Análise multirresíduos de pesticidas em tomate utilizando LC-MS/MS e avaliação dos efeitos de lavagem na descontaminação / Multiresidue analysis of pesticides in tomatoes using LC-MS/MS and evaluation of the effects of washing in decontaminating

Graziela Cristina Rossi de Moura Andrade

03 July 2013

Os pesticidas têm sido largamente empregados na agricultura para controle de pragas, doenças e ervas daninhas. O uso intensivo de pesticidas nas culturas de tomates, desrespeitando as boas práticas agrícolas, tem causado preocupações quanto à provável contaminação do produto final e muitos métodos multirresíduos têm sido empregados para avaliar e determinar os níveis de resíduos em amostras de alimentos. Para tanto, o objetivo deste estudo foi a validação do método usando QuEChERS no preparo de amostra e LC-MS/MS para a quantificação de resíduos de 61 pesticidas de diferentes classes químicas em tomate. A detecção foi realizada utilizando espectrômetro de massas no modo MRM dinâmico, o tempo de análise foi de 13 min com coluna analítica recheada com partículas de 1,8 \'mü\'m de partícula. Dos 61 pesticidas estudados, 46 estão de acordo com os parâmetros de validação da Comissão Européia e Anvisa, 15% dos pesticidas validados apresentaram efeito matriz médio e as recuperações ficaram entre 87 e 116% e coeficiente de variação de 5 a 17%. Mais de 85% dos compostos investigados apresentaram limites de detecção igual ou menor que 5 \'mü\'g kg-1 e de quantificação igual ou menor que 10 \'mü\'g kg-1. Foram analisadas 58 amostras de tomate coletadas em supermercados da cidade de Piracicaba, SP, Brasil. Doze compostos foram detectados em trinta e cinco amostras (60% do total analisado), todos abaixo do limite máximo de resíduos permitido no Brasil para acefato, acetamiprido, azoxistrobina, benalaxil, bromuconazol, diflubenzurom, imidacloprido, iprodiona, procloraz e tiametoxam, e 15 amostras positivas para metamidofós e 1 para oxamil, que não possuem uso autorizado para a cultura de tomate. Foi realizado um estudo de lavagem de tomates contaminados com produtos formulados (8 pesticidas) com água, solução com 10% de vinagre e com 10% de bicarbonato de sódio e analisada a casca e polpa, para avaliar a capacidade de remoção de cada procedimento. Todos os tratamentos de lavagens (n=3) diferiram estatisticamente para todos os pesticidas avaliados (n=8), com exceção do fipronil, para o qual as lavagens com solução de 10% de bicarbonato de sódio e água não apresentaram diferença no nível de significância de 5%. A lavagem com água ou outras soluções antes do consumo é indicada para a redução de resíduos de pesticidas em tomate e a retirada da casca também contribui para essa redução / Pesticides have been widely used in agriculture to control pests, diseases and weeds. The intensive use of pesticides in tomato crops disrespecting good agricultural practices have been causing concerns about the possible contamination of the final product and many multiresidue methods have been used in order to evaluate and determine the levels of residues in food samples. Therefore, the aim of this study was validate the method using QuEChERS sample preparation and LC-MS/MS for quantification of 61 pesticides residues from different chemical classes in tomato. Detection was performed using mass spectrometry in dynamic MRM mode, run time had 13 min and analytical column packed with 1,8 \'mü\'m particles. Of the 61 pesticides studied, 46 are in accordance with the validation parameters of the European Commission and ANVISA, 15% of the validated pesticides presented matrix effect, recoveries were between 87 and 116% and coefficient of variation 5 to 17%. More than 85% of the compounds investigated showed limits of detection less or equal than 5 \'mü\'g kg-1 and the limits of quantification less or equal than 10 \'mü\'g kg-1. 58 real samples of tomato were analyzed and collected in supermarkets in Piracicaba, SP, Brazil. Twelve compounds were detected in thirty-five samples (60% of the total analyzed), all below the maximum residue limit allowed in Brazil for acephate, acetamiprid, azoxystrobin, benalaxyl, bromuconazole, diflubenzuron, imidacloprid, iprodione, prochloraz and thiamethoxam, and 15 positive samples of methamidophos and 1 for oxamyl, which are not authorized to use at the culture of tomatoes. A wash study was conducted with spiked tomatoes using formulated products (8 pesticides) with water, 10% acetic acid, 10% sodium bicarbonate solution and analyzed concentration in the peel and pulp, in order to evaluate the capacity to remove pesticides in each procedure. All wash treatments (n= 3) differed significantly for all pesticides evaluated (n= 8), with the exception of fipronil, which the washing with 10% of sodium bicarbonate solution and water no showed difference in the level of significance 5%. The washing with water or other solutions before consumption is indicated for the reduction of pesticide residues in tomatoes and the peeling also contributes to this reduction

