加速溶剂萃取法快速提取黄连中的生物碱

探讨了快速溶剂萃取法（ASE）提取黄连中生物碱的可行性,并比较了该方法与回流提取法和超声提取法的优越性。以黄连中盐酸小檗碱的提取率为指标,以高效液相色谱法（HPLC）为检测方法,用正交实验对快速溶剂萃取法从黄连中提取盐酸小檗碱的工作条件进行优化。最佳仪器参数：提取溶剂为80%乙醇＋0.5%HCl,提取温度为130℃,静态提取时间为10 min,提取次数为1次。快速溶剂萃取法可作为黄连中生物碱分析测定的前处理方法。     

Comparison of GC-ICP-MS and HPLC-ICP-MS for species-specific isotope dilution analysis of tributyltin in sediment after accelerated solvent extraction

This study describes a direct comparison of GC and HPLC hyphenated to ICP–MS determination of tributyltin (TBT) in sediment by species-specific isotope dilution analysis (SS-IDMS). The certified reference sediment PACS-2 (NRC, Canada) and a candidate reference sediment (P-18/HIPA-1) were extracted using an accelerated solvent extraction (ASE) procedure. For comparison of GC and LC methods an older bottle of PACS-2 was used, whilst a fresh bottle was taken for demonstration of the accuracy of the methods. The data obtained show good agreement between both methods for both the PACS-2 sediment (LC–ICP–IDMS 828±87 ng g^–1 TBT as Sn, GC–ICP–IDMS 848±39 ng g^–1 TBT as Sn) and the P-18/ HIPA-1 sediment (LC–ICP–IDMS 78.0±9.7 ng g^–1 TBT as Sn, GC–ICP–IDMS 79.2±3.8 ng g^–1 TBT as Sn). The analysis by GC–ICP–IDMS offers a greater signal-to-noise ratio and hence a superior detection limit of 0.03 pg TBT as Sn, in the sediment extracts compared to HPLC–ICP–IDMS (3 pg TBT as Sn). A comparison of the uncertainties associated with both methods indicates superior precision of the GC approach. This is related to the better reproducibility of the peak integration, which affects the isotope ratio measurements used for IDMS. The accuracy of the ASE method combined with HPLC–ICP–IDMS was demonstrated during the international interlaboratory comparison P-18 organised by the Comité Consultatif pour la Quantité de Matière (CCQM). The results obtained by GC–ICP–IDMS for a newly opened bottle of PACS-2 were 1087±77 ng g^–1 Sn for DBT and 876±51 ng g^–1 Sn for TBT (expanded uncertainties with a coverage factor of 2), which are in good agreement with the certified values of 1090±150 ng g^–1 Sn and 980±130 ng g^–1 Sn, respectively.     

Microwave-assisted extraction and accelerated solvent extraction with ethyl acetate-cyclohexane before determination of organochlorines in fish tissue by gas chromatography with electron-capture detection

Focused open-vessel microwave-assisted extraction (FOV-MAE), closed-vessel microwave-assisted extraction (CV-MAE), and accelerated solvent extraction (ASE) were used for extraction before determination of organochlorine compounds (polychlorinated biphenyls, DDT, toxaphene, chlordane, hexachlorobenzene, hexachlorocyclohexanes, and dieldrin) in cod liver and fish fillets. Wet samples were extracted without the time-consuming step of lyophilization or other sample-drying procedures. Extractions were performed with the solvent mixture ethyl acetate-cyclohexane (1 + 1, v/v), which allowed direct use of gel-permeation chromatography without solvent exchange. For FOV-MAE, the solvent mixture removed water from the sample matrix via azeotropic distillation. The status of water removal was controlled during extraction by measuring the temperature of the distillate. After water removal, the temperature of the distillate increased and the solvent mixture became less polar. Only the pure extraction solvent allowed quantitative extraction of the organochlorine compounds. For CV-MAE, water could not be separated during the extraction. For this reason, the extraction procedure for wet fish tissue required 2 extraction steps: the first for manual removal of coextracted water, and the second for quantitative extraction of the organochlorine compounds with the pure solvent. Therefore, CV-MAE is less convenient for samples with high water content. For ASE, water in the sample was bound with Na2SO4. The reproducibility for each technique was very good (relative standard deviation was typically <10%); the slightly varying levels were attributed to deviations during sample cleanup and the generally low levels.     

