Strategies for the screening of antibiotic residues in eggs: comparison of the validation of the classical microbiological method with an immunobiosensor method

ABSTRACT

Efficient screening methods are needed to control antibiotic residues in eggs. A microbiological kit (Explorer® 2.0 test (Zeu Inmunotech, Spain)) and an immunobiosensor kit (Microarray II (AM® II) on Evidence Investigator? system (Randox, UK)) have been evaluated and validated for screening of antibiotic residues in eggs, according to the European decision EC/2002/657 and to the European guideline for the validation of screening methods. The e-reader? system, a new automatic incubator/reading system, was coupled to the Explorer 2.0 test. The AM II kit can detect residues of six different families of antibiotics in different matrices including eggs. For both tests, a different liquid/liquid extraction of eggs had to be developed. Specificities of the Explorer 2.0 and AM II kit were equal to 8% and 0% respectively. The detection capabilities were determined for 19 antibiotics, with representatives from different families, for Explorer 2.0 and 12 antibiotics for the AM II kit. For the nine antibiotics having a maximum residue limit (MRL) in eggs, the detection capabilities CCβ of Explorer 2.0 were below the MRL for four antibiotics, equal to the MRL for two antibiotics and between 1 and 1.5 MRLs for the three remaining antibiotics (tetracyclines). For the antibiotics from other families, the detection capabilities were low for beta-lactams and sulfonamides and satisfactory for dihydrostreptomycin (DHS) and fluoroquinolones, which are usually difficult to detect with microbiological tests. The CCβ values of the AM II kit were much lower than the respective MRLs for three detected antibiotics (tetracycline, oxytetracycline, tylosin). Concerning the nine other antibiotics, the detection capabilities determined were low. The highest CCβ was obtained for streptomycin (100 µg kg^–1).     

Evaluation and validation of a multi-residue method based on biochip technology for the simultaneous screening of six families of antibiotics in muscle and aquaculture products

The Evidence Investigator? system (Randox, UK) is a biochip and semi-automated system. The microarray kit II (AM II) is capable of detecting several compounds belonging to different families of antibiotics: quinolones, ceftiofur, thiamphenicol, streptomycin, tylosin and tetracyclines. The performance of this innovative system was evaluated for the detection of antibiotic residues in new matrices, in muscle of different animal species and in aquaculture products. The method was validated according to the European Decision No. EC/2002/657 and the European guideline for the validation of screening methods, which represents a complete initial validation. The false-positive rate was equal to 0% in muscle and in aquaculture products. The detection capabilities CCβ for 12 validated antibiotics (enrofloxacin, difloxacin, ceftiofur, desfuroyl ceftiofur cysteine disulfide, thiamphenicol, florfenicol, tylosin, tilmicosin, streptomycin, dihydrostreptomycin, tetracycline, doxycycline) were all lower than the respective maximum residue limits (MRLs) in muscle from different animal origins (bovine, ovine, porcine, poultry). No cross-reactions were observed with other antibiotics, neither with the six detected families nor with other families of antibiotics. The AM II kit could be applied to aquaculture products but with higher detection capabilities from those in muscle. The detection capabilities CCβ in aquaculture products were respectively at 0.25, 0.10 and 0.5 of the respective MRL in aquaculture products for enrofloxacin, tylosin and oxytetracycline. The performance of the AM II kit has been compared with other screening methods and with the performance characteristics previously determined in honey.     

A microbiological inhibition method for the rapid,broad-spectrum,and high-throughput screening of 34 antibiotic residues in milk

