Evaluation of capillary zone electrophoresis for the quality control of complex biologic samples: Application to snake venoms

Snake venoms constitute a very promising resource for the development of new medicines. They are mainly composed of very complex peptide and protein mixtures, which composition may vary significantly from batch to batch. This latter consideration is a challenge for routine quality control (QC) in the pharmaceutical industry. In this paper, we report the use of capillary zone electrophoresis for the development of an analytical fingerprint methodology to assess the quality of snake venoms. The analytical fingerprint concept is being widely used for the QC of herbal drugs but rarely for venoms QC so far. CZE was chosen for its intrinsic efficiency in the separation of protein and peptide mixtures. The analytical fingerprint methodology was first developed and evaluated for a particular snake venom, Lachesis muta . Optimal analysis conditions required the use of PDADMAC capillary coating to avoid protein and peptide adsorption. Same analytical conditions were then applied to other snake venom species. Different electrophoretic profiles were obtained for each venom. Excellent repeatability and intermediate precision was observed for each batch. Analysis of different batches of the same species revealed inherent qualitative and quantitative composition variations of the venoms between individuals.     

Influence of temperature control in capillary electrophoresis

We have investigated the influence of capillary temperature on migration time and peak area and have evaluated different cooling systems. It was found that for applied voltages below 15 kV (i.e. those most frequently used) temperature control effectively improves peak area reproducibility but has less effect on migration time.     

毛细管区带电泳用于酶微反应器酶解条件的研究

将氨基酰化酶通过戊二醛固定在毛细管内壁,制备毛细管酶微反应器,用毛细管区带电泳对毛细管酶微反应器的酶解产物进行分离,以生成物的峰面积优化底物N-乙酰-DL-蛋氨酸的酶解条件。实验结果表明,在温度37℃的条件下,10μg/mL N-乙酰-DL-蛋氨酸磷酸盐缓冲溶液(pH7.5)以4μL/min的速度通过15 cm长的毛细管酶微反应器,具有良好的酶解效果。利用毛细管酶微反应器对底物N-乙酰-DL-蛋氨酸进行酶解,每天酶解5次,10天后酶活仅下降了8.66%,说明制备的毛细管酶微反应器具有良好的稳定性。     

Analytical potential of enzyme-coated capillary reactors in capillary zone electrophoresis

Enzymes immobilized on the inner surface of an electrophoretic capillary were used to increase sensitivity and resolution in capillary zone electrophoresis (CZE). Sensitivity is enhanced by inserting a piece of capillary containing the immobilized enzyme into the main capillary, located before the detector, in order to transform the analyte into a product with a higher absorptivity. This approach was used to determine ethanol. In order to improve resolution, capillary pieces containing immobilized enzymes were inserted at various strategic positions along the electrophoretic capillary. On reaching the enzyme, the analyte was converted into a product with a high electrophoretic mobility, the migration time for which was a function of the position of the enzyme reactor. This approach was applied to the separation and determination of acetaldehyde and pyruvate. Finally, the proposed method was validated with the determination of ethanol, acetaldehyde, and pyruvate in beer and wine samples.     

Application of capillary zone electrophoresis with large-volume sample stacking to the sensitive determination of sulfonamides in meat and ground water

A CZE method with UV-Vis detection has been established and validated for the determination of nine sulfonamides: sulfapyridine, sulfamethazine, sulfamerazine, sulfamether, sulfadiazine, sulfadimethoxine, sulfamethoxazole, sulfachlorpyridazine, and sulfamethizole. Optimum separation was obtained on a 64.5 cm x 75 microm bubble cell capillary using a buffer containing 45 mM sodium phosphate and 10% methanol at pH 7.3, with temperature and voltage of 27 degrees C and 25 kV, respectively. p-Aminobenzoic acid was used as an internal standard . Taking into account the lack of sensitivity of the UV-Vis detection, the application of an on-line preconcentration methodology, such as large-volume sample stacking with polarity switching has been proposed. This procedure combined with a solvent extraction/SPE method applied for off-line preconcentration and cleanup provides a significant improvement in the LODs, ranging from 2.59 to 22.95 mug/L for the studied compounds; the quantification of these residues being possible below the levels established by EU legislation in animal food products, such as meat. Satisfactory recoveries were also obtained in the analysis of these compounds in ground water.     

