On-line coupling of immunoaffinity-based solid-phase extraction and gas chromatography for the determination of s-triazines in aqueous samples

The potential of immunoaffinity-based solid-phase extraction (IASPE) coupled on-line to gas chromatography (GC) for the determination of micropollutants was studied with emphasis on the interfacing of the immunoaffinity-based SPE and GC parts of the system. The cartridge containing the immobilized antibodies was coupled to the gas chromatograph via a reversed-phase cartridge (copolymer sorbent). After trace enrichment of the analytes on the immunoaffinity cartridge, they were desorbed and recollected on the reversed-phase cartridge by means of an acidic buffer. After clean-up and drying with nitrogen, desorption and transfer to the GC was done with ethyl acetate via an on-column interface in the partially concurrent solvent evaporation mode. The antibodies used in the immunoaffinity cartridge were raised against atrazine; several s-triazines were used as test compounds. Triazines that were structurally similar to atrazine, showed quantitative recovery. As an application, immunoaffinity SPE–GC was used for the analysis of river and waste water and orange juice. The selectivity of the system was such that non-selective flame ionization detection (FID) could be used to detect the analytes of interest in these complex matrices. The detection limits for 10-ml water samples were 15–25 ng/l for FID and about 1.5 ng/l for the nitrogen–phosphorus detection.     

Comprehensive two-dimensional gas chromatography with time-of-flight mass spectrometric detection for the trace analysis of flavour compounds in food

The practicability and potential of comprehensive two-dimensional gas chromatography coupled to time-of-flight mass spectrometry (GC x GC-TOF-MS) for the analysis of complex flavour mixtures in food were studied. With the determination of key flavour targets in dairy samples as an example, it was demonstrated that GC x GC dramatically improves the separation. As a consequence, identification and, more importantly, quantification down to the ng/g level can be performed more reliably: background interferences largely disappear. Next to the peak table generated from the GC-TOF-MS software after data processing, the additional use of well-ordered patterns in the 2D-plane and information from second-dimension retention times can substantially help the identification of unknowns. The technique was successfully used for an evaluation of extraction techniques and the characterisation of different types of samples.     

Determination of triazine herbicides in surface and drinking waters by off-line combination of liquid chromatography and gas chromatography-mass spectrometry

Summary Mass spectra of 12 triazines were obtained by electron impact (EI), positive-ion chemical ionization (PCI) and negative-ion chemical ionization (NCI) using methane and isobutane as reagent gases. EI mass spectrometry is more sensitive than PCI and NCI, although the chemical ionization modes increase selectivity markedly. A pre-column packed with polymer stationary phase was employed to preconcentrate surface and drinking water samples. After desorption of the analytes with ethyl acetate, an aliquot was injected directly into the GC-MS system. Atrazine and simizine were found in these samples at 10–80 ppt levels. The limits of detection for both herbicides were below 10 ppt in drinking water.     

Comprehensive two-dimensional gas chromatography with atomic emission detection and correlation with mass spectrometric detection: principles and application in petrochemical analysis

Comprehensive gas chromatography (GC x GC) has been combined with atomic emission detection (AED) to enable element-selective detection. Under optimised experimental conditions, the requirement of minimum five data points across a peak can be obtained even for analytes eluting early from the second-dimension column. Simple manipulation of the results allows the combined presentation of up to four sets of elemental data in one two-dimensional plot. GC x GC with AED and mass spectrometric (MS) detection in petrochemical analysis for fingerprinting as well as the identification of N- and S-containing unknowns is presented as an application.     

Role of the retaining precolumn in large-volume on-column injections of volatiles to gas chromatography

