电感耦合等离子体发射光谱法/质谱法检测地衣样品中主次微量元素的方法优化

地衣是应用广泛的大气污染生物监测器。电感耦合等离子体发射光谱法/质谱法(ICP-MS/AES)是植物元素定性定量分析的重要和高效的方法。但受严重大气污染影响,我国部分地区的地衣元素水平远高于其他植物,且在空间、时间、物种和元素类别方面存在巨大差异。虽然地衣在大气污染监测方面具有良好的应用前景,但我国地衣元素分析测试方面尚缺乏专门的方法学研究,这限制了大气质量的地衣生物监测在我国的开展。因此,有必要对地衣样品元素含量的ICP-MS/AES法进行优化。以国家一级标准物质GBW10014(圆白菜)、GBW10015(菠菜)、GBW10052(绿茶)和地衣标准物质(IAEA-336)为材料,探讨了地衣样品的不同消解方法、取样量、分析谱线、同位素、内标元素及仪器参数对ICP-MS和ICP-AES结果的影响。确定了适用于大批量地衣元素测试的干法灰化-碱熔ICP-AES和微波消解ICP-MS的优化条件,该优化条件具有线性关系好(r>0.999 0)、检出限低、准确度高和精密度好的特点。以优化后的测试方法测定采自我国太行山区和南极阿德利岛的地衣样品,结果表明太行山地衣体内元素含量远高于南极阿德利岛,大气沉降对太行山地衣元素组成的相对贡献也较大。验证了优化方法的适用性,为京津冀环境治理提供科学数据和技术支持。     

Multi-class pesticide analysis in human hair by gas chromatography tandem (triple quadrupole) mass spectrometry with solid phase microextraction and liquid injection

A method for the simultaneous detection and quantification of 22 pesticides from different chemical classes was developed using solid-phase microextraction (SPME) and gas chromatography tandem (triple quadrupole) mass spectrometry. Pesticides were extracted from 50 mg of pulverized hair with acetonitrile. The extract was submitted to two successive steps of direct immersion-SPME at 30 °C and 90 °C or to a liquid injection without SPME in order to obtain optimized conditions for each of the 22 analytes investigated. Validation parameters were significantly influenced by both the injection mode (SPME vs liquid injection) and the temperature of SPME. Limits of quantification ranged from 0.05 pg mg⁻¹ for trifluralin to 10 pg mg⁻¹ for pentachlorophenol. The application of the validated method to the analysis of samples collected from non-occupationally exposed volunteers demonstrated the presence of pesticides in all the samples tested. Altogether, 13 different analytes were detected at concentration above the limit of quantification.     

The determination of methylmercury in biological samples by HPLC coupled to ICP‐MS detection

The use of high‐performance liquid chromatography (HPLC) coupled to inductively coupled plasma mass spectrometry (ICP‐MS) for the determination of methylmercury (MeHg⁺) in fish tissue and hair samples is described. Analysis of these sample types is required when carrying out biomonitoring studies to determine human dietary exposure to this toxic mercurial compound. The developed method used a mobile phase containing an organic modifier and a sulfydryl compound (1:1 v/v methanol:water containing 0.01% v/v 2‐mercaptoethanol) to limit peak tailing and aid separation. The chromatographic separation was coupled to the ICP‐MS detector via a short piece of PEEK tubing, attached to the nebulizer. A cooled spraychamber and oxygen addition post‐nebulization were required to limit the solvent loading on the plasma and reduce carbon build‐up on the cones, respectively. The sample preparation procedure employed a drying step followed by digestion of the sample using tetramethylammonium hydroxide (TMAH) and heating in an open vessel microwave system. Two fish tissue certified reference materials (CRM), tuna fish CRM 463 and 464 (BCR, Brussels), a tuna fish proficiency test sample, IMEP‐20 (IRMM, Geel, Belgium) and a hair CRM NIES no. 13 (National Institute of Environmental Science, Japan), were used to evaluate the method. The recovery of MeHg⁺ for these four materials was between 83 and 100%, with precisions better than 6% for three separate extractions of the different materials. The limit of quantitation for MeHg⁺ using the developed protocol was 0.5 µg Hg g^?1. The stability of MeHg⁺ in the fish sample extracts was also assessed and losses of 14–16% were observed after storage of the extracts in a refrigerator at 5 °C, in high‐density polypropylene tubes, for 6 months. The developed protocol has been used previously with atmospheric pressure ionization mass spectrometry (API‐MS) to provide structural characterization and also with calibration via isotope dilution (IDMS) to provide high accuracy quantitation. Copyright © 2006 John Wiley & Sons, Ltd.     

