Mécanismes de régulation de la NADPH Oxydase NOX1 : rôle de la phosphorylation de NOXA1 ( NOX Activator 1 ) et de NOXO1 ( NOX Organizer 1) / Regulation of the NADPH oxidase NOX1 : a crucial role of NOXA1 (NOX Activator 1) and NOXO1 (NOX Organizer 1) phosphorylation

Debbabi, Maya

16 December 2011

Les NADPH oxydases constituent une famille d’enzymes dont la fonction est dédiée à la production de formes réactives de l’oxygène. NOX1, un des membres de cette famille, est abondamment exprimée dans le colon et sa dérégulation pourrait être associée aux maladies inflammatoires chroniques de l’intestin. Les mécanismes qui modulent l’activation de NOX1 demeurent mal connus. Au cours de ma thèse je me suis donc intéressée à l’étude de la phosphorylation de NOXA1 et NOXO1, deux sous-unités régulatrices du complexe NOX1 et ai démontré 1) que la phosphorylation de NOXA1 constitue un mécanisme de régulation négative de l’activité de NOX1 en vue de maintenir l’activité constitutive du complexe à un niveau adéquat et non excessif. 2) pour la première fois, que NOXO1β est phosphorylée et que cette phosphorylation entraîne une hyperactivation de NOX1. L’ensemble de ces données montre que NOX1 est finement régulée. Par ce biais, NOX1 pourrait être impliquée dans la défense anti-infectieuse de l’intestin. / The NOX family of NADPH oxidases are enzymes which function is dedicated to the production of reactive oxygen species. NOX1, a member of this family is expressed abundantly in the intestine and its disregulation could be linked to inflammatory diseases such as inflammatory bowel diseases. However, the molecular basis of NOX1 regulation remains unclear. During my thesis, I demonstrated that 1) NOXA1, the activator cytosolic subunit of the NOX1 complex, is phosphorylated and its phosphorylation prevents hyperactivation of NOX1 in order to maintain a constitutive activity which would not be too excessive. 2) phosphorylation of human NOXO1, the organizer subunit of the complex is a prerequisite of full activation of NOX1. Taken together, these results demonstrate that NOX1 is tightly regulated by phosphorylation events. By this mean, NOX1 could be involved in host immune defense of the intestine.

NOX1

FRO

Inflammation

Phosphorylation

NOXA1

NOXO1

Régulation

NOX1

Inflammation

Phosphorylation

NOXA1

NOXO1

Regulation mechanism

Reactive oxygen species

Efeito da carnosina na prevenção de crioinjúrias no sêmen de garanhões bons e maus congeladores / Effect of carnosine on the protection against cryoinjuries in semen of good and bad freezers\' stallions

