Simultaneous determination of nine anticoagulant rodenticides in soil and water by LC–ESI‐MS

A new and sensitive analytical method is presented to determine nine anticoagulant rodenticide (chlorophacinone, bromadiolone, pindone, diphacinone, warfarin, coumatetralyl, brodifacoum, floucomafen, and difenacoum) residues in water and soil samples by LC–ESI‐MS. Rodenticides were extracted from soil using a methanol and ammonium formate 30 mM mixture, while ethyl acetate was employed in the water samples. A Gemini 5 μm C₁₈ column was employed, and a mobile phase comprising a mixture of ammonium formate 30 mM and di‐n‐butylamine 30 mM in water (pH 3.5), ammonium formate 30 mM and di‐n‐butylamine 20 mM in water (pH 4.4), ammonium formate 30 mM in water (pH 6.5), and methanol in a gradient elution mode was selected. The method was fully validated and it was found to be selective and precise in terms of linearity and accuracy. Extraction recoveries ranged from 90 to 104% for the compounds studied, while the detection and quantification limits were between 0.09 and 2.2 μg/kg in soil or 0.08 and 1.7 μg/L in water. The method was applied to simultaneously measure these compounds in water and soil samples.     

气相色谱-质谱法同时快速测定血清中5种剧毒灭鼠剂

建立了同时快速测定血清样品中毒鼠强、氟乙酰胺、氟乙酸钠、甘氟Ⅰ与甘氟Ⅱ 5种灭鼠剂的气相色谱-质谱联用法。在pH 2.0条件下,以N,N-二乙基对苯二胺为衍生剂,N,N'-二环己基碳二亚胺为催化剂,氟乙酸钠在室温下振荡衍生5 min,衍生物与毒鼠强、氟乙酰胺、甘氟Ⅰ、甘氟Ⅱ一并被乙酸乙酯萃取,经50 ℃下氮吹浓缩后用气相色谱-质谱同时测定,采用选择离子监测(SIM)模式,基质标准外标法定量。方法选用SLB-IL59离子液体毛细管柱(30 m×0.25 mm×0.20 μm,最高温度:300 ℃),流速1.0 mL/min,经程序升温在15 min内成功地分离了5种灭鼠剂。结果显示,血清中氟乙酰胺的线性范围为0.02~2.0 mg/L,毒鼠强的线性范围为0.02~10 mg/L,其他目标物的线性范围为0.01~1.0 mg/L;检出限为0.001~0.002 mg/L (S/N=3),相关系数R²>0.995。在3个加标水平下,方法加标回收率介于84.0%和110.0%之间,相对标准偏差(n=6)介于2.9%和7.5%之间。方法操作简便、准确,灵敏度高,适于中毒病人的快速诊断检测。     

LC/MS/MS法同时测定卷烟主流烟气中4种TSNAs

烟草特有亚硝胺（TSNAs）是存在于、烟草制品和卷烟烟气中的一类有害物质。TSNAs在卷烟烟气中的含量很低,卷烟烟气背景复杂,化学成分达3800多种,卷烟烟气中TSNAs的准确定量难度很大。多年来,TSNAs的测量方法随着分析仪器的进步而不断发展,从薄层色谱到GC、LC,从填充柱到毛细管柱,从FID检测到氮磷检测器检测、热能分析仪检测、质谱检测。     

超高效液相色谱-串联质谱法同时快速筛查检测食品中的10种抗凝血类鼠药

创建了一种利用超高效液相色谱-串联质谱同时快速筛查检测食品中10种抗凝血类鼠药的方法。试样用乙腈提取,QuEChERS净化,以5 mmol/L乙酸铵和乙腈为流动相进行梯度洗脱,经Poroshell 120 EC-C18柱(100 mm×2.1 mm, 2.7 μm;美国Agilent公司)分离,采用电喷雾电离(ESI)负离子质谱在多反应监测(MRM)模式下检测。10种鼠药均在5～500 μg/L范围内呈现良好的线性关系(r>0.99)。在辣椒酱、面粉、醋和酱油4种样品中,10种鼠药的加标回收率均在72.6%～112%范围内,相对标准偏差均不大于11.2%,检出限均在0.5～4.5 μg/kg范围内。本方法快速、简便、灵敏、重现性好,能满足由此10种抗凝血类鼠药引发的突发性公共卫生安全事件的快速筛查与检测要求。     

