Étude de la régulation des canaux potassiques ROMK1 par un antidiabétique, la rosiglitazone implication des PPARgamma

Ait Benichou, Siham

January 2011

Les thiazolidinediones (TZDs) sont des médicaments antidiabétiques (agonistes des récepteurs nucléaires de type PPAR[gamma]) utilisés au cours des dix dernières années pour le traitement du diabète de type II. Malheureusement leur utilisation peut provoquer, chez certains patients, une rétention accrue de fluides et une formation d?oedèmes rénaux. Des études récentes suggèrent l'implication d'un canal sodique épithélial (ENaC), exprimé au niveau du tubule collecteur rénal, dans ces effets secondaires. En effet, la stimulation des PPAR[gamma] par les TZDs activent les canaux sodiques épithéliaux probablement via l'expression et l'activation de SGK1 (Serum and Glucocorticoid-regulated Kinase 1). Sachant que les transports des ions sodiques et potassiques sont étroitement liés au niveau rénal, notre objectif est de déterminer si les TZDs seraient impliqués dans la régulation des canaux potassiques (ROMK1). Nous montrons qu'en traitant les ovocytes de xénopes exprimant ROMK et PPAR[gamma], avec un TZDs comme la rosiglitazone (RGZ), le courant potassique mesuré par voltage-clamp (TEVC) est augmenté de deux fois. Cette augmentation est bloquée par l'utilisation d'un antagoniste de PPAR[gamma], le GW9662. Nous démontrons aussi l'implication de SGK1 dans la régulation de l'activité des canaux ROMK1 d'une part en mutant son site de phosphorylation sur ROMK1 (sérine 44) et d'autre part en utilisant son inhibiteur, GSK. Finalement les expériences d'immunofluorescences ont montré un recrutement de ROMK1 à la membrane des ovocytes traités à la RGZ. L'ensemble des données présentées dans ce travail suggère que la RGZ augmente le courant potassique en augmentant l'expression de SGK1.

Xenopus laevis

Oocyte

Rosiglitazone

SGK1

PPAR[gamma]

ROMK1

Oocyte-Granulosa Cell Signaling in 4-Vinylcyclohexene Diepoxide-Induced Ovotoxicity

Fernandez, Shannon Marie

January 2007

At birth, the mammalian ovary has a finite number of dormant primordial follicles. Repeated daily dosing of rats with the occupational chemical, 4- vinylcyclohexene diepoxide (VCD), depletes the ovary of small pre-antral follicles (primordial and primary follicles) through an increase in the natural process of atresia (apoptosis). In addition, in vitro exposure of postnatal day 4 (PND4) rat ovaries to VCD causes a similar depletion of ovarian follicles. Since many growth factors play crucial roles in the promotion of early folliculogenesis and follicle survival, it is possible that any number of factors and subsequent signaling pathways could be disrupted in response to VCD exposure. Therefore, the studies in this work address the hypothesis that VCD disrupts oocyte-granulosa cell survival pathways in the rat ovary, thereby compromising cell-cell communication and causing follicle cell death. The results from the first aim reveal that through the use of genomic analyses a subset of genes were determined to be affected via in vivo and in vitro exposure routes to VCD. The results of the second aim show that two transforming growth factor β (TGFβ) growth factors, growth and differentiation factor-9 (GDF-9), and bone morphogenetic factor-4 (BMP-4), are not likely involved in VCD-induced ovotoxicity as they were unable to prevent ovarian follicle loss in the presence of VCD. The results of the third aim reveal that expression of the c-Kit receptor, present on the oocytes, is decreased and its ligand, Kit Ligand (KL), produced from the granulosa cells, is increased in response to in vitro VCD exposure. In addition, attenuation of VCD-induced follicle loss occurs in the presence of exogenous KL. Finally, the results of the fourth aim examines the involvement of the AKT signaling molecule in response to VCD exposure, in which the active phosphorylated AKT is determined to be down-regulated by VCD. Taken together, these studies show that VCD is able to disrupt at least one of the cellular survival pathways that are crucial to maintain the ovarian follicle. As a result, a breakdown in cell-cell communication may occur at that level and contribute to an increase in follicular atresia and eventual cell death.

