Gas-chromatographic retention indices in dependence on the ratio of analytes to reference components

One of the main factors determining the interlaboratory reproducibility of gas-chromatographic retention indices is their linear dependence on the logarithms of the ratios of the amounts of analytes and reference components, which is rarely taken into account. It is found that the effect of this factor is much stronger for packed columns in comparison to that for more efficient capillary columns; it decreases with the sample dilution and with the increase in the temperature of gas-chromatographic separation. It was shown that the effect of relative amounts of components on their retention indices agrees with the main principles of the chromatographic plate theory and is associated with neither the overloading of chromatographic columns nor the nonlinearity of the adsorption isotherms. To improve the reproducibility of indices, it is recommended to use retention parameters measured at certain points in the front edges of the chromatographic peaks corresponding to similar intensities of the analytical signal rather than at the peak maxima.     

Retention indices as identification tool in pyrolysis-capillary gas chromatography

Pyrolysis-capillary gas chromatography (Py-cGC) represents important method to identify the analytes in the mixture after thermal degradation. This combines high effective analyte separation on-line coupled with thermal degradation process that depends on analyte structure. System of retention indices has been used for identification of the analytes after on-line pyrolysis and chromatographic separation. The pyrolysate composition has been studied during thermal degradation of polymethylmethacrylate (PMMA) at different pyrolysis temperatures and chromatographic column conditions. Homologues series of n-alkanes have been used for calculation of pyrolysate Kováts retention indices (I) and compared with mass spectrometric (MS) data of pyrolysate model mixture. To identify PMMA thermal degradation products the high density polyethylene (HDPE) as additive standard producing triplets of the olefin homologous series during co-pyrolysis has been used. These homologous series enable to calculate programmed temperature retention indices (ITPGC) to identify the analytes present in the pyrolysate. Calculated I values were compared with published I values databases to identify analytes yielded at different pyrolysis temperatures.     

Modification of the algorithm of determining chromatographic retention indices for compensating their dependence on the ratio of analytes and reference components

One of the main sources of the interlaboratory variation of chromatographic retention indices, especially in using packed columns, is their dependence on the ratio of the amounts of characterized analytes and reference components (γ). It is shown that this dependence can be compensated without any additional experiments. The recording of the retention parameters of the characterized and reference components at their fronts at the points corresponding to equal absolute intensities of the signals, rather than at the maxima of the chromatographic peaks provides the most reproducible values of retention indices, practically independent on the values of γ.     

Handling within run retention time shifts in two-dimensional chromatography data using shift correction and modeling

The use of PARAFAC for modeling GC × GC-TOFMS peaks is well documented. This success is due to the trilinear structure of these data under ideal, or sufficiently close to ideal, chromatographic conditions. However, using temperature programming to cope with the general elution problem, deviations from trilinearity within a run are more likely to be seen for the following three cases: (1) compounds (i.e., analytes) severely broadened on the first column hence defined by many modulation periods, (2) analytes with a very high retention factor on the second column and likely wrapped around in that dimension, or (3) with fast temperature program rates. This deviation from trilinearity is seen as retention time-shifted peak profiles in subsequent modulation periods (first column fractions). In this report, a relaxed yet powerful version of PARAFAC, known as PARAFAC2 has been applied to handle this shift within the model step by allowing generation of individual peak profiles in subsequent first column fractions. An alternative approach was also studied, utilizing a standard retention time shift correction to restore the data trilinearity structure followed by PARAFAC. These two approaches are compared when identifying and quantifying a known analyte over a large concentration series where a certain shift is simulated in the successive first column fractions. Finally, the methods are applied to real chromatographic data showing severely shifted peak profiles. The pros and cons of the presented approaches are discussed in relation to the model parameters, the signal-to-noise ratio and the degree of shift.     

