Your search keyword '"Lefèvre, Brigitte"' showing total 7 results

1. The nucleolus of the maternal gamete is essential for life.

Author

Lefèvre, Brigitte

Subjects

*NUCLEOLUS, *EMBRYOLOGY, *GAMETES, *MAMMALS, *CELL nuclei

Abstract

The article discusses the findings of the paper "The Maternal Nucleolus Is Essential for Early Embryonic Development in Mammals," by S. Ogushi and colleagues. In this study, researchers found out that the nucleolus of the maternal gamete and other nucleoplasmic elements, which remain undetermined, play a significant role in embryonic development.

Published

2008

2. Tetraspanins and Mouse Oocyte Microvilli Related to Fertilizing Ability.

Author

Benammar, Achraf, Ziyyat, Ahmed, Lefèvre, Brigitte, and Wolf, Jean-Philippe

Subjects

*TETRASPANIN, *OVUM proteins, *MICROVILLI, *ELECTRON microscopy, *METAPHASE (Mitosis)

Abstract

Our electron microscopy observations demonstrate for the first time that the number of microvilli on the mice oocyte membrane decreases when meiosis progresses from prophase I to metaphase II (MII) stage, and the morphology of the microvilli also changes. Microvilli are significantly shorter and larger on the ovulated oocyte membrane than at the previous stages. Although clathrin vesicles clearly disappear during oocyte maturation, exosome-like vesicles begin to be secreted at the metaphase I stage, more strongly at the MII stage. Multivesicular bodies are visible only at the MII stage. Since several oocyte tetraspanins are involved in the gamete interaction, Cd9 being congregated on the MII oocyte microvilli, we analyzed the effect of tetraspanin deletion on oocyte membrane morphology. The Cd9−/− and Cd9−/− Cd81−/− deletions are associated with a decreased microvilli density on the MII oocyte surface. Microvilli thickness is significantly increased whatever the deleted tetraspanin gene be. Only Cd9 deletion clearly disturbs the vesicular traffic, increasing the number of clathrin and exosome vesicles. Additional investigations are necessary to elucidate how tetraspanins modulate the microvilli morphology, likely in relation with cytoskeleton. The role of oocyte exosomes in gamete adhesion/fusion remains to be further studied. [ABSTRACT FROM AUTHOR]

Published

2017

3. Cholesterol Depletion Disorganizes Oocyte Membrane Rafts Altering Mouse Fertilization.

Author

Buschiazzo, Jorgelina, Ialy-Radio, Come, Auer, Jana, Wolf, Jean-Philippe, Serres, Catherine, Lefèvre, Brigitte, and Ziyyat, Ahmed

Subjects

*MICE reproduction, *CHOLESTEROL, *OVUM, *SPERMATOZOA, *FERTILIZATION (Biology), *LIPID rafts, *BIOLOGICAL membranes, *BIOMARKERS

Abstract

: Drastic membrane reorganization occurs when mammalian sperm binds to and fuses with the oocyte membrane. Two oocyte protein families are essential for fertilization, tetraspanins and glycosylphosphatidylinositol-anchored proteins. The firsts are associated to tetraspanin-enriched microdomains and the seconds to lipid rafts. Here we report membrane raft involvement in mouse fertilization assessed by cholesterol modulation using methyl-β-cyclodextrin. Cholesterol removal induced: (1) a decrease of the fertilization rate and index; and (2) a delay in the extrusion of the second polar body. Cholesterol repletion recovered the fertilization ability of cholesterol-depleted oocytes, indicating reversibility of these effects. In vivo time-lapse analyses using fluorescent cholesterol permitted to identify the time-point at which the probe is mainly located at the plasma membrane enabling the estimation of the extent of the cholesterol depletion. We confirmed that the mouse oocyte is rich in rafts according to the presence of the raft marker lipid, ganglioside GM1 on the membrane of living oocytes and we identified the coexistence of two types of microdomains, planar rafts and caveolae-like structures, by terms of two differential rafts markers, flotillin-2 and caveolin-1, respectively. Moreover, this is the first report that shows characteristic caveolae-like invaginations in the mouse oocyte identified by electron microscopy. Raft disruption by cholesterol depletion disturbed the subcellular localization of the signal molecule c-Src and the inhibition of Src kinase proteins prevented second polar body extrusion, consistent with a role of Src-related kinases in fertilization via signaling complexes. Our data highlight the functional importance of intact membrane rafts for mouse fertilization and its dependence on cholesterol. [ABSTRACT FROM AUTHOR]

Published

2013

4. Lamin A/C, Caspase-6, and Chromatin Configuration During Meiosis Resumption in the Mouse Oocyte.

Author

Arnault, Emilie, Doussau, Mireille, Pesty, Arlette, Lefèvre, Brigitte, and Courtot, Anne-Marie

Subjects

*INTERMEDIATE filament proteins, *CYSTEINE proteinases, *CHROMATIN, *MEIOSIS, *OVUM, *GERM cells, *HUMAN reproduction, *APOPTOSIS

