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Selenium redox cycling; isolation and characterization of a stimulatory component from tissue of loblolly pine for multiplication of somatic embryos; development of an assay to measure l-phenylalanine concentration in blood plasmaDeSilva, Veronica 25 June 2007 (has links)
Exogenously supplied organoselenium compounds, capable of propagating a selenium redox cycle, were shown to supplement natural cellular defenses against oxidants generated during biological activity. Phenylaminoalkyl selenides were developed in our laboratory as novel substrate analogs for the enzyme dopamine beta-monooxygenase. Recently, phenylaminoalkyl selenides were found to protect plasmid DNA and Molecular beacons from oxoperoxynitrate – mediated damage by scavenging this oxidant and forming the corresponding selenoxides as the sole selenium – containing products. Rate constants were determined for the reactions of the phenylaminoalkyl selenoxides with GSH at physiological pH and 25 degrees C. The kinetic data obtained in current and previous research was subsequently used in a MatLab simulation, which showed the feasibility of selenium redox cycling by GSH in the presence of a cellular oxidant, oxoperoxynitrate. Loblolly pine (LP, Pinus taeda) is the primary commercial species in southern forests covering 11.7 million hectares. Somatic embryogenesis (SE) is an effective technique to implement production of high value genotypes of LP. SE is a multi-step process, which includes initiation of somatic embryo (SME) growth from tree tissue, maintenance and multiplication of early stage SMEs and the maturation / germination phase. In this work, we isolated a substance from stage 2 or 3 LP female gametophyte (FG) tissue that stimulates early stage SME growth, and characterized this substance as citric acid on the basis of 1H NMR and mass spectrometry. We then demonstrated that topical application of citric acid to SMEs stimulates embryo colony growth at p = 0.05 for 3 of the 5 genotypes tested. Phenylketonuria (PKU) is an autosomal recessive disorder caused by an impaired conversion of L-phenylalanine (L-Phe) to L-tyrosine (L-Tyr). A novel assay based on enzymatic - colorimetric methodology (ECA) was developed in order to detect elevated concentrations of L-Phe in undeproteinized plasma of PKU patients via continuous spectrophotometric detection. We report here that L-Phe concentrations in undeproteinized plasma measured using our ECA were comparable to those determined on an amino acid analyzer based on Pearson correlation coefficients and a Bland and Altman comparison.
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Analyse simultanée des hormones stéroïdiennes et leurs formes chimiques dans les matrices d'eau et d'urine par SPE-LC-MS/MS en ligneClemente Naldi, Amanda 12 1900 (has links)
No description available.
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Desenvolvimento de métodos por cromatografia líquida acoplada à espectrometria de massas em tandem para análises de fármacos (LC-MS/MS no modo column switching com capilar monolítico de sílica híbrida), aminoácidos e neurotransmissores (HILIC-MS/MS) em amostras de plasma de pacientes esquizofrênicos. / Development of methods for liquid chromatography coupled to tandem mass spectrometry for drug analysis (LC-MS/MS in column switching mode with monolithic capillary hybrid silica), amino acids and neurotransmitters (HILIC-MS/MS) in plasma samples of schizophrenic patients.Diego Soares Domingues 26 August 2015 (has links)
A esquizofrenia é um transtorno neuropsiquiátrico crônico que afeta aproximadamente 1% da população mundial. As teorias neurobiológicas descrevem que a esquizofrenia é essencialmente causada por alterações bioquímicas e estruturais do cérebro, devido às disfunções nos sistemas glutamatérgico, dopaminérgico e serotoninérgico. Desta forma, a determinação das concentrações de aminoácidos e neurotransmissores em amostras de plasma de pacientes esquizofrênicos pode auxiliar na avaliação da eficácia da terapia. Além dos antipsicóticos, medicação de primeira linha no tratamento inicial da esquizofrenia, a maioria dos pacientes também faz uso concomitante de outras classes de fármacos, tais como antidepressivos, anticonvulsivantes e ansiolíticos para minimizar os sintomas associados a