Simultaneous Determination of 14 β-Receptor Agonists Residues in Mutton by High Performance Liquid Chromatography-Tandem Mass Spectrometry (HPLC-MS/MS)

[Objectives]A high performance liquid chromatography-tandem mass spectrometry(HPLC-MS/MS)method was established for the determination of 14β-receptor agonist residues in mutton.[Methods]Samples were hydrolyzed byβ-glucuronidase and extracted with 5%acetic acid-acetonitrile(1:99,V/V)solution.An Eclipse plus C 18 column was used for separation,and the MRM mode was used for qualitative analysis,and the external standard method was used for quantitative analysis of matrix standard solutions.[Results]Under the optimal conditions,the retention time of the 14 kinds ofβ-receptor agonists ranged from 1.0 to 9.5 min.When the mass concentration was in the range of 0.05-0.50μg/ml,the linear relationship ofβ-receptor agonists was good,with correlation coefficients(r)≥0.9992.The detection limits of the method were in the range of 0.04-0.87μg/kg,and the quantitative limits were in the range of 0.35-1.86μg/kg.The average recovery values were in the range of 82.8%-108.9%,with RSDs(n=6)in the range of 1.9%-6.7%.[Conclusions]The method is simple,sensitive,reproducible,accurate,and can be used for simultaneous determination of the 14 kinds ofβ-receptor agonist residues in mutton.

Determination of urine catecholamines and metanephrines by reversed-phase liquid chromatography-tandem mass spectrometry

The measurement of urine catecholamine and metanephrine concentrations is important for biochemical screening and diagnosis of pheochromocytoma.The goal of this work was to develop a simple liquid chromatography-tandem mass spectrometry(LC-MS/MS)method for determining catecholamines and metanephrines in urine to replace an existing liquid chromatographic method using electrochemical detection.Urine samples were prepared using Oasis weak-cation-exchange cartridges.The eluate was analyzed on an Agilent ZORBAX Eclipse Plus Phenyl-Hexyl column in 3 min.Adrenaline,noradrenaline,dopamine,metanephrine,normetanephrine,and their deuterated internal standards were monitored in positive electrospray ionization mode by multiple reaction monitoring(MRM).No evidence of ion suppression was observed.The assay was linear up to 5μmol/L for adrenaline,5μmol/L for noradrenaline,6.1μmol/L for dopamine,5.6μmol/L for metanephrine,and 34.6μmol/L for normetanephrine,with lower limits of quantification of 5,5,12,6 and 7nmol/L,respectively.The intra-day and inter-day precisions for all analytes ranged from 0.59%to 4.64%and1.98%to 4.80%,respectively.External quality assurance samples were assayed and showed excellent agreement with the target values.This simple method provides an improved assay for determining urine catecholamines and metanephrines.

Stable Isotope Dilution Analysis of Gibberellin Residues in Tomato Paste by Liquid Chromatography-Tandem Mass Spectrometry

An accurate and sensitive method for the simultaneous determination of gibberellic acid（GA3）, gibberellin A4（GA4） and gibberellin A7（GA7） residues in tomato paste was developed by coupling solid phase extraction to high performance liquid chromatography-tandem mass spectrometry（LC-MS/MS） with electrospray ionization based stable isotope dilution analysis（SIDA）. The isotope labeled internal standard can compensate for the losses during the extraction and cleanup steps and for discrimination due to ion suppression. After extraction from methanol, hydrophile lipophilic balance（HLB） solid phase extraction（SPE） column was tested for the capacity of the cleanup of the tomato paste in compared with C18 SPE column which is the common way to the detection of GAs, and the former gained better result. Spiked experiments were performed in the non-contaminated tomato pastes and the recoveries of GA3, GA4 and GA7 were 42.6%―75.0% in external standard method（ESM） and 91.1%―103.8% in internal standard method（ISM） respectively. The validities of this method were investigated and good analytical performance for the three GAs was obtained, including low limits of method detection（2 ng/g for GA3 and GA4, 0.3 ng/g for GA7）, excellent linear dynamic ranges（5―500 ng/g for GA3 and GA4, 1―100 ng/g for GA7） and good relative standard deviation ranges（4.8%―9.4% for the intra-day test and 3.5%―11.9% for the inter-day test）.