Evaluation of Soxhlet extraction, accelerated solvent extraction and microwave-assisted extraction for the determination of polychlorinated biphenyls and polybrominated diphenyl ethers in soil and fish samples

Three commonly applied extraction techniques for persistent organic chemicals, Soxhlet extraction (SE), accelerated solvent extraction (ASE) and microwave-assisted extraction (MAE), were applied on soil and fish samples in order to evaluate their performances. For both PCBs and PBDEs, the two more recent developed techniques (ASE and MAE) were in general capable of producing comparable extraction results as the classical SE, and even higher extraction recoveries were obtained for some PCB congeners with large octanol-water partitioning coefficients (K_ow). This relatively uniform extraction results from ASE and MAE indicated that elevated temperature and pressure are favorable to the efficient extraction of PCBs from the solid matrices. For PBDEs, difference between the results from MAE and ASE (or SE) suggests that the MAE extraction condition needs to be carefully optimized according to the characteristics of the matrix and analyte to avoid degradation of higher brominated BDE congeners and improve the extraction yields.     

Extraction of hydrocarbon contamination from soils using accelerated solvent extraction

Accelerated solvent extraction was studied as a method for the extraction of hydrocarbon contamination from wet and dry soils. Temperatures from 125 to 200 degrees C and six different solvents were investigated. Nonpolar solvents could not achieve complete recovery from wet soils at the temperatures studied. Optimum conditions were found to be 175 degrees C with dichloromethane-acetone (1:1, v/v) with 8 min heat-up time and 5 min static time. Quantitative recoveries for diesel range organics (DROs) and waste oil organics (WOOs) were obtained using the optimized conditions. The recovery of DROs and WOOs from three matrices at two concentrations (5 and 2000 mg/kg) averaged 115%. These results show that accelerated solvent extraction can generate results comparable to those obtained using Soxhlet or sonication.     

Arsenic extraction and speciation in carrots using accelerated solvent extraction, liquid chromatography and plasma mass spectrometry

Arsenic present in freeze-dried carrots was extracted using accelerated solvent extraction (ASE). Several parameters, including selection of the dispersing agent, extraction time, number of extraction cycles, particle size and extraction temperature, were evaluated to optimize the ASE method. Filtering and treatment with C-18 SPE cartridges were also evaluated as part of the sample preparation procedure before speciation analysis. The method was validated by spiking single arsenical and mixed arsenical standards on the dispersing agent and on portions of freeze-dried carrot prior to extraction. LC-ICP-MS was used to determine individual arsenic species in the carrot extracts. A weak anion-exchange column was used for the separation of As(III), As(v), monomethylarsonic acid (MMA), dimethylarsinic acid and arsenobetaine. Optimized sample preparation conditions were applied to the extraction of arsenic in nine freeze-dried carrot samples. Total arsenic concentration in the carrot samples ranged from less than 20 ng g(-1) to 18.7 microg g(-1), dry mass. Extraction efficiency, defined as the ratio of the sum of individual arsenic species concentrations to total arsenic, ranged from 80 to 102% for freeze-dried carrots with arsenic concentrations greater than the limit of quantitation. Inorganic As(III) and As(v) were the only species found in samples that contained less than 400 ng g(-1) total arsenic. MMA and an unidentified arsenic compound were present in some of the samples with higher total arsenic content.     