LC-ESI-MS/MS

Pesticidas

QuEChERS

Resíduos

Tomate

LC-ESI-MS/MS

Pesticides

QuEChERS

Residues

Tomato

Avaliação do potencial do pólen apícola como bioindicador de contaminação ambiental por agrotóxicos / Evaluation of potencial use of bee pollen as bioinidicator of environmental pesticide contamination

Oliveira, Renata Cabrera de, 1984-

08 August 2014

Orientadores: Susanne Rath, Sonia Claudia do Nascimento de Queiroz / Tese (doutorado) - Universidade Estadual de Campinas, Instituto de Química / Made available in DSpace on 2018-08-26T03:44:24Z (GMT). No. of bitstreams: 1 Oliveira_RenataCabrerade_D.pdf: 3973991 bytes, checksum: 53109a8e29cba1ca926627e521d33fd2 (MD5) Previous issue date: 2014 / Resumo: O uso frequente e indiscriminado de agrotóxicos na agricultura tem acarretado a presença de resíduos nos alimentos e contaminação ambiental, principalmente em países com grande potencial agrícola, como o Brasil. Para avaliar a presença de resíduos de agrotóxicos no ambiente, as abelhas e os produtos apícolas têm sido apontados como potenciais bioindicadores, podendo ser utilizados para monitorar grandes áreas devido às longas distâncias percorridas. Assim sendo, o potencial do uso do pólen apícola como bioindicador da contaminação ambiental por agrotóxicos foi avaliado neste trabalho. Para isso, foi necessário desenvolver e validar um método analítico para determinação de multirresíduos em pólen apícola, utilizando cromatografia a gás acoplada à espectrometria de massas sequencial (GC-MS/MS). Para definição das condições ótimas de extração, dois processos foram avaliados: o QuEChERS, e o de partição com acetonitrila. O QuEChERS mostrou ser mais eficiente (melhor seletividade e eficiência de extração) e foi validado para a determinação de 27 agrotóxicos. Estudos de sorção mostraram que os agrotóxicos são fortemente sorvidos no pólen. Nas amostras provenientes do apiário experimental na Embrapa em Jaguariúna/SP não foram encontrados níveis quantificáveis dos agrotóxicos pesquisados, enquanto a presença de resíduos de agrotóxicos nas amostras fornecidas por apicultores de Ribeirão Preto/SP foi confirmada e quantificada. Os métodos desenvolvidos e validados mostraram ser eficientes e podem ser utilizados no monitoramento ambiental quanto à presença de resíduos de agrotóxicos. Os resultados confirmam o potencial do pólen apícola como bioindicador de contaminação ambiental por agrotóxicos / Abstract: The extensive use of pesticides in agriculture crop has led to the presence of residues in food and environmental contamination, especially in countries with great agricultural potential, such as Brazil. To assess the presence of pesticide residues in the environment, honeybees and bee products have been mentioned as potential bioindicators, which can be used to monitor large areas due to long distances travelled. Therefore, the potential use of bee pollen as a bioindicator of environmental pesticides contamination has been reported in this work. For this it was necessary to develop and validate an analytical method for the determination of multiresidues in pollen, using gas chromatography coupled to tandem mass spectrometry (GC-MS/MS). For the definition of optimum extraction conditions, two procedures were evaluated: QuEChERS, and partition with acetonitrile. The QuEChERS proved to be more efficient (improved selectivity and extraction efficiency), and was validated for the determination of 27 pesticides. Sorption studies showed that pesticides are strongly sorbed in pollen. Unquantifiable levels of pesticides surveyed were found in the samples from experimental apiary at Embrapa in Jaguariúna/SP, while the presence of pesticide residues in samples provided by apiarists from Ribeirão Preto/SP was confirmed and quantified. The validated analytical methods proved to be efficient and can be used in environmental monitoring for the presence of pesticide residues. The results confirm the potential of bee pollen as a bioindicator of environmental pesticides contamination / Doutorado / Quimica Analitica / Doutora em Ciências

Bioindicador

Agrotóxicos

Polen apícola

GC-MS/MS

Bioindicator

Pesticides

Bee pollen

GC-MS/MS

Nova estratégia bioanalítica baseada em cromatografia líquida e espectrometria de massas em tandem para a quantificação de aminoácidos em matrizes biológicas: uma ferramenta clínica e experimental / New bioanalytical strategy based on liquid chromatography and tandem mass spectrometry for amino acids quantification in biological matrices: a clinical and experimental tool.