毛细管区带电泳法测定粉针剂中头孢拉定的含量

用毛细管区带电泳法测定头孢拉定的含量 ,未涂层毛细管柱 (75 μm×48.5cm ,有效长度 40cm) ,电压 2 8kV ,检测波长 2 3 0nm ,温度 2 0℃ ,进样 5×1 0 3Pa× 3s。运行缓冲液为 2 5mmol/L硼砂缓冲液。方法的线性范围 3 1 .2 2μg/mL～ 749.2 8μg/mL ,检测限为 1 .1 7μg/mL。     

A technique for capillary joining in capillary electrophoresis

Summary Aspects of cracking and joining capillaries have been investigated. Capillary coupling was achieved using various methods. The most successful used hydrofluoric acid-etched capillaries to form male and female ends which were then joined together. This type of joint was used to connect sections of capillary of similar and different internal diameters with minimal loss in resolution, peak width and number of theoretical plates. (Uridine and hypoxanthine was used as a test mixture). For hypoxanthine on a 50 m/50 m etched joined capillary 10 cm from the detector window the number of theoretical plates was 96.6% of that for hypoxanthine on an unbroken capillary. Following the relative success of capillary joining, a coupled capillary flowcell (50 m/200 m) was produced and evaluated.     

Purity control of oxytetracycline by capillary electrophoresis

The applicability of capillary electrophoresis for the purity control of oxytetracycline (OTC) was investigated. OTC is a broad-spectrum antibiotic belonging to the group of the tetracyclines. Several related substances can be present due to fermentation or degradation, such as 4-epioxytetracycline, -apooxytetracycline, β-apooxytetracycline, anhydrooxytet racycline, 2-acetyl-2-decarboxamidooxytetracycline, tetracycline and 4-epitetracycline. Using fused-silica capillaries, the influence of buffer type, buffer pH and buffer concentration were investigated. In all cases 1 mM EDTA was added to prevent metal-ion complexation. The influence of the buffer counter-ion type was examined. Consequently, some instrumental parameters were changed such as capillary length and diameter as well as capillary temperature and applied voltage. The following method is finally proposed: fused-silica capillary, l (effective length) = 38 cm, L (total length) = 44 cm, 50 μm I.D.; buffer, sodium carbonate 20 mM-EDTA 1 mM, pH 11.25; voltage, 10 kV; temperature, 10°C. Linearity, limit of detection and limit of quantitation were determined as well as the relative standard deviations for all the analytes involved. This method is less selective then existing liquid chromatographic methods but it may be used as a complementary tool in purity control and stability studies.     

Analysis of methylglyoxal in water and biological matrices by capillary zone electrophoresis with diode array detection

We describe a new method for the determination of methylglyoxal in water and biological matrices, using o-phenylenediamine as derivatizing agent and solid-phase extraction followed by capillary zone electrophoresis with diode array detection. 25 mM sodium phosphate running buffers at pH 2.2, 30 kV, and 25 degrees C allowed the best instrumental conditions for the optimum separation of methylglyoxal in a suitable analytical time (< 10 min), using an uncoated fused-silica capillary of 75 microm inner diameter and an effective length of 45.1 cm with an extended light path and the wavelength set to 200 nm. Under optimized instrumental conditions, good reproducibility of the migration time (< 1.1%), precision (< 5%), an excellent linear dynamic range from 0.1 to 3.6 mg/L (r(2) = 0.9997), and low limits of detection (7.2 microg/L) were obtained for methylglyoxal measurements, using the internal standard methodology. Assays on laboratory-spiked tap and ground water samples allowed a remarkable accuracy, presenting yields of 95.0 +/- 4.3 and 94.0 +/- 1.1%, respectively, and good performance to determine methylglyoxal in beer and yeast cells suspensions matrices was also obtained at trace level. The present methodology is a cost-effective alternative for routine quality control analysis, showing to be reliable, sensitive, and with a low sample volume requirement to monitor methylglyoxal in water and biological matrices.     

The determination of chlorophenols in waste water by capillary zone electrophoresis with an organic modifier

Summary Acapillary zone electrophoretic method has been optimized to improve selectivity and resolution in the analysis of chlorophenols in waste water. Use of a buffer system containing organic solvent dramatically improved the separation of chlorophenols. It was shown that selectivity was strongly affected by electrolyte pH and the presence of organic modifiers. The results show that the determination of all seventeen chlorinated derivatives of phenol in water can be achieved by use of a single organic modifier. For example, with acetone as organic modifier all 17 chlorophenols could be separated and determined within 20 min. The standard deviation of migration times and peak areas of the chlorophenols were in the ranges 0.48–0.67% and 3.9–5.1% respectively. Detection linear ranges covered two orders of magnitude of concentration with correlation coefficients of 0.998–1.000, except for 4-chlorophenol. Quantitative aspects of capillary zone electrophoresis are also discussed. It was concluded that capillary zone electrophoresis is a potential method for determination of chlorophenol pollutants in waste water.     

