毛细管电泳光导纤维发光二极管诱导荧光检测法同时测定肾上腺素和多巴胺

采用自行设计、组装的毛细管电泳光导纤维发光二极管诱导荧光检测装置,建立了同时测定肾上腺素(EP)和多巴胺(DA)的方法。采用胶束电动色谱分离模式,通过优化分离电压、十二烷基硫酸钠(SDS)浓度、背景电解质浓度和pH等影响因素,在最佳实验条件下,EP和DA的线性范围分别为2.2×10-9~1.1×10-7mol/L和2.6×10-8~1.2×10-6mol/L,EP和DA的检测限(S/N=3)分别为1.2×10-9mol/L和1.1×10-8mol/L。该方法可应用于人血浆中EP和DA含量的测定。     

毛细管电泳柱后衍生激光诱导荧光测定动物组织中卡那霉素类抗生素

采用毛细管电泳柱后衍生激光诱导荧光测定3种卡那霉素类抗生素。研究了在反向电渗流条件下HAc-NaAc缓冲液酸度和浓度对卡那霉素类抗生素分离的影响,研究了Na2B4O7缓冲体系和柱后衍生试剂萘二醛/2-巯基乙醇浓度对检测信号的影响。采用50 mmol/L HAc-NaAc(pH5.0) 0.5 mmol/L CTMAB溶液为分离缓冲液,样品在-15 kV下分离,与柱后衍生试剂1.0 mmol/L NDA 8.0 mmol/L 2-ME 35 mmol/LNa2B4O7(pH10.0)的30%(V/V)甲醇溶液反应,激发诱导荧光检测卡那霉素类抗生素检出限为3.6×10-5~5.2×10-5g/L;本方法用于动物组织中卡那霉素类抗生素残留检测,相对标准偏差小于7.2%;回收率为90.2%~95.3%(n=4)。     

毛细管电泳分离-激光诱导荧光检测生物胺

采用新合成的6-氧-[(1-琥珀酰亚胺)氧酰甲基]-荧光素乙酯(SOFE)作为柱前衍生试剂,毛细管电泳分离-激光诱导荧光检测了乙醇胺(EOA)、组胺(His)、甲胺(MA)、乙胺(EA)、酪胺(TYR)及苯乙胺(PEA)6种生物胺。在硼酸-硼砂缓冲溶液(pH8.5)中,室温(25℃)下衍生10min。用pH8.5的含25mmol/LSDS15%(V/V)乙腈的40mmol/L硼酸盐溶液作为电泳缓冲溶液,6种衍生物在15min内完全分离,检出限在2.5×10-11～8×10-11mol/L之间。该方法应用于酱油中生物胺的测定,结果令人满意。     

递质氨基酸的毛细管电泳-安培检测

研究了毛细管电泳安培检测氨基酸的方法。氨基酸用萘 -2,3 -二羧醛 (NDA)衍生为电活性物质。碳纤维电极采用1.5V ,30s固定电压电化学预处理 ,检测结果令人满意。作者还对最佳衍生反应条件 ,电极预处理条件对氨基酸衍生物电化学行为的影响进行了研究。该法对谷氨酸、甘氨酸、丙氨酸、γ -氨基丁酸的检出限分别为2.5×10-7、2.5×10-7、5.0×10-8、2.5×10-7 mol/L。     

芯片毛细管电泳-NDA柱前衍生荧光检测多巴胺及组胺

本文以汞灯为激发光源,利用自组装的高灵敏芯片毛细管电泳荧光光子计数器检测系统,NDA柱前衍生检测神经递质多巴胺和组胺。优化了NDA衍生多巴胺、组胺以及衍生后分离与检测的条件。本法多巴胺和组胺的检出限(S/N=3)分别为2.5×10-7mol/L、1.4×10-6mol/L。组胺和多巴胺可在45s内分离和检测。     

毛细管电泳-化学发光法测定人血清中的异烟肼

基于碱性介质中异烟肼对laminol-K3Fe(CN)6化学发光体系的增敏作用,设计了一个经毛细管电泳(CE)分离,在线化学发光检测异烟肼的新方法.研究并优化了毛细管电泳分离及化学发光检测的条件.在优化的实验条件下,该方法测定异烟肼的线性范围为4.0×10-7～1.0×10-5g/mL(R2=0.9984),检出限(3σ)为1×10-8g/mL,对6.0×10-6g/mL的异烟肼进行6次平行测定,其相对标准偏差为4.0%.方法已用于血清中异烟肼的测定.     