esta doença. Nesta tese, um método empregando a precipitação de proteínas (PPT) e a cromatografia líquida por interação hidrofílica acoplada à espectrometria de massas em tandem (HILIC-MS/MS) foi adequadamente desenvolvido e validado para a determinação de aminoácidos (aspartato, serina, glicina, alanina, metionina, leucina, tirosina e triptofano) e neurotransmissores (glutamato e ácido -aminobutírico) em amostras de plasma de 35 pacientes esquizofrênicos em tratamento com clozapina (27 pacientes) e olanzapina (8 pacientes) para avaliar a eficácia do tratamento, tendo como controle 38 voluntários sadios. O método HILIC-MS/MS apresentou linearidade do LIQ (9,7 pmol mL-1 - 13,3 nmol mL-1) ao LSQ (19,4 nmol mL-1 - 800 nmol mL-1), tempo de análise de 3,0 min, exatidão com EPR de -18 a 19% e precisão com CV de 0,1 a 16% (LIQ). A análise de variância (ANOVA), seguida por teste post-hoc de Duncan, revelou que os níveis médios plasmáticos (nmol mL-1) de metionina (F2,70 = 3,14, p = 0,049) de pacientes esquizofrênicos em tratamento com olanzapina foram significativamente mais elevados, quando comparados aos valores obtidos com o grupo controle (voluntários saudáveis), já o nível de glutamato em pacientes esquizofrênicos em tratamento com clozapina apresentaram tendência a valores mais altos (F2.70 = 2,50, p = 0,090). Já os métodos, PPT/LC-MS/MS e LC-MS/MS no modo column switching utilizando uma coluna monolítica de sílica híbrida com grupos cianopropil na primeira dimensão, foram desenvolvidos e validados para a determinação dos antipsicóticos (olanzapina, quetiapina, clozapina, haloperidol e clorpromazina), antidepressivos (mirtazapina, paroxetina, citalopram, sertralina, imipramina, clomipramina e fluoxetina), anticonvulsivantes (carbamazepina e lamotrigina), e ansiolíticos (diazepam e clonazepam) em amostras de plasma de pacientes esquizofrênicos para fins de monitorização terapêutica. O método PPT/LC-MS/MS apresentou linearidade do LIQ (0,2 ng mL-1 - 5,0 ng mL-1) ao LSQ (40,5 ng mL-1 - 10,5 g mL-1), exatidão com EPR de -9,7 a 8,0%, e precisão com CV de 0,1 a 12%. Já o método LC-MS/MS no modo column switching apresentou linearidade do LIQ (63,0 pg mL-1 - 1250,0 pg mL-1) ao LSQ (40,5 ng mL-1 - 10,5 g mL-1), exatidão com EPR de -14 a 12% e precisão com CV de 0,6 a 6,5%. A pré-concentração seletiva dos fármacos na coluna monolítica com grupos cianopropil incorporados e a remoção dos componentes endógenos da amostra biológica, antes da separação cromatográfica, favoreceram a seletividade e detectabilidade do método LC-MS/MS no modo column switching. Este método quando comparado ao de referência PPT/LC-MS/MS, através da análise de 10 amostras de pacientes esquizofrênicos, não apresentou diferença significativa (teste t) entre as concentrações plasmáticas, podendo ser aplicado na monitorização terapêutica. Além deste fato, este método automatizado favoreceu a precisão, a exatidão e a freqüência analítica. / Schizophrenia is a chronic neuropsychiatric disorder that affects approximately 1% of the world population. According to neurobiological theories, schizophrenia stems from biochemical and structural alterations in the brain due to dysfunction in the glutamatergic, dopaminergic, and serotonergic systems. Determining the concentrations of amino acids and neurotransmitters in plasma samples from schizophrenic patients may assist evaluation of therapy effectiveness. In addition to antipsychotics (the first-line drug in the initial treatment of schizophrenia), most patients concomitantly use other classes of drugs such as antidepressants, anticonvulsants, and anxiolytics to minimize the symptoms associated with this disease. To evaluate treatment efficacy, in this thesis a method based on protein precipitation (PPT) and hydrophilic interaction liquid chromatography coupled to tandem mass spectrometry (HILIC-MS/MS) has been properly developed and validated to determine amino acids (aspartate, serine, glycine, alanine, methionine, leucine, tyrosine, and tryptophan) and neurotransmitters (glutamate and -aminobutyric acid) in plasma samples obtained from 35 schizophrenia patients treated with clozapine (27 patients) or olanzapine (8 patients); 38 healthy volunteers served as controls. The HILIC-MS/MS method was linear for concentrations ranging from the LLOQ (9.7 pmol mL-1 - 13.3 nmol mL-1) to the