Destoxificação de hidrolisados lignocelulósico visando à obtenção de etanol 2G / Detoxification of lignocellulosic hydrolysates aiming at obtaining ethanol 2G

Gomes, Márcia Andréa

24 February 2015

The sugarcane bagasse has a high content of lignocellulosic material, which enables the study for the production of second-generation ethanol, requiring the application of a pretreatment that promotes the rupture of the fiber, to make accessible sugars for fermentation. There are several pretreatments aimed at the break and in the search for the most productive one, it is applied severe conditions of temperature and pressure. This promotes the formation of undesirable products in the bioethanol production process, requiring detoxification step for removal of inhibitors. In this study, we used the detoxifying step for two pretreatments, hydrothermal and acid. The methodology raised the pH of the hydrolysates resulting from the acid pretreatment to 7.0 with calcium oxide and then decay to pH 4.0 with phosphoric acid. The hydrolysates of the hydrothermal pretreatment had its pH reduced to 4.0 by addition of phosphoric acid, both pretreated were subjected to adsorption on activated carbon (1% w /v , 100 rpm , 30 minutes at 50 ° C), conditions chosen after design 22 after triplicate with the center point. The evaluation of the efficacy of these procedures was made as to the removal of toxic compounds depending on the fermentation yield with the yeast Saccharomyces cerevisiae, hydrolysates with and without detoxification, assessing the amount of released sugars for conversion into second-generation ethanol. According to the results , the change of pH combined with activated carbon adsorption led to higher fermentation yields in both pretreated 38.51% acid and hydrothermal 44.85% hydrolyzed , when compared to the yield of samples not detoxified , these results may be associated with interference of lignin in the pulp, which can form condensation products able to interfere with the detoxification. However the best results were found in the hydrolysate hydrothermally pretreated with 87.94% efficiency and fermentation alcohol content of 7.41%, compared to the pre-treated hydrolysate with acid and 5.11% 75.05% respectively. / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / O bagaço de cana-de-açúcar possui alto teor de material lignocelulósico, o que viabiliza o estudo para a produção do etanol de segunda geração, sendo necessária a aplicação de um pré tratamento que promova a ruptura da fração fibrosa, para tornar os açucares acessíveis para fermentação. Existem vários pré-tratamentos que visam essa quebra, e na busca pelo mais produtivo são aplicadas condições severas de temperatura e pressão. Isso propicia a formação de produtos indesejáveis ao processo de produção do bioetanol, sendo necessária a etapa de destoxificação para remoção os inibidores. Nesse trabalho, foi empregado a etapa de destoxificação para dois pré-tratados acido e hidrotérmico, na metodologia utilizada elevou-se o pH dos hidrolisados provenientes do pré-tratamento acido para 7,0 com oxido de cálcio e em seguida o decaimento ate pH 4,0 com acido fosfórico, os hidrolisados do pré-tratamento hidrotérmico tiveram seu pH reduzidos para 4,0 com a adição do acido fosfórico, ambos os pré-tratados foram submetidos a adsorção em carvão ativado (1% m/v, 100rpm, 30 minutos a 50°C), condições escolhidas apos planejamento 22 com triplicata no ponto central. Avaliação da eficácia destes procedimentos foi feita quanto a remoção dos compostos tóxicos em função do rendimento fermentativo com a levedura Saccharomyces cerevisiae, de hidrolisados com e sem destoxificação, avaliando a quantidade de açúcares liberados para conversão em etanol de segunda geração. De acordo com os resultados, a alteração de pH combinada a adsorção com carvão ativo propiciou maiores rendimentos fermentativos em ambos os hidrolisados pré-tratados acido 38,51% e hidrotérmico 44,85%, quando comparados ao rendimento de amostras não destoxificadas, a esses resultados pode estar associado a interferência da lignina no bagaço, que pode formar produtos de condensação capazes de interferir na destoxificação. No entanto os melhores resultados foram encontrados no hidrolisado pré-tratado hidrotémicamente com 87,94% de eficiência de fermentação e teor alcoólico de 7,41%, quando comparado ao hidrolisado pré-tratado com acido de 75,50% e 5,11%, respectivamente.