毛细管电泳-激光诱导荧光检测肌腱和肌腱细胞中的羟脯氨酸

建立毛细管电泳-激光诱导荧光检测(CE-LIF)分析羟脯氨酸的方法。肌腱和肌腱细胞中的胶原蛋白碱水解生成氨基酸,经异硫氰酸荧光素(FITC)衍生,采用LIF-CE分离测定胶原蛋白特异性氨基酸-羟脯氨酸。羟脯氨酸在0.5μg/L~8×103μg/L浓度范围内线性关系良好;检出限为0.5μg/L。相对迁移率和相对峰高的相对标准偏差(RSD)分别为5.0%和6.1%。测定了60份肌腱和9份细胞样品,加标回收率为95%~110%。将所建立的毛细管电泳方法与高效液相色谱法(HPLC)进行比较,两者测定结果相对误差为-1.9%~2.0%。本法仅需一次荧光标记,操作简单、快速灵敏,12min内完成一个分析周期,适于测定肌腱和细胞样品。     

一种以发光二极管为激发光源的荧光检测器

利用高亮度发光二极管作为激发光源组装了一荧光检测器并应用于毛细管电泳检测 ;激发光斑与毛细管检测池的耦合通过透镜加光阑组合方式实现 ;光纤用于收集并传输荧光信号 ,增加了光学系统的灵活性和紧凑性 ;光阑、检测池和光纤之间的校准简单、方便 ;用荧光素和异硫氰酸荧光素衍生的氨基酸考察了体系性能 ,最小检测浓度为0.18μmol/L(S/N=5) ,在2×10-7～4×10-5 mol/L范围内表现出较好的线性关系(r=0.993) ,结果表明该系统灵敏度达到了普通荧光检测器的指标     

NDA柱前衍生毛细管电泳高灵敏安培检测组胺

本文提出了毛细管电泳 2,3 萘二甲醛(NDA)柱前衍生高灵敏安培检测组胺的新方法,对衍生反应条件和电泳分析条件,包括衍生试剂浓度、衍生溶液的pH值、衍生反应时间、分离介质的pH值、进样时间和分离电压进行了优化,确定衍生溶液pH值为9.0,NDA浓度为5.0×10-4mol/L,CN-浓度为2.5×10-3mol/L时的衍生效果最佳;10mmol/LTris H3PO4(pH5.0)为最佳电泳缓冲液,检测电位为0.7V(vs.SCE)时,组胺检出限达6.8×10-8mol/L(S/N=3),较不衍生测定法灵敏度提高6倍,为测定痕量组胺提供了一个新方法。     

汞灯光源芯片毛细管电泳荧光电荷耦合器件检测系统

以宽谱带高压汞灯为光源的倒置荧光显微镜,配备电荷耦合器件(CCD)及微流控芯片,自组装芯片毛细管电泳荧光电荷耦合器件检测系统。选择不同激发波长(340~540 nm)荧光试剂,进行荧光检测,荧光素的检出限(S/N=3)为7.3×10-9mol/L,荧光素异硫氰酸酯(FITC)的检出限(S/N=3)为1.7×10-8mol/L,显示了该系统对荧光试剂选择范围宽、灵敏度高的特点。用该系统成功分离了FITC与荧光素、曙红与荧光素两种混合荧光试剂。实验表明,组装的芯片毛细管电泳CCD荧光检测系统是成功的。     

A capillary electrophoresis method for the determination of soluble monosaccharides in Ginkgo biloba leaves

A method for the simultaneous determination of six monosaccharides by pre-column derivatization with 1-phenyl-3-methyl-5-pyrazolone and capillary electrophoresis was developed in this work. The derivatization (i.e., reaction temperature, capillary electrophoresis duration, and extraction number) and separation (i.e., pH and buffer concentration) conditions for capillary electrophoresis were optimized. Results showed that the limits of detection under optimal conditions were in the range of 0.036–0.35 mg/L with a mean correlation coefficient >0.99. The recoveries were in the range of 87.3–108.49%, and the relative standard deviations of intra- and inter-day variations were in the ranges of 2.2–3.8 and 3.2–5.0%, respectively. The method was successfully applied to the analysis of six free monosaccharides in three types of Ginkgo biloba leaves.     

Determination of Amino Acids in Panax notoginseng by Microwave Hydrolysis and Derivatization Coupled with Capillary Zone Electrophoresis Detection

The microwave hydrolysis and derivatization coupled with capillary electrophoresis detection were developed for the separation and determination of the amino acids in Panax notoginseng.The experimental conditions for the microwave hydrolysis and derivatization were examined and optimized. Several parameters of capillary electrophoresis, such as pH value of background electrolyte, borate concentration and applied voltage were optimized. Under the selected conditions, 11 amino acids were completely separated. The real sample was analyzed and the results were satisfactory. Compared with that of conventional heat hydrolysis and derivatization, the analytical time of this method was significantly shortened.     