Oocyte

Granulosa Cell

Ovarian Toxicity

Follicle

Signal Transduction

Atresia

Role of TAp73 in Female Reproductive Aging and Fertility

Yavorska, Tetyana

15 November 2013

An increasing number of women delay childbearing and consequently face infertility and pregnancy complications associated with age. The central contributor to compromised reproductive performance is poor oocyte quality. Despite advances in assisted reproductive technologies, a strategy to overcome the damage that oocytes receive with age is yet to be identified. This work focuses on the influence of TAp73, a protein that decreases in mouse and human eggs with age, on the developmental capacity of mouse oocytes. TAp73 deficient mice were found to have fewer active mitochondria and compromised clearance of damaged material in their oocytes, possibly due to reduced mTOR-TAp73 axis signaling. These qualities were shown to contribute to low oocyte maturation rates. Additionally, TAp73 likely mediates the action of coenzyme Q10, which restores oocyte TAp73 levels and mitochondrial quality in aged mice. Together these findings suggest that TAp73 is a promising therapeutic target for improving oocyte function.

fertility

oocyte

metabolism

mitochondria

aging

TAp73

0380

0719

0307

Role of TAp73 in Female Reproductive Aging and Fertility

Yavorska, Tetyana

15 November 2013

An increasing number of women delay childbearing and consequently face infertility and pregnancy complications associated with age. The central contributor to compromised reproductive performance is poor oocyte quality. Despite advances in assisted reproductive technologies, a strategy to overcome the damage that oocytes receive with age is yet to be identified. This work focuses on the influence of TAp73, a protein that decreases in mouse and human eggs with age, on the developmental capacity of mouse oocytes. TAp73 deficient mice were found to have fewer active mitochondria and compromised clearance of damaged material in their oocytes, possibly due to reduced mTOR-TAp73 axis signaling. These qualities were shown to contribute to low oocyte maturation rates. Additionally, TAp73 likely mediates the action of coenzyme Q10, which restores oocyte TAp73 levels and mitochondrial quality in aged mice. Together these findings suggest that TAp73 is a promising therapeutic target for improving oocyte function.

fertility

oocyte

metabolism

mitochondria

aging

TAp73

0380

0719

0307

Analýza krátkých izoforem proteinů Argonaut z myších oocytů / Analysis of short Argonaute isoforms from mouse oocytes

Jankele, Radek

January 2015

AnalysisofshortArgonauteisoformsfrommouseoocytes Abstract: Argonaute proteins carrying small RNAs form the conserved core of RNA silencing mechanisms, which repress viruses, mobile genetic elements, and genes in a sequence specific manner. The microRNA (miRNA) pathway is a dominant mammalian RNA silencing mechanism in somatic cells, which post-transcriptionally regulates large fraction of genes and thereby adjusts protein levels. miRNA-guided Argonautes inhibit translation and induce deadenylation of complementary mRNAs, ultimately resulting in their decay. In contrast to RNA interference (RNAi), which employs Argonaute slicer activity to directly cleave perfectly complementary RNAs, an effective miRNA-mediated mRNA repression requires multiple Argonaute-associated protein factors and enzymes. The miRNA pathway has been implicated in many complex biological processes ranging from organogenesis, stress-response to haematopoiesis or cancer. Surprisingly, canonical miRNAs are not essential for oocytes and early embryonic development in mice. Even the most abundant miRNAs present in mouse oocytes are unable to effectively repress target genes. However, RNAi, which shares key enzymes with the miRNA pathway, is highly active in oocytes and early embryos. The cause of miRNA inactivity in mouse oocytes remains...

