Trace analysis of N-formylmorpholine in hydrocarbons and water by gas-liquid chromatography

Summary N-Formylmorpholine, which is a solvent used in the extraction of benzene, toluene and xylenes extraction from petroleum feedstocks, is determined in trace amounts in water and in aromatic hydrocarbons by gas-liquid chromatography using two stationary phases. Traces of N-formylmorpholine in hydrocarbons was determined on a column packed with 2.3% Bentone 34+4.6% DEGA on Chromosorb W AW treated with 1% KOH. Traces of N-formylmorpholine in water was determined on 20% SE-30 on Chromosorb W AW. The developed methods were examined and proved to give quantitative results.     

Trennung von Organophosphor-Pestiziden und ihren Metaboliten auf Glaskapillarsäulen

Zusammenfassung Organophosphor-Pestizide wurden als Rückstände in pflanzlichen Lebensmitteln an einer 25 m langen Dünnfilm-Glaskapillare mit DEGA getrennt. Die gute Trennleistung der Kapillare, die sich auch an Gemischen von Metaboliten und Isomeren zeigte, emöglichte in Verbindung mit einem phosphor-spezifischen, thermionischen Detektor die sichere Identifizierung der Rückstände bis zu 0,05 mg/kg.

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Separation of organophosphorus pesticides and their metabolites by glass-capillary gas chromatography

Summary Organophosphorus pesticide residues in plant material were separated by means of an open tubular column (25 m length) coated with DEGA. High separation performance was obtained even for metabolites and isomers. Residues could be safely identified down to 0.05 mg/kg with alkali flame thermionic detection.

     

Thermoresponsive Copolymers of Ethylene Oxide and N,N‐Diethyl Glycidyl Amine: Polyether Polyelectrolytes and PEGylated Gold Nanoparticle Formation

The synthesis of diblock as well as gradient copolymers of N,N‐diethyl glycidyl amine (DEGA) with ethylene oxide (EO) via anionic ring‐opening polymerization is presented. The polymers exhibit low polydispersities (≤1.13) and molecular weights in the range of 3300–10 200 g mol⁻¹. In PEG‐co‐PDEGA copolymers, incorporation of 4%–29% DEGA results in tailorable cloud point temperatures in aqueous solution and melting points depending on DEGA content. mPEG‐b‐PDEGA block copolymers can be quaternized to generate cationic double‐hydrophilic polyelectrolyte copolymers with polyether backbone. Furthermore, mPEG‐b‐PDEGA has been used as dual reducing and capping agent for gold nanoparticle synthesis.     

Fatty acids. IV. Synthesis of all the dimethylene-interrupted methyl octadecadiynoates and a study of their gas-liquid chromatographic properties.

All the dimethylene-interrupted methyl octadecadiynoates have been synthesised and the gas-liquid chromatographic behaviour of these isomers was studied on polar [Carbowax 20M, FFAP, DEGA, DEGS and Silar 10C (recently renamed as Apolar 10C)], semi-polar (XE-60) and non-polar (SE-30, OV-101 and Apiezon L) stationary phases. The possibility of identification and separation of these isomers is discussed. The delta3a,7a isomer was found to decompose on most polar phases and the delta2a,6a isomer could not be eluted from the Carbowax 20M phase.     

Exploiting styrene-maleic acid copolymer grafting chromatographic stationary phase materials for separation of membrane lipids

High performance liquid chromatography-mass spectrometry is one of the most commonly used strategies for lipid analysis. The development of versatile chromatographic stationary phases to meet the increasing demands for separation of complex lipids is very important. Styrene-maleic acid(SMA) copolymer is an amphiphilic polymer, which has been proven to have the ability to solubilize lipid molecules of various structures. In this study, styrene-maleic anhydride copolymer coated silica was first pr...     