Liquid Chromatography-Tandem Mass Spectrometry Assay to Detect Ethyl Glucuronide in Human Fingernail: Comparison to Hair and Gender Differences

Over the past decade, the use of hair specimens for the long-term detection of the alcohol biomarker ethyl glucuronide has been increasing in popularity and usage. We evaluated the usefulness of fingernail clippings as a suitable alterna-tive to hair for ethyl glucuronide detection. A liquid chromatography-tandem mass spectrometry method for the detection of ethyl glucuronide in fingernail clippings was fully validated and used to analyze the hair and/or fingernail specimens of 606 college-aged study participants. The limit of detection was 2 pg/mg, the limit of quantitation was 8 pg/mg and the method was linear from 8 to 2000 pg/mg. Intra- and inter-assay imprecision studies at three different concentrations (20, 40, 200 pg/mg) were all within 7.8% and all intra- and inter-assay bias studies at these levels were within 115.1% of target concentration. Ethyl glucuronide levels in fingernail (mean = 29.1 ± 55.6 pg/mg) were higher than ethyl glucuronide levels in hair (mean = 9.48 ± 22.3 pg/mg) and a correlation of the matched pairs was observed (r = 0.552, P < 0.01, n = 529). Evaluating each gender separately revealed that the correlation of male fingernail to male hair was large and significant (r = 0.782, P < 0.01, n = 195) while female hair to female fingernail was small yet sig-nificant (r = 0.249, P < 0.01, n = 334). The study results demonstrated that fingernail may be a suitable alternative to hair for ethyl glucuronide detection and may be the preferred sample type due to the lack of a gender bias.

Rapid and Sensitive Liquid Chromatography-Tandem Mass Spectrometry for Quantification of Glycyrrhetic Acid in Human Plasma

A simple, rapid and sensitive liquid chromatography-tandem mass spectrometry（LC-MS/MS） for the determination of glycyrrhetic acid in human plasma with ginsenoside Rh2 as internal standard was developed and validated. The plasma samples were prepared via liquid-liquid extraction with ethyl acetate. Chromatographic separation was accomplished on a Venusil MP-C18（50 mm×2.1 mm, 5 μm i.d.） column at 25 °C. The mobile phase consisted of acetonitrile/5 mmol？L-1 ammonium acetate（10：90, volume ratio） at a flow rate of 0.4 mL/min. Negative electrospray ionization was utilized as the ionization source. Glycyrrhetic acid and internal standard were determined via the mutiple reaction monitoring of precursor→production ion transitions at m/z 469→425, 409 and m/z 621→161, respectively. Each sample was chromatographed within 2.5 min. The lower limit of quantification was 0.50 ng/mL for 200 μL of plasma sample and the linear range was from 0.50 ng/mL to 800 ng/mL. The intra- and inter-day precisions were less than 8.76% in terms of relative standard deviation（RSD）, and the accuracy was within a range of -3.25%-1.32% in terms of relative error（RE）. The method was successfully applied to the pharmacokinetic studies of glycyrrhetic acid in healthy male Chinese volunteers after a single oral administration of 75 mg of glycyrrhizin.

Determination of okadaic acid related toxins from shellfish (<i>sinonovacula constricta</i>) by high performance liquid chromatography tandem mass spectrometry

Consumption of shellfish contaminated with algal toxins produced by marine dinoflagellates can lead to diarrhetic shellfish poisoning (DSP). It was therefore essential that there are analytical techniques to identify and quantify DSP toxins in shellfish. This new methodology could facilitate DSP monitoring and create a means of rapidly responding to incidents threatening public health. In the last years there were different analytical methods for DSP, such as mouse bioassay and LC-FLD. With the development of instrument, Liquid chromatography-mass spectrometry was substituted for other analytical methods with its good sensitivity and selectivity and without derivatization for the determination of DSP. In this report, a high performance liquid chromatogra-phytandem mass spectrometric(HPLC-MS/MS)method was developed for the simultaneous determination of okadaic acid (OA) and dinophysistoxins(DTX1) in Sinonovacula constricta. Optimization of pretreatment experiment was carried out to maximize recoveries and the effectiveness. The analytes were determined under multi-reactions monitoring (MRM) scan type with tandem mass analyzer using negative ion electrospray ionization (-ESI) mode .Finally, the detection and identification of OA and DTX-1 were based upon their retention times (RT) and the fragmentation patterns of their mass spectra. The method of LOQ for the two poisons was 0.02 mg·kg-1.The real sample test showed that this method could be used for sensitive, fast, and accurate determination of the two diarrheic shellfish poisons in shellfish.

