Fertility Preservation Laboratory, Sheba Medical Center, Tel Hashomer, Israel.
Faculty of Medicine, Sackler School of Medicine, Tel Aviv University, Tel Aviv, Israel.
Hum Reprod. 2024 Nov 1;39(11):2551-2564. doi: 10.1093/humrep/deae221.
What is the involvement of ovarian stroma in the anti-Müllerian hormone (AMH) signaling pathway and which stromal cells are involved?
Mouse and human ovaries show high expression of AMH receptor II (AMHR2) in the stromal fibroblasts surrounding the follicles and activation of the post-AMHR2 pathway by recombinant AMH was evidenced by increased phosphorylation of SMAD1,5 and 9, increased expression AMHR2 and upregulation of αSMA, suggesting fibroblast activation to initiate myofibroblast differentiation.
AMH secreted by small growing follicles, regulates ovarian activity. It suppresses initial primordial follicle (PMF) recruitment and FSH-dependent growth. AMH signal transduction is mediated by AMHR2, activating intracellular SMAD proteins and other signaling cascades to induce target-gene expression. Although AMHR2 expression has been reported within the follicle unit, there is evidence suggesting it may be identified in the stroma as well.
STUDY DESIGN, SIZE, DURATION: Fresh murine ovaries were extracted from BALB/c mice (6 weeks old; n = 12 and 21 days old; n = 56). Frozen-thawed ovarian fragments were obtained from 10 women, aged 18-35, who had undergone ovarian tissue cryopreservation and donated frozen ovarian tissue for research.
PARTICIPANTS/MATERIALS, SETTING, METHODS: Murine (6 weeks old) and human donor ovaries were immunostained for AMHR2 and Collagen 1α/αSMA/VCAM1, with additional vimentin staining in mice. Murine (21 days old) and human donor ovaries were used for fibroblast isolation and subsequent 7-day cultures. Prior to assessing AMH effects on isolated fibroblast culture, purity validation tests were implemented to ensure the absence of epithelial, immune, endothel, granulosa, and theca ovarian cell populations. The fibroblast culture's homogeneity was validated by RT-qPCR and western-blot assays, confirming negativity for E-cadherin, CD31, aromatase, CYP17A1, and positivity for αSMA and vimentin. Fibroblasts were then subjected to rAMH treatment in vitro (200 ng/ml) for 0-72 h, with an additional time point of 96 h for human samples, followed by RT-qPCR, western blot, and immunocytochemistry (ICC) for AMHR2 expression. AMHR2 post-receptor signaling was examined by pSMAD1,5,9 levels via western blot. Activated fibroblast marker, αSMA, was assessed via western blot and ICC.
Immunostaining of mouse and human ovarian tissue showed that stromal cells around follicles at all developmental stages exhibit high AMHR2 expression, while granulosa cells of growing follicles show considerably lower levels. The majority of these AMHR2-positive stromal cells were identified as fibroblasts (Collagen1α in mice and human; vimentin in mice). RT-qPCR, western blot, and immunostaining were performed on cultured mouse and human fibroblasts, confirming that they consisted of a pure fibroblast population (αSMA/vimentin positive and negative for other cell-type markers). A total of 99.81% (average 28.94 ± 1.34 cells/field in mice) and 100% (average 19.20 ± 1.39 cells/field in human samples) of these fibroblasts expressed AMHR2 (ICC). rAMH treated cultured fibroblasts showed increased pSMAD1,5 and 9 levels, demonstrating the effects of AMH on its downstream signaling pathway. pSMAD1,5 and 9 expression increased, as detected by western blot: 1.92-fold in mice (48 h, P = 0.026) and 2.37-fold in human samples (48 h, P = 0.0002). In addition, rAMH treatment increased AMHR2 protein expression, as observed in ICC (human): a 2.57-fold upregulation of AMHR2 Mean Fluorescence Intensity (MFI) (96 h, P = 0.00036), and western blot, showing a 4.2-fold time-dependent increase (48 h, P = 0.026) in mice and 2.4-fold change (48 h, P = 0.0003) in human donors. Exposure to rAMH affected AMHR2 transcription upregulation, with a 6.48-fold change (72 h, P = 0.0137) in mice and a 7.87-fold change (72 h, P < 0.0001) in humans. rAMH treatment induced fibroblast activation (αSMA positive), demonstrating the dynamic effects of AMH on fibroblast behavior. αSMA expression elevation was detected in ICC with a 2.28-fold MFI increase in humans (96 h, P = 0.000067), and in western blot with a 5.12-fold increase in mice (48 h, P = 0.0345) and a 2.69-fold increase in humans (48 h, P ≤ 0.0001). Activated AMHR2-positive stained fibroblast fractions were solely located around growing follicles, in both human and mice. In addition, a small population of AMHR2-positive stained theca cells (VCAM1 positive) was observed.
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LIMITATIONS, REASONS FOR CAUTION: Ex vivo, fibroblast gene expression might be changed by adhesion to the tissue-culture plate. Nevertheless, cultured fibroblasts (with and without rAMH) are subjected to the same conditions. Observations or significant differences can therefore be considered reliable. In addition, the presented effect of rAMH on fibroblasts is not directly linked to the known inhibitory effect of AMH on follicle activation.
Clarifying the populations of AMH-responsive cells in the ovary provides a foundation for further investigation of the complex AMH signaling across the ovary. The composition of AMH-releasing and -responsive cells can shed light on the communication network between follicles and their environment, which may elucidate the mechanisms behind the AMH inhibitory effect on PMF activation.
STUDY FUNDING/COMPETING INTEREST(S): This work was financially supported by grants from the Kahn Foundation. There are no competing interests in this study.
