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将小鼠胚胎一分为二后冷冻和解冻产生单卵双胞胎。

Production of monozygotic twins after freezing and thawing of bisected mouse embryos.

作者信息

Sotomaru Y, Kato Y, Tsunoda Y

机构信息

College of Agriculture, Kinki University, Nakamachi, Nara, 631-8505, Japan.

出版信息

Cryobiology. 1998 Sep;37(2):139-45. doi: 10.1006/cryo.1998.2111.

DOI:10.1006/cryo.1998.2111
PMID:9769164
Abstract

We examined the viability of mouse bisected embryos after freezing and thawing and produced monozygotic twin mice from these embryos. Two-cell embryos were collected from superovulated mature agouti, F1 hybrid (C57BL/6 x CBA) female mice. For bisection, one blastomere of the embryo was aspirated with a micropipette and injected into an empty zona pellucida. After culture for 24 to 28 h to the compacted 4- to 8-cell stage or 48 to 52 h to the late morula to blastocyst stage, the embryos were slowly frozen (-0.5 to -1.0 degrees C/min), thawed (30 degrees C/min), cultured for 24 h, and then transferred to recipient females. The bisected embryos without zonae pellucidae had developmental ability in vitro similar to those with zonae pellucidae (88% vs 89%). However, after freezing and thawing at the compacted 4- to 8-cell stage, bisected embryos with zonae pellucidae had higher viability than those without (60% vs 15%). Zona enclosed, bisected embryos frozen at the compacted 4- to 8-cell stage were more resistnat to freezing and thawing than those at the late morula to blastocyte stage (60% vs 23%). After transfer to recipients 26% of the zona enclosed bisected embryos frozen-thawed at the 4- to 8-cell stage developed to living fetuses a day 17.5 to 18.0 of pregnancy, which was slightly but not significantly lower than that of fresh bisected embryos (48%). On the other hand, only 5% of bisected embryos frozen-thawed at the late morula to blastocyst stage developed to young. The transfer of 15 sets of twin blastocysts as pairs that had been frozen and thawed at the compacted 4- to 8-cell stage yielded 2 (13%) sets of monozygotic twins.

摘要

我们检测了冻融后小鼠二分胚胎的活力,并从这些胚胎中培育出了单卵双生小鼠。从超排的成熟刺豚鼠F1代杂种(C57BL/6×CBA)雌性小鼠中收集二细胞胚胎。进行二分操作时,用微量移液器吸取胚胎的一个卵裂球并注入一个空的透明带中。培养24至28小时至致密化的4至8细胞期,或48至52小时至晚期桑椹胚至囊胚期后,将胚胎缓慢冷冻(-0.5至-1.0℃/分钟),解冻(30℃/分钟),培养24小时,然后移植到受体雌性小鼠体内。无透明带的二分胚胎在体外的发育能力与有透明带的胚胎相似(88%对89%)。然而,在致密化的4至8细胞期冻融后,有透明带的二分胚胎比无透明带的胚胎具有更高的活力(60%对15%)。有透明带包裹的、在致密化的4至8细胞期冷冻的二分胚胎比在晚期桑椹胚至胚泡期冷冻的胚胎更耐冻融(60%对23%)。在移植到受体小鼠后,26%的在4至8细胞期冻融的有透明带包裹的二分胚胎在妊娠第17.5至18.0天发育成活胎儿,略低于新鲜二分胚胎(48%),但差异不显著。另一方面,在晚期桑椹胚至囊胚期冻融的二分胚胎只有5%发育成幼仔。移植15组在致密化的4至8细胞期冻融的双囊胚对,产生了2组(13%)单卵双生小鼠。

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