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7. Multiparameter analysis of human oocytes at metaphase II stage after IVF failure in non-male infertility.

Author

P. Cohen-Bacrie, F. Miyara, F-X. Aubriot, P. Debey, A. Glissant, C. Nathan, S. Douard, A. Stanovici, F. Herve, M. Dumont-Hassan, and A.L. Meur

Subjects
*CHROMATIN, *ZYGOTES, *FERTILIZATION in vitro, *FERTILIZATION (Biology)
Abstract

BACKGROUND: Using fluorescence imaging, an a posteriori multiparametric analysis was performed of human oocytes which failed to give pronucleated zygotes after IVF in cases of very low rates of fertilization or complete fertilization failure. METHODS: The analysis included: (i) the state of the maternal and paternal chromatin; (ii) quality of the metaphase II oocytes; and (iii) cortical granule (CG) distribution. RESULTS: Most oocytes were arrested in metaphase II, but they were abnormal in 50% of cases. The incidence of spindle and chromosome aberrations was strongly influenced by maternal age (69% for 40- to 45-year-old women versus 35% for 26- to 33-year-olds), and sperm chromatin was always condensed in immature oocytes, and fully decondensed only in normal metaphase II. The migration of CGs appeared to be associated with achievement of nuclear maturation at the time of puncture. CONCLUSIONS: These factors, when analysed on a complete set of oocytes from the same patient, provided information about potential causes of IVF failure, and also represented part of an 'oocyte quality evaluation' to select the assisted fertilization technique most suitable for each patient. For example, when the majority of oocytes were judged non-fertilizable at a first attempt, no pregnancy was registered at any subsequent attempt. [ABSTRACT FROM AUTHOR]

Published
2003

8. Methylation changes in mature sperm deoxyribonucleic acid from oligozoospermic men: assessment of genetic variants and assisted reproductive technology outcome.

Author

Montjean D, Ravel C, Benkhalifa M, Cohen-Bacrie P, Berthaut I, Bashamboo A, and McElreavey K

Subjects
Case-Control Studies, Chi-Square Distribution, Chromosomes, Human, Y, DNA (Cytosine-5-)-Methyltransferases genetics, DNA Methyltransferase 3A, Female, Gene Frequency, Genetic Predisposition to Disease, Humans, Male, Odds Ratio, Oligospermia diagnosis, Oligospermia physiopathology, Oligospermia therapy, Phenotype, Pregnancy, Pregnancy Rate, Proteins genetics, RNA, Long Noncoding genetics, Risk Factors, Spermatozoa pathology, Treatment Outcome, DNA metabolism, DNA Methylation, Fertility, Genetic Variation, Oligospermia genetics, Reproductive Techniques, Assisted, Spermatozoa metabolism
Abstract

Objective: To characterize a potential genetic cause for methylation errors described in oligozoospermia., Design: Analysis of PEG1/MEST-DMR and H19-DMR methylation level in sperm, in parallel with the study of several genes on the Y chromosome, DNMT3A, and DNMT3L. Clinical outcome was also looked at regarding PEG1/MEST-DMR and H19-DMR methylation level in sperm., Setting: Research and diagnostic laboratories., Patient(s): One hundred nineteen normospermic and 175 oligozoospermic men consulting for couple infertility., Intervention(s): We studied PEG1/MEST-DMR and H19-DMR methylation profiles in 294 men. We searched for Y chromosome gene aberrations and for mutations in both DNMT3A and DNMT3L genes in men showing epimutations. Assisted reproductive technology (ART) outcomes were also investigated., Main Outcome Measure(s): Sperm samples were collected from 294 volunteers for genomic DNA isolation that was used to study methylation profiles in imprinted loci and Y chromosome SMCY, DNMT3A, and DNMT3L genes. Pregnancy rate was also studied after ART treatment using sperm showing epimutations., Result(s): Epimutations in H19-DMR and PEG1/MEST-DMR were found in 20% and 3% of oligozoospermic men, respectively. We identified an amino acid change in DNMT3A in one case and in DNMT3L in eight men with altered methylation profiles. No mutations were detected in SMCY or in selected Y chromsome genes. No correlation between ART outcome and epimutations was found., Conclusion(s): We observed epimethylations in spermatozoa of oligozoospermic individuals, but no association was found with genetic variants or in the ART outcome., (Copyright © 2013 American Society for Reproductive Medicine. Published by Elsevier Inc. All rights reserved.)

Published
2013
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9. Advantages of the two-step embryo transfer strategy in human IVF/ICSI cycles.

