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控制 PGF2α 合成、代谢和转运的酶系统在人胎盘中的差异表达。

Differential expression of the enzymatic system controlling synthesis, metabolism, and transport of PGF2 alpha in human fetal membranes.

机构信息

INSERM U767, Faculté des Sciences Pharmaceutiques et Biologiques, Université René Descartes, Paris, France.

出版信息

Biol Reprod. 2010 Jul;83(1):155-62. doi: 10.1095/biolreprod.109.080390. Epub 2010 Mar 31.

DOI:10.1095/biolreprod.109.080390
PMID:20357271
Abstract

The present study investigated the expression of genes and proteins associated with PGF2alpha biosynthesis, catabolism, and transport in matched amnion and choriodecidua of human term placenta. The concentration of PGF2alpha within fetal membranes depends on the balance between complex enzymatic systems responsible for, respectively, its synthesis-by prostaglandin-endoperoxide synthase 2 (PTGS2) and members of the aldo-keto reductase (AKR) family, AKR1C3 and AKR1B1-and its catabolic inactivation-through hydroxy-prostaglandin-dehydrogenase (HPGD). We observed that AKR1C3 shows equal basal expression (mRNA and protein) in choriodecidua and amnion but that AKR1B1 exhibits preferential expression in the choriodecidua. Expression of HPGD and solute carrier organic anion transporter family member 2A1 (SLCO2A1) was found primarily in the choriodecidua. We also evaluated whether an inflammatory environment induced by the gram-negative bacterial endotoxin lipopolysaccharide (LPS) affects expression of each candidate enzymes. The amnion responded to LPS with a small but significant decrease of AKR1B1 mRNA expression. In contrast, we found a significant increase in PTGS2 and AKR1C3 mRNA expression in choriodecidua after LPS challenge, but such regulation was confirmed only at protein levels for PTGS2 and not for AKR1C3. Our results suggest that the choriodecidua appears to be the main tissue, which expresses maximally all the components (synthesis, degradation, and transport) controlling PGF2alpha levels.

摘要

本研究调查了与 PGF2alpha 生物合成、分解代谢和转运相关的基因和蛋白在足月人胎盘匹配的羊膜和绒毛膜中的表达。胎儿膜内 PGF2alpha 的浓度取决于负责其合成的复杂酶系统之间的平衡 - 分别由前列腺素内过氧化物合酶 2(PTGS2)和醛酮还原酶(AKR)家族成员 AKR1C3 和 AKR1B1 以及其分解代谢失活 - 通过羟前列腺素脱氢酶(HPGD)。我们观察到 AKR1C3 在绒毛膜和羊膜中具有相同的基础表达(mRNA 和蛋白),但 AKR1B1 在绒毛膜中表现出优先表达。HPGD 和溶质载体有机阴离子转运家族成员 2A1(SLCO2A1)的表达主要在绒毛膜中发现。我们还评估了革兰氏阴性细菌内毒素脂多糖(LPS)引起的炎症环境是否影响每个候选酶的表达。羊膜对 LPS 的反应是 AKR1B1 mRNA 表达的微小但显著降低。相比之下,我们发现 LPS 刺激后绒毛膜中 PTGS2 和 AKR1C3 mRNA 表达显著增加,但这种调节仅在 LPS 刺激后仅在蛋白水平上得到证实,而不是在 AKR1C3 上。我们的研究结果表明,绒毛膜似乎是表达控制 PGF2alpha 水平的所有成分(合成、降解和转运)的主要组织。

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