HPLC法测定杜仲中维生素K1

为检测杜仲中维生素K1含量,采用了特异性强、分离效果好的高效液相色谱(HPLC)法,将样品经丙酮、石油醚提取,用失活磷酸盐处理过的氧化铝进行柱色谱净化处理,用极性不同的洗脱液将维生素K1从样品中分离出来,收集V(石油醚) V(乙醚)=97 3洗脱组分,浓缩定容,用C18色谱柱对维生素K1进行定性定量分析,流动相为V(甲醇) V(正己烷)=75 25,紫外检测波长为248 nm。结果表明,在流量为1.5 mL/min的条件下,维生素K1的保留时间为(2.18±0.1)min,r为0.999 3,回收率87.67%~95.12%,杜仲中的维生素K1含量为12.404 3μg/g。     

Determination of 1-aminocyclopropane-1-carboxylic Acid in Apple and Peach Extracts by High Performance Liquid Chromatography Coupled to a Fluorescence Detector

A new, sensitive, and simple HPLC method was described for the determination of 1-aminocyclopropane-1-carboxylic acid (ACC) in apple and peach extracts. The method was based on the derivatization of ACC with fluorescamine in borate buffer systems of pH 8.0 to yield a highly fluorescent product. The experimental parameters affecting the derivatization reaction efficiency were optimized by fluorimetric analysis. Under optimum derivatization conditions, the derivative product of ACC in apple and peach extracts without extra purification was successfully chromatographed on a C-18 column by HPLC coupled to fluorescence detection. The derivative product of ACC with fluorescamine could be well separated from other concomitant substances or their derivatives that might interfere with the determination of ACC. The linearity of ACC was measured in the range of 23.82–238.82 µg · L^?1 with a good correlation coefficient of 0.9997. Based on signal-to-noise ratio of 3, a low detection limit of 5.0 µg · L^?1 could be reached. The proposed method was applied successfully to the determination of ACC in the crude apple and peach extracts without extra purification with low RSDs of 0.19–1.9% and good recoveries of 90.89–104.4%. The sensitive HPLC quantitative method is of great significance for the investigations of ACC metabolism in plants.     

乳粉中维生素K1高效液相色谱测定方法的改进

通过改进流动相和样品处理方法，确定了最佳的流动相配比，缩短了分析时间（Rt=11min左右），降低了检出限（0．02μg／lOOg），维生素K1的最小检出浓度达到0．20μg／100g．     

用高效液相色谱测定食物中维生素B_1、B_2含量

本文着重介绍使用高效液相色谱荧光测定天然食品中维生素B_1、B_2含量。在测试维生素B_1时,使用键合C_(18)分析柱,流动相为CH_3OH-0.01M KH_2PO_4 45/55,流速1.5ml/min,Ex:390nm,EM:470nm,柱温45℃;测维生素B_2时用强阳离子交换柱,流动相CH_3OH/0.01M KH_2PO_4,CH_3OH由30～70分钟梯度淋洗,流速1.5ml/min,柱温45℃,Ex:449nm,EM:530nm。在上述条件下所测部分食物中维生素B_1的回收率是92.51～101.85%,变异系数2.14～6.57%;维生素B_2的回收率为89.91～95.18%,变异系数0.19～6.19%。部分食物样品的测试结果令人满意。     

柱前衍生-高效液相色谱法测定茶叶中的黄曲霉毒素B1

应用柱前衍生-高效液相色谱法测定茶叶中黄曲霉毒素B1的含量。样品采用乙腈(85+15)溶液提取,滤液用MycoSepTM226柱净化,加入正己烷和三氟乙酸衍生,经C18色谱柱分离,荧光检测器检测。黄曲霉毒素B1的质量浓度在0.20~10.0μg·L-1范围内与其峰面积呈线性关系,检出限(3S/N)为0.1μg·kg-1。在0.5,1.0,5.0μg·L-1等3个浓度水平进行加标回收试验,回收率在91.9%~102%之间,测定值的相对标准偏差(n=6)在1.5%~6.9%之间。     