Author

Yazbeck C, Ben Jamaa N, Hazout A, Cohen-Bacrie P, Junca AM, and Rougier N

Subjects
Adult, Blastocyst physiology, Cryopreservation, Female, Humans, Live Birth epidemiology, Ovulation Induction, Pregnancy, Pregnancy Rate, Pregnancy, Multiple, Sperm Injections, Intracytoplasmic, Embryo Transfer methods, Fertilization in Vitro methods
Abstract

The aim of this study was to evaluate the advantages of the two-step embryo transfer (ET) strategy combining a day 2/3 ET with a day 5/6 blastocyst transfer. In an observational comparative study, 400 infertile women were enrolled from two assisted reproductive technology (ART) units according to inclusion criteria: age below 42 years and at least three embryos obtained on day 2 thus allowing an extended in vitro culture. Two groups were defined according to the ET strategy adopted: group 1 had a two-step ET; and group 2 had a day 2/3 ET with (subgroup 2a) or without (subgroup 2b) blastocysts cryopreserved on day 5/6. Live birth rate was significantly higher in group 1 than in subgroups 2a and 2b (36.5% versus 29.4% and 13.4%, respectively; p < 10(-3)). Multiple pregnancy rates were comparable between groups. After adjusting on major prognostic factors, the two-step ET strategy was still associated with a significantly higher live birth rate than the day 2/3 ET (OR = 2.23; 95% CI: 1.32-3.77). The two-step ET provides better live birth rates than the cleavage-stage ET. It does not increase multiple pregnancy rates if the number of embryos transferred is limited. It also prevents cycle loss when embryos fail to develop into blastocysts.

Published
2013
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10. Blood type and ovarian reserve.

Author

de Mouzon J, Hazout A, Cohen-Bacrie M, Belloc S, and Cohen-Bacrie P

Subjects
Female, Humans, ABO Blood-Group System, Blood Grouping and Crossmatching, Ovary physiology
Published
2012
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11. Polymorphisms in MTHFR and MTRR genes associated with blood plasma homocysteine concentration and sperm counts.

Author

Montjean D, Benkhalifa M, Dessolle L, Cohen-Bacrie P, Belloc S, Siffroi JP, Ravel C, Bashamboo A, and McElreavey K

Subjects
Adult, Cohort Studies, Female, Gene Frequency, Genetic Predisposition to Disease, Homocysteine analysis, Humans, Infertility, Male blood, Infertility, Male physiopathology, Male, Osmolar Concentration, Semen Analysis, Ferredoxin-NADP Reductase genetics, Homocysteine blood, Infertility, Male genetics, Methylenetetrahydrofolate Reductase (NADPH2) genetics, Polymorphism, Single Nucleotide physiology, Sperm Count
Abstract

Objective: To investigate the relationship between MTHFR and MTRR genetic variants with respect to both blood plasma homocysteine concentration and sperm counts., Design: Polymerase chain reaction followed by specific enzymatic digestion to determine the genotype of the individuals and blood plasma homocysteine quantification by high-performance liquid chromatography., Setting: Research laboratory., Patient(s): Two hundred sixty-eight men seeking infertility counseling and 254 partners of infertile women., Intervention(s): We studied three MTHFR (c.1286A → C, c.665C → T and c.203G → A) and two MTRR (c.66A → G and c.524C → T) single-nucleotide polymorphisms and characterized sperm parameters in both oligozoospermic and normospermic men. A cohort of 522 men was examined for this study. A subgroup of 103 men was constituted for quantification of Hcy levels., Main Outcome Measure(s): Semen samples were collected for determinations of sperm concentration, motility, and morphology according to World Health Organization guidelines as well as for DNA isolation. Blood samples of the corresponding individuals were obtained to quantify plasma homocysteine levels., Result(s): We did not observe a relationship between homocysteinemia and sperm counts. The MTHFR c.665C → T variant is associated with mild hyperhomocysteinemia in blood plasma in the TT homozygous state., Conclusion(s): No association was found between MTHFR/MTRR genetic variants and sperm counts. Although no association was observed with reduced sperm counts, the MTHFR 665TT genotype is associated with a significant increase in blood plasma homocysteine levels., (Copyright © 2011 American Society for Reproductive Medicine. Published by Elsevier Inc. All rights reserved.)

Published
2011
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12. Malonaldehyde formation and DNA fragmentation: two independent sperm decays linked to reactive oxygen species.

