A reinervação do músculo extensor longo dos dedos (EDL) de ratos (rattus norvegicus) seria influenciada pelo uso do laser de baixa potência e do tecido adiposo na técnica de tubulização? / The reinnervation of extensor digitorius longus (EDL) of rats (Rattus norvegicus), would be influenciate by the association of adipose tissue and low power laser in tubulization technique by vein?

Moraes, Luis Henrique Rapucci

27 November 2009

Lesões nervosas periféricas com alterações morfofuncionais são de grande importância clínica, porque pode prejudicar a função, comprometendo a sensibilidade e/ou a motricidade do órgão alvo. Quando o nervo é lesado, o indivíduo torna-se impossibilitado de realizar suas atividades, seja profissional ou pessoal, e a partir do acidente esta situação se agrava ainda mais, pois tem início uma trajetória de sofrimento e humilhações decorrentes do tipo de assistência que passa a receber, tendo em vista, ainda, a fragilidade emocional e o abatimento moral de que passa a ser vítima. Na tentativa de reparo de lesões graves de nervos periféricos, várias técnicas têm sido utilizada, mas algumas com prejuízos funcionais para outras área do corpo, como por exemplo, quando se usa outro nervo no enxerto. Considerando que enxertos venosos tem tido bons resultados na capacidade regenerativa das fibras nervosas, e como elas são encontradas em abundância e em locais de fácil acesso cirúrgico, pensou-se em verificar se o tecido adiposo e o laser de baixa potência alterariam os resultados da reinervação, por tubulização, em músculos de contração rápida (EDL). Para isso foi utilizado 84 ratos (Rattus norvegicus) da linhagem wistar, machos, que foram divididos em 12 grupos (oito experimentais e quatro controles). Nos grupos experimentais (GE) foi utilizada tubulização de veia preenchida, ou não de tecido adiposo (GEVV e GEVG, respectivamente), com e sem tratamento de laser (GEVVL e GEVGL, respectivamente). Os grupos controles (GC) receberam os nomes de positivos (GCP) quando os animais não sofreram intervenção cirúrgica, e negativos (GCN) quando os animais foram submetidos à desnervação do nervo ciático. Todos os grupos tiveram os seus animais sacrificados em dois períodos, 45 e 150 dias, após o início do experimento. A certificação da recuperação foi feita por meio da análise dos músculos inervados por ele (EDL), comparando-os com os respectivos grupos controles. Técnicas de microscopia, Imunofluorescência (MyoD e miogenina), apoptose (Tunel), morfométricas e análise funcional do ciático, foram empregadas nesta investigação. Os resultados mostraram que aos 45 dias pós desnervação os dados dos grupos experimentais estavam mais próximos do grupo controle negativo, mas aos 150 dias eles estavam mais próximos aos do grupo controle positivo. Baseado nos dados obtidos pode-se concluir que o uso de tecido adiposo e do laser de baixa potência na técnica de tubulização do nervo ciático interferem na recuperação do músculo EDL desnervado. / The peripheral nerves injuries with morphofunctional alterations, have great clinical importance because could prejudice the function, committing the sensibility and/or the motricity of target organ. When nerve is damage, the individual becomes disabled to realize yours activities, either professional or personal, in the post accident periods, this situation aggravates each more, therefore initiate a trajectory of suffering and distressing despite of the kind of assistance that this person receives, in view of your emotional fragility and your moral discouragement that pass to be victim. In attempt to repair severe peripheral nerves lesions, many techniques had been used, but some present functional prejudices to other area of bodies, for example when other autologous nerve graft it is used. Considering that, vein graft had demonstrated good results in regenerative nerve fibers capacity, and the vein are found in abundance in many locals of chirurgic access, it thought in verify if the adipose tissue and low power laser could alter the reinnervation results, by tubulization technique, in fast twitch muscle (EDL). For this, was used 84 rats (Rattus norvegicus) wistar, male, divided in 12 groups (eight experimental and four controls). In the experimental groups (EG) was used tubulization by vein combined / or not with adipose tissue (EGV and EGVA, receptively), with or without laser treatment (EGVL and EGVAL, respectively). The controls groups (CG) was called of positives (CGP) when the animals did not subject to transaction nerve, and negatives (CGN) when the sciatic nerve was transaction in this animals. All groups had the animals scarified in two periods, 45 and 150 days post experiments beginning. The recuperation was notified by means of muscle innervated analysis (EDL), comparing with the respective controls groups. Microscope techniques, Immunofluorescence for (MyoD and Miogenin), apoptosis by (Tunel assay), morphometrics and sciatic functional analysis, were employed in this investigation. The results showed that in the 45 days post-dennervation, the data of experimental groups was nearest of negative control group (transaction sciatic nerve), but in the 150 days they was nearest to the positive control group. Based on this, could be conclude that the use of adipose tissue and low power laser used in the tubulization technique by vein in the sciatic nerve interfere in the recuperation of EDL muscle dennervated.

