HPLC-APCI(+)MS/MS分析动物源性食品中的硝基咪唑类药物残留量

运用高效液相色谱-大气压电离串联四极杆质谱(HPLC-APCI( )MS/MS)内标法分析动物源性食品中多种硝基咪唑类(nitroimidazoles)药物——甲硝唑(MNZ)、地美硝唑(DMZ)、替硝唑(TNZ)、洛硝唑(RNZ)的含量。样品添加氘代标示物HMMNI-D3、IPZ-OH-D3后,用乙腈提取,通过OASIS HLB C18SPE柱净化,Waters Sunfire C18色谱柱分离,采用梯度洗脱,流动相为0.1%甲酸水溶液和0.1%甲酸乙腈溶液;大气压电离源正离子MRM模式检测:MNZm/z172.0/82.1,172.0/128.0;DMZm/z142.0/81.1,142.0/96.1;TNZm/z248.0/121.0,248.0/93.1;RNZm/z201.0/140.0,201.0/110.0;IPZ-OH-D3m/z189.0/125.0,189.0/171.0;HMMNI-D3m/z161.0/58.0,161.0/143.1。方法定量下限(LOQ,S/N>10)0.2μg/kg,在质量浓度0.2~25.0μg/L范围内,峰面积与质量浓度成良好线性(r>0.999 1)。     

液相色谱-电喷雾电离质谱法测定水中的微囊藻毒素

通过固相萃取富集微囊藻毒素，并采用液相色谱-电喷雾电离质谱测定水中的微囊藻毒素-RR，-LR。分别在m／z为520．4、996．3时，采用选择离子扫描方式，提高检测灵敏度。该法检出限为0．01μg／L；线性定量范围为0．02～20μg／L。方法灵敏度高，实用性强，可为水质藻毒素风险评价和监测水处理脱毒效能，提供灵敏、准确的分析方法。     

高效液相色谱/串联质谱法测定奶粉中的硝基呋喃代谢物

用高效液相色谱／串联质谱（LC—MS／MS）法同时测定奶粉中呋喃唑酮、呋喃它酮、呋喃西林和呋喃妥因的代谢物。盐酸水解奶粉中蛋白结合的代谢物，同时加入2-硝基苯甲醛（2-NBA），37℃过夜衍生化。加入硫酸锌，调pH值至7．0后，再加入亚铁氰化钾去除蛋白。后用乙酸乙酯提取，正己烷净化，分析物采用电喷雾电离正离子（ESI＋）、多反应监测（MRM）模式检测，内标法定量。在添加浓度0．5—2μg/kg范围内，内标法回收率为89．5％～110．3％；相对标准偏差（RSD）小于11，3％。5-马啉代甲基-3-氨基-2-恶唑酮（5-methylmorpholino-3-amino-2-oxazolidinone，AMOZ）、3-氨基-2-恶唑酮（3-amino-2-oxazolidinone，AOZ）方法检出限为0．05μg／kg，氨基脲（semicarbazide，SEM）、1-氨基-乙内酰胺（1-amino—hydantoin，AHD）为0．1μg/kg。     

调味品中氯丙醇的GC/ECD和GC/MS/MS衍生化检测方法研究及应用

报道了调味品中氯丙醇的衍生化气相色谱(GC／ECD)和衍生化气相色谱双串联质谱法(GC／MS／MS)测定。GC／ECD测定酱油中3—氯—1，2—丙二醇(3—MCPD)的检出限达到0．01mg／kg，回收率为91％～104％，变异系数为2．27％～7．96％；GC／MS／MS同时测定酱油中1，3—二氯—2—丙醇、2，3—二氯—1—丙醇和3—氯—1，2—丙二醇，1，3—二氯—2—丙醇、2，3—二氯—1—丙醇的检出限为0．02mg／kg，3—氯—1，2—丙二醇的检出限为0．01mg／kg，回收率在92％～106％，变异系数为3．51％～13．33％。     

高效液相色谱-串联质谱联用测定富含淀粉食品中丙烯酰胺

以甲基阿烯酰胺作为内标物，用高效液相色谱／串联质谱（HPLC／MS／MS）法测定食品中的丙烯酰胺。均质后的食品样品，加入正己烷经液-液分配去除脂肪，用蒸馏水提取丙烯酰胺，Carrez试剂净化提取样品，净化液经离心后过0．45μm微孔滤膜，采用HPLC／MS／MS电喷雾电离（ESI），阳离子，多反应监测（MRM）模式检测，外标法定量。方法的线性范围为2～500μg／L，线性相关系数为0．9997，检出限为2μg／kg；高中低3个水平的加标回收率分别为99．4％、99．6％和98．4％；相对标准偏差（RSD）均小于7．8％。     