Author

Montjean D, Ménézo Y, Benkhalifa M, Cohen M, Belloc S, Cohen-Bacrie P, and de Mouzon J

Subjects
Humans, Lipid Peroxidation, Male, Membrane Lipids metabolism, Phospholipid Hydroperoxide Glutathione Peroxidase, Sperm Motility, DNA Fragmentation, Glutathione Peroxidase metabolism, Malondialdehyde metabolism, Reactive Oxygen Species metabolism, Spermatozoa metabolism
Abstract

Malondialdehyde (MDA), a product involved in membrane lipid peroxidation, was dosed in the sperm of 163 patients who had consulted the clinic regarding hypofertility. We attempted to determine if there was correlation between MDA content, sperm World Health Organization parameters and DNA fragmentation that results mainly from reactive oxygen species assaults. We found that no correlation could be established; however MDA and sperm decondensation were shown to be significantly linked. The impact of membrane polyunsaturated fatty acids and the role of phospholipid hydroperoxide glutathione peroxidase are discussed.

Published
2010
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13. Imprinting: RNA expression for homocysteine recycling in the human oocyte.

Author

Benkhalifa M, Montjean D, Cohen-Bacrie P, and Ménézo Y

Subjects
5-Methyltetrahydrofolate-Homocysteine S-Methyltransferase genetics, Adenosine analogs & derivatives, Adenosine metabolism, Betaine-Homocysteine S-Methyltransferase genetics, Blastocyst enzymology, Cystathionine beta-Synthase genetics, DNA Methylation, Ethionine analogs & derivatives, Ethionine metabolism, Female, Fertilization in Vitro, France, Humans, Oligonucleotide Array Sequence Analysis, Reverse Transcriptase Polymerase Chain Reaction, Gene Expression Regulation, Developmental, Gene Expression Regulation, Enzymologic, Genomic Imprinting, Homocysteine metabolism, Methionine metabolism, Oocytes enzymology, RNA, Messenger metabolism
Abstract

Objective: To investigate whether homocysteine, a well known inhibitor of methylation, which is produced after imprinting and other methylation processes, can be recycled to methionine in the oocyte, at least until the stage of maternal to zygotic transition (i.e., four- to eight-cell stage); before this stage, most of the biochemical processes are carried out with the use of maternal stores of protein and mRNA., Design: A first approach using microarrays and then reverse-transcription polymerase chain reaction (RT-PCR) for methionine synthase (5-methyltetrahydrofolate-homocysteine methyltransferase [MTR]), betaine-homocysteine methyltransferase (BHMT), and cystathionine-beta synthase (CBS)., Setting: Two private hospitals., Patient(s): Patients involved in IVF/ICSI procedures., Intervention(s): Germinal vesicle oocytes collected at the time of oocyte retrieval, RNA extraction amplification, RT-PCR, microarrays., Main Outcome Measure(s): mRNA expression of all the enzymes involved in the chain of methylation and recycling of homocysteine to methionine., Result(s): All of the enzymes required for methylation are present in the oocyte. Homocysteine can be recycled with BHMT and MTR., Conclusion(s): The human oocyte is able to regulate its Hcy level via remethylation using MTR and BHMT but not CBS. This aspect is important, because recent studies have shown that controlled ovarian hyperstimulation affects the homocysteine concentration in follicular fluid. This may regulate, at least in part, the risk of imprinting problems during IVF procedures., (Copyright 2010 American Society for Reproductive Medicine. Published by Elsevier Inc. All rights reserved.)

Published
2010
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14. Effect of growth hormone on oocyte competence in patients with multiple IVF failures.

Author

Hazout A, Junca Am, Ménézo Y, Demouzon J, and Cohen-Bacrie P

Subjects
Analysis of Variance, Chorionic Gonadotropin, Female, Gonadotropin-Releasing Hormone analogs & derivatives, Humans, Models, Biological, Pregnancy, Treatment Outcome, Fertilization in Vitro methods, Growth Hormone pharmacology, Oocytes drug effects
Abstract

In a preliminary, unpublished randomized study conducted in 2000 on 39 patients, including a placebo group, it was observed that the addition of growth hormone (GH) during ovarian stimulation in patients with poor-quality oocytes increased the pregnancy rate. However, the results were not statistically significant due to the small number of patients in each group. A protocol with 8 IU GH was tested in 291 patients with three or more previous failures of embryo transfer for no clearly identifiable reasons. The analysis was restricted to patients receiving either recombinant FSH or human menopausal gonadotrophin (HMG) (n = 245). They were compared retrospectively to all patients with three or more failures during the same period of time but stimulated only with recombinant FSH or HMG, without GH, in an observational study design. Co-stimulation with GH gave better results in terms of number of oocytes collected and embryos obtained. Pregnancy rate per retrieval was higher than in the control group (25.7% versus 18.2%, P < 0.01) and reached a level similar to the one observed in the study centre for the whole population. Ovarian stimulation associated with GH can be proposed for patients with a history of repeated assisted reproduction failures. An improvement of cytoplasmic competence is proposed as an explanation.