Jessica Silva Salgueiro

18 December 2015

Apesar da rápida expansão das aplicações da cromatografia líquida acoplada à espectrometria de massas em química clínica, a análise de metabólitos de baixo peso molecular e alta polaridade em matrizes biológicas ainda permanece como um grande desafio analítico. Dentre os compostos de grande importância no diagnóstico de doenças metabólicas que ainda carecem de melhores alternativas bioanalíticas destacam-se os aminoácidos. O presente estudo descreve o desenvolvimento e a validação de um novo método para a quantificação de 24 aminoácidos em plasma explorando a cromatografia líquida acoplada a espectrômetros de massas em tandem. Foi construído um método de detecção baseado em SRM (múltiplas reações selecionadas) com duas transições de massas para cada um dos 24 aminoácidos e os 19 padrões internos marcados com isótopos estáveis. Foram avaliadas três estratégias de separação cromatográfica e o melhor desempenho foi obtido com fase reversa com octadecilsilano (C18) com pareamento iônico com o ácido perfluoropentanoico. O método cromatográfico final permitiu a separação dos 24 aminoácidos, com resolução completa dos isômeros: leucina, isoleucina e allo-isoleucina, em 11 minutos incluindo o tempo de re-estabilização da coluna cromatográfica. Os limites de quantificação variaram em 113 fmol a 6 pmol injetados na coluna cromatográfica. A imprecisão obtida nos níveis testados para todos os aminoácidos foi inferior a 14%. O método apresentou linearidade para os intervalos testados chegando a 1,5 mmol.L-1 para vários compostos. Os ensaios de arraste mostraram que os limites máximos obtidos na linearidade não geram nenhuma interferência subsequente. A exatidão do método foi avaliada com amostras provenientes do programa de referência interlaboratorial European Research Network for evaluation and improvement of screening, Diagnosis and treatment of Inherited disorders of Metabolism (ERNDIM) e com o material de referência certificado do National Institute of Standards and Technology (NIST). Todos os analitos mostraram equivalência estatística com o método desenvolvido. / Despite the widespread use of liquid chromatography coupled to mass spectrometry applications in clinical chemistry, the analysis of low molecular weight and high polar metabolites in biological matrices remains as a major analytical challenge. Notwithstanding the key role played by amino acids in the diagnosis of metabolic diseases, there is still need for improvements in bioanalytical process of these analytes. The present study describes the development and validation of a new method for quantification of 24 amino acids in plasma based on liquid chromatography coupled to tandem mass spectrometry. Detection and quantification were achieved building a selected reaction monitoring method two mass transitions for each 24 amino acids and 19 stable isotope internal standards. Three chromatographic strategies for separation were evaluated, and best performance was achieved using reversed-phase octadecylsilane with perfluropentanoic acid as ion pairing agent. The separation method allowed separation of 24 amino acids with full resolution for isomers leucine, isoleucine and alloisoleucine in 11 minutes, including column equilibration time. The limits of quantification ranged from 113 fmol to 6 pmol (on column injection). Imprecisions for all evaluated levels and amino acids were less than 14%. The method is linear in all clinical intervals and extending up to 1.5 mmol.L-1. Carryover evaluation demonstrated absence of interference in the following injection throughout the analytical interval. Method accuracy was evaluated analyzing reference samples from European Research Network for evaluation and improvement of screening, Diagnosis and treatment of Inherited disorders of Metabolism (ERNDIM) and National Institute of Standards and Technology (NIST). Statistical equivalence was demonstrated for all analytes using the present method.

Aminoácidos

HILIC

LC-MS/MS

Pareamento iônico

Amino acids

HILIC

Ion pairing

LC-MS/MS

Challenge de l’analyse de dangers chimiques à l’état d’ultra-traces en matrices biologiques complexes / Challenge for the analysis of chemical hazard at ultra-traces levels in complex biological matrices

