高效毛细管电泳电导法快速检测复方维生素B片中的VBl、VBl2、VB6和VC

采用高效毛细管电泳电导法同时分离、测定了复方维生素B片中的主要成分VB1，VB12，VB6和VC的含量。研究了运行缓冲溶液的酸度和浓度、电泳电压、进样时间等因素对电泳的影响。在优化的实验条件下：40mmol/L Tris-4mmol/L H3BO3(pH8．0)的缓冲溶液中加入0．30mmol/L CTAB(溴化十六烷基三甲基铵)，分离电压为15kV，上述4组分在5min内得到良好的分离。维生素B1，B12，B6和VC的线性范围分别为5．5～1．0mg/mL；15～1．5mg／mL;1．0～0．40mg／mL和6．6～0．80mg／mL；检测限分别为0．80μg/mL，4．0μg/mL，0．50μg/mL，2．9μg/mL；5次测定峰高的相对标准偏差分别为2．2％，1．6％，3．9％，2．8％。5次测定的平均回收率分别为99％，94％，l00％，97％。     

毛细管电泳法测定复方芦丁片中的芦丁和维生素C

用毛细管电泳紫外检测法同时测定了复方芦丁片中芦丁和抗坏血酸的含量 ,研究了各种条件的影响 ,得到了优化的实验条件 ,在 30 mmol/L Na2 B4 O7-H3BO3( p H7.5 0 )缓冲溶液中 ,芦丁和维生素 C在 1 3min内得到了良好的分离 ,芦丁和维生素 C分别在 0 .5～ 0 .0 0 5 mg和 5 .0～ 0 .0 5 mg浓度范围内与电泳峰高呈现良好线性关系 ,检测下限分别为 0 .0 0 2 mg和 0 .0 1 mg,应用于实际样品的测定     

毛细管电泳法测定复方芦丁片的芦丁和维生素C

用毛细管电泳紫外检测法同时测定了复方芦丁片中芦丁和抗坏血酸的含量,研究了各种条件的影响,得到了优化的实验条件,在30mmol/L Na2B2O7-H3BO3(pH7.50)缓冲溶液中,芦丁和维生素C在13min内得到了良好的分离,芦丁和维生素C分别在0.5-0.005mg和5.0-0.05mg浓度范围内与电泳峰高呈现良好线性关系,检测下限分别为0.002mg和0.01mg,应用于实际样品的测定。     

毛细管区带电泳法测定复方芦丁片中芦丁和维生素C的含量

考察了缓冲溶液的pH、背景电解质浓度及分离电压对芦丁、维生素C及苯甲酸分离的影响，建立了以苯甲酸为内标，毛细管区带电泳法快速测定复方芦丁片中芦丁和维生素C含量的新方法。以3g/L硼砂－4g/L硼酸(pH8.18）为运行缓冲液，苯甲酸为内标，在分离电压为25kV，检测波长为254nm的电泳条件下，芦丁、维生素C和内标可在5min实现分离。芦丁的线性方程为：y=2．65x＋0．095（r＝0．9994），线性范围为0．025mg/mL－0．4mg/mL，维生素C的线性方程为：y＝3．1343x＋0．565（r＝0．9991），线性范围0．125mg/mL－1．0mg/mL。方法可用于复方芦丁片的质量控制。     

复方芦丁片中主要成分的毛细管电泳安培检测

用毛细管电泳安培检测法同时测定了复方芦丁片中芦丁和抗坏血酸的含量 ,研究了各种实验条件对分离效果的影响 ,得到了优化的实验条件。以直径为 5 0 μm的碳纤维微电极为工作电极 ,电极电位为+ 0 .80V(vs.Ag AgCl) ,4 0mmol L的Na2 B4O7 H3 BO3 (pH值为 7 5 0 )为缓冲溶液。在此条件下 ,芦丁和维生素C在 1 0min内得到了良好的分离。芦丁和维生素C分别在 5 .0×1 0 - 8～ 5 .0× 1 0 - 4 g mL、8.0× 1 0 - 8～ 5 .0× 1 0 - 4g mL浓度范围内与电泳峰电流呈现良好的线性关系 ;检测下限分别为 2 .0× 1 0 - 8、5 .0× 1 0 - 8g mL。方法应用于实际样品的测定 ,结果令人满意     