LC-MS/MS法同时测定人血浆中氯吡格雷及其羧酸代谢物的浓度

目的建立快速测定人血浆中氯吡格雷及其羧酸代谢物SR26334含量的LC-MS/MS法。方法乙醚-正己烷(4:1,V:V)2次液-液提取法(中性和酸化条件下),采用Teknokroma C_(18)色谱柱,以那格列奈和吡格列酮为内标,同时测定血浆中氯吡格雷和SR26334的浓度。流动相:甲醇-0.1%甲酸(80:20,V:V);流速:0.2mL·min^(-1);以多反应离子监测方式检测:氯吡格雷[M+H]^+,m/z 322.1→212.1;那格列奈[M+H]^+,m/z 318.3→166.2;氯吡格雷羧酸代谢物SR26334[M+H]^+,m/z 308.1→q98.1;吡格列酮[M+H]^+,m/z 357.2→134.2。结果氯吡格雷和内标那格列奈的保留时间分别在4.4和3.7min,SR26334和内标吡格列酮的保留时间分别在1.3和1.7min,氯吡格雷的线性范围为5～5000ng·L^(-1);SR26334的线性范围为20～2500μg·L^(-1)。提取回收率大于75%,方法回收率大于90%,日内、日间RSD小于10%(n=5)。结论本方法简便快速,适用于氧吡格雷制剂的新药临床研究和临床长期治疗病人血药浓度的常规监测。

LC-MS/MS法测定地氯雷他定的浓度及其在生物等效性研究中的应用

目的建立液相色谱-串联质谱(LC-MS/MS)法测定人血浆中地氯雷他定的浓度,并应用于2种地氯雷他定制剂的人体生物等效性研究。方法采用双周期自身随机交叉试验设计,18名男性健康志愿者分别单剂量口服地氯雷他定口腔崩解片(受试制剂)和地氯雷他定片(参比制剂)10 mg,采用LC- MS/MS法测定人血浆中地氯雷他定的浓度,利用3P97程序计算主要药动学参数,并对2种制剂进行生物等效性评价。结果受试制剂和参比制剂的t_(max)分别为(2.8±s 0.6)和(2.9±0.6)h,c_(max)分别为(4.8±2.1)和(5.0±2.2)μg·L^(-1),A UC_(0～96)分别为(59±30)和(58±26)μg·h·L^(-1),A UC_(0～∞)分别为(64±29)和(62±26)μg·h·L^(-1)。受试制剂的相对生物利用度为(103±32)%。经统计学检验,2种制剂的主要药动学参数间无显著差异。结论所建立的LC-MS/MS法适合于人体血浆中地氯雷他定的测定。地氯雷他定受试制剂和参比制剂具有生物等效性。

用HPLC-MS/MS法测定人血浆中的二甲双胍浓度

目的：建立高效液相色谱-质谱／质谱（HPLCMS／MS）联用法测定人血浆中二甲双胍浓度的方法。方法：血浆样品经乙腈沉淀蛋白质后，用HPLC—MS／MS法测定二甲双胍浓度。甲醇-乙腈10mmol／L乙酸铵溶液（20：20：60）为流动相，流速为0．2mL／min；采用大气压化学电离源，以多离子反应监测（MRM）方式进行正离子检测，二甲双胍和内标苯乙双胍的定量分析离子对分别为m／z 130．2→71．0和m／z 206．1→59．9。结果：血浆样品中二甲双胍线性范围为2．0～2000μg／L（n=7，r=0．9996），最低定量限为2．0μg／L。低、中、高（10、500、1500 μg／L）3种浓度的日内RSD分别为4．65％、2．84％和3．41％（n=5）；日间RSD分别为7．96％、3．98％和4．77%（n=5）；准确度为95．9％、97．4％和89．90%（n=5）。结论：本方法灵敏度高、专属性强、重现性好、准确，可用于人血浆中二甲双胍的含量测定。