ULOQ (19.4 nmol mL-1 - 800 nmol mL-1). The analysis time was 3.0 min. In the case of accuracy, RSE ranged from -18 to 19%. As for precision, CV lay between 0.1 and 16% (LLOQ). Analysis of variance (ANOVA) followed by post-hoc Duncan showed that the average methionine serum levels (nmol mL-1) (F2.70 = 3.14, p = 0.049) in schizophrenic patients treated with olanzapine were significantly higher as compared with the control group (healthy volunteers). The glutamate level in schizophrenic patients treated with clozapine tended to higher values (F2.70 = 2.50, p = 0.090). Concerning the analytical methods, PPT/LC-MS/MS and LC-MS/MS operating in the column-switching mode were developed and validated to determine antipsychotic (olanzapine, quetiapine, clozapine, haloperidol, and chlorpromazine), antidepressants (mirtazapine, paroxetine, citalopram, sertraline, imipramine, clomipramine, and fluoxetine), anticonvulsants (carbamazepine and lamotrigine), and anxiolytics (diazepam and clonazepam) in plasma samples taken from schizophrenic patients for therapeutic drug monitoring. A monolithic hybrid column containing silica with cyanopropyl groups in the first dimension was employed. The PPT/LC-MS/MS method was linear from the LLOQ (0.2 ng mL-1 - 5.0 ng mL-1) to the ULOQ (40.5 ng mL-1 - 10.5 g mL-1). In the case of accuracy, RSE ranged from -9.7 to 8.0%; as for precision, CV lay between 0.1 and 12%. LC-MS/MS in the column-switching mode was linear from the LLOQ (63.0 pg mL-1 - 1250.0 pg mL-1) to the ULOQ (40.5 ng mL-1 - 10.5 g mL-1). RSE ranged from -14 to 12%; CV lay between 0.6 and 6.5%. The drugs were selectively pre-concentrated in the monolithic column containing silica incorporated with cyanopropyl groups. For the LC-MS/MS method operating in the column-switching mode, the endogenous components of the biological sample of the LC-MS/MS method were removed before analysis. Analysis of 10 plasma samples obtained from schizophrenic patients did not reveal any significant differences (t test) between the LC-MS/MS method and the reference PPT/LC-MS/MS method. Therefore, LC-MS/MS can be applied in therapeutic monitoring, with the advantage that this method offers improved precision, accuracy, and analytical frequency.
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Développement de méthodologies analytiques pour l'étude de la migration depuis des contenants en matière plastique prévus pour des applications pharmaceutiques vers des solutions aqueuses et des fluides biologiques / Development of analytical methodologies for the migration study from plastic packaging material intended for pharmaceutical applications into aqueous solutions and biological fluidsPouech, Charlene 02 July 2014 (has links)
Résumé confidentiel / Résumé confidentiel
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Využití vysokoúčinných separačních metod pro chirální i achirální separace / The application of high-efficiency separation methods for chiral and achiral separationsŠubová, Martina January 2019 (has links)
In the first part of the doctoral thesis, the capillary electrophoresis was used to test the potential chiral separation properties of monosubstituted cyclodextrin derivatives, namely PEMEDA- and PEMPDA-β-cyclodextrins for the group of selected analytes. Both selectors exhibited excellent enantioseparation properties for N-boc-D,L-tryptophan, where the enantiomers were completely separated even at 0.5 mmol·l-1 concentration of the cyclodextrin derivative in the background electrolyte. However, the differences between the enantiodiscrimination properties of individual derivatives were minimal. The second test group consisted of two cyclodextrin derivatives, namely 2-O- and 3-O- cinnamyl-α-cyclodextrins. These derivatives are able to form supramolecular polymers in aqueous solutions that disintegrate at elevated temperature. The formation of these polymers was tested by NMR and DLS experiments. None of the tested cyclodextrin derivatives showed enantiodiscrimination properties towards a group of selected analytes. In the frame of antipredatory study, HPLC-MS/MS method working in HILIC mode was used for separation of ten pterin derivatives and riboflavin, which can be present as pigments in insects, reptiles or amphibians as a part of their warning coloration. The developed methodology was applied for...