Engenharia Química

Material lignocelulósico

Pré-tratamento

Destoxificação

Inibidores

Etanol 2G

Lignocellulosic materials

Pretreatment

Detoxification

Inhibitors

Ehanol 2G

CNPQ::ENGENHARIAS::ENGENHARIA QUIMICA

Clonagem gênica e caracterização de uma enzima tipoluciferase de coleópteros não bioluminescentes e sua relação com a origem da atividade luminescente

Prado, Rogilene Aparecida

06 March 2012

Made available in DSpace on 2016-06-02T20:20:33Z (GMT). No. of bitstreams: 1 4406.pdf: 2884968 bytes, checksum: a40d69433ee7cef0093f66b8c32c1bb8 (MD5) Previous issue date: 2012-03-06 / Universidade Federal de Minas Gerais / Bioluminescence in beetles is dependent on luciferase which evolved from AMP/CoA ligases. The cDNA of a luciferase-like enzime was cloned from the Malpighian tubules of Zophobas morio mealworm (Coleoptera: Tenebrionidae). The gene product of this cDNA displays weak luminescence and it is composed of 528 aminoacids residues with N-terminal and C-terminal sequences signal addressed to smooth endoplasmic reticulum membrane. Although having a low identity (26-32%) with beetle luciferases, this enzyme is a reasonable protoluciferase model to investigate the origin and evolution of beetle luciferases. The luciferin binding site is higly conserved among the beetle luciferases. However, in this protoluciferase of Z. morio, most of these residues of this motif are substituted by others. Using a site-directed mutagenesis survey some of aminoacids residues of this protoluciferase, which are located at correspondent luciferin binding site of luciferases, were replaced by the conserved residues of beetle luciferases. Most of the substitutions had negative effect on the luminescent activity, however, the substitution I327T, which is located in a β-hairpin motif close to the luciferin binding site, improved the luminescence activity. Such substitution indicates the importance of this motif for luciferase activity and indicates a possible route for the evolution of bioluminescence function of beetle luciferase. Since this enzyme is located in the Malpighian tubules, which are involved in excretion and metabolization of carboxylic substrates, this enzyme could be involved to excretion the some type of chemical compound. Regardless of the function the results show that the potential for bioluminescent activity is older and probably arose before the divergences of the Coleoptera bioluminescent families. / A bioluminescência em coleópteros é dependente das luciferases, enzimas que evoluíram das AMP-CoA ligases. O cDNA de uma enzima tipo-luciferase foi clonado dos túbulos de Malphighi de larvas de Zophobas morio (Coleoptera: Tenebrionidae). O produto gênico deste cDNA mostra naturalmente uma fraca luminescência na presença de MgATP e luciferina e possui 528 aminoácidos com sequências sinal na região N-terminal e C-terminal endereçadas a membrana do retículo endoplasmático liso. Apesar de ter uma baixa identidade (26-32%) com as luciferases de vaga-lumes, esta enzima é um modelo apropriado de protoluciferase para investigar a origem e evolução das luciferases de besouros. O sítio de ligação da luciferina é altamente conservado entre todas as luciferases de besouros; na protoluciferase de Z. morio porém, a maioria dos resíduos desta região é substituído por outros. Utilizando-se a técnica de mutagênese sitio-dirigida, alguns resíduos de aminoácidos desta protoluciferase, que são localizados na correspondente região do sítio ativo das luciferases, foram substituídos pelos resíduos conservados das luciferases. A maioria das substituições teve um efeito negativo sobre a atividade luminescente. Porém, a substituição I327T, cujo resíduo é localizado em um motivo grampo β, perto do sítio de ligação da luciferina, aumentou sua atividade luminescente. Tal substituição mostra a importância deste motivo para a atividade luciferásica e indica uma possível rota de evolução das luciferases de coleópteros. Uma vez que esta enzima foi extraída dos túbulos de Malpighi, é possível que esteja envolvida com a excreção de algum composto químico. Independente de sua função, os resultados do presente trabalho sugerem que o potencial para atividade bioluminescente é bem antigo nas ligases e provavelmente evoluíram antes da divergência das famílias de coleópteros bioluminescentes.