Abstract

After in vitro maturation (IVM), isolation of the healthiest oocytes is essential for successful in vitro fertilization. As germinal vesicle (GV) oocytes resume meiosis through healthy or apoptotic pathways without discernable morphological criteria, we checked for an apoptotic element acting at the nucleus level. We hypothesized that caspase-6 with its corresponding substrate, lamin A/C, could be a potential target candidate, because caspase-6 is the only functional caspase for lamin A/C. We used immunohistochemistry methods, Western blots, and a specific caspase-6 inhibitor to determine the presence of lamin A/C and caspase-6 during oogenesis and in isolated oocytes. Our results demonstrated that these proteins were always present and that their distributions were related to oocyte maturity, determined by chromatin configuration and oocyte diameter. Caspase-6 inhibition slowed meiosis resumption suggesting the involvement of caspase-6 in the oocyte apoptotic pathway. Lamin A/C and caspase-6 could be valuable tools in the knowledge of oocyte in vitro destiny. [ABSTRACT FROM AUTHOR]

Published

2010

5. Whole-body or isolated ovary 60Co irradiation: Effects on in vivo and in vitro folliculogenesis and oocyte maturation

Author

Pesty, Arlette, Doussau, Mireille, Lahaye, Jean-Baptiste, and Lefèvre, Brigitte

Subjects

*OVARIAN physiology, *COBALT isotopes, *IRRADIATION, *OVUM, *OVARIAN follicle, *DOSE-response relationship (Radiation), *CHROMATIN, *LABORATORY mice

Abstract

Abstract: For the first time, the effects of low doses of γ-radiation were studied on folliculogenesis and on isolated oocytes. After irradiation of adult mice, even at the lowest dose, a drastic loss of primordial follicles was observed in serial sections of ovaries, with, in opposite, no effect on the other follicle stages. Moreover, oocytes freshly recovered from the largest antral follicles of irradiated adult ovaries exhibited significantly less regular Ca2+ oscillations than controls. Finally, in vitro folliculogenesis demonstrated a smaller diameter of preantral follicles recovered from irradiated juvenile ovaries compared to control, and an increase in follicle atresia. Further on, PLC-β1 localization was not affected in the enclosed oocytes whereas chromatin configuration revealed that a quarter of them had prematurely resumed meiosis or was fragmented. These results raise the question of the risk of genetic and teratogenic effects on women submitted to chronic exposure even of very low radiation. [Copyright &y& Elsevier]

Published

2010

6. The Role of PLCβ1 in the Control of Oocyte Meiosis During Folliculogenesis.

Author

Pesty, Arlette, Broca, Ophélie, Poirot, Catherine, and Lefèvre, Brigitte

Subjects

*PHOSPHOLIPASE C, *OVUM, *MEIOSIS, *NUCLEOLUS, *CHROMATIN

Abstract

The dynamics of the subcellular distribution of PLCβ1 was investigated during meiosis competence acquisition and meiosis resumption in relation to oocyte diameter and to nonsurrounded-nucleolus or surrounded-nucleolus chromatin configurations. Oocytes collected after both in vivo and in vitro folliculogenesis were studied. In both conditions, at the beginning of the process, most oocytes exhibited a nuclear PLCβ1 associated with a nonsurrounded-nucleolus chromatin configuration. Then at the final stage of the process, the factors shifted mainly toward a cytoplasmic PLCβ1 and a surrounded-nucleolus chromatin configuration, typical of a preovulatory fertilizable oocyte. Additionally, only germinal vesicle oocytes with a diameter > 75 µm, and exhibiting cytoplasmic PLCβ1 distribution and surrounded-nucleolus chromatin configuration, resumed meiosis. Our findings demonstrate a strong correlation between oocyte diameter, chromatin configuration, and PLCβ1 localization. Thus, PLCβ1 localization appears to be a key factor determining the progressive acquisition of meiotic competence and final resumption of meiosis. [ABSTRACT FROM AUTHOR]

Published

2008

7. Natural uranium disturbs mouse folliculogenesis in vivo and oocyte meiosis in vitro

Author

Arnault, Émilie, Doussau, Mireille, Pesty, Arlette, Gouget, Barbara, Van der Meeren, Anne, Fouchet, Pierre, and Lefèvre, Brigitte

Subjects

*RODENTS, *URINARY organs, *HISTOPATHOLOGY, *APOPTOSIS

Abstract

Abstract: We investigated whether uranium intoxication affects female fertility by assessing its effects on ovarian function and on the oocyte. We treated two groups of female mice for 15 weeks with 5, 50 or 400mg/L of uranyl nitrate in drinking water. In the first group, mice were euthanized immediately after intoxication. Mice of the second group were paired after intoxication with untreated males. Dams and their female pups were euthanized 3 months after the end of intoxication. We assayed the kidneys, femurs and one ovary per female for U content and collected the other ovary for histology. The number and size of all the ovarian follicles were analyzed. Mice from the first group and female pups had significantly fewer large antral follicles (Ø >200μm) than the untreated mice. By contrast, dams in the second group had more secondary and early preantral follicles (Ø 70–110μm) than untreated mice. However, U had no effect on follicle atresia. We then analyzed the in vitro effects of U on oocyte maturation and fragmentation. GV-oocytes were cultured in the presence of 1mM uranyl acetate and observed for 72h. Oocyte maturation was slowed down by U during resumption of meiosis and at metaphase II. However, the rhythm and rate of oocyte fragmentation were similar to those of control mice. Our findings demonstrate that U induces changes in folliculogenesis and oocyte maturation in mice and could consequently represent a risk for women who are chronically exposed. [Copyright &y& Elsevier]

Published

2008