Published
2009
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15. Correlation between DNA damage and sperm parameters: a prospective study of 1,633 patients.

Author

Cohen-Bacrie P, Belloc S, Ménézo YJ, Clement P, Hamidi J, and Benkhalifa M

Subjects
Adult, DNA Fragmentation, Humans, In Situ Nick-End Labeling, Male, Prospective Studies, Sperm Injections, Intracytoplasmic, DNA Damage, Sperm Motility, Spermatozoa pathology
Abstract

Objective: To investigate DNA fragmentation by using terminal deoxyribonucleotidyl transferase-mediated dUTP nick-end labeling in relation to World Health Organization parameters and computer-aided sperm analysis (CASA) in sperm to determine the possibility of obtaining a correlation among CASA parameters, sperm morphology, and DNA fragmentation., Design: Sperm analysis according to World Health Organization parameters, terminal deoxyribonucleotidyl transferase-mediated dUTP nick-end labeling (TUNEL) for sperm DNA fragmentation, and CASA for sperm movement. Prospective study., Setting: All the patients were under clinical management, consulting for hypofertility at a fertility center in France., Patient(s): One thousand six hundred thirty-three men who were referred for infertility investigation, including a complete sperm analysis., Intervention(s): Sperm analysis and DNA damage testing., Main Outcome Measure(s): Sperm morphology, DNA fragmentation, and movement characteristics., Result(s): One third of the patients had a TUNEL rate of >30%. Analysis of the 21 semen parameters tested revealed that 7 of them were significantly correlated with the TUNEL results., Conclusion(s): World Health Organization sperm parameters and DNA damage are complementary, rather than strongly linked. This should be considered to more fully understand the paternal contribution in assisted reproductive technologies failures.

Published
2009
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16. Effect of maternal and paternal age on pregnancy and miscarriage rates after intrauterine insemination.

Author

Belloc S, Cohen-Bacrie P, Benkhalifa M, Cohen-Bacrie M, De Mouzon J, Hazout A, and Ménézo Y

Subjects
Abortion, Spontaneous epidemiology, Adult, Female, Humans, Male, Middle Aged, Multivariate Analysis, Pregnancy, Prognosis, Retrospective Studies, Sperm Motility, Abortion, Spontaneous etiology, Insemination, Artificial, Maternal Age, Paternal Age, Pregnancy Rate
Abstract

More than 17,000 intrauterine insemination (lUI) cycles were analysed retrospectively with respect to outcome according to differing aetiologies of infertility. The quantity and motility of spermatozoa in the final preparation used for insemination had a positive effect on the outcome, as classically observed in the past. It was found that advanced maternal age had a negative effect on the pregnancy rate and was associated with increased miscarriage rate. More interestingly, an exactly parallel effect was found for paternal age. The impact of increased age on necrospermia and sperm DNA structure is discussed as a probable direct cause of this paternal effect.

Published
2008
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17. Adequate ovarian follicular status does not prevent the decrease in pregnancy rates associated with high sperm DNA fragmentation.

Author

Frydman N, Prisant N, Hesters L, Frydman R, Tachdjian G, Cohen-Bacrie P, and Fanchin R

Subjects
Adult, Embryo Transfer, Female, Flow Cytometry, Humans, In Situ Nick-End Labeling, Infertility, Female genetics, Infertility, Female metabolism, Infertility, Female pathology, Infertility, Female physiopathology, Male, Ovulation Induction, Pregnancy, Pregnancy Rate, Prospective Studies, Spermatozoa metabolism, Treatment Outcome, DNA Fragmentation, DNA Repair, Embryo Implantation, Fertilization in Vitro, Infertility, Female therapy, Ovarian Follicle metabolism, Sperm-Ovum Interactions, Spermatozoa pathology
Abstract

Objective: Potential reparation of sperm DNA fragmentation in the oocyte may disturb any relationship between DNA-damaged sperm and the implantation ability of resulting embryos. To rule out this factor, we analyzed the consequences of sperm DNA fragmentation on IVF-ET outcome in women with healthy ovarian function., Design: Prospective study., Setting: Teaching hospital, France., Patient(s): All 117 women were <38 years old, who combined normal serum day-3 FSH and inhibin B levels with an adequate response to controlled ovarian hyperstimulation., Intervention(s): The DNA fragmentation rate was determined in the raw sperm used for conventional IVF by flow cytometric terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling assay. Cycles were sorted into two groups according to whether DNA fragmentation exceeded (high fragmentation [HF], n = 52) or did not exceed (low fragmentation [LF], n = 65) the 50th percentile of values (35%)., Main Outcome Measure(s): D2 embryo quality and implantation and ongoing pregnancy rates., Result(s): Patients' characteristics, raw semen parameters, fertilization rates, and embryology data were similar in HF and LF groups. Clinical (37.5% vs. 62.5%) and ongoing (23.5% vs. 57.8%) pregnancy rates per ET and implantation rates (24.5% vs. 42.4%) were lower in the HF group than in the LF group., Conclusion(s): High sperm DNA fragmentation spares fertilization and top embryo morphology rates but is associated with decreased IVF-ET outcome.