Bioquímica

Protoluciferase

Zophobas morio

Túbulos de Malpighi

Desintoxicação metabólica

AMP-CoA ligase

Protoluciferase

Malpighian tubules

AMP-CoA ligase

Detoxification

CIENCIAS BIOLOGICAS::GENETICA

Simulação de um aquecedor solar de água como etapa do processo de destoxicação da torta de mamona

Josenildo Araujo da Silva

00 December 2007

Diversos procedimentos têm sido utilizados para destoxicação da torta de mamona. Entre esses a solubilização das substâncias responsáveis pelo caráter tóxico desse resíduo, ricina e ricinina, em água quente e/ou soluções salinas aquecidas. Foram desenvolvidos algo ritmos para simular o aquecimento solar da água como estratégia para baixar custos no processo de destoxicação da torta de mamona, originária do processo de produção de biodiesel. Para isto foi utilizada a ferramenta computacional Simulink/MATLAB@. Foram então analisadas várias situações com base na proposta de aquecimento direto, por se tratar de uma forma de transferência de calor menos dispendiosa. São propostos modelos dinâmicos em diferentes graus de complexidade para uma avaliação prévia do processo de aquecimento da água por meio de energia solar. Apresentam-se os diagramas de blocos dos modelos computacionais, correspondentes a cada uma das etapas de elaboração. Os modelos matemáticos propostos proporcionaram importantes previsões para valores de temperatura nas diferentes fases de elaboração. apresentando-se como importante ferramenta de trabalho para uma próxima etapa que é a de validação experimental do modelo final / Algorithms have been developed in arder to simulate the water solar heating as a strategy for lowering castor bean pie destoxication costs, among from the biodiesel oil for production extraction processo Diverse procedure, substances solubilization, this residue toxic caracter factor, found in hot water and in some saline solutions, motivated this water heating modeling work, through solar energy, since this procedure type can and low cost to the above-mentioned methods, on account of this, one has used computational smulink/matlab in arder to simulate and to arise favorable conditions for this technique use strategies elaboration. One has, then, analized several situation, departing from a termal heating proposal, since this is a less expensive heat transference formo Of this form an objective function was proposal to create O variable that esteem the behavior of the system and better define the excellent conditions for the considered processo .Among these, the established variable as parameters for the simulated conditions, are presented the results, taking itself in account values of income for the process, existing in literature. One porpuses dynamic models, under complexity different degress, for a water heating process previous evaluation, through solar energy. Temperature variations, in the process diferrent stages, have been simulated, with simulink/matlab aid for the above-mentioned system behaviour analysis one presents computational models. blocks diagrams, correspondent to each one of the elaboration stage. Proposed mathematical models provided important previsions for temperature values, in the above-mentioned system different components, resulting as a work important tool for a next stage which is that one of the optimization

simulação (computadores)

métodos de simulação

aquecimento solar

aquecedores solares de água

torta de mamona - destoxicação

dissertações

computer simulation

simulation methods

solar heating

solar water heaters

detoxification of castor cake

dissertation

CIENCIAS BIOLOGICAS

Estudo dos efeitos da radiacao gama de sup(60)Co na peconha de Apis mellifera: aspectos bioquimicos, farmacologicos e imunologicos

COSTA, HELENA

09 October 2014

Made available in DSpace on 2014-10-09T12:45:13Z (GMT). No. of bitstreams: 0 / Made available in DSpace on 2014-10-09T13:56:31Z (GMT). No. of bitstreams: 1 07293.pdf: 5734585 bytes, checksum: d14fa6efc5fe260e124df558d69af5bd (MD5) / Tese (Doutoramento) / IPEN/T / Instituto de Pesquisas Energeticas e Nucleares - IPEN/CNEN-SP

radiation effects

ionizing radiations

gamma radiation

cobalt 60

bees

venoms

toxicity

detoxification

molecular structure

liquid column chromatography

high-performance liquid chromatography

Ampliação de escala da produção biotecnológica de xilitol a partir do bagaço de cana-de-açúcar / Evaluation of the biotechnological process for xylitol obtainment at different scales from the sugarcane bagasse hemicellulosic hydrolysate