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Patologie a fyziologie de novo syntézy purinů. / Pathology and physiology of de novo purine synthesis.Krijt, Matyáš January 2021 (has links)
Purines are organic compounds with miscellaneous functions that are found in all living organisms in complex molecules such as nucleotides, nucleosides or as purine bases. The natural balance of purine levels is maintained by their synthesis, recycling and degradation. Excess purines are excreted in the urine as uric acid. Purine nucleotides may be recycled by salvage pathways catalysing the reaction of purine base with phosphoribosyl pyrophosphate. A completely new central molecule of purine metabolism, inosine monophosphate, can be synthesized from precursors during the de novo purine synthesis (DNPS). DNPS involves ten steps catalysed by six enzymes that form a multienzymatic complex, the purinosome, enabling substrate channelling through the pathway. DNPS is activated under conditions involving a high purine demand such as organism development. Currently, three DNPS-disrupting disorders have been described: ADSL deficiency, AICA-ribosiduria and PAICS deficiency. All three disorders are caused by genetic mutations leading to the impaired function of particular enzyme causing insufficient activity of respective DNPS step, manifested biochemically by accumulation of substrate of deficient enzyme, biologically by disruption of purinosome formation and clinically by unspecific neurological features,...
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Multiple-approaches to the identification and quantification of cytochromes P450 in human liver tissue by mass spectrometrySeibert, C., Davidson, B.R., Fuller, B.J., Patterson, Laurence H., Griffiths, W.J., Wang, Y. January 2009 (has links)
No / Here we report the identification and approximate quantification of cytochrome P450 (CYP) proteins in human liver microsomes as determined by nano-LC-MS/MS with application of the exponentially modified protein abundance index (emPAI) algorithm during database searching. Protocols based on 1D-gel protein separation and 2D-LC peptide separation gave comparable results. In total, 18 CYP isoforms were unambiguously identified based on unique peptide matches. Further, we have determined the absolute quantity of two CYP enzymes (2E1 and 1A2) in human liver microsomes using stable-isotope dilution mass spectrometry, where microsomal proteins were separated by 1D-gel electrophoresis, digested with trypsin in the presence of either a CYP2E1- or 1A2-specific stable-isotope labeled tryptic peptide and analyzed by LC-MS/MS. Using multiple reaction monitoring (MRM) for the isotope-labeled tryptic peptides and their natural unlabeled analogues quantification could be performed over the range of 0.1-1.5 pmol on column. Liver microsomes from four individuals were analyzed for CYP2E1 giving values of 88-200 pmol/mg microsomal protein. The CYP1A2 content of microsomes from a further three individuals ranged from 165 to 263 pmol/mg microsomal protein. Although, in this proof-of-concept study for CYP quantification, the two CYP isoforms were quantified from different samples, there are no practical reasons to prevent multiplexing the method to allow the quantification of multiple CYP isoforms in a single sample.