Preparation and characterization of mixed-mode monolithic silica column for capillary electrochromatography

A silica-based monolithic stationary phase with mixed-mode of reversed phase (RP) and weak anion-exchange (WAX) for capillary electrochromatography (CEC) has been prepared. The mixed-mode monolithic silica column was prepared using the sol–gel technique and followed by a post-modification with hexadecyltrimethoxysilane (HDTMS) and aminopropyltrimethoxysilane (APTMS). The amino groups on the surface of the stationary phase were used to generate a substantial anodic EOF as well as to provide electrostatic interaction sites for charged compounds at low pH. A cathodic EOF was observed at pH above 7.3 due to the full ionization of residual silanol groups and the suppression in the ionization of amino groups. A variety of analytes were used to evaluate the electrochromatographic characterization and column performance. The monolithic stationary phase exhibited RP chromatographic behavior toward neutral solutes. The model anionic solutes were separated by the mixed-mode mechanism, which comprised RP interaction, WAX, and electrophoresis. Symmetrical peaks can be obtained for basic solutes because positively charged amino groups can effectively minimize the adsorption of positively charged analytes to the stationary phase.     

Factors influencing the synthesis and the post-modification of PEGylated pentafluorophenyl acrylate containing copolymers

Copolymerization reactions involving oligoethylene glycol acrylate (OEGA) or diethylene glycol acrylate (DEGA) with pentafluorophenyl acrylate (PFPA) have been performed by reversible addition fragmentation transfer (RAFT) polymerization. The effect of the reaction conditions on the nucleophilic acyl substitution reactions of PFPA was studied using a model amine (furfuryl amine). The resulting PEG/PFP functional copolymers were then used as scaffolds to produce a library of polymers by reaction with a range of amines.     

Liquid chromatographic resolution of gemifloxacin mesylate on a chiral stationary phase derived from crown ether

A new racemic fluoroquinolone antibacterial agent, gemifloxacin mesylate, has been successfully resolved on a chiral stationary phase (CSP) derived from (+)-(18-crown-6)-2,3,11,12-tetracarboxylic acid. Compared to the Crownpak CR(+) column, the CSP used in this study was more effective for the resolution of racemic gemifloxacin mesylate, especially in terms of analytical time. The resolution of gemifloxacin mesylate enantiomers on the CSP was found to be dependent on the type and content of organic and acidic modifiers in the aqueous mobile phase and the column temperature.     

The influence of water on the memory effect of the amylose tris(3,5-dimethylphenyl carbamate) stationary phase

Acid/base modifiers are sometimes used as additives in normal phase elution on columns packed with CHIRALPAK^® AD^®. These modifiers affect enantioseparations in ways that are not yet fully understood for the lack of systematic studies. Shifts of the selectivity of certain pairs of enantiomers upon exposure of the column to these modifiers is amply documented. Furthermore, once the modifier has been removed from the mobile phase, the modified selectivity remains, which has been named the Memory Effect. After a column has been exposed to an eluent stream containing acidic/basic modifiers, this particular column no longer separates certain enantiomeric pairs with the same selectivity as a modifier naive column. This makes the transfer of developed methods from one to other CHIRALPAK AD columns difficult to predict, if the selectivity needs to be similar between the two columns. We selected four enantiomeric pairs for a systematic study of this Memory Effect. The selectivity of 4-chlorophenylalanine ethyl ester improves after a solution of ethanesulfonic acid (ESA) is percolated through the column. The selectivity of Propranolol and Tröger's base increases after a solution of Diiospropylamine is percolated through the column. The selectivity of Propranolol and Tröger's base enantiomers is inversely affected by percolation of the acid solution. The 4-chlorophenylalanine ethyl ester enantiomers is inversely affected by percolation of the base solution. In contrast, the selectivity of trans-stilbene oxide (TSO) is not affected by either modifier. Analytical studies of the stationary phase suggest that slow protonation/deprotonation of water molecules attached to the carbamate moiety may be responsible for the acid/base Memory Effect. To further the understanding of the effect of water on the Memory Effect, mobile phases – spiked with water (0.01–0.43%) – were used to measure changes in the Memory Effect. Finally, we showed that the influence of water on the Memory Effect can be minimized by percolating through the column a sufficiently concentrated solution of the appropriate base while using dried mobile phases.     

Temperature optimization for the separation of PAHs on micropacked LC ODS columns

The effect of column temperature on the separation of the sixteen polycyclic aromatic hydrocarbons (PAHs) of mixture SRM 1647a of the US Environmental Protection Agency has been studied on different micropacked ODS columns. Isothermal temperature optimization was successfully used for complete separation of the PAHs on a polymeric ODS stationary phase, whereas temperature programmed conditions were selected for separation on a monomeric ODS stationary phase.     

