固相萃取净化及超高效液相色谱-串联质谱法测定橡胶制品中的13种N-亚硝胺

建立了固相萃取(SPE)净化、超高效液相色谱-串联质谱(UHPLC-MS/MS)测定橡胶制品中13种N-亚硝胺的方法。样品于密闭萃取瓶中于60 ℃下用甲醇超声萃取30 min,C₁₈固相萃取小柱对萃取液进行净化,经C₁₈色谱柱分离,最后用电喷雾正离子(ESI⁺)和多重反应监测模式(MRM)对13种N-亚硝胺进行定性、定量测定。实验中对样品前处理、色谱分离条件和质谱检测条件进行了优化。在优化的实验条件下,橡胶样品中添加N-亚硝基二甲胺(NDMA)与N-亚硝基-二乙基胺(NDEA)为500 μg/kg、其他组分均为50 μg/kg时,各组分的相对标准偏差(RSD,n=7)小于10%;在实际样品中的加标回收率为70.7%~117.0%;方法的检出限(LOD,以10倍标准偏差计)为0.5~500 μg/kg。方法可应用于橡胶制品中13种N-亚硝胺的测定。     

气相色谱-串联质谱法测定肉制品中10种挥发性N-亚硝胺类化合物

建立了气相色谱-串联质谱（GC-MS/MS）检测肉制品中10种挥发性N-亚硝胺类化合物残留量的方法。肉制品样品经同时蒸馏萃取法（SDE）萃取，采用冷冻去脂净化法，在多反应监测模式下分析，外标法定量。结果表明，采用优化后的条件，10种挥发性N-亚硝胺类化合物在1.00~1000 μg/L范围内线性关系良好，相关系数均在0.99以上。方法的检出限（LOD，S/N=3）和定量限（LOQ，S/N=10）分别为0.01~0.02 μg/kg和0.04~0.07 μg/kg。选取3种不同类型的肉制品（火腿肠、中式香肠和腌渍腊肉），在空白样品添加水平为LOQ水平、1.0、2.0 μg/kg时，10种挥发性N-亚硝胺类化合物的平均回收率为74.8%~94.3%，相对标准偏差小于8.3%。市售3类肉制品中6种挥发性N-亚硝胺类化合物（N-亚硝基二甲胺、N-亚硝基二乙胺、N-亚硝基吡咯烷、N-亚硝基哌啶、N-亚硝基二丁胺、N-亚硝基二丙胺）均有不同程度检出，且腌渍腊肉中每种挥发性N-亚硝胺类化合物的检出值最高。该方法操作简单，萃取充分，灵敏度高，试剂用量少，可满足实验室大量样品的日常检测需求。     

固相萃取-大体积程序升温进样气相色谱-三重四极杆串联质谱测定饮用水中3种挥发性N-亚硝胺

建立了固相萃取大体积程序升温进样气相色谱-三重四极杆质谱联用（GC-QqQ-MS/MS）同时测定饮用水中N-亚硝基二甲胺、N-亚硝基甲基乙基胺及N-亚硝基二乙基胺的分析方法。用椰壳活性炭固相萃取小柱萃取水样中待测物组分，少量二氯甲烷洗脱、无水硫酸钠脱水，大体积程序升温进样，气相色谱-三重四极杆质谱联用仪进行多反应监测（MRM）模式检测，外标法定量。3种N-亚硝胺在1~50 ng/L范围内线性关系良好，相关系数（r²）均大于0.999，在饮用水中进行10、20和50 ng/L水平的添加，3种待测物平均加标回收率为94.8%~109%，相对标准偏差（RSD）为4.44%~8.10%（n=5），定量限（LOQ）为0.08~0.7 ng/L。该法灵敏、准确、简单、可靠，适用于饮用水中3种N-亚硝胺组分的痕量检测。     

Optimization of parameters for the supercritical fluid extraction in the determination of N-nitrosamines in rubbers