Bichon, Emmanuelle

23 November 2016

L’étude du lien entre l’exposition de l’Homme aux substances chimiques, notamment via son alimentation,et sa santé est un sujet de préoccupation majeure dans notre société qui présente des challenges multiples.Nous nous sommes attelés à l’un d’entre eux par la production de données analytiques fiables relatives à la contamination des denrées alimentaires et des fluides biologiques humains. Le développement de méthodes analytiques reposant sur des technologies en rupture, à même de s’adresser aux paris de la mesure de composés chimiques émergents (e.g. les retardateurs de flamme bromés) ou historiques mais sous le prisme de la sensibilité et du haut débit (e.g. les stéroïdes, les pesticides organochlorés, les dioxines et les polychlorobiphényles) a été au cœur de ce travail. Le couplage GC/APCI/MS sur système triple quadripolaire s’est imposé au cours de nos évaluations. L’association de la chromatographie en phase gazeuse et de l’ionisation chimique à pression atmosphérique a apporté un gain en sélectivité remarquable comparée aux approches traditionnellement retenues dans le domaine et a autorisé l’exploration des ultra-traces dans des matrices biologiques complexes. Cette géométrie nous a permis d’innover en pratiquant des séparations rapides sur colonne capillaire ultra-courte de 2,5 m. La vitesse de balayage et l’excellente sensibilité de l’analyseur de masse nous ont en outre donné accès à une analyse quantitative fiable et multi-paramètres. Ce travail ouvre d’excellentes perspectives vis-à-vis de la production de données d’exposition externe et interne élargies en réponse aux défis à venir entourant la caractérisation de l’exposome Humain. / The study of the link between Human exposure tochemical substances (notably via his food the intake) and Health, is a major concern in our society and poses many challenges. We endeavoured to address one of them by producing reliable analytical data on foodstuffs and human biological fluids contamination. The development of analytical methods based on breakthrough technologies, capable of challenging theemerging (e.g. brominated flame retardants) or historical compounds measurement but through the prism of sensitivity and high throughput (e.g. steroids,organochlorine pesticides, dioxins andpolychlorobiphenyls), was at the heart of our work.Using a GC/APCI/MS with a triple quadripole systememerged as a favorable choice as our evaluations progressed. The association of gas chromatography and atmospheric pressure chemical ionisation brought in a remarkable gain in terms of selectivity, compared to the approaches traditionally selected in this field, andauthorized ultra-trace exploration in complex biologicalmatrices. This geometry allowed us to innovate by performing fast separations on an ultra-short 2.5 mcolumn. Besides, the mass analyser scan speed and high sensitivity gave us access to a reliable and multiparameters quantitative analysis. This work opens up excellent perspectives for the production of expanded external and internal exposure data to meet the future challenges surrounding Human exposome characterisation.

Gc/apci/ms/ms

Dangers chimiques

Stéroïdes

Gc/apci/ms/ms

Chemical hazards

Steroids

TWO-DIMENSIONAL TANDEM MASS SPECTROMETRY: INSTRUMENTATION AND APPLICATION

Lucas J Szalwinski (12469362)

27 April 2022

<p>Mass spectrometry has become the premium chemical identification method. The next advancement for mass spectrometry is the widespread use of mass spectrometers for on-site chemical/biological identification. Ion trap mass spectrometers have emerged as powerful on-site analytical platforms, in spite of limited mass resolution, due to their compatibility with ambient ionization methods and ready implementation of tandem mass spectrometry (MS/MS). However, conventionally operated ion traps are inefficient in accessing the entire tandem mass spectrometry dataspace. By operating the ion trap at a constant trapping voltage, more efficient tandem mass spectrometry scan modes are accessible. The most efficient is to acquire the entire tandem mass spectrometry data space and this work demonstrates three different methods of acquiring this data domain. These methods acquire the data in under a second and the best performing method was implemented in a miniature mass spectrometer without performance decrease. The impact of this device is most powerful when analysis requires the entire ionized sample be considered to determine the identity of the sample. This was shown to be useful for monitoring the lipid metabolism in a model microorganism. </p>

mass spectrometry

MS/MS

tandem mass specrometry

Quadrupole Ion Traps

2D MS/MS

Logical MS/MS

Design of an LC-MS/MS method for measuring concentrations of Cyclosporine A and Tacrolimus from dried blood spots

Hansson, Anna

January 2015

Patients that have undergone organ transplantation are life-long treated with immunosuppressant drugs and these have to be monitored regularly to get the desired effect of suppressing the immune system. To monitor the drug concentration normally a venous blood sample is collected at a clinic but the use of dried blood spots (DBS) as a matrix for drug monitoring for immunosuppressant drugs will make home sampling possible for this patient group. The aim of this study was to develop and validate a bioanalytical method for quantifying cyclosporine A and tacrolimus in dried blood spots. The method consist of punching out a 5 mm disc from a blood spot , followed by extracting the spot in a 96-well hydrophobic filter plate with 150 µL extraction solution containing internal standard (ascomycin and cyclosporine A d12) in a methanol water solution (80:20v/v%). The extract is then centrifuged through the filter plate down in a 96-deep well plate and injected on the LC-MS/MS, with an analysis time of 2.5min. The method will be validated in accordance with the guidelines set by the European Medicines Agency with additions specific to DBS. The method is not fully validated but will be in due time. The validated parameters show a robust and fast analysing method that has the prospects of being used for analysing DBS samples for patients and in the future can possibly be used by patients in home environment.