UHPLC-ESI-MS/MS法测定动物源食物提取物中肌肽与鹅肌肽的含量

建立了一种同时测定动物源提取物中肌肽(Carnosine)和鹅肌肽(Anserine)含量的超高效液相色谱-电喷雾串联三重四极杆质谱(UHPLC-ESI-MS/MS)分析方法。采用超高效液相分离系统,借助Inertsil Amide HP色谱柱(2. 1 mm×100 mm,3μm)以0. 1%乙酸水溶液-乙腈为流动相,梯度洗脱分离,利用峰面积外标法定量。经过优化,肌肽和鹅肌肽在1. 95～500μg/L质量浓度范围内与峰面积呈良好的线性关系,相关系数(r)均大于0. 998。肌肽和鹅肌肽的检出限分别为0. 12、0. 47μg/L。以低浓度低聚肽原料为基质,在低、中、高3个加标浓度下,肌肽的回收率为99. 3%～109%,相对标准偏差(RSD,n=6)为0. 98%～1. 1%;鹅肌肽的回收率为100%～113%,RSD为1. 0%～1. 1%。该法前处理简单、快速,重现性好,准确度高,适用于动物源食物提取物中肌肽和鹅肌肽的同时快速检测。     

Simultaneous determination of 103 pesticide residues in tea samples by LC‐MS/MS

A simple and sensitive method was developed and validated for the simultaneous determination of 103 pesticide residues in tea by LC‐MS/MS. For the analysis of the pesticide with polarity, thermal lability or low volatility, this LC‐MS/MS method has an advantage over GC. In this work, residual pesticides were extracted from the tea sample with ACN and then purified using Carb‐NH₂ SPE cartridges. Using the multiple reaction monitoring mode, the pesticides were quantified and identified by the most abundant and characteristic fragment ions. The recoveries obtained for each pesticide ranged between 65 and 114% at three spiked concentration levels. The intra‐day precisions were lower than 19.6%. Good linear relationships were observed with the correlation coefficients r² >0.996 for all analytes. The established method was successfully applied to the determination of pesticide residues in real tea samples.     

Quantification of urinary etheno-DNA adducts by column-switching LC/APCI-MS/MS

Lipid peroxidation induced etheno-DNA adducts are promutagenic and have been suggested to play a causal role in the development of human cancers. Therefore, human biomonitoring of etheno-DNA adducts in urine has been suggested as a potential marker for oxidative stress-related DNA damage. For quantitative determination, a column-switching LC/APCI-MS/MS method was developed for simultaneous analysis of epsilonAde, epsilondC, and epsilondA in human urine. Quantitative validation parameters (precision, within-day repeatability, and between-day reproducibility) yielded satisfactory results below 10%. Limit of quantification for epsilonAde, epsilondC, and epsilondA was 5.3 fmol, 7.5 fmol, and 1.3 fmol on column, respectively. Mean urinary excretion rates of a six healthy volunteers were 45.8 pmol epsilonAde/24 h, 96.8 pmol epsilondC/24 h, and 18.1 pmol epsilondA/24 h. The demonstrated levels of performance suggest a future applicability of this method to studies of cancer and other diseases related to oxidative stress in humans. To our knowledge, this is the first method described that allows simultaneous determination of epsilonAde, epsilondC, and epsilondA in human urine samples.     

SPE-HPLC和HPLC-ESI/MS法测定食品中微量苏丹红

采用商品化固相萃取柱富集纯化样品,建立了高效液相色谱测定食品中苏丹红的方法,并通过液质联用进行确证.采用外标法定, 平均回收率为90.2%～96.5%,相对标准偏差1.1%～2.3%.苏丹红Ⅰ、苏丹红Ⅱ、苏丹红Ⅲ、苏丹红Ⅳ的检出限分别为0.01、 0.01、 0.02、 0.02 μg/mL.     

Simultaneous determination of sixteen underivatized biogenic amines in human urine by HPLC-MS/MS

The broad group of biogenic amines includes polyamines and catecholamines, whose presence in human tissues and biological fluids can give important diagnostic information and act as marker of many pathologies. In particular, polyamines are involved in cancer cell growth while catecholamines act as neurotransmitters and hormones. Their simultaneous determination in biological tissues and fluids is therefore an important task. A high-performance liquid chromatography tandem mass spectrometry method is presented here for the simultaneous determination in urine of 16 biogenic amines: adrenaline (epinephrine), agmatine, cadaverine, dopamine, histamine, 3-methoxytyramine, noradrenaline (norepinephrine), norephedrine, octopamine, 2-phenylethylamine, putrescine, serotonin, spermidine, spermine, tryptamine, and tyramine. The method does not require any derivatization step. To guarantee the maximum of sensitivity, the mass spectrometer works in selected reaction monitoring mode, monitoring for each analyte the two most intensive transitions. Method validation includes the evaluation of limits of detection (that range from 0.3 to 6.6 μg L^?1), limits of quantitation (that range from 1.0 to 21.9 μg L^?1), linearity range (three orders of magnitude), recovery, intra- and inter-day precision on both concentration, and retention time. Recovery (R) is shown not to depend on the analyte concentration: the average R percent ranges from 72.9 to 100.0 %. Particular attention is devoted to the matrix effect and the correlated phenomena of ion enhancement or suppression in mass spectrometry detection.

