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Calcium as the central mediator of muscle dysfunction due to muscular dystrophyMillay, Douglas P. 22 August 2008 (has links)
No description available.
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Towards the Regulation and Physiological Role of the Mitochondrial Calcium- Independent Phospholipase A<sub>2</sub>Rauckhorst, Adam J. January 2014 (has links)
No description available.
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Pharmacological Inhibition of Cyclophilin Ameliorates Experimental Allergic EncephalomyelitisHuang, Zi L 01 January 2016 (has links)
A subset of cyclophilins have been implicated in mechanisms of neuroinflammation and neurodegeneration that contributes to the pathogenesis of Multiple Sclerosis. Mitochondrial dysfunction leading to mitochondrial permeability transition plays a pivotal role in axonal damage and disease progression in Multiple Sclerosis. Cyclophilin D (CypD) is a crucial regulatory component of the mitochondrial permeability transition pore and it was demonstrated that the cyclophilin D knockout animals showed reduced experimental allergic encephalomyelitis (EAE) clinical disease severity and axonal injury. We investigated the effect of N-methyl-4-isoleucine-cyclosporin (NIM811), a non-immunosuppressive and non-selective cyclophilin inhibitor, on the course and severity of EAE. EAE mice treated with NIM811 showed a significant reduction in clinical disease severity compared to vehicle treated mice. FACS analysis performed with the dissociated thoracolumbar spine showed that NIM811 treatment was associated with a reduction in CNS macrophages but does not alter T-helper lineage frequencies. In addition, we demonstrated NIM811’s effect on crude mitochondrial fraction obtained from brain and liver homogenates of both wild type and CypD knockout mice in order to determine drug specificity. Benefits observed from the pharmacological inhibition of cyclophilin may lead to a novel MS therapy but NIM811’s exact mechanism of action has yet to be elucidated.
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Reactive oxygen species generated by phenylarsine oxide facilitate neurotransmitter release at developing Xenopus neuromuscular synapseChu, Ling-ya 29 June 2012 (has links)
Phenylarsine oxide (PAO) is a membrane-permeable trivalent arsenic compounds, which interfere the biochemical activity of intracellular enzymes or proteins through reacting specifically with sulfhydryl and vicinal dithiol groups in the protein structure. Although the deleterious effects of arsenic compounds in bioorganisms have been extensively studied, however its role in the synaptogenesis is still obscure. Here we test the role of PAO on the synaptic activity at developing Xenopus neuromuscular synapse by using whole-cell patch clamp recording. Bath application of PAO dose-dependently increases the frequency of spontaneous synaptic currents (SSC frequency) and reaches its maximal effect at 10 £gM. The SSC frequency is robustly facilitated in 10~15 minutes after PAO application and then the release of neurotransmitter were abruptly ceased due to the degenerative collapse of the presynaptic motoneuron. Pretreatment of the culture with Ca2+ chelator BAPTA-AM significantly blunted the SSC frequency facilitation induced by PAO, suggesting a rise in Ca2+ in presynaptic motoneuron is a prerequisite. The PAO-induced SSC frequency facilitation is unaffected even that Ca2+ is eliminated from culture medium or addition of pharmacological Ca2+ channel inhibitor cadmium, indicating the influx of extracellular Ca2+ is not needed for the rise of [Ca2+]i. Depletion of endoplasmic reticulum Ca2+ pool with thapsigargin effectively hampered the PAO-induced SSC frequency facilitation. Pretreatment of ryanodine receptor inhibitor TMB-8 but not IP3 receptor inhibitor XeC significantly occluded the increase of SSC frequency elicited by PAO. Furthermore, bath application of the culture with either mitochondria oxidative phosphorylation uncoupler FCCP or mitochondrial permeability transition pore inhibitor cyclosporin A significantly abolished the SSC facilitating effect of PAO. Pretreatment the culture with TMB-8 and cyclosporin A have no addictive effects on the occlusion of PAO-induced SSC frequency facilitation, suggesting a consecutively released Ca2+ from internal store through ryanodine receptor and mitochondria is responsible for PAO-induced SSC frequency facilitation.
