25 results on '"Geoffroy-Siraudin, C"'
Search Results
2. Morphokinetics analysis of embryos derived from vitrified/warmed oocytes
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Montjean, D., Geoffroy-Siraudin, C., Gervoise-Boyer, M., Tourame, P., and Boyer, P.
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- 2015
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3. Risque reprotoxique masculin dans le secteur du bâtiment et travaux publics
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Bizet, P., Sari-Minodier, I., Metzler-Guillemain, C., Geoffroy-Siraudin, C., Botta, A., and Perrin, J.
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- 2010
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4. Chromosomes sexuels et méiose
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Guichaoua, M.-R., Geoffroy-Siraudin, C., Tassistro, V., Ghalamoun-Slaimi, R., Perrin, J., and Metzler-Guillemain, C.
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- 2009
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5. Les spermatozoïdes macrocéphales. Quels risques pour la fonction de reproduction ?
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Guichaoua, M.-R., Mercier, G., Geoffroy-Siraudin, C., Paulmyer-Lacroix, O., Lanteaume, A., Metzler-Guillemin, C., Perrin, J., and Achard, V.
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- 2009
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6. Normal live birth after vitrified/warmed oocytes intracytoplasmic sperm injection with immotile spermatozoa in a patient with Kartagenerʼs syndrome
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Montjean, D., Courageot, J., Altié, A., Amar-Hoffet, A., Rossin, B., Geoffroy-Siraudin, C., Tourame, P., and Boyer, P.
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- 2015
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7. Aspects génétiques de la tératozoospermie
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Guichaoua, M.-R., Geoffroy-Siraudin, C., Mercier, G., Achard, V., Paulmyer-Lacroix, O., and Metzler-Guillemain, C.
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- 2009
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8. O-078 Predictive factors of autologous Oocyte Post-warming Survival rate
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Montjean, D, primary, Pauly, V, additional, Geoffroy-Siraudin, C, additional, Gervoise-Boyer, M J, additional, and Boyer, P, additional
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- 2021
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9. Meiotic abnormalities in patients bearing complete AZFc deletion of Y chromosome
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Geoffroy-Siraudin, C., Aknin-Seiffer, I., Metzler-Guillemain, C., Ghalamoun-Slaimi, R., Bonzi, M.F., Levy, R., and Guichaoua, M.R.
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- 2007
10. Is it worth it to cryopreserve embryos with blastulation delay at day 5?
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Montjean, D., primary, Pauly, V., additional, Gervoise-Boyer, M., additional, Amar-Hoffet, Aurélie, additional, Geoffroy-Siraudin, C., additional, and Boyer, P, additional
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- 2019
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11. Normal live birth after vitrified/warmed oocytes intracytoplasmic sperm injection with immotile spermatozoa in a patient with Kartagener's syndrome
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Montjean, D., primary, Courageot, J., additional, Altié, A., additional, Amar-Hoffet, A., additional, Rossin, B., additional, Geoffroy-Siraudin, C., additional, Tourame, P., additional, and Boyer, P., additional
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- 2014
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12. La main : embryologie et principaux mécanismes malformatifs
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Perrin, J., primary, Geoffroy-Siraudin, C., additional, and Metzler-Guillemain, C., additional
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- 2008
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13. Artificial intelligence-powered assisted ranking of sibling embryos to increase first cycle pregnancy rate.