Purification of Complex of SAV1 with PP1A

SAV1 is a core component involved in the Hippo pathway which can control the organ size via regulating cell proliferation and apoptosis simultaneously. We explored the regulatory mechanism of SAV1. We established the HEK293T cell pool, the cells in which can stably express SAV1 by retroviruses infection and found that SAV1 stable cells reduced the movement of themselves and resulted in multicellular aggregation. We purified SAV1 interacting protein complex using streptavidin resin and subsequently analyzed the digested peptides by high performance liquid chromatography(HPLC)-MS/MS. Results show that about 150 proteins were identified in the complex of SAV1 with protein. TUBA1A, OTUD4, and ATD were identified as proteins interacting with SAV1. Importantly, PP1A, serine/threonine protein phosphatase PP1-alpha 1 catalytic subunit, was also in the top 10 list. The interaction between PP1A and SAV1 was detected by both co-immunoprecipitation(CO-IP) and immunostaining. Our results indicate that PP1A might be the phosphatase of SAV1 and may take part in the regulation of the Hippo pathway.     

Determination of 1-nitropyrene in low volume ambient air samples by high-performance liquid chromatography with fluorescence detection

To measure the actual exposure of a person to 1-nitropyrene (1-NP) in airborne particulate matter, it is considered more accurate to collect air samples with a portable air sampler than to sample at a fixed location. However, because the portable samplers can sample only small volumes, a sensitive method is needed to analyze the compounds that are collected on a filter. Here we describe a high-performance liquid chromatographic (HPLC) method with fluorescence detection that is sensitive and precise enough for use with portable air samplers. The developed column-switching system successfully removed the interfering substances in the samples with only a simple pretreatment. To improve the precision of the measurement, deuterated 1-NP was used as an internal standard, and it eluted immediately prior to 1-NP with sufficient resolution (R_s, 1.50). The detection limit was 0.32 fmol/injection, and the calibration range was from 2 to 100 fmol. The proposed method was applied to determining 1-NP in fine airborne particulate matter (PM_2.5) at two sites with low pollution levels. 1-NP was detected in all samples at concentrations in the low fmol/m³ range. The proposed method has enough sensitivity and precision to determine 1-NP in the limited air volume of the portable sampler.     

阿维菌素B1a纯物质的制备纯化研究

本研究致力于制备纯化出高纯阿维菌素B1a,为核磁定量及质量平衡法提供计量溯源纯物质,从而给阿维菌素标准物质(研制中)纯度定值时提供纯度参考标准。利用制备型液相色谱对阿维菌素原料(B1a含量为95.71%)进行纯化,除去痕量杂质,真空干燥及冷冻干燥后得到阿维菌素B1a高纯物质。建立了基于制备液相色谱-真空干燥的阿维菌素B1a高纯物质的制备纯化工艺:采用Agilent Prep HT XDB-C18型制备柱,流动相为水/甲醇(15∶85),进样量500μL,流速20.0m L/min。经超高效液相色谱(UPLC)检测,产品纯度达到99.74%,可以满足核磁定量及质量平衡法的要求,并利用液相色谱串联质谱以及核磁共振法对产品进行定性分析。     

Monolithic rod columns for HPLC based on divinylbenzene-styrene copolymer with 1-vinylimidazole and 4-vinylpyridine

Monolithic chromatographic columns for HPLC based on divinylbenzene-styrene both with 1-vinylimidazole and with 4-vinylpyridine are prepared. The monoliths were synthesized in glass tubes with the inner diameter of 2?mm. Texture, hydrodynamic and chromatographic properties of the prepared columns were studied. Linear solvation energy relationships model was applied for the characterization of columns selectivity It is shown that changing the on 1-vinylimidazole or 4-vinylpyridine content in the initial solution allows to change the selectivity of the columns. An examples of small molecules and some proteins separations are presented.     

Enantiomere und diastereomere 2-Methoxymethyl-pyrrolidin-1-dithiocarbonsäureester

Summary Formation of the 2-methoxymethyl-pyrrolidine-1-dithiocarboxylates2–4 and alkylation of2 and3 were studied. Enantiomeric and diastereomeric derivatives of4, the preparation of diastereomeric mixtures of4 by alkylation of3 in the presence of strong bases, and formation of6 by phase transfer alkylation of2 are described. The two enantiomers of 2-(4-bromophenyl)-2-oxo-ethyl 2-methoxymethylpyrrolidine-1-dithiocarboxylate2 have been characterized by X-ray analysis.