Kawai, Giulia Kiyomi Vechiato

03 March 2017

As espécies reativas de oxigênio são fundamentais na fisiologia espermática. No entanto, um desequilíbrio entre a produção e a capacidade antioxidante caracteriza o estresse oxidativo (EO). O espermatozoide é extremamente suscetível ao EO pois, dentre outras características, a membrana plasmática é rica em ácidos graxos poli-insaturados responsáveis por promoverem a fluidez necessária em processos fisiológicos como motilidade e fertilização. Por outro lado, essas insaturações são mais facilmente oxidadas e vulneráveis à peroxidação lipídica. Em função desta susceptibilidade, estas células dependem fortemente de compostos presentes no plasma seminal (PS) para a proteção contra esse evento. Dessa forma, a carnosina, dipeptídeo presente no PS pode ser uma das responsáveis pela proteção contra o acúmulo do MDA. No entanto, durante a criopreservação do sêmen equino é necessário retirar o PS. Em estudo recente, verificamos que esta remoção, torna os espermatozoides sensíveis ao subproduto extremamente deletério da peroxidação lipídica, o malondialdeído (MDA). Como a carnosina é removida junto com o plasma seminal durante a criopreservação, foram desenvolvidos 2 experimentos sequenciais visando a melhora da qualidade do sêmen criopreservado com adição de carnosina. Amostras de sêmen de sete garanhões foram tratadas com concentrações crescentes de carnosina adicionadas ao diluidor (1mM, 50mM e 100mM). Após a descongelação, as amostras foram divididas retrospectivamente em grupos de alta congelabilidade (AC: motilidade maior que 30%) e baixa congelabilidade (BC: motilidade menor que 30%). Amostras tratadas com 50mM apresentaram menor porcentagem de células com lesão de membrana plasmática e, quando tratadas com 100mM, células com maior amplitude do deslocamento lateral de cabeça. Amostras controle BC apresentaram menor porcentagem de células com DNA íntegro em relação às amostras AC. No entanto, houve um leve aumento na porcentagem de células com DNA íntegro em amostras BC com 100mM, não diferindo das amostras AC. Por outro lado, amostras BC criopreservadas com 50mM apresentaram maiores porcentagens de células com escore calculado de potencial de membrana mitocondrial e mais suscetíveis ao EO em relação ao controle. Apesar da proteção parcial, a maior suscetibilidade à peroxidação lipídica torna-se um problema, especialmente pelo fato de que espermatozoides equinos são mais suscetíveis ao MDA. Um motivo para este efeito seria a afinidade da carnosina em reagir com açúcares, o que poderia influenciar negativamente a atividade mitocondrial e o status oxidativo, ao diminuir a produção de piruvato pela via glicolítica. Desta forma, no experimento 2, amostras BC foram tratadas com a combinação de carnosina (0 e 50mM) e piruvato (0 e 5mM) em arranjo fatorial 2x2. Verificou-se que o tratamento com piruvato (5mM) proporcionou menos células com baixa atividade mitocondrial. Por outro lado, a carnosina (50mM), promoveu maior motilidade total, progressiva e células rápidas. Houve uma tendência de aumento nas células com velocidade progressiva e atividade mitocondrial na combinação de tratamentos. Não houve diferença entre os grupos na suscetibilidade ao EO que, no entanto, correlacionou-se negativamente com células móveis, rápidas e integridade de membrana plasmática e acrossomal. Estes resultados indicam que subprodutos da peroxidação lipídica, sendo o principal deles o MDA, podem causar danos ao DNA, às mitocôndrias e à cinética espermática. Neste contexto, a carnosina (100mM) parece ter um leve efeito protetor ao DNA contra o acúmulo de MDA. Além disto, 50mM de carnosina parece auxiliar na manutenção da velocidade progressiva e atividade mitocondrial quando associada ao piruvato (5mM). Assim, a carnosina e o piruvato podem ser utilizados na prevenção de crioinjúrias em amostras de baixa congelabilidade. / Reactive oxygen species (ROS) plays a key role in the sperm physiology. However, an imbalance between ROS production and antioxidant capacity characterize the oxidative stress (OE). The spermatozoa are extremely susceptible to EO because, among other characteristics, the plasma membrane is rich in polyunsaturated fatty acids responsible for promoting fluidity necessary in physiological processes such as motility and fertilization. However, these unsaturations are more easily oxidized and vulnerable to lipid peroxidation. Due to this susceptibility, these cells strongly depend on compounds present in the seminal plasma (SP) to protect against this event. Thus, carnosine, a dipeptide present in SP of stallions, may be a key factor on the protection against MDA accumulation. Nevertheless, during the equine sperm cryopreservation process, SP is removed. In a recent study, we observed that seminal plasma removal led to an increased susceptibility of equine spermatozoa to extremely deleterious product of lipid peroxidation, malondialdehyde (MDA). As the carnosine is removed together with the seminal plasma during cryopreservation, two sequential experiments were developed aiming to improve the quality of stallion cryopreserved semen by means of carnosine therapy. Samples from seven stallions were treated with increasing concentrations of carnosine added to the extender (1mM, 50mM and 100mM) and submitted to cryopreservation. After thawing, samples were classified as high freezeability (HF: total motility greater than 30%) and low freezeability (LF: total motility lower than 30%). Samples treated with 50mM presented lower percentage of sperm showing plasma membrane damage and, when treated with 100mM, a greater amplitude of the lateral head displacement was observed. Untreated LF samples showed a lower percentage of cells showing intact DNA in relation to HF samples. By contrast, when LF samples were treated with 100mM, there was an increase in the percentage of cells with intact DNA, which was similar to the HF samples. On the other hand, LF samples cryopreserved with 50mM had a higher percentage of cells showing high calculated mitochondrial membrane potential score and increased susceptibility to OE in relation to the control. Despite the partial protection, the increased susceptibility to lipid peroxidation is a concern since equine spermatozoa is highly vulnerable to the MDA. Those results could be due to the affinity of carnosine to react with sugars, which could negatively influence mitochondrial activity and an oxidative state by decreasing pyruvate production. Hence, in experiment 2, LF samples were treated with a combination of carnosine (0 and 50mM) and pyruvate (0 and 5mM) in a 2x2 factorial arrangement. We observed that samples treated with pyruvate (5mM) had decreased percentage of cells with low mitochondrial activity. On the other hand, carnosine (50mM) increased total motility, progressive motility and fast cells. We also observed a tendency to increased progressive velocity and mitochondrial activity in the combination of treatments. There was no difference on sperm susceptibility to OE between treatments. However, this variable correlated negatively with the percentage of motile and rapid cells as well as those showing intact membrane and acrosome. These results indicate that the byproduct of lipid peroxidation (MDA) may cause damage to DNA, mitochondria and sperm kinetics. In this context, carnosine (100mM) appears to have a mild protective effect on DNA against the accumulation of MDA. Furthermore, 50mM of carnosine seems to improve progressive velocity and mitochondrial activity when associated with pyruvate (5mM). Thus, carnosine and pyruvate can be used on cryoinjuries prevention in low freezeability samples.