The synaptic facilitating effect of PAO is eliminated while incubated with free radical scavenger n-acetylcysteine. Furthermore, treating cultures with complex III of electron transport chain (ETC) inhibitor antimycin A, but not complex I inhibitor rotenone, abolished PAO-induced facilitation of synaptic transmission. PAO elicited no facilitation effects on SSC frequency when pretreatment the culture with either thiol-modifying agent NEM or thiol-reducing agent DTT. Overall, results from our current study provide evidences that reactive oxygen species derived from PAO inhibition on complex III of ETC induce the open of MPT pore in mitochondria, the accompanied Ca2+ leak from mitochondria and Ca2+-induced Ca2+ release from endoplasmic reticulum resulted in a robustly release of neurotransmitter and a destructive damage on the neuron.
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Mechanism and Inhibition of Hypochlorous Acid-Mediated Cell Death in Human Monocyte-Derived MacrophagesYang, Ya-ting (Tina) January 2010 (has links)
Hypochlorous acid (HOCl) is a powerful oxidant produced by activated phagocytes at sites
of inflammation to kill a wide range of pathogens. Yet, it may also damage and kill the
neighbouring host cells. The abundance of dead macrophages in atherosclerotic plaques
and their colocalization with HOCl-modified proteins implicate HOCl may play a role in
killing macrophages, contributing to disease progression. The first part of this research was
to investigate the cytotoxic effect and cell death mechanism(s) of HOCl on macrophages.
Macrophages require efficient defense mechanism(s) against HOCl to function properly at
inflammatory sites. The second part of the thesis was to examine the antioxidative effects
of glutathione (GSH) and 7,8-dihydroneopterin (7,8-NP) on HOCl-induced cellular
damage in macrophages. GSH is an efficient scavenger of HOCl and a major intracellular
antioxidant against oxidative stress, whereas 7,8-NP is secreted by human macrophages
upon interferon-γ (IFN-γ) induction during inflammation and can also scavenge HOCl.
HOCl caused concentration-dependent cell viability loss in human monocyte derived
macrophage (HMDM) cells above a specific concentration threshold. HOCl reacted with
HMDMs to cause viability loss within the first 10 minutes of treatment, and it posed no
latent effect on the cells afterwards regardless of the HOCl concentrations. The lack of
caspase-3 activation, rapid influx of propidium iodide (PI) dye, rapid loss of intracellular
ATP and cell morphological changes (cell swelling, cell membrane integrity loss and
rupture) were observed in HMDM cells treated with HOCl. These results indicate that
HOCl caused HMDM cells to undergo necrotic cell death. In addition to the loss of
intracellular ATP, HOCl also caused rapid loss of GAPDH enzymatic activity and
mitochondrial membrane potential, indicating impairment of the metabolic energy
production. Loss of the mitochondrial membrane potential was mediated by mitochondrial
permeability transition (MPT), as blocking MPT pore formation using cyclosporin A (CSA)
prevented mitochondrial membrane potential loss.
HOCl caused an increase in cytosolic calcium ion (Ca2+) level, which was due to both
intra- and extra-cellular sources. However, extracellular sources only contributed
significantly above a certain HOCl concentration. Preventing cytosolic Ca2+ increase
significantly inhibited HOCl-induced cell viability loss. This suggests that cytosolic Ca2+
increase was associated with HOCl-induced necrotic cell death in HMDM cells, possibly
via the activation of Ca2+-dependent calpain cysteine proteases. Calpain inhibitors
prevented HOCl-induced lysosomal destabilisation and cell viability loss in HMDM cells.
Calpains induced HOCl-induced necrotic cell death possibly by degrading cytoskeletal and
other cellular proteins, or causing the release of cathepsin proteases from ruptured
lysosomes that also degraded cellular components. The HOCl-induced cytosolic Ca2+
increase also caused mitochondrial Ca2+ accumulation and MPT activation-mediated
mitochondrial membrane potential loss. MPT activation, like calpain activation, was also
associated with the HOCl-induced necrotic cell death, as preventing MPT activation
completely inhibited HOCl-induced cell viability loss. The involvement of both calpain
activation and MPT activation in HOCl-induced necrotic cell death in HMDM cells
implies a cause and effect relationship between these two events.
