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新生小鼠卵巢冷冻保存及异种移植后卵泡发育与卵母细胞成熟的研究

[Investigation of follicular development and oocyte maturation after cryopreservation and xenograft of newborn mouse ovaries].

作者信息

Qin Bo-Lin, Chen Xue-Jin, Shi Zhen-Dan, Li Wan-Li, Tian Yun-Bo

机构信息

The Laboratory of Developmental Biology, Xinhua Hospital, School of Medical Sciences, Shanghai Jiaotong University, Shanghai 200092, China.

出版信息

Sheng Li Xue Bao. 2006 Feb 25;58(1):41-6.

Abstract

In order to explore the feasibility of cryopreserving primordial follicles in attaining their developmental competence following freezing and thawing, ovaries from newborn mice were cryopreserved and the thawed ovaries were xenografted into kidney capsules of adult female mice. Ovaries were isolated from newborn B6C2F(1) female mice, infiltrated by Leibovitz 15 (L-15) medium containing 10% (V/V) fetal bovine serum (FBS) and 1.5 mol/L dimethylsulfoxide (DMSO), and then packed into 0.25 ml plastic straws. The ovaries contained in straws were frozen under nitrogen vapour at -40 degrees C in Cryocell 1200 programmable freezer, and stored in liquid nitrogen for periods ranging from 1 week to 6 months. Upon thawing, the straws were dipped into room temperature water for 1020 s, after which the ovaries were collected and washed in L-15 buffer containing 10% (V/V) FBS without DMSO to remove cryoprotectant. The thawed ovaries were transplanted into kidney capsules of 812-week old adult B6C2F(1) female recipient mice by two protocols, with either 1 or 2 ovaries in each capsule. Upon withdrawal after at least 14 d of transplantation, only 45.00% (72/160) of the ovaries were recovered from 40 recipients transplanted with 2 ovaries in each capsule, compared to 82.50% (33/40) in 20 recipients with only 1 ovary in each capsule. The grafted ovaries exhibited similar follicular developmental progression to that of natural ovaries. There were antral follicles present in the transplanted ovaries on day 14, whose number increased more substantially on day 19 after transplantation. Following stimulation of the recipient mice with 10 IU PMSG on day 19 after xenografting, follicles further developed to preovulatory stage with appearance of cumulus oocytes and enlarged antrum. Oocytes from these fully grown antral follicles were collected and matured in vitro in modified essential medium-alpha (MEMalpha). After 1617 h of culture, 40.90% of the oocytes exhibited germinal vesicle breakdown (GVBD) and among which 89.02% proceeded to the metaphase II (MII) stage as indicated by exclusion of the first polar body. The remaining oocytes were further cultured and 50.83% of which initiated GVBD by 2021 h of culture, but only 21.40% of which proceeded to MII. The above results demonstrated that the primordial follicles in newborn mouse ovaries were capable of sustaining freezing and thawing, and reinitiating development following xenograft into kidney capsule in adult recipient female mice. Production of mature oocytes from such re-developed follicles following gonadotrophin priming and the subsequent oocyte in vitro maturation implied immense prospect of application of this method to preserve female germ cells, conserve endangered species, establish animal gene stock, and utilize oocytes in assisted reproductive techniques.

摘要

为了探索冷冻保存原始卵泡在冻融后获得发育能力的可行性,将新生小鼠的卵巢进行冷冻保存,并将解冻后的卵巢移植到成年雌性小鼠的肾囊中。从新生B6C2F(1)雌性小鼠中分离出卵巢,用含有10%(V/V)胎牛血清(FBS)和1.5 mol/L二甲基亚砜(DMSO)的Leibovitz 15(L-15)培养基浸润,然后装入0.25 ml塑料细管中。细管中的卵巢在Cryocell 1200可编程冷冻机中于-40℃的氮蒸气下冷冻,并在液氮中储存1周至6个月。解冻时,将细管浸入室温水中1020 s,之后收集卵巢并在不含DMSO的含有10%(V/V)FBS的L-15缓冲液中洗涤以去除冷冻保护剂。解冻后的卵巢通过两种方案移植到812周龄成年B6C2F(1)雌性受体小鼠的肾囊中,每个囊中移植1个或2个卵巢。在移植至少14 d后取出时,在每个囊中移植2个卵巢的40只受体中,仅45.00%(72/160)的卵巢被回收,而在每个囊中仅移植1个卵巢的20只受体中,这一比例为82.50%(33/40)。移植的卵巢表现出与天然卵巢相似的卵泡发育进程。移植后第14天,移植的卵巢中有窦状卵泡,移植后第19天其数量增加更为显著。在异种移植后第19天用10 IU孕马血清促性腺激素(PMSG)刺激受体小鼠后,卵泡进一步发育到排卵前阶段,出现卵丘卵母细胞且窦腔扩大。从这些完全成熟的窦状卵泡中收集卵母细胞,并在改良的α-基本培养基(MEMα)中进行体外成熟培养。培养1617 h后,40.90%的卵母细胞出现生发泡破裂(GVBD),其中89.02%排出第一极体进入中期Ⅱ(MII)期。其余卵母细胞继续培养,培养2021 h时50.83%的卵母细胞开始出现GVBD,但只有21.40%进入MII期。上述结果表明,新生小鼠卵巢中的原始卵泡能够承受冻融,并在移植到成年受体雌性小鼠的肾囊后重新启动发育。经促性腺激素启动后从这些重新发育的卵泡中产生成熟卵母细胞,随后进行卵母细胞体外成熟培养,这意味着该方法在保存雌性生殖细胞、保护濒危物种、建立动物基因库以及在辅助生殖技术中利用卵母细胞方面具有巨大的应用前景。

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