高效液相色谱法同时测定中药材亳菊中多菌灵、吡虫啉和啶虫脒的残留量

建立了同时测定中药材亳菊中多菌灵、吡虫啉和啶虫脒残留量的高效液相色谱分析方法。样品经盐酸溶液超声提取,乙醚除杂,二氯甲烷萃取后,采用ODS柱,以V(乙腈):V(0.1%磷酸,三乙胺调pH至3.6)=14:86为流动相,270nm波长处检测。结果三种农药呈良好的线性关系(r为0.9997、0.9998和0.9999),最低检出浓度分别为0.04,0.02和0.1 mg/kg。方法的平均加标回收率范围分别为:83.8%～101.3%,81.8%～90.8%和83.6%～95.0%,对应的RSD分别为:3.9%～4.3%,2.6%～3.3%和3.5%～5.9%。方法能够满足多菌灵、吡虫啉和啶虫脒在中药材亳菊中残留分析的要求。     

高效液相色谱法测定黄瓜和油菜中的啶虫脒残留量

建立了一种高效液相色谱测定黄瓜和油菜中啶虫脒农药残留的方法。以乙腈提取,弗罗里硅土净化,采用Agilent 1100高效液相色谱仪带DAD检测器对待测组份进行了分离和测定,检测波长254 nm,使用C18不锈钢反相柱（250 mm×4.6 mmi.d.,5μm）,以V（乙腈）∶V（水）=30∶70作流动相,啶虫脒在0.05-2.00mg/L范围内呈良好的线性关系（r=0.9999）,方法的添加回收率范围为73.7%-85.6%。RSD为2.2%-10.3%,能够满足啶虫脒在黄瓜和油菜中残留分析的要求。     

Pesticides analysis by liquid chromatography and capillary electrophoresis

Nowadays, a wide range of pesticides are used in agricultural production, and their monitoring in samples of environmental and alimentary interest is of extreme importance to ensure, among others, the safety of consumption of foods. The aim of this work is to provide updated information about the major developments in CE and HPLC in pesticide analysis, covering relevant publications between 2004 and early 2006. The use of different sample pretreatment steps to provide a suitable extraction of these compounds from the different matrices as well as to increase the sensitivity of the determination is also discussed.     

Improved liquid chromatography combined with pulsed electrochemical detection for the analysis of etimicin sulfate

This paper describes an improved liquid chromatography method combined with pulsed electrochemical detection for the analysis of etimicin sulfate. In total, 22 impurities could be separated. A TSK‐GEL C₁₈ column (250 mm × 4.6 mm i.d., 5 μm) is used, and the mobile phase is composed of 40 mL of acetonitrile and 960 mL of an aqueous solution containing trifluoroacetic acid (15 mL/L), pentafluoropropionic acid (500 μL/L), 50% sodium hydroxide (8 mL/L) and sodium sulfate (1.5 g/L). The pH of the aqueous solution is adjusted to 3.5 with 0.8 M sodium hydroxide. The influence of the different chromatographic parameters on the separation was investigated. A quadruple potential‐time waveform was applied to the electrodes of the detection cell. 0.8 M sodium hydroxide was added post column to raise the pH to at least 12 before detection. A central composite experimental design was used to describe the relationship between factors and response values and to establish factorial analysis. Compared to previously published investigations, this improved method shows higher sensitivity, better separation ability and robustness and has been incorporated by the Chinese Pharmacopoeia 2015 for analysis of etimicin sulfate. A number of commercial samples of etimicin sulfate were also analyzed using this method.     

Capillary gas chromatography—atomic emission detection: A useful instrumental method in pesticide residue analysis of plant foodstuffs

The high selectivity of element-specific atomic emission detection has proven suitable for screening analysis of plant foodstuffs for pesticide residues by capillary gas chromatography, especially for those foodstuffs which contain high levels of matrix compounds. The elemental composition of a peak can, furthermore, be examined by looking at the partial emission spectra recorded during a GC run. This instrumental feature prevents false positive signal interpretation as a result of high concentration levels of eluting matrix compounds.     