Published
2008
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18. Antioxidants to reduce sperm DNA fragmentation: an unexpected adverse effect.

Author

Ménézo YJ, Hazout A, Panteix G, Robert F, Rollet J, Cohen-Bacrie P, Chapuis F, Clément P, and Benkhalifa M

Subjects
Adjuvants, Immunologic pharmacology, Administration, Oral, Antioxidants administration & dosage, Ascorbic Acid administration & dosage, Disulfides chemistry, Fertilization in Vitro methods, Guanosine analogs & derivatives, Guanosine metabolism, Humans, Male, Oxidative Stress, Reactive Oxygen Species, Sperm Injections, Intracytoplasmic methods, Antioxidants metabolism, DNA Fragmentation drug effects, Infertility, Male therapy, Spermatozoa drug effects, Spermatozoa metabolism
Abstract

Reactive oxygen species (ROS) have a negative impact on sperm DNA, leading to the formation of oxidative products such as 8-oxo-7,8-dihydroxyguanosine. This compound causes fragmentation and, thus, has a mutagenic effect. Patient treatment with oral antioxidant vitamins is, therefore, standard practice for male infertility, in an attempt to decrease formation of ROS and improve fertility. In this study, the DNA fragmentation index and the degree of sperm decondensation were measured using the sperm chromatin structure assay before and after 90 days treatment with antioxidant vitamins associated with zinc and selenium. Antioxidant treatment led to a decrease in sperm DNA fragmentation (-19.1%, P < 0.0004), suggesting that at least part of the decay was linked to ROS. However, it also led to an unexpected negative effect: an increase in sperm decondensation with the same order of magnitude (+22.8%, P < 0.0009). The opening of interchain disulphide bridges in protamines may explain this aspect, as antioxidant vitamins, especially vitamin C, are able to open the cystin net, thus interfering with paternal gene activity during preimplantation development. This observation might explain the discrepancy observed concerning the role of these antioxidant treatments in improving male fertility.

Published
2007
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19. High-magnification ICSI overcomes paternal effect resistant to conventional ICSI.

Author

Hazout A, Dumont-Hassan M, Junca AM, Cohen Bacrie P, and Tesarik J

Subjects
Adult, DNA Fragmentation physiology, Female, Humans, In Situ Nick-End Labeling, Male, Oocytes cytology, Ovulation Induction methods, Pregnancy, Pregnancy Outcome, Treatment Outcome, Infertility therapy, Microscopy, Interference, Sperm Injections, Intracytoplasmic methods, Spermatozoa cytology
Abstract

Previous studies have shown that repeated intracytoplasmic sperm injection (ICSI) failures can be caused by a paternal effect. Other studies have suggested that ICSI results are compromised if morphologically abnormal spermatozoa are injected into oocytes. This study was undertaken to evaluate the usefulness of a high-magnification optical system to select spermatozoa to be used for ICSI (high-magnification ICSI) in couples with repeated conventional ICSI failures. Couples with two or more previous conventional ICSI failures underwent an additional conventional ICSI attempt, followed by a high-magnification ICSI attempt. The outcomes of the two sequential attempts were compared. In 72 of these patients, sperm DNA integrity was assessed. In the whole group of 125 couples with repeated ICSI failures, high-magnification ICSI improved clinical outcomes (pregnancy, implantation, delivery and birth rates) without affecting biological outcomes (fertilization and cleavage rates, embryo morphology). The improvement of clinical ICSI outcomes was evident both in patients with an elevated degree of sperm DNA fragmentation and in those with normal sperm DNA status. It is concluded that high-magnification ICSI improves clinical outcomes in couples with previous repeated conventional ICSI failures.

Published
2006
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20. Serum antimüllerian hormone/müllerian-inhibiting substance appears to be a more discriminatory marker of assisted reproductive technology outcome than follicle-stimulating hormone, inhibin B, or estradiol.