HMDM cells depleted of intracellular GSH using diethyl maleate showed increased
susceptibility towards HOCl insult compared to HMDM cells with intact intracellular GSH
levels, indicating that intracellular GSH played an important role in protecting HMDM
cells against HOCl exposure. Intracellular GSH level in each HMDM cell preparation
directly correlated with HOCl concentration required to kill 50% of population for each
cell preparation, indicating intracellular GSH concentrations determine the efficiency of
GSH in preventing HOCl-induced damage to HMDM cells. Intracellular GSH and cell
viability loss induced by 400 μM HOCl were significantly prevented by 300 μM
extracellular 7,8-NP, indicating that added 7,8-NP is an efficient scavenger of HOCl and
out-competed intracellular GSH for HOCl. The amount of 7,8-NP synthesized by HMDM
cells upon IFN-γ induction was too low to efficiently prevent HOCl-mediated intracellular
GSH and cell viability loss.
HOCl clearly causes HMDM cells to undergo necrosis when the concentration exceeds the
intracellular GSH concentrations. Above this concentration HOCl causes oxidative damage
to the Ca2+ ion channels on cell and ER membranes, resulting in an influx of Ca2+ ions into
the cytosol and possibly the mitochondria. The rise in Ca2+ ions triggers calpain activation,
resulting in the MPT-mediated loss of mitochondrial membrane potential, lysosomal
instability and cellular necrosis.
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Targeted modulation of cardiac energetics via the creatine kinase systemOstrowski, Filip January 2013 (has links)
There is a large body of clinical and experimental evidence linking heart disease with impairment of myocardial energetics, particularly the creatine kinase (CK) system. The goal of the experiments described in this thesis was to develop and study models of increased CK phosphotransfer, by overexpressing the CK isoenzymes and/or augmenting intracellular creatine stores. Pilot experiments were performed in cultured cells, which were used to (a) study the effects of CK overexpression in vitro, and (b) validate constructs prior to generation of transgenic mice. Expression was verified at the protein level for all constructs in HL-1 and HEK293 cells, and enzymatic activity was confirmed. Mitochondrial CK (CKmt) was expressed in the mitochondria, as expected, and CKmt overexpression was associated with a significant reduction in cell death in a model of ischemia/reperfusion injury (68.1 ± 7.1% of control, p≤0.05). Transgenic mice overexpressing CKmt in the heart were generated by a targeted approach, using PhiC31 integration at the ROSA26 locus. Transgene expression was confirmed in vitro in embryonic stem cells, and in vivo at the mRNA and protein levels. There was only a modest increase in CKmt activity; therefore, homozygous transgenic mice were generated to increase expression levels, and had 27% higher CKmt activity than wild-types (p≤0.01). Mitochondrial localization of CKmt was confirmed by electron microscopy. Citrate synthase activity, a marker of mitochondrial volume, was ~10% lower in transgenic mice (p≤0.05). Baseline phenotyping studies found that CKmt-overexpressing mice have normal cardiac structure and function. These mice are currently being backcrossed onto a pure C57BL/6 background for further studies in models of heart disease. In addition to CKmt, transgenic mice overexpressing the cytosolic CK isoenzymes, CK-M and CK-B, were generated. Due to the modest level of expression observed at ROSA26, random-integration transgenesis was used, and multiple lines were generated for each construct (carrying 2 or 6 transgene copies in the CK-M line; 2, 3, or ~30 in CK-B). Transgene expression was validated at the mRNA, protein, and activity levels. These lines are currently being expanded for further validation and phenotyping studies. Previous experiments in our group have demonstrated that increasing intracellular creatine (Cr) reduces ischemia/reperfusion injury, and a series of in vitro experiments was performed to determine whether this effect may be mediated by inhibition of the mitochondrial permeability transition pore (mPTP). The mPTP plays a significant role in ischemia/reperfusion, and there is evidence linking the CK system to regulation of the mPTP. Therefore, a model was developed to test whether Cr affects mPTP opening in cardiac-derived HL-1 cells, as this mechanism may contribute to the protective effect observed in vivo. Cr incubation conditions were determined empirically, and 24-hour incubation with 5mM or 10mM Cr was found to significantly delay mPTP opening, to a similar degree to the established mPTP inhibitor, cyclosporin A. This provides evidence that Cr may exert protective effects in the heart by a variety of mechanisms, in addition to its traditional role in energy metabolism. In summary, the experiments conducted in this thesis have produced a range of tools for studying augmentation of the creatine kinase system as a therapeutic target in heart disease. The results of in vitro assays indicate that mitochondrial CK may be a particularly promising target, and that inhibition of the mitochondrial permeability transition pore may contribute to the cardioprotective effect of creatine. Finally, the transgenic models generated and validated over the course of this project will allow for a wide range of future studies into the potential benefits of CK overexpression in the mammalian heart.