LC-MS/MS测定尿液中可卡因及其代谢物苯甲酰爱康宁

目的建立尿液中可卡因(cocaine,COC)及其代谢物苯甲酰爱康宁(benzoylecgonine,BZE)的液相色谱-串联质谱分析方法。方法尿液经固相萃取后,用AllurePFP丙基柱分离,以V(甲醇):V(20mmol/L乙酸胺和0.1%甲酸的缓冲溶液)=80∶20为流动相,采用二级质谱多反应监测模式检测COC和BZE。按10mg/kg的剂量对豚鼠腹腔注射可卡因,给药后收集7d尿液。结果尿液中COC和BZE在2.0～100ng/mL质量浓度范围内线性关系良好(r=0.9995),最低检测限(LOD)为0.5ng/mL;回收率大于90%;日内和日间精密度均小于6%;豚鼠尿液中主要检测目标物是BZE,且BZE检测时限也较COC长。结论所建方法灵敏度高,选择性好,适用于尿液中可卡因和苯甲酰爱康宁的检测。

LC-MS-MS同时定量检测硒蛋氨酸和硒胱氨酸

目的建立同时测定硒蛋氨酸(SeMet)和硒胱氨酸(SeCys)含量的液相色谱-串联质谱法(LC-MS-MS)。方法色谱柱:Waters Symmetry C18(150mm×3.9mm,5μm);流动相:甲醇+0.1%七氟丁酸水溶液(35+65),流速为500μl/min;以氮气为碰撞气,利用多反应离子监测方式测定SeMet(MRMm/z198.1→181.0,198.1→152.0)和SeCys(MRMm/z337.0→248.0,337.0→88.2)信号。结果SeCys和SeMet检出限分别为2.0ng/ml和0.5ng/ml;以198.1→181.0为定量分析离子对,SeMet的线性回归方程为:y=707x+990,r=0.9993;以337.0→248.0为定量分析离子对,SeCys的线性回归方程为:y=64.3x+695,r=0.9999。结论该方法能够使2种含硒化合物在一次进样中实现完全分离和在线测定,能够满足快速准确检测SeCys和SeMet含量要求。

LC-MS法研究尼莫地平脂质体原位凝胶在家兔体内的药动学

目的研究尼莫地平脂质体原位凝胶在家兔体内的药动学。方法单剂量(尼莫地平0.5 mg·kg^(-1))于家兔后腿股四头肌肌内注射尼莫地平溶液剂、尼莫地平脂质体、泊洛沙姆188(P188)修饰的尼莫地平脂质体和尼莫地平脂质体原位凝胶,建立高效液相色谱-质谱(LC-MS)法测定血浆中尼莫地平的浓度。结果尼莫地平在0.8～800μg·L^(-1)范围内线性关系良好(r=0.999 2),提取回收率大于90%,日内、日问精密度RSD<15%。尼莫地平脂质体原位凝胶和脂质体的c_(max)分别为(88±s 18)和(224±64)μg·L^(-1);t_(max)分别为(2.0±0.7)和(0.29±0.14)h;AUC_(0-∞)分别为(402±15)和(273±28)μg·h·L^(-1)。尼莫地平脂质体原位凝胶的c_(max)、t_(max)、AUC_(0-∞)等药动学参数与尼莫地平脂质体和P188修饰的尼莫地平脂质体均有显著或极显著差异。结论尼莫地平脂质体原位凝胶经肌内注射后可延长药物在体内的驻留时间,具有一定的缓释作用并提高了尼莫地平的生物利用度。