In this study, we developed a microbiological inhibition method for the rapid screening of antibiotics in milk with Geobacillus stearothermophilus ATCC12980 as an indicator bacterium and an easy sample pretreatment. We observed that the limits of detection of the kit for 34 common antibiotic residues in milk, including β-lactams (13), aminoglycosides (6), tetracyclines (4), sulfonamides (6), macrolides (4), lincosamides (1), were lower than or close to the maximum residue limits formulated by the European Union and China. Moreover, the false-positive rate was 1% and the false-negative rates were less than 5%. The ruggedness of the method (the reproducibility of detection capability of different batches of medium) met requirements at determined levels and residual limits. The shelf life of the kit was more than 6 mo at 4°C. Additionally, we observed good correlations between the kit results and ultra-high-performance liquid chromatography-tandem mass spectrometry results for incurred milk (samples taken from animals treated with antibiotics according to the pre-slaughter medication data), which indicated that the kit was reliable for screening antibiotics in incurred samples. In conclusion, the kit has a broad application potential with high sensitivity, specificity, and reproducibility, stability, and reliability, combined with simple operation, low cost, and high-throughput capacity.     

Multiplex immunoassay based on biochip technology for the screening of antibiotic residues in milk: validation according to the European guideline

ABSTRACT

The Infiniplex for milk® (IPM) kit is a quick method for the simultaneous and qualitative detection of more than 100 molecules including antibiotic residues, mycotoxins, anti-inflammatories and antiparasitic drugs into a single test that does not require milk treatment.

The IPM® kit was validated according to the European decision EC/2002/657 and according to the European guideline for the validation of screening methods (2010). Our validation was focused only on antibiotic residues. The washing step was identified as the most critical step of the assay. Insufficient washes could cause a significant background noise that prevents imaging. Positive controls have to be freshly prepared each day (insufficient stability).

The method was specific with a low false-positive rate of 1.7% on 5 discrete test regions (DTR) ((beta-lactams, lincomycin, virginiamycin, quinolones and sulphonamides)) and a false-positive rate of 0% on the 26 other DTR. During our validation, the 42 determined detection capabilities CCβ for 12 antibiotic families (aminoglycosides, cephalosporins, lincosamides, macrolides, miscellaneous antibiotics, penicillins, phenolated polymixins, polypeptide antibiotics, quinolones, sulphonamides, tetracyclines) were at between once and twice the decision levels stated by the manufacturer. Forty CCβ determined were lower than the respective regulatory limits (i.e. MRL, RC, MRPL) in milk, except for tilmicosin (1.5 times the MRL) and neospiramycin (>1.25 times the MRL). The estimated CCβ of thiamphenicol, cloxacillin, danofloxacin, sulphathiazol, ceftiofur and sulphamonomethoxine were lower than or at the MRL. However, it was difficult to approach an accurate CCβ with only qualitative results. It is impossible to know whether or not we were close to the cut-off value. The software could be improved by differentiating between low-positive and high-positive results. The results of our participation in three qualitative proficiency tests in 2016 and 2017 for the detection of quinolones, tetracyclines and sulphonamides in cows’ milk were very satisfactory.     

Rapid multi-residue and multi-class qualitative screening for veterinary drugs in foods of animal origin by UHPLC-MS/MS

Multi-class UHPLC-MS/MS was developed for the analysis of more than 160 regulated or banned compounds of various classes: anthelmintics including benzimidazoles, avermectins and others; antibiotics including amphenicols, beta-lactams, macrolides, pyrimidines, quinolones, sulphonamides and tetracyclines; beta-agonists; corticosteroids; ionophores; nitroimidazoles; non-steroidal anti-inflammatory agents; steroids; and tranquillisers. Samples were extracted with acetonitrile, without any additional purification step, and analysed by using UHPLC-MS/MS. Validation was done in accordance with the guidelines laid down by European Commission Decision 2002/657/EC for qualitative screening methods. This simple method proved applicable to routine screening for residues in egg, honey, milk and muscle samples at half the maximum concentration permitted by the European Union for each drug. In most cases, the target value was set at 5?µg?kg^?1 for unauthorised compounds.     

