缺氧诱导的 microRNA-141 通过阻断 CXCL12β/CXCR2/4 信号转导调节滋养细胞凋亡、侵袭和血管生成。
Hypoxia-induced microRNA-141 regulates trophoblast apoptosis, invasion, and vascularization by blocking CXCL12β/CXCR2/4 signal transduction.
机构信息
Department of Obstetrics, Hainan General Hospital, Haikou, People's Republic of China.
Department of Obstetrics, Hainan General Hospital, Haikou, People's Republic of China.
出版信息
Biomed Pharmacother. 2019 Aug;116:108836. doi: 10.1016/j.biopha.2019.108836. Epub 2019 Apr 17.
BACKGROUND
An impaired trophoblast invasion ability contributes to the development of pre-eclampsia (PE), and can be induced by the altered expression of various microRNAs (miRs). MiR-141 and CXCL12β (C-X-C motif chemokine ligand 12) signaling regulate trophoblast invasion and vascularization capabilities during PE pathogenesis; however, their interactions and underlying mechanisms of action remain unclear. We investigated how miR-141 modulates trophoblast invasion, with a focus on its interaction with CXCL12β signaling.
METHODS
A PE model was established by using HTR-8/SVneo cells, which were first cultured with 2% O for 48 h, and then with 5% O. The expression of miR-141 in human villous trophoblast HTR-8/SVneo cells was modulated with mimics or an inhibitor, and analyzed by quantitative RT-PCR. CXCL12β levels were determined by ELISA. Cell apoptosis was determined by flow cytometry, and the invasion and vascularization capabilities of trophoblasts were evaluated by Transwell and tube formation assays, respectively. Binding of miR-141 with CXCL12β mRNA was verified by the dual luciferase assay. Protein levels were estimated by western blotting.
RESULTS
MiR-141 expression was significantly induced by hypoxia in HTR-8/SVneo cells. MiR-141 was found to promote apoptosis and inhibit the invasion and vascularization abilities of HTR-8/SVneo cells under conditions of hypoxia. MiR-141 could directly bind with the 3'UTR region of CXCL12β mRNA and inhibit its translation. In addition, we proved that miR-141 could inhibit the invasion and vascularization abilities, and promote the apoptosis of HTR-8/SVneo cells by targeting CXCL12β under hypoxic conditions. Furthermore, we demonstrated that arachidonic acid could reverse the invasion and apoptosis abilities of HTR-8/SVneo cells mediated by CXCL12β during hypoxia. In terms of mechanism, MiR-141 could downregulate MMP2, p62, and LC3B expression, and upregulate ROCK1 and RhoA expression in HTR-8/SVneo cells by targeting the CXCL12β gene during hypoxia. The effects of CXCL12βon HTR-8/SVneo cells could be reversed by arachidonic acid (ARA).
CONCLUSION
Induction of miR-141 by hypoxia promotes apoptosis, and inhibits the invasion and vascularization capabilities of HTR-8/SVneo cells by suppressing the CXCL12β and CXCR2/4 signaling pathways.
背景
滋养细胞侵袭能力受损是子痫前期(PE)发展的原因之一,这种能力的受损可由各种 microRNAs(miRs)的表达改变引起。miR-141 和 CXCL12β(C-X-C 基序趋化因子配体 12)信号在子痫前期发病机制中调节滋养细胞的侵袭和血管生成能力;然而,它们的相互作用和作用机制尚不清楚。我们研究了 miR-141 如何调节滋养细胞的侵袭,重点是其与 CXCL12β 信号的相互作用。
方法
使用 HTR-8/SVneo 细胞建立 PE 模型,首先将其在 2%O 中培养 48 h,然后在 5%O 中培养。用模拟物或抑制剂调节人绒毛滋养层 HTR-8/SVneo 细胞中 miR-141 的表达,并通过定量 RT-PCR 进行分析。通过 ELISA 测定 CXCL12β 水平。通过流式细胞术测定细胞凋亡,通过 Transwell 和管形成测定分别评估滋养细胞的侵袭和血管生成能力。通过双荧光素酶测定验证 miR-141 与 CXCL12β mRNA 的结合。通过 Western 印迹估计蛋白水平。
结果
miR-141 在 HTR-8/SVneo 细胞中受到缺氧的显著诱导。发现在缺氧条件下,miR-141 可促进细胞凋亡并抑制 HTR-8/SVneo 细胞的侵袭和血管生成能力。miR-141 可以直接与 CXCL12β mRNA 的 3'UTR 区域结合并抑制其翻译。此外,我们证明,在缺氧条件下,miR-141 可以通过靶向 CXCL12β 抑制 HTR-8/SVneo 细胞的侵袭和血管生成能力并促进其凋亡。此外,我们证明,花生四烯酸可以在缺氧时逆转 CXCL12β 介导的 HTR-8/SVneo 细胞的侵袭和凋亡能力。在机制方面,miR-141 通过靶向 CXCL12β 基因,在缺氧条件下可下调 HTR-8/SVneo 细胞中的 MMP2、p62 和 LC3B 表达,并上调 ROCK1 和 RhoA 表达。花生四烯酸(ARA)可以逆转 CXCL12β 对 HTR-8/SVneo 细胞的作用。
结论
缺氧诱导的 miR-141 通过抑制 CXCL12β 和 CXCR2/4 信号通路促进 HTR-8/SVneo 细胞凋亡,并抑制其侵袭和血管生成能力。
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