高效毛细管电泳,激光干涉检测快速分离二糖研究

首次报道一种高效毛细管电泳、激光干涉折射检测快速分离二糖的新方法。详细研究了四硼酸钠溶液中，ｐＨ值、四硼酸钠浓度及有机添加剂对二糖－硼酸络离子迁移行为的影响，发现在ｐＨ为９．７的０．１ｍｏｌ／Ｌ四硼酸钠溶液中，１０ｍｉｎ内４种二糖得到基线分离。采用自制激光干涉型折射指数检测器，不需对二糖衍生化处理，可直接进行在柱检测。     

单糖、多元醇亚砷酸络合物毛细管电泳分离研究

采用激光干涉检测方法系统研究了单糖、多元醇亚砷酸络合物的电泳行为;并考察了溶液中ｐＨ值、亚砷酸盐浓度对单糖、多元醇亚砷酸络合物淌度的影响。实验结果表明,在亚砷酸溶液中,单糖和多元醇的选择性好,峰形尖锐;从而建立了一种单糖、多元醇毛细管电泳分离及直接检测的新方法。     

高效毛细管电泳中的激光光热检测技术

集中介绍了激光光热分析在高效毛细管电泳检测上的应用；分析了各种光热检测构型的特点，阐述了影响光热信号的各种因素；指出了激光光热检测技术在高效毛细管电泳中的应用前景。     

毛细管电泳-间接激光光热干涉检测方法研究

本文提出毛细管电泳-间接激光光热干涉检测新方法。采用吸收系数大、吸收波长与泵浦激光(He-Ne)波长匹配性能较好的亚甲蓝溶液为背景电解质溶液,加入乙醇减少了毛细管壁对亚甲蓝的吸附作用。并将间接光热干涉检测法用于氨基酸毛细管电泳分离检测,对赖氨酸检测限达5×10^-6mol/L(S/N=2).     

激光回射束干涉相移效应的研究

激光回射束干涉相移效应的研究邓延倬，何金兰（武汉大学分析测试科学系，武汉，４３００７２）关键词激光，折射指数，干涉相移效应，毛细管电泳基于激光回射束干涉相移效应，曾首次用于光热测量［１］和微体积样品检测［２］．本文讨论这种效应的基本原理及其用于分析化...     

流动注射-毛细管电泳联用及应用进展

流动注射是一种高效进样及在线溶液处理手段。毛细管电泳是一种高分离效率、高选择性的分析技术,但传统的毛细管电泳间歇式进样方式效率低且难用于过程分析,将流动注射进样技术与毛细管电泳结合,既弥补了毛细管电泳的进样缺陷,又可兼具两者的优点。有关两种技术的联用一直都在探索之中。文中对近年流动注射一毛细管电泳联用及应用研究进行了综述。     

免疫亲和毛细管电泳的研究进展

免疫亲和毛细管电泳方法结合了免疫分析的高特异性和毛细管电泳分离的高效、快速、样品用量少等优点,是复杂样品中特定组分分析的重要方法之一。激光诱导荧光检测器的使用以及毛细管电泳分离前免疫预富集过程的引入,可以进一步提高分析测定的灵敏度,使其能够用于痕量物质的高灵敏测定。本文结合作者所在课题组的工作,对免疫亲和毛细管电泳的两种主要模式,即均相的毛细管电泳免疫分析(CEIA)和非均相的免疫亲和毛细管电泳(IACE)的研究进展进行了综述。     

芯片毛细管电泳-激光诱导荧光-电荷耦合器件检测系统

采用自组建的芯片毛细管电泳－激光诱导荧光－电荷耦合器件（CCD）检测系统在数十秒内满意地分离了曙红和荧光素。设计了一种进样、分 离电路,可以有效地消除进样通道的样品溶液向分离通道的渗漏。解决了由这种渗漏所引起的电泳峰变宽、拖尾等问题。提高了芯片毛细管电泳的分辨率和分离效率。     

基于适配体-金纳米粒子和光热-激光背向散射干涉技术的水中As(Ⅲ)的定量检测

针对As(Ⅲ)的检测问题,提出了一种基于适配体-金纳米粒子探针和光热-激光背向散射干涉原理的水中As(Ⅲ)的定量检测技术.结合了As(Ⅲ)适配体的金纳米粒子溶液呈现稳定的酒红色,对绿光有较强的吸收作用.采用532 nm的激光照射毛细管内的金纳米粒子溶液,由于光热效应溶液折射率发生变化,激光背向散射干涉(Back-Sca...     

毛细管电泳—激光干涉检测法测定饮料中蔗糖含量

本文将毛细管电泳－激光干涉检测法用于饮料中蔗糖的定量测定。结果表明，在样品浓度低于１０ｍｇ／ｍＬ时，检测信号与样品浓度成正比。样品不需衍生化处理直接进行测定，分析结果较为满意。     

