Gas chromatography of amino acids: Use of a fused-silica capillary column in the determination of plasma amino acids

A capillary chromatographic procedure using a fused silica column is described which can be used to quantitatively determine amino acids in plasma following the pre-chromatographic “clean-up” described in a recent paper [1]. In substituting this procedure for that involving a packed column, advantage has been taken of the greater resolving power to separate amino acids from background component peaks. In order to extend this advantage and provide a sound basis for quantitative analysis, the technique of cold on-column injection was employed. As a result, good precision of standard analysis was obtained with relative standard deviation (RSD) values for all amino acids of less than 4%. Application of the entire procedure to plasma samples yields RSD values of better than 10% for all amino acids with recoveries ranging from 72% to 104%. Simultaneous determination of plasma amino acid levels by gas chromatography (GC) using capillary columns and by classical ion exchange (CIE) showed reasonable agreement. Statistical evaluation showed no significant difference between twelve amino acids. Values for the remaining two, namely, phenylalanine and histidine are significantly different (p < 0.005). Comparison of the values obtained from GC capillary and packed columns reveals no significant difference between fourteen amino acids. Significant differences exist between results for phenylalanine and tyrosine (p < 0.001). It is concluded that there is good agreement between data obtained by GC capillary and CIE techniques and that differences between results for phenylalanine and histidine are method related.     

On-line hydrogenation of fatty acid methyl esters in capillary gas chromatography

An injection splitter in front of a glass capillary column was used for the hydrogenation of fatty acid methyl esters (FAME) mixtures. Hydrogenation followed by gas chromatographic analysis on capillary columns permitted detection and identification in complicated natural mixtures of branched fatty acids, showing minor structural differences, in quantities down to 10^?8g. The technique described, apart from its suitability for FAME analysis, shows promise for structure determination studies of other classes of compounds.     

Evaluation of syringe handling techniques for injections into vaporizing GC injectors

Unequal elution of sample components of different volatility out of the syringe needle is one of the major causes for discrimination occuring during the injection, i.e. the phenomena which results in peak areas for the high boiling compounds which are too small compared with the volatiles. This problem, associated with all vaporizing injectors that are used with syringes, can be minimized by careful choice of the needle handling technique. Various methods are compared experimentally. The “solvent flush” method is discussed in detail and demonstrated to be ineffective for reducing losses in the syringe needle. The “hot needle” technique, where the empty needle is preheated in the injector before pushing the plunger, was found to be superior or equal to an improved “solvent flush” method (which included preheating the needle and omitting the air plug between sample and flushing solvent. Generally it was found that the discrimination due to the syringe needle was reduced for larger sample volumes, although no further changes were noticed when these exceeded 2.5 to 3μl.     

Profiles of volatile metabolites in biological fluids using capillary columns

Nickel capillary columns coated with moderately polarstationary phases such as Witconol can be used for the separation of the organic volatile fraction from biological fluids. A “transevaporator” sampling technique for the collection of the organic volatiles on glass beads from as little as 5 to 500 μl of biological fluids (e.g. urine, serum, amniotic fluid, breast milk, saliva, etc.) is described. The organic volatiles are thermally desorbed from the glass beads into a short precolumn cooled in liquid nitrogen, which overcomes the problems associated with sample introduction onto narrow-bore capillary columns. The application of the full analytical technique to problems associated with the early detection of disease is illustrated.     

Glass capillary gas chromatography of amino acid enantiomers

Glass capillaries coated with Chirasil-Val, a chirally functionalised polysiloxane, are capable in principle of resolving all protein amino-acid enantiomers in a single run and within a short analysis time, thus allowing for example the quantitative amino acid determination by enantiomer labelling. The elution characteristics of the individual amino acids however are also dependent upon the chemical nature of the capillary wall surface, and a surface pretreatment is found to be necessary if all protein amino acids are to be analysed. Of the various methods of pretreatment tested, etching of borosilicate glass with gaseous HCl followed by deposition of colloidal silicic acid is considered to be the most suitable.     