Determination of Antimicrobial Residues in Honey by Liquid Chromatography Tandem Mass Spectrometry

Antibiotics are generally used worldwide against bacterial diseases in the treatment of food-producing animals. Since the residues of active agents or their metabolites can appear in these foods, the European Union, for instance, has set maximum residue limit concentrations for authorised veterinary drugs in foodstuffs. However, as yet, regulatory limits have not been established for honey and thus far, only recommendations exist. The aim of this study is to present a multiscreening method for residues in honey for the determination of 36 antimicrobial residues associated with several antibiotics of the B1 group (sulfonamides, trimethoprim, aminoglycosides, tetracyclines, quinolones and lincomycin) as well as the antibiotic griseofulvin. During the screening analysis, samples are hydrolysed in an acidified medium, purified on polymeric solid-phase extraction cartridges and subsequently analysed by reversed phase ion pair liquid chromatography tandem mass spectrometry. The liquid chromatographic separation was optimised by computer simulation with DryLab software. The positive identification of target compounds in suspicious samples was confirmed using earlier developed antibiotic class specific methods of which the aminoglycoside method is herein described in detail. The developed approaches were then applied to samples in the national monitoring program after their successful validation. Moreover, the screening and confirmatory methods were applied to proficiency test samples resulting in satisfactory identification and quantification. However, the analysis of real samples revealed that co-eluting target compounds can have considerable influence on the accuracy of this semi-quantitative multiscreening method.     

Residues of antibiotics and sulfonamides in honeys from Basque Country (NE Spain)

BACKGROUND: The aim of this work was to ensure that Label Basque market honey is free of veterinary residues. RESULTS: A total of 567 Basque honey samples were previously analyzed with the respective Charm II system—68 samples were presumptive positive for sulfonamides (SA‐s), 24 samples for tetracyclines (TC‐s), and no positive samples for chloramphenicol (CAP) (<0.3 µg kg^?1) residues. The residues were mostly confirmed by liquid chromatography fluorescence detection (LC‐FD) and tandem mass spectrometry (LC‐MS/MS), according to the latest European Union criteria for the analyses of veterinary drug residues (2002/657/EC). These techniques confirmed that 19 of the 68 samples, presumptive contaminated with SA‐s, contained sulfathiazole (STZ) residues at levels from 20 to 210 µg kg^?1, and the 24 samples presumptive contaminated with TC‐s, were also confirmed, showing tetracycline (TC) levels from 15 to 920 µg kg^?1. Linearity range, decision limit (CCα), detection capability (CCβ), precision and reproducibility were also determined. CONCLUSION: Residues of veterinary drugs were confirmed in a very limited number of honey samples: sulfathiazole (3.40%) and tetracycline (4.22%). This work reports the advantages of the Charm II assay, but also its limitations, detecting SA‐s in most (87.7%) of the heather (Erica vagans) honey samples. The false positives detected in this honey were assumed to be of an unknown compound that has not been confirmed as a drug residue. Until now, no studies have been performed to find out if other heather honeys of different geographical origins give similar false positives for SA‐s. Copyright © 2008 Society of Chemical Industry     

Validation of a commercial receptor kit Sulfasensor Honey for the screening of sulfonamides in honey according to Commission Decision 2002/657/EC

The Sulfasensor Honey kit is a receptor test dedicated to the screening of sulphonamide residues respectively in different matrices. The aim of this project was to evaluate and validate this kit according to the Community Reference Laboratory (CRL) guideline for the validation of screening methods to achieve the French control plan for honey. The test is robust, quick (90 min for 40 samples), easy to perform and easy to read. The false-positive rate was estimated to be 12.5%. The detection capabilities CCβ of the kit were lower than or equal to 25 μg kg(-1) for sulfamethazine, sulfamerazine, sulfathiazole and sulfapyridine, and between 25 and 50 μg kg(-1) for sulfadiazine and sulfadimethoxine, 150 μg kg(-1) for sulfaquinoxaline, and 1000 μg kg(-1) for sulfamethoxazole and sulfamethizole. Sulfanilamide was not detected by the kit. The kit was applicable to a wide variety of honeys (different floral and geographical origins, liquid or solid). This kit was used to implement the French control plan for the detection of antibiotic residues in honey in 2010 in parallel with an HPLC method. However, in 2011 the kit was replaced by an LC-MS/MS method for the screening and confirmation of sulfonamide residues in honey, which detects all the sulfonamides of interest.     