Evaluation of analyte protectants to improve gas chromatographic analysis of pesticides

A common problem in gas chromatography (GC) applications is the analyte losses and/or peak tailing due to undesired interactions with active sites in the inlet and column. Analytes that give poor peak shapes or degrade have higher detection limits, are more difficult to identify and integrate, and are more prone to interferences than stable analytes that give narrow peaks. For susceptible analytes, significant peak quality improvements are obtained when matrix components are present because they fill active sites, thus reducing analyte interactions. This phenomenon is called "matrix-induced chromatographic response enhancement." Several approaches have been proposed to minimize peak distortion phenomena and compensate for matrix-induced effects, which is especially important for accurate quantitation, but each approach has serious limitations for routine multi-pesticide analysis. In this study, we demonstrate the feasibility of using "analyte protectants" to provide a more convenient and effective solution to the problem than other approaches developed thus far. The protecting agents are added to extracts and matrix-free standards alike to provide the chromatographic enhancement effect even for the most susceptible analytes in a very dirty GC system. In this study, we evaluated 93 different compounds to find the most suitable ones for improving chromatographic quality of the signal. Because hydrogen bonding has been shown to be an important factor in analyte interactions with active sites, we mainly focused on additives with strong hydrogen bonding capabilities. Dramatic peak enhancements were achieved using compounds containing multiple hydroxy groups, such as sugars and sugar derivatives, and gulonolactone appears to be the most effective protecting agent for the most pesticides that we tested. The benefits of using analyte protectants versus alternative procedures for overcoming matrix-induced effects in quantitation include: (a) simpler procedure; (b) easier integration of peaks; (c) lower detection limits; (d) better quantitation; (e) less maintenance of the GC inlet; and (e) lower cost. However, long-term influences on the performance of the chromatographic system have yet to be established.     

Direct analysis of plasma samples for drug discovery compounds using mixed-function column liquid chromatography tandem mass spectrometry

A sensitive, efficient, high throughput, direct injection bioanalytical method based on a single column and high-performance liquid chromatography (HPLC) with tandem mass spectrometry (MS/MS) was developed for pharmacokinetic analysis of early drug discovery compounds in plasma samples. After mixing with a working solution containing an internal standard each plasma sample was directly injected into a polymer-coated mixed-function column for sample cleanup, enrichment and chromatographic separation. The stationary phase incorporates hydrophilic polyoxyethylene groups and hydrophobic groups to the polymer-coated silica. This allows proteins and macromolecules to pass through the column due to restricted access to the surface of the packing while retaining the drug molecules on the bonded hydrophobic phase. The analytes retained in the column with a largely aqueous liquid mobile phase were then chemically separated by switching to a strong organic mobile phase. The column effluent was diverted from waste to the mass spectrometer for analyte detection. Within 200 plasma sample injections the response ratio (analyte vs. internal standard, %CV = 4.6) and the retention times for analyte and internal standard were found consistent and no column deterioration was observed. The recoveries of test compound in various plasma samples were greater than 90%. The total analysis time was 相似文献   

Prediction of retention indexes. III. Silylated derivatives of polar compounds.

Polar compounds containing hydroxyl, amino and carboxyl groups, singly or in combination, can be chromatographed after the polar functional groups are silylated. The silylated derivatives of acids, alcohols, amines, diols, amino alcohols, amino acids are shown to behave chromatographically as hydrocarbons, and their retention indexes can be readily predicted from their base values. The column difference, namely, the difference between the retention indexes of the analyte on polar and non-polar columns is minimal for the silylated derivatives in comparison to that observed for the underivatized analytes. This minimal column difference is attributed to the hydrocarbon-like chromatographic characteristics of the silylated derivatives. The retention indexes of the silyl derivatives appear to correlate with the atom number Z of the analyte.     

Effect of ionic additives on the elution of sodium aryl sulfonates in supercritical fluid chromatography

Addition of a small amount of polar solvent (i.e., modifier) to CO2 in packed column supercritical fluid chromatography (SFC) has shown major improvements in both polar analyte solubility and interaction of the polar analyte with the stationary phase. Recently, the addition of an ionic component (i.e., additive) to the primary modifier by one of us has been shown to extend even further the application of SFC to polar analytes. In this work, the effect of various ionic additives on the elution of ionic compounds, such as sodium 4-dodecylbenzene sulfonate and sodium 4-octylbenene sulfonate, has been studied. The additives were lithium acetate, ammonium acetate, tetramethylammonium acetate, tetrabutylammonium acetate, and ammonium chloride dissolved in methanol. Three stationary phases with different degrees of deactivation were considered: conventional cyanopropyl, deltabond cyanopropyl, and bare silica. The effect of additive concentration and additive functionality on analyte retention was investigated. Sodium 4-dodecylbenzene sulfonate was successfully eluted using all the additives with good peak shape under isocratic/isobaric/isothermal conditions. Different additives, however, yielded different retention times and in some cases different peak shapes.     

