4.7 Article

Changing the start temperature and cooling rate in a slow-freezing protocol increases human blastocyst viability

Journal

FERTILITY AND STERILITY
Volume 79, Issue 2, Pages 407-410

Publisher

ELSEVIER SCIENCE INC
DOI: 10.1016/S0015-0282(02)04576-4

Keywords

blastocyst; cryopreservation; culture; embryo; IVF; viability

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Objective: To determine the effect of start temperature and cooling rate of a slow freezing protocol on human blastocyst viability. Design: Controlled-rate freezing of human blastocysts using different start temperatures and cooling rates. Setting: Private assisted reproductive technology unit. Patient(s): Patients donated with consent cryopreserved pronucleate embryos. Intervention(s): Culture of thawed pronucleate embryos in G III series media, containing hyaluronan, followed by cryopreservation of 36 blastocysts with subsequent noninvasive analysis of embryo metabolism. Main Outcome Measure(s): Pyruvate and glucose consumption and blastocyst reexpansion and quality. Result(s): Glucose consumption and blastocyst reexpansion after thaw were significantly higher when a start temperature of -6degreesC and a cooling rate of 0.5degreesC/min to -32degreesC were used compared with a start temperature of 20degreesC and a cooling rate of 2degreesC to -6degreesC, followed by cooling at 0.3degreesC to -35degreesC. Pyruvate uptake after thaw was not affected by the freezing procedure. Clinical use of the lower start temperature and quicker cooling rate, combined with culture in hyaluronan-based media, has led to the establishment of a 30% implantation rate. Conclusion(s): Human embryos cultured to the blastocyst stage in hyaluronan-based sequential media are readily cryopreserved and maintain their viability after thaw. (C) 2003 by American Society for Reproductive Medicine.

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