高效液相色谱-质谱法测定杜仲样品中环烯醚萜含量

建立了液相色潜-质谱联用测定不同杜仲样品中3种环烯醚萜类物质含量的方法。以50％的甲醇-水为溶剂采用超声波提取样品中的环烯醚萜类物质．采用选择离子方式（SIR），以丰度最高的[M＋Na]^＋特征离子作为监测离子进行定性和定量分析。其质荷比（m／z）分别为369（桃叶珊瑚甙，AU）、397（京尼平甙酸，GPA）和411（京尼平甙，GP）。方法的线性范围分别为AU：0．11～1．10μg，GPA：0．24—2．40μg，GP：0．31-4．65μg；相关系数r分别为：0．999，0．999，0．996。检出限依次为0．3、0．4、0．3ng；进行4次平行测定，平均回收率分别为98％、100％和95％，RSD分别为2．8％、3．1％和2．9％。该方法操作简便，重复性好，专属性强，准确可靠，适用于对复杂的天然产物样品的定性和定量分析。     

反相高效液相色谱／质谱法同时测定鸡肉中5种喹诺酮药物残留

采用反相高效液相色谱／四级杆串联质谱（RP-HPLC／MS／MS）同时测定鸡肉中的5种喹诺酮药物（quinolones，QNs）。均质后的鸡肉样品采用磷酸盐缓冲溶液和乙腈的混和溶液提取。提取液经正己烷液-液分配（LLP）去除脂肪后，用C18固相萃取（SPE）柱净化，氨化甲醇洗脱，洗脱液用氮气吹干，流动相定容后，分析物采用LC／MS／MS电喷雾电离（ESI），正离子，多反应监测（MRM）模式检测，外标法定量。在添加浓度2．5～10μg/kg范围内，5种QNs的回收率在79．8％～95．1％之间；相对标准偏差（RSD）均小于11．7％。环丙沙星、丹诺沙星、恩诺沙星检出限（LOD）为0．5μg／kg，沙托沙星为1．0μg／kg，氟甲喹为0．1μg／kg。     

林蛙油中农药残留的GC-MS/MS检测方法

首次建立了林蛙油中15种农药（p，p′DDE，O，p′-DDD，o p′-DDT，p，p′-DDT，BHC（α、β、γ、δ），异丙威，甲拌磷，六氯苯，百菌清，皮蝇磷，倍硫磷，甲氰菊酯）的GC—MS／MS残留检测方法。样品用乙酸乙酯提取、Florisil层析柱净化后，经GC—MS／MS检测，用外标法定量。15种农药在0．050～10．0mg／L范围内，线性关系良好，相关系数r≥0．996。当添加量在0．050—2．00mg／kg间，平均加标回收率为81％～117％，RSD为2．4％-18．2％，方法的检出限为0．050mg／kg。该方法准确、灵敏，适用于农药残留的分析。     

微波辅助萃取-液相色谱-串联质谱法测定植物源产品中的阿维菌素B1a残留量

建立了植物源产品茶叶、粮谷、中药材中阿维菌素B1a残留量的液相色谱-串联质谱（LC-MS／MS）测定方法。样品用丙酮-二氯甲烷（体积比1：1）微波辅助提取,提取液经石墨化炭黑／氨基（Carb／NH2）固相萃取小柱净化。采用Hypersil Gold C18色谱柱（150mm×2．1mm,5μm）,乙腈-2．5mmol／L乙酸铵水溶液为流动相,以电喷雾电离正离子（ESI＋）、多反应监测模式（MRM）定性、定量测定阿维菌素B1a,采用基质标准曲线外标法定量。在5—100μg／L范围内,阿维菌素B1a的峰面积与质量浓度呈线性关系,相关系数大于0．998,方法的检出限（S／N〉3）为5μg／k,定量限（S／N〉10）为10μg／kg。取有代表性的绿茶、小麦、丹参阴性样品进行加标回收试验,在10,50μg／kg加标水平下,回收率为75％-87％,相对标准偏差为4．04％-6．38％（n=5）。该法提取效果好、净化较彻底,灵敏度满足国内外限量标准的要求,适合复杂基质植物源产品中阿维菌素B1a残留量的测定。     

谷物中脱氧雪腐镰刀菌烯醇的高效液相色谱检测及质谱确证

建立了谷物中脱氧雪腐镰刀菌烯醇DON的高效液相色谱检测和质谱确证方法。样品用水提取,通过免疫亲和柱进行富集和净化,以Hypersil BDS C18柱为分离柱,乙腈-水（10：90,V/V）混合溶剂为流动相进行高效液相色谱分离和检测,利用大气压化学电离质谱（APCI）进行阻性结果的鉴定和确认。在小麦、大麦和面粉等样品中,本方法在0．1～10μg／g添加范围内的回收率为82．4％-103％,相对标准偏差1．4％-7．6％,检出限0．1μg／g。     