Extraction of polar and hydrophobic pollutants using accelerated solvent extraction (ASE)

Accelerated solvent extraction (ASE) shows higher recoveries for PAHs in comparison with traditional Soxhlet extraction, but in a fraction of time and with less solvent consumption. Better recoveries are especially achieved with PAHs of high reactivity, the latter being expressed by the structure-to-count ratio (SCR). To estimate polar pollutants including phenols/benzenediols, the sample was subjected to a combined in-situ derivatization/extraction approach using 2% v/v acetic anhydride in toluene. The main reason for the better recovery obtained in this way, in comparison with the classical ASE approach, is to overcome strong matrix-analyte interactions. Analogously, fatty acids were analyzed as methyl esters obtained by in-situ derivatization/extraction using boron trifluoride. Received: 28 December 1998 / Revised: 16 February 1999 / Accepted: 21 February 1999     

Extraction of polar and hydrophobic pollutants using accelerated solvent extraction (ASE)

Accelerated solvent extraction (ASE) shows higher recoveries for PAHs in comparison with traditional Soxhlet extraction, but in a fraction of time and with less solvent consumption. Better recoveries are especially achieved with PAHs of high reactivity, the latter being expressed by the structure-to-count ratio (SCR). To estimate polar pollutants including phenols/benzenediols, the sample was subjected to a combined in-situ derivatization/extraction approach using 2% v/v acetic anhydride in toluene. The main reason for the better recovery obtained in this way, in comparison with the classical ASE approach, is to overcome strong matrix-analyte interactions. Analogously, fatty acids were analyzed as methyl esters obtained by in-situ derivatization/extraction using boron trifluoride.     

快速溶剂萃取柚皮中的黄酮类化合物

采用快速溶剂萃取法从柚子皮中提取出黄酮类化合物,考察了不同的提取溶剂、提取时间、提取温度、循环次数等提取条件下的提取效果,并与微波法、超声波法及索氏提取法进行了对比.结果表明,快速溶剂萃取法提取柚子皮中的黄酮类化合物,在提取溶剂用量、提取时间和提取效率等方面,均优于传统的提取方法,且自动化程度高,为进一步开发利用柚子皮的药用价值提供了参考.     

Robust microwave-assisted extraction protocol for determination of total mercury and methylmercury in fish tissues

A rapid and efficient closed vessel microwave-assisted extraction (MAE) method based on acidic leaching was developed and optimized for the extraction of total mercury (Hg), inorganic mercury (Hg²⁺) and methylmercury (CH₃Hg⁺) from fish tissues. The quantitative extraction of total Hg and mercury species from biological samples was achieved by using 5 mol L⁻¹ HCl and 0.25 mol L⁻¹ NaCl during 10 min at 60 °C. Total Hg content was determined using inductively coupled plasma mass spectrometry (ICP-MS). Mercury species were measured by liquid chromatography hyphenated with inductively coupled plasma mass spectrometry (LC-ICP-MS). The method was validated using biological certified reference materials ERM-CE464, DOLT-3, and NIST SRM-1946. The analytical results were in good agreement with the certified reference values of total Hg and CH₃Hg⁺ at a 95% confidence level. Further, accuracy validation using speciated isotope-dilution mass spectrometry (SIDMS, as described in the EPA Method 6800) was carried out. SIDMS was also applied to study and correct for unwanted species transformation reactions during and/or after sample preparation steps. For the studied reference materials, no statistically significant transformation between mercury species was observed during the extraction and determination procedures. The proposed method was successfully applied to fish tissues with good agreement between SIDMS results and external calibration (EC) results. Interspecies transformations in fish tissues were slightly higher than certified reference materials due to differences in matrix composition. Depending on the type of fish tissue, up to 10.24% of Hg²⁺ was methylated and up to 1.75% of CH₃Hg⁺ was demethylated to Hg²⁺.     

Determination of acetanilide herbicides in cereal crops using accelerated solvent extraction, solid-phase extraction and gas chromatography-electron capture detector