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Entwicklung und Validierung eines Enzyme-linked Immunosorbent Assays (ELISA) für die Quantifizierung von Carbamazepin in Abwasser, Oberflächenwasser und TrinkwasserBahlmann, Arnold 17 April 2013 (has links)
Ein kompetitiver ELISA (Enzyme-linked Immunosorbent Assay) für den Nachweis von Carbamazepin (CBZ) mit einer Bestimmungsgrenze von ca. 30 ng/L wurde entwickelt und validiert. Dieser in Gewässern häufig auftretende anthropogene Marker wurde anschließend in einer Vielzahl an Proben aus Abwässern, Oberflächengewässern und Trinkwässern nachgewiesen. Der ELISA zeigte eine exzellente Präzision und erbrachte in allen Matrizes geringfügig höhere Analysenergebnisse als die Referenzmethode HPLC-MS/MS. Die beständige Überbestimmung der CBZ-Konzentration in Höhe von ca. 7 % konnte auf die Präsenz von Cetirizin und geringen Mengen des persistenten Metaboliten 10,11 Epoxy¬carbamazepin (EP-CBZ) zurückgeführt werden. Die Bindungseigenschaften des verwendeten Antikörpers wurden anhand der Kreuz¬reaktivi¬täten von 37 Substanzen eingehend untersucht. Nach Kopplung von Flüssig¬chromato¬graphie und ELISA konnte das strukturell nicht mit CBZ verwandte Anti¬histaminikum Cetirizin als Kreuzreaktand identifiziert werden. Der störende Einfluss dieses Kreuz¬reaktanden auf den CBZ-ELISA konnte nach einer Änderung des pH-Wertes im Proben¬puffer minimiert werden. Die pH-abhängige Selektivitätssteuerung ermöglichte überdies die Entwicklung eines Dual-Analyt-Immunoassays für die parallele Bestimmung von CBZ und Cetirizin. Darüber hinaus wurden die Metaboliten EP-CBZ, DiOH-CBZ, 2-OH-CBZ, 3-OH-CBZ und 10 OH-CBZ in Abwasser, Oberflächenwasser und Trinkwasser quantifiziert. DiOH-CBZ erwies sich als ähnlich persistent wie CBZ und wurde in besonders hohen Konzentrationen gefunden. Außerdem wurden mehrere weitere bislang nicht identifizierte Abbauprodukte von CBZ gefunden. Da weder Probenvorbereitung noch Probenanreicherung erforderlich sind, ist der Test schnell und kostengünstig durchführbar. Die für den Test nötigen Probenvolumen sind mit weniger als 1 mL sehr gering. Diese Eigenschaften erlauben ein Hochdurchsatzscreening und machen die Methode interessant für den Einsatz im Gewässermonitoring. / A competitive ELISA (enzyme-linked immunosorbent assay) for the quantitation of carbamazepine (CBZ) was developed and validated. A limit of quantitation (LOQ) of ca. 30 ng/L allowed for the quantitation of CBZ in many samples from wastewater, surface water and drinking water. The method was found to be excellently precise, but it displayed slightly higher results than obtained by the reference method liquid chromatography-tandem mass spectrometry (LC-MS/MS). The nearly constant overestimation of 7 % could be attributed to the presence of small amounts of cetirizine and the persistent metabolite 10,11 epoxy¬carbamazepine (EP-CBZ). The binding properties of the antibody were studied by determining the cross-reactivities of 37 compounds. Hyphenating liquid chromatography to ELISA led to the discovery of the cross-reactive antihistamine cetirizine that shares no obvious structural similarity with CBZ. The bias caused by cetirizine was eliminated by changing the pH value of the sample buffer. Moreover, the antibody’s pH-dependent selectivity enabled a dual-analyte immunoassay for the parallel determination of CBZ and cetirizine. Furthermore, the metabolites EP-CBZ, DiOH-CBZ, 2-OH-CBZ, 3-OH-CBZ and 10-OH-CBZ were quantified in wastewater, surface water and drinking water. DiOH-CBZ showed the highest concentrations of all analaytes investigated and was found to be equally persistent as CBZ. In addition, several further degradation products of CBZ were found that could not be identified. The ELISA allowed the detection of diurnal and seasonal fluctuations of analyte concentrations in wastewater and surface water. The anthropogenic marker CBZ enabled to trace wastewater from the source to the receiving waters. Since neither sample pretreatment nor enrichment is necessary, the method is very fast and cost-effective. Only a small sample volume (less than 1 mL) is needed making this ELISA an appropriate high-throughput screening tool for environmental monitoring.