Quantitation in capillary gas chromatography with emphasis on the problems of sample introduction

Sampling techniques for practical quantitative capillary GC have to meet certain principal requirements. Both the absolute and the relative peak areas (e.g. column loads) must be reproducible with high precision and at high accuracy; discrimination of certain constituents according to their volatility should not take place on sampling. On the basis of systematic studies, the three most reliable sampling techniques used for GC analyses with the aim of achieving precise and accurate quantitative data proved to be the following: On-column, injection, splitless PTV injection, and an optimized version of split sampling called “cooled needle split” injection. The on-column technique can be optimized by using precolumns with wider internal diameters and without stationary phase coatings to overcome the problems of large liquid sampling volumes and for automation. The PTV technique should only be used in the splitless mode because discrimination cannot be suppressed completely with the split mode. All three of the techniques can be operated automatically, either to avoid “human interference”, i.e. to improve precision or for unattended operation to save man-power.     

Differences in absorbance levels as found in capillary zone electrophoresis under stacking conditions

During some capillary zone electrophoresis (CZE) experiments, the baseline UV absorbance signal at 200 nm “jumped” from one stable level prior to the water plug (marking the flow of neutrals) to another stable level after the water plug. The phenomenon was further examined with distilled water as the sample and with different buffers, applied potentials, and salt concentrations in the buffer. It seems that there is an “isotachophoretic effect” on top of the CZE separations when running under stacking conditions. The effect results in a higher pH value of the buffer after the water plug compared to the pH prior to the plug. The nature of the buffer, the salt concentration in the buffer, and the applied potential all affect this phenomenon.     

Suitability of automated capillary and micro liquid chromatography for routine determination of drugs in human plasma samples from clinical pharmacokinetic investigations

One of the most widely acclaimed features of capillary and microcolumn LC, in comparison with conventional HPLC, is the enormous increase in mass sensitivity. Nevertheless, application of capillary and micro LC in quantitative trace bioanalysis, characterized by weak analyte concentrations in complex matrices, can only be of any practical utility if large sample volumes can be injected onto the columns without affecting chromatographic resolution and efficiency. Two applications of large volume injection in a non-eluting solvent (on-column focusing) for the quantitative analysis of drugs in biological fluids on both capillary and micro chromatographic systems are presented: the first example deals with a new selective H₁-antihistaminic drug, mizolastine, the second one with a well known calcium antagonist, diltiazem, and its main metabolites. For both compounds, results obtained on micro and capillary LC in comparison with conventional HPLC are reported. The results demonstrate that when conventional HPLC methods are transformed into either micro or capillary LC techniques, they gain in sensitivity. By means of an on-column focusing technique, it is possible to increase the sensitivity 3–5 fold in comparison to conventional HPLC methods, but not 50–60 fold as obtained on synthetic drug solutions. Column robustness, handiness, reproducibility, and suitability of micro systems for routine bioanalysis are discussed for both capillary and micro LC columns, as well as limits of the technique in trace organic analysis problems.     

The “disturbing zone” in overpressure layer chromatography (OPLC)

This paper describes the fundamental factors causing the “disturbing zone” in OPLC. This phenomenon of distorted substance zones appears when the OPLC separation is started with a dry layer and is due to interaction between the gas that is physically bound to the surface of the sorbent (m_a) and the gas molecules dissolved in the eluent (m_s). Possibilities for elimination of the adverse effects of disturbing zones ultimately depend on the establishment of operating conditions that inhibit their initial formation. Since modification of the location of the disturbing zone is only possible within a very narrow range, the sole solution to this problem is to conduct a pre-run, which may be carried out with hexane in the case of separation of apolar compounds. For separation of polar substances, the pre-run may also be performed with hexane or with a solvent of the mobile phase in which the components are unable to migrate. The selection of this solvent may be considered during the optimization of the eluent system.     

Narrow bore silica capillary columns for liquid-modified adsorption gas chromatography

Summary The preparation of narrow bore capillary columns for liquid-modified adsorption chromatography is described, and the advantages of this technique for rapid analysis of complex mixtures are discussed.Several applications to the analysis of complex mixtures are reported, and the possibility of on-column injection is demonstrated.     

