HPLC法检测玉米中痕量单端孢霉烯属族毒素

以对酞内酰胺苯甲酰氨（４－（２－ｐｈｔｈａｌｉｍｉｄｙ１）ｂｅｎｚｏｙ１ ｃｈｌｏｒｉｄｅ，简称ＰＩＢ－ＣＩ）为衍生试剂，建立了一种快速、灵敏分析单端孢霉烯属族毒素中脱氧雪腐镰刀菌烯醇的新方法，对衍生反应条件，衍生物分离及定量检测条件都进行了研究，衍生物用ＯＤＳ柱分离，紫外检测器检测（λ＝３００ｎｍ）乙腈＋水（５８＋４２Ｖ＋Ｖ）作流动相，检出限为６ｐｍｏｌ。用于分析玉米中的痕量ＤＯＮ，简化了样品处     

高效液相色谱法（荧光检测）分析人血浆中哌啶酸

本工作用丹磺酰氯柱前衍生比反相色谱（荧光检测）法分析了正常人和肝病患者血浆中哌啶酸－２的水平。样品用荧光胺提取法,除去血浆中的其他氨基酸和生物胺对检测的干扰。以哌啶酸－３为内标物,测得平均回收率为８４％。至少在４０ｐｍｏｌ至２ｎｍｏｌ范围内,浓度与响应的线性关系良好。两个哌啶酸的检测极限分别为２．０和２．５ｐｍｏｌ。对操作中应予注意的几个步骤作了讨论。     

N—羟基琥珀酰亚胺—间于甲氨基苯甲酸酯柱前衍生HPLC分离荧光检测？…

用Ｎ－羟基琥珀酰亚胺－间二甲氨基苯甲酸酯为柱前衍生试剂,Ｃ１８柱,含ｐＨ为４．０为１０ｍｍｏｌ／Ｌ柠檬酸－磷本氢二钠缓冲溶液的４０％的甲醇－水（Ｖ／Ｖ）溶液为流动相,反相高效液相色谱（ＲＰ－ＨＰＬＣ）分离荧光检测了氨、甲胺和乙胺,检出限分别为５．０、０．５和１．０ｐｍｏｌ,方法简便、快速。     

反相HPLC测定钒,铌,钽的2—（2—吡啶偶氮）—5—二乙氨基苯酚配合物

以２－（２－吡啶偶氮０－５－二乙氨基苯酚（ＰＡＤＡＰ）为柱前衍生试剂，在含０．１％酒石酸的１０ｍｍｏｌ／Ｌ（ｐＨ３．５）ＨＡｃ－ＮａＡｃ缓冲溶液的甲醇／水（５０∶５０，Ｖ／Ｖ）中（５８０ｎｍ检测），在Ｃ１８柱上于１１ｍｉｎ内实现了Ｖ、Ｎｂ、Ｔａ的同时分离及测定，检出限（Ｓ／Ｎ＝３）杰０．３４、０．２９、７．３０ｎｇ／ｍＬ．该法灵敏度高，用于矿样分析所得民推荐值相行，标准加入回收率为９９．０％～１０     

对酞内酰胺苯磺酰氯柱前衍生HPLC法测定仲丁胺残留量

本实验采用对酞内酰胺苯磺酰氯（Ｐｈｔｈａｌｉｍｉｄｙｌ－ｂｅｎｅｚｅｎｅｓｕｌｐｈｏｙｌｃｈｌｏｒｉｄｅ，简称Ｐｈｉｓｙｌ－Ｃｌ）衍生反相ＨＰＬＣ法进行仲丁胺残留分析，以紫外检测器测定，最低检出限６．２ｐｍｏｌ。     

