Separation and determination of some stereoisomers by capillary gel electrophoresis with cyclodextrin incorporated in polyacrylamide gel

Capillary gel electrophoresis (CGE) was successfully applied to the separation of optically active isomers and position isomers by incorporating a suitable cyclodextrin chiral selector in polyacrylamide gel. A commercially available ss-cyclodextrin (ss-CD) was used for enantioselectivity towards o-, m- and p-nitrobenzoic acid, o-, m- and p-hydroxybenzoic acid, o-, m- and p-toluic acid and the optical isomers of dansyl-D,L-leucine and R,S-1,1'-binaphthyl-2,2-dihydrogenphosphate. Especially the effect of organic solvents, such as acetonitrile, methanol, dimethylsulphoxide and others were examined in detail. The resolution varied to some extent with the addition of the organic solvent to the polyacrylamide gel and the running buffer solution. The possible mechanism has also been discussed. In addition, quantitative aspects of the separation of stereoisomers using CGE have been studied, showing that both the resolution and accuracy of the determinations were affected by the ratio of the enantiomers.     

Thin-layer chromatography of dihydric phenols

Summary Phenol, resorcinol, catechol, and hydroquinone were separated on thin layers of silica gel impregnated with silver nitrate. The incorporation of silver nitrate in the adsorbent layer results in the oxidation of ortho and para dihydric phenols to the corresponding benzoquinones, meta dihydric phenols are not changed, hence the separation of the dihydric isomers is possible.

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Zusammenfassung Phenol, o-, m- und p-Dihydroxybenzole werden auf mit Silbernitrat imprägnierten Kieselgel-Dünnschichtplatten aufgetrennt. Diese Trennung wird dadurch möglich, daß in Anwesenheit von Silbernitrat o- und p-Dihydroxybenzole zu den entsprechenden Benzochinonen oxydiert werden, bei m-Dihydroxybenzol diese Oxydation jedoch nicht eintritt.

     

High-performance liquid chromatography utilization of ionic liquids as mobile phase additives for separation and determination of the isomers of amino benzoic acids

For the isomers of amino benzoic acid, including o-, m-, p-amino benzoic acid, the beneficial effects of using the ionic liquid, 1-butyl-3-methylimidazolium tetrafluoroborate ([BMIm][BF₄]), as mobile phase additives on retention behavior and separation were investigated. Chromatographic separation of the o-, m-, p-amino benzoic acid was performed on a reversed-phase C18 column by ultraviolet detection at 245 nm. The effects of several chromatographic parameters, concentrations and pH values of [BMIm][BF₄] solutions, methanol concentration and length of alkyl chain on different ionic liquids, on the separation and determination of the isomers were evaluated. The optimized chromatographic conditions were established using an aqueous 0.5 μmol/L [BMIm][BF₄] solution (pH 3.0)/methanol (40:60, v/v) as mobile phase without need of gradient elution, with separation of three amino benzoic acids achieved within four min. The calibration curve showed good linearity over the tested range of 2 mg/L to 120 mg/L for the three isomers with a correlation coefficients of 0.9999. The recoveries of the three amino benzoic acids of spiked components were between 99.8% and 100%. The method has been successfully applied to the determination of p-amino benzoic acid in the pharmaceutical, Bromine Mitag Procaine Injection.     

Classification of olive leaves and pulps according to their cultivar by using protein profiles established by capillary gel electrophoresis

A method to classify olive leaves and pulps according to their cultivar using protein profiles obtained by capillary gel electrophoresis (CGE) has been developed. For this purpose, proteins were extracted using an enzyme-assisted method, which provided higher protein recoveries than other previously described methods. Ten and nine common peaks, for leaf and pulp samples, respectively, were identified in the 12 cultivars studied in this work. In addition, and using linear discriminant analysis of the CGE data, olive leaf and pulp samples belonging to 12 cultivars from different Spanish regions were correctly classified with an excellent resolution among all the categories, which demonstrated that protein profiles were characteristic of each cultivar.