液相色谱-质谱联用法测定牛奶中14种青霉素及相应青霉噻唑酸残留量

利用超高效液相色谱-串联质谱法(UPLC-MS/MS)同时测定牛奶中的7种青霉素类抗生素以及7种相应的青霉噻唑酸。样品经乙腈沉淀蛋白,上清液N2吹干后,用水溶解,加入正己烷萃取除去脂肪;提取液经ACQUITY UPLCBEH C18柱分离,乙腈-乙酸铵+甲酸水溶液洗脱。14种物质峰分离良好,定量限范围在5～20μg/kg。在10～50ng/mL质量浓度范围内线性良好,相关系数均大于等于0.999,牛奶中的加标回收率在90%～98%。     

Rapid determination of three anticoagulant rodenticides in whole blood by liquid chromatography coupled with electrospray ionization mass spectrometry

A rapid, sensitive and selective method for the simultaneous determination of bromadiolone, flocoumafen and brodifacoum in whole blood using warfarin as internal standard (IS) by high-performance liquid chromatography coupled with electrospray ionization mass spectrometry (HPLC/ESI-MS) has been developed and validated. The target compounds were extracted from the whole blood with ethyl acetate and separated on an XDB C18 column (150 mm x 2.1 mm i.d. x 5 microm) by using a mobile phase consisting of 0.2% acetic acid/methanol (12/88, v/v) at a constant flow rate of 0.50 mL/min. The analytes were detected using negative ESI-MS in the selected ion monitoring (SIM) mode. The molecular ions [M-H]- of m/z 527, 541,523 and 307 were selected for the quantification for bromadiolone, flocoumafen, brodifacoum and the IS, respectively. The calibration curves were linear (r2 > 0.995) in the concentration range of 0.50-100.00 ng/mL. The method showed a satisfactory sensitivity (0.05-0.5 ng/mL using 200 microL blood), precision (RSD < 11.9%), accuracy (recovery: 82.0-96.1%) and selectivity. This method was successfully applied to the determination of the analytes for the diagnoses of poisoned human beings and animals.     

Multiresidue determination of triarylmethane and phenothiazine dyes in fish tissues by LC-MS/MS

The occurrence of residues of malachite green and its leuco-metabolite in tissues of farmed fish for human consumption have long been of concern and there is extensive literature on methods of analysis and surveillance for these compounds. Recently, concern has been expressed that the use of other related compounds in place of malachite green may go undetected. This paper describes a new method for extending the range of triarylmethane and related phenothiazine dyes that can be detected in fish. In this procedure 13 parent compounds are monitored, with any potential leuco-forms being oxidized back to the parent prior to determination. The method utilizes a buffer–acetonitrile extraction followed by liquid–liquid extraction. Oxidant is added and the extracts further purified by cation exchange chromatography. Final determination is carried out using LC–MS/MS. The method has been validated to the standards of Commission Decision 2002/657/EC.     

SPE-UPLC-MS/MS同时测定水环境中4大类15种抗生素EI北大核心CSCD

建立了应用固相萃取-超高效液相色谱-串联质谱技术(SPE-UPLC-MS/MS)同时测定水环境中包括磺胺类、四环素类、大环内酯类和喹诺酮类在内的4大类15种抗生素的方法。采集的水样中加入同位素替代物后通过HLB固相萃取柱进行富集浓缩,UPLC-MS/MS进行测定,并采用内标法定量。结果表明,15种抗生素在0.5~50μg/L线性范围内检出限为0.04~0.09 ng/L,定量限为0.16~0.36 ng/L,样品加标回收率为59.5%~102.8%,相对标准偏差(RSD)均小于12%。该方法适用于水环境中痕量残留的抗生素检测。     

Simultaneous UPLC‐MS/MS determination of antiepileptic agents for dose adjustment

