Advantages of LC–MS–MS compared to LC–MS for the determination of nitrofuran residues in honey

In the framework of developing analyses for exogenous contaminants in food matrices such as honey, we have compared data obtained by high-performance liquid chromatography coupled with mass spectrometry (LC–MS) to those provided by high-performance liquid chromatography and tandem mass spectrometry (LC–MS–MS). Initial results obtained with LC–MS showed that the technique lacked selectivity, which is why the method was validated by LC–MS–MS. This method involves a solid-phase extraction (SPE) of nitrofuran metabolites and nitrofuran parent drugs, a derivatization by 2-nitrobenzaldehyde for 17 h, and finally a clean-up by SPE. The data obtained show that the limits of detection varied between 0.2 and 0.6 μg kg⁻¹ for the metabolites and between 1 and 2 μg kg⁻¹ for nitrofuran parent drugs. The method was applied to different flower honeys. The results showed that nitrofurans (used as antibiotics) are consistently present in this matrix, the predominant compound being furazolidone. Figure Working bees     

Comparison of liquid chromatography-isotope ratio mass spectrometry (LC/IRMS) and gas chromatography-combustion-isotope ratio mass spectrometry (GC/C/IRMS) for the determination of collagen amino acid δ13C values for palaeodietary and palaeoecological reconstruction

Results are presented of a comparison of the amino acid (AA) δ(13)C values obtained by gas chromatography-combustion-isotope ratio mass spectrometry (GC/C/IRMS) and liquid chromatography-isotope ratio mass spectrometry (LC/IRMS). Although the primary focus was the compound-specific stable carbon isotope analysis of bone collagen AAs, because of its growing application for palaeodietary and palaeoecological reconstruction, the results are relevant to any field where AA δ(13)C values are required. We compare LC/IRMS with the most up-to-date GC/C/IRMS method using N-acetyl methyl ester (NACME) AA derivatives. This comparison involves the analysis of standard AAs and hydrolysates of archaeological human bone collagen, which have been previously investigated as N-trifluoroacetyl isopropyl esters (TFA/IP). It was observed that, although GC/C/IRMS analyses required less sample, LC/IRMS permitted the analysis of a wider range of AAs, particularly those not amenable to GC analysis (e.g. arginine). Accordingly, reconstructed bulk δ(13)C values based on LC/IRMS-derived δ(13)C values were closer to the EA/IRMS-derived δ(13)C values than those based on GC/C/IRMS values. The analytical errors for LC/IRMS AA δ(13)C values were lower than GC/C/IRMS determinations. Inconsistencies in the δ(13)C values of the TFA/IP derivatives compared with the NACME- and LC/IRMS-derived δ(13)C values suggest inherent problems with the use of TFA/IP derivatives, resulting from: (i) inefficient sample combustion, and/or (ii) differences in the intra-molecular distribution of δ(13)C values between AAs, which are manifested by incomplete combustion. Close similarities between the NACME AA δ(13)C values and the LC/IRMS-derived δ(13)C values suggest that the TFA/IP derivatives should be abandoned for the natural abundance determinations of AA δ(13)C values.     

Liquid chromatography/isotope ratio mass spectrometry measurement of δ13C of amino acids in plant proteins

In archaeological studies, the isotopic enrichment values of carbon and nitrogen in bone collagen give a degree of information on dietary composition. The isotopic enrichments of individual amino acids from bone collagen and dietary protein have the potential to provide more precise information about the components of diet. A limited amount of work has been done on this, although the reliability of these studies is potentially limited by fractionation arising through hydrolysis of whole plant tissue (where reaction between amino acids and carbohydrates may occur) and, for certain amino acids, the use of derivatives (particularly trifluoroacetyl derivatives) for gas chromatography/isotope ratio mass spectrometry (GC/IRMS) analysis. The present study takes the approach of extracting the protein components of plant tissues before hydrolysis and using liquid chromatography/isotope ratio mass spectrometry (LC/IRMS), which does not require derivatisation, for measurement of the isotopic enrichment of the amino acids. The protocol developed offers a methodology for consistent measurement of the δ(13)C values of amino acids, allowing isotopic differences between the individual amino acids from different plant tissues to be identified. In particular, there are highly significant differences between leaf and seed protein amino acids (leaf minus grain) in the cases of threonine (-4.1‰), aspartic acid (+3.5‰) and serine (-3.2‰). In addition to its intended application in archaeology, the technique will be of value in the fields of plant sciences, nutrition and environmental food-web studies.     