Automated capillary liquid chromatography for simultaneous determination of neuroactive amines and amino acids

A method for the separation and quantitative determination of neuroactive amino acids (aspartate, glutamate, citrulline, arginine, glycine, taurine, gamma-aminobutyric acid) and neuroactive amines (noradrenaline, dopamine and serotonin) in a single chromatographic analysis is presented. The method is based on pre-column derivatization with o-phthalaldehyde and tert.-butyl thiol, on-column preconcentration and separation using 50 microns I.D. packed capillary columns, and detection by amperometry. Mass limits of detection are 80-900 amol for all neurotransmitters with RSDs of 0.71 and 4.6% or better for retention time and peak area, respectively. The method was demonstrated by application to the determination of neurotransmitters in microdialysis samples collected from striatum of live rats and tissue samples extracted from butterfly brains.     

Preparation of phenolic microspheres in water/“water” system

Phenolic microspheres were obtained by condensation of resorcinol and formaldehyde via a novel water/“water” suspension polymerization (WWSP) system, which was proposed and constructed for the first time. Resorcinol/formaldehyde aqueous solutions, ammonium sulfate aqueous solution, hydroxyethyl cellulose (HEC), and sodium hydroxyl were employed as water phase, “water” phase, stabilizer for protecting colloid, and catalyst, respectively. Stable and perfect phenolic microspheres were prepared in this special WWSP system. Particle sizes, size distribution, as well as morphology of microspheres were investigated by scanning electron microscope and computerized image analysis program. The results showed that particle size increased from 0.38 to 2.22 µm along with the increase of concentration of ammonium sulfate in “water” phase from 1.5% to 12.5% and the ratio of resorcinol to formaldehyde from 1:1.5 to 1:4. On the contrary, the particle size decreased from 1.80 to 0.30 µm with the increase of the amount of HEC from 0.1 to 1.0 g and amount of catalyst from 0.05 to 0.2 g. The polydispersity index value of the resulting microspheres is quite narrow, ranging from 1.01 to 1.30, which meant that the morphology of phenolic microspheres was unique. Copyright © 2011 John Wiley & Sons, Ltd.     

Analysis of volatile fatty acids in biological specimens by capillary gas chromatography

A method was developed to analyze and quantitate volatile fatty acids such as acetic, propionic, butyric, iso-butyric, valeric, and iso-valeric acid from samples of biological origin. A capillary column system including an automatic on-column injection device as well as a precolumn of larger internal diameter than the analytical column was elaborated for this purpose. In order to obtain well resolved and correctly quantifiable chromatographic peaks it turned out to be essential to work under acidic/aqueous conditions. To achieve a better sample transfer into the chromatographic system an organic solvent had to be used together with the aqueous milieu, thus improving wetting properties of the liquid sample plug introduced into the column. Cold on-column injection was applied in order to avoid discrimination of the various acids due to sample splitting and the automatic technique was chosen in view of the large number of samples from biological extractions which had to be analyzed.     

Efficient synthesis of monodisperse,highly crosslinked,and “living” functional polymer microspheres by the ambient temperature iniferter‐induced “living” radical precipitation polymerization

The facile and efficient one‐pot synthesis of monodisperse, highly crosslinked, and “living” functional copolymer microspheres by the ambient temperature iniferter‐induced “living” radical precipitation polymerization (ILRPP) is described for the first time. The simple introduction of iniferter‐induced “living” radical polymerization (ILRP) mechanism into precipitation polymerization system, together with the use of ethanol solvent, allows the direct generation of such uniform functional copolymer microspheres. The polymerization parameters (including monomer loading, iniferter concentration, molar ratio of crosslinker to monovinyl comonomer, and polymerization time and scale) showed much influence on the morphologies of the resulting copolymer microspheres, thus permitting the convenient tailoring of the particle sizes by easily tuning the reaction conditions. In particular, monodisperse poly(4‐vinylpyridine‐co‐ethylene glycol dimethacrylate) microspheres were prepared by the ambient temperature ILRPP even at a high monomer loading of 18 vol %. The general applicability of the ambient temperature ILRPP was confirmed by the preparation of uniform copolymer microspheres with incorporated glycidyl methacrylate. Moreover, the “livingness” of the resulting polymer microspheres was verified by their direct grafting of hydrophilic polymer brushes via surface‐initiated ILRP. Furthermore, a “grafting from” particle growth mechanism was proposed for ILRPP, which is considerably different from the “grafting to” particle growth mechanism in the traditional precipitation polymerization. © 2013 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem, 2013     