The study of the possibilities of supercritical fluid extraction (SFE) with N-nitrosamines in rubbers has been carried out. Home-made materials fortified with several N-nitrosamines were prepared in order to optimize the SFE parameters. A Plackett-Burman design was employed to evaluate the influence of those parameters to be controlled in SFE, such as pressure, temperature, static and dynamic time, restrictor temperature and volume of modifier while CO2 was used as the extraction fluid. An extra central composite design for the main factors (according to the previously obtained results) was also developed in order to refine the best supercritical conditions for the extraction of N-nitrosamines from rubbers. Gas chromatography with a nitrogen and phosphorus sensitive detector was used to achieve sensitivity and limits of detection for the concentrations expected in plastic materials. The proposed analytical method has shown to be useful in the determination of N-nitrosamines even for complex matrices.     

分散固相萃取-气相色谱-串联质谱法测定动物源性食品中9种N-亚硝胺类化合物

建立了分散固相萃取-同位素稀释-气相色谱-串联质谱同时测定动物源性食品中9种N-亚硝胺的方法。样品用乙腈提取,上清液经分散固相萃取（dSPE）净化后浓缩。选用DB-WAX极性毛细管色谱柱对待测物进行分离,经EI源电离后以多反应监测（MRM）模式采集数据并做定性筛查和定量分析。9种N-亚硝胺在相应的浓度范围内线性关系良好,相关系数均大于0.99,对4类典型的动物源性食品进行3个不同浓度的加标试验,平均回收率为62.5%~118%,RSD为2.11%~25.6%,检出限（LOD,S/N=3）为0.02~0.31 μg/kg。该方法成本低廉、灵敏可靠,适用于同时对动物源性食品中9种N-亚硝胺进行定性和定量测定。     

QuEChERS-同位素稀释-气相色谱-串联质谱法测定动物源性食品中9种N-亚硝胺类化合物

建立了同时测定动物源性食品中9种N-亚硝胺类化合物的气相色谱-串联质谱分析方法。当下动物源性食品中N-亚硝胺类化合物污染种类较多,对人体危害较大,但国标GB 5009.26-2016仅针对N-二甲基亚硝胺的检测,且存在样品前处理复杂、标准方法回收率低、再现性差等问题,因此建立同时快速检测多种N-亚硝胺类化合物的方法有一定现实意义。称取10.0 g样品,置于50 mL离心管中,加入200 μL内标工作液和10 mL乙腈,冷冻30 min后,加入4 g硫酸镁和1 g氯化钠进行脱水,以9000 r/min离心5 min。取5 mL上清液使用150 mg聚苯乙烯二乙烯苯(PLS-A)粉末净化,再使用1.6 g MgSO₄和0.4 g NaCl脱水,过0.22 μm滤膜,上机分析。在初始温度为50 ℃时采用程序升温模式,0.16 min后,以900 ℃/min的速率将温度升至220 ℃。采用毛细管气相色谱柱HP-Innowax(30 m×0.25 mm×0.25 μm)分离,使用电子轰击电离(EI)源检测,在多反应监测模式下,以保留时间和特征离子对信息进行定性和定量分析,使用内标法定量N-亚硝胺类化合物。结果表明,N-亚硝胺类化合物在0.1~50.0 μg/L范围内具有良好的线性关系,方法的检出限(S/N=3)和定量限(S/N=10)分别为0.03~0.30 μg/kg和0.10~1.00 μg/kg。对不同样品基质进行0.5、1.0、3.0 μg/kg3个水平的加标回收试验,9种N-亚硝胺类化合物的回收率为80.4%~98.5%, RSD(n=6)为2.41%~12.50%。应用建立的方法检测市面上常见的动物源性食品,除N-亚硝基乙胺、N-亚硝基吗啡胆碱外,其他7种N-亚硝胺类化合物均有不同程度检出。检测结果表明,腌制水产品中N-亚硝胺类化合物含量普遍高于其他样品。研究建立的方法操作简单,不需要长时间蒸馏提取,可快速对动物源性食品中N-亚硝胺类化合物进行定性和定量分析,且样品和试剂的消耗量更少,节省成本,对环境污染小。该法的建立对我国动物源性食品中N-亚硝胺类化合物残留水平的控制、检测标准的制定和采取相应的管理措施具有一定的理论和现实意义。     

Determination of the coumarin derivative cloricromene acid in rabbit plasma and platelets.

