. The average recovery was 82% with a relative standard deviation (RSD) of 10%. A coefficient of determination of R2 = 0.9992 was achieved for the analyte calibration curve, from 0.005 to 1 microg/mL. The limit of detection, determined from 3 times the standard deviation of 7 replicate extractions of the lowest fortification level (0.01 microg/g), was 0.005 microg/g with an RSD of 22%. LC/electrospray ionization/mass spectrometry in the positive-ion mode was used for identity confirmation of flumetsulam in the fortified soybean extract. The ions at m/z 326, 348, and 129 were observed.     

Comparison of solid phase extraction, saponification and gel permeation chromatography for the clean-up of microwave-assisted biological extracts in the analysis of polycyclic aromatic hydrocarbons

The feasibility of different clean-up procedures was studied for the determination of polycyclic aromatic hydrocarbons (PAHs) in biota samples such as oysters, mussels and fish liver. In this sense, once the samples were extracted--essentially with acetone and in a microwave system--and before they could be analysed by gas chromatography-mass spectrometry (GC-MS), three different approaches were studied for the clean-up step: solid phase extraction (SPE), microwave-assisted saponification (MAS) and gel permeation chromatography (GPC). The main aim of this work was to maximise the recoveries of PAHs and to minimise the presence of interfering compounds in the last extract. In the case of SPE, Florisil cartridges of 1, 2 and 5 g, and silica cartridges of 5 g were studied. In that case, and with oysters and mussels, microwave-assisted extraction and 5 g Florisil cartridges provided good results. In addition, the concentrations obtained for Standard Reference Material (SRM) NIST 2977 (mussel tissue) were in good agreement with the certified values. In the case of microwave-assisted saponification, the extracts were not as clean as those obtained with 5 g Florisil and this fact lead to overestimate the concentration of the heaviest PAHs. Finally, the cleanest extracts were obtained by GPC. The method was successfully applied to mussels, oysters and hake liver, and the results obtained for NIST 2977 (mussel tissue) were within the confidence interval of the certified reference material for most of the certified analytes.     

A new luminescent terbium 4-methylsalicylate complex as a novel sensor for detecting the purity of methanol

A new dinuclear terbium complex [Tb(2)(4-msal)(6)(H(2)O)(4)]·6H(2)O (1) (4-msal = 4-methylsalcylate) was synthesized. Its structure was determined by single crystal X-ray diffraction, and the complex was characterized by PXRD, FT-IR, fluorescence, TGA and DTA. Complex 1 exists as discrete molecules that are linked by extensive O-H … O hydrogen bonds into a 3D network. The luminescence lifetimes of 3 μM methanol solution and solid sample of 1 are 1.321 and 1.009 ms, respectively. The quantum yield of solid sample is 6.0%. The luminescence quenched more than 50% when 3% (vol/vol) different impurities (acetone, acetonitrile, chloroform, dichloromethane, dioxane, DMF, DMSO, ethanol, ether, ethyl acetate, glycol, H(2)O, hexane, TEA, THF and toluene or their mixture) were added. The inverse linear relationship between the Lg value of fluorescence intensity and the volume ratio of the minor component (to a maximum of 20%) is interpreted in terms of LgI = a-bX (I: luminescence intensity; X: volume ratio of impurities in methanol; a, b are constants). So 1 is a potential luminescent sensor for analyzing the purity of methanol.     

GC determination of nicotine in subcutaneous adipose tissue obtained by minimal trauma tissue biopsy

Summary Nicotine has been analyzed by gas chromatography nitrogen-phosphorus detection in tissue samples obtained by repeated minimal trauma tissue biopsies from human subcutaneous adipose tissue. For sample preparation, a single extraction step of the tissue samples with chloroform was performed at 30–45°C. Calibration curves generated with spiked porcine subcutaneous adipose tissue were linear over a concentration range from 0.20 to 100 μg g⁻¹, therefore, the limit of quantification was fixed at 0.20 μg g⁻¹. The limit of detection was found to be 0.05 μg g⁻¹ adipose tissue. The recovery of nicotinespiked porcine subcutaneous adipose tissue by chloroform extraction was 100±8%. The performance of the assay was not affected by the complex lipid matrix. The method was employed for analysis in a clinical study on nicotine penetration from a transdermal delivery system through the skin of moderate smokers. Presented at Balaton Symposium on High Performance Separation Methods, Siófok, Hungary, September 1–3, 1999.