The effect of water on separations in non-aqueous capillary electrophoresis systems

Summary Water, in concentrations up to 10%, has been added to organic solvents (dimethylsulphoxide,N-methylformamide, acetonitrile and methanol) used as the buffer solvents in electrophoresis media for non-aqueous capillary electrophoresis. Anionic and cationic test substances have been used to study the effect on separation selectivity and efficiency. The effect on the electroosmotic flow has also been studied. Water added in concentrations up to 0.5% had only a minor effect on the separation selectivity, efficiency or electroosmotic flow in the systems studied. These results indicate that small variations in the water-content of organic solvents are of only minor importance to the reproducibility of non-aqueous capillary electrophoresis systems. The reproducibility of selectivity might, however, be slightly improved by adding 0.1–0.5% water, because true non-aqueous solvents are likely to cause problems as a result of the variable absorption of water.     

Determination of chlorite in drinking water by on-line coupling of capillary isotachophoresis and capillary zone electrophoresis

An isotachophoresis (ITP)–capillary zone electrophoresis (CZE) combination was used for the determination of chlorite in drinking waters. No sample preparation is needed and no interfering by other anions in tap water was observed. The reached limits of detection with conductivity detector were 0.012–0.017 mg l⁻¹. By four-fold sample loading with a 30 μl valve, 0.005 mg l⁻¹ of chlorite was determined with R.S.D.=3.3%. The concentrations of 0.05 and 0.20 mg l⁻¹ were measured with R.S.D. of 2.2 and 2.7%, respectively. The recoveries of chlorite from drinking water were 96–106% in the range of 0.02–0.20 mg l⁻¹. The R.S.D. values of migration times (inter-day) were up to 1.3%. The time for analysis is about 15 min.     

Separation of organic and inorganic arsenic species by capillary zone electrophoresis

Summary Capillary zone electrophoresis has been used to separate arsenite, arsenate, dimethylarsinic acid, and phenyl-,p-aminophenyl-, ando-aminophenylarsinic acids. Identification and quantification of the arsenic species at mg L⁻¹ levels was possible by use of direct UV detection at 200 nm. The relative standard deviation (n=7) ranged from 0.97 to 1.52% for migration times and from 2.08 to 4.31% for peak areas. A method for rapid separation of inorganic arsenic species was also developed; by use of this method arsenite and arsenate could be separated within 2 min. Presented at Balaton Symposium on High-Performance Separation Methods, Siófok, Hungary, September 1–3, 1999     

Mechanism of sequence-based separation of single-stranded DNA in capillary zone electrophoresis

Separation of DNA by length using CGE is a mature field. Separation of DNA by sequence, in contrast, is a more difficult problem. Existing techniques generally rely upon changes in intrinsic or induced differences in conformation. Previous work in our group showed that sets of ssDNA of the same length differing in sequence by as little as a single base could be separated by CZE using simple buffers at high ionic strength. Here, we explore the basis of the separation using circular dichroism spectroscopy, fluorescence anisotropy, and small angle X-ray scattering. The results reveal sequence-dependent differences among the same length strands, but the trends in the differences are not correlated to the migration order of the strands in the CZE separation. They also indicate that the separation is based on intrinsic differences among the strands that do not change with increasing ionic strength; rather, increasing ionic strength has a greater effect on electroosmotic mobility in the normal direction than on electrophoretic mobility of the strands in the reverse direction. This increases the migration time of the strands in the normal direction, allowing more time for the same-length strands to be teased apart based on very small differences in the intrinsic properties of the strands of different sequence. Regression analysis was used to model the intrinsic differences among DNA strands in order to gain insight into the relationship between mobility and sequence that underlies the separation.     

Determination of egg white lysozyme by on-line coupled capillary isotachophoresis with capillary zone electrophoresis

An on-line coupled capillary isotachophoresis - capillary zone electrophoresis method for the determination of lysozyme in selected food products is described. The optimized electrolyte system consisted of 10 mM NH(4)OH + 20 mM acetic acid (leading electrolyte), 5 mM epsilon -aminocaproic acid +5 mM acetic acid (terminating electrolyte), and 20 mM epsilon -aminocaproic acid +5 mM acetic acid +0.1% m/v hydroxypropylmethylcellulose (background electrolyte). A clear separation of lysozyme from other components of acidic sample extract was achieved within 15 min. Method characteristics, i.e., linearity (0-50 micrograms/mL), accuracy (recovery 96+/-5%), intra-assay (3.8%), quantification limit (1 microgram/ml), and detection limit (0.25 microgram/mL) were determined. Low laboriousness, sufficient sensitivity and low running costs are important attributes of this method. The developed method is suitable for the quantification of the egg content in egg pasta.     