Simultaneous determination of positional isomers of benzenediols by capillary zone electrophoresis with square wave amperometric detection

A capillary zone electrophoresis method coupling square wave amperometric detection (SWAD) for the simultaneous determination of positional isomers of benzendiols (i.e. o-, m-, p-benzenediols) has been developed. Effects of several factors, such as the composition of the running buffer, the pH value, separation voltage, injection time and the potential applied to the working electrode, were investigated to acquire the optimum conditions. The efficacy of the boric acid and ascorbic acid in the running buffer were discussed. o-, m-, p-Benzendiols can be well separated within 8 min in a 50 cm length of 50 microm diameter fused-silica capillary at a separation voltage of +15 kV. Operated in a wall-jet configuration, a 100 microm Pt-disk electrode used as the working electrode exhibits good response for the analytes. The relation between peak current and analyte concentration was linear over two orders of magnitude with detection limits (S/N = 3) ranging from 0.5 to 1.5 microM for all analytes. The proposed method has been successfully applied to monitor the o-, m-, p-benzendiols contents in the environmental wastewater samples with satisfactory assay results.     

Colour changes in the uncatalyzed and Ag+ catalyzed oxidation of aromatic amines by persulphate ion

Summary A scheme has been proposed for the identification of some of the aromatic amines, viz., aniline, ethyl and methyl aniline, diethyl and dimethyl aniline, - and -naphthylamine, o-, m- and p-toluidine, o-, m- and p-anisidine, m- and p-phenetidine, o-, m- and p-phenylenediamine, carbazole, benzidine, o-tolidine, quinoline and iso-quinoline, p-xylidine and diphenylamine. It is based on the reaction of an aqueous persulphate solution with an alcoholic solution of the amine.

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Zusammenfassung Eine systematische Identifizierung einiger aromatischer Amine aufgrund der Oxydation mit Persulfatlösung wird beschrieben. Folgende Verbindungen werden dabei berücksichtigt: Anilin, Äthyl- und Methylanilin, Diäthyl- und Dimethylanilin, - und -Naphthylamin, o-, m- und p-Toluidin, o-, m- und p-Anisidin, m- und p-Phenetidin, o-, m- und p-Phenylendiamin, Carbazol, Benzidin, o-Tolidin, Chinolin und Isochinolin, p-Xylidin und Diphenylamin.

     

基于环糊精功能化介孔材料制备高选择性化学修饰电极

合成了SBA-15有序多孔氧化硅材料并用β-CD对其进行了修饰,制备了功能化介孔修饰碳糊电极（CD-SBA15/CPE）,利用循环伏安法（CV）、示差脉冲伏安法（DPV）等电化学技术,研究了修饰电极对硝基苯酚、硝基氯苯、苯二酚异构体的识别机理。研究表明：该修饰电极不仅能识别o-、m-、p-硝基苯酚、o-、p-硝基氯苯、o-、p-苯二酚异构体,且具有分辨率高、测定灵敏度高的特点。可望用于实际样品中同分异构体快速、灵敏和选择性检测。     

Highly efficient size separation of CdTe quantum dots by capillary gel electrophoresis using polymer solution as sieving medium

In this paper, we present a new method for highly efficient size separation of water-soluble CdTe quantum dots (QDs) based on CGE using polymer solution as sieving medium. CdTe QDs were synthesized in aqueous phase by a chemical route with mercaptopropionic acid as a ligand. In the alkaline solution, CdTe QDs possess negative charges and migrate to the anode in the electric field. In linear polyacrylamide sieving medium, the migration time of CdTe QDs was increased with the size of CdTe QDs. The effects of some factors, such as types, concentrations, and pH of sieving media, on the separation of CdTe QDs were investigated systematically. Highly efficient separation of CdTe QDs was obtained in linear polyacrylamide sieving medium, and collection of fractions was automatically accomplished by CGE technique. Our preliminary results show that CGE technique is an efficient tool for characterization and size-dependent separation of water-soluble nanoparticles. In addition, the fraction collection in CGE may be useful in certain special applications such as fabrication of nanodevices in the future.     