- Author
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Dissler N, Nogueira D, Keppi B, Sanguinet P, Ozanon C, Geoffroy-Siraudin C, Pollet-Villard X, and Boussommier-Calleja A
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- Humans, Female, Pregnancy, Adult, Fertilization in Vitro methods, Siblings, Artificial Intelligence, Pregnancy Rate, Embryo Transfer methods
- Abstract
Research Question: Could EMBRYOLY, an artificial intelligence embryo evaluation tool, assist embryologists to increase first cycle pregnancy rate and reduce cycles to pregnancy for patients?, Design: Data from 11,988 embryos were collected via EMBRYOLY from 2666 egg retrievals (2019-2022) across 11 centres in France, Spain and Morocco using three time-lapse systems (TLS). Data from two independent clinics were also examined. EMBRYOLY's transformer-based model was applied to transferred embryos to evaluate ranking performances against pregnancy and birth outcomes. It was applied to cohorts to rank sibling embryos (including non-transferred) according to their likelihood of clinical pregnancy and to compute the agreement with the embryologist's highest ranked embryo. Its effect on time to pregnancy and first cycle pregnancy rate was evaluated on cohorts with multiple single blastocyst transfers, assuming the embryologist would have considered EMBRYOLY's ranking on the embryos favoured for transfer., Results: EMBRYOLY's score correlated significantly with clinical pregnancies and live births for cleavage and blastocyst transfers. This held true for clinical pregnancies from blastocyst transfers in two independent clinics. In cases of multiple single embryo transfers, embryologists achieved a 19.8% first cycle pregnancy rate, which could have been improved to 44.1% with the adjunctive use of EMBRYOLY (McNemar's test: P < 0.001). This could have reduced cycles to clinical pregnancy from 2.01 to 1.66 (Wilcoxon test: P < 0.001)., Conclusions: EMBRYOLY's potential to enhance first cycle pregnancy rates when combined with embryologists' expertise is highlighted. It reduces the number of unsuccessful cycles for patients across TLS and IVF centres., (Copyright © 2024 The Authors. Published by Elsevier Ltd.. All rights reserved.)
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- 2024
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14. Competence of embryos showing transient developmental arrest during in vitro culture.
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Montjean D, Geoffroy-Siraudin C, Gervoise-Boyer MJ, and Boyer P
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- Adult, Blastocyst physiology, Embryo Implantation physiology, Embryo Transfer, Female, Fertilization in Vitro methods, Humans, Pregnancy, Pregnancy Rate, Sperm Injections, Intracytoplasmic methods, Vitrification, Blastocyst cytology, Cell Culture Techniques methods, Cryopreservation, Embryo Implantation genetics
- Abstract
Purpose: In vitro developing embryos may apparently show no developmental progress during 24 h and resume their development up to the blastocyst stage. The present study was conducted to assess their ability to implant and to give rise to a live birth when replaced at day 5 (fresh or vitrified/warmed) as compared to continuously developing embryos., Methods: Embryo development follow-up and grade were prospectively recorded in a photo database. The studied period was from April 2011 to July 2017. The studied embryos included transient arrested embryos (TAE) that showed the same developmental stage at two subsequent observations, i.e. between day 2 and day 3 (d2 and d3), between day 3 and day 4 (d3 and d4) and between day 4 and day 5 (d4 and d5). TAE were compared to continuously developing embryos (CDE). Elective day 5 embryo transfers were performed., Results: Woman age was higher in TAE (34.3±3.9) than in CDE (32.9±4.8) (p<0.01). TAE were more frequently (63.1%) observed after ICSI than after conventional IVF (55.9%) (p<0.01). Implantation rate was reduced in TAE as compared to CDE, after both fresh (10.0% vs 23.8% [p<0.01]) and vitrified/warmed (12.9% vs 19.0% [p<0.01]) embryo transfers. Delivery rate was also lower after the transfer of fresh (8.3% vs 19.4% [p<0.01]) and vitrified/warmed (8.5% vs 14.1% [p<0.01]) TAE as compared to CDE. Implantation and delivery rates were not statistically different whether embryo arrested between day 2 and day 3 (d2 and d3), between day 3 and day 4 (d3 and d4) or between day 4 and day 5 (d4 and d5)., Conclusion: TAE may be considered for transfer at a lower priority than CDE and associated with inferior prognosis than CDE.
- Published
- 2021
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15. No difference in congenital anomalies prevalence irrespective of insemination methods and freezing procedure: cohort study over fourteen years of an ART population in the south of France.