Análise funcional do ciático

Apoptose

Apoptosis

m- ATPase

m-ATPase

Miogenin

Miogenina

Muscle extensor digitorius longus

Músculo extensor longo dos dedos

MyoD

Myod

Sciatic functional analysis

Técnica de tubulização

Tubulization techniques

Characterization of the (pro)renin receptor in vitro and in vivo

Maschke, Ulrike

09 July 2012

Der (Pro)Renin Rezeptor (PRR) ist ein hoch konservierter Transmembranrezeptor, der ursprünglich beschrieben wurde Renin und Prorenin zu binden. Durch Bindung an Renin und Prorenin beeinflusst der PRR das Renin-Angiotensin-Systems und induziert eine MAP-Kinase-Signaltransduktion. Teile des PRR sind assoziiert mit der vakuolären H+-ATPase (vATPase), welche wichtig für die Azidifizierung zellulärer Organellen ist. Kürzlich wurde eine neue Funktion des PRR für den WNT/β-catenin Signalweg beschrieben. Hier dient der PRR als Verbindungsglied zwischen den WNT Rezeptoren und der vATPase. Die Mechanismen der Funktionen des PRR sind noch nicht verstanden, aber es wird angenommen, dass der PRR in die Regulation verschiedenster zellulärer Mechanismen involviert ist. Es gibt bis jetzt keine biochemische und strukturelle Charakterisierung des PRR. In der vorliegenden Arbeit wurden strukturelle Studien mit verschiedenen Konstrukten des extrazellulären Teils des PRR durchgeführt. Alle PRR Konstrukte (hsPRR (170-303), hsPRR (101-257) und hsPRR (166-257)) zeigten eine alpha-helikale Faltung und konnten nicht an Renin oder Prorenin binden. Der hsPRR (101-257) liegt in einem Konzentrations- und pH-abhängigen Monomer-/Oligomerequilibrium vor, während der hsPRR (166-257) als Monomer/Dimerequilibrium vorkommt. Diese Daten bilden die Grundlage für weitere strukturelle und funktionelle Untersuchungen. Konditionelle KO Mäuse sind eine exzellente Methode, um die physiologische Rolle des PRR in vivo zu untersuchen. Eines der wichtigsten Proteine des Wnt/β-catenin Signaltransduktionsweges, β-catenin, ist fundamental für die T-Zell Entwicklung. Aus diesem Grund wurde untersucht, ob die Deletion des PRR in T-Zellen ebenfalls zu einem Verlust von T-Zellen und zu einer Entwicklungsstörung führt. Die Ergebnisse zeigen, dass der PRR wichtig für eine vollständige T-Zellentwicklung ist und unterstützen die Hypothese, dass der PRR eine Rolle für Wnt/β-catenin Singaltransduktion in T-Zellen spielt. / The (pro)renin receptor (PRR) is an evolutionary conserved transmembrane receptor that was first discovered to bind renin and prorenin. Upon binding, PRR was shown to influence the activity of the renin-angiotensin-system (RAS) and to induce MAP kinase signalling. It was previously shown that a truncated, transmembrane part of PRR was associated to vacuolar H+-ATPase (vATPase), a proton pump which is important for acidification. Recently, a new function of PRR in the WNT/β-catenin signalling pathway was described. Here, the PRR was shown to be an adaptor between WNT receptors and the vATPase. The precise mechanisms by which PRR functions, are still elucidative but the PRR is supposed to regulate various cellular processes. Currently, no biochemical characterization or structural analysis is available for PRR. In order to gain understanding of the function of the PRR, structural studies were performed with several truncated proteins of the extracellular part of the PRR. All PRR proteins (hsPRR170-303, hsPRR 101-257 or hsPRR 166-257) showed an overall alpha helical folding and did not bind renin or prorenin. The oligomeric assembly of the proteins was investigated. The hsPRR (101-257) was shown to be in a concentration and pH dependent monomer/oligomer equilibrium, whereas hsPRR (166-257) is only present in a monomer/dimer equililibrium. These data are the basics for further structural and functional studies. Additionally, conditional KO animals are an excellent tool to investigate the physiological role of the PRR in vivo. As the major mediator of the Wnt/β-catenin signaling pathway, β-catenin, is crucial for T cell maturation, a conditionel deletion of PRR in T cells was analyzed. PRR deletion resulted in a loss of mature T cells. Moreover, a defect in T cell maturation in the thymus was determined. Our data showed that PRR is critical for proper T cell development and support the hypothesis that PRR contributes to Wnt/β-catenin signaling in T cells.

(Pro)Renin Rezeptor

T-Zell Entwicklung

Wnt/β-catenin Signaltransduktionsweg

v-ATPase

(pro)renin receptor

T cell development

Wnt/β-catenin pathway

v-ATPase

570 Biowissenschaften, Biologie

32 Biologie

WE 5200

ddc:570

Role of the (Pro)renin Receptor [(P)RR/ATP6ap2] in Osteoclast and Macrophage Physiology