Verstorben am 22. Juni 1996     

A simple chromatographic method for determining norfloxacin and enoxacin in pharmacokinetic study assessing CYP1A2 inhibition

We developed a simple assay method for the determination of serum and urine norfloxacin and enoxacin using reversed‐phase high‐performance liquid chromatography and perchloric acid precipitation for sample pre‐treatment. Optimized conditions can permit detection of norfloxacin and enoxacin in the same chromatogram, so either compound can be used as an internal standard for another determinant. Supernatants of the precipitated samples were analyzed by the octadecylsilyl silica‐gel column under ambient temperature and an ultraviolet wavelength of 272 nm. A mobile phase solvent consisting of 20 mm sodium dihydrogenphosphate (pH 3.0) and acetonitrile (85:15, v/v) was pumped at a flow rate of 1.0 mL/min. The calibration curves for norfloxacin and enoxacin at a concentration of 62.5–1000 ng/mL for serum and 250–4000 ng/mL for urine were linear (r > 0.9997). The recoveries of norfloxacin and enoxacin from serum and urine were >94% with the coefficient of variations (CV) <5%. The CVs for intra‐ and inter‐day assay of norfloxacin and enoxacin were <4.2 and <5.5%, respectively. This method can be applied to the pharmacokinetic study of norfloxacin and enoxacin after repeated administration to assess changes in CYP1A2 activity in healthy subjects. Copyright © 2010 John Wiley & Sons, Ltd.     

Studies on pharmacokinetics,body distribution,plasma protein binding rate,and excretion of 1-methyl hydantoin in rats in vivo

In this paper, plasma concentration, plasma protein binding rate, body distribution, and excretion of both oral and intravenous administration of rats were determined by high performance liquid chromatography (HPLC) combining with UV detector. The blood drug concentration of oral and intravenous administration was summarized. The bioavailability of T_1/2 was approximately 0.75?hr. At the meanwhile, the bioavailability was about 18.84?±?2.21%. The plasma protein binding rate of 1-methyl hydantoin was about 24.36?±?0.93%, belonging to low protein binding drug. The result shows that 1-methyl hydantoin can be rapidly distributed in various organs and tissues and quickly eliminated within 6?hr without accumulation in the organs. Its discharge from the urine and feces was 16.58?±?4.48% and 3.37?±?0.71%, respectively. All of the results showed that the recovery rate, liner relationship, specificity, stability, and precision of the method were good. The study also proved that 1-methyl hydantoin has been eliminated quite faster in rats.     

高效液相色谱法测定淡水鱼肝脏中维生素A_1和A_2

建立了用高效液相色谱法同时测定淡水鱼肝脏中VA_1和VA_2的方法。以μ-Porasil 3.9mm i.d.×150mm为色谱柱,混合溶剂(正己烷:乙醚=87:13)为流动相,采用紫外350mm,荧光,Ex 325nm、Em480nm双道检测,VA_1、VA_2的保留时间分别为26.25min和28.00min。采用不同波长条件下的紫外吸收特性对VA_2予以定性,以VA_1为内标物对VA_2予以定量。实验分析了几种淡水鱼肝脏中的VA_1和VA_2的含量。     

Transport behavior and efflux of Rg1 in rat pulmonary epithelial cells

The aim of this study was to investigate whether ginsenoside Rg1 could be transported into rat pulmonary epithelial cells and its transport behavior and efflux through the cells. A high-performance liquid chromatography coupled with 2487 UV-vis detector at 203 nm was applied. The mobile phase was 0.05% phosphate-acetonitrile (75:25, v/v). Cells were incubated with Rg1 (100 microg/mL) for a specific time, then lysed and sonicated in methanol to extract intracellular Rg1. Cells incubated with Rg1 and verapamil or KCN were processed by the same method. A 20 microL aliquot of sample was injected into the HPLC system to determine Rg1 concentration. The results showed that Rg1 could be transported into the epithelial cells with peak concentration of 1.28 microg/10(5) cells at 0.5 h. Metabolic inhibitor KCN and P-glycoprotein inhibitor verapamil could increase Rg1 concentration within the cells, indicating that efflux of Rg1 was energy-dependent and P-gp was likely to be involved. This is the first time that the transport behavior and efflux of Rg1 through rat pulmonary epithelial cells has been demonstrated. The phenomenon that Rg1 concentration in the cells decreased whereas that in the medium remained high indicated that a more effective means of drug administration should be found.     