In the present study the retaining precolumn, which is commonly used in a set-up for large-volume on-column injections, or when solid-phase extraction (SPE) or liquid chromatography is coupled to gas chromatography (CC), was removed after varying its length from the standard length of 3 m down to zero. A dramatic increase of the evaporation rate of the injected organic solvent was obtained from a typical value of 100 microl/min up to 300 microl/min. The increased evaporation rate allowed (i) injection of a larger volume in the same retention gap, (ii) faster injection/transfer of the organic solvent and (iii) reduction of the transfer temperature. As volatile compounds under partially concurrent solvent evaporation conditions are easily lost once the organic solvent has been removed via a solvent-vapour exit (SVE), the parameters for large-volume injection, i.e. the evaporation rate and injection speed, were optimised using accurate measurements of the real flow-rate of the carrier gas into the GC system. All these options have been evaluated over the last 4 years. In order to demonstrate that omitting the retaining precolumn had no effect on the application range of the on-column interface, analytes as volatile as benzene were injected into GC-MS using 50-200 microl of n-pentane solutions. Contaminants were extracted from river water and wastewater into n-pentane using in-vial liquid-liquid extraction. The detection limits for benzene, toluene, ethylbenzene and m-xylene were approximately 10 ng/l. To obtain optimum results the SVE had to be closed 1 s before the end of evaporation. Several brands of n-pentane were analysed to check for the presence of benzene. Most of them contained interfering compounds and benzene at the low microg/l level and therefore had to be cleaned by means of column chromatography. As another example C8-C17 alkylphenones were extracted from wastewater with n-hexane. Detection limits were 10-40 ng/l.     

Evaluation of modulators and electron-capture detectors for comprehensive two-dimensional GC of halogenated organic compounds

Different cryogenic and a heated GC x GC modulator(s) were evaluated and compared for the analysis of high-boiling halogenated compounds. The cryogenic modulators investigated were: (i) the longitudinally modulated cryogenic system; (ii) the liquid-nitrogen-cooled jet modulator (KT2001); (iii) a dual-jet CO2 modulator (made in-house); (iv) a semi-rotating cryogenic modulator (made in-house) and (v) a CO2 loop modulator (KT2003); the heated modulator was the slotted heater system (sweeper). Each modulator was optimised with respect to analyte peak widths at half height in the second-dimension. n-Alkanes, chlorinated alkanes, polychlorinated biphenyls (PCBs) and fluorinated polycyclic aromatic hydrocarbons (F-PAHs) were used as test analytes. The flow rate of the coolant was found to be an important parameter, i.e. the flow rate of the gaseous nitrogen in the KT2001, and of the liquid CO2 in the other cryogenic modulators. For the slotted heater the stroke velocity and pause time were important parameters. This modulator had a limited application range in terms of temperature due to a necessary 100 degrees C difference between sweeper and oven temperature. All cryogenic modulators were found to be suitable for the GC x GC analysis of high-boiling compounds, but the CO2 modulators are to be preferred to the KT2001 due to a wider application range and slightly narrower peaks. As regards the performance of three commercially available electron-capture detectors (ECDs), the aim was to obtain narrow peak widths in GC x GC, i.e. to avoid band broadening caused by the cell volume. The most important parameters were the flow rate of the make-up gas and the detector temperature which both should be as high as possible. Comparison of analyte peak widths obtained with ECD mode and flame ionisation detection (FID) showed that all ECDs exhibited band broadening compared to the FID. The narrowest peaks were obtained with the Agilent micro-ECD, which has a cell volume of only 150 microl.     

Development and optimization of a system for comprehensive two-dimensional liquid chromatography with UV and mass spectrometric detection for the separation of complex samples by multi-step gradient elution

Comprehensive two-dimensional liquid chromatography (LC x LC) is a powerful tool for the separation of complex biological samples. This technique offers the advantage of simplified automation and greater reproducibility in a shorter analysis time than off-line two-dimensional separation systems. In the present study, an LC x LC system is developed enabling simultaneous UV and MS detection, and which can be easily converted to a conventional reversed-phase LC-UV/MS system. In LC x LC, a 60-min reversed-phase LC separation with a linear solvent gradient in the first dimension is coupled to a second-dimension separation on a mixed-mode cation-exchange/reversed-phase column with a modulation time of 60s. The isocratic separation in the second-dimension column is optimized by the use of a multi-step gradient where the organic and the ionic modifier are varied independently. Intraday (n=3) and interday (n=4) variability of the retention times were evaluated with the complete system and found to be 0.5% and 0.7%, respectively. Good linearity was observed in calibration curves for three different compounds varying in polarity.     

