Évaluation de l'impact des xénobiotiques alimentaires sur la santé materno-foetale : rôle du Bisphénol A

Leclerc, François

January 2013

Au quotidien, nous sommes exposés à une multitude de xénobiotiques, des molécules exogènes à un organisme vivant et qui sont considérées toxiques pour ce dernier. Parmi tous ces xénobiotiques, le Bisphénol-A (BPA), un xénoestrogène, est l'un de ceux attirants le plus l'attention de la communauté scientifique. Des travaux effectués antérieurement par notre laboratoire ont mis en évidence des effets cytotoxiques sur les cellules placentaires (Benachour et Aris, 2009). À de très faibles concentrations, le BPA induit une augmentation significative de l'apoptose et de la nécrose des cytotrophoblastes. De plus, à ces mêmes concentrations, le BPA provoque une augmentation de l'expression et de la sécrétion de facteur de nécrose tumorale alpha (TNF-alpha), une cytokine clef dans les phénomènes d'inflammation. À un niveau cellulaire, la nécrose, l'apoptose ainsi que l'augmentation de la sécrétion de TNF-alpha sont des observations décrites dans les cas de prééclampsie (PE), de diabète gestationnel (DG) et de retard de croissance intra-utérin (RCIU). Ces travaux laissent croire à une plus grande accumulation du BPA chez les femmes ayant développé l'une de ces complications, ainsi qu'un rôle du BPA dans le développement physiopathologique de ces complications. Pour vérifier cette hypothèse, quatre groupes ont été formés, un groupe témoin où aucune pathologie n'est connue, un groupe de femmes ayant développé la prééclampsie, un groupe de femmes ayant développé un diabète gestationnel et finalement un groupe de femmes ayant eu une grossesse compliquée par un retard de croissance intra-utérin. Chacun de ces groupes était formé de 23 candidates sélectionnées dans une cohorte préexistante, la cohorte PÉRICARD. Pour chaque candidate, le Bisphénol A a été quantifié dans le sérum maternel, dans l'homogénat placentaire ainsi que dans le sérum foetal. Les dosages ont été effectués par chromatographie gazeuse couplée à un spectromètre de masse, l'une des méthodes les plus sensibles existantes pour la quantification du Bisphénol A. Nos résultats ont permis de mettre en évidence une accumulation différentielle du BPA dans le placenta de femmes ayant une grossesse avec prééclampsie et ayant mené à un retard de croissance intra-utérin. Le placenta de ces femmes a accumulé une plus forte quantité BPA que les femmes du groupe témoins. Ces résultats entérinent donc l'hypothèse d'une implication du BPA dans la prééclampsie et dans le retard de croissance intra-utérin.

Placenta

Retard de croissance intra-utérin

Diabète gestationnel

Prééclampsie

Bisphénol-A

Proposição de metodologia para estudo de uridina 5'-trifosfato trissódica e citidina 5'-monosfato dissódica e derivados em matriz biológica durante neuropatias periféricas / Proposition methodology for uridine 5'-triphosphate study trissódica and cytidine disodium 5'- monosfato and derivatives in biological matrix for peripheral neuropathies