The biology of acentriolar MTOCs in the mouse oocyte / La biologie des centres d?organisation des microtubules acentriolaires dans l`ovocyte de souris

Dziugiel, Malgorzata

13 June 2014

La méiose chez les femelles est un processus de réduction du génome permettant la formation d'un gamète haploïde, l'ovocyte. Dans la plupart des espèces animales, l'ovogénèse est associée à une élimination des centrioles, composants des centrosomes, qui sont les centres organisateurs des microtubules (MTOCs) canoniques. En l'absence de centrioles, le fuseau méiotique est assemblé grâce à la large contribution des MTOCs. Cependant, leur origine, l'importance de leur organisation et de la régulation de leur activité sont peu comprises. J'ai démontré que les MTOCs sont déjà présents dans les ovocytes précurseurs et sont progressivement rassemblés sur l'enveloppe nucléaire chez les ovocytes compétents pour les divisions méiotique. A l'entrée en méiose, les MTOCs sont distribués autour des chromosomes qui se condensent de façon strictement régulée au cours du temps. La perturbation de l'organisation des MTOCs par une surexpression de la kinase Polo-like 4 (Plk4) altère l'activité de nucléation des microtubules à l'entrée en méiose. L'activité anormale de ces MTOCs conduit à la formation de fuseaux non fonctionnels et à l'arrêt méiotique. / Female meiosis is a fundamental process of genome reduction leading to formation of a haploid gamete, the oocyte. In most animal species, oogenesis is associated with elimination of centrioles, constituents of centrosomes, which are canonical Microtubule Organizing Centers (MTOCs). In the absence of centrioles, meiotic spindle is assembled with a large contribution of acentriolar MTOCs. However, their origins, importance of organization and regulation of activity are poorly understood. I have shown that MTOCs pre-exist in the oocyte precursors and that they are progressively gathered on the nuclear envelope as oocytes gain competency for meiotic divisions. At entry into meiosis, MTOCs are redistributed around the condensing chromosomes in a strictly regulated timely fashion. Perturbation of such MTOC organization by transgenic overexpression of Polo-like kinase 4 (Plk4) leads to altered MT-nucleating activity at meiotic entry. Such abnormally active MTOCs mediate the formation of large and non-functional spindles and meiotic arrest.

MTOCs

PCM

Plk4

Assemblage du fuseau

Ovocyte

Oocyte

MTOCs

571.6

Alimentação de novilhas com uréia por curto prazo afeta a qualidade de complexos cumulus oócito e o desenvolvimento de embriões In vitro / Short-term urea feeding affect quality of cumulus oocyte complexes and In vitro embryo development