高效毛细管电泳电导法快速检测复方维生素B片中的VB1、VB12、VB6和VC

采用高效毛细管电泳电导法同时分离、测定了复方维生素B片中的主要成分VB1, VB12,VB6和VC的含量.研究了运行缓冲溶液的酸度和浓度、电泳电压、进样时间等因素对电泳的影响.在优化的实验条件下40 mmol/L Tris -4 mmol/L H3BO3 (pH 8.0) 的缓冲溶液中加入0.30 mmol/L CTAB(溴化十六烷基三甲基铵),分离电压为15 kV,上述4组分在5 min内得到良好的分离.维生素B1,B12,B6和VC的线性范围分别为5.5～1.0 mg/mL; 15～1.5 mg/mL; 1.0～0.40 mg/mL和6.6～0.80 mg/mL; 检测限分别为0.80 μg/mL, 4.0 μg/mL, 0.50 μg/mL, 2.9 μg/mL; 5次测定峰高的相对标准偏差分别为2.2%, 1.6%, 3.9%, 2.8%.5次测定的平均回收率分别为99%, 94%, 100%, 97%.     

高效毛细管电泳-安培检测法用于芦丁水解常数的研究

用高分辨率、高灵敏度的毛细管电泳-安培检测法对芦丁水解的速率常数进行了研究，建立了芦丁及其水解产物槲皮素的定量分析方法。在优化电泳条件下，该方法能同时检测芦丁和槲皮素的峰电流随水解反应的进行而发生的变化。根据芦丁随着水解时间的不同而发生的浓度变化，计算求得水解的速率常数，并总结了温度对速率常数影响的规律。将方法用于芦丁和槲皮素的检测，芦丁与槲皮素的检测限分别为0．6g／L和6．2mg／L；RSD(n=7)分别为2．36％和3．12％。用于槐米中芦丁检测的回收率为97．6％。分析结果表明，此法用于测定芦丁水解常数简便、直观，用于芦丁和槲皮素的检测可靠性和重现性均很好。     

毛细管电泳-柱端安培检测测定莲子心中荷叶碱、芦丁和金丝桃甙的含量

采用毛细管电泳-柱端安培检测测定莲子心中荷叶碱、芦丁和金丝桃甙的含量．研究了检测电位、运行缓冲液浓度和pH值,分离电压和进样时间对分离和检测的影响．以微碳圆盘电极（Ф=0.5ram）为工作电极,检测电位为＋0．95V（vs．Ag／AgCl）,pH为7．25的50mmol／L Na2B4O7和100mmol／L NaH2PO4缓冲液为运行液,当分离电压为15kV时,3种分析物在15min内完全分离．荷叶碱、芦丁和金丝桃甙的检出限（S／N=3）分别为0．02μg／mL、0．05μg／mL和0．04μg／mL．该方法已成功地应用于莲子心中上述3种活性成分的测定．     

毛细管电泳用于水产品中五种抗生素的同时测定

用毛细管电泳-紫外检测法同时测定水产品中的四环素(TC)、金霉素(CTC)、土霉素(OTC)、多西环素(DC)及氯霉素(CAP)的含量．研究了缓冲体系的酸度、浓度、添加剂、分离电压、进样时间以及温度等条件对分离的影响,得到了电泳的最优条件．在278nm波长处,分离电压为22kV,20mmol／L磷酸氢二钠-10mmol／L柠檬酸(pH值2．8,含0．25mmol／L Na2EDTA和体积分数为4．0％的吐温-80)运行缓冲液下,上述5种组份在25min内得到完全分离．5种抗生素的质量浓度和电泳峰面积在2．5～300．0mg／L和10．0～300．0mg／L范围内呈现良好的线性,TC、CTC、OTC、DC和CAP的相关系数(r)分别为0．9996、0．9992、0．9993、0．9934、0．9987,检测下限为0．5～1．5μg／mL。该方法灵敏度高,重现性好,操作简便,并已成功用于水产品鲫鱼中的5种抗生素残留的检测。     

复方维生素B片中主要成分的高效毛细管电泳电化学法检测

采用高效毛细管电泳－电化学检测法同时测定复方维生素B片中的主要成分维生素B1，B12，B6和C的含量；研究了电极电位，运行缓冲溶液的浓度和酸度，电泳电压和进样时间等对电泳的影响，以微铂电极为工作电极，检测电位＋0．5V（vs SCE)，在pH9.0的15mmol/L Tris-1mmol/L H3BO3缓冲溶液中，上述4组分在5min内获得基线分离；维生素B1，B12，B6和C的线性范围分别为2．1mg/L-1.0g/L,6.0mg/L-0.80g/L,1.4mg/L-0.72g/L和0．97mg/L-0.44g/L检出限分别为0．50mg/L,1.0mg/L,,0.65mg/L和0．40mg/L；5次测定峰高的相对标准偏差分别为2．4％，3．0％，3．1％，和2．5％，5次测定的平均回收率分别为99％，102％，98％和100％。     

