Cryopreservation of human failed maturation oocytes shows that vitrification gives superior outcomes to slow cooling
This study investigated whether failed maturation oocytes could be used to evaluate different cryopreservation procedures. A total of 289 failed maturation oocytes (GV and MI stages), obtained from 169 patients undergoing IVF treatment (mean age 33.84 ± 5.0) were divided into two different slow-cool...
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Veröffentlicht in: | Cryobiology 2010-12, Vol.61 (3), p.243-247 |
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Sprache: | eng |
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Zusammenfassung: | This study investigated whether failed maturation oocytes could be used to evaluate different cryopreservation procedures. A total of 289 failed maturation oocytes (GV and MI stages), obtained from 169 patients undergoing IVF treatment (mean age 33.84
±
5.0) were divided into two different slow-cooling groups (1.5
mol/l 1,2-propanediol
+
0.2
mol/l sucrose in either NaCl (group A) or choline chloride (ChCl) (group B) based cryopreservation solutions) and one vitrification group (15% ethylene glycol
+
15% dimethyl sulphoxide). Survival rate, in vitro maturation (IVM) rate, fertilization and developmental rate of cryopreserved oocytes were assessed. Regardless of the stage at which cryopreservation was performed (GV
+
MI), the slow cooling with ChCl based medium always gave significantly lower survival rate than the slow cooling in NaCl based medium (
p
=
0.01) and vitrification (
p
<
0.001). An extended study also showed statistically reduced survival rate between slow-cooling NaCl based medium and vitrification (
p
<
0.05). Global results of in vitro maturation and fertilization showed worse results between both slow-cooling NaCl and ChCl based media versus vitrification. In conclusion, for oocytes that had failed to mature, vitrification gave better survival, maturation, fertilization and also cleavage rates than the slow-cooling protocols. Four cells embryos were obtained only from vitrified in vitro matured MI oocytes. |
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ISSN: | 0011-2240 1090-2392 |
DOI: | 10.1016/j.cryobiol.2010.08.002 |