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抗苗勒氏管激素(AMH)信号通路中卵巢基质的参与情况以及涉及哪些基质细胞?
小鼠和人卵巢中的基质成纤维细胞在卵泡周围显示出高表达的 AMH 受体 II(AMHR2),并且通过重组 AMH 激活后 AMHR2 途径,通过增加 SMAD1、5 和 9 的磷酸化、增加 AMHR2 的表达和上调αSMA 来证实,表明成纤维细胞激活以启动肌成纤维细胞分化。
由小生长卵泡分泌的 AMH 调节卵巢活动。它抑制初始原始卵泡(PMF)募集和 FSH 依赖性生长。AMH 信号转导由 AMHR2 介导,激活细胞内 SMAD 蛋白和其他信号通路以诱导靶基因表达。尽管已经报道 AMHR2 表达存在于卵泡单位内,但有证据表明它也可能在基质中被识别。
研究设计、大小、持续时间:从 6 周大的 BALB/c 小鼠(n=12)和 21 天大的(n=56)中提取新鲜的鼠卵巢。从 10 名年龄在 18-35 岁之间的女性中获得冷冻解冻的卵巢组织碎片,她们接受了卵巢组织冷冻保存并捐赠了冷冻卵巢组织用于研究。
参与者/材料、设置、方法:对 6 周大的小鼠和人供体卵巢进行 AMHR2 和胶原 1α/αSMA/VCAM1 的免疫染色,并用额外的鼠 vimentin 染色。对 21 天大的人和人供体卵巢进行成纤维细胞分离和随后的 7 天培养。在评估 AMH 对分离的成纤维细胞培养物的影响之前,进行了纯度验证测试,以确保不存在上皮、免疫、内皮、颗粒细胞和卵泡膜细胞群体。通过 RT-qPCR 和 Western blot 分析确认成纤维细胞培养物的同源性,证实其 E-钙粘蛋白、CD31、芳香酶、CYP17A1 为阴性,αSMA 和 vimentin 为阳性。然后将成纤维细胞在体外(200ng/ml)用 rAMH 处理 0-72 小时,人样本再增加 96 小时的时间点,然后进行 RT-qPCR、Western blot 和免疫细胞化学(ICC)以评估 AMHR2 表达。通过 Western blot 检测 AMHR2 后受体信号 pSMAD1、5、9 水平。通过 Western blot 和 ICC 评估激活的成纤维细胞标志物αSMA。
对小鼠和人卵巢组织的免疫染色显示,所有发育阶段的卵泡周围基质细胞均表现出高 AMHR2 表达,而生长卵泡的颗粒细胞表达水平则明显较低。这些 AMHR2 阳性基质细胞中的大多数被鉴定为成纤维细胞(小鼠中的胶原 1α和人;小鼠中的 vimentin)。对培养的鼠和成纤维细胞进行 RT-qPCR、Western blot 和免疫染色,证实它们由纯成纤维细胞群体组成(αSMA/vimentin 阳性,其他细胞类型标志物阴性)。这些成纤维细胞中的 99.81%(平均每视野 28.94±1.34 个细胞/视野)和 100%(平均每视野 19.20±1.39 个细胞/视野)表达 AMHR2(ICC)。用 rAMH 处理的培养成纤维细胞显示出增加的 pSMAD1、5 和 9 水平,表明 AMH 对其下游信号通路的作用。通过 Western blot 检测到 pSMAD1、5 和 9 的表达增加:在小鼠中增加 1.92 倍(48 小时,P=0.026),在人样本中增加 2.37 倍(48 小时,P=0.0002)。此外,rAMH 处理增加了 AMHR2 蛋白表达,如 ICC(人)所示:AMHR2 平均荧光强度(MFI)的上调 2.57 倍(96 小时,P=0.00036),Western blot 显示 48 小时时(P=0.026)在小鼠中增加 4 倍,在人类供体中增加 2.4 倍(48 小时,P=0.0003)。rAMH 处理影响 AMHR2 转录上调,在小鼠中增加 6.48 倍(72 小时,P=0.0137),在人类中增加 7.87 倍(72 小时,P<0.0001)。rAMH 处理诱导成纤维细胞激活(αSMA 阳性),表明 AMH 对成纤维细胞行为的动态影响。通过 ICC 检测到 αSMA 表达升高,在人类中增加了 2.28 倍 MFI(96 小时,P=0.000067),在 Western blot 中在小鼠中增加了 5.12 倍(48 小时,P=0.0345),在人类中增加了 2.69 倍(48 小时,P≤0.0001)。在人类和小鼠中,活化的 AMHR2 阳性染色的成纤维细胞部分仅位于生长卵泡周围。此外,观察到一小部分 AMHR2 阳性染色的卵泡膜细胞(VCAM1 阳性)。
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局限性、谨慎原因:在体外,细胞黏附在组织培养板上可能改变成纤维细胞的基因表达。然而,用 rAMH 处理的培养成纤维细胞处于相同的条件下。因此,可以认为观察到的或显著差异是可靠的。此外,本文所提出的 rAMH 对成纤维细胞的作用与 AMH 对卵泡激活的已知抑制作用并不直接相关。
阐明 AMH 反应细胞在卵巢中的分布情况,为进一步研究 AMH 在卵巢中的复杂信号转导提供了基础。AMH 释放和反应细胞的组成可以阐明卵泡与其环境之间的通讯网络,这可能阐明 AMH 抑制 PMF 激活的机制。
研究资金/利益冲突:本工作得到 Kahn 基金会的资助。本研究无利益冲突。
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