手性氨基酸的毛细管电泳拆分研究

以咔唑-9-乙基氯甲酸酯（CEOC）作柱前荧光衍生试剂，在毛细管区带电泳和胶束电动色谱条件下，以不同配比的β-环糊精（β-CD）和脱氧胆酸钠（SDC）作手性选择剂，在两种不同分离模式下，对氨基酸衍生物进行了手性分离，同时对分离过程中的相关参数进行了优化，分别实现了8种和10种氨基酸的快速手性分离。     

瑞香狼毒多糖中单糖组成的毛细管区带电泳分析

采用1-苯基-3-甲基-5-吡唑啉酮(PMP)和1-(2-萘基)-3-甲基-5-吡唑啉酮(NMP)为衍生试剂,以反相高效液相色谱(RP-HPLC)和毛细管区带电泳(CZE)法对9种单糖衍生物进行了分离研究,对比确定了NMP衍生化CZE法在植物多糖单糖组成分析中的优越性。以NMP为柱前标记试剂,建立了毛细管区带电泳定量测定9种单糖的新方法。方法具有较好的重复性(相对标准偏差RSD小于4.3%),单糖衍生物检测限为0.85～1.6μmol/L,回收率为96.4%～104%。已应用于瑞香狼毒多糖样品的单糖组成分析。     

毛细管电泳技术在氨基酸分析中的研究进展

对毛细管电泳技术在氨基酸分析中的研究进展进行了综述,分析了直接法和衍生法对氨基酸进行分析的优缺点,详细叙述了毛细管电泳中的紫外、激光诱导荧光、电化学及质谱等检测方法在氨基酸分析中的应用,并重点总结了毛细管电泳在手性氨基酸分离中的应用.     

毛细管区带电泳分离药用海藻羊栖菜中氨基酸

1　引　　言羊栖菜作为一种药用海藻 ,入药主治甲状腺肿大、淋巴溃疡、动脉硬化等 ,并伴利尿剂 ,还可防止血凝障碍。羊栖菜中富含人体所需 18种氨基酸。目前 ,氨基酸的分析一般采用高效液相色谱法、气相色谱法和毛细管电泳法 ,由于毛细管电泳法具有试样用量小、分离效率高、分离速度快及灵敏度高等特点。因此 ,受到人们广泛重视。国内外曾有人采用异硫氰酸苯脂 (ＰＩＴＣ)作衍生化试剂 ,用毛细管电泳法对氨基酸进行分离 ,最好结果是从 18种氨基酸中可以分离出 15个峰。有多种重要的氨基酸重叠出峰。我们采用美国贝克曼公司生产的高效毛细管…     

氨基酸的分析方法及其应用进展

从衍生试剂角度,介绍了不同衍生化氨基酸的分析方法,包括离子交换色谱法、高效液相色谱法、气相谱法和毛细管电泳法,以及无需衍生化的直接分析法高效阴离子交换色谱-积分脉冲安培法,并总结了蛋白质、食品和生理体液样品中的氨基酸分析方法。     

毛细管电泳在手性氨基酸拆分中的研究进展

毛细管电泳(capillary electrophoresis,CE)作为一种强有力的手性分离技术,由于操作简单、试剂消耗少及柱效高等优点,受到广泛关注,是近年来手性分离领域的研究热点.氨基酸是组成蛋白质的基本单元,且大多数氨基酸具有手性中心,手性氨基酸是生命体系的一个重要特征.具有手性中心的氨基酸,其对映体间的生物活性往往存在着较大的差异,因此,氨基酸的手性拆分对了解人体及动物生命活动起着举足轻重的作用.主要总结了近5年来毛细管电泳的3种分离模式(毛细管区带电泳、胶束电动毛细管色谱、毛细管电色谱)在氨基酸手性拆分中的发展和应用.     

寡糖的毛细管电泳分析

多种寡糖经α－萘胺衍生化后，用硼砂作为电泳介质，实现了高效毛细管电泳分离。比较了毛细管区带电泳和胶束毛细管电动色谱分离寡糖α－萘胺衍生物的电泳行为，对影响分离度的诸因素进行了考察，选择了最佳分离条件。     

藏药蕨麻多糖水解单糖的毛细管区带电泳分离研究

以1-萘基-3-甲基-5-吡唑啉酮(NMP)为柱前衍生试剂,探讨了毛细管区带电泳模式下对藏药蕨麻多糖水解液中单糖的分离条件。实验采用58.5 cm×50μm i.d.毛细管(有效长度50 cm),55 mmol/L硼酸盐缓冲溶液(pH=9.46),柱温20℃,分离电压22 kV,进样10 s。该法不加任何添加剂,9种单糖可高效、快速基线分离,实现了对藏药蕨麻多糖水解液中单糖的分离和定量分析,结果令人满意。     

羧甲基聚合-β-环糊精作为选择剂应用于毛细管电泳法拆分手性化合物

提出了一种用毛细管电泳拆分3种未衍生化的氨基酸对映体(苯丙氨酸,酪氨酸,色氨酸)和一种手性药物(芬氟拉明)的方法.以水溶性羧甲基聚合-β-环糊精为手性选择荆,采用毛细管区带电泳模式,考察了手性选择剂浓度、缓冲溶液pH值、柱温及电压对分离的影响.4种手性化合物在各自优化的试验条件下,均达到基线分离.此法操作简单,可用于这4种手性化合物的质量控制.     