Rousselle, Anthony

05 December 2017

Vor zehn Jahren wurde der (Pro)Renin-Rezeptor [(P)RR] entdeckt und als neuer Bestandteil des Renin-Angiotensin-Systems beschrieben. Neuere Studien ergaben, dass der (P)RR mit der vakuolären H+-ATPase (V-ATPase) assoziiert sein kann, weshalb er auch V-ATPase associated protein 2 (ATP6ap2) genannt wird. In Osteoklasten befinden sich V-ATPase hauptsächlich an der zur Knochenoberfläche gerichteten Plasmamembran und transportieren Protonen in den extrazellulären Raum. Mäuse mit genetischer Deletion verschiedener V-ATPase-Untereinheiten charakterisiert durch einen Anstieg von Knochenmasse (Osteopetrose). In der vorliegenden Arbeit fanden wir heraus, dass (P)RR stark in reifen Osteoklasten in vitro und in vivo exprimiert wird. Mäuse mit genetischer Deletion des (P)RR in Osteoklasten wurden durch einen komplexen Knochen-Phänotyp mit reduzierter Knochendichte charakterisiert. (P)RR-defiziten Osteoklasten wiesen vermehrte Differenzierung und/oder Aktivität in vitro und in vivo auf. Wir postulieren deshalb, dass der (P)RR die in der Plasmamembran lokalisierten V-ATPase nicht direkt reguliert, sondern mit der physiologischen Aktivität der Osteoklasten durch andere Mechanismen interferiert. Macrophagen sind speziell auf die Immunabwehr ausgerichtete Fresszellen (Phagozyten). Phagozytose ist ein wesentlicher Zellprozess der die V-ATPase in Lysosomen braucht um die eingeschlossenen Pathogen zu zerstören. Wir generierten transgene Ratten mit konditionellen knockdown von (P)RR unter Nutzung eines Doxyzyclin-induzierten shRNA-Expressionssystems. Eine effiziente (P)RR-Depletion in Makrophagen wurde durch Behandlung mit Doxyzyclin in vivo im Trinkwasser und in vitro im Kulturmedium erreicht. Die vorliegende Arbeit zeigt, dass die Verschiebung des vesikulären pHs erst ziemlich spät nach (P)RR-Depletion auftritt. Wir fanden heraus, dass (P)RR-Depletion weder Phagozytose noch Endozytose beeinträchtigte, sondern für das Recycling des Transferrin-Rezeptors zur Plasmamembran wichtig ist. / A decade ago, the (pro)renin receptor [(P)RR] was discovered and depicted as a new component of the renin-angiotensin system. However, recent studies have put in evidence that the (P)RR associate with and regulate the vacuolar H+-ATPase (V-ATPase), hence its other name vacuolar H+-ATPase associated protein 2 (ATP6ap2). In osteoclasts, V-ATPases are mainly located at the plasma membrane facing the bone surface and extrude protons into the extracellular space. Mice with genetic deletion of various V-ATPase subunits are characterized by an increase of bone mass (osteopetrosis). In this work, we found that the (P)RR is highly expressed in mature osteoclasts in vitro and in vivo. Mice with genetic deletion of the (P)RR in osteoclasts developed a complex bone phenotype characterized by a reduced bone density. Osteoclasts lacking (P)RR displayed increased differentiation and/or activity in vitro and in vivo. We therefore suggest that the (P)RR does not directly regulate V-ATPases located at the plasma membrane but rather interferes with osteoclast physiology through other mechanisms. Macrophages are professionalized phagocytes crucial for immune response. Phagocytosis is an essential cellular process, which requires lysosomal V-ATPases for degradation of engulfed pathogens. We generated transgenic rats with a conditional depletion of the (P)RR with the use of a doxycycline-induced shRNA expression system. Efficient (P)RR depletion in macrophages was accomplished by doxycycline treatment in vivo in drinking water and in vitro in culture medium. In this work, we found that the impairment of vesicular pH occurs lately after (P)RR deletion. Also, we found that (P)RR deletion did not impair neither phagocytosis nor endocytosis but rather perturbed the recycling of the transferrin receptor to the plasma membrane.

(Pro)Renin-Rezeptor

vakuolären H+-ATPase

Osteoklast

Makrophage

Ansäuerung

vesikulärer Transport

(pro)renin receptor

vacuolar H+-ATPase

osteoclast

macrophage

acidification

vesicle trafficking

570 Biowissenschaften; Biologie

WF 9860

ddc:570

Etude d’une cible thérapeutique pour la maladie d’Alzheimer et mise au point de nouveaux modèles cellulaires de criblage / Study of a therapeutic target for Alzheimer's disease and development of new models of cellular screening

Dorard, Emilie

17 October 2016

Résumé confidentiel / Confidential abstract

Maladie d’Alzheimer

Modèle cellulaire

SAPPα

Α3-Na+K+ATPase

SET

Neuroprotection amyloïde-β1-42

Croissance axonale

Alzheimer's disease

Cell model

SAPPα

Α3-Na+K+ATPase

SET

Amyloid-β1-42 neuroprotection

Axonal growth

612.8

Aufreinigung und funktionelle Charakterisierung der peroxisomalen ABC-Transporter Pxa1p-Pxa2p aus Saccharomyces cerevisiae

