首页> 外文期刊>American Journal of Physiology >Ca2+- and PKC-dependent stimulation of PGE2 synthesis by deoxycholic acid in human colonic fibroblasts.
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Ca2+- and PKC-dependent stimulation of PGE2 synthesis by deoxycholic acid in human colonic fibroblasts.

机译:Ca2 +和PKC依赖性的人结肠成纤维细胞中脱氧胆酸对PGE2合成的刺激。

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摘要

We investigated prostanoid biogenesis by human colonic fibroblasts (CCD-18Co cells and nine primary fibroblast cultures) exposed to a primary (cholic, CA) or a secondary (deoxycholic, DCA) bile acid. Basal PGE2 levels in CCD-18Co cultures and fibroblast strains initiated from normal and adenocarcinomatous colon, respectively, were 1.7 +/- 0.3, 4.0 +/- 2.0, and 15.0 +/- 4.8 ng/mg protein. Peak levels 24 h after exposure to DCA (300 microM) rose, respectively, seven-, six- and sevenfold, but CA elicited no such responses. Increases in PGE2 synthesis were preceded by sequential increases in PGH synthase-2 mRNA and protein expression and were fully prevented by a nonselective (indomethacin) or a selective (celecoxib) nonsteroidal anti-inflammatory drug. DCA, but not CA, caused abrupt, transient increases in fibroblast intracellular Ca2+ concentration ([Ca2+]i) approximately 1 min after exposure. Increased [Ca2+]i was required for DCA-mediated induction of PGE2 synthesis, and protein kinase C was a further essential component of this signaling pathway. Colonic fibroblasts may be a major target for prostanoid biogenesis induced by fecal bile acids and, potentially, other noxious actions of these agents.
机译:我们研究了人结肠成纤维细胞(CCD-18Co细胞和九种原代成纤维细胞培养物)暴露于一次(胆汁,CA)或二次(脱氧胆汁,DCA)胆汁酸中前列腺素的生物发生。从正常结肠癌和腺癌结肠开始的CCD-18Co培养物中的基础PGE2水平分别为1.7 +/- 0.3、4.0 +/- 2.0和15.0 +/- 4.8 ng / mg蛋白。暴露于DCA(300 microM)后24小时的峰值水平分别上升了7倍,6倍和7倍,但CA并未引起这种反应。 PGE2合成的增加之前是PGH合酶2 mRNA和蛋白质表达的顺序增加,并且被非选择性(吲哚美辛)或选择性(塞来昔布)非甾体类抗炎药完全阻止。暴露后约1分钟,DCA(而非CA)导致成纤维细胞内Ca2 +浓度([Ca2 +] i)突然突然增加。 DCA介导的PGE2合成诱导需要[Ca2 +] i的增加,而蛋白激酶C是该信号通路的另一个重要组成部分。结肠成纤维细胞可能是粪便胆汁酸诱导的前列腺素类生物合成的主要靶标,并可能是这些药物的其他有害作用。

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