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Literature DB >> 23446455

L-carnitine supplementation during vitrification of mouse oocytes at the germinal vesicle stage improves preimplantation development following maturation and fertilization in vitro.

Adel R Moawad¹, Seang Lin Tan, Baozeng Xu, Hai Ying Chen, Teruko Taketo.

Abstract

Oocyte cryopreservation is important for assisted reproductive technologies (ART). Although cryopreservation of metaphase II (MII) oocytes has been successfully used, MII oocytes are vulnerable to the damage inflicted by the freezing procedure. Cryopreservation of germinal vesicle stage oocytes (GV-oocytes) is an alternative choice; however, blastocyst development from GV-oocytes is limited largely due to the need for in vitro maturation (IVM). Herein, we evaluated the effects of l-carnitine (LC) supplementation during vitrification and thawing of mouse GV-oocytes, IVM, and embryo culture on preimplantation development after in vitro fertilization (IVF). We first compared the rate of embryonic development from the oocytes that had been collected at the GV stage from three mouse strains, (B6.DBA)F1, (B6.C3H)F1, and B6, and processed for IVM and IVF, as well as that from the oocytes matured in vivo, i.e. ovulated (IVO). Our results demonstrated that the rate of blastocyst development was the highest in the (B6.DBA)F1 strain and the lowest in the B6 strain. We then supplemented the IVM medium with 0.6 mg/ml LC. The rate of blastocyst development improved in the B6 but not in the (B6.DBA)F1 strain. Vitrification of GV-oocytes in the basic medium alone reduced the rate of blastocyst development in both of those mouse strains. LC supplementation to the IVM medium alone did not change the percentage of blastocyst development. However, LC supplementation to both vitrification and IVM media significantly improved blastocyst development to the levels comparable with those obtained from vitrified/thawed IVO oocytes in both of the (B6.DBA)F1 and B6 strains. We conclude that LC supplementation during vitrification is particularly efficient in improving the preimplantation development from the GV-oocytes that otherwise have lower developmental competence in culture.

Entities: Chemical Disease Species

Mesh：

Substances：
Carnitine

Year: 2013 PMID： 23446455 DOI： 10.1095/biolreprod.112.107433

Source DB: PubMed Journal: Biol Reprod ISSN： 0006-3363 Impact factor: 4.285

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Cited

11 in total

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2. Mitochondrial regulation of [Ca²⁺]i oscillations during cell cycle resumption of the second meiosis of oocyte.

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3. Effects of Different Maturation Systems on Bovine Oocyte Quality, Plasma Membrane Phospholipid Composition and Resistance to Vitrification and Warming.

Authors: José F W Sprícigo; Mateus N Diógenes; Ligiane O Leme; Ana L Guimarães; Carolle V Muterlle; Bianca Damiani Marques Silva; David Solà-Oriol; Ivo Pivato; Luciano Paulino Silva; Margot A N Dode
Journal: PLoS One Date: 2015-06-24 Impact factor: 3.240

4. Effect of L-carnitine on in vitro developmental rate, the zona pellucida and hatching of blastocysts and their cell numbers in mouse embryos.

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5. Glycine increases preimplantation development of mouse oocytes following vitrification at the germinal vesicle stage.

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Journal: Sci Rep Date: 2016-11-15 Impact factor: 4.379

Review 6. Mass Spectrometric Analysis of L-carnitine and its Esters: Potential Biomarkers of Disturbances in Carnitine Homeostasis.

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7. Impact of L-carnitine supplementation on the in vitro developmental competence and cryotolerance of buffalo embryos.

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8. Acylcarnitine esters profiling of serum and follicular fluid in patients undergoing in vitro fertilization.

Authors: Akos Várnagy; Judit Bene; Endre Sulyok; Gábor L Kovács; József Bódis; Béla Melegh
Journal: Reprod Biol Endocrinol Date: 2013-07-17 Impact factor: 5.211

9. Production of blastocysts following in vitro maturation and fertilization of dromedary camel oocytes vitrified at the germinal vesicle stage.

Authors: Mohamed Fathi; Adel R Moawad; Magdy R Badr
Journal: PLoS One Date: 2018-03-15 Impact factor: 3.240

10. Deficiency of peroxiredoxin 6 or inhibition of its phospholipase A₂ activity impair the in vitro sperm fertilizing competence in mice.

Authors: Adel R Moawad; Maria C Fernandez; Eleonora Scarlata; Chandra Dodia; Sheldon I Feinstein; Aron B Fisher; Cristian O'Flaherty
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