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Inibição da transição de permeabilidade mitocondrial por cPTIO, um sequestrador de óxido nítrico / Inhibition of mitochondrial permeability transition by cPTIO, a nitric oxide scavengerFerreira, Vinicius Vercesi Almada Nogueira, 1986- 23 August 2018 (has links)
Orientador: Aníbal Eugênio Vercesi / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Ciências Médicas / Made available in DSpace on 2018-08-23T00:12:21Z (GMT). No. of bitstreams: 1
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Previous issue date: 2013 / Resumo: Além de essencial na respiração celular, a mitocôndria é considerada uma organela de papel fundamental em processos de sinalização e morte celular. A geração de espécies reativas de oxigênio (EROs) e de espécies reativas de nitrogênio (ERNs) pela mitocôndria podem ser consequência destes processos de sinalização tanto em condições fisiológicas quanto em patologias, tais como a dislipidemia e câncer. A transição de permeabilidade mitocondrial (TPM) é um tipo de permeabilização não-seletiva da membrana mitocôndrial interna que permite a passagem de moléculas de até 1,5 KDa, causando dissipação do potencial eletroquímico de H+ e inchamento da organela. O termo transição é usado porque a permeabilização pode ser parcialmente revertida, logo após o inicio do processo, pela adição de quelantes de Ca2+ como o EGTA, por exemplo, ou redutores tiólicos. A oxidação de grupamentos tiólicos promove a TPM. Os experimentos apresentados nesta tese indicam o composto 2-(4-Carboxyphenyl)-4,4,5,5-tetramethylimidazoline-l-oxyl-3-oxide (cPTIO) caracteriza-se como um inibidor da TPM. As pequenas alterações observadas em relação à respiração e fosforilação oxidativa não se correlacionam com a abertura do PTP, pelo menos com base na literatura corrente. Em outras palavras, a presença de cPTIO diminuiu os níveis de NOo mitocondrial e desviou a reação deste composto com o ânion superóxido diminuindo a produção de peroxinitrito, provável indutor de abertura do PTP nestas condições experimentais / Abstract: In addition to be the site of cellular respiration, the mitochondrion has important role in cell signaling for cell physiology and death. The generation of reactive oxygen species (ROS) and reactive nitrogen species (RNS) by the mitochondrion can participate in cellular signaling both in physiological and pathological conditions, such as dyslipidemia and cancer. The Mitochondrial Permeability Transition (MPT) is a non-selective inner membrane permeabilization that enables free passage of molecules up to 1.5 kDa, dissipating the H+ electrochemical gradient and the organelle's swelling. The term transition is applied because the permeabilization can be partially reverted, right after the beginning of the process, by chelating extramitochondrial Ca2+ with EGTA, for example, or by using thiol reducers. The oxidation of membrane protein thiols leads to MPT. The experiments shown in this thesis indicate that the compound 2-(4-Carboxyphenyl)-4,4,5,5-tetramethylimidazoline-l-oxyl-3-oxide (cPTIO) has proven to be a strong inhibitor agent of the MPT. The small changes observed in relation to respiration and oxidative phosphorylation did not correlate with the opening of PTP, at least on the basis of the current literature. In other words, the presence of cPTIO decreased levels of NOo and mitochondrial diverted reaction of this compound with superoxide anion decreasing production of peroxynitrite, likely inducing PTP opening under these experimental conditions / Mestrado / Biologia Estrutural, Celular, Molecular e do Desenvolvimento / Mestre em Fisiopatologia Médica
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O aumento de transição de permeabilidade em mitocôndrias de camundongos hipercolesterolêmicos é consequência do aumento de síntese de colesterol ou da deficiência da NADP-transidrogenase? / Is the higher mitochondrial permeability trasition of hypercholesterolemic mice due to increased cholesterol synthesis or to NADP-transhydrogenase deficiency?Marques, Ana Carolina, 1988- 24 August 2018 (has links)
