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通过异种移植评估冷冻保存的灵长类动物卵巢组织中的卵泡发育:青春期前组织对冷冻保护剂的选择不那么敏感。

Assessment of follicular development in cryopreserved primate ovarian tissue by xenografting: prepubertal tissues are less sensitive to the choice of cryoprotectant.

机构信息

Department of Obstetrics and Gynecology, Campus Grosshadern LMU Munich, 81377 Munich, Germany.

出版信息

Reproduction. 2011 Apr;141(4):481-90. doi: 10.1530/REP-10-0454. Epub 2011 Feb 3.

Abstract

Improvements in cancer survival rates have renewed interest in the cryopreservation of ovarian tissue for fertility preservation. We used the marmoset as a non-human primate model to assess the effect of different cryoprotectives on follicular viability of prepubertal compared to adult ovarian tissue following xenografting. Cryopreservation was performed with dimethylsulfoxide (DMSO), 1,2-propanediol (PrOH), or ethylene glycol (EG) using a slow freezing protocol. Subsequently, nude mice received eight grafts per animal from the DMSO and the PrOH groups for a 4-week grafting period. Fresh, cryopreserved-thawed, and xenografted tissues were serially sectioned and evaluated for the number and morphology of follicles. In adult tissue, the percentage of morphologically normal primordial follicles significantly decreased from 41.2 ± 4.5% (fresh) to 13.6 ± 1.8 (DMSO), 9.5 ± 1.7 (PrOH), or 6.8 ± 1.0 (EG) following cryopreservation. After xenografting, the percentage of morphologically normal primordial (26.2 ± 2.5%) and primary follicles (28.1 ± 5.4%) in the DMSO group was significantly higher than that in the PrOH group (12.2 ± 3 and 5.4 ± 2.1% respectively). Proliferating cell nuclear antigen (PCNA) staining suggests the resumption of proliferative activity in all cellular compartments. In prepubertal tissues, primordial but not primary follicles display a similar sensitivity to cryopreservation, and no significant differences between DMSO and PrOH following xenografting were observed. In conclusion, DMSO shows a superior protective effect on follicular morphology compared with PrOH and EG in cryopreserved tissues. Xenografting has confirmed better efficacy of DMSO versus PrOH in adult but not in prepubertal tissues, probably owing to a greater capacity of younger animals to compensate for cryoinjury.

摘要

癌症存活率的提高重新激发了人们对卵巢组织冷冻保存以保留生育能力的兴趣。我们使用狨猴作为非人类灵长类动物模型,评估了在异种移植后,与成年卵巢组织相比,不同冷冻保护剂对未成年和成年卵巢组织中卵泡活力的影响。使用二甲亚砜(DMSO)、1,2-丙二醇(PrOH)或乙二醇(EG)通过慢速冷冻方案进行冷冻保存。随后,每只裸鼠接受来自 DMSO 和 PrOH 组的 8 个移植物,进行 4 周的移植期。新鲜、冷冻保存-解冻和异种移植组织连续切片,并评估卵泡数量和形态。在成年组织中,形态正常的原始卵泡百分比从新鲜组织的 41.2%±4.5%显著下降至冷冻保存后的 13.6%±1.8%(DMSO)、9.5%±1.7%(PrOH)或 6.8%±1.0%(EG)。异种移植后,DMSO 组形态正常的原始卵泡(26.2%±2.5%)和初级卵泡(28.1%±5.4%)的百分比显著高于 PrOH 组(分别为 12.2%±3 和 5.4%±2.1%)。增殖细胞核抗原(PCNA)染色表明所有细胞区室的增殖活性均恢复。在未成年组织中,原始卵泡而非初级卵泡对冷冻保存具有相似的敏感性,且异种移植后 DMSO 和 PrOH 之间没有观察到显著差异。总之,与 PrOH 和 EG 相比,DMSO 在冷冻保存组织中对卵泡形态具有更好的保护作用。异种移植证实了 DMSO 与 PrOH 相比在成年组织中的效果更好,但在未成年组织中没有,这可能是由于年轻动物对冷冻损伤的补偿能力更强。

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