Suchmacher Neto, Mendel

January 2015

Made available in DSpace on 2016-03-15T14:17:03Z (GMT). No. of bitstreams: 2 7.pdf: 1019934 bytes, checksum: df1b248bb9c258918248c73b73272de2 (MD5) license.txt: 1748 bytes, checksum: 8a4605be74aa9ea9d79846c1fba20a33 (MD5) Previous issue date: 2015 / Fundação Oswaldo Cruz. Instituto de Tecnologia em Fármacos/Farmanguinhos. Rio de Janeiro, RJ, Brasil. / Uridina 5'-trifosfato trissódica (UTPt) e citidina 5'-monofosfato dissódica (CMPd) são nucleotídeos pirimidínicos do ácido nucleico. Eficácia e segurança de fármacos baseados na UTPt e CMPd, usados no tratamento para neuropatias periféricas já foram estudadas, no entanto informações sobre farmacocinética desses fármacos ainda não são conhecidas. O objetivo deste estudo foi propor metodologias para quantificar UTPt e CMPd em matrizes biológicas, baseando-se numa revisão sistemática da literatura. Levando em consideração que a biodisponibilidade das pirimidinas, durante as neuropatias periféricas é diferente da observada em voluntários sadios, os dados disponíveis acerca das concentrações plasmáticas do UTPt e CMPd não devem ser usados para estimar a dose de fármacos baseados nessas pirimidinas. Para diferenciar pirimidinas endógenas e exógenas em matrizes biológicas, estas últimas devem ser marcadas, antes da administração, com material radioativo tais como trício [3H] ou carbono 14 [14C]. Além disso, a cromatografia líquida de alta performance é a técnica mais aplicada para identificação e quantificação de pirimidinas radioativas. Nós concluímos que a radiomarcação de UTPt e CMPd, seguida de separação cromatográfica e detecção por UV e cintilografia líquida, seria uma metodologia factível para estudos de detecção e quantificação de derivados de UTPt e CMPd em matriz biológica / Pyrimidines uridine 5'-triphosphate trisodium (UTPt) and cytidine 5'-monophosphate disodium (CMPd) are standard nucleosides which make up nucleic acids. Efficacy and safety from UTPt and CMPd based drugs on peripheral neuropathies has already been studied. However, information regarding pharmacokinetics of UTPt and CMPd based drugs during pathological condition remains unknown. The aim of this study was to propose methodologies to quantify UTPt and CMPd in biological matrices, based on a systematic literature review. Concerning that the bioavailability of pyrimidines during peripheral neuropathies is different of observed in healthy volunteers, the available data regarding plasmatic levels of UTPt and CMPd should not be used to estimate the dose of UTPt and CMPd based drugs. Furthermore, to differentiate endogenous and exogenous pyrimidines in biological matrices the exogenous pyrimidines must be labeled with [3H] or [14C] before administration. Next, high-performance liquid chromatography (HPLC) has been the most applied technique for identification and quantitation of radiolabeled pyrimidines. We concluded that UTPt and CMPd radiolabelling, followed by chromatographic separation and detection by UV and liquid scintigraphy, is a feasible methodology for detection and quantitation of UTPt and CMPd derivatives in biological matrices.

Uridina 5'-Trifosfato Trissódica

Citidina 5'-Monofosfato Dissódica

Matriz Biológica

Uridine 5'-Triphosphate Trisodium

Cytidine 5'-Monophosphate Disodium

Biological Matrices

Uridina

Uridina Trifosfato

Citidina

Synthesis of Novel Nucleoside Analogs Targeting HCV

Alabdullah, Bader Saleh

13 December 2018

No description available.

Chemistry

Organic Chemistry

Pharmacy Sciences

Chemistry

Medicinal Chemistry

Organic Chemistry

Hepatitis C Virus

HCV

Modified Nucleosides

Anti-HCV Medications

Uridine Analogs

Sofosbuvir

Synthesis

Investigations into the mode of action of the DNA uridine endonuclease Mth212 of Methanothermobacter thermautotrophicus ΔH / Untersuchungen über die Wirkungsweise der DNA-Uridin Endonuklease Mth212 aus Methanothermobacter thermautotrophicus ΔH

Ciirdaeva, Elena

22 January 2010

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

Cytosin-Desaminerung

thermophiles Archaeon

Uridin-Endonuklease

Uridin-Reparatur

cytosine deamination

thermophilic archaeon

uridin endonuclease

uridine repair

4213

The role of P2Y[subscript]2 nucleotide receptor in lipoprotein receptor-related protein 1 expression and aggregated low density lipoprotein uptake in vascular smooth muscle cells