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Beltran Anzola A, Pauly V, Montjean D, Meddeb L, Geoffroy-Siraudin C, Sambuc R, Boyer P, and Gervoise-Boyer MJ
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- Embryo Transfer adverse effects, Embryo Transfer methods, France, Humans, Prevalence, Retrospective Studies, Risk Assessment, Congenital Abnormalities epidemiology, Cryopreservation methods, Reproductive Techniques, Assisted adverse effects
- Abstract
Purpose: A retrospective cohort study was conducted to evaluate and compare the prevalence of congenital anomalies in babies and fetuses conceived after four procedures of assisted reproduction technologies (ART)., Methods: The prevalence of congenital anomalies was compared retrospectively between 2750 babies and fetuses conceived between 2001 and 2014 in vitro fertilization with standard insemination (IVF), IVF with intracytoplasmic sperm injection (ICSI), IVF with frozen embryo transfer (FET-IVF), and ICSI with frozen embryo transfer (FET-ICSI). Congenital anomalies were described according to European Surveillance of Congenital Anomalies (EUROCAT) classification. The parental backgrounds, biologic parameters, obstetric parameters, and perinatal outcomes were compared between babies and fetuses with and without congenital anomalies. Data were analyzed by the generalized estimating equation., Results: Between 2001 and 2014, a total of 2477 evolutionary pregnancies were notified. Among these pregnancies, 2379 were included in the analysis. One hundred thirty-four babies and fetuses had a congenital anomaly (4.9%). The major prevalences found among the recorded anomalies were congenital heart defects, chromosomal anomalies, and urinary defects. However, the risk of congenital anomalies in babies and fetuses conceived after FET was not increased compared with babies and fetuses conceived after fresh embryo transfer, even when adjusted for confounding factors (p = 0.40)., Conclusions: There is no increased risk of congenital anomalies in babies and fetuses conceived by fresh versus frozen embryo transfer after in vitro fertilization with and without micromanipulation. Indeed, distribution of congenital anomalies found in our population is consistent with the high prevalence of congenital heart defects, chromosomal anomalies, and urinary defects that have been found by other authors in children conceived by infertile couples when compared to children conceived spontaneously.
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- 2017
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16. The first 50 live births after autologous oocyte vitrification in France.
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Anzola AB, Pauly V, Geoffroy-Siraudin C, Gervoise-Boyer MJ, Montjean D, and Boyer P
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- Female, France epidemiology, Humans, Pregnancy, Retrospective Studies, Sperm Injections, Intracytoplasmic, Vitrification, Cryopreservation methods, Live Birth, Oocytes
- Abstract
Purpose: The study aims to describe the newborn health parameters of the 50 first children conceived after autologous oocyte vitrification in France., Methods: The 50 children born after autologous oocyte vitrification/warming cycle (VAO children) have been retrospectively compared with 364 children conceived by micromanipulation using freshly recovered non-vitrified oocytes (ICSI children). Children included in the study were born between 2011 and 2015. Maternal characteristics (age, body mass index, smoking habits), obstetric outcomes (diabetes, hypertension, placenta previa, parity, mode of delivery), and perinatal outcome (twinning, sex, birth weight, macrosomia, birth defects) were analyzed. The generalized estimating equation for correlated data was performed to evaluate perinatal outcomes and caesarean section., Results: No statistically significant difference was found between VAO children and ICSI children, even after adjusting confounding factors (low birth weigh odds ratio (OR) 0.8, 95 % confident interval (CI) 0.3-2.2, adjusted (AOR) 0.5, 95 % CI 0.2-1.7; large for gestational age OR 1.5, 95 % CI 0.3-7.0, AOR 1.6, 95 % CI 0.3-7.5; birth defects OR 0.4, 95 % CI 0.1-3.2, AOR 0.5, 95 % CI 0.1-3.7; caesarean section OR 1.8, 95 % CI 0.9-3.4, AOR 1.8, 95 % CI 0.9-3.7)., Conclusions: According to our results, newborn health parameters of children conceived in our center by micromanipulation using vitrified/warmed autologous oocytes seem not to be different from children born after micromanipulation on freshly recovered oocytes.