Two methods for the determination of cloricromene acid in biological samples are described. Cloricromene acid is a catabolite of cloricromene, a coumarin derivative which is active in the cardiovascular system. After oral administration of cloricromene to a rabbit, plasma and platelets were taken at different times and cloricromene acid was then isolated by solid-phase extraction with Sep-Pak C18 cartridges using acetonitrile-tetrahydrofuran-20% aqueous acetic acid (15:11:74, v/v/v) as eluent. The analyses were performed by reversed-phase high-performance liquid chromatography (RP-HPLC) combined with fluorescence detection with excitation at 310 nm and emission at 390 nm. The limit of quantification by RP-HPLC was about 50 pg. The catabolite in the plasma was identified by continuous-flow fast atom bombardment mass spectrometry (CF-FAB-MS), also used as a complementary means of RP-HPLC determination. The results obtained by RP-HPLC and CF-FAB-MS showed good agreement.     

Determination of Alpha-Tocopherol Levels in Rat Microsomes by High-Performance Liquid Chromatography

Abstract

A rapid, simple and sensitive method is described for the routine determination of alphatocopherol in microsomes. After a single extraction step with n-heptane extracts are injected onto a normal phase column using n-heptane/isopropanol (99.3/0.7, v/v) for elution; a fluorescence detector set at 215 nm excitation wavelenght and a cut-off filter emitting at 320 nm are used for detection. Total run time is less than 4 minutes.     

Stability indicating methods for the determination of some anti-fungal agents using densitometric and RP-HPLC methods

Two chromatographic methods were developed for the determination of some anti-fungal drugs in the presence of either their degradation products or cortisone derivatives. The densitometric method determined mixtures of each of ketoconazole (KT), clotrimazole (CL), miconazole nitrate (MN) and econazole nitrate (EN) with the degradation products of each one. Mixtures of MN with hydrocortisone (HC) and of EN with triamcinolone acetonide (TA) were also successfully separated and determined by this technique. For KT and CL, a mixture of methanol:water:triethylamine (70:28:2 v/v) was used as a developing system and the spots were scanned at 243 nm and 220 nm for KT and CL, respectively. For MN and EN, a mixture of hexane:isopropyl alcohol:triethylamine (80:17:3 v/v) was used as a developing system and the spots were scanned at 225 nm for both drugs. The HPLC method determined mixtures of CL or EN with their degradation products which were separated and quantified on a Zorbax C8 column. Elution was carried out using methanol:phosphate buffer pH 2.5 (65:35 v/v) as a mobile phase at a flow rate of 1.5 ml/min and UV detection at 220 nm for CL. For EN, a mixture of methanol:water containing 0.06 ml triethylamine pH 10 (75:25 v/v) was used as a mobile phase at a flow rate of 1.5 ml/min and UV detection at 225 nm. The methods were also used to separate mixtures of CL with betamethasone dipropionate (BD) and EN with TA in a laboratory prepared mixture and in pharmaceutical preparations. The methods were sensitive, precise and applicable for determination of the drugs in pharmaceutical dosage forms.     

High-performance liquid chromatography with fluorescence detection for the simultaneous determination of 3,4-methylenedioxymethamphetamine, methamphetamine and their metabolites in human hair using DIB-Cl as a label

This paper describes a highly sensitive HPLC method for the simultaneous determination of 3,4-methylenedioxymethamphetamine (MDMA), 3,4-methylenedioxyamphetamine (MDA), amphetamine (AP) and methamphetamine (MP) in human hair samples. The amphetamines investigated were derivatized with the fluorescent reagent, DIB-Cl to yield highly fluorescent DIB-derivatives, which were then analyzed by HPLC with fluorescence detection at excitation and emission wavelengths of 325 nm and 430 nm, respectively. The separation was achieved on an ODS column with an isocratic mobile phase composed of acetonitrile-methanol-water (30:40:30, v/v/v). The limits of detection for the four compounds obtained by the proposed method ranged from 11 to 200 pg/mg. The method was successfully applied to the determination of MDMA and MDA in hair samples obtained from MDMA abuser.     