Orientadores: Anibal Eugênio Vercesi, Helena Coutinho Franco de Oliveira / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Ciências Médicas / Made available in DSpace on 2018-08-24T11:59:13Z (GMT). No. of bitstreams: 1
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Previous issue date: 2014 / Resumo: Os camundongos hipercolesterolêmicos (LDLr-/-) provenientes do Jackson Laboratory são modelos experimentais valiosos para o estudo da aterosclerose. Estes animais apresentam elevadas taxas de lipogênese, processo que consome grandes quantidades de NADPH. Pesquisas recentes revelaram que esta linhagem possui, além da deleção do gene do receptor de LDL, uma mutação no gene da NADP- transidrogenase (NNT). A falta da NNT pode gerar estresse oxidativo devido ao fornecimento deficiente de NADPH mitocondrial. O objetivo deste trabalho foi investigar a participação da elevação da lipogênese e da deficiência de NNT sobre o estado redox mitocondrial e suscetibilidade à transição de permeabilidade mitocondrial (TPM). Para tanto foram comparadas três linhagens de camundongos: LDLr-/- (deficiente do receptor de LDL e da NNT), C57BL6/J (deficiente apenas da NNT) e C57BL6/JUnib (controle). Foram avaliados: o controle respiratório mitocondrial (consumo de oxigênio), o estado redox de NAD(P) (fluorimetria), a susceptibilidade à transição de permeabilidade mitocondrial induzida por cálcio (inchamento e dissipação do potencial elétrico de membrana (??) sensíveis à ciclosprina A e a geração de peróxido de hidrogênio (H2O2) (Amplex red®) em mitocôndrias isoladas de coração e fígado. Observamos que não houve diferenças significativas nos parâmetros respiratórios mitocondriais nos dois tecidos das três linhagens estudadas. Como esperado, as mitocôndrias dos camundongos LDLr-/- e C57BL6/J não podem sustentar o estado reduzido de NADPH in vitro, uma vez que são deficientes de NNT. Observamos que houve diferenças significativas entre as 3 linhagens quanto à TPM da seguinte maneira: LDLr-/- > C57BL6/J > C57BL6/JUnib (controle) em mitocôndrias isoladas de fígado (inchamento e dissipação de ??) e em mitocôndrias de coração (??). Além disso, a produção de H2O2 por mitocôndrias hepáticas seguiu o mesmo padrão, sendo LDLr-/- > C57BL6/J > C57BL6/JUnib (controle). Em conjunto, estes resultados indicam que a maior suscetibilidade à TPM das mitocôndrias de camundongos LDLr-/- está correlacionada com diminuição de NADPH, tanto por aumento de consumo (devido a elevada lipogênese) quanto por diminuição de sua produção (deficiência em NNT) / Abstract: Hypercholesterolemic LDL receptor knockout mice (LDLr-/-) from Jackson Laboratory are valuable experimental models to study atherosclerosis development. These mice exhibit high rates of lipogenesis, a process that consumes large amounts of NADPH. It was recently discovered that the mice strain used to produce the LDLr-/- also carries a homozygous NADP-transhydrogenase (NNT) mutation. Loss of NNT may cause oxidative stress due to a poor supply of mitochondrial NADPH. The objective of this study was to investigate the role of elevated lipogenesis and NNT deficiency on the mitochondrial redox status and susceptibility to mitochondrial permeability transition (MPT). Three mice strains were compared: LDLr-/- mice (deficient of both LDL receptor and NTT), C57BL6/J (deficient in NNT only) and the wild type control mice C57BL6/JUnib. We evaluated the mitochondrial respiratory control (oxygen consumption), the NAD(P) redox status (fluorimetry), the susceptibility to calcium induced mitochondrial permeability transition (swelling and dissipation of membrane potential (??) sensitive to cyclosporin A) and the generation of H2O2 (Amplex red®) in isolated heart and liver mitochondria. We observed no significant differences in mitochondrial respiratory parameters in both tissues of the three mice strains studied. As expected, the mitochondria of LDLr-/- and C57BL6/J mice cannot maintain the NADP in the reduced state in vitro, since they are deficient in NNT. Regarding the susceptibility to MPT, we