Priscila Vaz de Arruda

15 July 2011

A conversão de biomassa vegetal em produtos químicos e energia é essencial a fim de sustentar o nosso modo de vida atual. O bagaço de cana-de-açúcar, matériaprima disponível em abundância no Brasil, poderá tanto ajudar a suprir a crescente demanda pelo etanol combustível como ser empregado para obtenção de produtos de valor agregado, tais como xilitol, além de trazer vantagens econômicas para o setor sucroalcooleiro. O xilitol, um poliol com poder adoçante semelhante ao da sacarose e com propriedades peculiares, como metabolismo independente de insulina, anticariogenicidade e aplicações na área clínica, no tratamento de osteoporose e de doenças respiratórias, é obtido em escala comercial por catálise química de materiais lignocelulósicos. A produção biotecnológica de xilitol como alternativa ao processo químico vem sendo pesquisada e os resultados revelam que a presença de compostos tóxicos nos hidrolisados hemicelulósicos resultantes do processo de hidrólise ácida contribui para sua baixa fermentabilidade. Isto se deve à inibição do metabolismo microbiano causada principalmente por compostos tais como ácidos orgânicos, fenólicos e íons metálicos. No presente trabalho foi avaliado o efeito de diferentes fontes de carbono (xilose, glicose e mistura de xilose e glicose) empregadas no preparo do inóculo de Candida guilliermondii FTI 20037 sobre a bioconversão de xilose em xilitol a partir de fermentações em frascos Erlenmeyer de hidrolisados hemicelulósicos submetidos a procedimentos de destoxificação. A condição de favorecimento deste bioprocesso foi empregada para a avaliação da ampliação de escala em fermentadores de 2,4L para 16L, utilizando como critério de ampliação o KLa (igual a 15h-1). De acordo com os resultados, os máximos valores dos parâmetros fermentativos como fator de conversão de xilose em xilitol e produtividade em xilitol foram alcançados com a utilização de inóculo obtido em xilose durante fermentação do hidrolisado destoxificado por resinas (YP/S = 0,81 g g-1 e QP = 0,60 g L-1 h-1, respectivamente), embora o emprego de carvão ativado tenha gerado valores de rendimento próximos para as diferentes fontes de carbono (YP/S variando de 0,78 a 0,80 g g-1). Considerando o valor de fator de conversão e que o procedimento de destoxificação com carvão ativado é o de menor custo e de mais fácil manipulação em comparação ao processo com resinas, os experimentos de ampliação de escala da produção de xilitol por C. guilliermondii foram realizados nesta condição de destoxificação e empregando-se xilose como fonte de carbono para o inóculo. Nesta etapa ficou evidente a viabilidade de ampliação de escala de produção de xilitol de fermentador de 2,4L para 16L, já que os valores dos parâmetros fermentativos avaliados foram semelhantes entre os fermentadores (valores médios: YP/S ≈ 0,68 g g-1 e QP ≈ 0,28 g L-1 h-1). No entanto, tais valores foram inferiores aos obtidos em frascos Erlenmeyer, possivelmente devido às condições de disponibilidade de oxigênio diferirem nos fermentadores de bancada, uma vez que o oxigênio é o parâmetro mais crítico neste bioprocesso. / The conversion of vegetable biomass into chemicals and energy is essential to sustain our current style of life. Sugarcane bagasse, a raw material abundantly available in Brazil, greatly contributes to the supply of the evergrowing demand for ethanol. Furthermore, biomass can be employed for obtaining value-added products, such as xylitol, as well as bring economical advantages for the sugar-ethanol sector. Xylitol, a polyol with sweetener power similar to that of saccharose and peculiar properties such as insulin-independent metabolism, anticariogenic power, and applications in the clinical area, in the treatment of osteoporosis and respiratory diseases, is obtained on a commercial scale by chemical catalysis of lignocellulosic materials. The biotechnological production of xylitol as an alternative to the chemical process has been researched and the results reveal that the presence of toxic compounds in hemicelllosics hydrolysates resulting from acid hydrolysis process contributes to its low fermentability. Such toxicity could be due to the inhibition of microbial metabolism promoted mainly by compounds such as organic acids, phenols and metallic ions. In the present work, the effect of different carbon sources (xylose, glucose and a mixture of xylose and glucose) used in the inoculum preparation of Candida guilliermondii FTI 20037 for the xylose-to-xylitol bioconversion by fermentation of hemicellulosics hydrolysates submitted to detoxification procedures in Erlenmeyer flasks was evaluated. The best condition for this bioprocess was employed to evaluate the scale up from the 2.4L to 16L fermentors, using KLa (equal to 15h-1) as scale-up criteria. According to the results the highest values of fermentative parameters such as xylitol yield and productivity were achieved with the use of inoculum cultivated on xylose during the fermentation of hydrolysate detoxified with resins (YP/S = 0.81 g g-1 and QP = 0.60 g L-1 h-1, respectively), although with the use of charcoal the yield value was similar (YP/S ranging for 0.78 to 0.80 g g-1), regardless of the carbon source employed. Considering the value of xylitol yield and that detoxification with activated charcoal is less expensive and more easily manipulated when compared to detoxification procedure with resins, the experiments for scale up xylitol production by C. guilliermondii were performed in such detoxification condition with xylose as the carbon source for the inoculum. At this stage it was evident the scale up xylitol production from a fermenter of 2.4L to 16L was feasible, since the values of fermentative parameters evaluated were similar to those of the fermentors (medium values YP/S ≈ 0.68 g g-1 e QP ≈ 0.28 g L-1 h-1). However, these values were lower than those obtained in Erlenmeyer flasks, maybe due to conditions of oxygen availability for they differ from those in fermentors, since oxygen is the most critical parameter in this bioprocess.