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- 2015
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17. Ex-vivo assessment of chronic toxicity of low levels of cadmium on testicular meiotic cells.
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Geoffroy-Siraudin C, Perrard MH, Ghalamoun-Slaimi R, Ali S, Chaspoul F, Lanteaume A, Achard V, Gallice P, Durand P, and Guichaoua MR
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- Animals, Cadmium administration & dosage, Cadmium analysis, Dose-Response Relationship, Drug, Flow Cytometry, Male, Rats, Rats, Sprague-Dawley, Sertoli Cells drug effects, Spermatogenesis drug effects, Testis chemistry, Testis cytology, Cadmium toxicity, Meiosis drug effects, Testis drug effects
- Abstract
Using a validated model of culture of rat seminiferous tubules, we assessed the effects of 0.1, 1 and 10 μg/L cadmium (Cd) on spermatogenic cells over a 2-week culture period. With concentrations of 1 and 10 μg/L in the culture medium, the Cd concentration in the cells, determined by ICP-MS, increased with concentration in the medium and the day of culture. Flow cytometric analysis enabled us to evaluate changes in the number of Sertoli cells and germ cells during the culture period. The number of Sertoli cells did not appear to be affected by Cd. By contrast, spermatogonia and meiotic cells were decreased by 1 and 10 μg/L Cd in a time and dose dependent manner. Stage distribution of the meiotic prophase I and qualitative study of the synaptonemal complexes (SC) at the pachytene stage were performed by immunocytochemistry with an anti SCP3 antibody. Cd caused a time-and-dose-dependent increase of total abnormalities, of fragmented SC and of asynapsis from concentration of 0.1 μg/L. Additionally, we observed a new SC abnormality, the "motheaten" SC. This abnormality is frequently associated with asynapsis and SC widening which increased with both the Cd concentration and the duration of exposure. This abnormality suggests that Cd disrupts the structure and function of proteins involved in pairing and/or meiotic recombination. These results show that Cd induces dose-and-time-dependent alterations of the meiotic process of spermatogenesis ex-vivo, and that the lowest metal concentration, which induces an adverse effect, may vary with the cell parameter studied., (Copyright © 2012 Elsevier Inc. All rights reserved.)
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- 2012
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18. Decline of semen quality among 10 932 males consulting for couple infertility over a 20-year period in Marseille, France.
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Geoffroy-Siraudin C, Loundou AD, Romain F, Achard V, Courbière B, Perrard MH, Durand P, and Guichaoua MR
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- Adult, Fertility, France, Humans, Infertility, Male pathology, Linear Models, Male, Spermatozoa physiology, Infertility, Male physiopathology, Semen physiology, Sperm Count trends, Sperm Motility, Spermatozoa cytology
- Abstract
Semen from 10 932 male partners of infertile couples was analysed and sperm parameter trends were evaluated at the Reproduction Biology Laboratory of the University Hospital of Marseille (France) between 1988 and 2007. After 3-6 days of abstinence, semen samples were collected. Measurements of seminal fluid volume, pH, sperm concentration, total sperm count, motility and detailed morphology of spermatozoa were performed. Sperm parameters were analysed on the entire population and in men with normal total numeration (≥40 million per ejaculate). The whole population demonstrated declining trends in sperm concentration (1.5% per year), total sperm count (1.6% per year), total motility (0.4% per year), rapid motility (5.5% per year) and normal morphology (2.2% per year). In the group of selected samples with total normal sperm count, the same trends of sperm quality deterioration with time were observed. Our results clearly indicate that the quality of semen decreased in this population over the study period.
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- 2012
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19. Validation of a rat seminiferous tubule culture model as a suitable system for studying toxicant impact on meiosis effect of hexavalent chromium.