Separation of the stereoisomers of racemic fluoroquinolone antibacterial agents on a crown-ether-based chiral HPLC stationary phase

Summary A chiral stationary phase derived from (+)-(18-crown-6)-2,3,11,12-tetracarboxylic acid has been successfully used for the direct separation of the enantiomers of recemic fluoroquinolines containing a primary amino group being investigated as antibacterial agents. The chromatographic resolution behavior was found to depend on the content and the type of acidic and organic modifiers in the mobile phase and on the column temperature.     

A new type of two-dimensional packed + capillary column GC system. II. System and applications

Summary A packed column containing immobilized SE-54 liquid phase on pellicular silica beads ZIPAX and having a high efficiency and high mass transfer rate has been successfully used in a two-dimensional packed+capillary column system without a cold trap. The application of this system is demonstrated by the analysis of C₆-C₈ aromatic hydrocarbons and lowboiling hydrocarbons present in natural oils, and of highboiling components present in low concentrations in a low-boiling solvent.     

Preparation of monolithic silica column with strong cation-exchange stationary phase for capillary electrochromatography

A monolithic silica based strong cation-exchange stationary phase was successfully prepared for capillary electrochromatography. The monolithic silica matrix from a sol-gel process was chemically modified by treatment with 3-mercaptopropyltrimethoxysilane followed by a chemical oxidation procedure to produce the desired function. The strong cation-exchange stationary phase was characterized by its substantial and stable electroosmotic flow (EOF), and it was observed that the EOF value of the prepared column remained almost unchanged at different buffer pH values and slowly decreased with increasing phosphate concentration in the mobile phase. The monolithic silica column with strong cation-exchange stationary phase has been successfully employed in the electrochromatographic separation of beta-blockers and alkaloids extracted from traditional Chinese medicines (TCMs). The column efficiencies for the tested beta-blockers varied from 210,000 to 340,000 plates/m. A peak compression effect was observed for atenolol with the mobile phase having a low phosphate concentration.     

The preparation of glass SCOT columns by the organic glue method

A technique for adhesion of fine particles (ca. 5 μ) of the 405 white diatomaceous support on the inner wall of glass tube with organic glue [poly (diethylaminoethyl methacrylate) acetate] is described. The coated tube was drawn to capillary column by using a machine designed according to Desty's. The capillary column was then coated with stationary phase (such as squaiane, QF-1, Dexsil 300, PEG 20 M, OV-1, SE 30 and etc.) by the conventional dynamic or static method. This preparation method has proved easy to duplicate and is simple. The coating efficiency (UTE %) is within 60–90. The theoretical plate number per meter of an SE 30 column is about 4000, and per meter of a PEG 20 M column is about 2500. The columns thus prepared have been successfully used to analyze petroleum hydrocarbons, essential oils, petrochemicals, pheromone, steroid metabolites and others.     

Temperature programmed retention indices: Calculation from isothermal data. Part 2: Results with nonpolar columns

The procedure for calculating linear temperature programmed indices as described in part 1 has been evaluated using five different nonpolar columns, with OV-1 as the stationary phase. For fourty-three different solutes covering five different classes of components, including n-alkanes and alkyl-aromatic compounds, both isothermal and temperature programmed indices were determined. The isothermal information was used to calculate temperature programmed indices. For several linear programmed conditions accuracies better than 0.51^T-units were usually obtained. The results are compared with published procedures. It is demonstrated that isothermal retention information obtained on one column can be transferred to another column with the same stationary phase but different column dimensions and/or phase ratio. The temperature programmed indices calculated in this way also have an accuracy better than 0.51^T-u. The temperature accuracy and precision of the GC-instrumentation used was of the order of 0.1°C. All calculations can be run with a Basic-programmed microcomputer.     

Phenylboronic acid modified solid‐phase extraction column: Preparation,characterization, and application to the analysis of amino acids in sepia capsule by removing the maltose

Maltose, a common auxiliary material of pharmaceutical preparation, may disturb the analysis of total amino acids in sepia capsule by aldolization. Therefore, it is necessary to remove the maltose through a convenient method. In this work, a phenylboronic acid modified solid‐phase extraction column has been synthesized and used to remove the maltose. The materials were synthesized by one step “thiol‐ene” reaction and the parameters of the column such as absorption capacity, recovery, and absorption specificity have been investigated. The results showed the column (0.5 cm of length × 0.5 cm of inner diameter) can absorb 4.6 mg maltose with a linear absorption and absorption specificity. Then this technique was applied in the quantification of amino acids in sepia capsule. After the optimization of the method, four kinds of amino acids, which were the most abundant, were quantified by high‐performance liquid chromatography with diode array detection. The amounts of the four kinds of amino acids are 1.5～2 times more than that without the treatment of solid‐phase extraction column, which almost overcomes the influence of the maltose. All the results indicate that the phenylboronic acid modified solid‐phase extraction column can successfully help to accurately quantify the total amino acids in sepia capsule.     