Determination of 226Ra, 232Th and 40K in teeth by use of gamma spectroscopy

This study entails the measurement of the specific activity of natural radionuclides (²²⁶Ra, ⁴⁰K and ²³²Th) in 18 tooth samples obtained from the clinic of the Universiti Sains Malaysia (USM), Penang, by using an HPGe detector. The specific activity of ²²⁶Ra, ⁴⁰K and ²³²Th was measured to estimate the hazard index of the radionuclides, radium equivalent activities (Ra_eq), external, internal hazard indices (H_ex, H_in), and absorbed dose (D_out, D_in). The maximum values of concentration of ²²⁶Ra, ²³²Th and ⁴⁰K in the tooth samples were found to be 60.82, 60.29 and 594.22?Bq kg^?1, respectively. Maximum values of Ra_eq, H_ex, H_in, D_out and D_in were found to be 192.78?Bq kg^?1, 0.520, 0.685, 89.29 and 169.81?nGy h^–1, Iγ and Iα as 0.702 and 0.304, respectively. The results were lower than the average world value (UNSCEAR). In addition, a strong correlation was found between the concentrations of ²²⁶Ra and Ra_eq, between energy and net area, as well as between radionuclides (²²⁶Ra, ⁴⁰K and ²³²Th) in tooth samples and age of volunteers. This study showed that the concentrations and hazard indices of tooth samples are below the recommended safe levels; therefore, the study area is considered safe in terms of radiological health hazards.     

Development of HPLC-MS/MS method for the simultaneous determination of metabolites of organophosphate pesticides,synthetic pyrethroids,herbicides and DEET in human urine

We developed an isotopic dilution high-performance liquid chromatography (HPLC)/tandem mass spectrometer (MS/MS) method to rapidly and accurately quantify nine metabolites of several classes of pesticide in 1 mL human urine specimens. The analytes covered in the method are two organophosphate (OP) pesticide metabolites: 3,5,6-trichloro-2-pyridinol (TCPy), 2-isopropyl-6-methyl-4-pyrimidinol (IMPY); three synthetic pyrethroid metabolites: 3-phenoxy benzoic acid (3-PBA), 4-fluoro-3-phenoxybenzoic acid (4-F-3-PBA) and trans-3-(2,2-dichlorovinyl)-2,2-dimethyl-1(1-cyclopropane) carboxylic acid (t-DCCA); three herbicide metabolites: 2,4-dichlorophenoxyacetic acid (DCPAA), 2,4,5-trichlorophenoxyacetic acid (TCPAA) and atrazine mercapturate; and one insect repellent: N,N-diethyl-meta-toluamide (DEET). The analytes are first deconjugated by incubating with acetate/β-glucuronidase buffer at 37°C for 17 h. The deconjugated analytes are extracted and concentrated from the urine matrix using solid-phase extraction cartridges, separated through C18 reversed phase HPLC, and analysed on MS/MS. The MS/MS was operated in positive and negative electrospray ionisation switch mode. Two ions from each analyte and one from each labelled internal standard are monitored for quantification and confirmation. The limit of detections (LODs) for all the analytes are in the low parts-per-trillion (0.05 ng/mL) except TCPy where it was 0.5 ng/mL) with a wide linear range (0.05 up to 40 ng/mL) and provides high accuracy (recoveries: 90–118%) and high precision (coefficient of variation <15%). The method accuracy was also verified by the analysis of proficiency testing urine samples. We analysed 101 urine samples for a recent California study cohort, and detection frequencies ranged from ~100% to 0%: 3-PBA (98%), IMPY (91%), TCPy, (89%), DCPAA (66%), 4-F-3-PBA (11%), TCPAA (0%).     

Urinary metabolic profiling of volatile organic compounds in acute exposed volunteers after an oil spill in Republic of Korea

The Herbei Spirit oil spill occurred in western Korea. A large number of people who participated in the cleanup tasks of the contaminated area were exposed to crude oil component. We developed a method to monitor volatile organic compound (VOC) metabolites in urine, and evaluate the acute exposure caused by the oil spill in exposed volunteer workers (n = 100, 20.7 ± 2.1 years, mean ± SD). Acidified urine samples were extracted by SPE, derivatized with trimethylsilyl, and analyzed using gas chromatography–mass spectrometry. Calibration curves were found to be linear from 3 to 1000 ng/mL (r² > 0.993). Accuracy was over 82.4%, and precision was less than 24.8%. Using this method, the VOC metabolites, except hippuric acid, were present at higher levels in the urine samples of volunteers after cleanup work. The levels of mandelic acid (MA) and trans,trans‐muconic acid (t,t‐MU) were increased significantly (p < 0.001). The exposure effect was greater in women than in men. The effect of smoking was analyzed in all exposed and non‐exposed groups, with non‐smokers showing increased MA and t,t‐MU levels related to exposure. The present method was reliable to determine VOC metabolites in urine and could be useful for biomonitoring of acute exposure effects of VOCs. Copyright © 2009 John Wiley & Sons, Ltd.     