HPLC-MS法评价2种茴拉西坦胶囊的人体生物等效性

目的建立HPLC-MS法测定人血浆中茴拉西坦的活性代谢物对甲氧基苯甲酰氨基丁酸(ABA)的浓度,比较2种茴拉西坦胶囊的人体生物等效性。方法 24名健康男性志愿者单剂量交叉口服受试制剂或参比制剂200 mg,采用HPLC-MS法测定血浆中不同时间点茴拉西坦代谢物ABA的血药浓度,计算主要药代动力学参数及相对生物利用度,评价2种制剂的生物等效性。结果受试制剂和参比制剂的主要药动学参数:Cmax分别为(9.30±5.13)和(8.70±3.17)μg/ml;tmax分别为(38.41±17.89)和(39.09±19.92)min;t1/2分别为(37.21±10.51)和(38.45±9.24)min;AUC0-t分别为(555.21±157.10)和(545.39±97.22)μg/(ml.min);AUC0-∞分别为(566.24±158.01)和(554.71±100.32)μg/(ml.min)。以AUC0-t和AUC0-∞计算,受试制剂的相对生物利用度F0-t和F0-∞分别为(101.22±17.17)%和(101.52±16.63)%。2种制剂的主要药代动力学参数差异无统计学意义。结论 2种茴拉西坦胶囊具有生物等效性。

LC-MS/MS法测定大鼠脑微透析液中7-乙基-10-羟基喜树碱的浓度

目的:建立一种能够测定大鼠脑微透析液中7-乙基-10-羟基喜树碱(7-Ethyl-10-Hydroxycamptothecin,SN-38)浓度的分析方法。方法:采用LC-MS/MS法,色谱柱为Agilent EclipsePlus C18反相柱(2.1 mm×100 mm,1.8μm);流动相为乙腈-0.1%甲酸,梯度洗脱;流速为0.3 ml/min;柱温为35℃。采用电喷雾离子化,多反应监测(multiple reaction monitoring,MRM)测定大鼠脑微透析液中SN-38(m/z 393.1→349.1)的浓度。结果:空白透析液无干扰;SN-38在0.1015～1015 ng/ml范围内线性关系良好(r=0.9995),定量下限为0.1015 ng/ml;回收率为97.54%～100.60%;精密度和稳定性均良好;脑微透析液中SN-38的浓度呈明显药动学过程,给药220 min后达到顶峰。结论:本实验所建立的LC-MS/MS分析方法专属性强、灵敏度高,可用于分析大鼠脑微透析液中SN-38的浓度。

QuEChERS法与UPLC-MS/MS法对土壤中五种磺酰脲类除草剂的快速检测

建立了一种土壤中5种磺酰脲类除草剂高效、快速、灵敏的检测方法。土壤中的磺酰脲残留物似因嘧磺隆、甲磺隆、绿磺隆、胺苯磺隆和苄嘧磺隆）采用缓冲盐改进的OuEChERS法提取．乙腈提取液经浓缩、甲醇／水（1／1，V/V）混合溶剂定容后进入超高效液相色谱一串联质谱（UPLC-MS／MS）进行分析。在优化好的色谱和质谱条件下，对基质效应进行了考察，结果表明。所有分析物体现了明显的基质减弱效应．采用基质匹配的校准曲线进行定量分析。在0．2～100．0μg／kg内，5种磺酰脲除草剂线性方程的R^2大于0．9969，定量限为0．07—0．10μg／kg。在低、中、高3种添加浓度的回收率为75．9％-94．0％，日内日间相对标准偏差小于11．5％．表明所建立的方法在土壤中磺酰脲除草剂的检测上具有潜在的应用前景．

HPLC-MS分析解毒化瘀中药组方水煎液乙酸乙酯分离部分化学成分

目的分析解毒化瘀中药组方水煎液乙酸乙酯分离部分化学组分。方法采用高效液相色谱-质谱联用（HPLC-MS）法,以甲醇-水为流动相,梯度洗脱,流量为1mL·min-1,采用ESI正离子模式进行质谱检测,相对分子质量扫描范围为50~1 000m/z。将检测得到的相对分子质量数据与Aglient中药成分数据库比对,对相似度得分在80%以上的化合物进行文献及来源药材成分检索,鉴定化合物。结果共鉴定出2-O-桂皮酰基-β-葡萄糖、淫羊藿属甙C、大黄二蒽酮A、欧芹脑、9,10-二甲氧基紫檀烷-3-O-β-D-葡萄糖甙、葛缕酮等18种化合物,2-O-桂皮酰基-β-葡萄糖、大黄二蒽酮A、大黄酚来源于大黄;9,10-二甲氧基紫檀烷-3-O-β-D-葡萄糖甙、异微凸剑叶莎醇、熊竹素来源于黄芪;欧芹脑、葛缕酮、茵陈蒿B来源于茵陈;淫羊藿新甙C、1,2-双（4-羟基-3-甲氧基苯基）-1,3-丙二醇来源于淫羊藿。7,9（11）-去氢茯苓酸、藜芦醇、赛仙鹤草酚C分别来源于茯苓、虎杖、仙鹤草;苍术内酯I来源于白术;决明萘乙酮-8-O-β-D-葡萄糖甙来源于虎杖和大黄;槲皮素来源于仙鹤草、淫羊藿、茵陈。结论采用HPLCMS法可明确中药组方水煎液乙酸乙酯分离部分的化学组分,为解毒化瘀中药组方的临床应用提供了理论依据。

