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滋养层氧化应激与游离胎儿-胎盘DNA的释放

Trophoblastic oxidative stress and the release of cell-free feto-placental DNA.

作者信息

Tjoa May Lee, Cindrova-Davies Tereza, Spasic-Boskovic Olivera, Bianchi Diana W, Burton Graham J

机构信息

Department of Pediatrics, Division of Genetics, Tufts-New England Medical Center, Boston, Massachusetts, USA.

出版信息

Am J Pathol. 2006 Aug;169(2):400-4. doi: 10.2353/ajpath.2006.060161.

Abstract

Considerable quantities of cell-free fetal DNA circulate in the maternal blood during human pregnancy, but the origin of the DNA remains uncertain. Circumstantial evidence suggests the placenta is the principal source, so we tested the hypothesis that release occurs from the syncytiotrophoblast after the induction of apoptotic changes. Villous explants from normal placentas delivered by elective caesarean section were cultured under normoxic conditions (10% oxygen) for up to 20 hours or exposed to hypoxia (0.5% oxygen) for 1 hour followed by reoxygenation. The concentration of beta-globin cell-free DNA in the supernatant, measured using real-time polymerase chain reaction methodology, was significantly increased at 20 hours after hypoxia-reoxygenation. Release was associated with increased apoptosis, confirmed by increased activation of caspase-3 on Western blotting, and immunolocalized to the syncytiotrophoblast; necrosis was also evidenced by release of lactate dehydrogenase. Both release of cell-free DNA and apoptosis could be significantly reduced by the addition of antioxidant vitamins C and E to the culture medium. This study provides the first evidence of a mechanistic and quantitative link between placental apoptosis/necrosis and release of cell-free DNA, hence confirming that maternal serum/plasma concen-trations of cell-free DNA may act as a biomarker of trophoblast well-being during pregnancy.

摘要

在人类孕期,母血中会循环着大量的游离胎儿DNA,但其来源仍不确定。间接证据表明胎盘是主要来源,因此我们检验了一个假设,即凋亡变化诱导后,游离胎儿DNA是从合体滋养层细胞释放出来的。对通过择期剖宫产分娩的正常胎盘绒毛外植体在常氧条件下(10%氧气)培养长达20小时,或暴露于低氧环境(0.5%氧气)1小时后再复氧。使用实时聚合酶链反应方法测定上清液中β-珠蛋白游离DNA的浓度,结果显示在低氧复氧后20小时显著增加。DNA的释放与凋亡增加有关,这通过蛋白质免疫印迹法检测到的caspase-3激活增加得到证实,且免疫定位在合体滋养层细胞;乳酸脱氢酶的释放也证明了坏死的发生。向培养基中添加抗氧化维生素C和E可显著减少游离DNA的释放及凋亡。本研究首次提供了胎盘凋亡/坏死与游离DNA释放之间存在机制和定量联系的证据,从而证实孕期母血/血浆中游离DNA的浓度可能作为滋养层细胞健康状况的生物标志物。

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