Polyacrylamide gel plugs enabling 2-D microfluidic protein separations via isoelectric focusing and multiplexed sodium dodecyl sulfate gel electrophoresis

In situ photopolymerized polyacrylamide (PAAm) gel plugs are used as hydrodynamic flow control elements in a multidimensional microfluidic system combining IEF and parallel SDS gel electrophoresis for protein separations. The PAAm gel plugs offer a simple method to reduce undesirable bulk flow and limit reagent/sample crosstalk without placing unwanted constraints on the selection of separation media, and without hindering electrokinetic ion migration in the complex microchannel network. In addition to improving separation reproducibility, the discrete gel plugs integrated into critical regions of the chip enable the use of a simple pressure-driven sample injection method which avoids electrokinetic injection bias. The gel plugs also serve to greatly simplify operation of the spatially multiplexed system by eliminating the need for complex external fluidic interfaces. Using an FITC-labeled Escherichia coli cell lysate as a model system, the use of gel plugs is shown to significantly enhance separation reproducibility in a chip containing five parallel CGE channels, with an average variance in peak elution time of only 4.1%.     

A platform method for plasmid isoforms analysis by capillary gel electrophoresis

In the production of novel biological products, plasmids are often engineered into delivery vectors for target genes, which can be used directly as vaccines or as intermediate products for gene/cell therapy. Plasmid DNA exists in several topological forms such as supercoiled, linear, and open circular. As supercoiled plasmid shows the highest efficiency in transfecting eukaryotic cells, the content of supercoiled plasmids becomes an important indicator of plasmid quality. CGE is an effective analysis method for separating different topological structures of plasmids. For the purpose of providing plasmid manufacturers and regulatory agencies with an efficient and readily used tool for monitoring the quality of plasmids, this article identifies the optimal separation and detection conditions of CGE, presents a platform-based plasmid analytical method, and uses plasmid of different sizes to verify the feasibility of this method. In terms of detector, the LIF detector has obvious advantages over the ultraviolet detector in sensitivity and resolution. Using the optimal CE condition (10× gel buffer), baseline separation of different topological forms and impurities can be achieved for different plasmid sizes (5.9, 7.8, 15.4 kb). In addition, 6.5 kb plasmid was used to compare the different separation technologies such as CGE-LIF, ion exchange chromatography and agarose gel electrophoresis. The result shows that CGE-LIF can provide better resolution and quantitation accuracy than ion exchange chromatography and agarose gel electrophoresis. CGE-LIF, as a quick and convenient method to separate and quantify plasmids, has the advantages of high sensitivity, high resolution, and high quantitative accuracy. Therefore, it is ideal for analysis of plasmids with different sizes, and it can also be used as a platform method for manufacturers and regulatory agencies to monitor the purity and stability of plasmids.     

Capillary gel electrophoresis of oligonucleotides using polymer solutions

Summary Capillary gel electrophoresis (CGE) has been recognized as an effective method for the analysis of oligonucleotides. CGE using polymer solutions is especially useful and effective compared with that using crosslinked gels, because of easy change of media. Replacement of media leads to the reproducible separation of analytes. We have investigated CGE analysis of oligonucleotides of less than 20 bases employing various kinds of polymers. Polyacrylamide, dextrin, dextran, pullakin, and poly(ethylene glycol) were used as sieving matrixes at concentrations of 0–30 %. Polydeoxythymidylic acids [p(dT)_11–20] were used as a test sample. These small oligonucleotides were successfully resolved on the basis of their base number by CGE using some of these polymer solutions. In particular, dextran was found to be effective and baseline separation was observed when a 30 % dextran solution was employed. Some validations such as linearity and reproducibility were also established and this method was found to be an adequate quality control method for small oligonucleotides. Finally, CGE using a 30 % dextran solution was successfully applied to impurity profiling of some synthetic oligonucleotides.     