Investigation of Pd content in C–Pd films for hydrogen sensor applications

Nanocomposite carbonaceous-palladium (Nc-C-Pd) films were synthesized by physical vapor deposition method (PVD). Scanning electron microscopy studies showed that they were composed of carbonaceous matrix containing Pd nanograins. Nc-C-Pd films were also characterized by thermogravimetric analysis, X-ray powder diffraction, and Fourier transform infrared (FTIR) spectral analysis. The content of Pd in films synthesized at different PVD conditions was determined based on TG measurements. Technological parameters of PVD process affected C/Pd ratio. FTIR spectra exhibited characteristic absorption bands for the precursors of carbonaceous-palladium samples (fullerene C₆₀ and palladium acetate). The influence of hydrogen on electrical properties of the films was tested by measuring their resistance in the presence of hydrogen (1% H₂/N₂).     

Estimation of uncertainty in measurement of boron in Zr–Nb alloy samples by BF4 − ion selective electrode

Boron doped zirconium–niobium alloy is employed for neutron reactivity control in advanced nuclear reactors. An accurate knowledge of the boron content and uncertainty associated with the measurement result is essential for reactivity calculations. In view of the refractory nature of the alloy, boron determination in these matrices is a challenging task for analytical chemists. Also due to non-availability of matrix-matched reference materials, direct solid analysis cannot be resorted to. With this in view, a simple and sensitive method based on potentiometric determination of boron as tetrafluoroborate with tetrafluoroborate ion selective electrode has been developed. After dissolving the sample, boron was quantitatively converted to BF₄ ⁻ with the addition of HF. Potential response was measured with Orion 9305 BN BF₄ ⁻ ion selective electrode. The response of the ion selective electrode was Nernstian in the range of 0.1–100.0 μg/g of boron in the solution. The method has been validated by two independent methods namely spectrophotometry and inductively coupled plasma-atomic emission spectrometry (ICP-AES). All identifiable sources of uncertainties in the methodology have been individually assessed. The combined uncertainty is calculated employing uncertainty propagation law. The expanded relative uncertainty in the measurement (coverage factor 2) is 6.50%.     

Liquid–liquid microextraction in a multicommuted flow system for direct spectrophotometric determination of iodine value in biodiesel

A flow-based procedure was developed for the direct spectrophotometric determination of the iodine value (IV) in biodiesel. The procedure was based on the microextraction/reaction of unsaturated compounds with triiodide ions in an aqueous medium by inserting the reagent solution between the aliquots of biodiesel without any pretreatment. The interaction occurred through the biodiesel film formed on the inner walls of the hydrophobic tube used as the reactor and at the aqueous/biodiesel interfaces. The spectrophotometric detection was based on the discoloration of the I₃⁻ reagent in the aqueous phase by using a glass tube coupled to a fiber-optic spectrophotometer as the detection cell. Reference solutions were prepared by dilution of biodiesel samples with previously determined IV in hexane. The analytical response was linear for IV from 13 to 135 g I₂/100 g with a detection limit of 5 g I₂/100 g. A coefficient of variation of 1.7% (n = 10) and a sampling rate of 108 determinations per hour were achieved by consuming 224 μL of the sample and 200 μg of I₂ per determination. The slopes of analytical curves obtained with three different biodiesel samples were in agreement (variations in slopes lower than 3.1%), thus indicating an absence of any matrix effects. Results for biodiesel samples from different sources agreed with the volumetric official procedure at the 95% confidence level. The proposed procedure is therefore a simple, fast, and reliable alternative for estimating the iodine value of biodiesel.     