LC-ESI MS/MS测定蜜胺餐具中三聚氰胺的迁移量

建立了液相色谱串联电喷雾正离子源质谱(LC-ESI MS/MS)检测蜜胺餐具中三聚氰胺迁移量的方法.采用强阳离子交换柱,流动相为乙腈-10 mmol/L乙酸铵/乙酸缓冲溶液(pH 4.0)(40:60,体积比),以多反应离子监测对三聚氰胺做定性定量分析.在水、3%乙酸、10%乙醇模拟物中,三聚氰胺在3.00～130.0...     

A Microcomputer Controlled Tandem Quadrupole Mass Spectrometer Using a Direct Liquid Introduction Probe for Screening Analysis

Abstract

The use of a direct liquid introduction probe with a short guard column as the method of sample introduction is explored. This technique is an alternative to the conventional direct probe method. The method is rapid, involatile compounds can be analyzed, and volatile compounds are not lost in the vacuum lock. Screening for trichlorophenol in urine, by observing the loss of [M-HCOCI]⁺, is used to test the technique. The advantages and disadvantages of split and splitless direct liquid introduction probes and column concentration are discussed. Detection limits in the low nanograms were observed, and samples may be analyzed every 30 seconds.     

Characterization of major degradation products of an adenosine A2A receptor antagonist under stressed conditions by LC‐MS and FT tandem MS analysis

Parkinson's disease (PD) is a very serious neurological disorder, and current methods of treatment fail to achieve long‐term control. SCH 420814 is a potent, selective and orally active adenosine A_2A receptor antagonist discovered by Schering‐Plough. Stability testing provides evidence of the quality of a bulk drug when exposed to the influence of environmental factors. Understanding the drug degradation profiles is critical to the safety and potency assessment of the drug candidate for clinical trials. As a result, identification of degradation products has taken an important role in drug development process. In this study, a rapid and sensitive method was developed for the structural determination of the degradation products of SCH 420814 formed under different forced conditions. The study utilizes a combination of liquid chromatography–tandem‐mass spectrometry (LC‐MS/MS) and Fourier Transform (FT) MS techniques to obtain complementary information for structure elucidation of the unknowns. This combination approach has significant impact on degradation product identification. A total of ten degradation products of SCH 420814 were characterized using the developed method. Copyright © 2009 John Wiley & Sons, Ltd.     

Basic drug analysis by strong cation-exchange liquid chromatography-tandem mass spectrometry: simultaneous analysis of amisulpride, and of metamfetamine and amfetamine in serum/plasma

In the HPLC of basic drugs and metabolites, good efficiency and peak shape can often be attained using strong cation‐exchange packings with isocratic 100% methanol eluents containing an ionic modifier at an appropriate pH* and ionic strength. Solvent extracts can be analysed directly, and use of ammonium acetate as modifier facilitates the use of atmospheric pressure chemical ionization (APCI)–tandem mass spectrometry, selected reaction monitoring mode. For the analysis of amisulpride and of metamfetamine/amfetamine in plasma (200 µL) after single oral doses in man, a column packed with Waters Spherisorb S5SCX (5 µm average particle size, 100 × 2.1 mm i.d.) was used with methanolic ammonium acetate (40 mmol/L, pH* 6.0, flow rate 0.5 mL/min) as eluent (35°C). Deuterated internal standards were used for each analyte. Detection was by positive‐mode APCI. Responses for all analytes were linear over the calibration ranges. Intra‐assay precision (RSD) was 2–18%, and inter‐assay precision was 2–12%. The limit of detection was 0.5 µg/L for all analytes. No significant matrix effects or isobaric interferences were noted. The total analysis time was 7 min. Similar methodology can be applied to a wide range of basic analytes using MS/MS detection. Copyright © 2010 John Wiley & Sons, Ltd.     

乳腺癌代谢物组模式特征发现方法及HPLC/M S/M S分析

提出一种基于单独最优特征组合和BP神经网络的代谢物组模式特征发现方法,并用其寻找到尿样中与乳腺癌最为相关的4种核苷,组成一组特异性检测参数.经HPLC/MS/MS联用法鉴定,它们是乳清酸核苷、1-甲酰化腺苷、S-腺苷-L-蛋氨酸及N²-甲酰化鸟苷.将这4种核苷作为输入变量,用BP神经分类网络建立乳腺癌诊断模型.留一法交叉验证和独立验证结果表明,该模型预测准确率达到90%以上.     