不同缓冲体系对毛细管电泳法分离15种核苷类化合物效果的比较

对毛细管电泳法分离15种核苷类化合物所用的不同缓冲液体系进行了系统比较,确定不同模式毛细管电泳法分析多种核苷类化合物的最适合背景缓冲液体系(BGE)。分别以四硼酸钠、磷酸氢二钠、乙酸钠、碳酸氢钠、乙酸铵和乙二胺(DEA)为背景电解质,对毛细管区带电泳(CZE)、毛细管电泳-电喷雾飞行时间质谱(CE-ESI-TOF/MS)以及胶束电动毛细管电泳(MEKC)3种模式进行比较,并对其中几种优势缓冲体系进行了优化。结果表明,CZE模式下使用四硼酸钠和磷酸氢二钠缓冲体系无法同时分离15种核苷类化合物,因此只适用于分析核苷类化合物数量较少的样品。而使用含有2%丙酮的300 mmol/L DEA能完全分开15种核苷类化合物,且分辨率和峰形良好。MEKC模式下,以25 mmol/L磷酸氢二钠(添加70 mmol/L十二烷基磺酸钠(SDS))为缓冲盐的分离结果最佳,并且此方法能成功应用于海洋生物海葵中核苷类化合物的分离。CE-ESI-TOF/MS分析中,以20 mmol/L乙酸铵(pH 10.0)为背景电解质,正离子模式检测,15种核苷类化合物的质谱信号均良好,检测灵敏度明显优于文献中报道的使用DEA缓冲体系的结果。本研究阐明了不同缓冲体系对15种核苷类化合物分离的适用性,为毛细管电泳技术在复杂基质中多种核苷类化合物的分离方法中的应用奠定了基础。     

Use of non-aqueous capillary electrophoresis for the quality control of commercial saffron samples

A non-aqueous capillary electrophoresis (NACE) method for quantifying the seven crocin metabolites that are the major biologically active ingredients of saffron was developed. Separation is done by using a fused silica capillary filled with a 12.5 mM H3BO3/37.5 mM sodium tetraborate methanolic solution as background electrolyte. The results obtained were compared with the total index "safranal value", widely used as a quality measure of saffron products. The comparison revealed that the proposed NACE method provides useful information not obtained in the safranal value. Infact, samples with a similar safranal value can contain crocin metabolites in different concentrations and relative proportions. This new method is very useful for quality control in commercial saffron samples.     

Determination of streptomycin in eggs yolk by capillary electrophoresis

Summary A capillary electrophoresis method for the determination of streptomycin in eggs is described. Analyses were performed on an uncoated silica capillary using a buffer solution of 30 mM sodium dihydrophosphate, 5 mM boric acid and 5 mM sodium tetraborate. Analytes were detected at 200 nm an the calibration curve was linear over the range of 0.16 to 2.0 μg g⁻¹ (r=0.999). The total analysis time was 7 min. The method has been successfully applied to the quantitative determination of streptomycin in hen eggs after drug ingestion and could used for evaluation of maximum residue limits.     

Continuous flow derivatization system coupled to capillary electrophoresis for the determination of amino acids

A derivatization system coupled to capillary electrophoresis for the determination of amino acids using 1,2-naphthoquinone-4-sulfonate as a labeling agent is described. In this system, amino acids are derivatized on-line in a three-channel flow manifold for sample, reagent and buffer solutions. The reaction takes place in a PTFE coil heated at 80 degrees C. The resulting solution, which contains the amino acid derivatives, is introduced into the electrophoretic system by means of an appropriate interface. Subsequently, amino acid derivatives are separated at 25 kV using a 40 mM sodium tetraborate aqueous solution with 30% (v/v) isopropanol solution as a running buffer. The electropherograms are monitored spectrophotometrically at 230 nm. The method has been applied to the determination of amino acids in feed samples and pharmaceutical preparations. A good concordance of the predicted values with those given by a standard amino acid analyzer is shown.     

蛋白质的毛细管电泳─激光回射干涉检测研究

本文用激光回射干涉检测法研究了酸性蛋白质的毛细管电泳行为。在较高的ｐＨ值和较高离子强度下，采用较短毛细管，减少了管壁对蛋白质的吸附作用，较好地分离了４个标准蛋白质及人血清中蛋白质。相对峰高和相对迁移时间具有较好的重现性。     

Validated method for L-ornithine-L-aspartate analysis in human plasma by capillary electrophoresis

A rapid capillary electrophoresis method for routine determination of two amino acids, L-ornithine and L-aspartic acid, in human plasma is reported. The method runs automatically, requires a minimum of sample preparation and moreover includes no extensive extraction and no gradient or derivatization procedure. Analyses were performed on an uncoated silica capillary using buffer solution composed with 10 mM sodium tetraborate and 1 M sodium hydroxide (pH=10.0). A capillary electrophoresis P/ACE system equipped with UV detection (200 nm), an automatic injector, a fluid cooled cartridge and System Gold data station was used in this study. The total analysis time under these conditions was 8.0 min. The calibration curve was linear in the range 10-280 microg mL-1 for L-aspartic acid and 20-280 microg mL-1 for L-ornithine (for both amino acids, r=0.999). The method was validated by inaccuracy (bias) and precision (RSD) studies by analysing samples. The method was successfully applied to the quantitative determination of L-ornithine-L-aspartate in human plasma and could be useful for clinical and bioavailability investigations.     

Determination of purines including 2,8-dihydroxyadenine in urine using capillary electrophoresis

For the purpose of rapid drug monitoring, methods have been developed for the determination of 2,8-dihydroxyadenine, allopurinol, oxypurinol, adenine, hypoxanthine, hippuric acid and xanthine in urine with and without sodium dodecyl sulfate as additive in sodium tetraborate running buffer. No sample preparation is necessary. 6-methylmercaptopurine and etofylline have been used as the internal standards. The limit of detection is 5 microM and the range of quantification stretches from 20 to 2000 microM. The capillary electrophoresis methods are simple, fast and robust.