基于L-谷氨酸的手性硅胶球的制备及其应用

无机介孔硅球因其具有足够的机械强度、热稳定性,以及适应多种流动相的优点,成为高效液相色谱(HPLC)柱填料中使用最广泛和最重要的材料。但在此研究领域中,并未见球形的全无机手性硅胶用作HPLC手性固定相。该文以无机球形介孔硅胶作为研究对象,通过堆砌硅珠法,以硅溶胶为原料,L-谷氨酸(L-Glu)为手性源,在手性环境中制造出脲醛树脂与胶体二氧化硅混合的小球,在550 ℃高温下煅烧除去树脂部分,制备基于L-Glu的无机介孔硅胶球。通过元素分析、红外光谱、扫描电镜、透射电镜和氮气吸附等表征证明这是一种具有规则球形的手性硅胶球,其手性来源于硅胶球自身的骨架和孔结构。将L-Glu手性硅胶球作为固定相制备了HPLC色谱柱,以正己烷-异丙醇(9∶1, v/v)作为流动相,流速为0.1 mL/min,考察了该手性柱对一系列外消旋化合物的拆分性能。实验表明,该手性柱拆分了15种外消旋化合物,其中特罗格尔碱、吡喹酮、3-苄氧基-1,2-丙二醇、1,2-环氧己烷、3-羟基-2-丁酮、2-甲基四氢呋喃-3-酮、异丙基缩水甘油醚达到基线分离;还分离了10种苯系位置异构体,o,m,p-氨基苯酚、o,p-氯苯酚、o,m,p-碘苯胺、o,m,p-甲苯胺、o,m,p-二硝基苯、o,m,p-氯苯胺、o,m,p-硝基苯酚、o,m,p-溴苯胺达到基线分离。实验表明,L-Glu手性硅胶球在手性分离方面具有良好的可行性,与普通硅胶相比不需要进一步修饰就可以有较好的手性分离效果,是一种低成本、制备便捷的手性无机硅胶固定相。     

Proton conducting polymer gel electrolytes with NO2 substituted carboxylic acids

Proton conducting polymer gel electrolytes based on different nitro substituted aromatic carboxylic acids have been studied. The conductivity of solution and gel electrolytes containing these acids has been found to depend upon the dissociation/acidity constant value of the acid and varies as  > σ (meta-). The addition of polymethylmethacrylate (PMMA) modifies the conductivity of these gel electrolytes which depends upon the dissociation constant and concentration of the acid present. The rate of change of conductivity of gel electrolytes with gelling polymer (PMMA) has been found to be different in the low and high PMMA regions which has been explained to be due to different mechanisms being responsible for the modification of conductivity in the low and high PMMA regions.     

Graphitic carbon nitride embedded hydrogels for enhanced gel electrophoresis

Here, we show, for the first time, the use of graphitic carbon nitride (g-C₃N₄) nanosheets to improve the resolution and efficiency of protein separation in gel electrophoresis. By loading 0.04% (m/v) g-C₃N₄ nanosheets into the polyacrylamide gel at 25 °C, the thermal conductivity increased approximately 80% which resulted in 20% reduction in Joule heating and overall increase of separation efficiency. Also, polymerization of acrylamide occurred in the absence of tetramethylethylenediamine (TEMED) when the polyacrylamide gel contained g-C₃N₄ nanosheets. Hence, the g-C₃N₄ act simultaneously as a polymerization catalyst as well as heat sinks to lower Joule heating effect on band broadening.     

High-performance liquid chromatographic resolution of enantiomers on chiral amine-bonded silica gel

Summary A chiral stationary phase with an immobilized, optically active diamine was prepared for the separation of enantiomers. The synthesis of the phase was carried out by bonding (–)trans-1,2-cyclohexanediamine to microparticulate silica gel through the coupling agent 3-glycidoxypropylsilane. The resolution of the racemic compounds catechin, 2,2-dihydroxy-1,1binaphthyl and trans-1,2-cyclohexandiol, is reported.     