Identification in residue analysis based on liquid chromatography with tandem mass spectrometry: Experimental evidence to update performance criteria

Liquid chromatography-tandem mass spectrometry (LC-MS/MS) is one of the most widely used techniques for identification (and quantification) of residues and contaminants across a number of different chemical domains. Although the same analytical technique is used, the parameters and criteria for identification vary depending on where in the world the analysis is performed and for what purpose (e.g. determination of pesticides, veterinary drugs, forensic toxicology, sports doping). The rationale for these differences is not clear and in most cases the criteria are essentially based on expert opinions rather than underpinned by experimental data. In the current study, the variability of the two key identification parameters, retention time and ion ratio, was assessed and compared against requirements set out in different legal and guidance documents. The study involved the analysis of 120 pesticides, representing various chemical classes, polarities, molecular weights, and detector response factors, in 21 different fruit and vegetable matrices of varying degrees of complexity. The samples were analysed non-fortified, and fortified at 10, 50 and 200 μg kg⁻¹, in five laboratories using different LC-MS/MS instruments and conditions. In total, over 135,000 extracted-ion chromatograms were manually verified to provide an extensive data set for the assessment. The experimental data do not support relative tolerances for retention time, or different tolerances for ion ratios depending on relative abundance of the two product ions measured. Retention times in today’s chromatographic systems are sufficiently stable to justify an absolute tolerance of ±0.1 min. Ion ratios are stable as long as sufficient response is obtained for both product ions. Ion ratio deviations are typically within ±20% (relative), and within ±45% (relative) in case the response of product ions are close to the limit of detection. Ion ratio tolerances up to 50% did not result in false positives and reduced the false negative rate for pesticides with product ions in the low S/N range to <5%. Without ion ratio criterion, two false positives were obtained in 105 non-fortified samples. Although the study has been conducted for pesticides residues in fruits and vegetables, the impact of these findings is believed to extend towards other application areas and possibly support adjustment or consolidation of criteria across other analytical domains.     

The advantages of evaporative light scattering detection in pharmaceutical analysis by high performance liquid chromatography and supercritical fluid chromatography

The evaporative light scattering detector (ELSD) has been used in pharmaceutical analysis by liquid and supercritical fluid chromatography. An ELSD equipped with interchangeable interfaces enables the use of various eluents (UV- or non-UV-absorbing) in isocratic or gradient mode. Analyses were performed on several non-UV-absorbing excipients and active substances. The narrow spread of the response factors of the various compounds investigated has indicated that the detector is suitable for direct raw quantitation of unknown samples in stability studies.     

Determination of phenols in water by on-line solid-phase disk extraction and liquid chromatography with electrochemical detection

Poly(styrene-divinylbenzene) (PS-DVB) membrane extraction disks were used as sorbents for the on-line solid phase extraction of 13 phenols (nitro and chlorophenols) in river and tap waters. Determination was performed by liquid chromatography with electrochemical detection (LC-ED). An acetate buffer-acetonitrile-methanol mixture as mobile phase and amperometric detection at +1100 mV were used. High water volumes, up to 250 ml, can be preconcentrated without loss of phenols (recoveries between 80% and 100%) except for the more polar ones. Moreover, detection limits between 0.01 and 0.1 μg l⁻¹ in tap water and between 0.1 and 1.0 μg⁻¹ in river water were obtained. The method has been applied to the analysis of two river water samples.     

A review of liquid chromatography in environmental pesticide analysis

Summary The use of liquid chromatography in environental pesticide analysis is reviewed. In addition to classical UV and electrochemical detectors, detection systems such as mass spectromytry and gas chromatographytype detectors are discussed. The applicability of supercritical fluid chromatography to pesticide analysis is also reviewed.Presented at the 18th International Symposium on Environmental Analytical Chemistry, Barcelona 5–8 September, 1988.     

Algorithms for the assessment of peak purity in liquid chromatography with photodiode-array detection. Part II

Two modifications of the algorithm based on the Gram-Schmidt orthogonalization technique for the assessment of peak purity are presented. The performance of this approah is investigated for liquid chromatography with photodiode-array detection (LC-DAD) data, although its applicability is not restricted to this experimental model. This method is applied to simulated and experimental data where two compounds are eluting, but can be applied when more compounds are eluting. The results are compared with the ones obtained previously with the first version of this algorithm.     