Impact of column temperature and mobile phase components on selectivity of hydrophilic interaction chromatography (HILIC)

The retention mechanism and chromatographic behavior for different polar analytes under hydrophilic interaction chromatography (HILIC) conditions have been studied by application of different mobile phases and stationary phases to various analytes at different temperatures. In addition to the commonly accepted mechanism of analyte liquid-liquid partitioning between mobile phase and water-enriched solvent layer which is partially immobilized onto the surface of the stationary phase, hydrogen-bonding, hydrophobic interaction, and ion-exchange interactions may also be involved. The predominant retention mechanism in HILIC separation is not always easily predictable. It can depend not only on the characteristics of the analytes but also on the selection of mobile and stationary phase compositions. The objective of this review is to evaluate the potential application of column temperature and mobile phase composition toward improving HILIC selectivity. The functional groups from analyte structures, stationary phase materials and organic mobile phase solvents will be highlighted.     

Rapid extraction and analysis of organic compounds from solid samples using coupled supercritical fluid extraction/gas chromatography

Summary Direct coupling of supercritical fluid extractions with gas chromatography (SFE-GC) allows the extraction, concentration, and gas chromatographic analysis of organic analytes from solid samples to be performed in less than 1 h. Coupling of the supercritical fluid extraction step with a capillary gas chromatographic column is achieved using a standard on-column injector and requires no modification of the gas chromatograph. Maximum sensitivity is achieved and analyte degradation or loss is minimized since the extracted species are quantitatively transferred into the fusedsilica capillary gas chromatographic column where they are cryogenically focused prior to normal gas chromatographic analysis using flame ionization (SFE-GC/FID) or mass spectral (SFE-GC/MS) detection. SFE-GC analysis yields good chromatographic peak shapes that compare favorably with those obtained using standard on-column injection techniques. Class-selective extractions can be achieved by performing multiple SFE-GC analyses with different extraction pressures. The ability of coupled SFE-GC to yield rapid extraction and analysis of organic analytes is demonstrated for a variety of samples including polycyclic aromatic hydrocarbons (PAHs) from treated wood, urban dust, and river sediment, phenolic species from wood smoke particulates, nicotine from tobacco, biological markers from coal, and flavor components from food products.

---

Schnelle Extraktion und Analyse von organischen Verbindungen aus festen Proben durch Kopplung von Extraktion mit überkritischen fluiden Phasen und GC

     

Automated screening of reversed‐phase stationary phases for small‐molecule separations using liquid chromatography with mass spectrometry

There are various reversed‐phase stationary phases that offer significant differences in selectivity and retention. To investigate different reversed‐phase stationary phases (aqueous stable C₁₈, biphenyl, pentafluorophenyl propyl, and polar‐embedded alkyl) in an automated fashion, commercial software and associated hardware for mobile phase and column selection were used in conjunction with liquid chromatography and a triple quadrupole mass spectrometer detector. A model analyte mixture was prepared using a combination of standards from varying classes of analytes (including drugs, drugs of abuse, amino acids, nicotine, and nicotine‐like compounds). Chromatographic results revealed diverse variations in selectivity and peak shape. Differences in the elution order of analytes on the polar‐embedded alkyl phase for several analytes showed distinct selectivity differences compared to the aqueous C₁₈ phase. The electron‐rich pentafluorophenyl propyl phase showed unique selectivity toward protonated amines. The biphenyl phase provided further changes in selectivity relative to C₁₈ with a methanolic phase, but it behaved very similarly to a C₁₈ when an acetonitrile‐based mobile phase was evaluated. This study shows the value of rapid column screening as an alternative to excessive mobile phase variation to obtain suitable chromatographic settings for analyte separation.     