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Geoffroy-Siraudin C, Perrard MH, Chaspoul F, Lanteaume A, Gallice P, Durand P, and Guichaoua MR
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- Animals, Flow Cytometry, Immunohistochemistry, Male, Mass Spectrometry, Rats, Rats, Wistar, Seminiferous Tubules cytology, Chromium toxicity, Meiosis drug effects, Models, Biological, Seminiferous Tubules drug effects
- Abstract
There is evidence that exposure to environmental factors is at least partly responsible for changes in semen quality observed over the past decades. The detection of reproductive toxicants under Registration, Evaluation and Authorisation of Chemicals (REACH) will impact animal use for regulatory safety testing. We first validated a model of culture of rat seminiferous tubules for toxicological studies on spermatogenesis. Then, using this model of culture, we assessed the deleterious effects of 1, 10, and 100 microg/l hexavalent chromium [Cr(VI)] on meiotic cells. The prophase I of meiosis was studied in vivo and ex vivo. Bromo-2'-deoxyuridine (BrdU) was used to describe the kinetics of germ cell differentiation. SCP3 labeling allowed to establish the distribution of the stages of the meiotic prophase I and to perform a qualitative study of the pachytene stage in the absence or presence of Cr(VI). The development of the meiotic step of pubertal rats was similar in vivo and ex vivo. The number of total cells appeared not affected by the presence of Cr(VI) irrespective of its concentration. However, the numbers of late spermatocytes and of round spermatids were decreased by Cr(VI) even at the lower concentration. The percentage of synaptonemal complex abnormalities increased slightly with the time of culture and dramatically with Cr(VI) concentrations. This model of culture appears suitable for toxicological studies. This study shows that Cr(VI) is toxic for meiotic cells even at low concentrations, and its toxicity increases in a dose-dependent manner.
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- 2010
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20. [European regulation REACH and the assessment of testicular toxicity].
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Perrard MH, Grenet C, Prisant N, Geoffroy-Siraudin C, Segretain D, Guichaoua MR, Pointis G, and Durand P
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- Animals, Cryptorchidism epidemiology, Fertility drug effects, Humans, Hypospadias epidemiology, Male, Oligospermia epidemiology, Sperm Count, Spermatogenesis drug effects, Testicular Diseases chemically induced, Testicular Neoplasms epidemiology, Testis embryology, Testis growth & development, Testis physiology, Environmental Pollutants toxicity, Testicular Diseases pathology
- Abstract
Several studies suggest that exposure to environmental pollutants is partly responsible for testicular pathologies that have considerably increased over the last decades (cryptorchidism, hypospadias, cancer, decrease in the number of ejaculated spermatozoa). However, the cellular and molecular mechanisms involved in this reprotoxicity remain mostly unknown. One of the challenges of the european regulation REACH is to improve the knowledge on the chemical, toxic and ecotoxic properties of substances used in everyday life. As for the testicular toxicity, the few in vivo models used are not always the most appropriate for mechanistic studies. Our laboratory has developed and validated on a physiological point of view, coculture systems of germ cells in bicameral chambers, which reproduce a blood-testis barrier, allowing the determination of the mechanisms responsible for the toxicity of organic or mineral compounds on spermatogenesis, while reducing greatly the number of animals required.
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- 2010
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21. [Sex chromosomes and meiosis].
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Guichaoua MR, Geoffroy-Siraudin C, Tassistro V, Ghalamoun-Slaimi R, Perrin J, and Metzler-Guillemain C
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- Chromobox Protein Homolog 5, Chromosomes, Human, X physiology, Chromosomes, Human, Y physiology, Female, Humans, Male, Ovary physiology, Recombination, Genetic, Spermatocytes physiology, Meiosis physiology, Sex Chromosomes physiology
- Abstract
Sex chromosome behaviour fundamentally differs between male and female meiosis. In oocyte, X chromosomes synapse giving a XX bivalent which is not recognizable in their morphology and behaviour from autosomal bivalents. In human male, X and Y chromosomes differ from one another in their morphology and their genetic content, leading to a limited pairing and preventing genetic recombination, excepted in homologous region PAR1. During pachytene stage of the first meiotic prophase, X and Y chromosomes undergo a progressive condensation and form a transcriptionally silenced peripheral XY body. The condensation of the XY bivalent during pachytene stage led us to describe four pachytene substages and to localize the pachytene checkpoint between substages 2 and 3. We also defined the pachytene index (PI=P1+P2/P1+P2+P3+P4) which is always less than 0.50 in normal meiosis. XY body undergoes decondensation at diplotene stage, but transcriptional inactivation of the two sex chromosomes or Meiotic Sex Chromosome Inactivation (MSCI) persists through to the end of spermatogenesis. Sex chromosome inactivation involves several proteins, some of them were now identified. Two isoforms of the HP1 protein, HP1beta and HP1gamma, are involved in the facultative heterochromatinization of the XY body, but the initiation of this process involves the phosphorylation of the protein H2AX by the kinase ATR whose recruitment depends on BRCA1. Extensive researches on the inactivation of the sex chromosomes during male meiosis will allow to a better understanding of some male infertilities.