observed significant differences among mitochondria from the 3 strains, as follows: LDLr-/- > C57BL6/J > C57BL6/JUnib (control) in isolated liver mitochondria (swelling and potential dissipation) and in heart mitochondria potential dissipation). Furthermore, the production of H2O2 by the liver mitochondria followed the same MPT pattern: LDLr-/- > C57BL6/J > C57BL6/JUnib (control). Together, these results indicated that the greater susceptibility of LDLr-/- mitochondria to MPT is correlated with decreased NADPH which is explained by both increased consumption (due to high lipogenesis) and decreased production (deficiency NNT) / Mestrado / Biologia Estrutural, Celular, Molecular e do Desenvolvimento / Mestra em Ciências
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Efeito do extrato de \'Tamarindus\' indica L. sobre a transição de permeabilidade de membrana em mitocôndrias isoladas de fígado de rato e atividade antioxidante \'in vitro\' / Effect of Tamarindus indica L. extract on the membrane permeability transition in isolated rat liver mitochondria and in vitro antioxidant activity.Uyemura, Valéria Tudella 04 May 2007 (has links)
Tamarindus indica L. é um componente natural amplamente consumido por humanos, apresentando propriedade antiinflamatória, antidiabética e antihepatotóxica. Além disso, como nós demonstramos previamente, o extrato apresenta atividade hipolipêmica e antioxidante. Neste trabalho, nós demonstramos o efeito do extrato de T. indica sobre mitocôndrias isoladas de fígado de rato. Na presença de Ca2+, o extrato causou um inchamento osmótico mitocondrial concentração-dependente, associado ao aumento da velocidade basal (V4), dissipação do potencial de membrana e liberação do Ca2+ pré-acumulado, os quais foram inibidos por ciclosporina A (CsA) e assim atribuídos a transição de permeabilidade da membrana mitocondrial (TPMM). A indução do inchamento osmótico mitocondrial foi prevenida por EGTA e vermelho de rutênio, indicando a dependência da TPMM de Ca2+. A oxidação de proteínas tiol mitocondrial, um mecanismo bem estabelecido como causador da TPMM, foi detectado. Entretanto, nenhuma alteração significante foi observada no estado redox de GSH. A oxidação de NAD(P)H e o acúmulo de espécies reativas de oxigênio produzidas pela mitocôndria foram observadas, em ambos os casos, foram prevenidas por CsA e/ou EGTA, indicando que são conseqüências da TPMM induzida pelo extrato de T. indica. Portanto, sem aparente envolvimento do estresse oxidativo no processo, sugerindo uma interação direta de compostos do extrato com grupos tiólicos de proteínas da membrana. O extrato de T. indica induziu uma depleção de ATP associada à TPMM, mostrando assim potencial para causar a morte celular por apoptose ou necrose, resultante da indução da TPMM por si ou pela depleção do ATP via TPMM. In vitro, o extrato apresentou capacidade scavenger de radicais livres, verificado pelo ensaio do DPPH, radical superóxido e radical hidroxil; e ainda foi capaz de diminuir a lipoperoxidação mitocondrial. Além disso, em baixas concentrações, o extrato mostrou uma propriedade quelante de Fe2+. / Tamarindus indica L. is a natural dietary component widely consumed by humans, presenting well established anti-inflammatory, anti-diabetic and anti-hepatotoxic properties. In addition, as we have previously demonstrated, extract presents hypolipemic and antioxidant activities. We show here the effects of T. indica extract on isolated rat liver mitochondria. In the presence of Ca2+, the extract caused mitochondrial concentration-dependent swelling, associated to, resting respiration increase (V4), membrane potential dissipation and release of pre-accumulated Ca2+, inhibited by cyclosporine A (CsA) and thus ascribable to mitochondrial permeability transition (MPT). This swelling induction was prevented by EGTA and ruthenium red, indicating strict dependence of MPT on Ca2+. Oxidation of mitochondrial membrane protein thiols, a well established mechanism causing MPT was detected. However, no significant change was observed in the GSH redox state, and the NADPH