Continuous on-line derivatization and selective separation of D-aspartic acid by a capillary electrophoresis system with a continuous sample introduction interface

A rapid and selective method is described for the separation of D-aspartic acid (D-Asp) using a continuous on-line derivatization system coupled to capillary electrophoresis (CE). D-Asp was derivatized using o-phthaldialdehyde/N-acetyl-L-cysteine (OPA/NAC). By on-line derivatization, amino acid enantiomers were automatically and reproducibly converted to the UV-absorbing diastereomer derivatives which were separated by capillary zone electrophoresis (CZE) in the presence of 10 mmol/L beta-cyclodextrin (beta-CD). Under the investigated separation conditions, D-Asp is resolved from L-aspartic acid (L-Asp) and other amino acids in a standard mixture of amino acids. The separation could be achieved within 4 min and the sample throughput rate can reach up to 16 h(-1). The repeatability (defined as relative standard deviation, RSD) was 3.21%, 3.58% with peak area evaluation and 3.72%, 4.03% with peak height evaluation for L-Asp and D-Asp.     

Repartition effect of aromatic polyaniline coatings on the separation of bioactive peptides in capillary electrophoresis

The capillary walls of fused-silica capillary electrophoresis (CE) columns were modified with a thin film of polyaniline (PANI), providing open-tubular columns with a stable coating containing aromatic groups and amine functionalities. Fast and efficient separations were observed for small bioactive peptides under acidic conditions on PANI-coated columns. The mechanism of separation is based on hydrophobic interactions between the analytes and the polymeric matrix. Good reproducibility was observed from run-to-run. Due to the simple derivatization procedure, method flexibility, the uniformity of the coating and its stability, conjugated polymers could find practical application in capillary zone electrophoresis (CZE) separations.     

Rapid and sensitive determination of phosphoamino acids in phosvitin by N-hydroxysuccinimidyl fluorescein-O-acetate derivatization and capillary zone electrophoresis with laser-induced fluorescence detection

A method was developed for the determination of phosphoamino acids by capillary zone electrophoresis-laser-induced fluorescence detection (argon ion laser, excitation at 488 nm and emission at 520 nm) using derivatization with N-hydroxysuccinimidyl fluorescein-O-acetate (SIFA). Different variables affecting the derivatization (SIFA concentration, derivatization pH, reaction temperature and reaction time) and the separation (type, pH and concentration of buffer, applied voltage and injection mode) were investigated in detail. The optimized separation conditions were 40 mM boric acid buffer (pH 9.2) for background electrolyte, 25 kV for the separation voltage, 25 degrees C for the capillary temperature and 5 s at 0.5 psi for the sample injection. Under the optimal conditions, the SIFA-labeled phosphoamino acids were fully separated within 7 min. The detection limits ranged from 0.1 to 0.3 nM, which are the lowest values reported for capillary electrophoresis (CE) methods. The proposed methodology allowed the rapid, sensitive and selective determination of phosphoamino acids in hen egg yolk phosvitin by the standard addition method. The recovery of these compounds in real sample was 94.0-103.5%. The developed method surpasses previously published CE methods in terms of detection limit, separation time, stability and simplicity of the electrophoretic procedure.     

On-column derivatization and analysis of amino acids, peptides, and alkylamines by anhydrides using capillary electrophoresis

This work demonstrates the use of an in-capillary procedure for derivatization of amino acids, peptides, and alkylamines by anhydrides using capillary electrophoresis (CE). Migrating in an uncoated fused-silica capillary, plugs of substrate and anhydride are injected separately and electrophoresed. Differential transport velocities permit the separate zones to penetrate each other under an applied field, thereby facilitating reaction. In initial experiments the extent of reaction between tryptophan and acetic anhydride was examined and product amounts quantitated by CE. In separate experiments a series of amino acids and peptides were injected into the capillary and reacted with phthalic anhydride on-column to yield the phthalic derivatized species. Finally, on-column derivatization of alkylamines with phthalic anhydride was investigated and electrophoretic mobility related to molecular weight of the derivatized amines. These procedures illustrate the use of the capillary as a microreactor in the facile synthesis of derivatized molecules and ease of quantitation of reaction products under conditions of electrophoresis.     