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- 2009
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22. [Macrocephalic spermatozoa. What would be the impact on reproduction?].
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Guichaoua MR, Mercier G, Geoffroy-Siraudin C, Paulmyer-Lacroix O, Lanteaume A, Metzler-Guillemin C, Perrin J, and Achard V
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- Adult, Female, Humans, Male, Middle Aged, Pregnancy, Pregnancy Rate, Retrospective Studies, Sperm Count, Sperm Injections, Intracytoplasmic, Spermatozoa physiology, Infertility, Male etiology, Reproductive Techniques, Assisted, Sperm Head pathology, Spermatozoa abnormalities
- Abstract
Objective: We want to highlight the risk of infertility and failure of Assisted Reproductive Technologies due to the presence of macrocephalic spermatozoa (MS) in the sperm at rate equalling or superior to 20% in at least one semen analysis., Patients and Methods: We did a retrospective analysis of 19 infertile patients presenting MS at average rate between 14.3 and 49.7%. For each patient, at least one semen analysis showed a MS rate equal or superior to 20%. We did an automated analysis of the spermatozoa surface for 13 patients and a detailed analysis of the MS morphology in 18 patients. Thirteen couples benefited of one or more IVF with or without ICSI., Results: The semen analysis shows an impairment of one or more parameter of the sperm in all patients. Three morphological aspects for MS were highlighted: MS with irregular head, MS with regular head, and MS with multiple heads, with a dominance of irregular heads. The spermatozoa surface analysis shows a significant increase of the average surface and of the standard deviation (p<0.0001). The average rate of pregnancies by transfer is decreased compared to usual rates in our laboratories (13% versus 28%)., Discussion and Conclusion: We want to sensitize biologist and clinical doctors to the existence of partial forms of this syndrome, which could be related to infertility with impaired sperm parameters and low pregnancy rates after FIV or ICSI.
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- 2009
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23. [Genetic aspects of the teratozoospermia].
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Guichaoua MR, Geoffroy-Siraudin C, Mercier G, Achard V, Paulmyer-Lacroix O, and Metzler-Guillemain C
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- Female, Humans, Infertility, Male pathology, Karyotyping, Male, Microscopy, Electron, Transmission, Mutation, Pregnancy, Pregnancy Outcome, Risk Factors, Sperm Injections, Intracytoplasmic adverse effects, Spermatozoa ultrastructure, Chromosome Aberrations, Infertility, Male genetics, Reproductive Techniques, Assisted adverse effects, Spermatozoa abnormalities
- Abstract
Recent mutation identification in well-known sperm defects gives proof that there are genetic causes of infertility. Familial forms and some features of the spermograms lead toward the genetic origin of these syndromes. For each syndrome, several clinical aspects and partial forms were described. In these latter, apparently normal spermatozoa coexist with those showing the phenotype of interest. Transmission electron microscopy is the better tool to characterize the specific details of each syndrome. The frequency of genetic teratozoospermia is weak, the most studied syndromes are the globozoospermia, the macrocephaly, the syndrome of decapitated spermatozoa and the dyplasia of the fibrous sheat. A mutation was identified for two from these syndromes, but the two mutations does not account for all the cases from each syndrome. The various clinical aspects observed for each syndrome suggest that either other mutations or other genes are probably involved in these spermatogenic failures. The use of spermatozoa from patients for intra cytoplasmic sperm injection (ICSI) may pose two problems: fertilization problems and genetic risk for the progeny, including chromosomic and genic risk. Except for total macrocephaly which is excluded from ICSI because of sperm chromosomal abnormalities, these syndromes are consistent with assisted fertilization, but with uncertain rates of fertilization and pregnancy.