oxidation and accumulation of mitochondria-generated reactive oxygen species that was observed, were prevented by CsA and/or EGTA, indicating that they are consequence of the MPT induced by T. indica extract. Therefore, no apparent oxidative stress condition is involved as cause of this process suggesting that direct interaction with membrane protein thiol groups of the compounds responsible for MPT induction occurs. T. indica extract led to MPTassociated ATP depletion, thus showing the potential to cause cell death by apoptosis or necrosis resulting from MPT induction per se or from ATP depletion by MPT. In vitro, the extract presented free radical scavenging ability, as assessed by the 2,2-diphenyl-1- picrylhydrazyl (DPPH), superoxide radicals and radical hydroxyl assays, and led to decreased lipid peroxidation in mitochondria, as assessed by the thiobarbituric acid reactive substances (TBARS) assay. In addition, the extract showed an iron chelanting property in low concentrations.
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Conditionnement pharmacologique par la ciclosporine A dans l’ischémie-reperfusion rénale / Pharmacological conditionning with Cyclosporin A in renal ischemia reperfusionLemoine, Sandrine 16 December 2014 (has links)
L'ischémie-reperfusion (IR) rénale entraîne des lésions de nécrose tubulaire aigue, nécessitant parfois une épuration extra rénale transitoire voir définitive. La mitochondrie joue un rôle important dans la physiopathologie de ces lésions d'IR en entrainant la mort cellulaire. L'étude de l'IR dans la cellule cardiaque a permis de mettre en évidence le rôle central du pore de transition de perméabilité mitochondriale (mPTP) dans le déclenchement de cette mort cellulaire. La ciclosporine (CsA) a été proposée comme thérapeutique pour protéger la cellule des lésions d'IR en retardant l'ouverture de ce mPTP. Cependant la CsA a des effets rénaux vasoconstricteurs aigus, nécessitant une validation expérimentale de sa protection dans l'IR rénale. Au cours de ce travail de thèse, nous avons mis au point un modèle murin d'IR rénale. Ensuite nous avons montré que le post-conditionnement à la CsA, ainsi que le post-conditionnement ischémique, permettent d'améliorer la fonction rénale avec un retard à l'ouverture du mPTP. Dans un deuxième travail, nous montrons que le pré conditionnement à la CsA est dose et temps dépendant, et médié en partie par l'augmentation d'expression d'une protéine chaperonne, l'Heat Shock Protéine 70 (HSP70). L'injection en bolus de CsA permet également d'améliorer la fonction rénale dans ce modèle d'IR avec un retard à l'ouverture du mPTP. Nos résultats ouvrent de nouvelles perspectives dans la protection rénale, notamment dans la réduction des épisodes d'insuffisance rénale aigue après chirurgie aortique ou en transplantation rénale / Ischemia-reperfusion (IR) is a situation encountered in transplantation or during aortic surgery, which can result in renal damages, requiring sometimes transient or definitive dialysis. Mitochondria play a crucial role in the pathophysiology of IR causing cell death. Previous studies of cardiac IR highlighted the role of mitochondrial permeability transition pore (mPTP). Cyclosporin A (CsA) has been proposed as a treatment to protect the kidney from IR by the delay of the opening of the mPTP. However, CsA has acute renal hemodynamic effects and a long-term toxicity, requiring an experimental validation of its protection in the renal IR. In this work, we developed a mouse model of renal IR. In a first study, we showed that the post-conditioning with CsA and ischemic postconditioning improve renal function with a delay of the opening of the mPTP. In a second study, we showed that a high dose of CsA injected just before the ischemia improves renal function and leads to the delay of the opening of mPTP mediated by an increase of HSP70. Our results open new perspectives in renal protection, especially for reducing episodes of acute renal failure in aortic surgery or in renal transplantation
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