首页> 外文期刊>The Journal of biological chemistry >Transcriptional regulation of insulin-like growth factor-II gene expression by cortisol in fetal sheep during late gestation.
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Transcriptional regulation of insulin-like growth factor-II gene expression by cortisol in fetal sheep during late gestation.

机译:妊娠晚期羊皮质醇对胰岛素样生长因子-II基因表达的转录调控。

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The objective of this study was to determine the mechanisms by which cortisol down-regulates hepatic insulin-like growth factor-II (IGF-II) gene expression in late gestation. Leader exons 6 and 7 of the ovine IGF-II gene, with their 5'-flanking regions, were first isolated. Characterization of transcription start sites revealed a unique site for exon 6 and three dispersed sites for exon 7. Nuclear run-on assays showed a 5-fold higher transcription rate of the IGF-II gene in liver of adrenalectomized fetuses compared with control animals, suggesting that regulation of IGF-II gene expression by cortisol is at the transcriptional level. RNase protection assays demonstrated hepatic leader exon 7 expression in adrenalectomized fetuses to be more than 2-fold higher than in controls, whereas it was reduced by 50 in cortisol-infused fetuses compared with controls. There was no effect on the expression of other leader exons. Functions of the upstream regulatory region of leader exon 7 (i.e. promoter P4) were investigated by luciferase transient expression. A region of -172 bases downstream relative to the first transcription site of leader exon 7 was shown to retain basal promoter activity and respond to cortisol. These results suggest that cortisol may induce the prenatal decline in ovine hepatic IGF-II expression by suppressing promoter P4 of the IGF-II gene.
机译:本研究的目的是确定皮质醇下调妊娠晚期肝脏胰岛素样生长因子-II (IGF-II) 基因表达的机制。首先分离出绵羊 IGF-II 基因的先导外显子 6 和 7,以及它们的 5' 侧翼区域。转录起始位点的表征揭示了外显子 6 的独特位点和外显子 7 的三个分散位点。核运行试验显示,与对照动物相比,肾上腺切除胎儿肝脏中IGF-II基因的转录率高出5倍,表明皮质醇对IGF-II基因表达的调节处于转录水平。RNase保护试验表明,肾上腺切除胎儿的肝前导外显子7表达比对照组高2倍以上,而与对照组相比,皮质醇输注胎儿的表达降低了50%。对其他前导外显子的表达没有影响。通过荧光素酶瞬时表达研究前导外显子 7(即启动子 P4)上游调控区的功能。相对于前导外显子 7 的第一个转录位点,下游的 -172 个碱基区域被证明保留基础启动子活性并对皮质醇有反应。这些结果表明,皮质醇可能通过抑制IGF-II基因的启动子P4诱导产前绵羊肝IGF-II表达下降。

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