Separation of Tic-hydantoin enantiomers,potent sigma-1 agonists,by high performance liquid chromatography and capillary electrophoresis

Stereospecific separations of seven Tic-hydantoin sigma-1 agonists were performed by both HPLC method using derivatized cellulose and amylose chiral stationary phases and capillary electrophoresis (CE) method using neutral and anionic cyclodextrins added in the background electrolyte (BGE). An optimal baseline separation (R_s > 3.3 with analysis times < 25 min) was readily obtained with all silica-based celluloses and amyloses using a normal-phase methodology. CE was used as an alternative technique to HPLC for the Tic-hydantoin derivatives separation. The enantiomers were fully resolved with highly sulfated β-cyclodextrins at pH 2.5 (R_s > 1.5 with analysis times <11 min). Both methods were validated in terms of linearity, detection and quantification limits. They were used to check the enantiomeric purity of the enantiomers.     

手性高效液相色谱拆分3-取代异吲哚-1-酮的研究

从伏牛花类植物中提取的生物碱Lennoxam ine^[1]、Nuevam ine和Chilenine,新研发的抗焦虑药Paz-inaclone^[2]和Pagoclone^[3]以及利尿、抗高血压药Chlortalidone^[4]等均含有光活性3-取代异吲哚-1-酮(2,3-二氢-1H -异吲哚-1-酮).这类化合物还是一类新型的不对称合成手性辅助基^[5].因此,光学纯的3-取代异吲哚-1-酮化合物在药物研发和不对称合成等领域具有应用前景.但有关它们的色谱拆分少见报道^[6,7].本文对15个外消旋3-取代异吲哚-1-酮样品进行高效液相色谱拆分研究,通过建立的手性色谱方法,不仅准确测定了相关产物的光学纯度,而且确认了N -取代邻苯二甲酰亚胺上手性辅助基在不对称合成过程^[8]中未发生消旋化.同时探讨了样品中3-位取代基对手性拆分的影响.     

1-甲基-1-乙氧基-1-烷硫基甲烷类化合物的合成研究

本文以乙缩醛和烷基硫醇为原料,在30－35℃于四氯化碳中反应20min左右,分别合成1－甲基－1－乙氧基－1－烷硫基甲烷,经红外光谱,质谱以及核磁共振谱检测,确证了产物结构。     

Determination of aflatoxin B1 in cereals by homogeneous liquid-liquid extraction coupled to high performance liquid chromatography-fluorescence detection

A simple and rapid method based on homogeneous liquid-liquid extraction coupled to HPLC with fluorescence detection was developed for the determination of aflatoxin B1 (AFB1) in the rice and grain samples after post-column derivatization. The proposed method eliminated the use of immunoaffinity columns for clean-up in the determination of AFB1. The parameters affecting recovery and preconcentration such as type and volume of organic solvent, volume ratio of water/methanol, concentration of phase separator reagent and extraction time were optimized. Under the optimized conditions, the calibration graph was linear in the concentration range of 0.01-1.0 ng/g with the detection limit of 0.003 ng/g. This method was successfully applied for the analysis of AFB1 in different cereal samples.     

Chromatographic characteristics of poly(1-vinylimidazole)-grafted silica in normal-phase HPLC

A stationary phase based on poly(1-vinylimidazole)-grafted silica has been prepared by the surface radical chain-transfer reaction. The stationary phase was characterized by infrared spectra, X-ray photoelectron spectroscopy and elemental analysis. Chromatographic characteristics of the stationary phase were investigated in normal-phase HPLC. The results showed that both weak polar compounds (polycyclic aromatic hydrocarbons, dialkyl phthalates) and polar compounds (anilines, phenols) could be successfully separated on this stationary phase, implying better separation performance than blank silica and conventional aminopropyl-bonded silica under the same conditions. The excellent performance can be attributed to multiple interactions between surface modifier and the analytes that might include dipole, hydrogen bonding, H-π, electrostatic and inductive interactions.     

Fully automated column-switching HPLC determination of aflatoxin M1 in milk using dialysis as sample preparation

A procedure has been developed for the automated determination of aflatoxin M1 in decreamed milk, by using on-line dialysis and subsequent trace enrichment on a reverse phase column. After foreflush to the analytical column the determination is performed with fluorescence detection. Fully automated analysis within 10 min is thus possible with reproducible dialysis recoveries above 50% (CV is 3.3%, n = 20) and detection levels of 50 ng/kg.