LC-MS/MS

Dried blood spots

Immunosuppressive drugs

Entwicklung einer Multimethode zur Probenaufarbeitung und Bestimmung von gas- und flüssigkeitschromatographisch erfassbaren Pestiziden in Hühnereiern

Hildmann, Fanny

05 September 2016

Die Rückstandsanalytik tierischer Lebensmittel ist eine anspruchsvolle Aufgabe aufgrund des hohen Lipidanteils der Proben sowie des sich stetig vergrößernden Wirkstoffspektrums. Heutzutage werden für die Probenaufarbeitung die DFG S 19 Methode, mit der vorrangig unpolare Analyten nachgewiesen werden und zunehmend die QuEChERS Methode eingesetzt, die insbesondere auf die Erfassung polarer Pestizide abzielt. In dieser Arbeit wurde eine moderne Multirückstandsmethode für Hühnereier entwickelt, um sowohl gas- als auch flüssigkeitschromatographisch (GC, LC) erfassbare Wirkstoffe zu analysieren. Dazu gehören unpolare PCBs, Pyrethroide und Organochlorpestizide, aber auch polarere Organophosphate, Triazole und Carbamate. Das Verfahren basiert auf der Extraktion mittels Matrix Solid Phase Dispersion, der Reinigung auf Grundlage einer modifizierten Gelpermeationschromatographie (GPC) und zwei verschiedenen Festphasenextraktionen (SPEs) für GC- und LC-erfassbare Pestizide sowie der Quantifizierung mittels GC- und LC-MS/MS. Dünnschichtchromatographisch wurde die effektive Entfernung hochmolekularer Lipide durch die modifizierte GPC und niedrigmolekularer Fette durch die SPEs belegt. Laut der für Ei durchgeführten Validierung erfüllten 164 der 172 untersuchten Pestizide und alle sechs PCBs die Leistungskriterien für die amtliche Rückstandskontrolle - zumeist am niedrigsten validierten Level (5 µg/kg bzw. 0,5 µg/kg). Ausnahmen bildeten sehr polare LC-Pestizide (z.B. Aminopyralid, Clopyralid, MCPA, Quinmerac) und pH-Wert-abhängige GC-Analyten (Nicotin, Tolylfluanid, Dichlofluanid), die auch mit den etablierten Verfahren schwierig zu analysieren sind. Weiterhin verdeutlichte die erfolgreiche Untersuchung von verschiedenen Ringversuchsmaterialien, dass die ursprünglich für Eier entwickelte Methode auch für mageres Geflügelfleisch und Sahne genutzt werden kann. Gegenüber den etablierten Verfahren wies die neue Methode deutliche Vorzüge auf. So belegte die Dünnschichtchromatographie, dass mit der neuen Methode Cholesterin, aber auch freie Fettsäuren besser abgetrennt werden als mit den etablierten Verfahren. Die neue Methode verbrauchte im Vergleich zur DFG S 19 Methode 46 % weniger Lösungsmittel und ermöglichte eine Verdopplung des Probendurchsatzes innerhalb von 8 h. Zudem eignete sich das entwickelte Verfahren laut den Validierungsdaten für GC-Analyten deutlich besser als die QuEChERS Methode und etwas besser als die DFG S 19 Methode (v.a. für Pyrethroide). Hinsichtlich der LC-Analyten unterschieden sich die neue und die QuEChERS Methode nur bei wenigen Analyten. Mit dem neuen Verfahren konnten folglich im Gegensatz zu den etablierten Methoden sowohl unpolare GC- als auch polare LC-Analyten sicher erfasst werden.

Multirückstandsanalyse

Lebensmittel tierischen Ursprungs

GC-MS/MS

LC-MS/MS

Dünnschichtchromatographie

Zirkoniumdioxid-beschichtetes Kieselgel

multi-residue analysis method

food of animal origin

GC-MS/MS

LC-MS/MS

thin layer chromatography

Zirconium-oxide-coated SPE phase

ddc:540

rvk:VN 8107

Method development and validation for the quantification of eight synthetic piperazines in blood and urine using liquid chromatography-tandem mass spectrometry (UFLC-ESI-MS/MS)