Therapeutic drug monitoring (TDM) of anti‐epileptic drugs (AED) is a routine application. Carbamazepine (CRB) is monitored as the parent drug while oxcarbazepine (OXC) and eslicarbazepine acetate (ESL) are monitored as their active metabolite (eslicarbazepine; MHD). We have developed a UPLC‐MS/MS method for determining CRB, OXC, ESL and MHD in plasma or serum with a simplified extraction protocol. The developed method detects sildenafil (SLD), which clinically interferes with AED and is likely to be co‐administered in epileptic patients suffering from sexual insufficiency (60%). MHD was prepared in‐house. AED were simultaneously determined in presence of SLD using gatifloxacin as an internal standard (IS). Separation was achieved using acetonitrile, methanol and 100 mm ammonium acetate in water (32:3:65, v /v/v) on an Intersil^®RP‐HPLC column (250 × 4.6 mm, 5 μm). A one‐step extraction was performed by simultaneous protein and phospholipids precipitation. Detection was done by tandem mass spectrometry. No relative matrix effect was observed. The method was linear (0.5–40 μg/mL for CRB, ESL and MHD and 0.05–4 μg/mL for OXC), accurate and selective. Recoveries were 64.41 ± 5.07, 45.62 ± 1.73, 61.41 ± 4.77 and 60.33 ± 1.36 for CRB, OXC, ESL and MHD, respectively. The method was successfully applied for TDM of AED.     

Simultaneous determination of major type‐B trichothecenes and the de‐epoxy metabolite of deoxynivalenol in chicken tissues by HPLC–MS/MS

In this study, a specific and sensitive LC–MS/MS method for the simultaneous analysis of type‐B trichothecenes (deoxynivalenol, 3‐acetyldeoxynivalenol, and 15‐acetyldeoxynivalenol) and the de‐epoxy metabolite of deoxynivalenol (de‐epoxy‐deoxynivalenol) in chicken muscle, liver, kidney, and fat tissues was developed and validated. The method involved an extraction step using ethyl acetate, followed by the evaporation of the supernatant, which was further purified by an Oasis HLB SPE cartridge (Waters, Milford, MA, USA). Chromatographic separation was performed on a C₁₈ column by detection with MS in multiple‐reaction monitoring mode and using a gradient elution program with 0.1% formic acid in water and methanol. The correlation coefficients (r) for each calibration curve were >0.99 within the experimental concentration range. The extraction recoveries ranged from 73.7 to 106.4%, with intraday and interday RSD < 11.6% at three levels of concentrations of 2, 10, and 100 μg/kg. The decision limits and the detection capabilities of the analytes in the chicken tissues ranged from 0.16 to 0.92 and 0.68 to 2.07 μg/kg, respectively. The results demonstrated the applicability of this sensitive procedure to the determination of trichothecenes in chicken tissue samples.     

Simultaneous determination of sulfoxaflor in 14 daily foods using LC-MS/MS

Sulfoxa?or residues in 14 daily foods, including rice, sorghum, chilli, cucumber, white pear, apple, egg, beef brisket, chicken breast, fish, pork liver, milk, pine nut and honey, were simultaneously determined using a modified QuEChERS and LC–MS/MS method. These foods were classified into three categories to be purified. A combination of 25 mg of octadecylsilane (C18) + 25 mg of primary and secondary amine (PSA) + 50 mg of graphitised carbon black (GCB) + 150 mg of MgSO₄ was used to purify the rice, sorghum, honey, apple and white pear. A combination of 25 mg of C18 + 50 mg of PSA + 50 mg of GCB + 150 mg of MgSO₄ was used to purify the chilli and cucumber. A combination of 50 mg of C18 + 25 mg of PSA + 50 mg of GCB + 150 mg of MgSO₄ was used to purify the pine nuts, egg, beef brisket, chicken breast, fish, pork liver and milk. The linearity coefficient values were greater than 0.9975. The limit of detection and limit of quantification were in the ranges of 0.7?1.8 and 2.0?5.0 μg kg^?1, respectively. Average recoveries of the sulfoxa?or at the 14 food matrices at spiking levels of 5.0, 10 and 50 μg kg^?1 ranged from 74.0% to 100.8%, and the relative standard deviation ranged from 2.2% to 11.2%. This is a simple and rapid method for the determination of sulfoxa?or residues in various kinds of daily foods.     

Simultaneous determination of 32 antibiotics in aquaculture products using LC-MS/MS

An analytical multiclass, multi-residue method for the determination of antibiotics in aquaculture products was developed and validated. A fast, cheap, and straightforward extraction procedure followed by liquid chromatography-tandem mass spectrometry analysis was proposed. This method covers 32 antibiotics of different classes, which are frequently used in aquaculture. Three different extraction procedures were compared, and the extraction with acetonitrile (0.1 vol. % formic acid) showed the best results. The selected extraction procedure was validated at four different fortification levels (10 μg kg^?1, 25 μg kg^?1, 50 μg kg^?1, and 100 μg kg^?1). Recoveries of the tested antibiotics ranged from 70 % to 120 %, with the relative standard deviation (RSD) of triplicates lower than 20 %. The limits of quantification (LOQ) ranged from 0.062 μg kg^?1 to 4.6 μg kg^?1, allowing for the analysis of trace levels of these antibiotics in aquaculture products. The method was applied to the analysis of selected antibiotics in fish and shrimp meat available in the Czech market.     

