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前列腺素介导胎儿肺对内胎炎症的反应。

Prostaglandins mediate the fetal pulmonary response to intrauterine inflammation.

机构信息

the Ritchie Centre, Monash Institute of Medical Research, Clayton, VIC, Australia.

出版信息

Am J Physiol Lung Cell Mol Physiol. 2012 Apr 1;302(7):L664-78. doi: 10.1152/ajplung.00297.2011. Epub 2012 Jan 27.

DOI:10.1152/ajplung.00297.2011
PMID:22287609
Abstract

Intra-amniotic (IA) lipopolysaccharide (LPS) induces intrauterine and fetal lung inflammation and increases lung surfactant and compliance in preterm sheep; however, the mechanisms are unknown. Prostaglandins (PGs) are inflammatory mediators, and PGE(2) has established roles in fetal lung surfactant production. The aim of our first study was to determine PGE(2) concentrations in response to IA LPS and pulmonary gene expression for PG synthetic [prostaglandin H synthase-2 (PGHS-2) and PGE synthase (PGES)] and PG-metabolizing [prostaglandin dehydrogenase (PGDH)] enzymes and PGE(2) receptors. Our second study aimed to block LPS-induced increases in PGE(2) with a PGHS-2 inhibitor (nimesulide) and determine lung inflammation and surfactant protein mRNA expression. Pregnant ewes received an IA saline or LPS injection at 118 days of gestation. In study 1, fetal plasma and amniotic fluid were sampled before and at 2, 4, 6, 12, and 24 h after injection and then daily, and fetuses were delivered 2 or 7 days later. Amniotic fluid PGE(2) concentrations increased (P < 0.05) 12 h and 3-6 days after LPS. Fetal lung PGHS-2 mRNA and PGES mRNA increased 2 (P = 0.0084) and 7 (P = 0.014) days after LPS, respectively. In study 2, maternal intravenous nimesulide or vehicle infusion began immediately before LPS or saline injection and continued until delivery 2 days later. Nimesulide inhibited LPS-induced increases in PGE(2) and decreased fetal lung IL-1β and IL-8 mRNA (P ≤ 0.002) without altering lung inflammatory cell infiltration. Nimesulide decreased surfactant protein (SP)-A (P = 0.05), -B (P = 0.05), and -D (P = 0.0015) but increased SP-C mRNA (P = 0.023). Thus PGHS-2 mediates, at least in part, fetal pulmonary responses to inflammation.

摘要

羊膜内(IA)脂多糖(LPS)可诱导子宫内和胎儿肺部炎症,并增加早产羊的肺表面活性剂和顺应性;然而,其机制尚不清楚。前列腺素(PGs)是炎症介质,PGE2 在胎儿肺表面活性剂产生中具有既定作用。我们的第一项研究旨在确定 IA LPS 对 PGE2 浓度的反应以及 PG 合成(前列腺素 H 合酶-2(PGHS-2)和 PGE 合酶(PGES))和 PG 代谢(前列腺素脱氢酶(PGDH))酶和 PGE2 受体的肺基因表达。我们的第二项研究旨在用 PGHS-2 抑制剂(尼美舒利)阻断 LPS 诱导的 PGE2 增加,并确定肺部炎症和表面活性剂蛋白 mRNA 表达。妊娠母羊在妊娠 118 天时接受 IA 生理盐水或 LPS 注射。在研究 1 中,在注射前和注射后 2、4、6、12 和 24 小时以及随后的每天对胎儿血浆和羊水进行采样,然后在 2 或 7 天后分娩胎儿。羊膜液 PGE2 浓度在 LPS 后 12 小时和 3-6 天增加(P <0.05)。胎儿肺 PGHS-2 mRNA 和 PGES mRNA 分别在 LPS 后 2(P = 0.0084)和 7 天(P = 0.014)增加。在研究 2 中,母亲静脉内尼美舒利或载体输注在 LPS 或生理盐水注射前立即开始,并持续到 2 天后分娩。尼美舒利抑制 LPS 诱导的 PGE2 增加,并降低胎儿肺 IL-1β 和 IL-8 mRNA(P ≤0.002),而不改变肺炎症细胞浸润。尼美舒利降低表面活性剂蛋白(SP)-A(P = 0.05)、-B(P = 0.05)和 -D(P = 0.0015),但增加 SP-C mRNA(P = 0.023)。因此,PGHS-2 至少部分介导了胎儿肺部对炎症的反应。

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