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Equilibration time with cryoprotectants, but not melatonin supplementation during in vitro maturation, affects viability and metaphase plate morphology of vitrified porcine mature oocytes

Gonzalez-Plaza, Alejandro (author)
Univ Murcia, Spain; Inst Biomed Res Murcia IMIB Arrixaca, Spain
Brullo, Cristiano (author)
Univ Bologna, Italy; Univ Bologna, Italy
Cambra, Josep M. (author)
Univ Murcia, Spain; Inst Biomed Res Murcia IMIB Arrixaca, Spain
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Garcia, Manuela (author)
Univ Murcia, Spain; Inst Biomed Res Murcia IMIB Arrixaca, Spain
Iacono, Eleonora (author)
Univ Bologna, Italy; Univ Bologna, Italy
Parrilla, Inmaculada (author)
Univ Murcia, Spain; Inst Biomed Res Murcia IMIB Arrixaca, Spain
Gil, Maria Antonia (author)
Univ Murcia, Spain; Inst Biomed Res Murcia IMIB Arrixaca, Spain
Martinez, Emilio A. (author)
Univ Murcia, Spain; Inst Biomed Res Murcia IMIB Arrixaca, Spain
Martinez-Serrano, Cristina (author)
Linköpings universitet,Avdelningen för barns och kvinnors hälsa,Medicinska fakulteten
Cuello, Cristina (author)
Univ Murcia, Spain; Inst Biomed Res Murcia IMIB Arrixaca, Spain
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 (creator_code:org_t)
2022-05-24
2022
English.
In: Reproduction in domestic animals. - : Wiley. - 0936-6768 .- 1439-0531. ; 57:S5, s. 58-63
  • Journal article (peer-reviewed)
Abstract Subject headings
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  • The aims of this study were to investigate the effects of different equilibration times with cryoprotectants on viability and metaphase plate morphology of vitrified-warmed porcine mature oocytes (Experiment 1) and to evaluate the effects of supplementation with 10(-9) M melatonin during in vitro maturation on these parameters (Experiment 2). In Experiment 1, 2,392 mature oocytes were vitrified using different equilibration times of oocytes with cryoprotectants (3, 10, 15, 20, 30, 40, 60 and 80 min). Fresh oocytes matured in vitro for 44 hr (n = 509) were used as controls. In Experiment 2, a total of 573 COCs were used. COCs were matured with 10(-9) M melatonin supplementation or without melatonin (control). Some oocytes from each group were vitrified with a 60-min equilibration time with cryoprotectants according to the results of Experiment 1. The remaining oocytes from each maturation group were used as fresh control groups. In both experiments, oocytes were stained with 2 ,7 -dichlorodihydrofuorescein diacetate and Hoechst 33342 to assess viability and metaphase plate morphology, respectively. Vitrification and warming affected (p < .01) oocyte viability compared with controls, which were all viable after 44 hr of IVM. In Experiment 1, the longer the equilibration time with cryoprotectants, the higher the viability. Oocytes equilibrated for 60 and 80 min had the highest (p < .05) viability and similar metaphase plate characteristics to the fresh control oocytes. In Experiment 2, supplementation with melatonin during in vitro maturation had no effect on oocyte viability or metaphase plate morphology of vitrified-warmed oocytes. In conclusion, under our experimental conditions, vitrified porcine mature oocytes equilibrated with cryoprotectants for 60 or 80 min exhibited the highest viability and similar metaphase plate characteristics to fresh controls. Furthermore, supplementation with 10(-9) M melatonin during in vitro maturation had no effect on these parameters.

Subject headings

LANTBRUKSVETENSKAPER  -- Veterinärmedicin -- Klinisk vetenskap (hsv//swe)
AGRICULTURAL SCIENCES  -- Veterinary Science -- Clinical Science (hsv//eng)

Keyword

cryotop; melatonin; oocyte; porcine; vitrification

Publication and Content Type

ref (subject category)
art (subject category)

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