铂－锇共显色衍生配合物的高效液相色谱研究

研究了Ｏｓ（Ⅱ）和４，４’二（二乙氨基）苯硫酮与Ｐｔ（Ⅱ）共显色所衍生的配合物，于ＮｕｃｌｅｏｓｉｌＣ＿８柱上，用含３×１０￣（－３）ｍｏｌ／ＬＤＬ－樟脑－１０－磺酸和０．０２ｍｏｌ／ＬＨＡｃ－ＮａＡｃ（ｐＨ３．５）的乙腈－丙酮－水（７２：５：２３，Ｖ／Ｖ）作流动相（１．０ｍＬ／ｍｉｎ）分离并检测。线性范围为０．２～４．０μｇ／ｍＬＰｔ；检测限为１．０ｎｇＰｔ。此方法已应用于抗癌药物顺铂和卡铂的分析。     

4—（6—甲基—2—苯并噻唑偶氮）间苯三酚反相高效液相色谱分离测定钒钴镍铬

作以新研制的４－（６－甲基－２－苯并噻唑偶氮）间苯三酚为柱前衍生试剂，用含１０ｍｍｏｌ／Ｌ的ｐＨ６．８０的ＨＡｃ－ＮａＡｃ缓冲溶液，１０ｍｍｏｌ／Ｌ ＴＢＡ．Ｂｒ和１×１０＾－４ｍｏｌ／ＬＥＤＴＡ的甲醇－水溶液（７８：２２，Ｖ／Ｖ）作流动相，在Ｃ１８柱上，１１ｍｉｎ内反相ＨＰＬＣ分离测定了Ｃｒ（Ⅵ），Ｖ（Ⅴ），Ｃｏ（Ⅱ），Ｎｉ（Ⅱ）。当Ｓ／Ｎ＝３时，其检出限分别是Ｖ（Ⅴ）５．４５ｎｇ，Ｃｏ（Ⅱ）     

牙本质中天冬氨酸消旋化程度的测定——手性毛细管气相色谱法与高效液相色谱法的比较

应用手性毛细管气相色谱法（酸性异丙醇、三氟乙酸酐为衍生试剂）、高效液相色谱法（邻苯二甲醛－Ｎ－乙酰－Ｌ－半胱氨酸为手性衍生试剂）同时测定人类第一磨牙牙本质中天冬氨酸的消旋化程度，结果表明，两者均可有效地用于天冬氨酸对映体的分离测定，但气相色谱检测限（０．２ｐｍｏｌ）低于高效液相色谱（１．０ｐｍｏｌ），而变异系数（７％）、总分析时间（１００ｍｉｎ）均高于高效液相色谱（分别对应为４％，３１ｍｉｎ）。     

反相高效液相色谱柱前衍生荧光法测定肠粘膜中的谷氨酰胺

以邻苯二甲醛及３－巯基丙酸为衍生试剂,５０ｍｍｏｌ／Ｌ磷酸缓冲液（ｐＨ７．０）－乙腈（９４∶６,Ｖ／Ｖ）为流动相,在ＬｉｃｈｒｏｓｏｒｂＲＰ１８（１５０ｍｍ×４．６ｍｍｉ．ｄ．,５μｍ）柱上,研究并建立了测定动物肠粘膜中谷氨酰胺（Ｇｌｎ）的柱前衍生荧光ＲＰ－ＨＰＬＣ法。样品与衍生剂按４∶１进行衍生反应,Ｅｘ＝２３０ｎｍ,Ｅｍ＝３８９ｎｍ;流速为２．０ｍＬ／ｍｉｎ。Ｇｌｎ的保留时间为３．１５８ｍｉｎ,检测限为２５μｍｏｌ／Ｌ（Ｓ／Ｎ＝３．５）,线性范围为５０～３２００μｍｏｌ／Ｌ,ｒ＝０．９９９６。     

多联吡啶螯合物反相高效液相色谱法分离测定铜(Ⅱ)、钴(Ⅱ)、汞(Ⅱ)