Coacervative microextraction ultrasound-assisted back-extraction technique for determination of organophosphates pesticides in honey samples by gas chromatography–mass spectrometry

Coacervative microextraction ultrasound-assisted back-extraction technique (CME-UABE) is proposed for the first time for extracting and preconcentrating organophosphates pesticides (OPPs) from honey samples prior to gas chromatography–mass spectrometry (GC–MS) analysis. The extraction/preconcentration technique is supported on the micellar organized medium based on non-ionic surfactant. To enable coupling the proposed technique with GC, it was required to back extract the analytes into hexane. Several variables including, surfactant type and concentration, equilibration temperature and time, matrix modifiers, pH and buffers nature were studied and optimized over the relative response of the analytes. The best working conditions were as follows: an aliquot of 10 mL 50 g L⁻¹ honey blend solution was conditioned by adding 100 μL 0.1 mol L⁻¹ hydrochloric acid (pH 2) and finally extracted with 100 μL Triton X-114 100 g L⁻¹ at 85 °C for 5 min using CME technique. Under optimal experimental conditions, the enrichment factor (EF) was 167 and limits of detection (LODs), calculated as three times the signal-to-noise ratio (S/N = 3), ranged between 0.03 and 0.47 ng g⁻¹. The method precision was evaluated over five replicates at 1 ng g⁻¹ with RSDs ≤9.5%. The calibration graphs were linear within the concentration range of 0.3–1000 ng g⁻¹ for chlorpirifos; and 1–1000 ng g⁻¹ for fenitrothion, parathion and methidathion, respectively. The coefficients of correlation were ≥0.9992. Validation of the methodology was performed by standard addition method at two concentration levels (2 and 20 ng g⁻¹). The recoveries were ≥90%, indicating satisfactory robustness of the methodology, which could be successfully applied for determination of OPPs in honey samples of different Argentinean regions. Two of the analyzed samples showed levels of methidathion ranged between 1.2 and 2.3 ng g⁻¹.     

Novel concept for the mass spectrometric determination of absolute isotopic abundances with improved measurement uncertainty: Part 1 – theoretical derivation and feasibility study

The development of a new method for the experimental determination of absolute isotopic abundances using a modified isotope dilution mass spectrometry (IDMS) technique is described. The intention and thus main application will be the quantification of molar masses M of highly enriched materials with improved measurement uncertainty (U_rel(M) ≈ 10^?8 with k = 2). In part 1 of the current work, the theoretical foundation of the new method and its mathematical derivation is shown in detail, while part 2 will cover the experiments based on the new method described. Its core idea is the introduction of a virtual element (VE) consisting of all isotopes but the one having the largest or smallest abundance. IDMS is used to determine the mass fraction of this VE in its matrix, namely the element itself. A new set of equations serve to calculate all isotopic abundances (even the large one omitted with the introduction of the VE) merely from the mass fraction of the VE. A comprehensive uncertainty budget according to the Guide to the Expression of Uncertainty in Measurement (GUM) was set up in order to discuss and validate the novel concept. The hypothetical input data of the uncertainty budget were estimated to resemble a silicon material highly enriched with respect to ²⁸Si used in the context of the international Avogadro Project. Considering the calculated results, the experimental determination of the molar mass of the above mentioned silicon seems very promising. As far as the authors know, this will be the first time IDMS was applied to determine a molar mass.     

A confirmatory method for the determination of phenolic endocrine disruptors in honey using restricted-access material–liquid chromatography–tandem mass spectrometry

