Department of Physiology and Anatomy, University of North Texas Health Science Center, Fort Worth, Texas, United States.
Texas College of Osteopathic Medicine, University of North Texas Health Science Center, Fort Worth, Texas, United States.
Am J Physiol Cell Physiol. 2024 Jun 1;326(6):C1776-C1788. doi: 10.1152/ajpcell.00091.2024. Epub 2024 May 13.
Circulating cell-free mitochondrial DNA (ccf-mtDNA) is an indicator of cell death, inflammation, and oxidative stress. ccf-mtDNA in pregnancies with placental dysfunction differs from that in healthy pregnancies, and the direction of this difference depends on gestational age and method of mtDNA quantification. Reactive oxygen species (ROS) trigger release of mtDNA, yet it is unknown whether trophoblast cells release mtDNA in response to oxidative stress, a common feature of pregnancies with placental pathology. We hypothesized that oxidative stress would induce cell death and release of mtDNA from trophoblast cells. BeWo cells were treated with antimycin A (10-320 µM) or rotenone (0.2-50 µM) to induce oxidative stress. A multiplex real-time quantitative PCR (qPCR) assay was used to quantify mtDNA and nuclear DNA in membrane-bound, non-membrane-bound, and vesicle-bound forms in cell culture supernatants and cell lysates. Treatment with antimycin A increased ROS ( < 0.0001), induced cell necrosis ( = 0.0004) but not apoptosis ( = 0.6471), and was positively associated with release of membrane-bound and non-membrane-bound mtDNA ( < 0.0001). Antimycin A increased mtDNA content in exosome-like extracellular vesicles (vesicle-bound form; = 0.0019) and reduced autophagy marker expression (LC3A/B, = 0.0002; p62, < 0.001). Rotenone treatment did not influence mtDNA release or cell death ( > 0.05). Oxidative stress induces release of mtDNA into the extracellular space and causes nonapoptotic cell death and a reduction in autophagy markers in BeWo cells, an established in vitro model of human trophoblast cells. Intersection between autophagy and necrosis may mediate the release of mtDNA from the placenta in pregnancies exposed to oxidative stress. This is the first study to test whether trophoblast cells release mitochondrial (mt)DNA in response to oxidative stress and to identify mechanisms of release and biological forms of mtDNA from this cellular type. This research identifies potential cellular mechanisms that can be used in future investigations to establish the source and biomarker potential of circulating mtDNA in preclinical experimental models and humans.
循环无细胞线粒体 DNA(ccf-mtDNA)是细胞死亡、炎症和氧化应激的标志物。胎盘功能障碍妊娠中的 ccf-mtDNA 与健康妊娠中的不同,这种差异的方向取决于孕龄和 mtDNA 定量方法。活性氧(ROS)触发 mtDNA 的释放,但尚不清楚滋养层细胞是否会对氧化应激做出反应而释放 mtDNA,这是胎盘病理妊娠的一个常见特征。我们假设氧化应激会诱导滋养层细胞死亡并释放 mtDNA。BeWo 细胞用抗霉素 A(10-320µM)或鱼藤酮(0.2-50µM)处理以诱导氧化应激。使用多重实时定量 PCR(qPCR)测定法来定量膜结合、非膜结合和囊泡结合形式的 mtDNA 和核 DNA,在细胞培养上清液和细胞裂解物中。抗霉素 A 处理增加了 ROS(<0.0001),诱导了细胞坏死(=0.0004)但没有诱导细胞凋亡(=0.6471),并且与膜结合和非膜结合 mtDNA 的释放呈正相关(<0.0001)。抗霉素 A 增加了外泌体样细胞外囊泡(囊泡结合形式)中的 mtDNA 含量(=0.0019),并降低了自噬标志物的表达(LC3A/B,=0.0002;p62,<0.001)。鱼藤酮处理不影响 mtDNA 释放或细胞死亡(>0.05)。氧化应激诱导 mtDNA 释放到细胞外空间,并导致 BeWo 细胞中非凋亡性细胞死亡和自噬标志物减少,这是一种体外人滋养层细胞模型。自噬和坏死的交叉可能介导了暴露于氧化应激的妊娠中胎盘 mtDNA 的释放。这是第一项研究,旨在测试滋养层细胞是否会对氧化应激做出反应而释放线粒体(mt)DNA,并确定从这种细胞类型释放和 mtDNA 的生物学形式的机制。这项研究确定了潜在的细胞机制,可以在未来的研究中用于建立临床前实验模型和人类中循环 mtDNA 的来源和生物标志物潜力。
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