Ferreira, Fernanda Altieri

31 August 2007

A utilização de uréia na alimentação de fêmeas bovinas pode prejudicar o desempenho reprodutivo destes animais, provavelmente decorrente do aumento do teor de nitrogênio uréico plasmático (NUP). O objetivo deste estudo foi avaliar se alimentação com uréia por curto prazo oferecida a novilhas, e conseqüente aumento de NUP, exerce influência sobre a quantidade, qualidade e competência dos complexos cumulus-oócito (CCO). O experimento teve duração de 62 dias, dividido em oito semanas e dois períodos. Foram utilizadas 40 novilhas mestiças mantidas a pasto, alocadas a dois tratamentos, utilizando-se delineamento \"cross-over\": dieta sem uréia (SU): 5 kg (matéria original) de silagem de milho e 1 kg de concentrado/animal/dia ou dieta com uréia (U): 5 kg de silagem de milho e 1 kg de concentrado contendo 75 g de uréia/animal/dia. Os animais selecionados a cada semana receberam as dietas por seis dias, uma única vez ao dia. No sexto dia de oferecimento das dietas, foram realizadas aspiração folicular (OPU) e colheita de sangue, em jejum e 3 horas após a alimentação. Imediatamente após a OPU, foi realizada contagem total de CCO recuperados e classificação dos mesmos em viáveis e inviáveis. Apenas os viáveis foram destinados à produção In vitro de embriões. Em relação ao teor de NUP, houve efeito de interação entre tratamento e tempo de colheita (P=0,04) e dentro de cada tempo foi observado aumento significativo (P<0,01) para os animais do tratamento U. Não foi observado efeito de tratamento em relação ao número total de CCO recuperados por animal (média ± EPM: SU=9,15 ± 0,82 vs. U=8,82 ± 0,95), nem sobre a porcentagem de CCO viáveis sobre total de CCO recuperados por animal (SU=73,61% ± 2,47 vs. U=70,26% ± 2,31). A taxa de clivagem obtida no dia 3 após a inseminação In vitro (IIV) e as taxas de blastocisto nos dias 6, 7 e 9 após a IIV, não foram influenciadas pelo tratamento. Porém, no 11º pós IIV, houve diminuição (P=0,04) da taxa de blastocistos eclodidos para o tratamento U (SU=82,50% ± 0,05 vs. U=64,33% ± 0,07). Apesar do aumento do teor de NUP observado nas novilhas do tratamento U, a quantidade, qualidade e competência dos CCO durante as primeiras clivagens até atingirem o estádio de blastocisto In vitro não foram influenciadas pelo oferecimento de 75 g de uréia na dieta, durante seis dias. Porém, foi observada redução da taxa de eclosão dos blastocistos das novilhas do tratamento U. / Urea feeding offered to bovine dams may damage their reproductive performance, probably due to an increase in levels of plasmatic urea nitrogen (PUN). The aim of this study was evaluate if short-term urea feeding of heifers, following high PUN levels, would have an influence on the quantity, quality and competence of cumulus-oocyte complexes (COC). Trial lasted 62 days, divided into eight weeks and two periods. Forty crossbred grazing heifers were allocated to one of two treatments, using a cross-over design: diet without urea (WU): 5 kg (as fed) of corn silage and 1 kg of concentrated/animal/day, or diet with urea (U): 5 kg of corn silage and 1 kg of concentrated with 75 g of urea/animal/day. Heifers selected in each week received these diets once a day, for six days. On the sixth day of diets? offer, ovum pick-up (OPU) and blood sampling at fasting and 3 hours after feeding were carried out. Immediately after OPU, total COC recovered was counted and classified as either viable or unviable. Only viable were destined to In vitro embryo production. In relation to PUN level, there was a significant interaction between treatment and sampling time (P=0.04) and a significant (P<0.01) increase in animals undergoing U treatment for each of the test times. No significant effect was observed relative to either the total number of recovered COC per animal (mean ± SEM: WU=9.15 ± 0.82 vs. U=8.82 ± 0.95), or the viable COC as a percentage of total recovered COC per animal (WU=73.61% ± 2.47 vs. U=70.26% ± 2.31). Cleavage ratio assessed on day 3 post In vitro insemination (IVI) and blastocyst ratio on days 6, 7 and 9 post IVI were not influenced by treatments. However, there was a significant treatment effect (P=0.04) in relation to hatched blastocysts on day 11 after IVI (WU=83% ± 0.05 vs. U=64% ± 0.07). Even though higher PUN levels were observed in animals from treatment U, quantity, quality and competence of the COC during first cleavages until reaching the blastocyst stage In vitro were not influenced by adding 75 g of urea on the diet offered to heifers, during six days. Neverthless, a decline in hatched blastocysts rate was observed in heifers of treatment U.

Bovine (female)

Bovinos (fêmeas)

Embrião

Embryo

Oócito

Oocyte

Urea

Uréia

Profiling L-serine Transport Throughout Growth and Meiotic Maturation in Mouse Oocytes

Zhang, Han

27 May 2019

With the increasing demand for assisted reproduction, more knowledge and understanding towards health requirements of oocytes and their inner workings are required. With current IVF success rates of approximately 40%, oocyte and embryo culture conditions in vitro can be improved by first understanding the finer details of oocyte function. As such, there is a need to better understand the mechanisms through which oocytes can acquire certain nutrients. This thesis focuses on the amino acid serine, which has been shown to improve outcome in developing embryos and also plays a variety of roles in the body that may carry over to oocyte health as well. Using radiolabeled [3H] serine, we measured uptake of serine as a function of time throughout growth and meiotic maturation in mouse oocytes. Serine transport appeared in oocytes during growth and became absent in mature eggs. With a competition assay using substrates diagnostic for several different amino acid transporter systems and culture with and without sodium in the external medium, I identified Na+-dependent SNAT7 of the System A/N (SLC38) family to be the most likely transporter in oocytes. Quantitative RT-PCR was consistent with this result. Transporter activity is also not activated by progression of meiotic maturation, as indicated by unperturbed transport when dbcAMP was provided to maintain meiotic arrest. However, a biological regulator of arrest, NPPC, resulted in enhanced transport activity in vitro. This may be due to signalling mechanisms of the NPPC pathway affecting regulation of serine uptake, which presents a direction for future research.