Carnosina

Carnosine

Criopreservação espermática

Equine sperm

Espécies reativas de oxigênio

Malondialdehyde

Malondialdeído

Reactive oxygen species

Sêmen equino

Sperm cryopreservation

Optical probes for enhanced targeting of cancer

García Guzmán, Claudia María

January 2017

The diagnosis of cancer in early stages is an unmet clinical need, especially in view that current treatments for cancer cannot address metastatic disease. Cancer aberration processes are associated to an increase in the production of reactive oxygen species (ROS). Chemical probes that can specifically detect these species are potentially useful as medical diagnostics and research tools for cancer imaging. One of the aims of my thesis was the design and synthesis of the activatable fluorescent probes based on small molecule fluorophores modified with chemically reactive moieties. The activation of these moieties by defined targets (e.g. ROS) results in the activation of the fluorophore and subsequent emission of a fluorescent signal. Two libraries of fluorescence probes for the detection of ROS have been designed and synthesised: 1) hydrocyanine-based probes as silent fluorophores that can be activated with superoxide ions, 2) coumarin-based hydrogen peroxide probes with red-shifted fluorescent properties and different boronate activatable groups for hydrogen peroxide sensing. We have performed in vitro assays to evaluate the fluorescence response of our probes as well as experiments in relevant live cells to assess their application for detection of ROS in live cells with molecular resolution. Moreover, cancer cells also overexpress Epidermal Growth Factor Receptors (EGFR). Surface-enhanced Raman scattering (SERS) nanotags that can recognize specifically EGFR receptors in cells are promising tools for the enhanced diagnosis of cancer. Two near-infrared cyanine Raman reporters were synthesized with a carboxylic group that was conjugated to cysteamine for derivatization of gold nanoparticles (AuNPs). This work was performed in the CSIR-NIIST (Kerala, India), where I did a 3-month PhD placement. I conjugated the cyanine reporters to spherical AuNPs of 40 nm diameter, and measured their Raman intensity and stability. The best SERS nanotags were selected for encapsulation with PEG and subsequently derivatization with anti-EGFR-EP22 antibodies. In vitro characterization of the SERS nanotags was performed: SERS and absorbance spectra, electron microscopy images as well as SERS imaging experiments in A549 lung cancer cells.

Etude de l’effet antibactérien de surfaces traitées à l'aide de composés du titane et de leur applicabilité dans les industries agroalimentaires / Study of the antibacterial effect of surfaces treated with titanium compounds and their applicability in the agro-food industries