以三联吡啶衍生物６，６”－二甲基－４＇－苯基－２，２＇：６＇，２”－三联吡啶（ＴＰＹ）作柱前显色剂，于ＡｃｃＱ－Ｔａｇ柱上，用内含２．０×１０～（－６）ｍｏｌ／Ｌ ＴＰＹ和０．６ ｍｏｌ／Ｌ　ＮａＡｃ－ＨＡｃ缓冲溶液（ｐＨ＝３．５）的甲醇－水溶液（５５：４５，Ｖ／Ｖ）作流动相，流速为１．０ ｍＬ／ｍｉｎ，并以紫外－可见检测器于３１０ｎｍ处进行检测，开发了一种 ＲＰ－ＨＰＬＣ法同时分离测定铜（Ⅱ）、钴（Ⅱ）、汞（Ⅱ）的方法。该方法简便快速，灵敏度高，对于铜、钴、汞的检测限分别是０．００２０、０．００５５和０．００４０ｍｇ／Ｌ。用于实际样品测定，结果满意。     

Thin-layer chromatography of mycotoxins

TLC has become an extremely powerful, rapid and in most instances inexpensive separation technique in mycotoxicology. This review presents achievements of its applications in this field. General technical aspects of the TLC of mycotoxins that are discussed include extraction and clean-up procedures, adsorbents and solvent systems, detection methods, two-dimensional TLC, high-performance TLC (HPTLC), quantitation and preparative TLC (PLC). Special applications of TLC deal with multi-mycotoxin analyses and with structurally related or individual mycotoxins (aflatoxins, sterigmatocystins, versicolorins, ochratoxins, rubratoxins, patulin, penicillic acid, mycophenolic acid, butenolide, citreoviridin, trichothecenes, cytochalasans, tremorgenic toxins, epipolythiopiperazine-3,6-diones, hydroxyanthraquinones, zearalenone, citrinin, secalonic acids, cyclopiazonic acid, PR toxin, roquefortine, xanthomegnin, viomellein and naphtho-gamma-pyrones).     

真菌毒素的液相色谱分离和检测

本文研究了一项分离棒曲霉素,青霉酸,赭曲霉素A和B,桔青霉素,玉米赤霉烯酮及柄曲霉素七种真菌毒素的高效液相色谱分离和检测方法。为实现分离,选择了反相方式。流动相为乙腈-水(55:45v/V),并添加了2.5mm草酸,pH为5.5。流量1.0ml/min。文中讨论了流动相中乙腈%、添加草酸的浓度对七种真菌毒素k’值的影响,对柱效N的影响,并从原理上讨论了保留机理。本文也综合地讨论了检测条件。也讨论了有关定量分析的参数,建立了一种较好的分析七真菌毒素的痕量定量方法。     

Analysis of glutathione adducts of patulin by means of liquid chromatography (HPLC) with biochemical detection (BCD) and electrospray ionization tandem mass spectrometry (ESI-MS/MS)

Abstract  A novel method for the identification of glutathione/electrophile adducts that are inhibiting glutathione-S-transferase (GST) activity was developed and applied for the analysis of the mycotoxin patulin. The method is based on high-performance liquid chromatography (HPLC) coupled to a continuous-flow enzyme reactor serving as biochemical detector (BCD) in parallel to electrospray mass spectrometric detection (ESI-MS). This HPLC-BCD technique combines a separation step and the detection of the inhibition and is therefore ideally suited for the analysis of the activity of single patulin/glutathione adducts within a complex mixture of adducts. Two out of at least 15 detected patulin–glutathione adducts showed strong GST inhibition. In ESI-MS, the inhibitory active adducts were characterized by [M + H]⁺ ions with m/z 462.1138 and m/z 741.2011, respectively. They could be identified as a dihydropyranone adduct containing one molecule glutathione and a ketohexanoic acid bearing two glutathione molecules. Graphical Abstract  OnlineAbstractFigure Electronic supplementary material  The online version of this article (doi:) contains supplementary material, which is available to authorized users.     

