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钾离子诱导的去极化对培养的胎鼠大脑皮质细胞中生长抑素基因表达的影响。

Effect of potassium-induced depolarization on somatostatin gene expression in cultured fetal rat cerebrocortical cells.

作者信息

Tolón R M, Sánchez Franco F, de los Frailes M T, Lorenzo M J, Cacicedo L

机构信息

Servicio de Endocrinología, Hospital Ramón y Cajal, Madrid, Spain.

出版信息

J Neurosci. 1994 Mar;14(3 Pt 1):1053-9. doi: 10.1523/JNEUROSCI.14-03-01053.1994.

DOI:10.1523/JNEUROSCI.14-03-01053.1994
PMID:7907136
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6577592/
Abstract

The stimulatory effect of potassium depolarization upon somatostatin (SS) mRNA levels in primary cultures of fetal cerebrocortical cells was analyzed. Depolarizing stimuli, such as 56 mM K+ exposure for 30 min, elicited an increase in immunoreactive somatostatin (IR-SS) release to the media and decreased SS mRNA levels. These were increased when exposure to depolarization stimuli was prolonged up to 3 or more hr. At this time, potassium (30 and 56 mM) acted as a secretagogue, stimulating SS secretion, but was also effective in stimulating SS mRNA levels, suggesting that SS secretion can be coupled to SS mRNA accumulation. These changes were inhibited by the Ca2+ channel antagonist verapamil. In contrast, Na+ channel blockade by TTX did not modify the 24 hr potassium-induced increase in SS mRNA, although it partially abolished potassium-induced SS secretion. Examination of the rate of disappearance of SS mRNA levels after inhibition of mRNA transcription by actinomycin-D revealed that K+ stimulation of cerebrocortical cells stabilized the SS mRNA. These results suggest that the induction of SS mRNA expression by K+ is dose dependent, and involves the modulation of ion channels. The time-course study confirmed that the K(+)-induced SS mRNA accumulation is time dependent, chronic activation of the Ca2+ channels being necessary to stimulate SS gene expression. K+ stimulation may also increase the level of SS mRNA in cerebrocortical cells by reducing its rate of degradation.

摘要

分析了钾离子去极化对胎儿脑皮质细胞原代培养物中生长抑素(SS)mRNA水平的刺激作用。去极化刺激,如暴露于56 mM K⁺ 30分钟,会使培养基中免疫反应性生长抑素(IR-SS)的释放增加,并降低SS mRNA水平。当去极化刺激的暴露时间延长至3小时或更长时间时,这些水平会升高。此时,钾离子(30 mM和56 mM)作为促分泌剂,刺激SS分泌,但对刺激SS mRNA水平也有效,这表明SS分泌可能与SS mRNA积累相关。这些变化被钙离子通道拮抗剂维拉帕米抑制。相比之下,河豚毒素(TTX)阻断钠离子通道并没有改变钾离子在24小时内诱导的SS mRNA增加,尽管它部分消除了钾离子诱导的SS分泌。在用放线菌素-D抑制mRNA转录后,检测SS mRNA水平的消失速率,结果显示钾离子刺激脑皮质细胞可使SS mRNA稳定。这些结果表明,钾离子对SS mRNA表达的诱导具有剂量依赖性,且涉及离子通道的调节。时间进程研究证实,钾离子诱导的SS mRNA积累具有时间依赖性,钙离子通道的慢性激活对于刺激SS基因表达是必要的。钾离子刺激还可能通过降低其降解速率来增加脑皮质细胞中SS mRNA的水平。