Schreiber, Gabriele

19 December 2007

Die peroxisomalen ABC-Transporter Pxa1p und Pxa2p sind Halbtransporter. Genetische Studien ergaben Hinweise, dass sie zur Bildung aktiver Transporter heterodimerisieren und am Import von langkettigen Fettsäuren in die Peroxisomen von S. cerevisiae beteiligt sind. Es wurden epitopmarkierte Varianten der Proteine als Komplex isoliert. Damit wurde gezeigt, dass Pxa1p und Pxa2p ein stabiles Heterodimer bilden. Zur Charakterisierung der ATP Bindeeigenschaften wurden die Transporter mit 8-azido-[alpha-32P]-ATP inkubiert und kovalent verknüpft. Dabei konnte gezeigt werden, dass Pxa1p und Pxa2p eine unsymmetrische Bindung des ATP Analogons aufweisen. Pxa2p bindet deutlich mehr azido-ATP als Pxa1p, bei sehr ähnlichen Dissoziationskonstanten. Die reduzierte ATP Bindung von Pxa1p spiegelt sich durch degenerierte Sequenzmotive der an der ATP Bindung beteiligten Sequenzen wieder. Die isolierten ABC-Transporter wurden für ATPase Messungen eingesetzt. Sie zeigten eine basale ATPase Aktivität, die durch Zugabe langkettiger Coenzym A aktivierter Fettsäuren, wie Oleoyl-CoA und Palmitoyl-CoA stimulierbar war. Eine Lysin Mutation im Walker A Motiv von Pxa1p hatte keine Funktionalitätseinbuße zur Folge. Dieselbe Mutation bei Pxa2p führte im Wachstumstest auf Festmedium mit Ölsäure als Kohlenstoffquelle zu einem deutlich verlangsamten Wachstum. Diese Ergebnisse korrespondieren mit der beobachteten unsymmetrischen ATP Bindung von Pxa1p und Pxa2p, da bei dem schwächer bindenden Pxa1p die Mutation wirkungslos blieb. Keine Übereinstimmung war bei den ATPase Aktivitätsmessungen der aufgereinigten Mutanten zu verzeichnen. Beide Mutanten zeigten eine unbeeinträchtigte ATPase Aktivität. Die ABC-Transporter wurden in Proteoliposomen eingebaut und für Transportmessungen mit einem Spin-Label markierten Oleoyl-CoA verwendet. Die Transportmessungen zeigten einen ATP abhängigen Transport, woraus geschlossen wurde, dass Pxa1p-Pxa2p tatsächlich Coenzym A Ester langkettiger Fettsäuren transportiert. / The peroxisomal ABC-transporters Pxa1p and Pxa2p are half transporters. Previous genetic investigations have demonstrated that Pxa1p and Pxa2p have to dimerise in order to build a functional transporter, which is very likely involved in the import of long chain fatty acids into peroxisomes of S. cerevisiae. In this work, tagged versions of the proteins were purified as a complex. This proved for the building of a stable hetero dimer. For characterisation of the ATP binding properties, the transporters were incubated and cross linked with 8-azido-[alpha-32P]-ATP. This revealed an asymmetric binding of the ATP analogue. Pxa2p binds much more azido-ATP, than Pxa1p, while the dissociation constants are rather similar. The poorer ATP binding of Pxa1p is reflected by degenerated sequence motifs in the nucleotide binding fold. The purified ABC-transporters have been used for ATPase assays. They showed a basal ATPase activity, which could be stimulated by addition of long chain fatty acid CoAs, like oleoyl-CoA and palmitoyl-CoA. Mutants with a lysine mutation in the walker A motive of Pxa1p led to no functional impairment, while the corresponding lysine mutation in Pxa2p led to reduced growth on agar plates with oleic acid as sole carbon source. The result corresponds with the ATP binding properties of Pxa1p. Because of the poorer ATP binding, even in the wild type protein, the mutation was not supposed to have a big influence. No accordance was found in respect to the ATPase measurements of the isolated mutant proteins. Both mutants revealed unaffected ATPase activity. The purified ABC-transporters were reconstituted in proteoliposomes and used for translocation assays of a spin-labelled oleoyl-CoA derivative. The measurements revealed an ATP dependent transport of the oleoyl-CoA analogue. This led to the conclusion, that Pxa1p-Pxa2p is indeed the transporter of long chain acetyl CoA esters, which were transported in an ATP dependent manner.

ABC-Transporter

Peroxisomen

Fettsäuretransport

ATPase Aktivität

SL-Oleoyl-CoA

Flippase

Rekonstitution

ABC-transporter

peroxisomes

fatty acid transport

ATPase activity

SL-Oleoyl-CoA

flippase

reconstitution

570 Biowissenschaften, Biologie

32 Biologie

WD 5100

WF 9500

ddc:570

Influência de densidades do laser de baixa intensidade sobre o músculo masseter de ratos Wistar / Influence of densities of low level laser on the masseter muscle of rats Wistar

Dias, Fernando José

28 May 2010

A laserterapia tem sido muito utilizada como tratamento alternativo em pacientes com dores crônicas relacionadas às disfunções temporomandibulares. Isso se deve aos efeitos: analgésico, antiinflamatório, miorrelaxante, de redução da fadiga durante as contrações tetânicas, aumento da força de mordida e diminuição da dor orofacial. Embora sejam observados resultados clínicos, ainda não é bem compreendido o seu efeito em nível celular. Assim, este estudo tem como objetivo analisar os efeitos das diferentes densidades (doses) de irradiação do laser de baixa intensidade (LLLI), em nível celular, sobre o músculo masseter de ratos Wistar. Os animais foram alocados aleatoriamente em 6 grupos (n=10), receberam 10 irradiações do laser (GaAlAs,780nm, 5mW e spot 0,04cm²) sobre o músculo masseter esquerdo variando a densidade de energia (I. 0; II. 0,5; III. 1,0; IV. 2,5; V. 5,0 e VI. 20 J/cm²). Após as 10 irradiações os músculos masseteres foram obtidos dos animais sob anestesia para análises: 1. Histoenzimológicas para atividade da nicotinamida adenina dinucleotídeo diaforase(NADH), succinato desidrogenase (SDH) e adenosina trifosfatase (ATPase), 2. Microscopia de luz (HE), 3. Microscopia eletrônica de transmissão e 4. Imunohistoquímica para fator de crescimento do endotélio vascular (VEGF) e o receptor 2 para VEGF (VEGFR-2). A atividade do NADH nos grupos IV, V e VI (30±1,26; 33,47±2,15; 31,67±1,77 - fibras intermediárias) apresentou um aumento significativo (p>0,05) no metabolismo oxidativo em relação aos demais grupos. Na atividade do SDH, o aumento foi discreto, com aumento significativo (p>0,05), apenas no grupo V (32,2±1,61 fibras intermediárias), com o padrão de aumento metabólico muito parecido nas reações de NADH e SDH. A atividade da ATPase não revelou diferenças entre os grupos tanto em meio ácido como no alcalino. A microscopia de luz revelou fibras musculares arredondadas e núcleos periféricos achatados, os quais tornaram mais arredondados com as densidades maiores de energia. Ultraestruturalmente as irradiações com as maiores densidades de energia revelaram mitocôndrias de tamanhos e formas variadas e cisternas do retículo sarcoplasmático dilatadas entre as miofibrilas. As análises qualitativas mostraram um padrão de aumento a expressão do VEGF e VEGFR-2 proporcionais à densidade de energia do laser usada. Conclui-se que o laser com densidades maiores foi capaz de aumentar o metabolismo oxidativo, sem alterar a capacidade contrátil, aumentar o volume do núcleo, modificar a ultraestrutura das fibras musculares e as expressões do VEGF e VEGFR-2. / The laser therapy has been widely used as an alternative treatment in patients with chronic pain related to temporomandibular disorders. This is due to the effects: analgesic, anti inflammatory, muscle relaxant, reducing fatigue during tetanic contractions, increased bite strength and decrease in orofacial pain. Although clinical results are observed, is not well understood its effect on the cellular level. This study aims to analyze the effects of different densities (doses) irradiation of low level laser therapy (LLLI) on cellular level, on the masseter muscle of rats. The animals were randomly assigned to 6 groups (n=10), received 10 laser irradiation (GaAlAs, 780nm, 5mW spot and 0.04 cm²) on the left masseter muscle by varying the energy density (I. 0; II. 0.5; III. 1.0; IV. 2.5; V. 5.0 and VI. 20 J/cm²). After 10 irradiations the masseter muscles were obtained from animals under anesthesia for analysis: 1. Histoenzimologic for nicotinamide adenine dinucleotide (NADH), succinate dehydrogenase (SDH) and adenosine triphosphatase (ATPase), 2. Light microscopy (HE), 3. Transmission electron microscopy and 4. Immunohistochemistry for vascular endothelial growth factor (VEGF) and receptor 2 for VEGF (VEGFR-2). The activity of NADH in groups IV, V and VI (30±1,26; 33,47±2,15; 31,67±1,77 - intermediate fiber) increased significantly (p> 0.05) in oxidative metabolism in relation to other groups. The activity of SDH showed a slight increase, only the group V (32,2±1,61 intermediate fiber) increased significantly (p> 0.05), but the pattern of metabolic increase was very similar in both reactions. The ATPase activity showed no differences between groups nor in acid or alkaline. The qualitative analysis showed a pattern of increased expression of VEGF and VEGFR-2 directly proportional to the energy density of laser. Light microscopy showed rounded muscle fibers and peripheral flattened nuclei, which become more rounded with the highest energy densities. Ultrastructurally the irradiation with higher energy densities showed mitochondria of different sizes and shapes and dilated cisterns of sarcoplasmic reticulum between the myofibrils. It is concluded that higher densities of laser was able to increase the oxidative metabolism without altering the contractile capacity, increasing nuclei volume, modify ultrastructure of muscle fibers and the expressions of VEGF and VEGFR-2.