Barthomeuf, Marion

26 October 2017

Les biofilms en industries agroalimentaires (IAA) représentent un problème récurrent aux conséquences économiques et de sécurité sanitaire. Le développement de surfaces photoactives aux propriétés antibactériennes pourrait faciliter leur élimination. Une solution serait de déposer une couche mince de dioxyde de titane (TiO2) sur des matériaux rencontrés dans les IAA. Les objectifs de cette thèse ont donc été d’optimiser des couches minces de TiO2 aux propriétés antibactériennes et d’étudier les mécanismes impliqués dans la photocatalyse. Les dépôts sont réalisés par pulvérisation cathodique radiofréquence dans différentes conditions (température, PO2, durée), d’abord sur substrat de verre puis sur acier inoxydable 316La caractérisation des couches minces par microscopie à balayage, diffraction des rayons X, a montré des différences dues au changement de substrat. Les différentes optimisations ont conduit à l’obtention de couches minces possédant une activité photocatalytique et des propriétés antibactériennes sur des souches représentatives de la flore retrouvée dans les IAA de la filière « viande » : L. monocytogenes, Y. enterocolitica et P. fragi. Des diminutions de la population bactérienne entre 1,5Log et 3Log ont été observées. La production d’espèces réactives de l’oxygène (H2O2, ¿OH, O2-¿) a été étudiée par des méthodes spectrocolorimétriques. L’H2O2 à la surface de la couche mince serait converti en ¿OH. L’étude des mécanismes de réponse de L. monocytogenes face à la photocatalyse des couches minces a été initiée par une approche transcriptomique, en suivant l’exp / Biofilms in food industries represent a recurrent problem with economic and health safety implications. The development of photoactive surfaces with antibacterial properties could facilitate their elimination. One solution would be to deposit a thin layer of titanium dioxide (TiO2) on conventional materials used in food plants. The objectives of this thesis were the optimization of thin films of TiO2 with antibacterial properties and to study the mechanisms involved in photocatalysis. Deposits were made by radio-frequency sputtering under different conditions (temperature, oxygen partial pressure, duration), first on a glass substrate and then on 316 stainless steel. Characterization of thin layers by scanning microscopy, diffraction of X-ray, showed differences due to substrate changeTiO2 thin layers obtained either on glass or stainless steel showed photocatalytic and antibacterial properties on representative strains of the flora found in the meat industry: Listeria monocytogenes, Yersinia enterocolitica and Pseudomonas fragi. Decreases in the bacterial population between 1.5Log and 3Log were observed. The production of reactive oxygen species (ROS) was studied by spectrocolorimetric methods. It seems that H2O2 on the surface is converted in another ROS, ¿OH. Finally, the study of the bacterial response mechanisms to photocatalysis, especially for L. monocytogenes, was initiated by a transcriptomic approach by following the expression of genes involved in the response to oxidative stress. However, the method used requires an optimization in order to be used for the bac

Photocatalyse

TiO2

Iaa

Bactéries

Biofilm

Espèces réactives de l’oxygène.

Photocatalysis

TiO2

Agro-Food industries

Bacteria

Biofilm

Reactive oxygen species.

Estresse oxidativo em membranas de eritrócito avaliado por ressonância paramagnética eletrônica / Oxidative stress in erythrocyte membranes evaluated by electron spin resonance

Mendanha Neto, Sebastião Antônio

26 March 2010

Submitted by Luciana Ferreira (lucgeral@gmail.com) on 2014-08-15T11:21:25Z No. of bitstreams: 2 license_rdf: 23148 bytes, checksum: 9da0b6dfac957114c6a7714714b86306 (MD5) Dissertacao Sebastiao Antonio Mendanha Neto.pdf: 1242328 bytes, checksum: d0f39ae03faaec981292f99cefebb8ea (MD5) / Made available in DSpace on 2014-08-15T11:21:25Z (GMT). No. of bitstreams: 2 license_rdf: 23148 bytes, checksum: 9da0b6dfac957114c6a7714714b86306 (MD5) Dissertacao Sebastiao Antonio Mendanha Neto.pdf: 1242328 bytes, checksum: d0f39ae03faaec981292f99cefebb8ea (MD5) Previous issue date: 2010-03-26 / Conselho Nacional de Pesquisa e Desenvolvimento Científico e Tecnológico - CNPq / The oxidative stress effects promoted by hydrogen peroxide (H2O2) and 2,2 -Azobis(2- methylpropionamidine)dihydrochloride (AAPH) in proteins and lipids of the erythrocyte membrane were investigated by testing the oxidative hemolysis, the formation of malondialdehyde (MDA) in addition to spectroscopic electron paramagnetic resonance (EPR) of lipid spin label 5-DOXIL stearic acid (5-DSA) and 3-maleimide proxyl (5-MSL) that binds covalently to erythrocyte s membrane proteins. The spectral parameter 2Ak obtained directly from the EPR spectra of spin label 5-DSA structured in the lipid bilayer of the erythrocyte membrane was sensitive to changes in the dynamics of lipids resulting on the oxidation of membrane proteins. The oxidation of proteins observed for very low concentrations of H2O2 (starting at 100 μM) were confirmed with spin label 5-MSL. Lipid peroxidation indicated the oxidative hemolysis and formation of MDA occurred at concentrations of H2O2 about 8 times larger (starting at 800 μM). Ascorbic acid and -tocopherol protect the membrane by hemolysis and MDA tests, but did not prevent the stiffening of the erythrocyte membrane. The spectra of the spin label 5-MSL revealed the existence of two distinct thiol groups in erythrocyte membrane proteins that differ in their structural configurations and sensitivity to oxidative attack. The SH site that has higher exposure to solvent and less reactivity to spin label 5-MSL was the most vulnerable to oxidation. It is well known that upon oxidation hemoglobin binds to the membrane and the results of this study suggest that this effect may be accompanied by a further increase in the parameter 2Ak of the spin label 5-DSA. Catalase present in erythrocytes proved to be an effective protector of lipid peroxidation and oxidation of membrane proteins induced by hydrogen peroxide. / Os efeitos do estresse oxidativo promovido pelo peróxido de hidrogênio (H2O2) e pelo 2,2 -Azobis(2-metilpropanamida) dicloridrato (AAPH) nas prote´ınas e lipídios da membrana de eritrócito foram investigados através do teste da hemólise oxidativa, da formação do malondialde ıdo (MDA) além da espectroscopia de ressonância paramagnética eletrônica (RPE) do marcador de spin lipídico 5-DOXIL estearato (5-DSA) e do marcador de spin 3-maleimida proxil (MAL-5) que se liga covalentemente `as proteínas da membrana de eritrócito. O parâmetro espectral 2Ak obtido diretamente dos espectros de RPE do marcador de spin 5-DSA estruturado na bicamada lipídica da membrana de eritrócito foi sensíıvel `as alterações na dinâmica dos lipídios resultantes da oxidação das proteínas da membrana. A oxidação das proteínas observada para concentrações baixas de H2O2 (a partir de 100 μM) foram confirmadas com o marcador MAL-5. A peroxidação lipídica indicada pela hemólise oxidativa e formação de MDA ocorreu em concentrações de H2O2 cerca de 8 vezes maiores (a partir de 800 μM). O ácido ascórbico e alfa-tocoferol protegem a membrana pelos testes de hemólise e MDA, mas não evitaram o enrijecimento da membrana do eritrócito. Os espectros do marcador MAL-5 revelaram a existência de dois grupos tióis distintos nas proteínas da membrana de eritrócito que diferem quanto a suas configurações estruturais e sensibilidade aos ataques oxidativos. O sítio SH de maior exposiçãoo ao solvente e menor reatividade ao marcador MAL-5 foi o mais vulnerável `a oxidação. É bem conhecido que neste processo oxidativo a hemoglobina se liga à membrana e os resultados deste trabalho sugerem que este efeito pode ser acompanhado por um aumento adicional no parâmetro 2Ak do marcador 5-DSA. A catalase presente nos eritrócitos se revelou como um eficiente protetor da oxidação lipídica e protéica da membrana induzidas por H2O2.