LeBlanc, Raquel Alecia

03 November 2016

Synthetic piperazines are chemically-produced compounds that contain a six-member ring with two opposing nitrogen atoms. Several piperazine derivatives, namely 1- benzylpiperazine (BZP), 1-(3-trifluoromethylphenyl)-piperazine (TFMPP), and 1-(3- chlorophenyl)-piperazine (mCPP), have fallen into the “designer drugs” category due to their increasing recreational use as a “legal” alternative to ecstasy (3,4-methylenedioxymethamphetamine). These compounds share similar stimulant and physiological effects with amphetamines which make them desirable to young adults in party-type atmospheres. BZP, a Schedule I drug for its high abuse potential and no accepted medical use, is the only recreationally-abused synthetic piperazine currently federally controlled in the United States. The purpose of this research was to develop and validate a reliable method to identify and quantify eight forensically significant synthetic piperazines in blood and urine using ultra-fast liquid chromatography-electrospray ionization-tandem mass spectrometry (UFLC-ESI-MS/MS). The method was validated according to the Scientific Working Group for Forensic Toxicologists (SWGTOX) guidelines for quantitative analysis for both matrices and includes the following analytes: 1-benzylpiperazine (BZP), 1-(4-fluorobenzyl)-piperazine (FBZP), 4-methyl-1-benzylpiperazine (MBZP), 1-(4-methoxyphenyl)-piperazine (MeOPP), 1-(para-fluorophenyl)-piperazine (pFPP), 1-(3-chlorophenyl)-piperazine (mCPP), 2,3-dichlorophenylpiperazine (DCPP), and 1-(3-trifluoromethylphenyl)-piperazine (TFMPP). All samples were prepared by fortifying 100 µL of certified drug-free whole blood and urine (UTAK Laboratories, Inc., Valencia, CA, U.S.A.) with certified reference standards (Cayman Chemical, Ann Arbor, MI, U.S.A.) of each analyte at desired concentrations and standard additions of 1-benzylpiperazine-d7, 1-(3-chlorophenyl)-piperazine-d8, and 1(-3-trifluoromethylphenyl)-piperazine-d4 internal standards (Cerilliant, Round Rock, TX, U.S.A). After pretreatment with 1 mL phosphate buffer, samples underwent solid phase extraction (SPE) on mixed-mode copolymeric columns (Clean Screen®, UCT Inc., Levittown, PA, U.S.A.). Eluents were evaporated to dryness with low heat (65°C) and nitrogen gas. Samples were reconstituted with a 50:50 mixture of methanol and 2mM ammonium formate buffer with 0.2% formic acid before being analyzed by a UFLC (Shimadzu Corporation, Kyoto, Japan) and 4000 QTRAP ESIMS/MS (SCIEX, Framingham, MA, U.S.A.) system. Analyses were performed with multiple reaction monitoring scans in positive ionization mode using ions and voltages obtained from a manual compound optimization. Analytes were separated on a reversed phase column (Kinetex® F5, Phenomenex®, Torrance, CA, U.S.A.) with a binary gradient consisting of a 2mM ammonium formate buffer with 0.2% formic acid and methanol with 0.1% formic acid. The flow rate was 0.400 mL/min. Analyst™ (SCIEX) software was used for data collection and MultiQuant™ (SCIEX) software was used for quantitation. The total run time was 11.5 minutes with equilibrations. All calibration curves in both matrices exhibited R2 values > 0.99 using a weighting factor of 1/x. A linear dynamic range of 20-2000 ng/mL was used for all analytes in both matrices, except for BZP in urine which ranged from 50-2000 ng/mL. In blood, the limit of quantitation was 10 ng/mL for mCPP and TFMPP and 20 ng/mL for BZP, FBZP, MBZP, MeOPP, pFPP and DCPP. In urine, the limit of quantitation was 10 ng/mL for MeOPP, mCPP, TFMPP and DCPP, 20 ng/mL for FBZP, MBZP and pFPP and 50 ng/mL for BZP. When a 200 ng/mL concentration was evaluated, the SPE procedure showed percent recoveries ranging from 80-95% for blood; except for BZP, FBZP, and MeOPP which had recoveries of 60%, 60%, and 105%, respectively. Percent recoveries ranged from 82-94% for urine; except for BZP and FBZP which had recoveries of 66% and 68%, respectively. Bias and precision were assessed at concentrations of 50, 200, and 700 ng/mL. All samples were calculated within ±20% bias and within ±20% coefficient of variation. The highest concentration evaluated that did not produce carryover in subsequent matrix blanks was 5000 ng/mL. Ionization was suppressed for all analytes in both matrices by 45-95%. Matrix effects were present but were determined to be insignificant. Of the drugs evaluated, caffeine, dibenzylpiperazine, and 1-(4-chlorophenyl)-piperazine (pCPP) produced chromatographic peaks in the method; however, pCPP was the only substance that affected quantitation of an analyte. It increased the peak area of mCPP by almost 50% when present at the same concentration which suggests this method is unable to differentiate between isomeric pairs. This is a sensitive, reliable, and robust method with a wide linear dynamic range to account for the presence of these analytes in both blood and urine. This research will provide for the identification and quantitation of these substances in forensic casework.