Ampliação de escala

Bagaço de cana-de-açúcar

Candida guilliermondii

Destoxificação

Hidrolisado hemicelulósico

Xilitol

Candida guilliermondii

Detoxification

Scale-up

Xylitol

Rôle des facteurs de l’hôte dans le maintien des prophages chez les entérobactéries / Host factors involvement in prophage maintenance in Enterobacteriaceae

Delannoy, Maëlle

15 December 2016

Les prophages sont des vecteurs majeurs de l’évolution des génomes bactériens et ont des rôles divers dans le processus adaptatif de leurs hôtes et peuvent leur apporter un avantage sélectif. Au cours de l’évolution, certains gènes prophagiques peuvent être perdus, notamment ceux codant pour des protéines du cycle lytique. Cependant, alors que certains de ces prophages défectifs sont capables de s’exciser, ils sont maintenus dans le génome de l’hôte, suggérant une pression sélective pour les conserver. C’est le cas du prophage défectif KplE1 chez E. coli K12. Dans l’équipe, des travaux ont mis en évidence que le maintien en lysogénie de différents prophages était sous le contrôle du terminateur de la transcription bactérien Rho. Afin d’identifier de nouveaux facteurs de l’hôte impliqués dans le maintien des prophages, j’ai développé un crible génétique qui m’a permis d’identifier plusieurs candidats impliqués dans le métabolisme général, la détoxification du NO ou qui appartiennent à un autre prophage défectif. Mon travail a été de discriminer lesquels de ces candidats jouaient un rôle significatif dans le maintien des prophages. Sur les trois gènes impliqués dans la détoxification du NO, seule l’expression de norV ou norW permet le maintien de KplE1. NorV réduit le NO et cette réduction nécessite l’utilisation d’un électron généré par l’oxydation du NADH par NorW. J’ai pu également montrer que l’expression du gène norV permettait le maintien d’un autre prophage fonctionnel (HK620) partageant le même module de recombinaison spécifique de site que KplE1. L’ensemble de mes résultats montre qu’il existe un lien co-évolutif important entre les prophages et leurs hôtes. / Prophages play recognized roles in their host genomes evolution and adaptation to variable ecosystems. They can provide to their host selective advantages that increase their competitiveness. Upon evolution, some prophage genes can be lost, especially those coding for lytic cycle capacity. While some of the defective prophages are perfectly competent for excision, they prove to be maintained in bacterial genomes, suggesting the involvement of a selective pressure. This is the case for our defective prophage model: KplE1 in E. coli K12. Previous work in our laboratory demonstrated that lysogeny maintenance of various prophages was controlled by Rho which is the bacterial transcription termination factor. In order to identify new host factors involved in prophage maintenance, I developed a genetic screen. This screen allowed me to identify candidate genes involved in bacterial general metabolism, in NO detoxification and also some genes that belong to another defective prophage. I determined which candidate genes actually played a role in KplE1 maintenance. Among the three genes involved in NO detoxification, I showed that norV or norW individual expression allowed KplE1 maintenance. NorV reduces NO and this reduction needs an electron produced by NorW NADH oxidation. I also showed that norV expression allowed the maintenance of another functional prophage (HK620) that shares the same site specific recombination module as KplE1. Together, my results illustrate the coevolution between prophages and their hosts.