A method was developed to determine eight acetanilide herbicides from cereal crops based on accelerated solvent extraction (ASE) and solid-phase extraction (SPE) followed by gas chromatography-electron capture detector (GC-ECD) analysis. During the ASE process, the effect of four parameters (temperature, static time, static cycles and solvent) on the extraction efficiency was considered and compared with shake-flask extraction method. After extraction with ASE, four SPE tubes (graphitic carbon black/primary secondary amine (GCB/PSA), GCB, Florisil and alumina-N) were assayed for comparison to obtain the best clean-up efficiency. The results show that GCB/PSA cartridge gave the best recoveries and cleanest chromatograms. The analytical process was validated by the analysis of spiked blank samples. Performance characteristics such as linearity, limit of detection (LOD), limit of quantitation (LOQ), precision and recovery were studied. At 0.05 mg/kg spiked level, recoveries and precision values for rice, wheat and maize were 82.3-115.8 and 1.1-13.6%, respectively. For all the herbicides, LOD and LOQ ranged from 0.8 to 1.7 μg/kg and from 2.4 to 5.3 μg/kg, respectively. The proposed analytical methodology was applied for the analysis of the targets in samples; only three herbicides, propyzamid, metolachlor and diflufenican, were detected in two samples.     

Determination of pharmaceuticals in biosolids using accelerated solvent extraction and liquid chromatography/tandem mass spectrometry

An analytical method was developed to quantitatively determine pharmaceuticals in biosolid (treated sewage sludge) from wastewater treatment plants (WWTPs). The collected biosolid samples were initially freeze dried, and grounded to obtain relatively homogenized powders. Pharmaceuticals were extracted using accelerated solvent extraction (ASE) under the optimized conditions. The optimal operation parameters, including extraction solvent, temperature, pressure, extraction time and cycles, were identified to be acetonitrile/water mixture (v/v 7:3) as extraction solvent with 3 extraction cycles (15 min for each cycle) at 100 °C and 100 bars. The extracts were cleaned up using solid-phase extraction followed by determination by liquid chromatography coupled with tandem mass spectrometry. For the 15 target pharmaceuticals commonly found in the environment, the overall method recoveries ranged from 49% to 68% for tetracyclines, 64% to 95% for sulfonamides, and 77% to 88% for other pharmaceuticals (i.e. acetaminophen, caffeine, carbamazepine, erythromycin, lincomycin and tylosin). The developed method was successfully validated and applied to the biosolid samples collected from WWTPs located in six cities in Michigan. Among the 15 target pharmaceuticals, 14 pharmaceuticals were detected in the collected biosolid samples. The average concentrations ranged from 2.6 μg/kg for lincomycin to 743.6 μg/kg for oxytetracycline. These results indicated that pharmaceuticals could survive wastewater treatment processes, and accumulate in sewage sludge and biosolids. Subsequent land application of the contaminated biosolids could lead to the dissemination of pharmaceuticals in soil and water environment, which poses potential threats to at-risk populations in the receiving ecosystems.     

Optimised accelerated solvent extraction of PCBs and PAHs from compost

This study is the first thorough method optimisation for accelerated solvent extraction (ASE) of polychlorinated biphenyls (PCBs) and polycyclic aromatic hydrocarbons (PAHs) from chemically dried compost. For PCBs, optimised solvent composition, temperature, pressure, number of static cycles, duration, and flush volume were as follows: toluene/acetone 1?:?3 (v/v), 120°C, 2000?psi, 3?×?5?min, and 50%, respectively. Limits of quantification and method precision were between 0.16 and 2.46?µg?kg^?1 dw and 6–17% respectively for individual PCBs. Absolute recoveries of isotope-labelled extraction standards used for each of the analytes ranged from 65 to 105% and relative recoveries were between 85 and 99%. The method proofed to be robust and was successfully applied to different compost samples.

The optimisation of PAHs extraction was performed and resulted in the following conditions: solvent: hexane/acetone 1/3 (v:v), temperature: 140°C, pressure: 1500?psi, extraction time: 3?×?5?min, and 50% flush volume. Limits of detection and method precision for individual PAHs were between 1.1 and 37.2?µg?kg^?1?dw and 12–34% respectively. Absolute and relative recoveries ranged from 24 to 68% and from 85 to 99%, respectively. Optimal extraction conditions for PAHs were more difficult to determine due to the inhomogeneous distribution of PAHs in samples. However, the method appeared to be feasible and suggestions for further improvements are presented.     

