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内皮素前体mRNA在无血管人羊膜中的表达与调控

Expression and regulation of endothelin precursor mRNA in avascular human amnion.

作者信息

Sunnergren K P, Word R A, Sambrook J F, MacDonald P C, Casey M L

机构信息

Cecil H. and Ida Green Center for Reproductive Biology Sciences, University of Texas Southwestern Medical Center, Dallas 75235-9051.

出版信息

Mol Cell Endocrinol. 1990 Jan 2;68(1):R7-14. doi: 10.1016/0303-7207(90)90174-7.

Abstract

Posttranslational processing of preproendothelin in endothelial cells gives rise to endothelin, a 21 amino acid polypeptide that is a potent vasoconstrictor. Endothelin production is believed to be mediated principally by transcriptional mechanisms. Previously, preproendothelin mRNA expression has been detected only in vascular endothelial tissue and cells. In this study, we found that preproendothelin mRNA is expressed in an avascular human tissue, namely, amnion, an extraembryonic fetal membrane. Preproendothelin mRNA was not detected in avascular chorion laeve tissue (also an extraembryonic fetal membrane), in the highly vascularized fetal trophoblast, or in maternal uterine tissues. Furthermore, we found that preproendothelin gene expression is retained in human amnion cells maintained in primary monolayer culture. Using the amnion cells in primary monolayer culture to investigate the regulation of preproendothelin mRNA expression, we found that epidermal growth factor (EGF) and interleukin-1 (IL-1) act to stimulate preproendothelin mRNA levels; in addition, the induction of preproendothelin mRNA by either of these agents is enhanced upon simultaneous treatment with cycloheximide. These findings are indicative that preproendothelin gene expression in amnion is regulated positively by EGF and IL-1 and that inhibition of protein synthesis leads to superinduction of preproendothelin mRNA. In human umbilical cord endothelial cells, neither IL-1 nor EGF stimulate preproendothelin mRNA expression but inhibition of protein synthesis does lead to increased levels of preproendothelin mRNA. The amnion, therefore, provides a useful system for expansion of our understanding of the tissue specific expression and regulation of preproendothelin mRNA.

摘要

内皮细胞中前内皮素原的翻译后加工产生内皮素,这是一种由21个氨基酸组成的多肽,是一种强力血管收缩剂。内皮素的产生被认为主要由转录机制介导。此前,仅在血管内皮组织和细胞中检测到前内皮素原mRNA表达。在本研究中,我们发现前内皮素原mRNA在一种无血管的人体组织即羊膜(一种胚外胎膜)中表达。在无血管的平滑绒毛膜组织(也是一种胚外胎膜)、高度血管化的胎儿滋养层或母体子宫组织中未检测到前内皮素原mRNA。此外,我们发现前内皮素原基因表达在原代单层培养的人羊膜细胞中得以保留。利用原代单层培养的羊膜细胞研究前内皮素原mRNA表达的调控,我们发现表皮生长因子(EGF)和白细胞介素-1(IL-1)可刺激前内皮素原mRNA水平;此外,用环己酰亚胺同时处理时,这两种因子中任一种对前内皮素原mRNA的诱导作用都会增强。这些发现表明,羊膜中前内皮素原基因表达受到EGF和IL-1的正向调控,并且蛋白质合成的抑制会导致前内皮素原mRNA的超诱导。在人脐带内皮细胞中,IL-1和EGF均不刺激前内皮素原mRNA表达,但蛋白质合成的抑制确实会导致前内皮素原mRNA水平升高。因此,羊膜为扩展我们对前内皮素原mRNA的组织特异性表达和调控的理解提供了一个有用的系统。

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