MiR-218-5p promotes trophoblast infiltration and inhibits endoplasmic reticulum/oxidative stress by reducing UBE3A-mediated degradation of SATB1

IF 3.6 3区 生物学 Q3 CELL BIOLOGY Journal of Cell Communication and Signaling Pub Date : 2023-05-16 DOI:10.1007/s12079-023-00751-0
Xiao Gu, Xiaomei Sun, Yanling Yu, Lei Li
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Abstract

This research evaluated the effects of miR-218-5p on trophoblast infiltration and endoplasmic reticulum/oxidative stress during preeclampsia (PE). The expression of miR-218-5p and special AT-rich sequence binding protein 1 (SATB1) in placental tissues from 25 patients with PE and 25 normal pregnant subjects was determined using qRT-PCR and western blotting. Cell invasion and cell migration were detected by performing Transwell assays and scratch assays, respectively. MMP-2/9, TIMP1/2, HIF-1α, p-eIF2α, and ATF4 expression in cells was assessed through western blotting. Intracellular reactive oxygen species were detected using 2,7-dichlorodihydrofluorescein diacetate, and intracellular malondialdehyde and superoxide dismutase activities were determined with kits. Dual-luciferase and RNA pull-down assays were performed to verify the interaction between miR-218-5p and UBE3A. Co-immunoprecipitation and western blotting were used to detect the ubiquitination levels of SATB1. A rat model of PE was established, and an miR-218-5p agomir was injected into rat placental tissues. The pathological characteristics of placental tissues were detected via HE staining, and MMP-2/9, TIMP1/2, p-eIF2α, and ATF4 expression in rat placental tissues was determined through western blotting. MiR-218-5p and SATB1 were expressed at low levels, while UBE3A was highly expressed in the placental tissues of patients with PE. The transfection of an miR-218-5p mimic, UBE3A shRNA, or an SATB1 overexpression vector into HTR-8/SVneo cells promoted trophoblast infiltration and inhibited endoplasmic reticulum/oxidative stress. It was determined that UBE3A is a target of miR-218-5p; UBE3A induces ubiquitin-mediated degradation of SATB1. In PE model rats, miR-218-5p alleviated pathological features, promoted trophoblast infiltration, and inhibited endoplasmic reticulum/oxidative stress. MiR-218-5p targeted and negatively regulated UBE3A expression to inhibit ubiquitin-mediated SATB1 degradation, promote trophoblast infiltration, and inhibit endoplasmic reticulum/oxidative stress.

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MiR-218-5p通过减少ube3a介导的SATB1降解,促进滋养细胞浸润,抑制内质网/氧化应激
本研究评估了miR-218-5p对子痫前期(PE)滋养细胞浸润和内质网/氧化应激的影响。采用qRT-PCR和western blotting检测25例PE患者和25例正常孕妇胎盘组织中miR-218-5p和特殊AT-rich sequence binding protein 1 (SATB1)的表达。采用Transwell法和划痕法分别检测细胞侵袭和细胞迁移。western blot检测细胞中MMP-2/9、TIMP1/2、HIF-1α、p-eIF2α、ATF4的表达。用2,7-二氯双氢荧光素检测细胞内活性氧,用试剂盒检测细胞内丙二醛和超氧化物歧化酶活性。通过双荧光素酶和RNA下拉实验验证miR-218-5p与UBE3A之间的相互作用。采用免疫共沉淀法和免疫印迹法检测SATB1泛素化水平。建立大鼠PE模型,将miR-218-5p agomir注射到大鼠胎盘组织中。HE染色检测大鼠胎盘组织病理特征,western blotting检测大鼠胎盘组织中MMP-2/9、TIMP1/2、p-eIF2α、ATF4的表达。MiR-218-5p和SATB1在PE患者胎盘组织中低表达,而UBE3A在PE患者胎盘组织中高表达。在HTR-8/SVneo细胞中转染miR-218-5p模拟物、UBE3A shRNA或SATB1过表达载体可促进滋养细胞浸润,抑制内质网/氧化应激。我们确定UBE3A是miR-218-5p的靶标;UBE3A诱导泛素介导的SATB1降解。在PE模型大鼠中,miR-218-5p减轻病理特征,促进滋养细胞浸润,抑制内质网/氧化应激。MiR-218-5p靶向并负调控UBE3A表达,抑制泛素介导的SATB1降解,促进滋养细胞浸润,抑制内质网/氧化应激。
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来源期刊
CiteScore
6.40
自引率
4.90%
发文量
40
期刊介绍: The Journal of Cell Communication and Signaling provides a forum for fundamental and translational research. In particular, it publishes papers discussing intercellular and intracellular signaling pathways that are particularly important to understand how cells interact with each other and with the surrounding environment, and how cellular behavior contributes to pathological states. JCCS encourages the submission of research manuscripts, timely reviews and short commentaries discussing recent publications, key developments and controversies. Research manuscripts can be published under two different sections : In the Pathology and Translational Research Section (Section Editor Andrew Leask) , manuscripts report original research dealing with celllular aspects of normal and pathological signaling and communication, with a particular interest in translational research. In the Molecular Signaling Section (Section Editor Satoshi Kubota) manuscripts report original signaling research performed at molecular levels with a particular interest in the functions of intracellular and membrane components involved in cell signaling.
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