Prophages

Maintien lysogénie

NorV

Détoxification du NO

Recombinaison spécifique de site

Coévolution

Prophages

Lysogeny maintenance

NorV

NO detoxification

Site specific recombination

Coevolution

579

Caractérisation des fonctions neuroprotectives des interfaces sang-cerveau au cours du développement normal, dans les tumeurs périventriculaires et dans un modèle d’excitotoxicité périnatale / Characterization of the neuroprotective functions of blood-brain interfaces during normal development, in periventricular tumors and in a model of perinatal excitotoxic injury

Vasiljevic, Alexandre

21 December 2017

Les interfaces sang-cerveau comme la barrière hémato-encéphalique (BHE), les plexus choroïdes (PC) ou les organes circumventriculaires (OCV), constituent des barrières physiologiques nécessaires au fonctionnement du système nerveux central. Ces barrières sont à la fois « physiques », constituées de jonctions serrées, et « enzymatiques ». Longtemps considérées comme immatures chez le fœtus, ces barrières sont en réalité présentes précocement au cours du développement. Leurs caractéristiques et leurs propriétés restent peu connues chez l'homme. Nos travaux montrent que les PC expriment, précocement au cours du développement, des protéines de jonction serrée, les claudines (CLDN) 1, 2 et 3 chez le rat et chez l'homme. Cette expression est dynamique au cours du développement avec une apparition progressive de la CLDN2 pouvant avoir un lien avec la sécrétion du liquide céphalo-rachidien. Les CLDN 1 et 3 sont identifiées chez le fœtus humain au niveau de l'organe sous-commissural (OSC), un des OCV. La CLDN5 est exprimée précocement au niveau de la BHE chez le rat et chez l'homme et son expression est altérée dans un modèle d'excitotoxicité néonatale. Nos travaux montrent également que l'analyse du profil des CLDN est utile en pathologie tumorale notamment dans la compréhension et le diagnostic de tumeurs développées à partir des PC ou de l'OSC. Enfin, diverses enzymes antioxydantes et de détoxification dont l'époxyde hydrolase microsomale sont exprimées à 22 semaines d'aménorrhée principalement au niveau des PC du fœtus humain. Ces données suggèrent des capacités de détoxification des PC, d'installation précoce au cours du développement chez l'homme / Blood-brain interfaces including blood-brain barrier (BBB), choroid plexuses (CP) or circumventricular organs (CVO) are physiological barriers required for brain homeostasis. These barriers are “physical”, with tight junctions, and “enzymatic”. Though long considered immature in fetuses, these barriers are present from an early stage of development. Their characteristics and their properties are largely unknown in humans. Our work demonstrates that CP express tight junction-associated proteins claudins (CLDN) 1, 2, and 3 at early stages of development in rat and human. This expression is dynamic during development as shown by the progressive increase of CLDN2 immunopositivity that may follow increase in cerebrospinal fluid secretion. CLDN 1 and 3 are identified in human fetal subcommissural organ (SCO), one of the CVO. CLDN5 is early expressed in rat and human BBB and its expression is disrupted by excitotoxic injury. Our work also shows that CLDN immunohistochemical profile is useful in tumoral pathology, notably to better understand and diagnose tumors arising from CP or the SCO. Finally, various antioxidant and detoxifying enzymes such as the microsomal epoxide hydrolase are expressed at 22 weeks of gestation in the human fetus, mainly in CP. These results suggest a high detoxifying capacity for the CP during development in humans

Interfaces sang-cerveau

Plexus choroïdes

Claudine

Développement

Tumeurs cérébrales

Détoxification

Excitotoxicité

Blood-brain interfaces

Choroid plexus

Claudin

Development

Brain tumors

Detoxification

Excitotoxicity

612.8

Exposition néonatale aux œstrogènes : effets sur leur métabolisme, le développement ovarien et la fonction de reproduction chez la ratte / Neonatal estrogen exposure in the rat : effects on metabolism, ovarian development and reproductive function