A new strategy for the analysis of tetracycline residues in foodstuffs by a surface plasmon resonance biosensor

A new strategy was developed for the establishment of an indirect tetracycline assay using surface plasmon resonance (SPR). The principle for the assay is based on the most important resistance mechanism against tetracycline in gram-negative bacteria. Tetracyclines release the 46.6 kDa Tet repressor protein (TetR) from the tet operator (tetO), a biotinylated short double strand DNA sequence bound to a streptavidin biosensor chip. Tetracyclines present in a sample solution bind to the repressor protein, inducing a conformational change accompanied with a reduction of the affinity constant of TetR to tetO. We were able to quantify tetracycline residues in spiked raw milk samples in concentrations corresponding to the maximum residue limit (MRL) set by the European Union. Honey samples could also be analysed but with lower sensitivity. The assay detects seven of the most commonly used tetracyclines in veterinary medicine. Nine antibiotics of five other antibiotic classes were tested and no interference with the SPR assay was found. Thus, the described principle forms the basis for screening assays to routinely test for tetracycline residues in foodstuffs.     

Development of a new screening method for the detection of antibiotic residues in muscle tissues using liquid chromatography and high resolution mass spectrometry with a LC-LTQ-Orbitrap instrument

A liquid chromatography-high resolution mass spectrometry (LC-HRMS) method was developed for screening meat for a wide range of antibiotics used in veterinary medicine. Full-scan mode under high resolution mass spectral conditions using an LTQ-Orbitrap mass spectrometer with resolving power 60,000 full width at half maximum (FWHM) was applied for analysis of the samples. Samples were prepared using two extraction protocols prior to LC-HRMS analysis. The scope of the method focuses on screening the following main families of antibacterial veterinary drugs: penicillins, cephalosporins, sulfonamides, macrolides, tetracyclines, aminoglucosides and quinolones. Compounds were successfully identified in spiked samples from their accurate mass and LC retention times from the acquired full-scan chromatogram. Automated data processing using ToxId software allowed rapid treatment of the data. Analyses of muscle tissues from real samples collected from antibiotic-treated animals was carried out using the above methodology and antibiotic residues were identified unambiguously. Further analysis of the data for real samples allowed the identification of the targeted antibiotic residues but also non-targeted compounds, such as some of their metabolites.     

Optimisation of a new two‐plate screening method for the detection of antibiotic residues in meat

A two‐plate microbiological method to screen residues of the most commonly used antibiotics in animal production, named new two‐plate test (NTPT), has been optimised and validated, according to criteria derived from the European Commission Decision 2002/657/CE. This screening method used two media at different pH seeded with a single bacteria strain (Bacillus subtilis). The method consists of a simple extraction, followed by the application of the extract on Petri plates. The method detected, in pork and chicken muscles, most of the antibiotics from six groups (tetracyclines, (fluoro)quinolones, penicillins, macrolides, aminoglycosides and sulfonamides) and florfenicol at concentration very close to maximum residue limits used in the EU. The screening capacity of the NTPT was compared with another screening technique, the Premi‐Test^®, by analysing spiked samples as well as real samples of meat from pork and chicken sold for local consumption, in the Red River Delta region (Vietnam). The NTPT described here appeared to detect more samples than the Premi‐Test^®, showing its interest for Vietnamese control laboratories, as a screening method to monitor antibiotic residues in chicken and pork meat, before sending the suspected samples to the confirmatory step.     