Author

Hazout A, Bouchard P, Seifer DB, Aussage P, Junca AM, and Cohen-Bacrie P

Subjects
Adult, Anti-Mullerian Hormone, Biomarkers blood, Female, Humans, Multivariate Analysis, Osmolar Concentration, Predictive Value of Tests, Pregnancy, Pregnancy Rate, Retrospective Studies, Time Factors, Treatment Outcome, Estradiol blood, Fertilization in Vitro, Follicle Stimulating Hormone blood, Glycoproteins blood, Inhibins blood, Ovulation Induction, Testicular Hormones blood
Abstract

Objective: To test the hypothesis that the concentration of early follicular phase serum antimullerian hormone (AMH) or mullerian-inhibiting substance (MIS) is a useful marker of ovarian response and assisted reproductive technology (ART) outcome., Design: Retrospective analysis of day 3 serum samples drawn before treatment., Setting: Private ART program., Patient(s): One hundred nine consecutive serum samples from women younger than 42 years of age who were undergoing ovulation induction for IVF., Intervention(s): Follicular aspiration for IVF after ovarian stimulation with FSH in a down-regulated cycle using GnRH-a treatment., Main Outcome Measure(s): Correlations between day 3 serum AMH/MIS, E2, FSH, inhibin B levels, and IVF outcome (i.e., number of retrieved mature oocytes, number and quality of embryos obtained, ongoing clinical pregnancy rates). Multivariate regression analysis on categorical data was performed to describe a predictive model of clinical pregnancy outcome., Result(s): Mean serum AMH/MIS value for clinical pregnancy (n = 38) was 2.4 ng/mL, in comparison to 1.1 ng/mL for those who did not become pregnant (n = 71). No differences were noted in mean values for day 3 FSH, inhibin B, or E2 between groups. Multivariate regression analysis demonstrated that day 3 serum AMH/MIS had the greatest independent contribution in predicting pregnancy outcomes., Conclusion(s): These data demonstrate a strong association between day 3 serum AMH/MIS level and IVF outcome in women younger than 42 years of age. Higher AMH/MIS concentrations are associated with a greater number of mature oocytes, a greater number of embryos, and ultimately a higher clinical pregnancy rate. Furthermore, AMH/MIS may offer greater prognostic value than other currently available serum markers of ART outcome.

Published
2004
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21. Multiparameter analysis of human oocytes at metaphase II stage after IVF failure in non-male infertility.

Author

Miyara F, Aubriot FX, Glissant A, Nathan C, Douard S, Stanovici A, Herve F, Dumont-Hassan M, LeMeur A, Cohen-Bacrie P, and Debey P

Subjects
Age Distribution, Chromatin pathology, Female, Humans, Incidence, Infertility, Female epidemiology, Infertility, Female genetics, Male, Metaphase, Microtubules, Pregnancy, Sperm-Ovum Interactions, Spermatozoa, Treatment Failure, Chromosome Aberrations, Fertilization in Vitro, Infertility, Female pathology, Oocytes pathology
Abstract

Background: Using fluorescence imaging, an a posteriori multiparametric analysis was performed of human oocytes which failed to give pronucleated zygotes after IVF in cases of very low rates of fertilization or complete fertilization failure., Methods: The analysis included: (i) the state of the maternal and paternal chromatin; (ii) quality of the metaphase II oocytes; and (iii) cortical granule (CG) distribution., Results: Most oocytes were arrested in metaphase II, but they were abnormal in 50% of cases. The incidence of spindle and chromosome aberrations was strongly influenced by maternal age (69% for 40- to 45-year-old women versus 35% for 26- to 33-year-olds), and sperm chromatin was always condensed in immature oocytes, and fully decondensed only in normal metaphase II. The migration of CGs appeared to be associated with achievement of nuclear maturation at the time of puncture., Conclusions: These factors, when analysed on a complete set of oocytes from the same patient, provided information about potential causes of IVF failure, and also represented part of an 'oocyte quality evaluation' to select the assisted fertilization technique most suitable for each patient. For example, when the majority of oocytes were judged non-fertilizable at a first attempt, no pregnancy was registered at any subsequent attempt.

Published
2003
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22. Chromatin configuration and transcriptional control in human and mouse oocytes.