- Published
- 2009
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24. Analysis of the intratesticular control of spermatogenesis by ex-vivo approaching.
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Perrard MH, Prisant N, Geoffroy-Siraudin C, Segretain D, Pointis G, Guichaoua MR, and Durand P
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- Animals, Humans, Male, Receptors, Androgen metabolism, Spermatozoa, Spermatogenesis drug effects, Testis metabolism
- Abstract
Spermatogenesis involves the realization of a particular genetic program which requires a specific environment ("niche"). Multiplication, differentiation and apoptosis of male germ cells are finely regulated by pituitary hormones (mainly LH and FSH), and by a complex network of factors originating from both the somatic cells and the germ cells of the testis. It is becoming clear that hormones and intra-testicular regulatory factors can compensate, at least in part, for the absence of some hormones or factors including FSH and LH or androgen receptors. Since, most of the growth factors, cytokines and neurotrophins produced within the testis are widely expressed in the organism, the attempts to understand their role in spermatogenesis by "classical" knock-out strategies have been often disappointing. Therefore an important aspect of our previous work was to settle and characterize carefully two systems of cocultures of testicular germ cells with somatic cells in bicameral chambers. For instance, we showed for the first time that the whole meiotic step could be performed in vitro in a mammalian species (the rat). Moreover, all our data indicate that our co-culture systems enable to highlight mechanisms pertinent to the physiological processes. Sperm parameters have been deteriorated considerably during the past 4-5 decades. There is now evidence that chemical exposure is at least partly responsible for these testicular diseases. If a large number of environmental pollutants are able to affect male fertility and to exert carcinogenic effects, their cellular and molecular mechanisms are still unidentified. The cultures in bicameral chambers that we settled can be used to study the effects of a toxicant when added in the basal compartment of the culture chamber, which appears relevant to the in vivo situation. Taken together our results indicate that our in vitro culture systems, which allow screening for the effect of biological activity of different physiological factors, can be also helpful to study that of any chemicals on both survival and multiplication/differentiation of somatic and/or spermatogenic cells on a relatively long time period.
- Published
- 2009
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25. [The hand: embryology and main malformative mechanisms].
- Author
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Perrin J, Geoffroy-Siraudin C, and Metzler-Guillemain C
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- Gene Expression Regulation, Developmental, Hand Deformities, Congenital genetics, Hedgehog Proteins genetics, Hedgehog Proteins physiology, Homeodomain Proteins genetics, Humans, Infant, Newborn, Intercellular Signaling Peptides and Proteins genetics, Intercellular Signaling Peptides and Proteins physiology, Transcription Factors genetics, Amniotic Band Syndrome diagnosis, Embryonic Development genetics, Fingers abnormalities, Hand embryology, Hand Deformities, Congenital embryology, Limb Buds embryology, Polydactyly embryology, Syndactyly embryology
- Abstract
Upper limb bud appears in the cervical region of the embryo during the fifth week of development. It is made of epithelia and underlying mesenchyme. Diffusible growth factors, expressed by the apical ectodermal ridge, direct the proximal-distal growth. Other factors are expressed by zone of polarizing activity and ectoderm. They induce together anterior-posterior growth and dorsal-ventral polarity of the limb bud. The development of axial skeleton pattern is controlled by transcription factors from the HOX family, which are expressed in a stripe along the proximal and distal edges of the limb bud. Embryologic mechanisms of the main hand malformations are described, as well as their known genetic or mechanical aetiologies.
- Published
- 2008
- Full Text
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