ATPase

ATPase

Laser de baixa-intensidade

light microscopy

Low-level laser therapy

metabolismo oxidativo

microscopia de luz

NADH

NADH

oxidative metabolism

SDH

SDH

ultraestrutura

ultrastructural

VEGF

VEGF

VEGFR-2

VEGFR-2

Efeito da glicose sobre os mecanismos de extrusão de prótons em células MDCK. / Effect of glucose on mechanisms of proton extrusion in MDCK cells.

Damasceno, Rosélia dos Santos

14 June 2010

Este estudo investigou o efeito da glicose sobre a atividade e expressão da isoforma 1 do trocador Na+/H+ (NHE1) e da H+-ATPase do tipo vacuolar, em células MDCK (Mardin Darby Canine Kidney), linhagem derivada de rim de cão, que apresenta características similares às células principais e intercalares das porções distais do néfron. Por microscopia de fluorescência, se avaliou a velocidade de recuperação do pHi (dpHi/dt) e a capacidade tamponante (<font face=\"symbol\">bi). A partir desses parâmetros, se calculou o efluxo de H+ (JH+). Por Western blot, se avaliou a expressão de NHE1 e da subunidade E da H+-ATPase do tipo vacuolar. Resultados: Na condição controle o efluxo de H+ foi de 6.27 ± 0.51 mM/min (n = 9). O tratamento agudo com glicose (25 mM) aumentou o efluxo de H+ via NHE1, o qual foi modulado pela PI3 cinase. Na mesma condição, não se observou alterações na atividade da H+-ATPase. O tratamento crônico com glicose (25 mM) induziu significante aumento do efluxo de H+, via NHE1 e H+-ATPase. O efeito estimulador da glicose sobre a atividade de NHE1 e H+-ATPase foi dependente da atividade da p38 MAP cinase. Além disso, o tratamento crônico com glicose (25 mM) induziu fosforilação do sistema ezrin/radixin/moesin (ERM) e Akt. Conclusões: Nossos resultados indicam que no tratamento agudo com glicose (25 mM), o NHE1 foi modulado pela PI3 cinase. Contudo, no tratamento crônico com glicose (25 mM), a atividade do NHE1 foi modulada pelo sistema ERM/Akt e a atividade da H+-ATPase foi modulada pela p38 MAP cinase. / This study investigated the effect of glucose on the activity and expression of Na+/H+ exchanger isoform 1 (NHE1) and vacuolar H+-ATPase, in Mardin Darby Canine Kidney (MDCK) cells from dog kidney, with similar characteristics to principal and intercalated cells of the distal nephron. The pHi recovery rate (dpHi/dt) and the buffering capacity (<font face=\"symbol\">bi) was evaluated through fluorescence microscopy. From these parameters the H+ efflux (JH+) was calculated. By Western blot, the NHE1 and H+-ATPase (E subunit) expression was evaluated. Results: In the control situation the H+ efflux was 6.27 ± 0.51 mM/pH units (n = 9). Acute treatment with glucose (25 mM) increased the H+ efflux via NHE1, which was modulated by PI3 kinase. In the same condition, the H+-ATPase activity did not change. Chronic treatment with glucose (25 mM) induced significant increase in H+ efflux via NHE1 and H+-ATPase. The stimulatory effect of glucose on the NHE1 and H+-ATPase activity was dependent on p38 MAP kinase activity. Furthermore, chronic treatment with glucose (25 mM) induced Ezrin/radixin/moesin (ERM) and Akt phosphorylation. Conclusions: Our results indicate that during the acute treatment with glucose (25 mM), the NHE1 is modulated by PI3 kinase. However, during chronic treatment with glucose (25 mM), NHE1 activity was modulated by the ERM/Akt system and of H+-ATPase activity was modulated by p38 MAP Kinase.