The present work describes the development and validation of an analytical method based on liquid chromatography (LC), coupled with tandem mass spectrometry (MS/MS) that allows the determination and confirmation of several endocrine-disrupting chemicals (EDCs) in honey. The EDCs studied were nine phenols of different nature: chlorophenols (2,4-dichlorophenol, 2,4,5-trichlorophenol, and pentachlorophenol), alkylphenols (4-tert-butylphenol, 4-tert-octylphenol, and 4-n-octylphenol) bisphenols (bisphenol-A and bisphenol-F), and 4-tert-butylbenzoic acid. The method incorporates a restricted-access material (RAM), coupled on-line to the LC-MS/MS system, which allows direct injection of the matrix into the RAM-LC-MS/MS system. The optimized method developed, RAM-LC-MS/MS, was applied to fortified honey samples, affording detection limits in the 0.6–7.2 ng g⁻¹ range, calculated for a signal-to-noise ratio of 3. In addition, the method was validated as a quantitative confirmatory method according to European Union Decision 2002/657/EC. The validation criteria evaluated were linearity, repeatability, reproducibility, recovery, decision limits, detection capabilities, specificity, and ruggedness. Repeatability and within-laboratory reproducibility were evaluated at two concentration levels, being ±11% or below at 20 ng g⁻¹. The decision limits (CC_α) and detection capabilities (CC_β) were in the 1.7–12.6 and 2.8–21.6 ng g⁻¹ range, respectively.     

Sequence determination and resonance assignments of an Azomonas siderophore using 13C natural abundance 13C–1H HNCA experiment

The determination of the amino acid sequence of small peptides as siderophores is commonly performed using long-range HMBC correlation experiments. However, this type of experiment can lead to ambiguities in the assignment resulting in erroneous primary sequence determination. In this paper, we propose to use an HNCA type experiment on a ¹⁵N-labelled sample in order to avoid these ambiguities. This experiment was successfully used to determine the primary sequence of azoverdin, a siderophore produced by Azomonas.     

Exploiting adsorption and desorption at solid–liquid interface for the fluorometric monitoring of glibenclamide in adulterated drinks

Nowadays, the use of a drug to modify a person's behavior with criminal intentions has become a growing public concern. In fact, stealthy drink spiking with certain drugs can cause the incapacitation of a potential victim of assault and in extreme cases can even lead to death. Belonging to the group of drugs used to commit drug-facilitated crimes is glibenclamide, which not only exhibits high sedation secondary effects but when subject to an overdose intake can lead to intense hypoglycemic episodes that could end with death. Suicide attempts and homicides through overdose with glibenclamide have already been reported.     

Rapid and cost-effective LC–MS/MS method for determination of hydroxycitric acid in plasma: Application in the determination of pharmacokinetics in commercial Garcinia preparations

Garcinia cambogia is one of the most commonly used anti-obesity dietary supplements, and hydroxycitric acid (HCA) is a major constituent in the commercial preparations of Garcinia. High doses of HCA are often consumed without much awareness of its pharmacokinetic and toxicokinetic parameters, and therefore, a complete understanding of its effects is lacking. The first step in understanding these parameters is the availability of a reliable bioanalytical method. Here, we present the first report on a UPLC–MS/MS method for analysis of HCA in rat plasma after a simplified and cost-effective protein precipitation. Chromatographic separation of the analytes in the supernatant was achieved using hydrophilic interaction liquid chromatography, where mass parameters were optimized and a rapid 5-min quantitative assay was developed. The method was highly sensitive, accurate, precise and linear in the concentration range of 10.5–5000 ng/mL (validated according to the United States Food and Drug Administration guidelines). Further, the method was successfully used to describe the pharmacokinetic profile of HCA in rat plasma after the administration of pure HCA and commercial Garcinia preparations.     

HPLC–based methods for the determination of levetiracetam in biological and pharmaceutical samples

Levetiracetam is one of the new generation anti–epileptic agents (also known as anticonvulsants or antiseizure drugs). Following its approval for marketing in 2000, levetiracetam has been widely used in the treatment of epilepsy due to its broad spectrum effects. One of the advantages of this antiseizure drug is its rapid and complete absorption after oral administration. It has also minimal drug–drug and food interactions, and shows more than 95% bioavailability. The determination of levetiracetam in various samples is carried out using several analytical methods including HPLC–based methods. HPLC–based methods are used for different pharmaceutical analyses and play an important role in drug monitoring during patient follow–ups. This review provides a summary of the HPLC–based methods used in the determination and quantification of levetiracetam in biological fluids and pharmaceutical preparations.     