Toxicology

BZP

LC-MS/MS

Designer drug

Method development

Piperazine

Avaliação das concentrações plasmáticas e teciduais de vildagliptina em ratos diabéticos e sadios através de microdiálise

Andrade, Cristiane de

January 2013

Objetivo: Avaliar a farmacocinética da vildagliptina em animais sadios e diabéticos, através da análise dos níveis plasmáticos totais e livres teciduais, empregando-se a técnica de microdiálise. Metodologia: A doença foi induzida nos animais através da administração de 42mg/kg de aloxano através da via intravenosa (i.v.). A vildagliptina foi administrada nas doses de 50 mg/kg (n = 6) e 75 mg/kg (n = 6) via i.v. nos animais diabéticos e na dose de 50 mg/kg (n = 6) nos animais sadios. As concentrações plasmáticas foram quantificadas por CLAE-EM-EM em método desenvolvido e validado. A ligação às proteínas plasmáticas foi determinada por microdiálise, assim como a avaliação tecidual. As sondas de microdiálise foram calibradas in vitro através de diálise e retrodiálise e in vivo utilizando retrodiálise. Para determinação das concentrações teciduais, uma segunda metodologia foi desenvolvida e validada em CLAE-EM-EM. Avaliações compartimentais (software Scientist ®) e não compartimentais (software Excel ®) foram realizadas. Resultados e Discussão: A ligação as proteínas plasmáticas apresentou um valor médio de 9,44 % ± 3,23, condizente com valores encontrados na literatura. Os valores de Ke, clearance, tempo de meia vida, MRT e VDss não apresentaram diferença estatística significativa entre as diferentes doses administradas nos animais diabéticos e entre os animais sadios. As calibrações in vitro por diálise e retrodiálise apresentaram uma recuperação média de 30%, sem diferença estatística entre as duas metodologias empregadas (α = 0,05). A recuperação in vivo também apresentou o mesmo valor médio de recuperação. A penetração tecidual do fármaco em animais diabéticos para as diferentes doses estudadas apresentou mesmo valor nos tecidos estudados, uma média de 0,20. A penetração tecidual semelhante no animal diabético pode ser devido ao dano similar entre os órgãos sofrido durante a indução da doença. Já os animais sadios apresentaram penetração tecidual similar no músculo sem diferença estatística significativa em relação aos diabéticos, entretanto no fígado foi observada uma penetração quarenta e quatro vezes inferior a observada no músculo. Essa disparidade pode ser atribuída a diferença de expressão de proteínas transportadoras no fígado do animal diabetico quando comparado ao sadio. O perfil farmacocinético plasmático foi semelhante entre os dois grupos avaliados, sendo que os parâmetros não diferiram estatisticamente (α = 0,05). Foi empregado o modelo de dois compartimentos para prever as concentrações teciduais. A previsão supõe concentrações superiores as encontradas experimentalmente, contradizendo dados de literatura. Esses dados são inéditos na literatura e demostram a importância da determinação do fármaco em tecidos alvo, uma vez que nem sempre modelos matemáticos conseguem prever a realidade fisiológica. Conclusões: As metodologias analíticas para quantificação da vildagliptina em microdialisado e plasma foram desenvolvidas e validadas, seguindo os requisitos do FDA. O perfil farmacocinético plasmático foi adequadamente descrito pelo modelo de 2 compartimentos. Os perfis teciduais obtidos nesse trabalho podem contribuir para o melhor entendimento dos mecanismos farmacológicos envolvidos e contribuir para futura otimização de terapias. / Objective: To evaluate the pharmacokinetics of vildagliptin in healthy and diabetic animals using a microdialysis technique. Methodology: Diabetes was induced in animals by administration of 42 mg/kg of alloxan intravenously (iv). Vildagliptin was administered intravenously as 50 mg/kg (n = 6) and 75 mg/kg doses (n = 6) in the diabetic animals and as a 50 mg/kg dose (n = 6) in healthy animals. Plasma concentrations were quantified by a HPLC-MS-MS method developed and validated. The plasma protein binding was determined by microdialysis and tissue evaluation. Microdialysis probes were calibrated in vitro using dialysis and retrodialysis and in vivo using retrodialysis. A second method was developed and validated using HPLC-MS-MS to determine tissue concentrations. Results and Discussion: Mean plasma protein was 9.44% ± 3.23, consistent with values reported in the literature. The values of Ke, clearance, half-life, MRT and Vdss showed no statistical difference between the evaluated doses in diabetic animals and between healthy animals (α = 0.05). Calibrations in vitro by dialysis and retrodialysis showed mean recovery of 30%, with no statistical difference between the two methodologies. Mean recovery in vivo also showed the same value. The tissue penetration of the drug in diabetic animals for the different doses studied showed the same value in both tissues studied, an mean of 0.20. The tissue penetration similar in diabetic animals could be due to the similar damage suffered between organs during induction of the disease. The healthy animals showed similar muscle penetration, compared with diabetics animals, although the liver showed a penetration forty four times lower than muscle. This discrepancy can be attributed to differential expression of transporter proteins in the liver of diabetic animals, when compared to the healthy group. The plasma pharmacokinetic profile was similar between the investigated groups, and the parameters did not differ. The two-compartment model was employed to describe the data and used to predict the concentration in the tissues. This is the first study to present these tissue profiles, which presented concentrations below the estimated by the model. These data demonstrate the importance of determining the drug inside the target tissue, as the mathematical models sometimes cannot predict physiology. Conclusions: The analytical methods for the quantification of vildagliptin in microdialysate and plasma were developed and validated by following the requirements of the FDA. The plasma pharmacokinetic profile was correctly described by the model of two compartmental models. The novel tissue profiles obtained in this study may contribute to a better understanding of the pharmacological mechanisms involved and contribute to optimization of future therapies.