Chalmey, Clémentine

27 November 2013

L'ovaire est au cœur de la physiologie de la reproduction féminine. Il est à la fois à l'origine des ovocytes nécessaires à la fécondation et acteur des régulations endocrines du système reproducteur. Les ovocytes de l'ovaire fœtal sont groupés en amas bordés de cellules somatiques et d'une membrane basale, formant les cordons ovariens. Ces cordons ovariens se fragmentent pour former les follicules ovariens: un ovocyte bordé de cellules somatiques et d'une membrane basale. Cette fragmentation se déroule sur une courte période (/in utero/ chez la femme et juste après la naissance chez les rongeurs) et fait intervenir une vague de mort cellulaire programmée touchant les ovocytes pendant leur méiose et un remodelage de la membrane basale. La formation des follicules est une période cruciale du développement ovarien puisque le stock de follicules formés à l'issue de ce processus est non renouvelable. Son altération peut donc être à l'origine de troubles de la fonction de reproduction chez le futur adulte. Il existe une fragile homéostasie œstrogénique en place au moment de la formation folliculaire: chez la femme, l'ovaire se développe /in utero/, sous l'influence des œstrogènes circulants maternels et la production ovarienne fœtale. Chez les rongeurs, les follicules se forment lors de la levée de l'imprégnation hormonale maternelle au moment de la naissance. Nous avons souhaité comprendre comment le 17b-œstradiol (E2), œstrogène endogène, pouvait contribuer à la mise en place des follicules. Pour cela, des rattes Sprague-Dawley ont été traitées pendant la période de formation des follicules avec de l'E2 à différentes doses entre 0.01 et 10 µg/jour. Nos travaux démontrent que le traitement de rattes par des œstrogènes entre leur naissance et 3 jours induit une réduction dose-dépendante de leur nombre d'ovocytes. Bien que le traitement entrave le développement normal du système de détoxication hépatique et ovarien, l'animal est capable d'accroître ses capacités d'élimination des œstrogènes. Ces capacités sont toutefois insuffisantes pour bloquer les effets du traitement. Quelle que soit la dose d'E2 utilisée (0.1 ou 10 µg/jour), la puberté est plus précoce chez les femelles exposées mais toutes sont fertiles, au moins transitoirement. Cependant le traitement induit une dégradation rapide des capacités reproductives. L'E2 modifie la dynamique folliculaire chez l'adulte, longtemps après l'arrêt du traitement. Si une forte dose d'E2 réduit la survie des ovocytes lors de la formation des follicules et conduit à une infertilité secondaire due à un dysfonctionnement général du tractus reproducteur, une dose faible n'affecte pas la survie des ovocytes à court terme mais conduit à une sénescence reproductive précoce vraisemblablement d'origine ovarienne. L'origine de ces troubles pourrait résider dans les effets précoces de l'exposition à E2 : cette molécule altère le transcriptome ovarien et induit de nombreuses lésions de l'ADN des cellules ovariennes. / The ovary is not solely the unique source of oocytes necessary for fertilization but also a crucial conductor of endocrine regulations of the reproductive system. In the fetal ovary, oocytes grouped in clusters are surrounded by somatic pre-granulosa cells, altogether delineated by a basement membrane and constituting ovarian cords. The formation of the definitive ovarian functional units requires their fragmentation into follicles formed by a single oocyte surrounded by granulosa cells and delineated by a basement membrane. This partitioning occurs within a tiny period and is dependent on the correct timing of the meiotic process, on an apoptotic wave that specifically targets oocytes and the remodelling of the basement membrane. Follicle formation is a crucial event of ovarian development because the follicle stock formed at the end of this process is non-renewable. Therefore, any disturbance of this process can lead to reproductive abnormalities in adulthood. Recent data on endocrine disruptors displaying estrogenic activity have involved the fragile estrogenic homeostasis in the process. We aimed at better understanding how the endogen estrogen 17b-estradiol (E2) contributes to follicle formation. To assess it, Sprague-Dawley rats were treated with E2 at different doses during follicle formation, /i.e./ in the 3 days following birth. We show that although this treatment impairs the development of the hepatic and ovarian detoxification systems, the female neonate is able to increase its estrogen clearance capabilities. Nevertheless, E2 treatment within this critical period triggers a dose-dependent decrease of oocyte number per ovary. Regardless of the E2 dose, puberty is advanced. All treated females are at least transiently fertile, yet these reproductive capabilities rapidly decline. A high (10 µg/day) dose of E2 leads to a secondary infertility characterized by anovulation that probably result from a dysfunction of the whole reproductive tract. By contrast, a lower (0.1 µg/day) dose of E2, that does not significantly modify neonatal oocyte survival, leads to a progressive reproductive senescence likely due to ovarian failure. Long-term troubles may originate from precocious E2 impact on the ovary since it disturbs ovarian transcriptome and produces many lesions on ovarian cell DNA.