High-performance liquid chromatographic determination of uranium using solvent extraction and bis(salicylaldehyde) tetramethylethylenediimine as complexing reagent

The reagent bis(salicylaldehyde)tetramethylethylenediimine has been used for the determination of dioxouranium(VI), based on complexation in aqueous solution at pH 6, followed by extraction in chloroform and HPLC determination on a Hypersil ODS (3 μm) column. The complex was eluted with the ternary mixture methanol-acetonitrile-water (40:30:30, v/v/v), with UV detection at 260 nm. Oxovanadium(IV), iron(III), copper(II), cobalt(II), nickel(II) and palladium(II) were completely separated and did not interfere in the determination of uranium. The linear calibration range and detection limits have been obtained. The method has been applied to the determination of uranium together with copper, iron and nickel in mineral ore samples.     

Stability-indicating methods for determination of tiapride in pure form, pharmaceutical preparation, and human plasma

Four different stability-indicating procedures are described for determination of tiapride in pure form, dosage form, and human plasma. Second derivative (D2), first derivative of ratio spectra (1DD), spectrofluorimetric, and high-performance column liquid chromatographic (LC) methods are proposed for determination of tiapride in presence of its acid-induced degradation products, namely 2-methoxy-5-(methylsulfonyl) benzoic acid and 2-diethylaminoethylamine. These approaches were successfully applied to quantify tiapride using the information included in the absorption, excitation, and emission spectra of the appropriate solutions. In the D2 method, Beer's law was obeyed in the concentration range of 1.5-9 microg/mL with a mean recovery of 99.94 +/- 1.38% at 253.4 nm using absolute ethanol as a solvent. In 1DD, which is based on the simultaneous use of the first derivative of ratio spectra and measurement at 245 nm in absolute ethanolic solution, Beer's law was obeyed over a concentration range of 1.5-9 microg/mL with mean recovery 99.64 +/- 1.08%. The spectrofluorimetric method is based on the determination of tiapride native fluorescence at 339 nm emission wavelength and 230 nm excitation wavelength using water-methanol (8 + 2, v/v). The calibration curve was linear over the range of 0.2-3 microg/mL with mean recovery of 99.66 +/- 1.46%. This method was also applied for determination of tiapride in human plasma. A reversed-phase LC method performed at ambient temperature was validated for determination of tiapride using methanol-deionized water-triethylamine (107 + 93 + 0.16, v/v/v) as the mobile phase. Sulpiride was used as an internal standard at a flow rate of 1 mL/min with ultraviolet detection at 214 nm. A linear relation was obtained over a concentration range of 2-30 microg/mL with mean recovery of 99.66 +/- 0.9%. Results were statistically analyzed and compared with those obtained by applying the reference method. They proved both accuracy and precision.     

Determination of the analgesic components of Spasmomigraine tablet by liquid chromatography with ultraviolet detection

A procedure was developed for the determination of the analgesic components of Spasmomigraine tablets, which are ergotamine (I), propyphenazone (II), caffeine (III), camylofin (IV), and mecloxamine (V). They were subjected to high-performance liquid chromatography on a column (300 x 3.9 mm, 10 rlm particle size) packed with micro-Bondapak C18. Separations were achieved with the mobile phase methanol-water-triethylamine (60 + 40 + 0.1, v/v/v) flowing at a rate of 1.5 mL/min, and quantitative determination was performed at 254 nm at ambient temperature for I-III; acetonitrile-25 mM KH2PO4-acetic acid (45 + 55 + 0.2, v/v/v), flowing at a rate of 1.5 mL/min and detection at 234 nm at ambient temperature, was used for IV and V. Methyl paraben was used as an internal standard. The detection limits were 0.35 (I), 5.0 (11), 1.5 (111), 3.0 (IV), and 2.0 microg/mL (V). The method was accurate (mean recovery 98+/-2%, n = 4) and precise (coefficient of variation <5%, n = 5). The proposed method is rapid and sensitive and, therefore, suitable for the routine control of these ingredients in multicomponent dosage forms.     