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Immunochemical and chromatographic methods for two anthropogenic markers of contamination in surface watersCarvalho, Jose Joao 08 December 2011 (has links)
Koffein (1,3,7-Trimethylxanthin) und Coprostanol (5beta-cholestan-3beta-ol) wurden im Berliner Oberflächenwasser nachgewiesen. Ihre Konzentrationen korrelierten mit dem Verunreinigungsgrad der Proben, was nahelegt, dass sie sich als Marker für menschliche Aktivität eignen. Bemerkenswerterweise wurde Koffein in jeder einzelnen Oberflächenwasserprobe oberhalb der Bestimmungsgrenze von 0,025 µg/L gefunden. Um Oberflächenwasserproben in größeren Serien zu untersuchen, war die Entwicklung zweier neuer Methoden erforderlich: ein Immunoassay, basierend auf einem monoklonalen Antikörper für Koffein und eine dispersive flüssig-flüssig Mikroextraktionsmethode (DLLME), gefolgt von Flüssigkeitschromatographie gekoppelt mit Tandem-Massenspektrometrie (LC-MS/MS) für Coprostanol. Der entwickelte Koffein-Immunoassay zeigt die beste je erhaltene Nachweisgrenze für Koffein (0,001 µg/L), erlaubt Hochdurchsatz-Analysen und erfordert keine Probenvorbereitung. Der Assay wurde auch erfolgreich für die Messung von Koffein in Getränken, Haarwaschmitteln, Koffeintabletten und menschlichem Speichel angewendet. Antikörper gegen Coprostanol sind nicht kommerziell erhältlich. Eine neue Strategie Anti-Coprostanol-Antikörper zu generieren wurde erarbeitet, die eine analoge Verbindung – Isolithocholsäure (ILA) – als Hapten verwendet, mit der eine Gruppe von Mäusen immunisiert wurde. Ein polyklonales Anti-ILA-Serum wurde produziert, welches Coprostanol bindet, aber die niedrige Affinität erlaubte nicht den Aufbau eines Immunoassays, der die Messung von Umweltkonzentrationen des Anayten (im Bereich ng/L) zulässt. Spezifische Anti-ILA-Immunglobuline G wurden auch in den Faeces der Mäuse gefunden. Coprostanol wurde in den Wasserproben durch die Verwendung einer neuentwickelten LC-MS/MS-Methode unter APCI-Ionisation (atmospheric pressure chemical ionisation) gemessen. Konzentrationen oberhalb von 0,1 µg/L wurden nach Voranreicherung der Probe mittels DLLME bestimmt. / Caffeine (1,3,7-trimethylxanthine) and coprostanol (5beta-cholestan-3beta-ol) were detected in samples of Berlin’s surface water. Their concentrations correlated with the contamination status of the samples, suggesting their usefulness as markers of human activity. Remarkably, caffeine concentrations were always well above the limit of quantitation of 0.025 µg/L. In order to screen surface water samples in larger series, the development of two novel methods was required: a monoclonal antibody-based immunoassay for caffeine and a dispersive liquid-liquid microextraction (DLLME) method, followed by liquid chromatography tandem mass spectrometry (LC-MS/MS) for coprostanol. The caffeine immunoassay developed shows the best analytical limit of detection (LOD) obtained so far for caffeine (0.001 µg/L), allows high-throughput analysis, and does not require sample pre-treatment. The assay was also successfully employed to measure caffeine in beverages, shampoos, caffeine tab-lets, and human saliva. Antibodies to coprostanol are not commercially available. A new strategy to generate anti-coprostanol antibodies was elaborated using an analogous com-pound as hapten – isolithocholic acid (ILA) – and immunizing a group of mice. A polyclonal anti-ILA serum was produced, which binds coprostanol but the low affinity did not permit setting up an immunoassay to measure environmental concentrations of the analyte (in the range of ng/L). Specific anti-ILA immunoglobulin G were also found in the faeces of the immunized mice. Coprostanol was quantified in the water samples using a newly developed LC-MS/MS method using atmospheric pressure chemical ionisation (APCI). Concentrations above 0.1 µg/L were determined after sample preconcentration using DLLME. This extraction method also proved to be successful for enrichment of coprostanol-related compounds such as cholesterol, cholestanol, cholestanone, ergosterol, and stigmasterol.