LC/MS/MS for identification of in vivo and in vitro metabolites of jatrorrhizine

The in vivo and in vitro metabolism of jatrorrhizine has been investigated using a specific and sensitive LC/MS/MS method. In vivo samples including rat feces, urine and plasma collected separately after dosing healthy rats with jatrorrhizine (34 mg/kg) orally, along with in vitro samples prepared by incubating jatrorrhizine with rat intestinal flora and liver microsome, respectively, were purified using a C(18) solid-phase extraction cartridge. The purified samples were then separated with a reversed-phase C(18) column with methanol-formic acid aqueous solution (70:30, v/v, pH3.5) as mobile phase and detected by on-line MS/MS. The structural elucidation of the metabolites was performed by comparing their molecular weights and product ions with those of the parent drug. As a result, seven new metabolites were found in rat urine, 13 metabolites were detected in rat feces, 11 metabolites were detected in rat plasma, 17 metabolites were identified in intestinal flora incubation solution and nine metabolites were detected in liver microsome incubation solution. The main biotransformation reactions of jatrorrhizine were the hydroxylation reaction, the methylation reaction, the demethylation reaction and the dehydrogenation reaction of parent drug and its relative metabolites. All the results were reported for the first time, except for some of the metabolites in rat urine.     

Tandem mass spectrometry of synthetic polymers

The detailed characterization of macromolecules plays an important role for synthetic chemists to define and specify the structure and properties of the successfully synthesized polymers. The search for new characterization techniques for polymers is essential for the continuation of the development of improved synthesis methods. The application of tandem mass spectrometry for the detailed characterization of synthetic polymers using the soft ionization techniques matrix‐assisted laser desorption/ionization mass spectrometry (MALDI‐MS) and electrospray ionization mass spectrometry (ESI‐MS), which became the basic tools in proteomics, has greatly been increased in recent years and is summarized in this perspective. Examples of a variety of homopolymers, such as poly(methyl methacrylate), poly(ethylene glycol), as well as copolymers, e.g. copolyesters, are given. The advanced mass spectrometric techniques described in this review will presumably become one of the basic tools in polymer chemistry in the near future. Copyright © 2009 John Wiley & Sons, Ltd.     

动物源性食品中吡喹酮残留量的LC-MS/MS测定

应用固相萃取液相色谱-串联质谱法(LC-MS/MS)技术建立了动物源性食品中吡喹酮药物残留的检测方法。用乙酸乙酯提取样品中的吡喹酮残留,提取液经碱性氧化铝小柱净化,LC-MS/MS测定,在10~40μg/kg范围内添加回收率为91%~111%,定量下限(LOQ)为10μg/kg。本文还讨论了吡喹酮残留物的提取条件、流动相对吡喹酮ESI离子化的影响,并借助准MS/MS/MS技术探讨了吡喹酮主要质谱碎片的产生机理。     

Streamlined pentafluorophenylpropyl column liquid chromatography-tandem quadrupole mass spectrometry and global (13)C-labeled internal standards improve performance for quantitative metabolomics in bacteria

Streamlined quantitative metabolomics in central metabolism of bacteria would be greatly facilitated by a high-efficiency liquid chromatography (LC) method in conjunction with accurate quantitation. To achieve this goal, a methodology for LC-tandem quadrupole mass spectrometry (LC-MS/MS) involving a pentafluorophenylpropyl (PFPP) column and culture-derived global (13)C-labeled internal standards (I.Ss.) has been developed and compared to hydrophilic interaction liquid chromatography (HILIC)-MS/MS and published combined two-dimensional gas chromatography and LC methods. All 50 tested metabolite standards from 5 classes (amino acids, carboxylic acids, nucleotides, acyl-CoAs and sugar phosphates) displayed good chromatographic separation and sensitivity on the PFPP column. In addition, many important critical pairs such as isomers/isobars (e.g. isoleucine/leucine, methylsuccinic acid/ethylmalonic acid and malonyl-CoA/3-hydroxybutyryl-CoA) and metabolites of similar structure (e.g. malate/fumarate) were resolved better on the PFPP than on the HILIC column. Compared to only one (13)C-labeled I.S., the addition of global (13)C-labeled I.Ss. improved quantitative linearity and accuracy. PFPP-MS/MS with global (13)C-labeled I.Ss. allowed the absolute quantitation of 42 metabolite pool sizes in Methylobacterium extorquens AM1. A comparison of metabolite level changes published previously for ethylamine (C2) versus succinate (C4) cultures of M. extorquens AM1 indicated a good consistency with the data obtained by PFPP-MS/MS, suggesting this single approach has the capability of providing comprehensive metabolite profiling similar to the combination of methods. The more accurate quantification obtained by this method forms a fundamental basis for flux measurements and can be used for metabolism modeling in bacteria in future studies.