High performance liquid chromatography with post-column photolysis of pesticides for generation of fluorophores

Summary Several classes of pesticides have been found to respond to a high performance liquid chromatography post-column reaction detector that employs UV photolysis with an optional reaction with o-phthalicdicarboxaldehyde-2-mercaptoethanol (OPA-MERC) reagent followed by fluorescence detection. Photolysis of most of the N-methylcarbamates, carbamoyl oximes, carbamothioic acids, dithiocarbamates, and phenylureas tested produced primary amines which reacted with OPA-MERC to form the respective derivatives. In some cases, substituted aromatic pesticides such as phenylcarbamates, phenylamides, and phenylureas photolyzed to chemical species which had native fluorescence. This technique was successfully applied to a method for pesticide analyses in groundwater and vegetation. For aldicarb sulfone, a pesticide that did not absorb UV light, use of acetone as a photosensitizer enhanced detection.     

Multi-component calibration and analysis in liquid chromatography

Multi-wavelength detectors offer improved detection capabilities for liquid chromatographic methods, but require improvements in data analysis methodology to utilize all the available information. In this work, various methods for improving the quantitative results obtained from liquid chromatography with full spectrum fluorescence detection were studied. The availability of multi-wavelenght information allows overlapped chromatographic peaks to be resolved. Different approaches were investigated for developing calibration models that use all of the available spectral information, and are compatible with a variety of methods for quantification, including factor analysis, Kalman filtering and rank annihilation. These methods were compared for their ability to resolve overlapped chromatographic peaks and their accuracy in quantification.     

Determination of prednisolone and prednisone in plasma by liquid chromatography with fluorescence detection

After a single-step extraction from plasma (250 μl) with dichloromethane, the drugs and dexamethasone (internal standard) are oxidized by copper(II) acetate to the corresponding glyoxal and converted into the fluorescent quinoxalines by reaction with 1,2-diamino-4,5-methylenedioxybenzene. The quinoxalines are separated within 55 min by reversed-phase liquid chromatography with isocratic elution. The detection limits for prednisolone and prednisone added to plasma are 3 ng ml^?1 in plasma (signal-to-noise ratio=3).     

Advances in capillary electrophoresis: the challenges to liquid chromatography and conventional electrophoresis

In the 1980s, capillary electrophoresis (CE) developed rapidly into a first-class analytical separation technique. Its advances in instrumentation and method development will not only enhance or complement existing mature separation techniques such as liquid chromatography and conventional slab gel electrophoresis, but will also severely challenge these separation methods. A brief overview of the most striking achievements of CE in the 1980s is given. which illustrates the challenges to liquid chromatography and conventional slab gel electrophoresis, and some detailed discussions are presented to highlight the advantages of CE. New developments in CE that can be expected for the 1990s include especially column technology, separation chemistry and instrumentation, which will serve further to diversify and improve the applicability of this technique in areas which are poorly addressed by other separation methods. This paper considers and speculates on the technological advancements that can be expected to emerge for CE in the 1990s.     

Evaluation of automated and manual hot-splitless,cold-splitless (PTV), and on-column injection technique using capillary gas chromatography for the analysis of organophosphorus pesticides

Three different injection modes were compared for the analysis of organophosphorus pesticides. Differing results were found for several compounds depending on their chemical structure and thermostability. The programmed temperature vaporizing injector used in this study seemed to be the most promising sampling device for pesticide residue analysis in biological samples.     

Development of chemical isotope labeling liquid chromatography mass spectrometry for silkworm hemolymph metabolomics

Silkworm (Bombyx mori) is a very useful target insect for evaluation of endocrine disruptor chemicals (EDCs) due to mature breeding techniques, complete endocrine system and broad basic knowledge on developmental biology. Comparative metabolomics of silkworms with and without EDC exposure offers another dimension of studying EDCs. In this work, we report a workflow on metabolomic profiling of silkworm hemolymph based on high-performance chemical isotope labeling (CIL) liquid chromatography mass spectrometry (LC-MS) and demonstrate its application in studying the metabolic changes associated with the pesticide dichlorodiphenyltrichloroethane (DDT) exposure in silkworm. Hemolymph samples were taken from mature silkworms after growing on diet that contained DDT at four different concentrations (1, 0.1, 0.01, 0.001 ppm) as well as on diet without DDT as controls. They were subjected to differential ¹²C-/¹³C-dansyl labeling of the amine/phenol submetabolome, LC-UV quantification of the total amount of labeled metabolites for sample normalization, and LC-MS detection and relative quantification of individual metabolites in comparative samples. The total concentration of labeled metabolites did not show any significant change between four DDT-treatment groups and one control group. Multivariate statistical analysis of the metabolome data set showed that there was a distinct metabolomic separation between the five groups. Out of the 2044 detected peak pairs, 338 and 1471 metabolites have been putatively identified against the HMDB database and the EML library, respectively. 65 metabolites were identified by the dansyl library searching based on the accurate mass and retention time. Among the 65 identified metabolites, 33 positive metabolites had changes of greater than 1.20-fold or less than 0.83-fold in one or more groups with p-value of smaller than 0.05. Several useful biomarkers including serine, methionine, tryptophan, asymmetric dimethylarginine, N-Methyl-D-aspartic and tyrosine were identified. The changes of these biomarkers were likely due to the disruption of the endocrine system of silkworm by DDT. This work illustrates that the method of CIL LC-MS is useful to generate quantitative submetabolome profiles from a small volume of silkworm hemolymph with much higher coverage than conventional LC-MS methods, thereby facilitating the discovery of potential metabolite biomarkers related to EDC or other chemical exposure.     