Espécies reativas de oxigênio

Radicais livres

Ressonância paramagnética eletrônica

Reactive oxygen species

Free radicals

Electron paramagnetic resonance

CIENCIAS EXATAS E DA TERRA::FISICA

Disfunção mitocondrial no tecido adiposo perivascular e seu papel nas alterações vasculares em modelo experimental de obesidade / Mitochondrial dysfunction in perivascular adipose tissue and its role in obesity-associated vascular changes

Rafael Menezes da Costa

18 December 2015

A obesidade desencadeia mudanças estruturais e funcionais no tecido adiposo perivascular (PVAT), levando a um desequilíbrio em favor de substâncias vasoconstritoras e pró- inflamatórias, bem como alterações em suas vias de sinalização no vaso. Um importante mecanismo proposto para explicar a perda do efeito anticontrátil do PVAT na obesidade é o estresse oxidativo. Espécies reativas de oxigênio (EROs) possuem papel importante na modulação da função vascular mediada pelo PVAT. Considerando que a mitocôndria representa fonte potencial de EROs nas células, o presente estudo testou a hipótese que a disfunção mitocondrial no PVAT está envolvida na perda do efeito anticontrátil do PVAT em modelo experimental de obesidade. Este estudo avaliou se a matriz mitocondrial nas células que compõem o tecido adiposo periaórtico representa fonte importante de EROs, e se as mesmas contribuem para as alterações na regulação, pelo PVAT, da reatividade vascular. Nosso estudo demonstrou que animais obesos apresentaram disfunção vascular e perda do efeito anticontrátil do PVAT. O estresse oxidativo está envolvido na disfunção do PVAT, com participação significativa da mitocôndria na geração de EROs, capazes de modular a reatividade vascular. A obesidade favoreceu a disfunção mitocondrial, reduzindo o consumo de oxigênio. Estes eventos favoreceram o aumento na geração de peróxido de hidrogênio mitocondrial no PVAT, o qual prejudica a ação anticontrátil deste tecido por ser ativador direto da via de contração RhoA/Rho cinase / Obesity promotes structural and functional changes in the perivascular adipose tissue (PVAT), favoring the release of vasoconstrictor and proinflammatory substances, as well as altering the vascular signaling pathways activated by PVAT-derived factors. Oxidative stress is an important mechanism proposed to explain the loss of anticontractile effects of the PVAT in obesity. Reactive oxygen species (ROS) play an important role in the modulatory effects of PVAT on vascular function. Considering that mitochondria are a potential source of ROS in the cells, the present study tested the hypothesis that mitochondrial dysfunction leads to the loss of the anticontractile effects of PVAT in obesity. We evaluated whether the mitochondrial matrix of the cells that make up the periaortic fat tissue constitute a major source of ROS, and if mROS contribute to defective regulation of vascular reactivity by the PVAT. Our study shows that obese animals exhibit vascular dysfunction and loss of anticontractile effects of PVAT. Oxidative stress is involved in PVAT dysfunction, with a significant contribution of mitochondria to ROS generation. Obesity promotes mitochondrial dysfunction, reducing oxygen consumption. These events increase the generation of mitochondrial hydrogen peroxide in the PVAT, which impairs the anticontractile effects of this tissue via direct activation of the RhoA / Rho kinase pathway