On-column complexation and simultaneous separation of vanadium(IV) and vanadium(V) by capillary electrophoresis with direct UV detection

An on-column complexation method has been developed for the simultaneous determination of V(IV) and V(V). Vanadium species were chelated with aminopolycarboxylic acids to form anionic complexes which were separated by capillary zone electrophoresis (CZE) with direct UV detection. Ethylenediaminetetraacetic acid (EDTA), diethylenetriaminepentacetric acid (DTPA), nitrilotriacetic acid (NTA), and N-2-hydroxyethylethlendiaminetriacetric acid (HEDTA) were investigated as both ligand and running electrolyte. Of the ligands studied the complexes of EDTA with V(IV) and V(V) resulted in the highest selectivity and UV response.The conditions used for on-column complexation and separation, including pH, and electrolyte ligand concentration, were examined to achieve reasonable separation selectivity and detection sensitivity. The optimum separation of the anionic forms of V(IV) and V(V) was obtained by use of CZE with UV detection at 185 nm and an electrolyte containing 5 mmol L(-1) EDTA at pH 4.0. Linear calibration plots were obtained in the concentration range10-300 micro mol L(-1); detection limits were 3 micro mol L(-1) for V(IV) and 1 micro mol L(-1) for V(V). The proposed method was demonstrated for the determination of vanadium in groundwater spiked with V(IV) and V(V).     

On-line preconcentration of niobium(V) and tantalum(V) as 4-(2-pyridylazo) resorcinol-citrate ternary complexes in geological samples by ion interaction high-performance liquid chromatography

4-(2-Pyridylazo) resorcinol (PAR) and citrate were used as pre-column complexing agents for the determination of Nb(V) and Ta(V) as ternary complexes in geological samples. Aliquots of 2 ml of the standard and sample solutions containing the Nb(V) and Ta(V) complexes were loaded onto a concentrator column (C18, 0.4 cm x 4.6 mm) with a carrier mobile phase comprising 20% (v/v) methanol and containing 5 mM acetic acid, 5 mM citric acid and 10 mM tetrabutylammonium bromide (TBABr), pH 6.5 at 2 ml/min for 2 min, with the effluent being directed to waste. An automatic switching valve was then switched to flush both complexes from the concentrator column onto a C18 analytical column using a mobile phase comprising 32% (v/v) methanol and containing 5 mM acetic acid, 5 mM citric acid and 3 mM TBABr, pH 6.5 for 2.5 min. The switching valve was then switched back to the original position, and cleaned with methanol for 7 min to eliminate unwanted species still adsorbed to the concentrator column. This procedure prevented later eluting compounds from reaching the analytical column, which reduced the overall run time. The detection limits of Nb(V) and Ta(V) (determined at a signal-to-noise ratio of 3, detection wavelength of 540 nm and a 2-ml sample volume) were 0.012 and 0.039 ppb for Nb(V) and Ta(V), respectively. Recoveries of Nb(V) and Ta(V) were 99.4 and 96.2%, respectively. The HPLC results obtained from the reference granite and basalt samples agreed well with inductively coupled plasma MS and certified values, but the HPLC method yielded slightly low values of the Nb/Ta ratio.     

Simultaneous capillary electrophoretic separation and detection of P(V) and As(V) As heteropoly-blue complexes

A capillary electrophoretic (CE) method was developed for the simultaneous determination of P(V) and As(V). A Mo(VI)-ascorbic acid reagent reacted with a mixture of trace amounts of P(V) and As(V) to form the corresponding heteropoly-blue complexes in 0.05 M acetate buffer (pH 3.5). When 0.05 M malonate buffer was used as a migration buffer, the peaks due to their migrations were well separated in the electropherogram, and the pre-column complex-formation reaction was applied to the simultaneous CE determination of P(V) and As(V) with direct UV detection at 220 nm. With the proposed method, the calibration curves were linear in the concentration range of 5 x 10(-7) - 1 x 10(-4) M, with a detection limit of 1 x 10(-7) M (a signal-to-noise ratio of 3). Interference from foreign ions was also discussed.     