Cães

Cell membranes

Células epiteliais

Dogs

Epithelial cells

Fluorescence microscopy

Glicose

Glucose

H+ATPase vacuolar

Intracellular pH

Membranas celulares

Membrane transporters

Microscopia de fluorescência

Na+/H+ exchanger

pH intracelular

Transportadores de membrana

Trocador Na+/H+

Vacuolar H+ATPase

Enriquecimento ambiental como estratégia neuroprotetora em ratos submetidos à hipóxia-isquemia neonatal

Rojas, Joseane Jiménez

January 2015

A hipóxia-isquemia (HI) é a principal causa de mortalidade no período perinatal e, nos sobreviventes, a incidência de comorbidades neurológicas é elevada. O encéfalo imaturo, altamente susceptível ao insulto hipóxico-isquêmico, é bastante sensível a estímulos ambientais tais como o enriquecimento ambiental (EA). Os objetivos deste estudo foram: 1) investigar o desempenho comportamental em um novo teste de memória e aprendizagem, o Ox-maze; 2) analisar a atividade das enzimas Na+,K+-ATPase, catalase (CAT) e glutationaperoxidase (GPx) no hipocampo; 3) caracterizar os neurônios piramidais da região CA1 hipocampal quanto à arborização dendrítica; 4) analisar alterações astrocíticas e sinápticas pela avaliação da imunoreatividade das proteínas GFAP e sinaptofisina usando a técnica de imunofluorescência e, 5) quantificar a densidade celular por meio de cortes semifinos da região CA1 do hipocampo de animais hipóxico-isquêmicos expostos a um ambiente enriquecido. Ratos com sete dias de idade foram divididos em quatro grupos e submetidos ou não ao procedimento cirúrgico de acordo com o grupo experimental ao qual pertenciam: controle mantido em ambiente padrão (CTAP), controle em ambiente enriquecido (CTAE), HI em ambiente padrão (HIAP) e HI em ambiente enriquecido (HIAE). Passado o período de EA (1h/dia, 6 dias/semana, 9 semanas iniciando após o desmame), os parâmetros mencionados foram avaliados nos animais. Os dados indicaram que a HI causou um prejuízo na memória e no aprendizado no teste do “OX-maze”, o qual foi revertido pelo efeito do ambiente enriquecido. A HI causou diminuição da atividade enzimática da Na+,K+-ATPase no hipocampo contralateral, assim como uma redução na imunorreatividade à sinaptofisina e nadensidade neuronal, sendo que o EA foi efetivo na recuperação da atividade da enzima Na+,K+-ATPase e dos níveis de sinaptofisina no hipocampo contralateral à lesão. As atividades de CAT e GPX não foram alteradas pela HI em nenhum dos grupos avaliados, mesmo resultado encontrado nas análises de GFAP e de padrão de arborização dendrítica. Por fim, neste estudo foi observado o importante efeito lesivo causado pela HI neonatal e o papel do EA como estratégia neuroprotetora na recuperação funcional, na atividade da Na+,K+-ATPase e na expressão de sinaptofisina. Este estudo traz avanços em busca dos mecanismos pelos quais a melhora funcional ocorre em animais HI expostos ao EA, mas pode-se verificar que não fica totalmente esclarecido como esta estratégia atua. Outros estudos são necessários para a identificação de possíveis mecanismos que atuem como mediadores da resposta funcional do EA após um evento isquêmico. / Hypoxia-ischemia (HI) is the main mortality cause in perinatal period and, in survivors, the incidence of neurological disabilities is elevated. The immature brain, highly susceptible to hypoxic-ischemic insult, is sensible to environmental stimuli, as environmental enrichment (EE). The aims of this study were to investigate: 1) behavioral performance in a new memory and learning task, the oxmaze task; 2) evaluate Na+,K+-ATPase, catalase (CAT) and glutathione peroxidase (GPx) activities in the hippocampus; 3) characterizes dendritic arbor in pyramidal neurons from CA1 region from hippocampus; 4) analyze alterations in hippocampal synaptophysin and GFAP immmunoreactivity and, 5) analyze neuronal density alterations in hippocampus of hypoxic-ischemic rats exposed to enriched environment. Seven-day-old rats were divided into four groups: controlmaintained in standard environment (CTSE), control submitted to EE (CTEE), HI in standard environment (HISE) and HI in EE (HIEE). Past the end of EE period (1 hour/day, 6 days/week, 9 weeks), mentioned parameters were evaluated in animals. Present results indicate learning and memory in the “OXmaze” task were impaired in HI rats and this effect was recovered after EE. On the contralateral hemisphere, HI caused a decrease in Na+,K+-ATPase activity that was recovered by EE. Results also indicate that HI damage decreases hippocampal synaptophysin immunoreactivity and neuronal density, moreover EE was effective in recovering synaptophysin levels on contralateral to the lesion hippocampus. The activities of GPx and CAT were not changed by HI in any group evaluated, some result founded on GFAP immunoreactivity and dendritic arborization characterization analysis. In conclusion, the important effect of HI lesion and the role of EE like neuroprotective strategy on functional impairment and on Na+,K+-ATPase activity and synaptophysin immunoreactivity was proven. Although this study have important advances in search of mechanisms by which the functional enhancement occurs in the animals submitted to HI and exposed to EE, it can be seen that it is not completely clear how this approach works. Further studies are needed to identify possible mechanisms that act as mediators of EE functional response after an ischemic event.