Espécies reativas de oxigênio

Mitocôndria

Obesidade

Reatividade vascular

Tecido adiposo perivascular

Mitochondria

Obesity

Perivascular adipose tissue

Reactive oxygen species

Vascular reactivity

Disfunção mitocondrial no tecido adiposo perivascular e seu papel nas alterações vasculares em modelo experimental de obesidade / Mitochondrial dysfunction in perivascular adipose tissue and its role in obesity-associated vascular changes

Costa, Rafael Menezes da

18 December 2015

A obesidade desencadeia mudanças estruturais e funcionais no tecido adiposo perivascular (PVAT), levando a um desequilíbrio em favor de substâncias vasoconstritoras e pró- inflamatórias, bem como alterações em suas vias de sinalização no vaso. Um importante mecanismo proposto para explicar a perda do efeito anticontrátil do PVAT na obesidade é o estresse oxidativo. Espécies reativas de oxigênio (EROs) possuem papel importante na modulação da função vascular mediada pelo PVAT. Considerando que a mitocôndria representa fonte potencial de EROs nas células, o presente estudo testou a hipótese que a disfunção mitocondrial no PVAT está envolvida na perda do efeito anticontrátil do PVAT em modelo experimental de obesidade. Este estudo avaliou se a matriz mitocondrial nas células que compõem o tecido adiposo periaórtico representa fonte importante de EROs, e se as mesmas contribuem para as alterações na regulação, pelo PVAT, da reatividade vascular. Nosso estudo demonstrou que animais obesos apresentaram disfunção vascular e perda do efeito anticontrátil do PVAT. O estresse oxidativo está envolvido na disfunção do PVAT, com participação significativa da mitocôndria na geração de EROs, capazes de modular a reatividade vascular. A obesidade favoreceu a disfunção mitocondrial, reduzindo o consumo de oxigênio. Estes eventos favoreceram o aumento na geração de peróxido de hidrogênio mitocondrial no PVAT, o qual prejudica a ação anticontrátil deste tecido por ser ativador direto da via de contração RhoA/Rho cinase / Obesity promotes structural and functional changes in the perivascular adipose tissue (PVAT), favoring the release of vasoconstrictor and proinflammatory substances, as well as altering the vascular signaling pathways activated by PVAT-derived factors. Oxidative stress is an important mechanism proposed to explain the loss of anticontractile effects of the PVAT in obesity. Reactive oxygen species (ROS) play an important role in the modulatory effects of PVAT on vascular function. Considering that mitochondria are a potential source of ROS in the cells, the present study tested the hypothesis that mitochondrial dysfunction leads to the loss of the anticontractile effects of PVAT in obesity. We evaluated whether the mitochondrial matrix of the cells that make up the periaortic fat tissue constitute a major source of ROS, and if mROS contribute to defective regulation of vascular reactivity by the PVAT. Our study shows that obese animals exhibit vascular dysfunction and loss of anticontractile effects of PVAT. Oxidative stress is involved in PVAT dysfunction, with a significant contribution of mitochondria to ROS generation. Obesity promotes mitochondrial dysfunction, reducing oxygen consumption. These events increase the generation of mitochondrial hydrogen peroxide in the PVAT, which impairs the anticontractile effects of this tissue via direct activation of the RhoA / Rho kinase pathway

Espécies reativas de oxigênio

Mitochondria

Mitocôndria

Obesidade

Obesity

Perivascular adipose tissue

Reactive oxygen species

Reatividade vascular

Tecido adiposo perivascular

Vascular reactivity

Alterações na homeostase redox das células beta pancreáticas em resposta à glicose. / Modulation of the redox state by glucose in pancreatic beta cells.