Vildagliptina

Farmacocinética

Microdialise

Diabetes

Vildagliptin

Microdialysis

Pharmacokinetics

HPLC-MS-MS

Devenir des antibiotiques lors du traitement aérobie et anaérobie des boues de STEPs pour une valorisation agronomique

Ezzariai, Amine

15 September 2018

L’utilisation massive des antibiotiques contribue à leur accumulation dans les boues des stations d’épurations. L’application directe des boues est parmi les sources de dissémination des antibiotiques et des gènes de résistance aux antibiotiques. Le compostage et la méthanisation sont parmi les bioprocédés de traitement des boues qui permettent d’éliminer ou réduire les teneurs de certains antibiotiques. Dans ce travail, une boue primaire de la STEP de Marrakech a été contaminée par trois familles d’antibiotiques (macrolides, tétracyclines, fluoroquinolones) pour conduire 4 essais de compostage à différentes doses (dont un essai témoin) et un essai deméthanisation en mode semi-continu. Les résultats du compostage ont montré que l’augmentation des concentrations d’antibiotiques retarde la dégradation de la matière organique et affecte le ratioC/N. De même, la phase thermophile est perturbée, retardée et réduite dans le temps. Pour la méthanisation, une concentration unique et réaliste a été testée. Dans ces conditions, aucun effet sur la production du biogaz ou sur la dégradation de la matière organique n’a été observé. Afin de suivre la dissipation des trois familles d’antibiotiques utilisées au cours du compostage et de la méthanisation, une approche analytique basée sur l’extraction accélérée par solvant (ASE) suivie par l’application d’une méthode des ajouts dosés avant quantification par chromatographie liquide couplée à de la spectrométrie de masse en tandem (UPLC-MS/MS) a du être mise en point. Le compostage et la méthanisation permettent de réduire significativement les concentrations des molécules parents appartenant à la famille des macrolides et des tétracyclines. Par contre,l’élimination des fluoroquinolones est non-significative et ne dépasse pas 30%. Au cours du compostage, la dissipation des macrolides se fait en phase de stabilisation tandis que la phase de maturation est impliquée dans la dissipation des tétracyclines. Les concentrations encirprofloxacine (fluoroquinolone) semblent légèrement évoluer au cours du procédé probablement en raison d’une adsorption/désorption sur le co-substrat lignocellulosique utilisé. Concernant la méthanisation, l’élimination des macrolides et des tétracyclines est significative durant la stabilisation du procédé mais n’atteinds pas les rendements observés lors du compostage. Ladiminution des concentrations des molécules parents est probablement accompagnée par une biotransformation des antibiotiques sous forme de métabolites qui à ce stade ne sont pas connus.La question de la rémanence de certaines molécules comme les fluoroquinolones, interpelle quand au risque d’antibiorésistance. Ainsi, la valorisation des composts/digestats comme amendements organiques des sols dois à terme conduire à une réflexion concernant la réglementation qui inclus la présence de molécule de la classe des antibiotiques.

Antibiotiques

Macrolides

Tétracyclines

Fluoroquinolones

Compostage

Méthanisation

ASE

LC-MS-MS