oocyte

NPPC

L-serine

amino acid transport

reproduction

Efeitos do fator de crescimento dos fibroblastos 8 (fgf8) na maturação in vitro de complexos cumulus-oócito bovinos

Sanches, Lorena

January 2016

Orientador: José Buratini Júnior / Resumo: A maturação in vitro (MIV) é uma etapa fundamental da produção in vitro de embriões bovinos (PIV). A conclusão prematura da maturação nuclear durante a MIV é considerada como uma das principais causas da eficiência limitada da PIV. Em camundongos, o fator de crescimento dos fibroblastos 8 (FGF8) regula a atividade do peptÌdeo natriurético tipo C (NPPC) aumentando a expressão de seu receptor (NPR2) e contribuindo assim para o bloqueio meiótico. O principal objetivo deste trabalho foi testar os efeitos do FGF8 sobre a dinâmica da quebra da vesícula germinativa e progresso da meiose durante a MIV induzida com FSH ou ampirregulina (AREG) em bovinos. Paralelamente, os efeitos do FGF8 sobre a expansão do cumulus e metabolismo da glicose também foram testados. Na MIV induzida com AREG, mas não com FSH, o FGF8 diminuiu a porcentagem de oócitos com quebra da vesícula germinativa às 6 e 9 horas do cultivo, enquanto aumentou a expressão do RNAm do NPPC, mas não do NPR2, nas células do cumulus. Distintamente, na MIV com FSH, o FGF8 diminuiu a porcentagem de oócitos em Meiose I às 9 horas de cultivo. O FGF8 não afetou a porcentagem de oócitos em Meiose II às 22 horas da MIV, nem a expansão do cumulus, embora tenha aumentado a expressão do RNAm de genes da cascata ovulatória [prostaglandina endoperoxido sintase 2 (PTGS2) e desintegrina e metaloproteinase de domínio contendo proteÌna 10 (ADAM 10)]. Além disso, o FGF8 diminuiu o consumo de glicose e a produção de lactato na MIV com FSH, m... (Resumo completo, clicar acesso eletrônico abaixo) / Mestre

Complexo cumulus-oócito

FGF8

Bovinos.

Oocyte cumulus complex

Bovine

Estudo em larga escala dos efeitos da idade sobre os parâmetros reprodutivos e viabilidade de oócitos equinos após injeção intracitoplasmática de espermatozóide (ICSI) usando sêmen sexado / Large-scale study of age effects on reproductive parameters and viability of equine oocytes after intracytoplasmatic sperm injection (ICSI) using sexed semen