Quantitative determination of porphyrins, their precursors and zinc protoporphyrin in whole blood and dried blood by high-performance liquid chromatography with fluorimetric detection

Methods for the determination of porphyrins, delta-aminolevulinic acid (ALA), porphobilinogen (PBG) and zinc protoporphyrin of heme biosynthesis in whole blood and dried blood are described. Erythrocyte porphyrins and the precursors ALA and PBG were extracted from whole blood (50 microliter) with 0.3 ml of methanol and 1.5 M hydrochloric acid (2:1, v/v). Zinc protoporphyrin was extracted with an acetone-pyridine-Sterox solution. Other major interfering metabolites were removed by centrifugation. An aliquot of the supernatant was injected onto the reversed-phase C18 column for detection of porphyrins with excitation wavelength at 405 nm and emission wavelength at 630 nm. The mobile phase was 0.1 M phosphate-methanol-tetrahydrofuran (18:30:16, v/v/v), pH 5.38. The ALA and PBG were derivatized with o-phthalaldehyde before injection. The detection excitation wavelength occurred at 330 nm and the emission wavelength at 418 nm. The mobile phase was 0.1 M phosphate-methanol (7.5:5), pH 3.38. For the dried blood specimen of filter paper, two 0.64-cm discs punched out from the blood-impregnated filter paper were placed in a test tube containing 200 microliter of 0.9% saline for 60 min or longer at room temperature and then treated as whole blood.     

微波辐射辅助快速检测微量亚硝胺的研究

分析了分光光度法对于溶液中亚硝胺回收率过低的原因,发现去亚硝基化反应 产物NOBr在吹离溶液过程中分解成为光度法无法检测的NO_x（x < 2）鉴于此,在 装置中增加一个CrO_3氧化管,将生成的NO_x（x < 2）转化成可被显色检测的 NO_2,使亚硝胺回收率高于90%,接近公认标准方法－热能分析仪（TEA）法的类似 指标（76% ～ 96%）;而检测限可达2 * 10~(-8) mol/L。发现微波辐射能使亚硝 胺在低于其沸点的温度下挥发和/或分解,并将其用于倩光度法检测,可以在3 min之内将样品中的亚硝胺收集以供测定,形成快速同时检测环境样品（如烟草） 中微量亚硝胺和氮氧化物的新方法。     

Determination of N-nitrosamines in latex by sequential supercritical fluid extraction and derivatization

A new method to determine N-nitrosamines in latex products has been developed by combination of supercritical fluids and chemical derivatization. A new design for a liquid trap has been introduced. A factorial fractional design was used in order to evaluate the influence of the different factors affecting the process. Factors such as pressure, temperature, static and dynamic time, restrictor temperature and volume of an hydrobromic acid-acetic anhydride mixture (1:10, v/v) were included in the design. CO2 was used as the extraction fluid. Gas chromatography with nitrogen and phosphorus sensitive detection was employed to achieve good sensitivity attending to the molecular structure of these compounds (N-nitrosamines and their corresponding secondary amines). The obtained results have shown to be useful to increase selectivity and reduce sample handling.     

Determination of n-acetylmuramoyl-l-alanyl-d-isoglutamine in liposomes by HPLC

A method using reversed-phase high-pressure liquid chromatography (with spectrometric detection at 218nm) is described for the determination in new pharmaceutical preparations (liposomes) of a new immunostimulating agent (N-acetylmuramoyl-l-alanyl-d-isoglutamine). Separation was achieved with a mu-bondapak column and phosphate buffer (pH 2.5)-methanol mixture (93:7 v/v) as eluent, at a flow-rate of 2 ml min . Sodium acetate was used as an internal standard. The detector response at 218 nm was linear in the range 10-170 mug ml . The method is simple and accurate.     