Valle, Maíra Mello Rezende

02 October 2014

As espécies reativas de oxigênio são capazes de influenciar a secreção de insulina, porém ainda não está clara a influência da glicose, principal secretagogo deste hormônio, sobre a homeostase redox das células beta pancreáticas. Incubações por 1 e 48 horas com diferentes concentrações de glicose (2,8; 5,6; 8,3; 11,1; 16,7 e 20 mM) demonstraram que esta é capaz de alterar não só o conteúdo de superóxido, produzido pela mitocôndria e NADPH oxidase, mas também o sistema antioxidante, alterando a concentração de GSH e a expressão das enzimas antioxidantes. Além disso, aumenta a interação Rac1/Sod1, que mantém a NADPH oxidase ativa. Porém, não apresenta endossomas de sinalização redox, os redoxossomas, em resposta a glicose. Estas alterações podem afetar eventos chave para este tecido endócrino, como a secreção de insulina e a morte celular. / ROS production in pancreatic beta cells has been associated with the insulin secretion process but the mechanism by which glucose affects the redox state in these cells remains unknown. In order to address this issue, we evaluated the effect of 1 or 48 hours incubation of pancreatic beta cells with various glucose concentrations (2.8, 5.6, 8.3, 11.1, 16.7 and 20 mM). Glucose loading induced superoxide production by mitochondria and NADPH oxidase complex, and enhanced the antioxidant capacity by increasing GSH content and modulate expression of antioxidant enzymes. Glucose also promoted Rac1/Sod1 interaction that maintains NADPH oxidase activated. These cells however did not present redox endosomes, the redoxosomes, in response to glucose loading. These effects might be associated with the process of insulin secretion and pancreatic beta cell death.

Espécies reativas de oxigênio

Glicose

Glucose

Ilhotas pancreáticas

Nox2

Nox2

Pancreatic islets

Rac1

Rac1

Reactive oxygen species

Sod1

Sod1

Superoxide

Superóxido

Efeitos do ácido ascórbico nos biomarcadores de estresse oxidativo induzido por exercício físico exaustivo / Effects of ascorbic acid on oxidative stress biomarkers induced by exhaustive exercise