Dissmore, Tixieanna

January 1900

Doctor of Philosophy / Department of Human Nutrition / Denis M. Medeiros / Laman Mamedova / The internalization of aggregated low-­density lipoprotein (agLDL) may involve the actin cytoskeleton in ways that differ from the endocytosis of soluble LDL. Based on previous findings the P2Y[subscript]2 receptor (P2Y[subscript]2R) mediates these effects through interaction with filamin‐A (FLN‐A), an actin binding protein. Our findings also showed that uridine 5’‐ triphosphate (UTP), a preferential agonist of the P2Y[subscript]2R, stimulates the uptake of agLDL, and increases expression of low‐density lipoprotein receptor related protein 1 (LRP 1) in cultured mouse vascular smooth muscle cells (SMCs). The strategy of this research was to define novel mechanisms of LDL uptake through the modulation of the actin cytoskeleton in order to identify molecular targets involved in foam cell formation in vascular SMCs. For this project, we isolated aortic SMCs from wild type (WT) and P2Y[subscript]2R‐/‐ mice to investigate whether UTP and the P2Y[subscript]2R modulate expression of LRP 1 and low‐density lipoprotein receptor (LDLR). We also investigated the effects of UTP on uptake of DiI‐labeled agLDL in WT and P2Y[subscript]2R‐/‐ vascular SMCs. For LRP1 expression, cells were stimulated in the presence or absence of 10 [mu]M UTP. To determine LDLR mRNA expression, and for agLDL uptake, cells were transiently transfected for 24 h with cDNA encoding hemagglutinin-­tagged (HA-­tagged) WT P2Y[subscript]2R or a mutant P2Y[subscript]2R that does not bind FLN‐A, and afterwards treated with 10 [mu]M UTP. Total RNA was isolated, reversed transcribed to cDNA, and mRNA relative abundance determined by RT-­PCR using the delta-­delta Ct method with GAPDH as control gene. Results show SMCs expressing the mutant P2Y[subscript]2R that lacks the FLN‐A binding domain exhibit 3‐fold lower LDLR expression than SMCs expressing the WT P2Y[subscript]2R. There was also decrease in LRP1 mRNA expression in response to UTP in P2Y[subscript]2R‐/‐ SMCs compared to WT. Actinomycin‐D (20 [mu]g/ml) significantly reduced UTP-­induced LRP1 mRNA expression in P2Y[subscript]2R‐/‐ SMCs (P < 0.05). Compared to cells transfected with mutant P2Y[subscript]2R, cells transfected with WT P2Y[subscript]2R showed greater agLDL uptake in both WT VSMC and P2Y[subscript]2R-­/-­ cells. Together these results show that both LRP 1 and LDLR expressions are dependent on an intact P2Y[subscript]2R, and P2Y[subscript]2R/ FLN‐ A interaction is necessary for agLDL uptake.

Molecular Biology (0307)

Nutrition (0570)

Identifizierung und Charakterisierung exogener und endogener endothelialer Faktoren für die Ätiopathogenese der Atherosklerose