Assay of the Related Compounds Thiamphenicol, Florphenicol, and Chloramphenicol by CE

The purpose of this study was to examine the migration behaviour of a mixture of thiamphenicol, its two analogues florphenicol and chloramphenicol, and four impurities found in thiamphenicol. Capillary zone electrophoresis was performed with phosphate–borate or borate running buffers, pH 8.5, with or without addition of sodium dodecylsulphate (SDS). Although the compounds could not be resolved in the absence of SDS, supplementation of both types of buffer, at concentrations of 100 mM and higher, with 50 mM SDS enabled separation. On the basis of migration time and resolution, 100 mM borate buffer containing 50 mM SDS was identified as the best for the study. The accuracy and precision of the method were good under these conditions.     

Electrophoretic behavior study and determination of some active components in Chinese medicinal preparations by capillary electrophoresis

The determination of icariin (IC), rhein (RH), chrysophanol (CH), physcion (PHY), glycyrrhetic acid (GE), and glycyrrhizic acid (GI), in traditional Chinese preparations, Anshen Bunao oral liquid and Maren pill, has been investigated by micellar electrokinetic capillary electrophoresis. With borate buffer (10 mM), SDS (20 mM) and acetonitrile (10%) as background electrolyte (pH 9.55), 20 kV applied voltage and 254 nm UV detection, the six active compounds were completely separated within 10 min. The effects of buffer pH, concentration of borate, SDS and modifier on electrophoretic behavior and separation are discussed. Regression equations revealed linear relationships (correlation coefficients: 0.9960-0.9999) between the peak-area of each component and the content. In addition, the levels of the six active compounds in two kinds of traditional Chinese medicinal preparations were easily determined with recoveries of from 94.7% to 106.4%.     

Surfactant‐coated graphitized multiwalled carbon nanotubes as the pseudostationary phase in electrokinetic chromatography for the analysis of phytochemical compounds in biological fluids

This report describes the use of surfactant‐coated graphitized multiwalled carbon nanotubes (SC‐GMWNTs) as a novel pseudostationary phase in CE with diode array detection for the determination of phenolic acids and tanshinones in herbal and urine samples. Several parameters influencing the separation were studied, such as the concentrations of SDS, GMWNTs, and isopropanol; choice of carbon nanotubes; sodium borate content; and buffer pH. The results revealed that the presence of SC‐GMWNTs in buffer enhanced the separation efficiency for the target analytes relative to conventional micelles due to the strong interaction between the surface of the GMWNTs and the target compounds. Under the optimum conditions, the method showed good linearity, with correlation coefficients higher than 0.9950. LODs were in the range of 0.71–3.10 μg/mL. Furthermore, satisfactory separations were achieved with good recovery values in the range of 89.97 and 103.30% when 10 mM borate, 30 mM SDS, 10% isopropanol, and 6 μg/mL SC‐GMWNTs were introduced into the buffer solution.     

Determination of baicalin, chlorogenic acid and forsythin in Chinese medicinal preparation by capillary electrophoresis

Summary The determination of baicalin, chlorogenic acid and forsythin in a traditional Chinese medicinal preparation, Shuanghuanglian oral liquid, has been investigated by micellar electrokinetic capillary electrophoresis using borate buffer, SDS and acetonitrile as background electrolyte, 15 kV applied voltage and UV detection, the three active compounds were completely separated within 15 min. The effect of buffer pH, concentration of borate and SDS are discussed. Regression equations reveal linear relationships between the peak-area of each component and content. In addition, the levels of three active compounds in traditional Chinese medicinal preparation, Shuanghuanglian oral liquid, were easily determined with recoveries of 95.20–105.73%.     

Analysis of glycopeptide antibiotics using micellar electrokinetic chromatography and borate complexation

Micellar electrokinetic chromatography (MEKC) was investigated as a technique for the separation and analysis of the following related glycopeptide antibiotics: alpha-avoparcin, beta-avoparcin, ristocetin A, ristocetin B and vancomycin. Sodium dodecyl sulfate (SDS) micelles were employed as the pseudostationary phase in conjunction with borate or CHES buffers at pH 9.2. A complete separation of the glycopeptides was achieved only when two separation mechanisms were employed simultaneously: (i) differential partitioning of the glycopeptides into SDS micelles; and (ii) differential complexation of the glycopeptides with the borate anion from the borate buffer. Quantitatively, linearity was confirmed for each antibiotic from 0.5 to 40 ppm, with correlation coefficients (r(2)) ranging from 0.9996 (vancomycin and beta-avoparcin) to 0.9986 (alpha-avoparcin). Detection limits ranging from 0.01 ppm (vancomycin) to 0.2 ppm (avoparcin) were achieved, and the mean recovery of avoparcin at the 10 ppm level was 99.2%.     