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Detecció dels metabòlits del plastificant di(2-etilhexi)l ftalat com a marcadors de l'ús de transfusions en l'esportMonfort Mercader, Núria, 1983- 19 December 2012 (has links)
El di(2-etilhexil) ftalat (DEHP) és un plastificant que s’afegeix als productes de clorur de polivinil (PVC) per a dotar-los de més flexibilitat. El material mèdic fet de PVC, i en particular els dispositius i bosses que s’utilitzen en les transfusions de sang, conté el DEHP com additiu. Així, el receptor d’una transfusió està altament exposat a aquest compost. L’objectiu de la tesi va ser estudiar els metabòlits del DEHP en orina com a possibles marcadors de la pràctica d’una transfusió de sang en l’esport.
Es va desenvolupar i validar un mètode d’anàlisi per cromatografia líquida acoblada a espectrometria de masses en tàndem per a la quantificació dels principals metabòlits del DEHP en orina humana: mono-(2-etilhexil) ftalat (MEHP), mono-(2-etil-5-hidroxihexil) ftalat (MEHHP), mono-(2-etil-5-oxohexil) ftalat (MEOHP), mono-(2-carboximetilhexil) ftalat (2cx-MMHP) i mono-(2-etil-5-carboxipentil) ftalat (5cx-MEPP). El mètode es va aplicar a mostres procedents de voluntaris sans (grup control), de pacients hospitalitzats que havien rebut una transfusió de sang i de pacients hospitalitzats sotmesos a tractaments mèdics amb materials de PVC i no a transfusions. Es van obtenir diferències significatives en les concentracions dels tres metabòlits estudiats (MEHP, MEHHP, MEOHP) entre les mostres dels pacients transfosos respecte els altres dos grups de població. El mètode també es va aplicar a mostres d’orina de vint-i-cinc voluntaris sans que s’havien sotmès a un procediment d’autotransfusió. Els resultats van indicar concentracions elevades dels cinc metabòlits del DEHP en orina fins a les 48 hores després d’haver rebut la sang.
Finalment, es van determinar les concentracions dels cinc metabòlits de DEHP en una població d’esportistes i es van calcular límits de referència que permetessin sospitar d’una transfusió. Així doncs, els resultats indiquen que la mesura dels metabòlits de DEHP en orina pot ser usada com una eina pel cribatge de l’ús de transfusions en l’esport. / The plasticizer di(2-ethylhexyl)phthalate (DEHP) is used in polyvinyl chloride products (PVC) to increase its flexibility. Medical devices made of PVC, especially blood bags used in blood transfusions, contain DEHP as additive. Therefore, subjects submitted to blood transfusion are widely exposed to this compound. The aim of the project was to evaluate DEHP metabolites in urine as possible markers of the use of a blood transfusion in sports.
An analytical method was developed and validated to quantify the main DEHP metabolites mono-(2-ethylhexyl)phthalate (MEHP), mono-(2-ethyl-5-hydroxyhexyl)phthalate (MEHHP), mono-(2-ethyl-5-oxohexyl)phthalate (MEOHP), mono-(2-carboxymethylhexyl)phthalate (2cx-MMHP) and mono-(2-ethyl-5-carboxypentyl)phthalate (5cx-MEPP), in human urine by liquid chromatography tandem mass spectrometry. The methodology was applied to samples belonging to healthy volunteers (control group), hospitalized patients subjected to blood transfusions and hospitalized patients subjected to medical treatments involving plastic material different to blood transfusions. Significant differences were obtained in the concentrations of the three metabolites studied (MEHP, MEHHP, MEOHP) between transfused patients samples’ and the other two population groups. The method was also applied to urine samples from twenty-five healthy volunteers who were subjected to an autologous blood transfusion. The results indicated high concentrations of the five DEHP metabolites in urine up to 48 hours after the blood transfusion.
Finally, the concentration of the five DEHP metabolites were evaluated in a sportsmen population and reference limits to allow suspicion of blood transfusion were calculated. Thus, the results indicate that the DEHP metabolites could be used as markers of blood transfusions in sports.
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