Fatty acid profiling of raw human plasma and whole blood using direct thermal desorption combined with gas chromatography-mass spectrometry

Gas chromatography (GC) has in recent times become an important tool for the fatty acid profiling of human blood and plasma. An at-line procedure used in the fatty acid profiling of whole/intact aquatic micro-organisms without any sample preparation was adapted for this work. A direct thermal desorption (DTD) interface was used to profile the fatty acid composition of human plasma and whole human blood of eight volunteers in a procedure omitting the usual lipid extraction steps that precede sample methylation in the traditional (off-line) protocols. Trimethylsulfonium hydroxide (TMSH) was used as reagent for thermally assisted methylation. In a fully automated manner, the liner of the GC injector is used as a sample-and-reaction container with the aid of the DTD interface. The fatty acid methyl ester (FAME) profiles obtained using this novel approach, were very identical to those obtained when the traditional off-line protocol was applied. FAME yields obtained in the at-line DTD method were found to be very similar for saturated fatty acids, but significantly higher for polyunsaturated fatty acids compared to off-line yields. As a result of the contribution of circulating cell membranes in blood, substantial differences were observed when the amount of FAMEs obtained in whole human blood and human plasma samples were compared after their analysis. Thanks to the fully automated operation of this novel procedure, large series of analyses can easily be performed.     

Fast Temperature Programming in Gas Chromatography using Resistive Heating

The features of a resistive-heated capillary column for fast temperature-programmed gas chromatography (GC) have been evaluated. Experiments were carried out using a commercial available EZ Flash GC, an assembly which can be used to upgrade existing gas chromatographs. The capillary column is placed inside a metal tube which can be heated, and cooled, much more rapidly than any conventional GC oven. The EZ Flash assembly can generate temperature ramps up to 1200°/min and can be cooled down from 300 to 50°C in 30 s. Samples were injected via a conventional split/splitless injector and transferred to the GC column. The combination of a short column (5 m×0.25 mm i. d.), a high gas flow rate (up to 10 mL/min), and fast temperature programmes typically decreased analysis times from 30 min to about 2.5 min. Both the split and splitless injection mode could be used. With n-alkanes as test analytes, the standard deviations of the retention times with respect to the peak width were less than 15% (n = 7). First results on RSDs of peak areas of less than 3% for all but one n-alkane indicate that the technique can also be used for quantification. The combined use of a short GC column and fast temperature gradients does cause some loss of separation efficiency, but the approach is ideally suited for fast screening as illustrated for polycyclic aromatic hydrocarbons, organophosphorus pesticides, and triazine herbicides as test compounds. Total analysis times – which included injection, separation, and equilibration to initial conditions – were typically less than 3 min.     

Use of a Drying Cartridge in On-Line Solid-Phase Extraction–Gas Chromatography–Mass Spectrometry

A drying cartridge was used and optimized for the in-line elimination of water from the desorption eluent in on-line solid phase extraction–gas chromatography (SPE–GC). The cartridge is essentially a small stainless-steel precolumn packed with a drying agent which can be regenerated by simultaneous heating and purging with a moisture-free gas. The drying cartridge was mounted on an additional valve instead of between the SPE–GC transfer valve and the on-column injector to enable regeneration of the cartridge during the GC run and, thus, to increase sample throughput. Three drying agents were tested, viz. sodium sulfate, silica, and molecular sieves. Although molecular sieves have the highest capacity, silica was preferred because of practical considerations. Large-volume injections were performed through the in-line drying cartridge using a mixture of 23 microcontaminants ranging widely in polarity and volatility. Four solvents were tested. With pentane and hexane, the more polar analytes were retained by the drying cartridge. Ethyl acetate and methyl acetate gave much better (and closely similar) recoveries for all analytes. Because water elimination on the silica cartridge proved to be less critical than with ethyl acetate, this solvent was finally selected. The entire SPE–drying cartridge–GC set-up was combined with mass spectrometric (MS) detection for the determination of a mixture of micropollutants in real-life water samples. With 10-ml tap water samples spiked at the 0.5 μg/l level, for the majority of the test compounds the analyte recoveries generally were 60–106%, and (full-scan) detection limits typically were 0.01–0.03 μg/l. Some very polar analytes such as, e.g. dimethoate, were (partially) sorbed onto the silica packing of the drying cartridge.