Validation of two ELISA kits for the screening of tylosin and streptomycin in honey according to the European decision 2002/657/EC

Antibiotics are mixed with the food of bees to fight against diseases. No maximum residue limits have been set for honey. Recommended concentrations (RCs) have been published by European Union Reference Laboratories for tylosin and streptomycin. The objective of this project was to select and validate enzyme-linked immunosorbent assay (ELISA) kits for the screening of tylosin and streptomycin/dihydrostreptomycin residues to be implemented in the French honey control plan. Four ELISA kits for tylosin and five ELISA kits for streptomycin were evaluated. At the end, one kit each was selected and validated for tylosin (TECNA AB620) and streptomycin (Europroxima). Both ELISA kits for tylosin and streptomycin are specific, robust, fast and easy-to-use tests. The detection capability CCβ of tylosin A was less than or equal to 10?µg?kg^?1 (half the RC). The CCβ of desmycosin (the hydrolysed product of tylosin A in acidic conditions) is approximately 200?µg?kg^?1, which is five times the RC for tylosin (20?µg?kg^?1). Thus, this kit is fit for the screening of tylosin A but is unsuitable to detect desmycosin. The detection capability CCβ of streptomycin was less than or equal to 10?µg?kg^?1 (one fourth the RC). The cross-reactivity with dihydrostreptomycin was equal to 136%. Both ELISA kits were applicable to a wide variety of honey (single flower and multiflower, different floral origins, different geographic origins, different consistencies [liquid or solid] and different colours).     

高通量抗生素残留初筛试剂盒的研制及应用

以动物源性食品中常见的单一或配伍使用的抗生素为检测目标,开发基于微生物显色原理的高通量快速检测其残留的初筛试剂盒。选取嗜热脂肪芽孢杆菌（Bacillus sterothermophilus CICC 10392）作为指示菌,优化其微胶囊包埋条件,并固定于96 微孔板中,结合前期研究成果制成可同时对禽畜肉中常见的4 类抗生素进行联合初筛的试剂盒,克服了因菌种活化耗时较长及液体菌种运输困难等问题。结果表明：以0.1 g/mL聚乙烯醇为载体、pH 6.0的硼酸-磷酸盐溶液为交联剂对初始吸光度（A600 nm）为0.8的指示菌进行包埋,其机械强度、细胞活性及检测效果最好;该试剂盒对四环素类检出限为40～60 μg/kg,氨基糖苷类检出限为60～120 μg/kg,大环内酯类检出限为60～100 μg/kg,β-内酰胺类检出限为20～40 μg/kg,四环素与氨基糖苷类配伍使用检出限为20～40 μg/kg,β-内酰胺类与氨基糖苷类配伍使用检出限为10 μg/kg,符合国内外对抗生素残留限量的要求;用色谱法对试剂盒检测的70 份样品进行验证,无假阴性存在,说明该试剂盒结果可靠,可用于动物源性食品中抗生素残留的初筛检测。     

Development and validation of a methodology to qualitatively screening veterinary drugs in porcine muscle via an innovative extraction/clean-up procedure and LC-MS/MS analysis

A qualitative multiresidue method that facilitates rapid monitoring of veterinary drugs in porcine muscle is described. The method comprises the application of an innovative extraction/clean-up procedure, namely liquid–liquid extraction with partition at very low temperature (LLE-FPVLT), and analysis by liquid chromatography coupled to tandem mass spectrometry (LC-MS/MS). Besides the high selectivity, sensitivity and specificity, this high-throughput method proved to be quite general as 34 veterinary drugs (from six distinct classes: tetracyclines, sulfonamides, penicillins, quinolones, macrolides and benzimidazoles) could be successfully detected. The whole screening procedure was validated according to the directives from European Commission Decision 2002/657/EC and guidelines for the validation of screening methods. Acceptable values for the evaluation parameters were achieved for all analytes (except for ampicillin, clindamycin and erythromycin). Finally, these very promising results have strengthened the possibility of inclusion of such a methodology as an integral part of the National Residue Control Plan scope of the Ministry of Agriculture, Livestock and Food Supply of Brazil.     