UPLC-MS/MS法检测中药制剂中的27种非法添加化药成分

该文建立UPLC-MS/MS法同时检测减肥类、壮阳类、降糖类、解热镇痛类中药制剂中易被添加的27种化药成分。样品用甲醇提取,采用Agilent Eclipse Plus C18 RRHD色谱柱(3.0 mm×150 mm,1.8μm)分离,以0.1%甲酸水溶液和乙腈为流动相,梯度洗脱,流量0.5 mL/min,柱温35℃,进样体积1μL,采用电喷雾离子源(ESI),正离子模式,多反应监测(MRM)进行检测。所测27种非法添加化药成分在一定范围内呈良好的线性关系(r2>0.99),各组分均分离良好,低、中、高3个添加水平的平均回收率为80.4%~120.9%,相对标准偏差(relative standard deviation,RSD)为0.8%~7.8%,检出限0.0061~0.3750μg/g,定量限0.0204~1.2500μg/g。该方法专属性强、灵敏度高、操作简便,可用于中药制剂中27种非法添加化药成分的定量分析。

SPE-UPLC-MS/MS快速测定豆制品中的乌洛托品

建立了一种固相萃取-超高效液相色谱质谱联用(SPE-UPLC-MS/MS)测定豆制品中乌洛托品的分析方法。样品经粉碎后,采用乙腈提取,ProElut PXA小柱净化,Shim-pack XR-ODS色谱柱分离,在电喷雾正离子模式下用质谱仪进行MRM分析。结果表明:乌洛托品在0～160μg/kg范围内呈现良好的线性关系,线性相关系数为0.9998,该方法对应的检出限和定量限分别为0.3μg/kg和1μg/kg在5～100μg/kg添加水平下,乌洛托品回收率为88.4%～97.1%,相对标准偏差为5.39%～8.74%。该方法简便,快速,可成功应用于豆制品中乌洛托品的检测。

Determination of Residual Amount of 15 Plant Growth Regulators in Bean Sprouts by HPLC-MS/MS

[Objectives]This study was conducted to effectively monitor PGR residues in bean sprouts to provide guarantee for the food safety of agricultural products.[Methods]A high-performance liquid chromatography-tandem mass spectrometry(HPLC-MS/MS)method for the determination of residues of 15 plant growth regulators(PGRs)in bean sprouts was established using bean sprouts as an experimental material.Samples were extracted with a solution containing 5%acetic acid-acetonitrile(1∶99,V/V),purified with anhydrous magnesium sulfate,and diluted with methanol solvent to constant volume.The solutions were filtered through 0.22μm filtering membrane and the target analytes were separated on a Phenomenex H18 column.The identification of each compound was established by retention time matching along with the accurate mass measurement of the precursor ions and their main fragment ions.The quantification was carried out using matrix-matched external standard method.[Results]The retention time of the 15 PGRs were found in the range from 5.8-11.7 min under the optimized conditions.The linear relation was good in the concentration range of 0.005-0.050μg/ml,and the correlation coefficients of the 15 PGRs were≥0.9990.The limits of detection were in the range of 0.03-0.92 g/kg,and the limits of quantification were in the range of 0.50-2.10μg/kg.The average recovery in the recovery test at 3 concentration levels was 80%-110%,and the relative standard deviations were in the range of 2.8%-7.5%.[Conclusions]This method is simple and accurate,and can quickly qualitatively and quantitatively analyze the residues of 15 PGRs in bean sprouts.The proposed procedure was simple,quick and accurate for the simultaneous determination of the 15 PGRs in bean sprout.