Effect of mobile phase anionic additives on selectivity,efficiency, and sample loading capacity of cationic drugs in reversed-phase liquid chromatography

In the present work, we study the effect of mobile phase anionic additive type and concentration on the selectivity, efficiency, and sample loading capacity of cationic drugs in reversed-phase liquid chromatography (RPLC). The type and concentration of an anionic additive are known to have a strong effect on the absolute retention of cations in RPLC; in contrast they have only a small effect on the selectivity of one cation relative to a second as seen here. This is mainly due to the similarity of the ion pair formation constants between the selected cations. The limiting retention factors of cations (i.e. the retention factor of the fully ion-paired analyte at very high additive concentration) are roughly proportional to their inherent hydrophobicities (i.e. the retention factor of the analyte in the absence of the anionic additive). With a given anion, differences in ion pairing strength between the solutes are required for effective selectivity adjustment. Based on the Wade–Lucy–Carr (W–L–C) kinetic model of overload peaks, the approach we developed in our previous work was used to study the effect of mobile phase anionic additives type and concentration on the limiting plate count (N₀) and sample loading capacity (ω_0.5) of various cationic drugs. Under linear chromatographic conditions, where the analyte exhibits its smallest peak width and thus maximum apparent plate count, the type and concentration of anionic additives have almost no effect on peak width. In comparison to neutral analytes the sorption isotherms of cationic species are very easily overloaded even when many fewer moles of cations as compared to neutrals are injected. We showed that different anionic additives profoundly affect the cations’ “overload profiles” (i.e. plots of plate count versus amount injected) by changing the sample loading capacities. The increase in sample loading capacities with different anions show the same order as the extent of ion pairing between the anions and the basic analytes. The detrimental effect of sample overloading on peak width can be greatly diminished by using either a stronger ion pairing agent or a higher concentration of a given ion pairing agent. Both effects operate by increasing the sample loading capacity, thereby allowing more solute to be injected. We believe that the increase in sample loading capacity described above is due in part to the increase in the number of ion-exchange sites as more anions sorb to the stationary phase. At the same time, the formation of a neutral ion-paired analyte also increases the amount of cation which can be loaded onto the stationary phase by allowing a greater fraction of the analyte to be present in the stationary phase as an electrically neutral (i.e. ion-paired) species.     

Modeling the effects of type and concentration of organic modifiers, column type and chemical structure of analytes on the retention in reversed phase liquid chromatography using a single model

A previously proposed model for representing the retention factor (k) of an analyte in mixed solvent mobile phases was extended to calculate the k of different analytes with respect to the nature of analyte, organic modifier, its concentration and type of the stationary phase. The accuracy of the proposed method was evaluated by calculating mean percentage deviation (MPD) as accuracy criterion. The predicted vs. observed plots were also provided as goodness of fit criteria. The developed model prediction capability compared with a number of previous models (i.e. LSER, general LSER and Oscik equation) through MPD and fitting plots. The proposed method provided acceptable predictions with the advantage of modeling the effects of organic modifiers, mobile phase compositions, columns and analytes using a single equation. The accuracy of developed model was checked using the one column and one analyte out cross validation analyses and the results showed that the developed model was able to predict the unknown analyte retention and the analytes retentions on unknown column accurately.     

Gas chromatographic system for the identification of halogenated pesticides by retention indices using n-alkanes as standards

A gas chromatographic system for the evaluation of linear temperature-programmed retention indices allowing n-alkanes to be adopted as the reference retention markers for any type of analyte, irrespective of the atoms present in their molecules, is described. It is based on the simultaneous use of two different detectors (a flame ionization detector and a specific detector suitable for the sample components), both connected (in parallel) to the same column outlet. The performance of this system has been tested by measuring the retention indices of fifteen chlorinated pesticides under conditions of linear programming temperature, by adopting an electron-capture detector as the specific detector. The reliability of the retention indices thus determined has been proven by verifying that they can be reproduced under different chromatographic conditions.     

Gas chromatography with mass spectrometry analysis of phosphoserine,phosphoethanolamine, phosphoglycerol,and phosphate

A new, rapid, sensitive, robust, and reliable method has been developed for the qualitative analysis of phosphoserine, phosphoethanolamine, phosphoglycerol, and phosphate using gas chromatography with mass spectrometry and two‐step trimethylsilylation. The method employs hexamethyldisilazane for silylation of the phosphate and hydroxyl groups in the first phase and bis(trimethylsilyl)trifluoroacetamide for silylation of the less‐reactive amino groups in the second phase. This order is of key importance for the method because of the different reactivities of the two reagents and the mechanism of derivatization of the active groups of the analytes. Trimethylsilylated derivatives of the analytes were identified on the basis of their retention times and mass spectra. The probable structures of the major fragments were identified in the spectra of the trimethylsilylated derivatives and characteristic m/z fragments were selected for each analyte. Fragments with m/z 73 and 299 occurred in the spectra of all the analytes. The characteristic retention data were employed to calculate the retention indices of the individual silylated phosphorylated substances in the hydrocarbon range C₁₂–C₁₉ for the DB‐5ms column. The method was employed to measure the polar fraction of the hydrolysate of the cytoplasmic membrane of Bacillus subtilis. The detection limits vary between 5 μg/mL (trimethylsilylated phosphate) and 72 μg/mL (trimethylsilylated phosphoethanolamine).     