糖类衍生物在毛细管区带电泳下的分离研究

以新合成的1-萘基-3-甲基-5-吡唑啉酮(NMP)为柱前衍生试剂,采用毛细管区带电泳模式考察并优化了糖类衍生物的分离条件。实验采用58.5cm×50μmi.d.毛细管(有效柱长50cm),55mmol/L硼酸盐缓冲溶液(pH9.46),柱温20℃,分离电压22kV,进样10s,在不加任何添加剂的情况下,高效、快速地实现了9种糖的基线分离,并在最优化条件下进行了唐古特白刺实际样品的分离分析,结果令人满意。     

Mobility behaviour of amino acids on silica static phase: micelles activated separations

A new method for separation of several amino acids using mobile phases (MPs) containing mixed micelles as well as 1-butanol and aprotic organic solvents as modifying additives has been developed. The effect of experimental factors (the ratio of MP components, nature of stationary phase) on separation of amino acids is investigated and all conditions for separation are optimized. It was found that separation of three amino acids l-lysine, l-histidine and l-tryptophan on silica gel stationary phase in the interval from micrograms to milligrams is available. The proposed method is simple and allows determining the amino acids in the linear interval of 0.1-1.5mg.     

A capillary electrophoresis detection scheme for underivatized amino acids based on luminol-BrO- chemiluminescence system

A novel chemiluminescence (CL) detection scheme has been developed for detecting underivatized amino acids following capillary electrophoresis (CE) separation. This detection was based on the inhibitory effect of amino acids on the CL reaction between luminol and BrO⁻ in alkaline aqueous solution. Detection of amino acids was accomplished with a borate-based background electrolyte at pH 9.2. The luminol was used as a component of the separation carrier electrolyte. Parameters affecting CE-CL separation and detection, such as the pH value, the concentration of electrolyte and CL reagent on the resolution were optimized. The relative standard deviation for the analysis of amino acids was less than 1.5% for the migration time and 4% for the peak height. The mass limits of detection were from 7 to 144 fmol for the 7 amino acids. This method has been applied of 7 amino acids in amino acid injection.     

Influence of soluble polymer polyvinylpyrrolidone on separation of small peptides and amino acids by microchip-based capillary electrophoresis

In microchip-based capillary electrophoresis, the resolution and separation efficiency of small peptides and amino acids can be noticeably improved by adding a low molecular weight (30,000) soluble polymer additive, polyvinypyrrolidone in the separation medium. Several separation conditions such as injection time and electrophoretic buffer have been investigated and optimized. Using an electro-stacking scheme, the resolution and separation efficiency of small peptides and amino acids can be enhanced significantly. Under the optimal conditions, the separation of fluorescein isothiocyanate Isomer I-labeled small peptides and amino acids was successfully achieved within 100 s.     

New triazine spectroscopic reagent for the separation of DL-amino acids by micellar electrokinetic chromatography

An approach to the chiral separation of racemic mixtures of amino acids by means of micellar electrokinetic chromatography after derivatization with a new triazine spectroscopic reagent, 3-(4,6-dichloro-1,3,5-triazinylamino)-7-dimethylamino-2-methylphenazine (DTDP), has been evaluated. It was found that the derivatives of the aliphatic amino acids such as serine, valine and arginine, could produce a strong UV absorption at 282 nm, whose apparent molar absorptivities are of 10(-4) M(-1) cm(-1), and thus the concentration of the amino acids down to 3 x 10(-7) M can still give a detectable signal (S/N = 3). Beta-Cyclodextrin (beta-CD) added to the buffer system was used as a chiral selector, and separation conditions were optimized. The presence of an organic modifier (2-propanol) was also a prerequisite for the chiral separation. The best results for the chiral separation of DTDP-amino acids were achieved in a mixed sodium dodecylsulfate-beta-CD-borate-2-propanol medium at pH 9.0. Compared to some of the commonly used derivatization methods, the present one offers a relatively stable derivative and strong UV absorption for the spectroscopically inert amino acids, thus enabling amino acids to be separated and detected by CE even with a simpler UV detector.     

采用含原位聚合阴离子交换整体柱的微芯片分离氨基酸

采用原位聚合法,制备了以2-甲基丙烯酰氧乙基三甲基氯化铵(META)为功能单体的强碱性季铵盐离子交换型微整体柱,构建了带微整体柱的复合式微流控芯片;以氨基酸-H2O2-Lum inol化学发光体系为样品对象,根据氨基酸等电点的差异,在原位聚合微整体柱上进行分离实验。进行了苯丙氨酸-白氨酸、苯丙氨酸-组氨酸、苯丙氨酸-精氨酸3组氨基酸混合体系的分离,获得了很好的分离结果。优化并讨论了影响氨基酸分离效果的多种因素,如缓冲液pH值、洗脱液pH值和洗脱液流速等。在优化条件下,苯丙氨酸-精氨酸的分离度达到1.6,结果显示出整体柱与微流控体系相结合的可行性。     