The Modified New Two Plates Test for Detecting Tetracycline,Beta-Lactam,and Sulfonamide Antibiotic Residues in Kidney and Muscle of Cattle Slaughtered in North-East Benin

In Benin, veterinary antibiotics are widely used for cattle breeding. This livestock contributes to 57% of the locally produced meat. The aim of this study was to assess the impact of the large use of antibiotics by determining the contamination level with antibiotic residues in bovine meat, in North Benin. Kidney and muscle samples taken from 50 bovine carcasses in the 2 main slaughterhouses of Parakou were analyzed for the presence of antibiotic residues by a screening method modified from the “New Two Plates Test” (NTPT), to identify tetracyclines, sulfonamides, and beta-lactam groups of antibiotics. Thirteen kidney and muscle samples were subjected to liquid chromatography coupled to tandem mass spectrometry analysis for the confirmation of tetracycline and sulfonamide residues. After modified NTPT screening, tetracycline residues were identified in 54% of cattle carcasses while beta-lactam and sulfonamide residues were present, respectively, in 2 and 6% of sampled animals. The LC-MS/MS analysis confirmed the presence in the kidney tissue of oxytetracycline, epi-oxytetracycline, tetracycline, and epi-tetracycline at maximum levels, respectively, of 1380, 350, 190, and 230 μg kg^?1. Sulfamethazine residues were confirmed in one of cattle carcass at very high levels of 3900 μg kg^?1 in kidney and 2220 μg kg^?1 in muscle. Antibiotic residue levels were found above the maximum residue limit applied in the European legislation in 38% of the carcasses subjected to the LC-MS/MS analysis. These high levels of contamination with antibiotic residues are a potential threat for the health of consumers, and are of concern regarding the selection of antibiotic-resistant bacteria in animals and humans.     

Determination of Antibiotic Residues in Honey by High-Performance Liquid Chromatography with Electronspray Ionization Tandem Mass Spectrometry

The aim of the present study was to develop a rapid and simple method for the detection and quantification of antibiotic and antibacterial residues in honey using liquid chromatography with electronspray ionization tandem mass spectrometry. Two different extraction methods were used. The first method uses water and 1% formic acid in acetonitrile for the determination of sulfonamides while the second uses phosphate buffer, 10% trichloroacetic acid, and acetonitrile as the extracting solvent for the determination of tetracyclines, amphenicols, fluoroquinolones, penicillin g, trimethoprim, and tiamulin. The multi-residue method was validated in a thyme honey matrix. Thirty-six different antibiotics and residues from four different families (sulfonamides, tetracyclines, amphenicols, fluoroquinolones) and some individual antibiotics (penicillin g, trimethoprim, and tiamulin) were tested in 20 honey samples originating from Cyprus and Greece. The decision limits (CCα) were from 0.1 to 9.2 μg kg^?1; the detection capabilities (CCβ) were from 0.3 to 27.6 μg kg^?1 while recoveries were from to be between 65.0 and 116.1%. The method was successfully applied to commercial samples from different types of honey from Greece and Cyprus. Among them, oxolonic acid, sulfathiazole, and sulfadimethoxine were found in three honey samples. Finally, proficiency testing was applied to the proposed method while analysis of certified samples showed good method performance characteristics.     

Validation of a liquid chromatography-tandem mass spectrometry screening method to monitor 58 antibiotics in milk: a qualitative approach

A multi-residue method was developed for monitoring antibiotic residues in milk using liquid chromatography coupled to a tandem quadrupole mass spectrometer (LC/MS-MS). Two very short extractions followed by two LC/MS-MS acquisitions allowed the screening of 58 antibiotics belonging to eight different families (penicillins, cephalosporins, sulfonamides, macrolides, lincosamides, aminoglycosides, tetracyclines, and quinolones). This method is currently implemented in the laboratory in a qualitative way, i.e. monitoring the presence or absence of residue in a sample and identification of the analyte before the confirmation step. In order to assess the performance of this method, a validation strategy described in an internal guideline for the validation of screening methods was applied. The aim of the validation was to prove sufficient sensitivity of the method to detect all the targeted antibiotics at the level of interest (maximum residue limit, MRL) at least. According to European Commission Decision 2002/657/EC, the suitable sensitivity of a screening method can be demonstrated when the CCβ is below or equal to the MRL and so the false-compliant rate below or equal to 5% at the MRL level. The validation scheme was established in order to take into account various variability factors: the apparatus response, the interday repeatability, the matrix effect, etc. The results of the validation clearly demonstrate the suitability of this method for the detection and identification of more than 50 antibiotics and they are in agreement with the results obtained in routine analysis.     