Tölle, Markus

31 May 2006

Für die Ätiopathogenese der Atherosklerose spielen eine Vielzahl von Mediatoren eine Rolle. Dabei werden durch das Endothel sowohl protektive als auch schädliche Mediatoren sezerniert. High Density Lipoproteine (HDL) stellen einen bedeutenden protektiven Marker für das kardiovaskuläre Risiko dar, u.a. durch die Aktivierung der endothelialen NO-Synthase (eNOS). HDL besteht zu 50 % aus Proteinen und zu 50 % aus Lipiden. Welche Komponenten des HDL für die eNOS Aktivierung verantwortlich sind, ist nicht bekannt gewesen. Im ersten Abschnitt dieser Promotionsarbeit konnte erfolgreich gezeigt werden, dass die Lysophospholipide, Sphingosin-1-Phosphat (S1P) und Sphinsosylphosphorylcholin (SPC), die strukturelle Bestandteile der Lipidfraktion von HDL darstellen, für einen Teil der HDL induzierten eNOS Aktivierung durch Stimulation des S1P3-Rezeptors verantwortlich sind. Diese eNOS Aktivierung wird durch den intrazellulären Einstrom von Calcium und durch die Aktivierung der Akt-Kinase induziert. Im zweiten Abschnitt dieser Promotionsarbeit konnte nachgewiesen werden, dass das oral verfügbare Lysophospholipid-basierte Medikament, FTY720, das ein strukturelles Analogon des S1P ist, den HDL induzierten Signaltransduktionsweg der eNOS Aktivierung in gleicher Weise induziert. Im dritten Abschnitt dieser Promotionsarbeit konnte ein neuartiges endothelabhängig sezerniertes gemischtes Dinukleosidpolyphosphat, Uridin-Adenosin-Tetraphosphat (Up4A), identifiziert werden. Up4A ist ein Agonist an den P2X- und P2Y-Purinrezeptoren. Up4A induziert bei Applikation in eine isoliert perfundierte Rattenniere hauptsächlich über die Aktivierung des P2X1-Rezeptors und des P2Y2/P2Y4-Rezeptors eine starke Vasokonstriktion im renalen Perfusionsgebiet mit einhergehender Erhöhung des mittleren renalen Perfusionsdrucks. Die direkte Infusion von Up4A in vivo in eine WKY-Ratte führt zu einer signifikanten Erhöhung des mittleren arteriellen Blutdrucks. / In the pathogenesis of atherosclerosis many mediators are included. Therefore the endothelium plays a crucial part by secreting protective but also deleterious factors. High density lipoproteins are an established protective factor in the risk profile of cardiovascular events especially by activating the endothelial NO synthase (eNOS). HDL is composed of 50 % proteins and 50 % lipids. Which component of HDL is responsible for the eNOS activation was not known. In the first part of this dissertation it could be shown, that the lysophospholipids, sphingosine-1-phosphate (S1P) and sphingosylphosphorylcholine (SPC), which are structural compounds of the lipid fraction of HDL, are responsible for a significant part of the HDL induced eNOS activation by stimulating the specific S1P3 receptor. In the signal transduction mechanism the activation of Akt kinase and an influx of calcium is involved. In the second part of this dissertation it could be shown, that the orally active lysophospholipide based drug FTY720, which is a structural analogue of S1P, is able to induce the same signal transduction mechanism activated by HDL including the stimulation of the S1P3 receptor. In the last part of this dissertation a new endothelium dependent vasoconstrictor, the dinucleoside polyphosphate uridine-adenosine-tetraphosphate (Up4A), could be for the first time identified. Up4A is a potent agonist of the P2X- and P2Y-purinoceptors. Via activating the P2X1 receptor and the P2Y2/P2Y4 receptor Up4A induce a strong vasoconstriction in the renal perfusion system in the model of the isolated perfused rat kidney with an adjacent increase of the mean perfusion pressure. By injection of Up4A in vivo in a Wistar Kyoto rat the mean arterial pressure also increase significantly.

Atherosklerose

endotheliale NO-Synthase

High Density Lipoprotein

Lysophospholipide

Sphingosin-1-Phosphat

Sphingosylphosphorylcholin

S1P3-Rezeptor

Dinukleosidpolyphosphat

Uridin-Adenosin-Tetraphosphat

P2X1-Rezeptor

P2Y2-Rezeptor

P2Y4-Rezeptor

atherosclerosis

endothelial NO synthase

High Density Lipoprotein

lysophospholipide

sphingosine-1-phosphate

sphingosylphosphorylcholine

S1P3 receptor

dinucleoside polyphosphate

uridine-adenosine-tetraphosphate

P2X1 receptor

P2Y2 receptor

P2Y4 receptor

610 Medizin

33 Medizin

YC 1104

YC 1118

ddc:610

Efeito da imunização com enzimas recombinantes do metabolismo de nucleotídeos de Schistosoma mansoni sobre o desenvolvimento da esquistossomose mansônica experimental