Author

Miyara F, Migne C, Dumont-Hassan M, Le Meur A, Cohen-Bacrie P, Aubriot FX, Glissant A, Nathan C, Douard S, Stanovici A, and Debey P

Subjects
Animals, Blotting, Western, Humans, Mice, Phosphorylation, Phosphotransferases antagonists & inhibitors, RNA Polymerase II metabolism, Zygote metabolism, Chromatin physiology, Gene Expression Regulation physiology, Oocytes physiology, Transcription, Genetic physiology
Abstract

In vitro maturation of human oocytes at the germinal vesicle (GV) stage could offer an alternative in several cases of female infertility. It however rests on a better knowledge of the quality of human oocyte. Using fluorescence imaging of DNA and of the transcription sites, combined with electron microscopy, we show that human oocytes follow size-dependent changes in chromatin configuration, transcription sites distribution and nuclear ultrastructure that follow those observed in mouse GV oocytes. We thus analyzed in mouse GV oocytes the phosphorylation dependence of the transcriptional activity. We show by Western blot that, while active GV oocytes have approximately the same proportion of hypo- and hyperphosphorylated forms of the RNA polymerase II (RNAP II), the hyperphosphorylated form is almost absent from inactive oocytes. We also show that (1) RNAP II-dependent transcription is much less sensitive to various kinase inhibitors in mouse oocytes than in somatic cells or mouse one-cell embryos, although the phosphorylation equilibrium of RNAP II was largely shifted towards the hypo-phosphorylated form upon treatment with these inhibitors (2) RNAP I is completely insensitive to kinase inhibitors in GV oocytes., (Copyright 2003 Wiley-Liss, Inc.)

Published
2003
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23. Embryos with high implantation potential after intracytoplasmic sperm injection can be recognized by a simple, non-invasive examination of pronuclear morphology.

Author

Tesarik J, Junca AM, Hazout A, Aubriot FX, Nathan C, Cohen-Bacrie P, and Dumont-Hassan M

Subjects
Cleavage Stage, Ovum, Embryo Transfer, Female, Humans, Pregnancy, Pregnancy Rate, Pregnancy, Multiple, Cell Nucleus ultrastructure, Embryo Implantation, Embryo, Mammalian physiology, Embryo, Mammalian ultrastructure, Sperm Injections, Intracytoplasmic, Zygote ultrastructure
Abstract

Embryos are conventionally selected for transfer based on the evaluation of the cleavage speed and extent of blastomere fragmentation. Here we examined whether the predictive value of these criteria, as indicators of the chance of embryo implantation, can be further potentiated by adding previously described criteria reflecting the regularity of pronuclear development. In a group of embryos selected for transfer in 380 fresh embryo transfer cycles according to the conventional criteria, the transfer of only those embryos that developed from zygotes judged normal at the pronuclear stage (pattern 0) gave significantly higher pregnancy (44.8%) and implantation (30.2%) rates compared with the pregnancy (22.1%; P < 0. 05) and implantation rates (11.2%; P < 0.001) for the transfers of only those embryos that developed from zygotes judged abnormal (non-pattern 0). The transfer of only one pattern 0 embryo was sufficient for the optimal chance of pregnancy (no differences in pregnancy rates after transfer of one, two or three pattern 0 embryos), whereas the transfer of two pattern 0 embryos mostly resulted in a twin pregnancy. The inclusion of the criteria based on pronuclear morphology can thus lead to the application of a single embryo transfer policy and optimize the selection of embryos for transfer and cryopreservation.

Published
2000
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24. Differentiation of spermatogenic cells during in-vitro culture of testicular biopsy samples from patients with obstructive azoospermia: effect of recombinant follicle stimulating hormone.

Author

Tesarik J, Greco E, Rienzi L, Ubaldi F, Guido M, Cohen-Bacrie P, and Mendoza C

Subjects
Acrosome drug effects, Acrosome pathology, Biopsy, Cell Differentiation drug effects, Cytoplasm drug effects, Cytoplasm pathology, Humans, In Vitro Techniques, Male, Recombinant Proteins pharmacology, Reproductive Techniques, Spermatocytes drug effects, Spermatocytes pathology, Testis pathology, Follicle Stimulating Hormone pharmacology, Oligospermia pathology, Oligospermia therapy, Spermatids drug effects, Spermatids pathology, Spermatogenesis drug effects
Abstract

In-vitro differentiation of spermatogenic cells is a potential approach to the treatment of male sterility due to spermatogenic arrest. This is a pilot study evaluating meiotic, morphogenetic and cytoplasmic maturation of spermatogenic cells from 18 patients with obstructive azoospermia, during in-vitro culture of partly disintegrated testicular biopsy samples in the presence or absence of recombinant follicle stimulating hormone (rFSH). Meiotic progression was detectable only in the presence of rFSH in culture medium. FSH-dependent condensation, peripheral migration and protrusion of spermatid nuclei, together with FSH-independent flagellar growth, were the main events indicating post-meiotic sperm cell differentiation. rFSH also promoted the progression of spermatid cytoplasmic maturation, reflected by acceleration of acrosomal development. These differentiation events appeared to be mediated by humoral activity of Sertoli cells, without the need for a direct Sertoli-sperm cell contact. These findings provide a background for similar studies in patients with non-obstructive azoospermia. If reproducible in the latter group, transmeiotic in-vitro differentiation of primary spermatocytes may be useful in cases of complete maturation arrest, whereas the development of culture-specific forms may help select viable spermatids in cases of complete spermiogenesis failure.