Development and validation of a methodology to qualitatively screening veterinary drugs in porcine muscle via an innovative extraction/clean-up procedure and LC-MS/MS analysis

A qualitative multiresidue method that facilitates rapid monitoring of veterinary drugs in porcine muscle is described. The method comprises the application of an innovative extraction/clean-up procedure, namely liquid-liquid extraction with partition at very low temperature (LLE-FPVLT), and analysis by liquid chromatography coupled to tandem mass spectrometry (LC-MS/MS). Besides the high selectivity, sensitivity and specificity, this high-throughput method proved to be quite general as 34 veterinary drugs (from six distinct classes: tetracyclines, sulfonamides, penicillins, quinolones, macrolides and benzimidazoles) could be successfully detected. The whole screening procedure was validated according to the directives from European Commission Decision 2002/657/EC and guidelines for the validation of screening methods. Acceptable values for the evaluation parameters were achieved for all analytes (except for ampicillin, clindamycin and erythromycin). Finally, these very promising results have strengthened the possibility of inclusion of such a methodology as an integral part of the National Residue Control Plan scope of the Ministry of Agriculture, Livestock and Food Supply of Brazil.     

Validation of a commercial receptor kit Sulfasensor® Honey for the screening of sulfonamides in honey according to Commission Decision 2002/657/EC

The Sulfasensor® Honey kit is a receptor test dedicated to the screening of sulphonamide residues respectively in different matrices. The aim of this project was to evaluate and validate this kit according to the Community Reference Laboratory (CRL) guideline for the validation of screening methods to achieve the French control plan for honey. The test is robust, quick (90?min for 40 samples), easy to perform and easy to read. The false-positive rate was estimated to be 12.5%. The detection capabilities CCβ of the kit were lower than or equal to 25?µg?kg^?1 for sulfamethazine, sulfamerazine, sulfathiazole and sulfapyridine, and between 25 and 50?µg?kg^?1 for sulfadiazine and sulfadimethoxine, 150?µg?kg^?1 for sulfaquinoxaline, and 1000?µg?kg^?1 for sulfamethoxazole and sulfamethizole. Sulfanilamide was not detected by the kit. The kit was applicable to a wide variety of honeys (different floral and geographical origins, liquid or solid). This kit was used to implement the French control plan for the detection of antibiotic residues in honey in 2010 in parallel with an HPLC method. However, in 2011 the kit was replaced by an LC-MS/MS method for the screening and confirmation of sulfonamide residues in honey, which detects all the sulfonamides of interest.     

Analysis of chloramphenicol in honeys of different geographical origin by liquid chromatography coupled to electrospray ionization tandem mass spectrometry.

A sensitive liquid chromatography tandem mass spectrometry (LC-MS/MS) method was developed to detect trace amounts of the antibiotic chloramphenicol (CAP) in honey. The methodology entailed a solid-phase extraction of aqueous honey solutions followed by liquid-liquid partitioning, filtration and direct injection onto the LC-MS/MS system. Honey extracts were spiked with an isotopically labelled internal standard (d(5)-CAP) to compensate for analyte loss and potential ion suppression during the MS stage. Detection of the analyte was achieved by negative ionization electrospray in the selected reaction monitoring (SAM) mode. For confirmation, four characteristic mass transitions were monitored each for the analyte and the surrogate standard. The method was validated according to the latest European Union criteria for the analyses of veterinary drug residues in food. At all three fortification levels studied (0.1, 0.2, 0.5 microg kg(-1)) the method was accurate to within 15%. The repeatability and within-laboratory reproducibilities were <12 and 18%, respectively. The decision limit (CC alpha) and detection capability (CC beta) were both <0.1 microg kg(-1). The procedure provides a sensitive and reliable method for the determination of residues of chloramphenicol in honey. Numerous raw honeys of various geographical origins were analysed, showing extensive contamination particularly those of Chinese origin.