低温解冻卵巢皮质中次级卵泡的体外生长。

IF 6 1区 医学 Q1 OBSTETRICS & GYNECOLOGY
Hui Cheng, Fu Wei, Julieta S Del Valle, Tessa H R Stolk, Judith A Huirne, Joyce D Asseler, Gonneke S K Pilgram, Lucette A J Van Der Westerlaken, Norah M Van Mello, Susana M Chuva De Sousa Lopes
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引用次数: 0

摘要

研究问题:能否从培养低温解冻的人类卵巢皮质组织中获得次级卵泡?在相同的培养条件下,我们从顺式女性供体(cOVA)的低温解冻人卵巢皮质组织中获得了高质量的次级卵泡,但从反式男性供体(tOVA)中却没有获得:以前曾有人从成年顺式女性供体新鲜获得的卵巢皮质组织开始,将单层卵泡中的卵母细胞体外培养成分裂期 II 阶段(MII)的卵母细胞。这涉及到一个多步骤的培养方案,第一步包括从单层卵泡向多层次级卵泡的过渡。鉴于用于生育力保存的卵巢皮质(来自顺式女性和逆式男性供体)都是低温保存的,因此研究来自低温解冻卵巢皮质的单层卵泡在培养过程中的生长潜力至关重要:研究设计、规模、持续时间:将来自成年反式男性供体(n = 3)和成年顺式女性供体(n = 3)的低温保存-解冻卵巢皮质组织用于体外培养,按照两种已公布的培养方案中描述的第一个培养步骤(7-8天和21天)进行培养,并与来自反式男性供体(n = 3)的新鲜分离卵巢皮质和培养前的卵巢皮质进行比较:卵巢皮质组织取自正在接受性别确认手术并使用睾酮的成年男性变性捐献者,以及在化疗前为保留生育能力而接受输卵管切除术的成年顺式女性捐献者。卵巢皮质在培养期之前(第 0 天)或之后进行固定。通过组织学和免疫荧光评估卵泡的存活、生长和形态:我们对培养后卵泡发育的不同阶段(原始卵泡、初级卵泡、次级卵泡和闭锁卵泡)进行了量化,观察到无论使用哪种培养基,次级卵泡的比例都在增加,基质区的 COLIV 沉积也在增加。从 cOVA 中获得的次级卵泡的质量与培养前的质量相当。然而,与培养前的tOVA次级卵泡相比,在相同的培养条件下,tOVA(新鲜和冷冻)次级卵泡的质量较低,含有直径较小的卵母细胞、表达异常水平KRT19和类固醇生成标记物STAR的颗粒细胞,并且缺乏ACTA2+ theca细胞:研究结果的广泛意义:我们的研究表明,低温解冻的cOVA可用于在培养后生成高质量的次级卵泡,现在可以对这些卵泡进行进一步测试,以评估它们生成可用于临床的功能性MII卵母细胞的潜力。然而,对 tOVA(新鲜和低温)使用相同的培养方案并不能产生高质量的次级卵泡,这表明要么睾酮处理会影响卵泡质量,要么需要调整培养方案才能从 tOVA 中获得高质量的次级卵泡。重要的是,在使用tOVA优化体外卵泡生成时必须谨慎:本研究由欧洲研究理事会联合资助 OVOGROWTH(ERC-CoG-2016-725722,J.S.D.V.和 S.M.C.D.S.L.获得)、诺和诺德基金会(reNEW NF21CC0073729,H.C、F.W.、J.S.D.V.和 S.M.C.D.S.L.),以及国家留学基金委(CSC 202008320362 和 CSC 202008450034,分别给 H.C.和 F.W.)。作者没有利益冲突需要声明:不适用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
In vitro growth of secondary follicles from cryopreserved-thawed ovarian cortex.

Study question: Can secondary follicles be obtained from cultured cryopreserved-thawed human ovarian cortical tissue?