Quantitative analysis of chromium(V) by EPR spectroscopy

A procedure to accurately quantitate chromium(V) in environmental and medicinal chemistry samples was developed using electron paramagnetic resonance spectroscopy (EPRS) as the method of detection. It was found to have an error in the order of +/-10% and a detection limit of 0.010 mM (0.5 mg l(-1)) chromium(V). The method has been used to quantitate the formation of chromium(V) in the interaction of chromium(VI) with fulvic acid and a simple model of this acid, viz, 1.2-dihydroxybenzene. Analysis of solutions obtained from the reaction of 1,2-dihydroxybenzene with chromium(VI) demonstrated that even when the organic substrate was present in a 182-fold excess, the maximum chromium(V) concentration attained represented just 1.44% of the initial chromium(VI). Reactions between chromium(VI) and fulvic acid yielded similar results. It was therefore concluded that at background environmental concentrations of chromium and fulvic acid, the production of chromium(V) is insignificant, however, its possible importance in contaminated systems cannot be disregarded on this basis alone. The method for quantitative analysis reported in this paper should be an invaluable tool for investigations into the significance of chromium(V) in the toxicological mechanism of chromium(VI) and its role as a mutagenic agent.     

Selective solid‐phase extraction using a molecularly imprinted polymer for the analysis of patulin in apple‐based foods

The aim of this work was to evaluate the use of a molecularly imprinted polymer as a selective solid‐phase extraction sorbent for the clean‐up and pre‐concentration of patulin from apple‐based food products. Ultra high pressure liquid chromatography coupled to ultraviolet absorbance detection was used for the analysis of patulin. The molecularly imprinted polymer was applied, for the first time, to the determination of patulin in apple juice, puree and jam samples spiked within the maximum levels specified by the European Commission No. 1881/2006. High recoveries (>77%) were obtained. The method was validated and found to be linear in the range 2–100 μg/kg with correlation coefficients greater than 0.965 and repeatability relative standard deviation below 11% in all cases. Compared with dispersive solid‐phase extraction (QuEChERS method) and octadecyl sorbent, the molecularly imprinted polymer showed higher recoveries and selectivity for patulin. The application of Affinisep molecularly imprinted polymer as a selective sorbent material for detection of patulin fulfilled the method performance criteria required by the Commission Regulation No. 401/2006, demonstrating the suitability of the technique for the control of patulin at low ppb levels in different apple‐based foods such as juice, puree and jam samples.     

Speciation of antimony(III) and antimony(V) in cell extracts by anion chromatography/inductively coupled plasma mass spectrometry

An analytical method for the separation and quantification of Sb(III) and Sb(V) using anion chromatography with ICP-MS is presented. The optimum conditions for the separation of the antimony species were established with 15 mmol/L nitric acid at pH 6 as eluent system on a PRP-X100 column. The retention times for antimony(V) and antimony(III) were 85 s and 300 s with detection limits of 0.06 microg/L and 0.29 microg/L, respectively. The proposed method was applied to cell extracts of Leishmania donovani, which were incubated with antimony(III) and antimony(V). Some metabolism seemed to occur within the cells.     

A Coulometric Analysis Method and an Ion-exclusion Chromatographic Method for the Determination of Antimony(V) in Large Excess of Antimony(III)

A coulometric analysis method and an ion-exclusion chromatographic method were developed for the determination of antimony(V) in a large excess of antimony(III). Antimony(V) reacted with potassium iodide in a high concentration hydrochloric acid; the liberated iodine was determined by the standard-addition method using coulometrically generated iodine. Using a Dionex ICE-AS1 ion-exclusion column, antimony(V) was eluted with 40 mmol/L sulfuric acid; on the other hand, antimony(III) was strongly retained on the column. The content, expressed as the amount ratio of antimony(V) to antimony(III), was 0.035% in a 10 g/kg antimony(III) solution prepared from an antimony(III) oxide reagent by the coulometric analysis method and 0.036% in a 1 g/kg antimony(III) solution prepared from the same antimony(III) oxide by the ion-exclusion chromatographic method. The results of both methods were in good agreement with each other. The detection limit of antimony(V) in antimony(III) oxide by the former method was 0.004% of antimony(III), and that by the latter method was 0.002% of antimony(III).