Published
1998
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25. Germ cell apoptosis in men with complete and incomplete spermiogenesis failure.

Author

Tesarik J, Greco E, Cohen-Bacrie P, and Mendoza C

Subjects
Annexin A5 analysis, Annexin A5 metabolism, DNA Fragmentation, Humans, Male, Oligospermia, Phosphatidylserines analysis, Phosphatidylserines metabolism, Spermatids cytology, Apoptosis, Infertility, Male pathology, Spermatogenesis, Spermatozoa pathology
Abstract

Germ cell apoptosis was evaluated in 11 men suffering from nonobstructive azoospermia and enrolled in a spermatid conception programme. In six of these patients, round spermatids (Sa stage) were the most advanced spermatogenic cells recovered from testicular biopsy samples. This condition is referred to as complete spermiogenesis failure. In the remaining five men, a few late elongated spermatids (Sd stage) were unexpectedly found in the testicular biopsy samples on the day of treatment. This condition is referred to as incomplete spermiogenesis failure. Germ cell apoptosis in both groups of patients was examined by analysing cell smears prepared from mechanically disintegrated testicular tissues using terminal deoxyribonucleotidyl transferase-mediated dUTP nick-end labelling (TUNEL), which detects apoptosis-specific DNA fragmentation, and annexin-V binding, detecting apoptosis-related translocation of plasma membrane phosphatidylserine to the membrane's outer surface. Both methods were combined, in double-fluorescence labelling preparations, with immunocytochemical detection of proacrosin, a specific germline marker. Patients with complete spermiogenesis failure had significantly higher frequencies of primary spermatocytes and round spermatids carrying the apoptosis-specific DNA damage in comparison with patients with incomplete spermiogenesis failure. Surprisingly, apoptosis-related phosphatidylserine externalization occurs rarely until the advanced stages of spermiogenesis. Since externalized phosphatidylserine is expected to be involved in the recognition of apoptotic cells by phagocytes, apoptotic spermatocytes and round spermatids may not be removed easily by phagocytosis. The high frequency of DNA damage in round spermatids from patients with complete spermiogenesis failure explains the low success rates of spermatid conception in these cases. The evaluation of apoptosis can help predict success rates of spermatid conception.

Published
1998
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26. Combined use of proacrosin immunocytochemistry and autosomal DNA in situ hybridisation for evaluation of human ejaculated germ cells.

Author

Mendoza C, Benkhalifa M, Cohen-Bacrie P, Hazout A, Ménézo Y, and Tesarik J

Subjects
Acrosome physiology, Acrosome ultrastructure, Antibodies, Monoclonal, Cell Nucleus physiology, Chromosomes, Human, Pair 15, Chromosomes, Human, Pair 16, DNA Probes, Ejaculation physiology, Humans, Male, Meiosis, Oligospermia, Spermatids physiology, Spermatozoa immunology, Acrosin immunology, Enzyme Precursors immunology, Immunohistochemistry methods, In Situ Hybridization, Fluorescence methods, Spermatozoa physiology
Abstract

The recently reported human pregnancies and births after fertilising oocytes with round spermatids recovered from the ejaculate of men with non-obstructive azoospermia have underscored the need for a more accurate evaluation of the nuclear and cytoplasmic maturation status of ejaculated germ cells. In this study we describe our first experience with a method combining the immunocytochemical visualisation of proacrosin with autosomal DNA fluorescence in situ hybridisation (FISH) to assess ejaculated germ cells from patients with a spermiogenesis defect. The proacrosin immunoreactivity, analysed with the use of the monoclonal antibody 4D4, has been detected in cells of round spermatid size presenting a haploid FISH figure as well as in larger cells whose ploidy corresponds to primary and secondary spermatocytes. These observations are in agreement with previously published results obtained, with the use of the same antibody, by immunocytochemical analysis of histological sections of testicular tissue. All the cells of round spermatid size possessing proacrosin immunoreactivity were found to be haploid by FISH. On the other hand, some of the haploid cells of round spermatid size did not possess proacrosin immunoreactivity. The structural pattern of proacrosin immunoreactivity was highly variable both in spermatids and in younger spermatogenic cells. These data show that cell size is the main criterion to be used for the identification of ejaculated round spermatids, whereas the presence of the developing acrosome represents only an auxiliary criterion. The scoring of acrosomal development in ejaculated spermatids may be useful as part of pre-treatment diagnosis before the inclusion of infertile couples in a spermatid conception programme.

Published
1996
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