Summary answer: We obtained high-quality secondary follicles from cultured cryopreserved-thawed human ovarian cortical tissue from cis female donors (cOVA), but not from trans masculine donors (tOVA) in the same culture conditions.

What is known already: The in vitro growth of oocytes present in unilaminar follicles into metaphase II stage (MII) oocytes has been previously achieved starting from freshly obtained ovarian cortical tissue from adult cis female donors. This involved a multi-step culture protocol and the first step included the transition from unilaminar follicles to multilayered secondary follicles. Given that the ovarian cortex (from both cis female and trans masculine donors) used for fertility preservation is cryopreserved, it is crucial to investigate the potential of unilaminar follicles from cryopreserved-thawed ovarian cortex to grow in culture.

Study design, size, duration: Cryopreserved-thawed ovarian cortical tissue from adult trans masculine donors (n = 3) and adult cis female donors (n = 3) was used for in vitro culture following the first culture step described in two published culture protocols (7-8 days and 21 days) and compared to freshly isolated ovarian cortex from trans masculine donors (n = 3) and to ovarian cortex prior to culture.

Participants/materials, setting, methods: Ovarian cortical tissue was obtained from adult trans masculine donors undergoing gender-affirming surgery while using testosterone, and from adult cis female donors undergoing oophorectomy for fertility preservation purposes before chemotherapy. The ovarian cortex was fixed either prior (day 0) or after the culture period. Follicular survival, growth, and morphology were assessed through histology and immunofluorescence.

Main results and the role of chance: We quantified the different stages of follicular development (primordial, primary, secondary, and atretic) after culture and observed an increase in the percentage of secondary follicles as well as an increase in COLIV deposition in the stromal compartment regardless of the culture media used. The quality of the secondary follicles obtained from cOVA was comparable to those prior to culture. However, in the same culture conditions, the secondary follicles from tOVA (fresh and cryo) showed low-quality secondary follicles, containing oocytes with small diameter, granulosa cells that expressed abnormal levels of KRT19 and steroidogenic-marker STAR and lacked ACTA2+ theca cells, when compared to tOVA secondary follicles prior to culture.

Limitations, reasons for caution: The number of different donors used was limited.

Wider implications of the findings: Our study revealed that cryopreserved-thawed cOVA can be used to generate high-quality secondary follicles after culture and those can now be further tested to evaluate their potential to generate functional MII oocytes that could be used in the clinic. However, using the same culture protocol on tOVA (fresh and cryo) did not yield high-quality secondary follicles, suggesting that either the testosterone treatment affects follicular quality or adapted culture protocols are necessary to obtain high-quality secondary follicles from tOVA. Importantly, caution must be taken when using tOVA to optimize folliculogenesis in vitro.

Study funding/competing interest(s): This research was funded by the European Research Council Consolidator Grant OVOGROWTH (ERC-CoG-2016-725722 to J.S.D.V. and S.M.C.D.S.L.), the Novo Nordisk Foundation (reNEW NNF21CC0073729 to H.C., F.W., J.S.D.V., S.M.C.D.S.L.), and China Scholarship Council (CSC 202008320362 and CSC 202008450034 to H.C. and F.W.), respectively. The authors have no conflicts of interest to declare.

Trial registration number: N/A.

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来源期刊
Human reproduction
Human reproduction 医学-妇产科学
CiteScore
10.90
自引率
6.60%
发文量
1369
审稿时长
1 months
期刊介绍: Human Reproduction features full-length, peer-reviewed papers reporting original research, concise clinical case reports, as well as opinions and debates on topical issues. Papers published cover the clinical science and medical aspects of reproductive physiology, pathology and endocrinology; including andrology, gonad function, gametogenesis, fertilization, embryo development, implantation, early pregnancy, genetics, genetic diagnosis, oncology, infectious disease, surgery, contraception, infertility treatment, psychology, ethics and social issues.
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