Simultaneous determination of arsenic and selenium species in fish tissues using microwave-assisted enzymatic extraction and ion chromatography-inductively coupled plasma mass spectrometry

A microwave-assisted enzymatic extraction (MAEE) method was developed for the simultaneous extraction of arsenic (As) and selenium (Se) species in fish tissues. The extraction efficiency of total As and Se and the stability of As and Se species were evaluated by analyzing DOLT-3 (dogfish liver). Enzymatic extraction using pronase E/lipase mixture assisted by microwave energy was found to give satisfactory extraction recoveries for As and Se without promoting interspecies conversion. The optimum extraction conditions were found to be 0.2 g of sample, 20 mg pronase E and 5 mg lipase in 10 mL of 50 mM phosphate buffer, pH 7.25 at 37 °C. The total extraction time was 30 min. The speciation analysis was performed by ion chromatography-inductively coupled plasma mass spectrometry (IC-ICP-MS). The accuracy of the developed extraction procedure was verified by analyzing two reference materials, DOLT-3 and BCR-627. The extraction recoveries in those reference materials ranged between 82 and 94% for As and 57 and 97% for Se. The accuracy of arsenic species measurement was tested by the analysis of BCR 627. The proposed method was applied to determine As and Se species in fish tissues purchased from a local fish market. Arsenobetaine (AsB) and selenomethionine (SeMet) were the major species detected in fish tissues. In the analyzed fish extracts, the sum of As species detected was in good agreement with the total As extracted. However, for Se, the sum of its species was lower than the total Se extracted, revealing the presence of Se-containing peptides or proteins.     

Desorption of BTEX from activated charcoal using accelerated solvent extraction: evaluation of occupational exposures

A procedure for the determination of benzene, toluene, ethylbenzene and o-xylene, m-xylene and p-xylene (BTEX) in occupational environments is proposed. These compounds are extracted from activated charcoal using accelerated solvent extraction. Operational parameters are optimized and quantitative recovery is obtained using acetonitrile as the extraction solvent and 1-mL extraction cells, a preheat time of 2 min, a temperature of 160 °C, a pressure of 1,500 psi, a static period of 5 min, a flush volume of 110%, two cycles and a purge time of 90 s. Determination of BTEX compounds is carried out by gas chromatography using a flame ionization detector. The recoveries, obtained for a confidence level of 95%, are 91 ± 4, 100 ± 3, 104 ± 2, 93 ± 4, 99 ± 2 and 99 ± 2% for benzene, toluene, ethylbenzene, o-xylene, m-xylene and p-xylene, respectively. The detection limits are 0.5 μg for benzene, 0.7 μg for toluene and 1.0 μg for the other compounds. The proposed procedure has been applied to real samples collected in several workplaces, like a microbiology laboratory, an analytical chemistry laboratory, a printer’s, a car repair shop and a petrol station. From the results obtained, it can be concluded that the occupational exposures determined are always acceptable because they are lower than the tenth part of the recommended exposure limits (VLA-ED and VLA-EC).     

Multiresidue determination of organophosphorus pesticides in ginkgo leaves by accelerated solvent extraction and gas chromatography with flame photometric detection

A rapid and simple method using accelerated solvent extraction and solid-phase extraction cleanup was developed and validated for the determination of 15 organophosphorus pesticides in ginkgo leaves by capillary gas chromatography with flame photometric detection. The pesticides were extracted at 100 degrees C under 1500 psi pressure in <20 min. The average recovery from 10 g ginkgo leaves, fortified at 3 levels ranging from 0.05 to 1.00 mg/kg, was 95.2% with a relative standard deviation of 4.6%. The limits of detection ranged from 1.11 x 10(-3) mg/kg (dimethoate) to 4.44 x 10(-3) mg/kg (dichlorvos). The proposed method showed acceptable accuracy and precision while minimizing environmental concerns, time, and labor. Furthermore, the method could be easily applied to the monitoring of these 15 organophosphorus pesticides in ginkgo leaves.     