Open tubular capillary electrochromatography of underivatized amino acids using Rh(III) tetrakis(phenoxyphenyl)porphyrinate as wall modifier

The separation of 17 “common” underivatized amino acids was attempted by open tubular capillary electrochromatography (OT-CEC) in fused-silica capillaries coated with Rh(III) tetrakis(phenoxyphenyl)porphyrinate (Rh(III)TPP(m-OPh)₄OAc) using sodium phosphate and Tris–phosphate buffers as background electrolytes (BGEs). The OT-CEC separation of amino acids was compared with that obtained by capillary zone electrophoresis in bare fused-silica capillaries using the same BGEs. The amino acids were not derivatized and the UV-absorption detection was set at 200 nm. Depending on the experimental conditions at least 15 amino acids were separated. The best separations were obtained in a Rh(III)TPP(m-OPh)₄OAc-coated capillary in 50 mM Tris–100 mM phosphate buffer at pH 2.25. Separation of the critical triplet Val–Ile–Leu was always at least indicated being better at higher BGE concentrations. Regarding the sensitivity of the method, lower concentration limits of detection (LODs) in the coated capillary were obtained for Thr, Gly, Tyr, and Val; the other amino acids exhibited lower LODs in the uncoated capillary. The separation of acidic amino acids was not achieved.     

Synthesis and application of dehydroabietylisothiocyante as a new chiral derivatizing agent for the enantiomeric separation of chiral compounds by capillary electrophoretic

A new chiral derivatizing reagent, dehydroabietylisothiocyante (DHAIC), was synthesized and used for the enantiomeric separation of chiral compounds in capillary electrophoresis (CE). The synthetic route to obtain DHAIC is described. The separation conditions for the chiral separation of several chiral compounds, such as protein amino acids and chiral drug DOPA were optimized. Best results for the chiral separation of DHAIC derivatized amino acids and DOPA were obtained in a running buffer consisted of 50 mM borate (pH 9.5), 5 mM sodium dodecyl sulphate (SDS) and 20% acetonitrile for amino acids and 60 mM Na₂HPO₄ (pH 8.0), 17 mM SDS and 25% acetonitrile for DOPA. Under the conditions studied, chiral separation of five amino acids including Ser, Val, Ala, Thr, Cys and a chiral drug DOPA as their diastereomeric DHAIC derivatives has been achieved by micellar electrokinetic chromatography (MEKC).     

Chiral separation of dansyl amino acids in capillary electrophoresis using mono-(3-methyl-imidazolium)-beta-cyclodextrin chloride as selector

Enantioseparations of fourteen dansyl amino acids were achieved by using a positively-charged single-isomer beta-cyclodextrin, mono-(3-methyl-imidazolium)-beta-cyclodextrin chloride, as a chiral selector. Separation parameters such as buffer pH, selector concentration, separation temperature, and organic modifier were investigated for the enantioseparation in order to achieve the maximum possible resolution. Chiral separation of dansyl amino acids was found to be highly dependent on pH since the degree of protonation of these amino acids can alter the strength of electrostatic interaction and/or inclusion complexation between each enantiomer and chiral selector. In general, the chiral resolution of dansyl amino acids was enhanced at higher pH, which indicates that the carboxylate group on the analytes may interact with the imidazolium group of cationic cyclodextrin. For most analytes, a distinct maximum in enantioresolution was obtained at pH 8.0. Moreover, the chiral separation can be further improved by careful tuning of the separation parameters such as higher selector concentration (e.g. 10 mM), lower temperature, and addition of methanol. Enantioseparation of a standard mixture of these dansyl amino acids was further achieved in a single run within 30 min.     

Analysis of amino acids in human vascular endothelial (ECV-304) cells by microchip electrophoresis with fluorescence detection

A rapid and sensitive method was developed for the analysis of amino acids by microchip electrophoresis with Hg-lamp excitation fluorescence detection. Fluorescein-isothiocyanate (FITC) was chosen to estimate the sensitivity of this system, and the detection limit (S/N = 3) with FITC was 1.7 nM, which showed that the system was sensitive as well as simple. Two derivatizing agents, FITC and ortho-phthalaldehyde (OPA) were employed to label amino acids and were compared in the same fluorescence detection system with an Hg lamp as the excitation source. The separation parameters were optimized in detail. Optimum separation of OPA-labeled amino acids was obtained in less than 200 s with 20 mM borate buffer (pH 9.0) containing 20% acetonitrile and 10 mM beta-cyclodextrin. Detection limits for amino acids (alanine (Ala), taurine (Tau), glycine (Gly), glutamic acid (Glu), and aspartic acid (Asp)) of 0.38-1.0 muM were achieved. The method was successfully applied to analysis of amino acids in human vascular endothelial cells (ECV-304). The average amount of amino acids in single ECV-304 cells is estimated to be 5.84 fmol for Ala, 2.78 fmol for Tau, 1.15 fmol for Gly, 3.10 fmol for Glu, and 1.30 fmol for Asp.