Method of intracellular naphthalene-2,3-dicarboxaldehyde derivatization for analysis of amino acids in a single erythrocyte by capillary zone electrophoresis with electrochemical detection

A novel method of intracellular derivatization was developed. In this method, the derivatization reagents [naphthalene-2,3-dicarboxaldehyde (NDA) and CN-] were introduced into living cells by electroporation for the derivatization reaction. After completion of derivatization reaction in cells, a single cell was drawn into the capillary tip by electroosmotic flow. Then the lysing solution was introduced into the capillary by diffusion. Once the individual cell was lysed, the derivatized amino acids in the individual cell were separated by capillary zone electrophoresis and detected by end-column amperometric detection at the outlet of the capillary. This method of intracellular NDA derivatization confined the analytes and the derivatization reagents to the volume of a single cell expanded. For an 8-microm erythrocyte, the contents were diluted by a factor of only ca. 1.6. The method was used to determination of amino acids in single erythrocytes. Six amino acids were identified and quantified.     

毛细管电泳法分析藏红花植物细胞多糖中单糖组成

以对甲氧基苯胺为衍生试剂,采用毛细管电泳法分析了藏红花植物细胞多糖中的单糖组成。对衍生条件进行了优化,并对毛细管分离条件进行了系统的研究。衍生反应在醋酸含量9.5%(v/v)、80 ℃下反应2 h的衍生产率最大,衍生产物紫外检测波长234 nm。在优化的毛细管电泳分离条件(未涂层熔融石英毛细管柱(60 cm(有效长度50 cm)×50 μm),柱温25 ℃,电压20 kV,使用350 mmol/L硼酸电解液(pH 10.21),压力(3.4475 kPa)进样5 s)下,基线分离了11种结构相近的醛糖(来苏糖、木糖、核糖、葡萄糖、甘露糖、半乳糖、鼠李糖、纤维二糖、麦芽糖、乳糖)、酮糖(果糖)的衍生产物。应用该方法定量检测了藏红花植物细胞多糖水解物中糖的成分,各糖的回收率为94.3%～105.4%,相对标准偏差为3.3%～4.6%。     

Direct determination of gentamicin components by capillary electrophoresis with potential gradient detection

A simple and fast method was developed to determine non-UV active compounds directly without derivatization. The usefulness of the method was demonstrated by detecting the major components in aminoglycoside antibiotic mixtures using capillary zone electrophoresis with potential gradient detection. Under optimized separation conditions (0.2 mM cetyltrimethylammonium bromide (CTAB), 1 mM ammonium citrate, pH 3.5), gentamicin was separated into three major peaks (C1, C1a, and C2+C2a) within 15 min. This method showed better sensitivity than other capillary electrophoresis (CE) methods for determining underivatized gentamicin. The linear range was from 10 to 500 ppm. Because of its good repeatability and simplicity, this new method could be a good alternative for the current assays given by US Pharmacopoeia and European Pharmacopoeia.     

Nonaqueous capillary electrophoresis with laser-induced fluorescence detection: a case study of comparison with aqueous media

A novel method based on separation by nonaqueous capillary electrophoresis (NACE) combined with laser-induced fluorescence (LIF) detection was developed and compared with classic aqueous modes of electrophoresis in terms of resolution of solutes of interest and sensitivity of the fluorescence detection. Catecholamines derivatized with 4-chloro-7-nitro-2,1,3-benzoxadiazole (NBD-Cl) were chosen as test analytes for their subtle fluorescence properties. In aqueous systems, capillary zone electrophoresis (CZE) was not suitable for the analysis of test analytes due to complete fluorescence quenching of NBD-labeled catecholamines in neat aqueous buffer. The addition of micelles or microemulsion droplets into aqueous running buffer can dramatically improve the fluorescence response, and the enhancement seems to be comparable for micellar electrokinetic chromatography (MEKC) and microemulsion electrokinetic chromatography (MEEKC). As another alternative, NACE separation was advantageous when performing the analysis under the optimum separation condition of 20 mM sodium tetraborate, 20 mM sodium dodecyl sulfate (SDS), 0.1% (v/v) glacial acetic acid, 20% (v/v) acetonitrile (ACN) in methanol medium after derivatization in ACN/dimethyl sulfoxide (DMSO) (3:2, v/v) mixed aprotic solvents containing 20 mM ammonium acetate. Compared with derivatization and separation in aqueous media, NACE-LIF procedure was proved to be superior, providing high sensitivity and short migration time. Under respective optimum conditions, the NACE procedure offered the best fluorescence response with 5-24 folds enhancement for catecholamines compared to aqueous procedures. In addition, the mechanisms of derivatization and separation in nonaqueous media were elucidated in detail.