Synthesis of novel hyperbranched poly(ester‐amide)s based on neutral α‐amino acids via “AD + CBB′” couple‐monomer approach

A series of novel hyperbranched poly(ester‐amide)s (HBPEAs) based on neutral α‐amino acids have been synthesized via the “AD + CBB′” couple‐monomer approach. The ABB′ intermediates were stoichiometrically formed through thio‐Michael addition reaction because of reactivity differences between functional groups. Without any purification, in situ self‐polycondensations of the intermediates at elevated temperature in the presence of a catalyst afforded HBPEAs with multihydroxyl end groups. The degrees of branching (DBs) of the HBPEAs were estimated to be 0.40–0.58 and 0.24–0.54 by quantitative ¹³C NMR with two different calculation methods, respectively, depending on polymerization conditions and structure of monomers. The influences of catalyst, temperature, and intermediate structure on the polymerization process and molecular weights as well as properties of the resultant polymers were investigated. FTIR, NMR, and DEPT‐135 NMR analyses revealed the branched structure of the resultant polymers. The HBPEAs possess moderately high molecular weights with broad distributions, glass transition temperatures in the range of ?25.5 to 36.5 °C, and decomposition temperatures at 10% weight loss under nitrogen and air in the regions of 243.4–289.1 °C and 231.4–265.6 °C, respectively. Among them, those derived from D ,L ‐phenylalanine display the lowest degree of branching, whereas the highest glass transition temperature and the best thermal stability. © 2010 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem, 2010     

Solute focusing technique for on-column injection in capillary gas chromatography

A novel solute focusing technique for on-column injection of liquid samples onto capillary GC columns is described. The focusing technique allows injection of 8.0 microliters or more of sample without producing the peak distortion or splitting observed under conventional on-column injection conditions. The experimentally determined performance of the technique is given for a wide volatility range sample. Solute focusing is useful in situations where on-column injection of 1.0 microliter or greater is required.     

On-column injection onto capillary columns. Part 2: Study of sampling conditions; practical recommendations

During one year continuous use of on-column injection, the typical advantages described in our first report have fully been confirmed. In addition the analysis of large sample volumes has proved promising. Only minor modifications have been applied to the on-column injector device. Broad evidence has been gathered showing that full separation efficiency of the capillary columns after on-column injection is attained only when cold trapping or the solvent effect, as band shortening mechanisms, are working- While, under the conditions of on-column injection, cold trapping is less efficient than with other injection techniques, the opposite holds true for the solvent effect. Compared with splitless injection, the danger of excessive solvent condensation on the column is increased. A working rule is presented for establishing the optimal chromatographic conditions for handling large sample volumes while ensuring full separation efficiency yet avoiding harm to the column.     

Precision of an automated all-glass capillary gas chromatography system with an electron capture detector for the trace analysis of estrogens

Subnanogram detection of steroids has become increasingly important today. One applicable method for gas chromatographic determination of subnanogram quantities of estrogens as halogenated derivatives is electron capture detection. HFB-derivatives of 7 different estrogens were automatically injected onto a prolonged narrow bore wall-coated glass capillary column. Normal split injection could not be used for this trace analysis because of too much loss of sample. Only small amounts of sample were available from which double analysis had to be performed. Cross-contamination of the automatic sampling system as well as precision of retention times and peak areas were determined. The type of injection described showed better quantitative results compared to the splitless injection technique. All details of the system used together with the results are this discussed in this paper.     

Mass Spectra of 2- and 6-Substituted-3-Pyrones: Competition Between “RETRO-DIELS-ALDER” Fragmentation and Substituent Loss

The mass spectra of a series of 6-hydroxy-3-pyrones and their derivatives showed a marked dependence upon the nature of the substituent. The “retro-Diels-Alder” reaction is the primary decomposition observed for the parent compounds, while the α-cleavage (substituent loss) competes with the “retro-Diels-Alder” reaction for their derivatives. An interpretation of this difference based on the charge location and the thermochemical data is proposed.