In Vitro Anti-Diabetic Activities and UHPLC-ESI-MS/MS Profile of Muntingia calabura Leaves Extract

Anti-diabetic compounds from natural sources are now being preferred to prevent or treat diabetes due to adverse effects of synthetic drugs. The decoction of Muntingia calabura leaves was traditionally consumed for diabetes treatment. However, there has not been any published data currently available on the processing effects on this plant’s biological activity and phytochemical profile. Therefore, this study aims to evaluate the effect of three drying methods (freeze-drying (FD), air-drying (AD), and oven-drying (OD)) and ethanol:water ratios (0, 50, and 100%) on in vitro anti-diabetic activities of M. calabura leaves. In addition, an ultrahigh-performance-liquid chromatography–electrospray ionization tandem mass spectrometry (UHPLC-ESI-MS/MS) method was used to characterize the metabolites in the active extract. The FD M. calabura leaves, extracted with 50% ethanol, is the most active extract that exhibits a high α-glucosidase and α-amylase inhibitory activities with IC₅₀ values of 0.46 ± 0.05 and 26.39 ± 3.93 µg/mL, respectively. Sixty-one compounds were tentatively identified by using UHPLC-ESI-MS/MS from the most active extract. Quantitative analysis, by using UHPLC, revealed that geniposide, daidzein, quercitrin, 6-hydroxyflavanone, kaempferol, and formononetin were predominant compounds identified from the active extract. The results have laid down preliminary steps toward developing M. calabura leaves extract as a potential source of bioactive compounds for diabetic treatment.     

离子色谱-柱切换技术同步测定饮料中的三氯蔗糖、葡萄糖、果糖和蔗糖

建立了一种离子色谱-柱切换-安培检测技术同步测定饮料中三氯蔗糖、葡萄糖、果糖和蔗糖的方法。以CarboPac PA10阴离子交换保护柱和分析柱进行分离,用水和250 mmol/L NaOH梯度淋洗,脉冲安培检测。弱保留糖类在25 mmol/L NaOH流动相淋洗下分离检测,通过柱切换将保护柱切换至分析柱后,同时切换至250 mmol/L NaOH淋洗,三氯蔗糖仅通过较短的保护柱分离,4种糖类能够得到同步检测。4种糖类在0.01~20 mg/L范围内有良好的线性关系和较低的检出限,重复性好,样品测定的回收率分别为90.38%~102.88%（三氯蔗糖）、95.56%~102.75%（葡萄糖）、101.66%~114.33%（果糖）和105.03%~106.49%（蔗糖）。该方法可广泛应用于食品中强保留物质的测定。     

Simultaneous determination of uric acid and creatinine in biological fluids by column-switching liquid chromatography with ultraviolet detection

A column-switching liquid chromatographic method for the simultaneous determination of uric acid and creatinine in human serum and urine was developed. Creatinine and uric acid were separated by size-exclusion chromatography on a hydrophilic gel column (C1) and creatinine eluted from Cl was separated from proteins by filtration through a longer hydrophilic gel column (C2). The creatinine fraction eluted from C2 was transferred to a weakly acidic cation-exchange column (C3) and then to a strongly acidic cation-exchange column (C4). Uric acid eluted from Cl after creatinine was transferred to an anion-exchange column (C5) and then to a hydrophilic gel column (C6). The mobile phase was a mixed buffer of pH 5.1 (propionic acid-succinic acid-NaOH, 60:15:60 mmol/1 in water). Diluted serum and urine could be injected onto C1, and Cl was backflushed after the transfer of uric acid from Cl to C5.

Creatinine and uric acid in the eluate were determined by measuring their ultraviolet absorption at 234 and 290 nm, respectively. The recovery of uric acid and creatinine added to diluted serum (20-fold dilution, concentration 20 and 5 μmol/1, respectively) was 98.9±0.56% and 100.9±1.29%, respectively. The recovery of uric acid and creatinine added to diluted urine (100-fold dilution, concentration 50 and 100 μmol/l, respectively) was 99.4±0.72% and 98.7±1.45%, respectively (mean±R.S.D., n=6).