Enantioseparation and quality control of biperiden in pharmaceutical formulations by capillary electrophoresis

An original capillary electrophoretic method has been developed and applied for the enantioselective analysis of the antiparkinson drug biperiden in pharmaceutical formulations, using a modified cyclodextrin as the chiral selector. Baseline enantioseparation of the racemic compound was achieved in less than 7 min using an uncoated fused silica capillary (50 μm i.d. and 48.5, 40.0 cm, total and effective length, respectively), filled with a background electrolyte consisting of a 50 mM phosphate buffer at pH 3.5 supplemented with 3% (w/v) β-cyclodextrin sulphate and applying a voltage of 20 kV, reversed polarity. Samples were injected by pressure (50 mbar, 90 s) at the cathodic end of the capillary and detection wavelength was 195 nm (bandwidth: 10 nm). A simple and fast pre-treatment procedure allowed the complete extraction of the drug from commercial formulations (sustained release tablets and ampoules for injections) without any interference from the matrix. Good linearity was found in the 1–50 μg/mL concentration range; the limit of quantitation was 1 μg/mL and the limit of detection was 0.4 μg/mL. Precision and accuracy were good, with R.S.D. values always lower than 2.8% and a mean recovery value of 101.1%. The method was suitable for the quality control of biperiden in commercial formulations.     

An automatic sampling device for capillary zone electrophoresis

An automatic sampling device has been developed for capillary zone electrophoresis. The sample is introduced to the column electrokinetically by rapidly exchanging buffer for sample in a narrow channel drilled in a plexiglass block. The autosampler is capable, under computer control, of performing multiple sample injections from a large volume sample source (such as a reaction vessel) as the sample concentration changes, and thus presents the possibility of analyzing time-varying processes by CZE. Peak area reproducibility in electropherograms obtained after use of the sampler is less than 1% and efficiency is more than 2.2 × 10⁵ theoretical plates.     

高效毛细管区带电泳法快速测定尿液中的肌酐

建立了一种快速测定尿中肌酐浓度的高效毛细管电泳方法。利用非涂层石英毛细管(64.5 cm×50μm i.d),以pH 2.5,0.1 mmol/L H3PO4作为电泳缓冲液,检测波长191 nm,用0.05 Pa压力进样4 s,在电压16 kV快速分离尿液中的肌酐,采用外标法定量。肌酐的迁移时间约为5.5 min,肌酐浓度在34.5~8840μmol/L范围内呈良好的线性(r2=0.999)。平均日内精密度为2.5%,日间精密度为3.0%。回收率94.1%~99.0%。与全自动生化分析仪碱性苦味酸速率法相比有良好的相关性(r=0.990,n=56)。高效毛细管电泳法测定尿肌酐可应用于临床样品的检测。     

Rapid capillary zone electrophoresis method for the determination of metal cations in beverages

A rapid and reliable capillary zone electrophoresis method for the determination of inorganic cations was developed. The complete separation of K⁺, Ba²⁺, Ca²⁺, Na⁺, Mg²⁺, Mn²⁺, Ni²⁺, Cd²⁺, Li⁺ and Cu²⁺ can be achieved in 4 min with a simple electrolyte composed by 10 mM imidazole as the carrier buffer and background absorbance provider and acetic acid as the complexing agent (pH 3.60). Injection was performed hydrostatically by elevating the sample at 10 cm for 30 s. The running voltage was +25 kV at room temperature. Indirect UV-absorption detection was achieved at 185 nm. The detection limit was in the range between 0.06 mg/l (Mg²⁺) and 0.57 mg/l (K⁺) and the quantification limits ranged from 0.10 mg/l (Ni²⁺) to 0.80 mg/l (Cu²⁺). The calibration graphs were linear in the concentration range from the quantification limit till at least 1 g/l in K⁺, 10 mg/l in Ba²⁺, Ca²⁺, Mg²⁺, Mn²⁺, Ni²⁺ and Cd²⁺, 40 mg/l in Na⁺ and 12 mg/l in Li⁺ and Cu²⁺. The repeatability, intraday and interday analysis were ≤1.55% and ≤3.64% for migration time and ≤3.38% and ≤3.63% for peak area. The method developed has been applied to several beverage samples with only a simple dilution and filtration treatment of the sample. The proposed method is simple, fast, cheap and it is achieved with common products in either laboratory. For these reasons, it is a very useful method for routine analysis.