Siliceous mesocellular foam for high-performance liquid chromatography: Effect of morphology and pore structure

Spherical siliceous mesocellular foam (MCF) particles with an average particle size of 4.8 μm have been successfully prepared. These spherical particles were tailored in pore sizes and surface areas. They were functionalized with C₈ or C₁₈ groups, and applied towards reversed phase high-performance liquid chromatography (HPLC) column separations. Their high surface areas gave rise to very good retention characteristics, as illustrated in the separation of a series of alkylbenzene solutes with increasing chain length. The highly interconnected porous structure and ultralarge pore size of MCF allowed the columns to be used at high flow rates without much loss in column efficiency. The column efficiency and peak symmetry were further improved by eliminating the micropores of the stationary phase. The reversed phase column packed with C₁₈-modified spherical MCF particles provided for excellent separation of different deoxynucleosides, illustrating the broad applicability of these materials due to their controlled pore size.     

Determination of remoxipride in human plasma and urine by reversed-phase ion-pair high-performance liquid chromatography.

A sensitive method is described for the measurement of remoxipride in human plasma and urine. Remoxipride and its internal standard are extracted from plasma or urine at pH 12 with a mixture of hexane and methyl tert.-butyl ether. After washing the organic phase with base, the compounds are extracted into acid and analyzed on a C18 column with ultraviolet detection at 214 nm. The mobile phase is composed of acetonitrile and aqueous buffer (sodium perchlorate and phosphoric acid, pH 1.7). The limits of reliable quantitation for remoxipride are 12.5 and 50 ng/ml for plasma and urine, respectively. The run times are 6 min for plasma and 3 min for urine. The method has been successfully used to assay remoxipride clinical study samples. This mobile phase has also been successfully applied to the analysis of other basic drugs such as cimetidine, codeine, diltiazem and quinidine with minor modifications.     

Microwave-Assisted Preparation of a β-Cyclodextrin-Based Stationary Phase for Open Tubular Capillary Electrochromatography

Fluorescein isothiocyanate was used as a label to show that a 3-aminopropylmethyldimethoxysilane (KH 550)-modified capillary column was prepared by microwave irradiation. A bromoacetate-substituted β-cyclodextrin (Br-β-CD) was successfully bound to the KH 550-modified column as a chiral stationary phase for open tubular capillary electrochromatography. Compared with conventional synthesis, the microwave-assisted process significantly decreased the preparation time of the stationary phase from 16 h to 40 min. Baseline chiral separation of 1-phenyl-1,2-ethanediol was achieved using the Br-β-CD modified column.     

Determination of selected phenothiazines in human plasma by solid-phase extraction and liquid chromatography with coulometric detection

A new analytical method, based on liquid chromatography with coulometric detection, has been developed and applied to the determination of selected phenothiazines (chlorpromazine, promazine, fluphenazine and levomepromazine) in human plasma. The drugs were separated on a Discovery pentafluorophenylpropyl column, using a mobile phase composed of acetonitrile (32%) and a pH 1.9 phosphate buffer (68%). Promethazine was used as the internal standard. Detection was carried out at an oxidation potential of +0.500 V. A novel clean-up procedure was developed by means of solid-phase extraction, using cyanopropyl cartridges, which gave good extraction yield for all the analytes, with absolute recovery values higher than 91.0%. The detector response was linear over a plasma concentration range of 0.5-250.0 ng mL⁻¹ for chlorpromazine, promazine and levomepromazine and of 0.2-4.0 ng mL⁻¹ for fluphenazine. Precision results, expressed by the intra-day and the inter-day relative standard deviation values, were good, being lower than 3.9%. Accuracy data were satisfactory as well.The method has been successfully applied to the analysis of drug plasma levels of psychiatric patients undergoing therapy with selected phenothiazines.