Toxicologie de la reproduction

Œstrogènes

Xéno-œstrogènes

Ovaire

Ovocytes

Follicule ovarien

Apoptose

Détoxication

Fertilité

Reproductive toxicology

Estrogen, Xeno-estrogens

Ovary

Oocyte

Ovarian follicle

Apoptosis

Detoxification

Fertility

Metody dekotoxifikace hydrolyzátů lignocelulózových materiálů / Detoxification of lignocellulose hydrolyzates

Vašíčková, Monika

January 2017

The aim of this work was study of the detoxification of lignocellulose material hydrolysates and to investigate sawdust suitability as a substrate for microbial production of PHA by bacteria Burkholderia cepacia and Burkholderia sacchari. In the experimental part of the work the most suitable way of detoxification of model and real hydrolysate was studied. After that, detoxification methods used were evaluated. Criteria for evaluation were concentration of polyphenols as the most important microbial inhibitors and reduction saccharides as the main carbon substrate. Furthermore, fermentability of the hydrolysates was also tested by cultivation of two bacteria capable of PHA accumulation. Burkholderia sacchari demonstrated higher ability to accumulate PHA then Burkholderia cepacia. Then in the summary – most effective way for detoxification was ‚overliming‘. Major increase of PHB in biomass was obtained when Burkholderia sacchari was cultivated on media gained by application of overliming of real lignocellulose hydrolysate. However, total gains of PHB were more likely low and then sawdust can not be considered as a substrate for PHB production at industrial scale.

Rôle du domaine extracellulaire d’ABCG2 dans l’homéostasie des porphyrines / Role of the extracellular domain of ABCG2 in porphyrin homeostasis

Desuzinges-Mandon, Elodie

23 November 2010

ABCG2 est un transporteur de la famille ABC impliqué dans le phénotype de résistance aux drogues développé par certaines cellules, par exemple les cellules cancéreuses. Ce transporteur a aussi un rôle physiologique de détoxication de composés endogènes, notamment les porphyrines, molécules indispensables mais qui présentent une toxicité potentielle. Cette toxicité nécessite une prise en charge particulière, évitant à ces composés d’être libres en solution. Dans ce contexte, nous avons fait l’hypothèse qu’ABCG2 pourrait participer à cette détoxication en limitant l’accumulation des porphyrines dans les cellules en les présentant à un partenaire extracellulaire. Nous montrons qu’ABCG2 transporte de l’hème ainsi que certains de ses dérivés et précurseurs et que ces porphyrines, contrairement aux autres substrats d’ABCG2, se fixent sur un domaine extracellulaire spécifique d’ABCG2, ECL3, composé d’environ 70 acides aminés. L’affinité d’ECL3 pour les porphyrines est de 0,5 à 3,5 μM, suffisamment affine pour permettre leur fixation après transport.Nous montrons aussi que l’albumine sérique humaine, impliquée dans la détoxication de l’hème, récupère les porphyrines fixées sur ECL3 par une interaction directe avec ABCG2. L’ensemble de ce travail a donc permis d’une part de mieux comprendre le rôle d’ABCG2 dans la régulation de l’homéostasie des porphyrines, notamment l’hème, et d’autre part, de façon originale, d’identifier le mécanisme moléculaire par lequel cette détoxication s’effectue. / ABCG2 belongs to the ABC-transporter family, involved in drug resistance developed by cells, notably cancer cells. This transporter has also a physiological role of endobiotic detoxification, in particular porphyrins that are essential but potentially toxic molecules. This toxicity implies a specific handle, to avoid them to remain free in solution. In that context, we hypothesized that ABCG2 participate to this detoxification, limiting the intracellular porphyrin accumulation by presenting them to an extracellular partner. We show that ABCG2 transports heme and some of its derivatives and precursors. Interestingly, these porphyrins, unlike other ABCG2 (non-porphyric) substrates, can bind to an extracellular domain, specific of ABCG2, ECL3, 70 residues-long. ECL3 displays affinities for porphyrins in the range of 0.5 to 3.5 μM, high enough to allow their binding after transport. We also show that human serum albumin, implicated in heme detoxification, releases porphyrins bound to ECL3 by a direct interaction with ABCG2. This work established a better comprehension of ABCG2 role in porphyrin and in particular heme homeostasis regulation. In addition, our results contribute to elucidate part of the molecular mechanism by which such regulation is carried out.

Porphyrines

Détoxication

Albumine

Interaction protéine-ligand

Transporteur ABC

ATP-Binding cassette transporters

Porphyrins

Detoxification

Albumin

Protein–ligand interactions

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