Anomalous temperature dependence of gas chromatographic retention indices of polar compounds on nonpolar phases

The character of the temperature dependences of the retention indices RI(Т) of polar sorbates on nonpolar stationary phases was found to depend on the dosed amounts of sorbates, but not on column overloading. A physicochemical model was suggested to explain the observed anomalies in RI(Т).     

The effect of column characteristics on the minimum analyte concentration and the minimum detectable amount in capillary gas chromatography

The need for faster and more efficient separations of complex mixtures of organic compounds by gas chromatography has led to the development of small inner diameter open tubular columns. Owing to their decreased plate height, extremely narrow peaks are obtained. When differently sized columns with equal plate numbers are compared, injection of a fixed amount of a solute will give the highest detector signals for the smallest bore columns. When P is defined as the ratio of the column inlet and outlet pressures, it can be seen from theory that under normalized chromatographic conditions the minimum detectable amount (Q_º) for a mass flow sensitive detector increases proportionally to the square of the column diameter for P = 1. In the situation of greater interest in the practice of open tubular gas chromatography where P is large, a linear relationship is derived between Q_º and the column diameter. It is a widespread misunderstanding, however, that narrow bore capillary columns should be used for this reason in trace analysis. If a fixed relative contribution of the injection band width to the overall peak variance is allowed, a decreased plate height drastically restricts the maximum sample volume to be injected. It is shown that the minimum analyte concentration in the injected sample (C_º) is inversely proportional to the column inner diameter when a mass flow sensitive detector is used. For actual concentrations less than C_º, sample preconcentration is required. The effect of peak resolution and selectivity of the stationary phase in relation to C_º and Q_º will be discussed as well. The validity of the given theory is experimentally investigated. Minimum analyte concentrations and minimum detectable amounts are compared using columns with different inner diameter.     

Influence of mobile phase composition on retention factors in different HPLC systems with chemically bonded stationary phases

The influence of mobile phase composition on the retention of selected test analytes in different normal- and reversed-phase chromatographic systems is studied. A novel adsorption model for an accurate prediction of the analyte retention in the column chromatography with binary mobile phase is proposed. Performance of the model is compared with the retention model reported in the literature. Both models are verified for different HPLC systems by use of three criteria: (a). the sum of squared differences between the experimental and theoretical data, (b). approximation of the standard deviation, and (c). the Fisher test.     

The Effect of Column and Eluent Fluorination on the Retention and Separation of non-Fluorinated Amino Acids and Proteins by HPLC

The effect of column and eluent fluorination on the retention and separation of non-fluorinated amino acids and proteins in HPLC is investigated. A side-by-side comparison of fluorocarbon column and eluents (F-column and F-eluents) with their hydrocarbon counterparts (H-column and H-eluents) in the separation of a group of 33 analytes, including 30 amino acids and 3 proteins, is conducted. The H-column and the F-column contain the n-C₈H₁₇ group and n-C₈F₁₇ group, respectively, in their stationary phases. The H-eluents include ethanol (EtOH) and isopropanol (ISP) while the F-eluents include trifluoroethanol (TFE) and hexafluorosopropanol (HFIP). The 2 columns and 4 eluents generated 8 (column, eluent) pairs that produce 264 retention time data points for the 33 analytes. A statistical analysis of the retention time data reveals that although the H-column is better than the F-column in analyte separation and H-eluents are better than F-eluents in analyte retention, the more critical factor is the proper pairing of column with eluent. Among the conditions explored in this project, optimal retention and separation is achieved when the fluorocarbon column is paired with ethanol, even though TFE is the most polar one among the 4 eluents. This result shows fluorocarbon columns have much potential in chromatographic analysis and separation of non-fluorinated amino acids and proteins.