高效液相色谱荧光检测法测定蔬菜中残留的甲氨基阿维菌素苯甲酸盐

建立了甘蓝和蘑菇中甲氨基阿维菌素苯甲酸盐的固相萃取-高效液相色谱荧光分析方法。蔬菜样品用乙酸乙酯提取,提取液旋转浓缩近干后用少量乙酸乙酯溶解,再经PRS固相萃取(SPE)柱净化,洗脱液经氮气吹干后用氮甲基咪唑和三氟乙酸酐衍生,衍生物用高效液相色谱分析,采用外标法定量。在添加浓度1.0～20.0 μg/kg范围内,平均添加回收率为78.6%～84.9%,日内相对标准偏差(RSD)为2.7%～6.0%,日间RSD为3.1%～8.9%,检出限为0.10 μg/kg。甲氨基阿维菌素苯甲酸盐衍生物在0.002～0.10 mg/L范围内呈良好的线性关系,相关系数为0.9999。     

Isolation and determination of paspalitrem-type tremorgenic mycotoxins using liquid chromatography with diode-array detection

A liquid chromatographic (LC) method is described for the isolation and determination of the tremorgenic mycotoxins paxilline (Penicillium paxilli NRRL 6110), paspaline, paspalinine and paspalicine (Claviceps paspali). Following a Soxhlet extraction of a mould-contaminated matrix using chloroform, the crude extract was partitioned between hexane and 80% aqueous methanol. The latter fraction, containing the desired toxin(s), was evaporated to dryness, the residue dissolved in methylene chloride and the solution analysed by liquid chromatography using a Supelcosil LC-Si column eluted with methylene chloride-diethyl ether (9 + 1, v/v). A mixture containing standards of these compounds was similarly analysed. All toxins were detected using a UV diode-array detector. The generated UV spectra and chromatographic data of the standard toxins were stored in a computer as a library and used to identify these toxins in a crude mixture. The purity of the separated peaks and the amount of toxin in the crude mixture were also determined. The toxins were isolated by selectively collecting the eluted peaks using a programmable fraction collector equipped with a peak level sensor. Further confirmation of compound identity was achieved by mass spectrometry using the direct inlet probe method. In comparison with methods used previously to isolate these toxins, the present technique is fast and allows the acquisition of complete UV spectral information and chromatographic data and the isolation of multiple toxins in a single chromatographic operation.     

Validation of a method for the analysis of quinolones residues in bovine muscle by liquid chromatography with electrospray ionisation tandem mass spectrometry detection

A liquid chromatography-tandem mass spectrometry method for the determination and confirmation of nine quinolones was optimised and validated according to Commission Decision 2002/657/EC. Analytes were extracted from veal muscle with water and extracts purified with 96-well plates Oasis HLB cartridges. Separation was carried out in a silica-based C₁₈ column (50 mm × 2.1 mm) with mobile phases consisting of water/acetonitrile mixtures containing acetic acid. Linear calibration curves in the ranges 4-400 and 50-800 ng g⁻¹, with correlation coefficients at least 0.995, were obtained for all the analytes. At concentration levels above 10 ng g⁻¹, quantification errors were lower than 10% and repeatability and within-laboratory reproducibility standard deviations below 6% and 10%, respectively. Decision limits and detection capabilities are reported.