Table 2. Development to the hatched blastocyst stage of in vitro-produced expanded blastocysts vitrified using the MVAC or Cryotop device, warmed and cultured in vitro for 72 h.
| Vitrification method | No. of cryopreserved embryos |
No. of hatched embryos (%) |
||
| 24 h | 48 h | 72 h | ||
| Solution control | 117 | 73a | 94 | 109 |
| (62.4%) | (80.3%) | (93.2%) | ||
| MVAC | 110 | 53ab | 88 | 102 |
| (48.2%) | (80.0%) | (92.7%) | ||
| MVAC in LN2 | 114 | 40b | 82 | 104 |
| (35.1%) | (71.9%) | (91.2%) | ||
| Cryotop | 114 | 61ab | 89 | 102 |
| (53.5%) | (78.1%) | (89.5%) | ||
Six replications were performed. a, b Values within a single column that have different superscripts are significantly different at P < 0.05 using one-way ANOVA. Solution control: IVP expanded blastocysts that were exposed to vitrification and warming solutions. MVAC: IVP expanded blastocysts that were vitrified by inserting the MVAC device containing them into a precooled 0.25-ml plastic straw. MVAC in LN2: IVP expanded blastocysts that were vitrified by plunging the MVAC device containing them directly into LN2. Cryotop: IVP expanded blastocysts that were vitrified by the Cryotop method. No significant difference in development to the hatched blastocyst stage was detected between the treatment groups at P < 0.05 using one-way ANOVA.