Enriquecimento ambiental

Hipóxia-isquemia encefálica

Neuroproteção

Hipocampo

Memória

Proteína glial fibrilar ácida

ATPase trocadora de sódio-potássio

Sinaptofisina

Neonatal hypoxia-ischemia

Environmental stimulation

Plasticity

Neuronal density

CA1 activity

Antioxidant enzymes

Hippocampal area

Synaptophysin

GFAP

Na+

K+-ATPase

Characterization of Plasmodium falciparum membrane transporters as potential antimalarial targets / Caractérisation de transporteurs membranaires de Plasmodium falciparum en tant que potentiel cibles thérapeutiques

Bosne, Stéphanie

10 October 2014

La découverte de nouveaux agents antipaludiques est primordiale. A travers le monde, les chercheurs se sont focalisés sur plusieurs stratégies. Les plus développées sont : soit les tests de molécules issues de bibliothèques chimiques dans une recherche phénotypique (comme le test direct d’agents sur des cultures de parasites in vitro), soit la recherche de nouvelles molécules agissant sur l’activité d’une cible ou d’une voie spécifique et essentielle. Cette thèse est centrée sur le second type d’approche. Nous nous sommes intéressés aux transporteurs membranaires de P. falciparum. Pour cela, nous exprimons les protéines d’intérêt dans la levure et nous les purifions. Nous optimisons les tests fonctionnels, dans le but de : a) déterminer l’effet des molécules sur les cibles spécifiques ; b) tester leur effet sur les cultures d’érythrocytes infectés par P. falciparum in vitro ; c) vérifier leur toxicité sur des cellules de mammifères ; et d) réaliser le test des molécules les plus efficaces in vivo dans un modèle de paludisme murin. Notre travail actuel est focalisé sur l’ATPase6 de P. falciparum (PfATP6) et l’adénylate translocase (PfAdT), deux protéines membranaires essentielles localisées respectivement sur le réticulum endoplasmique et la membrane mitochondriale. Nous exprimons de manière hétérologue PfATP6 dans les membranes de levure, nous purifions la protéine et mesurons une activité ATPase spécifique. Nous avons ainsi pu tester une bibliothèque chimique importante et identifier des inhibiteurs spécifiques. Ces derniers ont ensuite été testés pour évaluer leur effet sur les stades érythrocytaires du parasite in vitro et leur cytotoxicité sur des cellules de mammifères. Pour le transporteur PfAdT, nous procédons comme pour PfATP6, mais nous avons choisi un autre type de test fonctionnel dans lequel la protéine est directement exprimée sur la membrane plasmique d’E. coli. Cela devrait permettre de mesurer le transport d’ATP radiomarqué, et l’identification d’inhibiteurs spécifiques dont les effets pourront être évalués sur des cultures de parasites in vitro et dans des essais de cytotoxicité. / New drug discovery for malaria treatment urges, now more than ever. There is no optimal solution to the search for new antimalarials. Worldwide, researchers have focused their energies on several strategies. The most commonly employed are: either by screening molecules issued from chemical libraries in a phenotypic way (i.e., direct testing of drugs on in vitro parasite cultures), or by searching for new molecules acting upon the activity of a specific essential target or pathway. This PhD thesis centers on the second type of approach. We are interested in targeting membrane transporters of P. falciparum. For this, we plan to express proteins of interest in yeast and proceed to their isolation. With optimized functional tests, we aim to: a) Determine the effect of molecules upon specific targets; b) Test their effect on P. falciparum in vitro erythrocytes cultures; c) As well as verify their toxicity on mammalian cells; and d) Perform in vivo testing of the best molecules on a rodent model for malaria. Our actual work is focused on the P. falciparum Ca2+ - ATPase 6 (PfATP6) and adenylate translocase (PfAdT), two essential membrane proteins localized on the endoplasmic-reticulum and the mitochondrial membrane, respectively. We were able to express heterologously PfATP6 in yeast membranes, purify the protein and measure a specific ATPase activity. With this, we have tested a large chemical library and identified specific inhibitors. These were then tested for their effect on in vitro blood stages of P. falciparum and for their cytotoxicity on mammalian cells. For the ATP/ADP carrier PfAdT, we proceeded as previously done with PfATP6 but we have also chosen another type of functional test where we express directly this protein in the plasma membrane of E. coli. This will enable in the future the measurement of radiolabelled ATP uptake, and the identification of specific inhibitors that could then be tested for their effect on P. falciparum in vitro cultures and for their cytotoxicity.

