Program in Biology of Reproduction, Center for Biomedical Research and Innovation (CiiB), Universidad de los Andes, Santiago 7620001, Chile.
IMPACT, Center of Interventional Medicine for Precision and Advanced Cellular Therapy, Santiago 7620001, Chile.
Int J Mol Sci. 2024 Jan 30;25(3):1678. doi: 10.3390/ijms25031678.
Successful implantation requires coordinated migration and invasion of trophoblast cells into a receptive endometrium. Reduced forkhead box M1 (FOXM1) expression limits trophoblast migration and angiogenesis in choriocarcinoma cell lines, and in a rat model, placental FOXM1 protein expression was significantly upregulated in the early stages of pregnancy compared to term pregnancy. However, the precise role of FOXM1 in implantation events remains unknown. By analyzing mice blastocysts at embryonic day (E3.5), we have demonstrated that FOXM1 is expressed as early as the blastocyst stage, and it is expressed in the trophectoderm of the blastocyst. Since controlled oxygen tension is determinant for achieving normal implantation and placentation and a chronic hypoxic environment leads to shallow trophoblast invasion, we evaluated if FOXM1 expression changes in response to different oxygen tensions in the HTR-8/SVneo first trimester human trophoblast cell line and observed that FOXM1 expression was significantly higher when trophoblast cells were cultured at 3% O, which coincides with oxygen concentrations in the uteroplacental interface at the time of implantation. Conversely, FOXM1 expression diminished in response to 1% O that resembles a hypoxic environment in utero. Migration and angiogenesis were assessed following FOXM1 knockdown and overexpression at 3% O and 1% O, respectively, in HTR-8/SVneo cells. FOXM1 overexpression increased transmigration ability and tubule formation. Using a 3D trophoblast invasion model with trophospheres from HTR-8/SVneo cells cultured on a layer of MATRIGEL and of mesenchymal stem cells isolated from menstrual fluid, we observed that trophospheres obtained from 3D trophoblast invasion displayed higher FOXM1 expression compared with pre-invasion trophospheres. Moreover, we have also observed that FOXM1-overexpressing trophospheres increased trophoblast invasion compared with controls. HTR-8/SVneo-FOXM1-depleted cells led to a downregulation of , , and mRNA expression. Our current findings suggest that FOXM1 participates in embryo implantation by contributing to trophoblast migration and early trophoblast invasion, by inducing transcription activation of genes involved in these processes. Maternal-fetal communication is crucial for trophoblast invasion, and maternal stromal cells may induce higher levels of FOXM1 in trophoblast cells.
成功的着床需要滋养细胞协调迁移并侵入接受性的子宫内膜。叉头框转录因子 M1(FOXM1)表达的减少限制了绒毛膜癌细胞系中的滋养细胞迁移和血管生成,并且在胎盘 FOXM1 蛋白的表达在妊娠早期与足月妊娠相比显著上调的大鼠模型中。然而,FOXM1 在着床事件中的精确作用仍然未知。通过分析胚胎期(E3.5)的小鼠胚泡,我们已经证明 FOXM1 在胚泡阶段表达,并且它在胚泡的滋养外胚层中表达。由于受控的氧张力是实现正常着床和胎盘形成的决定因素,而慢性低氧环境导致浅滋养细胞浸润,因此我们评估了 FOXM1 在 HTR-8/SVneo 人早孕期滋养细胞系中对不同氧张力的反应是否发生改变,并观察到当滋养细胞在 3%O 下培养时,FOXM1 的表达显著升高,这与着床时胎盘界面的氧浓度相吻合。相反,FOXM1 的表达在 1%O 时减少,类似于子宫内的低氧环境。在 HTR-8/SVneo 细胞中分别在 3%O 和 1%O 下进行 FOXM1 敲低和过表达后,评估迁移和血管生成。FOXM1 过表达增加了穿越能力和管状形成。使用 HTR-8/SVneo 细胞的滋养球在 MATRIGEL 层上培养的 3D 滋养细胞侵袭模型和从月经液中分离的间充质干细胞,我们观察到与侵袭前的滋养球相比,来自 3D 滋养细胞侵袭的滋养球显示出更高的 FOXM1 表达。此外,我们还观察到 FOXM1 过表达的滋养球与对照相比增加了滋养细胞的侵袭。HTR-8/SVneo-FOXM1 耗尽的细胞导致 、 和 mRNA 表达下调。我们目前的研究结果表明,FOXM1 通过促进滋养细胞迁移和早期滋养细胞浸润,通过诱导参与这些过程的基因的转录激活,参与胚胎着床。母体-胎儿通讯对于滋养细胞浸润至关重要,母体基质细胞可能会诱导滋养细胞中更高水平的 FOXM1。
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