Liu J, Van der Elst J, Van den Broecke R, Dhont M
Infertility Center, Department of Obstetrics and Gynecology and Department of Gynecologic Oncology, Ghent University Hospital, B-9000 Ghent, Belgium.
Biol Reprod. 2001 Jan;64(1):171-8. doi: 10.1095/biolreprod64.1.171.
The objectives of the present study were to achieve 1) oocyte maturation, 2) oocyte competence of fertilization, and 3) oocyte competence of embryogenesis with oocytes from primordial follicles obtained from cryopreserved newborn mouse ovaries by using a two-step method. In the first step, frozen-thawed newborn mouse ovaries were transplanted under the kidney capsule of recipients for the initiation of growth from the primordial follicle stage on. In the second step, growing preantral follicles in the ovarian grafts were recovered and cultured. The results demonstrated that primordial follicles were able to be recruited to preantral follicles during the period of transplantation, and preantral follicles could be mechanically isolated from ovarian grafts. Under the present in vitro culture conditions, 85.8% of the isolated follicles (n = 332) from ovarian grafts survived the 12-day in vitro culture process, 84.9% of the recovered oocytes (n = 285) were germinal vesicle breakdown (GVBD)-competent, and 76% of the oocytes that underwent GVBD (n = 242) developed to the metaphase II (MII) stage. In the in vitro fertilization experiments, 75.4% of 142 inseminated MII oocytes underwent fertilization and cleavage to the 2-cell stage. Subsequently, 79.7% of the 2-cell-stage embryos (n = 69) progressed to the late morula-early blastocyst stage. Transfer of late morula-early blastocyst embryos resulted in the production of live offspring. From our experiments, it may be concluded that in vivo maturation by grafting followed by in vitro maturation of frozen-thawed primordial follicles can restore fertility in mice. This model could be useful for a similar application in the human.
本研究的目的是通过两步法,利用从冷冻保存的新生小鼠卵巢中获得的原始卵泡卵母细胞,实现以下目标:1)卵母细胞成熟;2)卵母细胞受精能力;3)卵母细胞胚胎发生能力。第一步,将冻融后的新生小鼠卵巢移植到受体的肾包膜下,以使原始卵泡阶段开始生长。第二步,回收并培养卵巢移植物中生长的窦前卵泡。结果表明,在移植期间原始卵泡能够被募集到窦前卵泡,并且窦前卵泡可以从卵巢移植物中机械分离出来。在当前的体外培养条件下,来自卵巢移植物的85.8%的分离卵泡(n = 332)在12天的体外培养过程中存活,84.9%的回收卵母细胞(n = 285)具有生发泡破裂(GVBD)能力,并且76%经历GVBD的卵母细胞(n = 242)发育到中期II(MII)阶段。在体外受精实验中,142个受精的MII卵母细胞中有75.4%发生受精并分裂到2细胞阶段。随后,69个2细胞期胚胎中有79.7%发育到桑葚胚晚期-早期囊胚阶段。移植桑葚胚晚期-早期囊胚胚胎产生了活的后代。从我们的实验可以得出结论,通过移植进行体内成熟,随后对冻融的原始卵泡进行体外成熟,可以恢复小鼠的生育能力。该模型可能对人类的类似应用有用。