Novel concept for the mass spectrometric determination of absolute isotopic abundances with improved measurement uncertainty: Part 2 – Development of an experimental procedure for the determination of the molar mass of silicon using MC-ICP-MS

The isotopic abundances and thus molar mass M(Si) of a silicon crystal material with natural isotopic abundances have been measured for the first time using multicollector-ICP-mass spectrometry (MC-ICP-MS) in combination with a novel concept of a modified isotope dilution mass spectrometry (IDMS)-method. This experimental work is the further development of part 1 of this series of papers. While part 1 describes the theoretical background and the mathematical derivation of the novel concept in detail, the measurements presented here serve to validate the novel concept and give experimental proof of its capability. Moreover, the also new method for the analytical calculation of calibration factors needed in the determination of absolute isotope amount ratios has been tested successfully. Silicon isotopic abundances have been measured directly from an aqueous alkaline matrix following a new sample preparation protocol developed within the framework of this study. A molar mass of M(Si) = 28.08548(13) g/mol with an associated relative uncertainty of u_rel = 4.6 × 10^?6 (k = 1) has been measured. This is in excellent agreement with the current IUPAC value for the molar mass of natural silicon M(Si_nat) = 28.08550(15) g/mol with u_rel = 5.3 × 10^?6 (k = 1). An uncertainty budget according to the Guide to the Expression of Uncertainty in Measurement (GUM) was calculated to assess the presented results and to validate the novel concept with the help of experimental data. The development of a new experimental procedure is presented in detail and the contributions to the uncertainty are discussed in comparison to part 1 of this work.     

Estimation of measurement uncertainty of pesticides,polychlorinated biphenyls and polyaromatic hydrocarbons in sediments by using gas chromatography–mass spectrometry

The evaluation of the uncertainty associated to analytical methods is essential in order to demonstrate quality of a result. However, there is often lack of information about uncertainty of methods to estimate persistent organic pollutants concentration in complex matrix. Current work has thoroughly evaluated uncertainty associated to quantification of several organochloride pesticides, PCBs and PAHs in sediments. A discussion of the main contributions to the overall uncertainty is reported, allowing authors to establish the accuracy of results and plan future improvements. Combined uncertainties ranged between 5–9% (pesticides), 4–7% (PCBs) and 5–10% (PAHs), being uncertainty derived of calibration the main contribution. Also, the analytical procedure was validated analysing a standard reference material (IAEA-408).     

Rapid and simple method for determination of hexabromocyclododecanes and other LC–MS–MS-amenable brominated flame retardants in fish

In this study, a novel analytical approach for simultaneous determination of hexabromocyclododecane isomers (HBCDs), tetrabromobisphenol A (TBBPA), three brominated phenols, and four hydroxylated derivatives of polybrominated diphenyl ethers (OH-PBDEs) was developed and validated for muscle tissue of both lean and fatty fish. The rapid, simple, and high-throughput sample-preparation procedure was based on acetonitrile extraction then purification by dispersive solid-phase extraction (d-SPE) with a combination of C₁₈ and primary–secondary amine (PSA) sorbents. Ultra-high performance liquid chromatography (UHPLC) coupled to tandem mass spectrometry (MS–MS) was used for identification and quantification of the analytes. Method recovery for both matrices ranged from 80 to 115 % with relative standard deviations (RSDs) <13 % for all analytes. Limits of quantification (LOQs) were in the range 0.1–1 μg kg^?1 wet weight. The validated method was used for analysis of brominated compounds in 32 fish and five bivalve samples collected from different European markets within the monitoring survey organized in the framework of the CONffIDENCE project. Of the 12 targeted analytes, only α-HBCD, 2,4-dibromophenol (2,4-DBP), and 2,4,6-tribromophenol (2,4,6-TBP) were quantified in the samples. α-HBCD was found in six fish samples (herring and mackerel) in the range of 0.8–2.5 μg kg^?1 wet weight. 2,4-DBP and 2,4,6-TBP were found in three blue mussel samples in the range of 19.6–43.5 and 2.3–7.5 μg kg^?1 wet weight, respectively.