Araujo, Reno Roldi de

16 June 2015

O objetivo do presente estudo foi comparar o efeito da idade de doadores de oócitos sobre os parâmetros reprodutivos, a taxa de recuperação e qualidade de oócitos após ICSI utilizando sêmen sexado. Éguas Pôneis de Polo (n = 79) e Puro-Sangue (n = 23) doadoras de oócitos (400-600kg e 3-29 anos) foram utilizados durante as estações reprodutivas de 2009/2010 e 2011 no hemisfério Sul (San Luis, Argentina) e norte (Kentucky, EUA), respectivamente. As éguas foram divididas em três categorias experimentais: Jovens (YM: 3-10 anos), Meia Idade (MA: 11-17a) e Idosas (OM&ge;18a). Um total de 326 oócitos recuperados in vivo a partir de folículos pré-ovulatórios (n=279) e folículos imaturos em crescimento (n=47). Desses, 224 oócitos foram recuperados, classificado e dirigido a um programa comercial ICSI com Pôneis de Polo (primeira estação). Durante a segunda estação, 57 oócitos foram recuperados a partir de folículos pré-ovulatórios e 47 oócitos de folículos em crescimento e congelados em nitrogênio líquido para ser usado posteriormente em outro estudo. Os pontos experimentais avaliados foram: intervalos (dias) entre a aspiração ou a ovulação (AS/OV) ao PGF, PGF ao GnRH (Dia 0=GnRH), AS/OV ao Dia 0, e AS/OV ao Dia&#43;1; edema uterino (UE); tonus cervical (CT); diâmetro máximo do folículo dominante (MdF1) em D0 e D&#43;1, e a taxa de crescimento folicular. O número total de aspirações, o número de folículos aspirados e oócitos por aspiração e/ou folículo, o grau de expansão das células do cúmulos, a presença e qualidade do corpo polar (PB), o volume ooplasma, o intervalo de GnRH a aspiração, a GnRH a ICSI, e a taxa de clivagem (CR) depois da ICSI também foram avaliados. Foram observadas diferenças significativas entre as três categorias experimentais (YM, MA e OM) para: intervalos (dias) entre PGF-GnRH, AS/OV-GnRH, AS/OV-Day 1, edema uterino no Dia 0, CT em Dia 1, MdF1 no D0 e D&#43;1 e volume de ooplasma. A taxa de recuperação in vivo (RR) não foi afetada pela idade (média de 102%, 85% e 73,4% de oócitos recuperados por ciclo, por F1 e por folículo, respectivamente, P> 0,05). O CR não diferiu entre as por ciclo, por F1 e por folículo, respectivamente, P> 0,05). O CR não diferiu entre as categorias experimentais. Em conclusão, um efeito de envelhecimento pode ser observado em vários parâmetros reprodutivos em éguas. Os ovócitos no presente estudo tiveram um menor volume de ooplasma para OM comparados com YM, mas isso não foi eficaz em predizer a viabilidade dos oócitos ou o potencial para o desenvolvimento para a avaliação da taxa de clivagem após ICSI utilizando sêmen sexado / The aim of the present study was to compare the effect of oocyte donors` age on reproductive parameters, recovery rate and quality of oocytes after ICSI using sexed semen. Polo Ponies (n=79) and Thoroughbred (n=23) oocyte donor mares (400-600kg and 3-29 years) were used during the 2009/2010 and 2011 reproductive seasons in the Southern (San Luis, Argentina) and in the Northern hemispheres (Kentucky, USA), respectively. Mares were divided into three experimental categories: Young Mares (YM: 3-10&#1059;), Middle Age Mares (MA: 11-17&#1059;) and Old Mares (OM18&#1059;). A total of 326 oocytes were recovered in vivo from pre-ovulatory follicles (n=279) and immature-growing follicles (n=47). From those, 224 oocytes were recovered, sorted and directed to a commercial ICSI program with Polo Ponies (first season). During the study`s second season, 57 oocytes were recovered from pre-ovulatory follicles and 47 oocytes from growing follicles and frozen in liquid nitrogen to be used in another study. The evaluated experimental end-points were: Intervals (days) between aspiration or ovulation (AS/OV) to PGF, PGF to GnRH (Day 0=GnRH), AS/OV to Day 0, and AS/OV to Day &#43; 1; uterine edema (UE); cervical tone (CT); maximum diameter of dominant follicle (MdF1) on D0 and D&#43;1, and follicular growth rate. Total number of aspirations, number of follicles aspirated and oocytes recovered per aspiration and/or follicle, the degree of cumulus cell expansion, the presence and quality of polar body (PB), the ooplasm volume, the interval from GnRH to aspiration, GnRH to ICSI, and the cleavage rate (CR) after ICSI were also evaluated. Significant differences between the three experimental categories (YM, MA and OM) were observed for: intervals (days) between PGF-GnRH, AS/OV-GnRH, AS/OV-Day &#43;1, uterine edema on Day 0, CT on Day &#43;1, MdF1 on D0 and D&#43;1 and ooplasm volume. The in vivo recovery rate (RR) was not affected by age (average of 102%, 85% and 73.4% of oocyte recovered per cycle, per F1 and per follicle, respectively; P>0.05). The CR did not differ among experimental categories. In conclusion, an effect of aging could be observed in several reproductive parameters in mares. The oocytes in the present study had a smaller ooplasm volume for OM compared to YM, but this was not effective in predicting oocyte viability or the potential to development through evaluation of the cleavage rate after ICSI using sexed semen

Aging

Embriões

Embryos

Envelhecimento

miRNA

miRNA

mtDNA

mtDNA

Oócito

Oocyte