Determination of seven compounds in Tang Maikang granule by high-performance liquid chromatography

An accurate and sensitive high-performance liquid chromatography method is developed and applied to the determination of seven compounds in a kind of traditional Chinese medicinal preparation of Tang Maikang Granule. The method is performed on Hypersil C(18) column (250- x 4.6-mm i.d., 5 microm), and different mobile phases and detectors are selected according to the various compounds. For astragaloside IV, an evaporative light scattering detector (ELSD) is used with a gradient of methanol-water at an eluent gas rate of 2.0 mL/min, under a drift tube temperature of 80 degrees C. Formononetin and calycosin are also eluted by a gradient of methanol-water, but a photodiode array (PDA) detector is used at a wavelength of 254 nm for formononetin and calycosin. A PDA detector at a wavelength of 230 nm is used for paeoniflorin, with methanol-water (30:70, v/v) as the mobile phase. For danshensu and protocate chualdehyde, an eluent of methanol-0.5% acetic acid (12:88, v/v) is used, with PDA detection at 280 nm. For berberine, methanol and water containing 0.1% sodium dodecanesulphonate (SDS) and 0.1% phosphorous acid (70:30, v/v) is employed as the mobile phase, also using a PDA detector, but the detection wavelength is 265 nm. The intra- and interrun precision (relative standard deviation) of this method is less than 5% for seven analytes.     

免疫亲和柱净化/柱前衍生化-高效液相色谱荧光检测法测定粮谷中的T-2毒素

建立了免疫亲和柱净化/柱前衍生化-高效液相色谱荧光检测器测定粮谷中T-2毒素含量的方法。样品经甲醇-水(体积比为80∶20)混合溶剂提取,通过免疫亲和柱(IAC)净化,以氰酸蒽(1-AN)为衍生化试剂、4-二甲基氨基吡啶(DMAP)为催化剂进行衍生,以ZORBAX Eclipse XDB-C18 柱为分离柱,乙腈-水(体积比为80∶20)为流动相进行高效液相色谱分离及荧光检测，荧光检测的激发波长为381 nm，发射波长为470 nm。T-2毒素的质量浓度为0.01~1.5 mg/L时与峰高呈良好的线性,相关系数为0.9985。在0.01~1.5 μg/g添加水平下，回收率为79.7%~94.5%,相对标准偏差小于7%；检出限（S/N＝3）为0.01 μg/g。该方法净化效果好,灵敏度高,操作简便快速。     

Determination of T-2 toxin in cereal grains by liquid chromatography with fluorescence detection after immunoaffinity column clean-up and derivatization with 1-anthroylnitrile

1-Anthroylnitrile (1-AN) has been shown to be an efficient labelling reagent for the determination of T-2 toxin (T-2) by high-performance liquid chromatography (HPLC)-fluorescence detection. This reaction has been used to develop a sensitive, reproducible and accurate method for the determination of T-2 in wheat, corn, barley, oats, rice and sorghum. The method uses immunoaffinity columns containing antibodies specific for T-2 for extract clean-up, pre-column derivatization with 1-AN and HPLC with fluorescence detection for toxin determination. Ground cereal samples were extracted with methanol-water (80:20, v/v), the extracts were purified by immunoaffinity columns and the toxin was quantified by reversed-phase HPLC with fluorometric detection (excitation wavelength 381 nm, emission wavelength 470 nm) after derivatization with 1-AN. Recoveries from the different cereals spiked with T-2 at levels ranging from 0.05 to 1.5 microg/g were from 80 to 99%, with relative standard deviations of less than 6%. The limit of detection was 0.005 microg/g, based on a signal-to-noise ratio of 3:1.