Picchi, Monike Garlipp

18 May 2015

O objetivo deste estudo foi avaliar os efeitos da suplementação de vitamina C nos biomarcadores de estresse oxidativo induzido por exercício físico exaustivo. A amostra foi composta por 13 indivíduos do sexo masculino, fisicamente ativos, com idades entre 18 e 33 anos, IMC médio 23,65 ± 3,5 kg/m² e VO2max de 50,94 ± 5,2 ml.kg-1.min-1. Estes indivíduos foram submetidos a um protocolo de exercício exaustivo (40 minutos de corrida a 70-75% do VO2max, e aumento da velocidade para 90% do VO2max até a exaustão), randomizados duplo cego em duas fases (placebo X vitamina C). Na fase vitamina C eles ingeriram 500 mg de vitamina C por dia, durante 7 dias, antes do protocolo exaustivo, e na fase placebo eles ingeriram por sete dias placebo antes do mesmo protocolo. Foram coletadas amostras de sangue antes do exercício, logo após, 1h, 2h, 4h e 24h após para determinação dos biomarcadores de estresse oxidativo. As duas fases foram homogêneas, os indivíduos apresentaram consumo alimentar similar e não houve diferença na duração e intensidade do exercício. Os resultados mostram que o uso de suplemento de vitamina C favoreceu maiores níveis séricos de ácido ascórbico em relação ao placebo logo depois do exercício até 4 horas após, e por isso poupou a eliminação dos outros antioxidantes, -tocoferol e retinol, que estavam em menores concentrações séricas até 2 horas após o exercício, e do GSH, que se manteve em menores concentrações até 24 horas após. Enquanto com uso de placebo, já que os níveis de ácido ascórbico eram menores, houve uma maior liberação destes outros antioxidantes, e o -tocoferol e retinol começaram a ser consumidos 1 hora após o exercício, para combater os radicais livres formados, até 24 horas após. Apesar da CAT não ser alterada nem pela suplementação nem pelo exercício exaustivo, o FRAP foi maior na fase vitamina C e se manteve estável nas 24h após o exercício. O ácido úrico não apresentou diferença significativa, e seu uso foi poupado por outros antioxidantes séricos nas duas intervenções. Nas duas fases os indivíduos conseguiram combater os radicais livres formados pelo exercício exaustivo, já que os marcadores de peroxidação lipídica (MDA, TBARS e FOX) não aumentaram após o exercício em nenhuma das intervenções, não houve aumento de oxidação protéica (AOPP e PC). Os marcadores de lesão hepática (TGO), lesão muscular (CK) e tecidual (LDH) se comportaram de maneira igual com ou sem uso de vitamina C. As vantagens do uso adicional de vitamina C são: a maior proteção antioxidante desde o ínicio do exercício, já que apresenta maiores concentrações séricas de vitamina C e de FRAP, o menor grau de peroxidação lipídica, avaliado pelo MDA, o menor grau de oxidação protéica, avaliado pelas PC e a menor dependência do GSH como antioxidante endógeno. Sendo assim, uso de uma dose modesta de vitamina C, por um curto período de tempo, foi capaz de auxiliar na proteção antioxidante, sem nenhum efeito danoso aos indivíduos. / The objective of this study was to evaluate the effects of vitamin C supplementation on oxidative stress biomarkers induced by exhaustive exercise. The sample consisted of 13 males, physically active, aged 18 to 33 years, mean BMI 23.65 ± 3.5 kg/m² and 50.94 ± 5.2 VO2max ml.kg-1. min-1. These individuals were subjected to an exhaustive exercise protocol (40 minutes of running at 70-75% of VO2max, and increased speed to 90% VO2max until exhaustion), randomized double-blind in 2 phases (placebo X vitamin C). In vitamin C phase they ingested 500 mg vitamin C per day for 7 days before exhausting protocol and the placebo phase, they ingested placebo for 7 days prior to the same protocol. Blood samples were taken before exercise, immediately after, 1h, 2h, 4h and 24h after for determination of biomarkers of oxidative stress. The two phases were homogeneous, the subjects had similar food consumption and no difference in the duration and intensity of exercise. The results show that the use of vitamin C supplement favored higher serum levels of ascorbic acid relative to placebo soon after exercise to 4 hours after, and therefore spared the elimination of other antioxidants, -tocopherol and retinol, which were lower serum concentrations up to 2 hours after exercise, and GSH, which remained at lower levels within 24 hours. As with the use of placebo, as the ascorbic acid levels were lower, there was a greater release of these other antioxidants, and -tocopherol and retinol began to be consumed in 1 hour of exercise to combat free radicals formed by 24 hours. Despite the CAT not be altered or by supplementation or by exhaustive exercise, the FRAP was higher in vitamin C phase and remained stable in the 24 hours after exercise. Uric acid showed no significant difference, and its use has been spared by other serum antioxidants in 2 interventions. In 2 phases individuals able combat free radicals formed by exhaustive exercise, since the lipid peroxidation markers (MDA, TBARS and FOX) did not increase after exercise in any of the interventions, there was no increase in protein oxidation (AOPP and PC) . The markers of liver injury (AST), muscle damage (CK) and tissue (LDH) behaved equally with or without use of vitamin C. The advantages of the additional use of vitamin C are: the highest antioxidant protection since the beginning of exercise, since it has higher serum concentrations of vitamin C and FRAP, the lowest degree of lipid peroxidation, measured by MDA, the lowest level of protein oxidation, rated by PC and less dependent on GSH as an endogenous antioxidant. Thus, use of a modest dose of vitamin C, for a short period of time, was able to assist in antioxidant protection, with no harmful effect on individuals.

Antioxidantes

Antioxidants

Espécies reativas de oxigênio

Exercício exaustivo

Exhaustive exercise

Reactive oxygen species

Suplementação

Supplementation

Vitamin C

Vitamina C

Effects of Complex Formation of DNA with Positively Charged Polyamines and Polypeptides on the Products of Oxidative Damage to DNA 2-Deoxyribose by Hydroxyl Radicals

Tegomoh, Modeste N

01 December 2015

It is known that histones and other DNA-binding polycations protect DNA from radiation damage mediated by hydroxyl radicals. Until recently, this protection of DNA has mainly been attributed to compaction and aggregation. It was hypothesized that chemical repair of DNA sugar radicals by donation of hydrogen atom from polycations also significantly contributes to DNA protection. To test this hypothesis, the relative yields of low-molecular weight characteristic products of oxidation of DNA sugar were compared in X-irradiated samples of naked DNA and DNA complexes with a number of polycations by using an HPLC-based method of DNA damage product quantification. The variation in the percent contribution of the C1„ sugar damage product ongoing from free DNA to DNA-polycations complexes is in agreement with the hypothesis that chemical repair of DNA sugar radicals by donation of hydrogen atom from polycations contributes to the overall DNA protection against hydroxyl radical-mediated damage.

DNA damage

oxidative stress

reactive oxygen species

hydroxyl radicals

DNA protection

Life Sciences