市售大黄及三黄片中蒽醌类活性成分的胶束电动毛细管色谱含量测定

建立了胶束电动毛细管色谱分离和测定大黄及其制剂三黄片中蒽醌类活性组分的方法．考察了背景电解质pH、表面活性剂浓度、有机改性剂种类和浓度对分离的影响．实验结果表明：在缓冲液pH为9．5、SDS浓度为25mmol／L、乙氰浓度为20％时的优化条件下,大黄及三黄片中蒽醌类活性组分得到基线分离且方法具有较好的重现性．     

胶束电动毛细管色谱法检测红曲米中的莫纳可林K

建立了测定红曲米中莫纳可林K含量的胶束电动毛细管色谱(MEKC)方法。考察了运行缓冲液的种类、pH及其浓度、有机添加剂、十二烷基硫酸钠(SDS)的浓度和分离电压等实验条件对电泳分离效果及检测灵敏度的影响。在优化的实验条件下,以20 mmol/L硼砂(pH 10.6,含10%(体积分数)乙醇和40 mmol/L SDS)作为缓冲溶液,莫纳可林K能在23 min内实现很好的基线分离,线性范围为5.00～100.00 mg/L,线性相关系数为0.9976,检出限(以信噪比(S/N)为3计)为0.13 mg/L,加标回收率为98.5%～99.5%。精密度和稳定性试验中,峰面积和迁移时间的相对标准偏差均小于3%,表明重复性良好。该方法简便、快速、灵敏,可用于红曲米中莫纳可林K含量的测定。     

High-Speed Separation of Oleanolic acid and Ursolic acid from the Fruit of Ligustrum Lucidum ait and Crataegus by Cyclodextrin-Modified Micellar Electrokinetic Chromatography

ABSTRACT

A cyclodextrin-modified micellar electrokinetic chromatography (CD-MEKC) technique for determining oleanolic acid and ursolic acid in the fruit of Ligustrum lucidum Ait and Crataegus was developed. The two bio-active components were successfully separated within 4 minutes using a pH 8.5 sodium borate buffer containing 60mM SDS and 2mM γ-CD. The correlation coefficients of the linear calibration graphs for the analyses exceeded 0.9980. The effects of pH, SDS, γ-CD, sodium borate and temperature on separation were also investigated.     

胶束电动毛细管色谱分离氨基酸和磷酸化氨基酸

本文报道了胶束电动毛细管色谱分离、汞灯诱导荧光电荷耦合器件检测分析氨基酸和磷酸化氨基酸的 4-氟 - 7-硝基苯 - 2 - 口恶 - 1 ,3-丫唑衍生物。研究表明 ,在 p H9.35的 1 0 mmol/L硼砂和 1 0 mmol/L十二烷基硫酸钠的电泳缓冲介质中 ,5种氨基酸和 3种磷酸化氨基酸在 1 0 min内完全分离 ,检测灵敏度为 1 .2 1× 1 0 - 8～ 5 .2 1×1 0 - 8mol/L ,分离效率达 7.3× 1 0 5～ 3.0× 1 0 5/m理论塔板数 ,结果令人满意     

Micellar electrokinetic chromatography of enkephalin-related peptides with laser-induced fluorescence detection

Eight enkephalin-related peptides were derivatized using fluorescein isothiocyanate (FITC), and the derivatization products were separated and detected by capillary electrophoresis with laser-induced fluorescence detection. The optimum molar ratio of FITC and peptide for derivatization was found to be 40:1, and 5 mmol/L sodium borate buffer (pH 9.2) was selected as derivatization media in order to get the high efficiency. Enkephalin-related peptides were completely separated in the pH range of 10.51-10.60 in a running buffer consisting of 100 mmol/L sodium borate and 60 mmol/L sodium dodecyl sulfate (SDS). The detection limit for these eight enkephalins ranged from 0.18 to 2.25 nmol/L, and the linear response range was 1.0 x 10(-6) to 1.0 x 10(-9) mol/L with correlation coefficients between 0.9947-0.9988. A separation efficiency as high as 380000 theoretical plates could be obtained for these analytes.