Neris, Débora Meira

29 August 2012

Made available in DSpace on 2016-08-17T18:39:46Z (GMT). No. of bitstreams: 1 5245.pdf: 1568165 bytes, checksum: 9fc25ff9dc83339e50628c08854efd2c (MD5) Previous issue date: 2012-08-29 / Universidade Federal de Sao Carlos / Schistosimiasis mansoni is a neglected chronic parasitic disease that affects thousands of people worldwide, caused by the trematode Schistosoma mansoni. In the infected host the disease is characterized by the presence of granuloma, imunnopathological response of the cellular infiltration against egg antigens. Thus, the host-parasite relation favors hepatosplenomegaly, acite and hepatic fibrosis. Current chemotherapy is based on the use of Praziquantel (PZQ), used against all species of Schistosoma spp for over 30 years. The main issue is that the PZQ is practically inactive against immature schistosomula and favors the resistance growth of the existent lineages, which makes the study for new drugs and vaccines that can contribute to the control of this disease even more urgent. One of the paths on the search for new therapeutic targets is the study of essential enzymes to the S. mansoni. In particular, it is known that the enzymes Adenylate Kinase 1 and 2 (ADK), Uridine cytidine Kinase 1 and 2 (UCK), Hypoxanthine guanine phosphoribosyltransferase (HGPRT) e Purine nucleoside phosphorilase 1 (PNP) are found on the metabolic pathways of the parasite s nucleotide, participating in the metabolism of purines and pyrimidines. Our goals in this study were to assess the immunization with these enzymes, using the S. mansoni cercariae infected murine model, and subsequently analyze the acting in oviposition and growth of adult worms. Our results showed that the immunization in Balb/c mice with the UCK enzyme was capable of inducing a specific immune response, which favored a significant reduction of the parasitic load (adult worms). However, it was not possible to observe significant reduction in the number of eliminated eggs. Regarding the immunization with PNP and HGPRT enzymes, the mice had a reduction in the number of eggs per gram of feces. The data obtained are considered interesting and can be new targets for immunotherapy against schistosomiasis mansoni. Thereby, new assays must be made with different dosages of the enzymes for a better assessment on how these enzymes modulate the parasitic load through the eggs reduction, reduction in the adult worms retrieving, as well as the antibody levels during the murine infection by the S.mansoni. / A esquistossomose mansônica é uma doença parasitária, crônica e negligenciada que afeta milhares de pessoas ao redor do mundo, causada pelo trematódeo Schistosoma mansoni. No hospedeiro infectado a doença é caracterizada pela presença do granuloma, resultado imunopatológico do infiltrado celular contra antígenos dos ovos A quimioterapia atual é baseada no uso do Praziquantel (PZQ), usado contra todas as espécies de Schistosoma spp há mais de 30 anos. O principal problema é que o PZQ é praticamente inativo contra esquistossomulos imaturos e favorece o desenvolvimento de resistência das linhagens existentes. Um dos caminhos na busca por novos alvos terapêuticos é o estudo de enzimas que são essenciais para o S. mansoni. Em especial, sabe-se que as enzimas Adenilato Quinase 1 e 2 (ADK), Uridina Citidina Quinase 1 e 2 (UCK), Hipoxantina-guanina fosforibosiltransferase (HGPRT) e Purina Nucleosídeo Fosforilase 1 (PNP) são encontradas nas vias metabólicas de nucleotídeos do parasito, participando do metabolismo de purinas e pirimidinas. A estratégia de utilizar enzimas do parasito na esquistossomose mansônica murina foi de avaliar uma resposta induzida por estas enzimas quando aplicadas em camundongos BALB/c e desafiados com cercarias de S. mansoni. Desta forma, avaliamos a fase crônica de camundongos imunizados e infectados com S. mansoni, onde foram analisadas amostras parasitológicas, hematológicas, sorológicas e fluidos da cavidade peritoneal. Nosso objetivo neste estudo foi avaliar a imunização com essas enzimas, usando o modelo murino infectado com cercarias de S. mansoni e posteriormente avaliar a ação na oviposição e desenvolvimento de vermes adultos. Nossos resultados demonstraram que a imunização em camundongos Balb&#8725;c com a enzima UCK foi capaz de induzir uma resposta imune específica, a qual favoreceu a diminuição significativa da carga parasitária (vermes adultos). No entanto, não foi possível observar redução significativa no número de ovos eliminados. Em relação à imunização com as enzimas PNP e HGPRT os camundongos que receberam as imunizações com PNP e HGPRT tiveram redução no número de ovos por grama de fezes. Os dados obtidos são considerados interessantes e podem ser considerados novos alvos para a imunoterapia contra a esquistosomose mansônica. Dessa forma, novos ensaios deverão ser realizados com diferentes doses das enzimas para melhor avaliar como essas enzimas modulam a carga parasitária através da redução de ovos, diminuição na recuperação de vermes adultos, assim como os níveis de anticorpos durante a infecção murina pelo S. mansoni.

Biotecnologia

Imunização

Schistosoma mansoni

Purinas

Pirimidinas

Enzimas recombinantes

Esquistossomose mansônica

Adenilato Quinase 1 e 2

Uridina Citidina Quinase 1 e 2

Purina Nucleosídeo Fosforilase1

Schistosomiasis mansoni

Immunization

Purine nucleoside phosphorilase 1

OUTROS