Improved methods for urinary atrazine mercapturate analysis--assessment of an enzyme-linked immunosorbent assay (ELISA) and a novel liquid chromatography-mass spectrometry (LC-MS) method utilizing online solid phase extraction (SPE)

Elimination of interfering substances in urine by solid phase extraction (SPE) prior to analysis resulted in 10-fold improvement in the sensitivity of atrazine mercapturate (AM) enzyme-linked immunosorbent assay (ELISA) compared to previous reports. Of the two tested SPE systems, Oasis^® HLB and MCX, the mixed-mode MCX gave good recoveries (82%) of AM in spiked samples measured by ELISA, whereas the reverse-phase HLB phase was not compatible with the immunochemical method. At relatively high concentrations of urinary AM (>20 ng mL⁻¹), sample dilution was effective enough for the elimination of interfering substances. The new liquid chromatography-mass spectrometry (LC-MS) method developed for AM utilizes online-SPE with Oasis^® HLB, column switching and a stable-isotope internal standard. The limit of quantification (0.05 ng mL⁻¹) indicates improved sensitivity compared with most previously published LC-MS methods for AM. Validation of all three methods, LC-MS, ELISA + SPE and ELISA + dilution with spiked urine samples showed good correlation between the known and measured concentrations with R² values of 0.996, 0.957 and 0.961, respectively. When a set (n = 70 plus 12 blind duplicates) of urine samples from farmers exposed to atrazine was analyzed, there was a good agreement (R² = 0.917) between the log normalized data obtained by ELISA + SPE and LC-MS. High correlation among the data obtained by the two tested methods and the LC-MS method by the Center of Disease Control and Prevention (CDC), together with low variability among the blind duplicates, suggests that both methods reported here would be suitable for the analysis of urinary AM as a biomarker for human exposure of atrazine.     

Effects of species and sites on metal concentrations in byssal threads of two mytilids

Concentrations of 11 metals (Al, Cu, Fe, Mg, Mn, Mo, Ni, Pb, Sr, V and Zn) were determined by inductively coupled plasma quadruple mass spectrometer measurements in byssus of two mytilid species Mytilus galloprovincialis and Xenostrobus securis from three sites situated along the coastline of Ría de Vigo (NW Spain). The species coexist only at one of those sites, thus it was possible to compare the impact of both factors, site and species, on metal concentrations. Principal component and regression analyses showed a dominant effect of mussel species and not the site. In all samples, the highest concentration was observed for iron in accordance with the literature data for M. galloprovincialis. One order of magnitude higher concentrations of iron detected in the byssus of X. securis than that of M. galloprovincialis are discussed considering a different microstructure of byssus threads as shown by transmission electron microscopy images.     

Glyphosate and aminomethylphosphonic acid in human hair quantified by an LC-MS/MS method

An LC-MS/MS method for hair testing of glyphosate and aminomethylphosphonic acid (AMPA), its main biodegradation product, has been developed. After decontamination, 50 mg of hair was ground and sonicated in water for 2 h. The method was fully validated in the 5–500 pg/mg range for glyphosate and 10–500 pg/mg for AMPA, and the limits of detection were 2 and 5 pg/mg, respectively. Matrix effect for glyphosate and AMPA was compensated by an isotope-labeled internal standard. Hair samples from four farmers who regularly used glyphosate and one farmer who used glyphosate but not his wife and 14 hair samples from nonoccupationally exposed subjects were tested. Glyphosate was found in head hair of three farmers, with concentration in the range 14–188 pg/mg. The fourth was found negative but with hair colored in red. Glyphosate was detected in 10 of 14 hair samples from nonoccupationally exposed subjects at concentrations of 11.5 pg/mg or lower and only in one segment (0–3 cm) of the farmer's spouse (6 pg/mg). AMPA was detected in five subjects, above the limit of quantification only in two of three occupationally exposed subjects with positive glyphosate. Further studies should be conducted to validate this potential new biomarker that could be useful for assessing long-term exposure to glyphosate.     

Determination of hydroxylated metabolites of polycyclic aromatic hydrocarbons in human hair by gas chromatography–negative chemical ionization mass spectrometry

The study describes the determination of mono-hydroxylated polycyclic aromatic hydrocarbons (OH-PAHs), metabolites of PAHs, in human hair. Twelve selected OH-PAHs from two to four rings, generally determined in urine analysis, were investigated as markers of human exposure to PAHs. Following hydrolysis of hair specimens of 50–300 mg with 1 M NaOH, OH-PAHs were extracted using dichloromethane and submitted to an optimized derivatization with (2S,4R)-N-heptafluorobutyryl-4-heptafluorobutoyloxy-prolyl chloride. Compounds were then analyzed using gas chromatography–negative chemical ionization mass spectrometry (GC–NCIMS). The average inter-day and intra-day variability was 12% and 17%, respectively. The average recovery was 52% and the limits of detection and quantification ranged from 20 and 66 pmol/g for 1-OH-phenanthrene (i.e., 3.9 and 12.8 pg/mg) to 311 and 1030 pmol/g for 2-OH-benzo(c)phenanthrene (i.e., 75.9 and 251 pg/mg). The influence of hair washing with water as decontamination step, and enzymatic treatment (β-glucuronidase) to hydrolyze conjugated derivatives were also tested. The application of the developed method to the analysis of 30 hair specimens (17 from non-smoker and 13 from smoker volunteers) demonstrated inter-individual qualitative and quantitative variations. According to the easiness of hair sampling and based on the extended detection windows provided by hair analysis, this method is proposed as a new promising tool for the assessment of human chronic exposure to PAHs.