Fast and accurate determination of hemoglobin A1c using an automated sample processor

Summary The ion-exchange Chromatographic determination of hemoglobin A1c has been performed with minicolumns and an automated sample processor (Prep 1) in order to reduce sample preparation time and increase reproducibility. Since the non-availability of accurate standards makes the evaluation of the new method difficult, the different sample fractions were monitored by HPLC with UV detection (reference method). The centrifugal method has been improved until each hemoglobin fraction can be qualitatively and quantitatively recognized by the microprocessor software on the basis of the retention time. The coefficient of variation for Hb1Ac in normal samples (n=8) was 6.9% (mean 2.61%). The new method requires 30 min for 12 simultaneous determinations

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Schnelle und genaue Bestimmung von Hämoglobin A1c mit Hilfe eines automatischen Processors

Zusammenfassung Die ionenaustausch-chromatographische Bestimmung von Hämoglobin A1c wurde mit Hilfe von Minisäulen und einem automatischenProcessor (Prep 1) durchgeführt, um Arbeitszeit einzusparen und die Reproduzierbarkeit zu erhöhen. Da die Nichtverfügbarkeit genauer Standards eine Auswertung der neuen Methode erschwert, wurden die Probefraktionen mit Hilfe der HPLC mit UV-Detektor überwacht. Das Zentrifugalsystem wurde verbessert, so daß jede Fraktion qualitativ und quantitativ mit der Mikroprocessor-Software aufgrund der Retentionszeit erkannt werden konnte. Der Variationskoeffizient für HbA1c in normalen Proben (n=8) betrug 6,9% (Mittel 2,61%). Das Verfahren benötigt für 12 Simultanbestimmungen 30 min.

     

Spectrophotometric determination of total phenolics by solvent extraction and sorbent extraction optosensing using flow injection methodology

Flow injection analysis (FIA) procedures for the Spectrophotometric determination of phenol involving in-line concentration by solvent and sorbent extraction have been developed. The imine product formed in the reaction between phenol and 4-aminoantipyrine (4-AAP) is either extracted into chloroform (solvent extraction) or is temporarily retained on C₁₈-modified silica material contained in a microcolumn (sorbent extraction). In the latter case two variants of detection have been used namely the Spectrophotometric measurement of the methanolic eluent containing the concentrated dye and at-column optosensing of the retained reaction product followed by methanol elution to maintain reversibility of the process. In the solvent extraction procedure a 10-fold increase of sensitivity compared to the common FIA method without extraction is achieved but no corresponding improvement in detectability is observed. Under optimized conditions the detection limit amounts to 8 μg l⁻¹. Using sorbent extraction methodology, high concentration factors can be obtained when large sample volumes are used. The only limitation in getting correspondingly lower detection limits are an increasingly high and variable blank value with sampling volume. The detection limits obtained for measurement of the absorbance in the eluent and on-column optosensing are 11 μg l⁻¹ and 0.4 μg l⁻¹, respectively. A study of the extractability of various phenol derivates using both solvent and sorbent extraction revealed lower relative response rates compared to the FIA method without extraction. Phenolics that possess an additional acidic group are present in ionized form at the high pH of the assay and are not extractable at all.     

加速溶剂萃取-气相色谱-串联质谱法同时测定贝类中64种农药残留

建立了加速溶剂同步萃取净化-气相色谱-串联质谱(GC-MS/MS)同时测定贝类中64种农药残留的方法。加速溶剂萃取的萃取溶剂为90%(v/v)乙腈水溶液,萃取温度为85℃、冲洗体积60%萃取池体积、循环次数1次,同时使用0.8 g N-丙基乙二胺(PSA)和0.8 g石墨化炭黑(GCB)在线净化,提取液浓缩定容后,在多反应监测(MRM)模式下测定,外标法定量。结果表明,64种农药在10.0～1 000μg/L范围内呈现良好的线性关系,决定系数(r²)均大于0.989,方法的定量限为2.0～10.0μg/kg;对文蛤空白基质进行加标回收试验,添加水平为5.0、10.0和100μg/kg以及定量限水平,得到的平均回收率为69.4%～129.7%,精密度为0.7%～16.0%(n=6)。该方法提取和净化同步完成,操作简单,重复性好,灵敏度高,能够满足于贝类水产品中多种农药残留的同时筛查。