Reversed phase partition chromatographic separation of divalent copper with N-n-octylaniline on silica gel

A novel separation method was developed for the extraction and chromatographic separation of copper(II). The quantative extraction of 25.0–125.0 μg copper(II) has been observed from 0.05 to 0.25 mol/L of ascorbic acid at pH 9.0–12.0 with 0.087 mol/L N-n-octylaniline (liquid anion exchanger) coated on silica gel at a flow rate of 1.0 ml/min. The extracted metal ion has been recovered by eluting with 25.0 ml of 1.0 mol/L hydrochloric acid and determined spectrophotometrically by rubeanic acid method. The various influencing parameters viz. acid concentrations, reagent concentration, eluates effect of pH, and effect of flow rate on extraction were studied. The method is free from large number of interferences from cations and anions. A scheme for mutual separation of copper(II), gold(III) and bismuth(III) has been developed. Copper(II) has been separated from ayurvedic (Herbal) medicine and synthetic mixtures corresponding to alloy. The log–log plot of N-n-octylaniline concentration versus the distribution coefficient indicates that the probable extracted species is [.     

Inspection of the reversal of enantiomer migration order in ligand exchange micellar electrokinetic capillary chromatography

Enantiometers of D,L-phenylalanine were separated by capillary electrophoresis based on the principle of ligand exchange. Copper (II) complex of 4-hydroxy-L-proline was used as chiral selector. The separation and the migration order of D- and L-phenylalanine were strongly affected by adding an anion surfactant sodium dodecylsulfate (SDS). Without SDS in the electrolyte, the separation was also carried out but the resolution was very small. With SDS added into the electrolyte, the resolution decreased with increasing concentration of SDS until 5.0 mM. When the concentration of SDS in the electrolyte was over 5.0 mM, inversion of the migration order of DL-phenylalanine was observed and the resolution was also increased with increasing concentration up to 20 mM. It was interesting to find that the inversion of the migration order took place not only in the enantioscparation but also in the positional isomers. A family of a fluorinated amino acid, o-, m- and p-fluoro-D,L-phenylalanine was separated and the inversion of the migration order is discussed.     

Guanosine gel for sequence-dependent separation of polymorphic ssDNA

The separation of fluorescent-labeled ssDNA fragments of equal length based on differences in sequence was achieved through the use of guanosine gels (G-gels) formed by guanosine-5'-monophosphate (GMP) in capillary gel electrokinetic chromatography (CGEKC) with LIF detection. Baseline resolution was achieved for homodimers and homopentamers of A, T, and C. G-gel CGEKC provided better resolution than CZE, MEKC, or a sieving gel in CGE. Resolution improved with increasing GMP, indicating that the interaction is linked to structural organization of the G-gel. Fluorescence intensity and anisotropy show that the order of interaction with G-gels is T>C>A. We then investigated four conformationally similar, polymorphic 76-mers with A/G substitutions that are utilized in forensic DNA typing. Resolution was achieved by CGEKC but not CZE or CGE. In CGEKC, the negatively charged G-gels and oligonucleotides electromigrate toward the positive inlet while being driven by EOF to the negative outlet. The net forward velocity is the greatest for oligonucleotides most closely associated with the slower, more cumbersome G-gel network. For the 76-mers, resolution increases with increasing difference in guanosine content between strands and, for a given difference, with increasing total guanosines in the strands.     

Simultaneous determination of dihydroxybenzene positional isomers by capillary electrochromatography using gold nanoparticles as stationary phase

The paper describes the enhanced separation of o-, m-, p-dihydroxybenzene by capillary electrochromatography (CEC) using gold nanoparticles (AuNPs) as stationary phase. The effect of the AuNPs concentration upon separation was investigated. The experimental parameters, including separation voltage, pH, and concentration of running buffer, were optimized. Under the optimum conditions, a good resolution of three dihydroxybenzene isomers was obtained within 15 min in a 50 cm effective length capillary modified with 0.02 nmol/L AuNPs at a separation voltage of 16 kV in a 50 mmol/L acetate buffer (pH 5.0). The linear ranges were from 10(-6) to 10(-4) mol/L and the detection limits were as low as 10(-7) mol/L. This method was successfully used to analysis two kinds of hair coloring agent sample with recoveries in the range of 90-105% and relative standard deviations (RSD) less than 5.0%.