Inhibiteurs anti-plasmodium

Cytotoxicité

Criblage in vitro

Activité biochimique

Antiplasmodium inhibitors

Cytotoxicity; in vitro screening

In vitro screening

Biochemical activity

Etude des sous-unités a de la v-ATPase : caractérisation de leurs interactions avec les protéines SNAREs et étude de l’expression par des gliomes de la sous-unité rénale a4 / Studies of the a-subunits of v-ATPase : characterization of their interactions with SNARE proteins and study of the expression of the renal a4 subunit by gliomas

Gleize, Vincent

20 October 2011

La v-ATPase est une pompe à protons. Elle permet l’acidification d’organelles, ce qui est indispensable à de nombreux processus cellulaires. Cette enzyme est composée de 14 sous-unités différentes, organisées en deux domaines, le domaine catalytique V1 et le domaine membranaire V0. La sous-unité a du domaine V0 est essentielle au transport des protons. Il en existe 4 isoformes (a1 à a4) et des variants d’épissage (a1-I à a1-IV pour a1) permettant à la v-ATPase d’être adressée vers différents compartiments et donc d’être impliquée dans différents processus. Deux projets visant à étudier cette sous-unité ont été réalisés.En plus de son rôle dans le transport des protons, il a été montré que le domaine V0 de la v-ATPase est impliqué dans des évènements de trafic membranaire, tel que l’exocytose de vésicules de sécrétion. Ce rôle semble nécessiter des interactions avec les protéines SNAREs. J’ai montré, pendant la première partie de ma thèse, que les sous-unités flag-a1-I et flag-a1-IV sont toutes deux adressées aux granules de sécrétion de cellules neurosécrétrices et interagissent avec les protéines SNAREs VAMP2 et syntaxine-1. De façon intéressante la syntaxine-1 semble interagir préférentiellement avec la sous-unité a1-I qui dans les neurones est l’isoforme adressée aux terminaisons nerveuses. Les sous-unités a1-IV ne diffèrent d’a1-I que par l’ajout de 7 acides aminés dans sa moitié N-terminale. Le domaine d’interaction de la sous-unité a avec la syntaxine-1 semble donc être localisé dans cette région.Dans la deuxième partie de ma thèse, j’ai mis en évidence et étudié l’expression de la sous-unité rénale a4 dans des gliomes humains. Ces tumeurs sont les tumeurs cérébrales les plus fréquentes et sont en général associées à un mauvais pronostic. L’OMS distingue, en fonction de paramètres histologiques, les astrocytomes (de grade I à IV), les oligodendrogliomes et les gliomes mixtes (chacun de grade II ou III). Cette classification est controversée, notamment à cause de son manque de reproductibilité, et la prise en compte de marqueurs moléculaires semble s’imposer comme une solution pour la renforcer.J’ai quantifié par RT-PCR quantitative l’expression du gène ATP6V0A4 (codant la sous-unité a4) dans 188 prélèvements de gliomes humains. Nous avons ainsi montré que l’expression de la sous-unité a4 peut être utilisée comme marqueur diagnostique des oligodendrogliomes anaplasiques (35 % l’expriment). Dans un prélèvement, la présence de la codélétion 1p/19q et l’expression de a4, tout deux marqueurs indépendants des oligodendrogliomes, permettra le renforcement du diagnostique oligodendrogliome anaplasique. De plus a4 est fréquemment exprimée par les astrocytomes pilocytiques (70%), où elle est associée à la duplication en tandem de la région chromosomique 7q34 située à proximité directe du gène ATP6V0A4. Enfin une observation prometteuse est que l’expression de a4 pourrait être un marqueur de mauvais pronostic pour les patients atteints d’oligodendrogliome anaplasique ne présentant pas la co-délétion 1p/19q, observation qui devra être confirmée sur une plus grande cohorte de patients. / Vacuolar type H+-ATPase is a proton pump, which acidifies numerous organelles, crucial for many cellular processes. This enzyme is composed of 14 different subunits organized in two domains, a catalytic V1 domain and a V0 membrane domain. The a-subunit of V0 is essential for proton transport. There are 4 isoforms of a (a1 to a4) and splicing variants (a1-I to a1-IV for the a1 subunit). v-ATPases containing different a-subunit isoforms are localized in different compartments allowing v-ATPase to participate in different processes. The a-subunits were studied in this work in two distinct projects.Besides its role in proton pumping, V0 domain of v-ATPase is implicated in organelles trafficking events, like vesicles exocytosis. This role seems to require interactions of V0 with SNARE proteins. During my thesis work, I showed that flag-a1-I and flag-a1-IV are both targeted to secretion granules in PC12 neurosecretory cells. These subunits interact with the SNARE proteins VAMP2 and syntaxin-1. Interestingly, syntaxin-1 seems to preferentially interact with the a1-I subunit, isoform which in neurons is sorted to nerve terminals. The only difference between a1-I and a1-IV subunits is the addition of 7 amino acids in the N-terminal half of a1-IV. So syntaxin-1 probably interacts with a1-I at this location. In a second project, I studied the expression of the renal a4-subunit in human gliomas. These tumors are the most frequent brain tumors and are generally associated with a poor prognosis. Based on histological parameters,WHO distinguishes, astrocytomas (grade I to IV), oligodendrogliomas and oligoastrogliomas (each of grade II or III). This classification suffers of a lack of reproducibility, which could be overcome by the identification of specific molecular markers.In the present work, by real time quantitative PCR, ATP6V0A4 gene (encoding the renal a4) expression was quantified in 188 human glioma biopsies. We established a4 expression as a new marker of grade III oligodendrogliomas (35 % express it), independent of the 1p/19q codeletion, an established marker of oligodendrogliomas. Moreover, a4 is expressed in 70% of pilocytic astrocytomas, in which it is associated with the tandem duplication of 7q34, localized at direct proximity of the ATP6V0A4 gene. Of promising interest is the observation that a4 expression could be considered as a bad prognostic marker for patients with 1p/19q non-deleted oligodendrogliomas, an observation that should be confirmed on larger cohorts of patients.

V-ATPase

Exocytose

Syntaxine-1

VAMP2

ATP6V0A4

Gliome

Oligodendrogliome

Codélétion

1p/19q

KIAA1549:BRAF

Marqueur moléculaire

V-ATPase

Exocytosis

Syntaxin-1

VAMP2

ATP6V0A4

Glioma

Oligodendroglioma

Codeletion

1p/19q

KIAA1549:BRAF

Biomarker